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Loyola University Chicago Loyola eCommons Master's eses eses and Dissertations 1979 A Study of Factors Affecting Healing of Developing Periapical Lesions in Immature Teeth of Dogs James Edward McCormick Loyola University Chicago is esis is brought to you for free and open access by the eses and Dissertations at Loyola eCommons. It has been accepted for inclusion in Master's eses by an authorized administrator of Loyola eCommons. For more information, please contact [email protected]. is work is licensed under a Creative Commons Aribution-Noncommercial-No Derivative Works 3.0 License. Copyright © 1979 James Edward McCormick Recommended Citation McCormick, James Edward, "A Study of Factors Affecting Healing of Developing Periapical Lesions in Immature Teeth of Dogs" (1979). Master's eses. Paper 3024. hp://ecommons.luc.edu/luc_theses/3024

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Page 1: A Study of Factors Affecting Healing of Developing ... · Orthodontics has introduced direct bonding brackets to aid asthetics and home care. New types of wires are used which are

Loyola University ChicagoLoyola eCommons

Master's Theses Theses and Dissertations

1979

A Study of Factors Affecting Healing of DevelopingPeriapical Lesions in Immature Teeth of DogsJames Edward McCormickLoyola University Chicago

This Thesis is brought to you for free and open access by the Theses and Dissertations at Loyola eCommons. It has been accepted for inclusion inMaster's Theses by an authorized administrator of Loyola eCommons. For more information, please contact [email protected].

This work is licensed under a Creative Commons Attribution-Noncommercial-No Derivative Works 3.0 License.Copyright © 1979 James Edward McCormick

Recommended CitationMcCormick, James Edward, "A Study of Factors Affecting Healing of Developing Periapical Lesions in Immature Teeth of Dogs"(1979). Master's Theses. Paper 3024.http://ecommons.luc.edu/luc_theses/3024

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A STUDY OF FACTORS AFFECTING HEALING

OF DEVELOPING PERIAPICAL LESIONS IN

IHMATURE TEETH OF DOGS

by

James Edward HcCormick, D.H.D.

A Thesis Submitted to the Faculty of the Graduate School

of Loyola University of Chicago in Partial Fulfillment

of the Requirements for the Degree of

Master of Science

May, 1979

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DEDICATION

To my "best buddy" and wife, Ann, whose love,

understanding, and especially patience allowed me

to continue my educational pursuits.

ii

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AC~~OWLEDGMENTS

To Dr. Franklin Weine, my committee chairman, teacher, and

friend, I extend my gratitude and special thanks for directing

this study and providing an excellent and well balanced graduate

education.

To Dr. Marshall Smulson, I extend my respect for your un­

failing dedication to endodontic education and inexhaustible

friendship to colleagues and students.

To Dr. Joseph Maggio, I express my appreciation for your

friendship, guidance, and critical eye during the entire study

and my two years of endodontic education.

To Dr. Hal McReynolds, my friend and advisor, I thank you

for your help in examining and evaluating the histological sec­

tions.

To Dr. Ioannis Scarpa, I offer my sincere appreciation

for allowing me to use your research instruments and for your

guidance in conducting a scientific research project.

To Dr. Ronald Jew and Dr. Richard Munaretto, my friends

and classmates, I extend my sincerest thanks for your hours

of technical and theoretical assistance which made this project

possible.

iii

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VITA

The author, James Edward McCormick, was born in Owen Sound,

Ontario, Canada on the first of July, 1946.

He obtained his elementary education at Quilchena School in

Vancouver, British Columbia, Canada, and his secondary education

at Prince of Wales High School in Vancouver, British Columbia, Canada

where he graduated with honors in June of 1964.

In September of 1964 he entered the University of British Columbia

and obtained three years of pre-dental science education. Honors in­

cluded the Faculty of Science Merit Award in his sophomore year and the

Provincial Government Scholarship Awards in each of his predental edu­

cation years.

In September of 1967 he entered the University of British Columbia

School of Dentistry where he graduated in June of 1971 with the degree

of Doctor of Dental Medicine, l1agna Cum Laude. Honors included Omicron

Kappa Upsilon national dental honor society, Biochemistry Award, Oral

Biology Award, B.C. Dental Wives Scholastic Bursary, and the Provincial

Government Scholarship Award in each of his dental education years.

In June of 1971 he was an associate in a general dentistry private

practice in Vancouver, B.C, for four months before beginning his own

private practice in Kelouna, B.C, in September of 1971. During the fol­

lowing six years of general dentistry, he was the continuing dental edu­

cation representative for the Kelouna and District Dental Society and

iv

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a Director of the B.C. Chapter of the Academy of General Dentistry.

In September of 1977 he entered the Loyola University School

of Dentistry and began a dual course of study leading to the didactic

degree of Master of Science in Oral Biology and a Certificate of

Specialty Training in Endodontics.

v

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TABLE OF CONTENTS

Dedication. . . .

Acknowledgements.

Vita.

Table of contents

List of tables.

List of figures

Chapter

I. Introduction ...... .

II. Review of the literature

III. Materials and methods ..

IV. Results ..

V. Discussion

VI. Summary and conclusions.

VII. References

VIII. Tables and figures

vi

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4

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62

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LIST OF TABLES

Table

I. Comparison of radiographic findings after one week of infection and at sacrifice .•

II. Individual periapical tissue pH values at various intervals during the experiment

III. Average periapical tissue pH values at various intervals during the experiment comparing effects of paste inserted •

IV. Comparison of clinical findings after one week of infection and at sacrifice.

V. Clinical findings at time of sacrifice comparing effects of paste inserted

VI. Average periapical tissue pH values of the experimental teeth at various intervals during the experiment . •

VII. Radiographic findings at time of sacrifice comparing effects of paste inserted ..•.

vii

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96

97

99

100

101

102

103

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LIST OF FIGURES

Figure

1. Preoperative radiographic survey .

2. Radiographic survey after one week of infection with S. faecalis ..••

3. Radiographic survey of one week animal

4. Radiographic survey of one month animal

at

at

5. Radiographic survey of three month animal

6. Radiographic survey of six month animal at

7. Apex of control tooth in one week animal .

sacrifice.

sacrifice

at sacrifice

sacrifice

8. Furcation area of control tooth in one week animal

9. Gingival sulcus of control tooth in one week animal.

10. Apex of control tooth in one month animal. . 11. Apex of control tooth in three month animal.

12. Apex of control tooth in six month animal. . . 13. Apex of infected-only tooth in one week animal

14. Acute inflammatory cellular infiltrate . 15. Alveolar bone around infected-only tooth

in one week animal •

16. Apex of infected-only tooth in one month animal.

17. Chronic inflammatory cellular infiltrate

18. Furcation area of infected-only tooth in one man th animal . • • . . . • . • • . . .

19. Apex of infected-only tooth in three month animal.

viii

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105

105

107

107

109

109

111

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113

113

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115

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119

119

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Figure

20. Apex of acidic-treated tooth in one week animal ..

21. Apex of acidic-treated tooth in three month animal

22. Isolated periodontal ligament attachment ...•••

23. Apex of acidic-treated tooth in three month animal

24. Cyst-like area adjacent to root apex .•..•.•

25. Apex of acidic-treated tooth in six month animal

26. Apex of basic-treated tooth in one week animal

27. Proliferating epithelium

28. Embedded dentin ...

29. Isolated periodontal ligament attachment

30. Apex of basic-treated tooth in one month animal .•

31. Dentin and cementum resorption

32. Apex of basic-treated tooth in three month animal .•

33. Well differentiated epithelial sling

34. Socket of basic-treated tooth in six month animal ••

ix

. . . .

Page

123

125

125

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CHAPTER I

INTRODUCTION

Dentistry has evolved into a dynamic field with new techniques

being introduced to better facilitate the treatment needs of our patients.

The focal infection theory has finally been discarded and replaced by

sound scientific and biological principles. The age old cure of extrac­

tion to relieve a toothache has been replaced by sophisticated methods

to maintain the patient's natural dentition. The long overdue general

recognition of preventive dentistry has been well accepted by the dental

profession and public at large.

In the past fifty years, there have been revolutionary changes in

each phase of dentistry. The periodontist no longer utilizes the painful

pushback procedure of alveolar denudation or other "mutilectomy" tech­

niques. The importance of matching soft tissue and bony contours is now

well accepted. New surgical techniques such as the apically repositioned

flap or bone and soft tissue grafts have been introduced to better facili­

tate the patient's needs.

Orthodontics has introduced direct bonding brackets to aid asthetics

and home care. New types of wires are used which are easier to manipu­

late and which can be tempered to provide more spring action. The torque

and activation forces are being incorporated into the bracket design

rather than the arch wire while cephalometries is aided by computer anal­

ysis. In addition, adult orthodontics is becoming routine and greatly

1

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improves the functional and psychological outlook for these people who

previously were condemned to extraction and prosthetic replacement.

Prosthodontics has incorporated a thorough understanding of the

role of occlusion into their treatment regimen. The introduction of

fully adjustable articulators has been a major contribution. Overden­

tures have greatly aided the retention of removable prostheses while new

impression materials have been discovered which have improved dimen­

sional stability for longer periods of time.

Operative dentistry has modified the cavity design principles of

G.V. Black to minimize reduction of sound tooth structure. New re­

storative materials such as composite resins have been introduced and

the acid-etch technique has improved temporary therapy for fractured

teeth.

Oral surgery has developed surgical techniques to improve tooth

to jaw or jaw to cranial base relationships. Maxillary osteotomy pro­

cedures are now being used to reposition segments or all of the upper

jaw while mandibular osteotomy procedures are used to correct retro­

gnathic or prognathic javT relationships.

However, innovations of endodontic methods have not been so nu­

merous. Endodontic pioneers such as Coolidge, Blayney and Sharp in

the early twentieth century stressed the importance of thorough canal

preparation followed by hermetic sealing of the root canal in the apical

region. These principles, reinforced by sixty years of success, remain

as the foundation of modern endodontics.

2

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For many years, the treatment of pulpally involved immature teeth

with periapical involvement has been a perplexing problem to the dentist.

The introduction of the apexification technique has been an exciting in­

novation to simplify therapy and greatly enhance the degree of success (1).

This technique, being relatively new, is subject to differences of opin­

ion. Controversy concerning the materials used and the underlying mech­

anism of repair has led to numerous studies of root end induction to

further understand this dynamic technique. The purpose of this study is

to further clarify some of the conditions by which hard tissue repair

occurs at the apices of pulpless immature teeth.

3

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CHAPTER II

REVIEH OF THE LITERATURE

NORMAL TOOTH DEVELOPMENT AND ROOT FORMATION

Schour, Massler, and Brescia (2) described tooth development be­

ginning as a proliferation of basal cells in the oral epithelium when

the embryo is five to six weeks old. This forms an ectodermal thicken­

ing in the region of the future dental arches and is called the dental

lamina. Tooth buds develop by rapid cellular proliferation at discrete

points along the dental lamina which produces knobs of ectodermal cells

extending into the underlying mesenchyme. Unequal growth in the tooth

bud results in a shallow invagination on its deeper surface and the

enamel organ becomes evident with the inner and outer enamel epithelial

layers surrounding the stellate reticulum and the stratum intermedium.

With continued cellular proliferation, the bud stage of the enamel organ

passes through the cap and bell stages.

The organizing influence of the inner enamel epithelial cells

causes the underlying mesenchymal cells to proliferate and condense into

the dental papilla (the future dental pulp). After lining up opposite

the cells of the inner enamel epithelium, mesenchymal cells differentiate

into odontoblasts and lay down an organic matrix which calcifies to form

dentin as the odontoblasts recede from the enamel organ. Once the first

layer of dentin has formed, the ameloblasts move away from their position

and leave behind an organic matrix which when mineralized forms enamel.

4

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After enamel and dentin formation has reached the future cementa­

enamel junction, the development of the root begins. The inner and

outer enamel epithelium come together at a point termed the cervical

loop to form Hertwig's epithelial root sheath. The root sheath then

forms the epithelial diaphragm by bending inwards to a horizontal plane

which narrows the wide cervical opening of the tooth germ. Skillen (3)

believed the enamel organ extended apically as a stimulative layer to

root development. Orban (4) stated the plane of the epithelial diaphragm

remains relatively fixed while the epithelium proliferates coronally,

resulting in a lengthening of the epithelial root sheath. Diab and

Stallard (5) substantiated this spatial stability concept in an autora­

diographic analysis using tritiated thymidine on the developing teeth of

rats. Skillen (3) described the cells of the root sheath as being very

rudimentary in character. They activated root dentin formation but

lacked the physiologic properties necessary for the secretion of enamel.

Schour, Massler, and Brescia (2) stated the epithelial proliferation

stimulates mesench)~al cells in the dental papilla to differentiate into

odontoblasts and form root dentin. Diab and Stallard (5) found a direct

correlation between the number of root sheath cells preparing to divide

and the process of odontoblastic differentiation. The radioactive index

of the root sheath cells rose rapidly when dentin was first formed and

dropped to zero when root dentin formation stopped. Kenney and Ramfjord

(6), using isotopes to study root formation in rhesus monkeys, agreed

that the root sheath plays a role in odontoblastic differentiation.

5

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The next stage of root development involves cementum deposition

on the root surface. Connective tissue cells from the surrounding dental

sac differentiate into cementoblasts. Gottliep (7) theorized Hertwig's

sheath must degenerate prior to cementum formation and that no cementum

will form in areas where the epithelial root sheath remains on dentin.

Schour, Massler, and Brescia (2) stated that connective tissue elements

of the surrounding dental sac proliferate into the epithelial root

6

sheath dividing it into a network of epithelial strands. When these con­

nective tissue cells come into contact with the outer surface of the root

dentin, they differentiate into cementoblasts and deposit a layer of cemen­

tum onto the root dentin. Owens (8) speculated that as the connective

tissue cells come in contact with the cells of the inner layer of Hertwig's

sheath they differentiate into cementoblasts. Diab and Stallard (5)

found that cementum formation was more closely related to the develop­

mental stage and function rather than the state of cellular activity in

the root sheath. They found that completion of the root by cementum

formation in some instances took place only after the disintegration of

the root sheath, while in other cases cementum formed over the root

sheath which trapped epithelial cells between the cementum and dentin.

Their conclusion that cementum formation is dependent neither on the pre­

sence nor the absence of an epithelial root sheath has been substantiated

by Kenney and Ramfjord (6). Skillen (3) stated that cementum formation

begins when the teeth are in occlusion due to the stimulation caused by

the forces of mastication. He felt this masticatory stress will also

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have a decided influence on the manner in which the apex is finally com­

pleted. Owens (8) believed that cementum formation begins during tooth

eruption when the root is about two-thirds formed and there is a need

for more substantial tooth attachment.

Schour, Massler, and Brescia (2) noted that proliferation of epithe­

lium in the diaphragm lags behind that of the pulpal connective tissue

in the later stages of root development and apposition of dentin and cemen­

tum results in the final narrowing of the apical foramen. Owens (8) stated

that pulpal cells trapped in the dentin give rise to a bone like tissue,

osteodentin, which contributes to the highly cellular root apex. Although

it is generally agreed that root formation is completed about 3 years after

the eruption of teeth, Friend (9) concluded that this process takes con­

siderably longer.

Bernick, et al., (10) described how the connective tissue elements

of the dental sac mature into the periodontal ligament. Schour, Massler,

and Brescia (2) reported that remnants of the epithelial root sheath per­

sist as the epithelial rests of Malassez in the periodontal ligament. How­

ever, Diab and Stallard (5) and Kenney and Ramfjord (6) showed that la­

belled cells of the epithelial diaphragm did not migrate into the perio­

dontal ligament. The function of the epithelial rests is now surrounded

by speculative conjecture.

TREATMENT METHODS FOR IMMATURE TEETH

Zeldow (11) recommended four available methods of treatment for

pulpally involved and pulpless immature teeth. If the pulp remains vital,

7

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he recommended using a pulpotomy technique to allow normal root develop­

ment to continue. However, if the pulp is necrotic, conventional root

canal treatment, endodontic surgery, or apexification procedures may be

used for immature teeth.

A pulpotomy procedure is the treatment of choice for a young in­

completely developed tooth with a vital pulp (1,12,13,14,15,16,17).

This technique will allow the healthy radicular pulp and Hertwig's

epithelial root sheath to continue to function in order to complete the

development of the immature root apex (11,18). A wide variety of ma­

terials have been used in the pulpotomy method to obtain continued root

growth. Successful results have been reported using formocresol (1),

calcium hydroxide (12,19,20,21,22,23,24,25,26,27,28,29,30,31), zinc

oxide and eugenol (32,33,34), a mixture of zinc oxide-metacresyl acetate­

camphorated parachloropehnol (35), iodoform Chlumsky paste (36), and

glycerite of iodine paste (36). Torneck (37), performing vital pulpotomies

on immature monkey teeth without using any medication, reported that root

formation may continue but this growth is irregular and retarded. Further­

more, subsequent breakdown and necrosis of the remaining pulpal tissue

can lead to apical abscess formation and root resorption.

Bodenham (21) and Krakow,~ al., (23), stated that pulp extirpa­

tion and conservative root canal treatment after root maturation are not

routinely needed. They suggested that definitive root canal treatment

should only be performed when a subsequent pathological condition is de­

tected by radiographic examination or appropriate clinical tests such as

tenderness to percussion or sinus tract formation. However, chronic

8

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inflammation may remain in the pulpal tissue and cause resorption and ap­

position on the canal walls, and pulpal calcifications may slowly render

these canals non-negotiable to endodontic instrumentation (38). Fischer

(39) has shown that teeth having pulp chambers obliterated by hard tis­

sue appear to be homogenous on radiographs, but in fact contain vital

pulpal remants. He stated that this remaining connective tissue is more

susceptible to infection or necrosis which will ultimately lead to peri­

apical pathosis. While studying pulpotomy procedures in immature pre­

molar teeth of dogs, Vojinovic (36) found that after apical closure,

pulpal necrosis could still occur and lead to destructive processes in

periapical and bifurcation areas. With these unfavorable sequellae in

mind, pulpotomy is only regarded as a temporary measure which leaves a

healthy radicular pulp to permit completion of the incompletely devel­

oped root. Pulp extirpation and conservative endodontic treatment are

recommended when root development is complete (11,12,15,19,26,28,30,31,

32,33,34,35,36,38,39).

If the pulp is necrotic, one of the other three methods outlined

by Zeldow (11) must be employed. The first technique involves bio­

mechanical cleansing and obturation of the root canal. The obturation

of the root canal space has been accomplished by using Diaket (41,42,43)

oxidized regenerated cellulose and amalgam (44,45), or gutta-percha and

a sealer (15,46,47,48,49). Various techniques for the complete oblitera­

tion of the root canal space with a hand-rolled or otherwise customized

gutta-percha point have been described (34,50,51,52).

9

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Boyle (53) explained the healing process as a deposition of cemen­

tum onto the root end to cover the root filling material and obliterate

any lumen still present at the apex. He stated this process will only

occur in the absence of infection. Moodnick (28) reported that since

granulation tissue is a necessary precursor for healing, the removal of

the bulk of necrotic tissue, medication, sterilization, and obturation

of the root canal will result in a high percentage of successful cases.

However, the problems associated with treating immature teeth by con­

ventional endodontic methods are well known. Friend (9) and Duell (41)

noted that root development in the labia-lingual plane tends to lag be­

hind development in the mesio-distal plane (see diagram page 11). The

divergent or blunderbluss canal has an apical dimension wider than the

root canal and the narrowest portion of the root canal is in the cervi­

cal region of the immature tooth. Furthermore, according to Ingle (54),

the incompletely developed canal wall is not fully calcified which makes

it very porous. As a result, the wide open, sometimes divergent, apex

makes it very difficult to obtain a hermetic apical seal which is one of

the basic requirements for successful endodontic therapy (51).

Zeldow's (11) second method of treating non-vital immature teeth

utilized surgical intervention and has been widely advocated in the past.

Maxmen (55) and Ingle (56) described the post resection canal filling

technique utilizing a ball burnisher at the apex as a matrix against which

gutta-percha may be packed. A warm burnisher is then used to remove excess

gutta-percha and to seal the apex. Patterson (51) and Sommer, Ostrander,

and Crowley (52) preferred to fill the canal first with gutta-percha

10

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11

MESIO-DISTAL AND LABIO-LINGUAL VIEWS OF CANAL

MORPHOLOGY AT VARIOUS STAGES OF ROOT DEVELOPMENT

(1) DIVERGENT WALLS* (2) PARALLEL WALLS*

(3) TAPERING WALLS* (4) MATURE APEX"'~

* as seen on intraoral periapical radiograph

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before surgically exposing the apex to remove excess gutta-percha with a

warm burnisher. This method will reduce surgical exposure time and min­

imize post-operative sequellae. Grossman (51) and Law (26) advocated

filling the canal with gutta-percha before performing a root resection

at a level which ensures an apical seal. Another popular surgical tech­

nique mentioned by numerous authors (19,34,43,54,58,59) involved ob­

literating the canal with gutta-percha followed by the surgical approach

of apicoectomy and placement of a reverse amalgam restoration.

However, numerous reports (30,48,60,61,62,63) discuss the disad­

vantages of the surgical technique. From the patient's viewpoint, this

method is the least desirable as it is an emotionally traumatic and un­

comfortable procedure for a young patient. The surgical procedure may

not be well tolerated and patient management can be a problem in a young

apprehensive individual. Due to the difficulty in obtaining an adequate

apical seal against the thin friable dentinal walls, a root resection is

often necessary to obtain a greater bulk of root structure for the place­

ment of the reverse alloy filling. This procedure will terminate root

development and possibly create an unfavorable crown root ratio and hence

a guarded prognosis for the treated tooth. Anatomic reasons may limit

this procedure to anterior teeth, and if the periapical lesion is ex­

tensive, profound anaesthesia may be difficult to maintain throughout the

entire procedure. Despite a period of initial bone apposition, long term

follolv up of some surgical cases reveals resorption and subsequent periapi­

cal rarefaction. Cooke and Rowbotham (60) speculated that these failures

may be related to the permeability of cementum in young teeth.

12

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Ideally, the problem of the blunderbuss apex could be solved by

changing the morphology of the apical portion of the root to allow for

routine obturation of the root canal with gutta-percha. Zeldow's (11)

third method of treating immature pulpless teeth was the induction of

biological apical continuation or apexification. There are two basic

approaches to this treatment regimen. The canals are cleansed as well

as their irregular walls permit, and intracanal drug therapy may be used

in addition to obtain favorable conditions in the root canal. The first

approach, as advocated by Frank (58), involved filling the canal to the

apex with a paste dressing. On the other hand, Ostby (64) induced bleed­

ing into the apical portion of the canal while the coronal portion of the

root canal was filled with gutta-percha. When apical closure has occurred

using either of these methods, the canal can be sealed conventionally

using condensed gutta-percha.

Hany investigators (11,28,33,34,58,60,61,65,66,67,68) who have re­

ported successful clinical cases of induced apical closure seemed to feel

that elements of Hertwig's sheath were responsible. They assumed that

the formative activity of Hertwig's sheath can be preserved in pulpless

teeth in spite of pathological changes in the periapical tissues. Then,

once the infection has been eliminated and more favorable conditions have

been created in the root canal, Hertwig's sheath will resume its role in

root apex formation.

Subsequent histological investigations (18,69,70,71,72,73,74) have

indicated that Hertwig's sheath does not play a role in root end induction

of necrotic immature teeth. The origin of the newly formed apical barrier

13

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is the transformation of undifferentiated mesenchymal cells of the sur­

rounding periapical tissue into hard tissue forming cells such as cement­

oblasts (18,69,70,72,73,75,76,77,78,79,80,81,82).

HISTORICAL PERSPECTIVE OF APEXIFICATION

Several reports in the literature are of historical interest in the

development of the apexification procedure. In 1929, Applebaum (83)

described two cases of cementum plug formation at the apices of immature

teeth in spite of marked infection present in these teeth. Easlick (84)

in 1943 reported a vital pulpotomy procedure using a zinc oxide-glycerite

of iodine paste in an immature per~:a~ent incisor which had been fractured

and thus exposed by trauma. Seven months later, completion of root de­

velopment was seen. Johnson (85) in 1945 packed the apical portion of

a pulpless immature root with bone-like salts in a gelatin base. Com­

plete calcification of the root canal was seen on radiographs taken five

months later. In 1950 Israel (47) first treated th~ initial symptoms to

make an acutely abscessed immature incisor comfortable. He then filled

the coronal half of the root canal with gutta-percha and silver cement.

Twenty months later when the apex was almost closed, he refilled the

canal completely with gutta-percha using a lateral condensation technique.

Herbert (86) in 1959 placed a polyantibiotic paste in the apical root

canal of two immature teeth with periapical radiolucencies. Radiographs

taken four years later showed that the periapical radiolucencies had dis­

appeared and apical calcification had occurred.

In 1960 Cooke and Rowbotham (60) showed it was possible to obtain

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either continued root formation or an apical closure by calcific repair

in apparently pulpless teeth. Their treatment procedure involved thorough

canal debridement followed by canal disinfection with tricresol formalin

or beechwood creosote. When the tooth was free of symptoms, they intro­

duced an antiseptic paste of zinc oxide, iodoform, cresol, and thymol to

within two or three millimeters of the apex. They reported continued

success in the stimulation of apical closure, but noted that continued

root development after pulpal death was atypical in form and less pointed

than the corresponding normal tooth.

15

Ostby (64) was an advocate of the role a blood clot plays in peri­

apical healing. In 1961, he published a report of a traumatized pulpless

incisor tooth with a large radiolucent lesion around an undeveloped apex.

Following canal debridement and sterilization, overinstrumentation and

laceration of the periapical tissues induced bleeding and subsequent blood

clot formation in the root canal. The coronal half of the canal was filled

with gutta-percha and a sealer. A one year recall radiograph revealed

that the radiolucency was gone and apical closure had occurred. Ostby

explained that the initial fibrin clot served as a matrix for ingrowing

granulation tissue which in turn was gradually transformed into fibrous

connective tissue. This process started at the foramen and proceeded into

the root canal. The formation of granulation tissue resulted in the re­

sorption of surrounding canal walls followed by the deposition of cellular

cementum as the transformation into fibrous tissue took place.

Following the same line of reasoning, ~1oodnick (28) in 1963 proposed

that the simple removal of the bulk of necrotic tissue, medication and

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sterilization of the root canal, and the obturation of the root canal

with gutta-percha a few millimeters short of the apex would provide

healing at the apex. He reported eighty percent success in fifty cases

treated in this manner. He pointed out that granulation tissue is a

necessary precursor of healing and that radiolucent periapical lesions

as a result of pulpal inflammation consist of granulation tissue which

will undergo repair once the bulk of canal irritants are removed.

Ball (65) in 1964 presented a case report of a necrotic immature

central incisor which was cleansed and treated with a phenol-camphor

dressing on a shortened paper point. When the acute phase had subsided,

he inserted a radiopaque polyantibiotic paste into the root canal and

five months later the apex had achieved full development. The poly­

antibiotic paste, instead of an antiseptic paste, was used to avoid the

possibility of chemical irritation to the periapical tissues.

In 1964, Kaiser (87) presented reports of root end induction in

non-vital permanent teeth. He was the first to report that calcium hy­

droxide had the capacity to induce physiologic closure of immature pulp­

less teeth.

Crabb (88) in 1964 used a mixture of calcium hydroxide and dis­

tilled water to achieve apical closure in immature teeth. He stated that

mechanical cleansing of the root canal is of major importance in the suc­

cess of root canal treatment.

Friend (42) in 1966 treated eighty-seven necrotic teeth with open

apices by first providing symptomatic therapy until the teeth were com­

fortable and a negative culture obtained. Then he filled the canals with

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Diaket and placed a permanent restoration. He reported continued root

growth or calcification across the end of the root filling material in

twenty of the eighty-seven cases treated.

In 1966 Rule and Winter (68) achieved sealing of immature apices

with calcified material after filling the canal with a resorbable iodo­

form paste or a polyantibiotic paste for seven months. They suggested

the final gutta-percha root filling could then be inserted one to two

millimeters short of the apex. One year recall radiographs revealed

closure of the root apex by calcified material.

Bouchon (89) in 1966 treated the acute symptoms of an abscessed

incisor in an eight year old boy. Following canal sterilization, Wal­

koff's iodoform paste was inserted halfway to the apex. Apical closure

was seen fifteen months later and conventional root canal therapy with

gutta-percha and a sealer was performed. A one year recall radiograph

showed complete healing.

Based on the osteogenic potential (90,91,92,93) and antibacterial

properties (94) of calcium hydroxide, Frank (58) in 1966 gave a course

of therapy to resume apical development based on normal physiological

patterns. The root canal could then be obliterated by conventional

lateral condensation techniques. He noted that the prime effort was to

reduce the canal contaminants by biomechanical instrumentation and medi­

cation followed by the partial reduction of the root canal space with a

resorbable paste seal of calcium hydroxide and camphorated parachloro­

phenol. He has noted four basic patterns of apical development: (a)

normal development continues; (b) an obliterated apex results without

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18

any change in the size of the root canal; (c) despite the lack of radio­

graphic evidence, an instrument inserted into the canal will feel a defin­

ite stop which ensures that a thin calcific bridge has formed; and (d) a

radiographically demonstrable calcific bridge forms slightly coronal to

the apex (see diagram page 19). Any of these four results is considered

successful as it permits obturation of the root canal with gutta-percha

and a sealer. Frank (61) and Frank and Weine (95) re-emphasized the im­

portance of this technique and extended its usefulness to nonsurgical

treatment of the perforative defect of internal resorption.

Day (96) in 1967 treated a pulpless incisor of a ten year old girl

until he obtained a negative culture. He then filled the canal with cal­

cium hydroxide paste and a six month recall radiograph revealed a calci­

fied barrier at the apex. He then filled the canal conservatively with

gutta-percha.

In 1967 Michanowicz and Michanowicz (67) treated immature pulpless

teeth by first treating the acute symptoms and obtaining two successive

negative cultures. Then they placed a paste of calcium hydroxide and

sterile water at the apex with a plugger followed by filling the remainder

of the canal with gutta-percha and a sealer. They presented several cases

illustrating root end closure of immature teeth so treated.

The use of the apexification technique has been advocated in the

recent dental literature (31,97,98). Successful case reports have been

given using calcium hydroxide mixed with various vehicles including cam­

phorated parachlorophenol (20,33,63,79,95,99,100,101,102), methyl cellu­

lose (66,103,104), water (40,105,106,107,108), Ringer's solution (18,103,

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SUCCESSFUL CLINICAL RESULTS OF APEXIFICATION PROCEDURES

(a) normal root maturation

(c) clinical barrier but no radiographic evidence

Q

'1\. §)'

I ~·

(

u (b) apex closes but canal retains

divergent configuration

(d) radiographic barrier short of apex

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109,110,111), metacresol acetate (62,76), and iodoform (110,111). Suc­

cessful reports of apexification on immature human teeth have also been

published using a zinc oxide-metacresol acetate-camphorated paramono­

chlorophenol mixture (35), iodoform Chlumsky paste (82), and a trical­

cium phosphate resorbable ceramic (112). Nevins (113) has reported the

induction of hard tissue formation within the root canal of a human pulp­

less immature tooth using a collagen-calcium phosphate gel. Barker and

Mayne (114) reported three cases of natural apexification in the absence

of any treatment subsequent to trauma. Shusterman (115) presented the

unsuccessful long term result of the reverse filling and replantation of

an avulsed immature incisor.

HISTOLOGICAL REPORTS OF APEXIFICATION IN HUMAN TEETH.

The first report on the histological nature of the newly formed

apex of a huma~ tooth was published by Heithersay (66) in 1970. The

development of a vertical fracture necessitated extraction of this tooth

which had been successfully ·apexified previously. The newly formed

apical barrier was a mixture of pulpal tissue remnants, and regular and

irregular interglobular dentin covered by thick layers of cellular and

acellular cementum with attached periodontal membrane. Cvec (18) and

Citrome (116) speculated that the surviving pulpal remnants were respon­

sible for the repairative dentin formation seen in this tooth.

Holland, Souza and Russo (74) in 1973 induced root end closure using

a mixture of calcium hydroxide and iodoform in six teeth for thirty days

before extracting these teeth for orthodontic reasons. Histological ex­

amination of the apical barrier revealed a mixture of osteodentin and

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cellular cementum.

Klein and Levy (76) in 1974 presented a case report of a successful

root end induction procedure using a mixture of calcium hydroxide and

metacresol acetate. Then the canal was filled with gutta-percha and

sealer but a gross overfill led to a subsequent root resection. Histo­

logical examination of the root apex revealed a mixture of cellular and

acellular cementum.

Cvec and Sundstrom (117) in 1974 studied the histological nature

of the apex of twelve human teeth extracted for orthodontic or prosthet­

ic reasons following root end closure using a paste of calcium hydroxide

and saline. The apical barrier consisted of cementum-like tissue as

well as the presence of calcified areas similar to that induced by cal­

cium hydroxide implanted in the subcutaneous tissues of rats as reported

by Mitchell and Shankwalker (90). A similar finding was reported by Ham,

Patterson, and Mitchell (72,73) in root end induction experiments on im­

mature teeth in primates.

Piekoff (79) in 1976 described a case report of the successful root

end closure of an abscessed immature incisor using a mixture of calcium

hydroxide and camphorated parachlorophenol. The tooth was extracted and

examined histologically following fracture of the tooth which occurred

during post and core preparation. The calcified cap was highly irregular

and showed intermingling of a number of tissues including bone and cemen­

toid.

In 1977 Holland, Mello and Nery (118) extirpated the pulps of

twenty mature vital human teeth and inserted a calcium hydroxide paste.

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--

The teeth were extracted from two to eighteen days later. They showed

that calcium hydroxide maintains the vitality of the apical pulp stump

and induces apical closure by a cementum-like hard tissue deposition.

However, Weinstein and Goldman (119) performed a similar procedure on

five adult monkeys but they waited for up to three hundred and thirty

days before examining the apical tissues histologically. They found

there was no apical bridging by calcified tissue, and thirty-seven of

forty teeth treated showed periapical inflammation and granuloma forma­

tion. They concluded the metabolism of the mature apex is different from

the immature apex and that calcified tissue will not form at the mature

apex in response to calcium hydroxide as it will in the immature apex.

Vojinovic (82) in 1977 reported on the histological nature of the

apices of four immature human teeth extracted for orthodontic or prosthet­

ic reasons which previously had root end induction procedures by a variety

of methods. Two of these teeth were treated with iodoform Chlumsky paste:

one tooth had a vital pulp extirpation subsequent to trauma while the

other had a necrotic pulp and acute apical periodontitis. Histological

examination of these two teeth revealed identical apical barriers com­

posed of a conglomerate of cementum and immature bone with small cavities

filled with undifferentiated soft tissue. Another tooth with an acute

apical periodontitis was treated by an induced blood clot which led to

the formation of a calcified apical barrier composed of irregular dentin.

They concluded the structure of the apical barrier does not depend on the

kind of paste used to fill the canal nor on the degree of pathological

changes present in the periapical tissues. The fourth tooth had a mortal

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extirpation of the pulp using arsenic and no further apical development

occurred.

Due to the difficulty in performing controlled studies on humans

for histological examination of block sections or extracted teeth, a

series of investigations on animals were performed to learn more about

the mechanism and nature of the apexification process. Monkeys and dogs

have been used as experimental models.

APEXIFICATION STUDIES IN PRIMATES

The first primate study was published by Steiner and Van Hassel

(120) in 1971. They selected the rhesus monkey as an experimental model

since it is closely related to man and the experimental results would be

more comparable to actual clinical practice. In order to test their ex­

perimental apexification procedure under the most unfavorable situation

likely to be encountered clinically, the pulps of the experimental teeth

of five rhesus monkeys were macerated and innoculated >vith Streptococcus

faecalis and the occlusal access cavities were sealed with a temporary

restoration. Three months later, periapical radiolucent lesions had de­

veloped. Then the teeth were debrided and a paste filling of calcium

hydroxide and camphorated parachlorophenol was inserted into the root

canals. The monkeys were sacrificed nine months later and an apical bar­

rier was present in eight out of nine experimental teeth. Histological

examination showed that the apical hard tissue bridge was cementum while

serial sections gave the impression that cementum formation proceeded

from the periphery of the apex to the center of the root in a series of

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decreasing concentric rings. Complete apical closure did not occur as

there was still continuity between the original root canal and the perio­

dontal ligament.

Dylewski (70) in 1971 overinstrumented eight immature incisors of

24

a single rhesus monkey and immediately placed a dressing of calcium hy­

droxide and camphorated parachorophenol. Histological examination seventy­

one days later revealed granulation tissue repair of bone defects and peri­

apical destruction. Instead of a continuation of normal root development

guided by Hertwig's sheath, the repair process occurring at the apex was

characterized by proliferation and differentiation of the apical connec­

tive tissue into a calcified material identified as osteodentin. Dentinal

tubules were not seen and the gro~vth pattern was trabecular and continuous

with the predentin on the canal wall. Complete apical closure was not

seen in any of the experimental teeth. Dylewski found it was not possible

to correlate the histological repair process with the radiographic find­

ings. This finding agreed with Spedding, Mitchell, and McDonald (121)

who showed that radiographic interpretation of calcified repair is mis­

leading.

In 1972 Ham, Patterson, and Mitchell (72,73) reported on the com­

parison between a calcium hydroxide-camphorated parachlorophenol mixture

and an induced blood clot as apexifying agents in four young monkeys. The

experimental teeth were left open to saliva for three days and then sealed

for two months to create chronic infection and periapical lesions before

the root end induction procedures were started. Apical bridge formation

four months later was seen more often and in greater amounts with the

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calcium hydroxide mixture. However, both methods showed incomplete apical

closure composed of cellular cementum and no evidence was found of Hert­

wig's sheath guiding this apical development. They found if pulpal ne­

crosis was incomplete, a more normal type of root continuation could be

expected. They also reported that a negative culture gave a much better

prognosis for continued apical development since no teeth with positive

cultures showed apical closure. A vital dye was used after filling the

teeth to demonstrate calcified tissue formation after treatment of the

immature teeth.

Attempting to determine the biological effects of endodontic pro­

cedures on developing incisor teeth, Torneck, ~ al., (37,80,122,123)

conducted an extensive series of experiments on young monkeys as follows.

In 1970 Torneck and Smith (37) described the effect of partial and

total pulp removal of five immature incisor teeth in a female monkey.

They performed a total pulpectomy on three teeth and partial pulpectomy

on two teeth. They sealed the access cavities with amalgam and sacri­

ficed the animal about one year later. Following histological examina­

tion of the experimental teeth, they concluded that root formation after

total pulpectomy may occur but this growth is irregular and retarded.

When most of the pulp was removed, the alveolar bone of the fundus ten­

ded to grow into the apical end of the canal. Any calcific bridging of

the apex was related to the ingrowth of bone rather than the deposition

of dental hard tissues. The presence of pulpal tissue in the apical

part of the root canal indicated the regenerative capacity of this tissue

as well as the difficulty in removing all pulpal remnants during

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debridement procedures. Here there was an acceleration in the rate of

foraminal closure by irregular dentin without a proportionate increase

in root length. Subsequent breakdown and necrosis of these pulpal rem­

nants led to apical abscess formation and root resorption. The partial

pulpectomy procedure in two teeth resulted in later necrosis of the re­

maining vital tissue and periapical abscess formation. There was no

evidence of root end closure after partial pulp removal.

In 1973 Torneck, Smith, and Grindall (80) showed that it was pos­

sible to create periapical lesions in the immature incisors of four mon­

keys by leaving the teeth open to salivary contamination for time periods

ranging from seven to ninety-five days. Despite evidence of rather

severe and extensive disease in the periapical tissues, some potential

for continued root formation and apical closure remained. The source of

the repair tissue was related to residual odontogenic cells of the pulp

and periapical tissue which grew into the pulp space. The apical barrier

which formed was an irregular deposition of dentin, cementum and bone.

26

As a result of the Torneck study, Citrome (116) speculated that the mon­

key has great recuperative powers and may not be a suitable animal model

for apexification studies.

In a subsequent study in 1973, Torneck, Smith and Grindall (122)

left immature incisors of six monkeys open to salivary contamination for

periods of fourteen to ninety-two days. Then the teeth were instrumented,

irrigated, dried, and medicated with camphorated parachlorophenol before

sealing with amalgam. The experimental teeth were examined histologically

after time periods varying from fourteen to sixty-three days. They found

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a lesser degree of postoperative root formation and apical closure when

medicating the canals and sealing the access cavities as compared with

leaving the canals open to saliva as done in a previous study (80). They

stated that when the pulp and periapical tissues of an immature tooth

are severely injured and infected, a purulent exudate may form. Leaving

the tooth open will provide a pathway for drainage of this exudate. How­

ever, sealing this canal in the presence of this exudate, or factors

resulting in its formation, can be detrimental rather than beneficial

to the apexification process.

27

In a fourth study by Torneck, Smith, and Grindall (123) in 1973,

thirteen immature incisors in five monkeys were left open to salivary con­

tamination for varying periods of time from thirty-nine to 196 days.

Following biomechanical preparation, a dressing of calcium hydroxide and

camphorated parachlorophenol was placed in the root canals and the access

cavities sealed with amalgam. Histological examination from forty-nine

to 194 days later showed apical barriers composed of irregular dentin,

cellular cementum and bone were present in ten out of thirteen experi­

mental teeth. Furthermore, the root end closure was more advanced than

when no treatment was provided (80) or when medication and a temporary

seal was used (122). Hence, the use of a calcium hydroxide and cam­

phorated parachlorophenol mixture as a temporary paste seal will accel­

erate the apexification process. However, they showed that the presence

of a closed apex is not indicative of a normal periodontium. Moderate

to severe inflammation which remained in the periodontal space was re­

lated to residual debris in the main canal and necrotic tissue in the

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spaces and crevices of the apical bridge.

Narang and Wells (77) in 1973 implanted decalcified allogeneic

bone matrix into surgically prepared cavity preparations in the apices

of monkeys teeth. They showed new cementum formation within the canals

and indicated that an implanted material which is acceptable to the host

will cause cementogenesis in the tooth apex. Nevins (78) points out

that this material is difficult to prepare so that it will conform to

the shape of the root canal for an apexification procedure.

Myers and Fountain (124) instrumented immature incisors of four

monkeys and left them open to salivary contamination. Then they reinstru­

mented the teeth and filled them with either an induced blood clot, whole

blood, or saline before closing these teeth with a cavit seal. They

found that ingrowth of connective tissue into the root canal space of

monkeys did not occur as Ostby (64) had shown in dogs. They felt this

was due to residual infection in the dentinal tubules which was toxic to

tissue growth. Six immature cuspids which were left open to salivary

contamination for the duration of the experiment showed apical closure

or bridging by a cementoid-osteoid type of tissue. Like Torneck (80),

they showed that apexification in immature monkey teeth will occur in

the presence of salivary contamination.

Koenigs,~ al., (125), in 1975 simulated the conditions of an

open apex by overinstrumenting through the apex of twenty mature teeth

in four monkeys. They filled the apical three millimeters of the canals

with a tricalcium phosphate resorbable ceramic. The rest of the canal

was filled with laterally condensed gutta-percha followed by a temporary

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seal. Histological examination two to twenty-four weeks later revealed

incomplete apical barriers had formed which resembled cementum. Regen­

eration of the periodontal ligament occurred and a minimal inflammatory

response was seen. They concluded there was no trapped debris in the

apical bridge when using this ceramic which differed from Torneck's (123)

results using a calcium hydroxide mixture. Driskell (126) has used this

ceramic as a tissue implant in experimentally created bone defects in

dogs. As the ceramic resorbs, new tissues can proliferate and calcify

to replace the ceramic. This process is accompanied by a remarkably low

inflammatory response.

In 1975 Nevins,~ al., (78), used polyethylene tubes with one

open end of three millimeters diameter to simulate an open apex. These

tubes were filled with a gel composed of native calf skin collagen fibrils

and mineral solutions and implanted into the subcutaneous connective tis­

sue of rats. Histological examination after eight weeks showed that the

collagen-calcium phosphate gel was capable of inducing cellular differen­

tiation and mineralized scar tissue formation.

In 1976, Nevins,~ al., (127), conducted a short term three month

study of immature teeth filled with collagen-calcium phosphate gel in

four monkeys. They showed the gel acts as a resorbable substrate and in­

duces hard tissue ingrowth to effect a physiologic closure of the root

canal space. Histological examination revealed that this tissue was a

vascularized cellular osteoid or cementum with pulpal remnants and osteo­

dentin. A periodontal ligament was usually formed at the apex and no

ankylosis between tooth and bone was observed. During this study,

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Donlon (128) took blood samples from the monkeys every four weeks to see

if the gel induced a humoral immune response. Gel diffusion and hemag­

glutination tests showed that no antibodies were produced in response to

the collagen-mineral gel. He explained that this may not be a lack of

response by the immune system, but rather an active process of T-cell

suppression of B-cell function.

Nevins, et al., (129), in 1978 conducted a long term primate study

comparing the collagen-calcium phosphate gel with calcium hydroxide. They

used six monkeys and sacrificed three at three months and the other three

at ten months. They found an equal rate of success since five out of

seven using calcium hydroxide and fifteen out of twenty-one teeth using

the gel showed continued apical development. Unlike the gel, calcium hy­

droxide did not induce hard tissue ingrowth into the root canal space.

They postulated that the collagen fibers are chemotactic for host fibro­

blasts and also form a microscaffold capable of supporting cellular mi­

gration. The mineral crystals may serve as a nidus and seed connective

tissue ingrowth which contributes to its ultimate mineralization.

Heide and Kerekes (130) performed pulpectomy procedures on eight

immature monkey incisors. They immediately inserted a calcium hydroxide

paste and a temporary seal. Three months later, five out of the eight

experimental teeth showed an apical barrier of hard tissue.

APEXIFICATION STUDIES IN DOGS

The first study using dogs as experimental animals was performed

by Camp (131) in 1968. He compared the rate of apical development in

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young dogs' teeth using two different pastes and found that a mixture of

calcium hydroxide and camphorated parachlorophenol was slightly more

effective than a paste of calcium hydroxide and distilled water.

Torneck and Tulananda (132) in 1969 created experimental abscesses

in mature dogs' premolar teeth by extirpating the pulp and leaving these

teeth open to saliva for twenty to one hundred and eighteen days. Histo­

logical examination of these teeth showed that osteodentin was present

in the apical portion of the tooth and this represented an attempt to

effect hard tissue repair in teeth whose pulps had not been completely

removed or destroyed. They showed that it was very difficult to com­

pletely remove all pulp tissue during pulpectomy procedures in dogs'

premolar teeth.. They also provided evidence that no repair occurred

in regions where pus accumulated or where the infla~matory exudate was

intense.

In 1971 Holland,~ al., (133) exposed immature dogs' teeth to the

oral environment following a pulpectomy procedure. They filled the

teeth with calcium hydroxide alone or in combination with iodoform. In

eighty percent of the experimental teeth, a bridge of hard tissue formed

which was composed of cementum and/or irregular dentin. The treatment

pastes worked equally well.

Binnie and Rowe (134) in 1973 studied the effects of calcium hy­

droxide and water, calcium hydroxide and blood salts, and Grossman's

root canal sealer on the periapical tissues of pulpless teeth of young

beagle dogs. Sixty eight premolar canals were opened and the pulps re­

moved. Twenty-eight canals were filled immediately with one of the

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three materials while the remaining forty canals were left open to

saliva for one week before filling thirty of these canals with one of

the three materials. The teeth were examined histologically at periods

ranging from one to sixteen weeks. Calcium hydroxide alone 1vas found

to produce the fewest and least severe inflammatory responses in the

periapical tissues and the highest percentage of successful apical

closure. Furthermore, they found the percentage of successful treat­

ments was similar for both the immediate and delayed calcium hydroxide

groups. They stated that calcium hydroxide and water seemed particu­

larly effective in infected environments. They speculated that it

could be due to some bactericidal effect of calcium hydroxide in the

tissues. Binnie and Rowe (135) also showed that the use of calcium

hydroxide does not stimulate epithelial proliferation in the periodontal

space of dogs' premolars. Calyxyl and Grossman's root canal sealer were

less successful in inducing apical closure and were associated with a

higher incidence of severe periapical inflammatory response.

In 1975 Mager (136) compared the effects of calcium hydroxide

with resorbable tricalcium phosphate to close experimentally created

open apices in dogs' teeth. After five months, an acute inflammatory

reaction with no evidence of apical closure was present in the teeth

treated with the ceramic. This result is vastly different from Koenigs'

(125) study using monkeys. In the calcium hydroxide treated teeth, a

mild chronic inflammation vJas present and calcification was observed

at the perforation sites.

In 1974, Vojinovic (36) removed the pulps of young dogs premolars.

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Some of the canals had iodoform-Chlumsky paste added immediately while

the other canals were left open to saliva for one week before inserting

the same paste. Histological examination of these teeth from forty­

five to two hundred and sixty-five days later revealed that the root

ends had closed but in overall length they were shorter than the un­

treated contralateral teeth. The apices were closed by an irregular

calcified mass of cementum, osteodentin, and immature bone. This tis­

sue was a product of the formative activity of cells originating from

the successive differentiation of fibroblasts in the young granulation

tissue in the periapex. He stated that the structure of the apical

part of the root depends primarily on the presence or absence of the

radicular pulp.

In 1975 Vojinovic (137) compared the root end induction qualities

of calcium hydroxide with the iodoform-Chlumsky paste in pulpless im­

mature premolars of six dogs. After the treatment pastes were inserted,

half the dogs were sacrificed two months later while the other three

dogs were sacrificed seven months later. He found that calcium hydrox­

ide was more effective since apical closure was more rapid and complete.

The apical barrier formed using calcium hydroxide was more compact,

larger, and penetrated further into the apical part of the root canal.

The iodoform-Chlumsky paste was a chronic irritant as revealed by the

larger number of lymphocytes, plasma cells, and occasional mast cells

seen adjacent to the paste.

England and Best (71) in 1977 removed the pulps of forty immature

premolars in seven dogs. One half of the teeth were sealed with cavit

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after being exposed to saliva for one week while the remaining twenty

teeth were left open to salivary contamination for the duration of the

experiment. The dogs were sacrificed seven to eleven weeks later for

histological examination of the experimental teeth. Apical closure by

a calcified bridge of cellular cementum occurred in eighty-six percent

of the open group and fifty percent of the closed group. Like Torneck

(122), he felt the smaller incidence of success in the closed group was

due to the lack of a pathway for drainage of an inflammatory exudate

which accumulated in the root canal and periapical tissues and impeded

the apexification process. He also showed that apical closure in im­

mature dogs' teeth will occur in the presence of periapical lesions

without the insertion of a treatment paste. He concluded that host re­

sistance could be much greater in dogs than in humans.

Citrome (116) in 1977 compared the effects of calcium hydroxide,

collagen-calcium phosphate gel and the formation of a blood clot as

inducers of root end closure in immature pulpless teeth in two dogs.

Following the removal of pulpal tissue and the insertion of the treat­

ment pastes, a vital dye was used to identify post-operative calcifica­

tions. He found that all teeth treated with calcium hydroxide showed

apical calcifications three months later with a mild if any inflammatory

reaction present. However, the teeth treated with an induced blood clot

or the collagen-calcium phosphate gel showed severe inflammatory reac­

tions and little evidence of apexification. He pointed out that all

materials tested so far in monkeys have been successful, but not so in

the dog. He concluded that the dog was a more sensitive animal and

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hence the appropriate animal model for apexification studies.

THE ROLE OF pH IN INFLMINATION

The acidity or alkalinity of a solution is an expression of the

relative proportions of hydrogen and hydroxyl ions present. Sorenson

(138,139) in 1909 related the concentration of hydrogen ions in a solu-

tion according to a scale running from zero to fourteen with the mid-

point seven being neutrality, i.e., where there are equal concentrations

of hydrogen and hydroxyl ions. This scale defined pH as the negative

log of the hydrogen ion concentration in grams per litre (i.e. pH=

+ -log10

[H ]). Hence the pH of pure water is seven. By adding an acid

to a neutral solution, the concentration of hydrogen ions increases and

the pH decreases. By adding a base to a neutral solution, the number

of hydroxyl ions increases with a corresponding decrease in the hydrogen

ion concentration. The net effect is an increase in pH and the solution

becomes alkaline.

According to Menkin (140), normal tissue pH in humans is slightly

alkaline with a range of 7.2 to 7.4. Wolpert,~ al., (141) indicated

that the normal tissue pH in mongrel dogs varies from 7.1 to 7.2 and

parallels serum pH. Glinz and Clodius (142) have stated that tissue pH

measurement can be used as a circulatory test to determine whether the

oxygen supply to tissues is sufficient for normal aerobic metabolism.

In aerobic metabolism, glucose or glycogen is transformed into pyruvic

acid which enters Krebb's cycle to supply further sources of energy.

However, insufficient blood supply results in a relative lack of oxygen

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and tissue cells will be forced into anaerobic metabolism. Anaerobic

glycolysis converts pyruvate into lactic acid which results in an in­

creased lactate concentration in tissues (141). Blood stasis with

increased carbon dioxide concentration is an additional factor adding

to the tissue acidosis. Goldstein (143) reported that poor diffusion

properties of necrotic tissue will limit access to growth substances

and elimination of growth products. Furthermore, phagocytic cells

called to the area will undergo a respiratory burst of glycolysis during

the ingestion of particles and decrease the pH within the phagocytic

cells (144). Some phagocytic cells, especially polymorphonuclear leuko­

cytes, will succumb as the pH of an exudate falls (140) and release

their acidic contents to further lower the pH. All of these factors

are important in the acute inflammatory process.

The acute inflammatory reaction is a dynamic phenomenon which is

initiated at a normal alkaline tissue pH. According to ~fenkin (140),

in an acutely inflamed area there is a blockage or damage to vascular

channels. Due to decreased tissue perfusion, cellular energy is obtained

by anaerobic glycolysis which results in the formation of lactic acid.

This lactic acid production is mainly responsible for the changes in

local pH of the exudate. The polymorphonuclear leukocytes are the

first cells to arrive in the early stages of inflammation. Menkin re­

ported that as the pH drops below 6.8, the polymorphonuclear leukocyte

succumbs and is replaced by the macrophage. As the pH drops below 6.5,

all leukocytes either die or display signs of severe cell injury which

results in pus formation. He concluded that acute inflammation may be

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considered a function of the hydrogen ion concentration. However,

an old focus of pus may have an alkaline pH. Menkin stated:

"in a very old focus, e.g., as seen in a cold abscess or

in an old inspissated suppurative lesion, the pH of such

material may actually be alkaline in nature."

This is because proteolysis is also a cardinal feature of inflammation.

He stated that breakdown of proteins and the production of amines and

ammonia will eventually result in an. alkaline suppurative focus in

chronic inflammation.

When an acute inflammatory focus enters into the repairative phase,

there is an increase in the local vascularity of the inflamed area and

the pH of the exudate again becomes neutral or slightly alkaline. In

animal studies, Menkin (140) has shown that if an alkaline pH is main­

tained in a wound, granulocytes will migrate to the site and resolution

will be rapid.

Mitchell and Shankwalker (90) and Yoshiki and Mori (145) have

confirmed the ability of calcium hydroxide to initiate ectopic calci­

fication. However, Pisanti and Sciaky (92,93) have shown that the cal­

cium in the hard tissue barrier was derived from the serum and not from

the calcium hydroxide paste used. Numerous investigators (27,66,96,97,

145,146) suggest that the high hydroxyl ion concentration may be the

factor that induces calcification. Furthermore, Tronstad (147) states

that the success of calcium hydroxide in counteracting inflammatory re­

sorption may be due to its high pH. Tronstad, ~ al., (148) report that

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the optimum condition for hard tissue resorption is an acidic pH where

acid hydrolases are active and demineralization takes place. An in­

crease in pH will neutralize lactic acid and inactivate acid phosphatase.

They stated that an alkaline pH and the presence of calcium ions may

activate alkaline phosphatase which has been proposed to play a role in

hard tissue formation and the repair process.

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CHAPTER III

MATERIALS ru~D METHODS

Six healthy five month old purebred beagle littermates, each weigh-

ing between 7.1 and 9.3 kilograms, were used in this study. The animals

were obtained, treated and maintained at the Loyola University Medical

Center Animal Research Facility. The dogs were ear marked "QL", "QM",

"QP", "QQ", "QR" and "QT" to aid identification and kept in two cages,

the three males in one and the three females in the other cage. The an-

imals were under continuous veterinary supervision and maintained on a

diet of standard laboratory meal and water ad libitum.

RADIOGRAPHIC SURVEYS

Preoperative radiographs were taken to verify that apical closure

was not completed prior to treatment. Subsequent films were made during

each operative session and at the time of sacrifice. Following the ap-

propriate sedation or anaesthesia of the experimental animal, lateral

jaw radiographs were taken using a portable hand-held X-ray generator

giving sixty kvp. at twenty milliamperes using a 0.2 second exposure

time and an X-ray source-to-film distance kept close to twenty centi-

metres. Occlusal ultra-speed dental X-ray film* was used and developed

for twenty seconds in Insta-Neg**, fixed for forty seconds in Insta-Fix**

* Kodak DF-46, Eastman Kodak Company, Rochester, New York. ** Microcopy, Culver City, California.

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40

and ~vashed with water for five minutes in,a portable light-tight de-

veloping box.

SEDATION AND ANAESTHESIA

Each animal was premedicated with an intramuscular injection of

one cc. of Inovar Vet* per seven to nine kilograms of body weight to

sedate the animals and make them more manageable.

At the same time the tranquilizer was administered, the dogs re-

ceived subcutaneous injections of one cc. of Atropine Sulfate Injection

U.S.P.** (0.5.mg./ml.) to limit salivary flow and facilitate operative

procedures.

When anaesthesia of surgical depth was required following sedation,

a foreleg was shaved with electric shears, the large anterior vein lo-

cated, and an intravenous injection of Sodium Pentobarbital Injection***

(65 mg./ml.) was administered. This i~~ediate acting barbiturate was

injected slowly to obtain adequate anaesthesia as determined by the loss

of pedal and corneal reflexes and passage through the excitory stage to

deep, regular respiration. The average dosage needed to achieve this

level was approximately two cc. and provided about one to one and one-

half hours of working time. Maintenance doses of one cc. were given as

needed,

*Pitman-Moore, Inc., Washington Crossing, New Jersey. 1'1' Hed Tech, Inc. , Elwood, Kansas. *** W.A. Butler Company, Columbus, Ohio.

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41

PREOPERATIVE PREPARATION

The animals were obtained at an age of 120 days to ensure that the

premolar teeth were not fully developed. When a radiographic survey was

taken on one of these dogs at the age of 126 days, the primary premolars

were still present and the permanent premolars were seen in an early pre-

eruption stage. Subsequent visual and radiographic examinations followed

the loss of primary premolars and eruption of the permanent premolars.

Radiographs taken when the dogs were 170 days old (Figure 1) verified

that the fully erupted permanent premolars still had incompletely de-

veloped root apices and that the operative phases of this study could

begin.

The preparation of a broth containing a kno•vn concentration of

Streptococcus faecalis microorganisms was prepared in order to deliver

a known number of organisms to each experimental tooth. A human isolate

of this organism, maintained in a refrigerated tube with a solid media

slant of Trypticase Soy agar, was supplied by the Loyola University

Dental School Department of Microbiology. A sample of this culture,

sent to the Loyola University Hospital, was identified as a gamma

hemolytic variety of Streptococcus faecalis. An inoculate of this cul-

ture was transferred to a flask containing Brain-Heart Infusion broth

and incubated for fourteen hours. Then, the optical density of 0.24

of this broth culture was determined using a spectrophotometer and a

Brain-Heart Infusion broth blank. Successive dilutions of this broth

culture in sterile water were prepared and equal volumes from each di-

lution tube spread out onto Trypticase Soy agar plates. These plates

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were incubated for twenty-four hours at 37°C. The number of colonies

per plate was determined and the dilution factor applied to determine

the concentration of microorganisms in the fourteen hour broth culture.

A solution containing Streptococcus faecalis organisms having an optical

density of 0.24 was determined to contain 2.63 x 10 8 organisms per mill­

iliter.

The day before the initial operative procedure on each dog, a

flask containing Brain Heart infusion broth was inocculated with Strep­

tococcus faecalis organisms and incubated overnight for fourteen hours.

The broth culture was then centrifuged and the supernatant fluid dis­

carded. The remaining pellet of microorganisms was washed in sterile

saline and centrifuged before discarding the supernatant fluid. This

procedure was repeated three times to remove any remaining media solu­

tion. The final pellet of microorganisms was resuspended in saline and

diluted until an optical density of 0.24 was obtained against a saline

blank. This saline solution now contained 2.63 x 10 8 Streptococcus

faecalis organisms per milliliter and could be used for innoculation

during the first operative procedure on each dog treated that day. This

method was repeated each day during the initial operative procedures.

INITIAL OPERATIVE PROCEDURE

Due to the length of time needed for the first treatment session,

two animals were operated on each of three consecutive days. All animals

received identical therapy. The first two animals, at the age of 169

days, were premedicated, weighed, prepared for treatment and anaesthetized

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to the desired effect as described previously. Radiographs were taken

followed by a clinical periodontal examination in order to obtain ini­

tial records. A mild gingivitis, typical for this age and breed of dog,

was present, but there was no evidence of calculus deposits or perio­

dontitis. The maxillary and mandibular second and third premolar teeth

were used which provided a total of sixteen wide open root apices in

each of the six animals.

The maxillary right second and left third premolars, termed the

"control" teeth, had no operative procedures performed in order to ob­

serve normal root development. The mouths of the animals were held

open with a spring loaded mouth prop and coronal access was gained into

the pulp chambers of the remaining experimental teeth using a sterile

#556 carbide bur in a high speed handpiece. The length of the canals

was determined radiographically with endodontic files in place as des­

cribed by Weine (1).

A pH determination of the periapical tissue immediately adjacent

to the apical foramen was taken using pH microelectrodes (see page 44)

and a standard laboratory pH meter. During this procedure, the glass

standard Ml-408 microelectrode*, which was protected by a bevelled

stainless steel sleeve, was inserted into the root canal to the level of

the apical foramen in order to establish contact with periapical tissues.

The calomel reference 111-402 microelectrode*, its' tip coated with

* Microelectrodes, Inc., Londonderry, New Hampshire.

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44

PHOTOGRAPH OF Eli MICROELECTRODES (actual size)

LEGEND

G - Glass standard microeiectrode C - Calomel reference microelectrode

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EKG gel* to aid conduction, was placed on the buccal attached gingiva

in the region of the tooth being tested. The pH was measured following

a one minute period of stabilization for the pH meter. Calibration of

the electrodes prior to, and following, insertion of the electrodes was

performed using standard buffers of pH four, seven and ten.

Under radiographic control, the pulps were removed using barbed

broaches, Hedstrom files, and copious sterile saline irrigation. Great

care was taken to remove as much of the pulpal tissue as possible to the

level of the radiographic apex without damaging the thin, friable den­

tinal walls of the root canal. Then, paper points were inserted to con­

trol hemorrhage and dry the canals.

In order to infect each of the experimental teeth with an equal

number of~· faecalis microorganisms, twenty-five microliters of the

freshly prepared saline and~ faecalis solution were drawn into a fifty

microliter pipette and inserted into the root canals. Hence, each tooth

was infected with approximately 675 ~· faecalis microorganisms. Cotton

pellets were placed in the pulp chambers and the teeth were double

sealed with a stop of base plate gutta-percha followed by Class I amal­

gam restorations. A radiographic survey was taken before the animals

were returned to their cages. Before beginning the second operative

session, a period of one week was allowed for the spread of periapical

infection.

* Redux Creme, Hewlitt-Packard Medical Electronics, Waltham, Mass.

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SECOND OPERATIVE PROCEDURE

The dogs were again treated in groups of two on three consecutive

days. Following appropriate anaesthesia, the premolar teeth were ex­

amined for tooth mobility and sinus tract formation. The restorations

were removed from the appropriate experimental teeth and a pH reading

was taken of the tissue slightly beyond the root apex. The root canals

were copiously irrigated with sterile saline, carefully instrumented

with endodontic files to remove any remaining soft tissue, and dried

with sterile paper points.

A thick acidic paste of methylcellulose, sterile water, and hy­

drochloric acid was mixed to a pH = 3 while an alkaline paste of methyl­

cellulose, sterile water, and sodium hydroxide was mixed to a pH 11.

The pH of these pastes was verified by a pH meter before they were

packed into five cc. disposable syringes. The acidic paste was in-

jected into the maxillary right third premolars and the mandibular left

second premolars while the basic paste was inserted into the maxillary

left second premolars and the mandibular right third premolars. No

attempt was made to keep the paste within the confines of the root canal.

Sterile cotton pellets were inserted into the pulp chambers and the access

cavities were sealed as before with gutta-percha and amalgam. Radiographs

were taken and each dog received an intraperitoneal injection of the vital

dye Procion Red H-8B* (lOOmg. per kg. of body.weight) dissolved in ten cc.

of sterile saline. This fluorescent vital'dye was used to demonstrate

* Polysciences, Inc., Warrington, Pennsylvania

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formation of any calcified tissue added to the apex after treatment of

these teeth.

The pattern of control and experimental second and third premolar

teeth in each dog is summarized in the following table:

3 2 2 3 c - control I - infected control

A c B c A - infected and acidic treated B - infected and basic treated

B I A I Total of six dogs

3 2 2 3 Total of sixteen canals per dog

SACRIFICE PROCEDURE

The six dogs were sacrificed at four different post-treatment in-

tervals: one female at one week; t~.;ro males at one month; one male at

three months; and two females at six mont:-,.::;,

The animals were anaesthetized, radiographed, and examined for

mobility, sinus tract formation, or exfoliation of the treated teeth.

The restorations were removed from all the experimental teeth and a pH

reading was taken of the apical region. Each animal was sacrificed by

giving an intravenous injection of five cc. of Beuthanasia-D*, a highly

concentrated solution of sodium pentobarbital, specifically designed for

rapid and painless euthenasia of animals within ten seconds after admin-

istration of the drug. The soft tissue was disected from the surrounding

* Burns-Biotec Laboratories Division, Chromalloy Pharmaceutical, Inc., Oakland, California.

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bone and jaw sections containing the experimental and control teeth were

removed using an electric reciprocating bone saw and immediately placed

in a ten percent neutral buffered formalin solution for fixation.

HISTOLOGICAL PREPARATION

Unnecessary hard tissue was removed with high speed burs to facil­

itate tissue fixation. The formalin solutions were changed every twenty­

four hours for the first few days and the specimens remained in formalin

for at least two weeks. The jaw sections were then removed from the

fixative and rinsed under running water for twenty-four hours.

The specimens were decalcified for four to five weeks in a solution

made up of equal parts of solutions of fifty percent formic acid and

twenty percent sodium citrate until they were radiographically radiolu­

cent and of a rubber-like consistency. They were trimmed with a razor

blade into blocks containing the premolar teeth and decalcified for sev­

eral more days to allow better penetration. The individual blocks were

dehydrated in increasing concentrations of alcohol, embedded in paraffin,

and seven micron sections were cut and mounted on glass slides. The

sections were deparaffinized, hydrated, and alternately left unstained

for fluorescent microscopy and stained with hematoxylin and eosin or

Masson's trichrome connective tissue stain for light microscopic examin­

ation. A complete radiological and histological examination and evalua­

tion of the reactions of the teeth and associated periapical structures

was conducted.

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CHAPTER IV

RESULTS

The dogs did not seem to suffer any ill effects from the operative

procedures and all animals appeared healthy with no serious weight loss

throughout the study.

CONTROL TEETH

Two maxillary premolars in each animal, which served as vital con­

trol teeth, displayed no adverse clinical signs throughout the study.

These teeth were not mobile and did not have any associated draining

sinus tracts.

Radiographic findings (Table I), in all animals at the beginning

of the study and in the one week animal at sacrifice, revealed that the

control teeth had open apices and the walls of the root canals were

widely divergent from the middle third of the root to the apex (Figures

1,2, and 3). The one month animals at sacrifice showed complete closure

of the apex in one canal, partial closure in four canals, while three

canals still had blunderbuss configurations (Figure 4). The apical de­

velopment of the distal root tended to lag behind that of the mesial

root. The apices of all control teeth were completely formed in the

three and six month animals at sacrifice (Figures 5 and 6).

Histological examination of the control teeth in the one week ani­

mal revealed an open apex, a healthy periodontal ligament, epithelial

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so

attachment, and surrounding alveolar bone (Figures 7,8, and 9). The

pulpal tissue consisted of loose connective tissue with a layer of odon­

toblasts lining the dentinal walls. Hertwig's epithelial sheath was

clearly seen as a two-cell wide band of epithelium running at right

angles to the long axis of the tooth toward the center of the tooth to

form an apical diaphragm. In the one month animals, similar findings

were evident in two of the four control teeth. The other t\vo teeth

showed partial apical closure and a mild pulpal hyperemia and congested

blood vessels were seen in the dental pulp (Figure 10). The three and

six month animals' control teeth had completed apical development. The

periodontal ligament was narrower and composed of dense fibrous con­

nective tissue. Reversal lines were evident in the cribriform plate.

Mild hyperemia was present in the pulpal tissue. The apical arboriza­

tion of the root canal was clearly evident with the main canal break­

ing up into a complexity of fine channels which radiate peripherally

through the apical cellular cementum (Figures 11 and 12). An absence

of an inflammatory response was evident in the periapical tissues of

the control teeth throughout the duration of this study.

INFECTED-ONLY TEETH

Two mandibular premolars in each animal, which served as infected

pulpless control teeth, had the pulps extirpated and were infected with

S. faecalis for the duration of the experiment.

The periapical tissue pH values (Table II) were recorded in all

experimental teeth at various intervals during the experiment. The

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average initial periapical tissue pH (Table III) of the infected-only

teeth in each animal ranged from 7.05 to 7.21 with an overall average of

7.12. The average periapical tissue pH at sacrifice ranged from 6.88 to

7.15 in the individual animals with an overall average of 7.04.

Clinical results (Table IV) show that all of the infected-only

teeth had a mobility of two or greater after the first week of infection

to the end of the experiment. The six month animals had exfoliated all

of the infected-only teeth while the rest of the animals still retained

these teeth at the time of sacrifice (Table V). There were eight out of

sixteen teeth after one week of infection and three out of twelve teeth

at the time of sacrifice that had draining sinus tracts (Table IV).

Radiographic findings (Table I) showed that all infected-only

teeth had periapical and bifurcation radiolucent lesions present after

one week of infection to the end of the study. These lesions did not

noticeably increase in size radiographically after one more week as seen

in the one week animal at sacrifice (Table VII). However, all other

radiolucent lesions did increase in size radiographically with in­

creasing post-operative sacrifice intervals. There was no evidence of

apical closure in any of the infected-only teeth (Table I).

Histological evaluation of the infected-only tee~h in the one week

animal revealed severe degenerative changes (Figure 13). No evidence of

vital pulp tissue or Hertwig's sheath was demonstrated. The epithelial

attachment remained and periodontal ligament was present in the coronal

two-thirds of the interproximal root surfaces. However, the attachment

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apparatus was totally lacking in the apical and bifurcation areas and

was replaced by a proliferating sling of epithelial tissue which was

two to four cells in thickness. Severe loss of periapical and furca­

tion alveolar bone was seen and these areas had a severe acute inflam­

matory infiltrate (Figure 14) consisting mainly of polymorphonuclear

leukocytes, with but a few mononuclear cells evident. No evidence of

dentin or cementum resorption was seen. The surrounding alveolar bone

was seen to be resorbing on the lesion side and bone deposition (Fig­

ure 15) was demonstrated on the non-lesion side.

52

In the one month animals, the loss of periodontal attachment was

more extensive. There were only isolated areas of periodontal ligament

attachment while the remaining areas were replaced by an epithelial sling.

This epithelial proliferation was well differentiated into a stratified

squamous epithelium of two to ten cells thick and rete pegs of loose con­

nective tissue were seen extending into the epithelium (Figure 16). A

basal layer or stratum germinativum and a prickle cell layer or stratum

spinosum were now evident. A chronic inflammatory infiltrate (Figure 17)

was seen in the subepithelial layers consisting of lymphocytes, plasma

cells, and macrophages. The alveolar bone in the furcation was nearly

absent (Figure 18) while bone apposition and resorption was seen on the

lesion side of the periapical alveolar bone. No resorption of dentin or

cementum was evident nor was any remaining evidence of Hertwig's sheath

seen.

In the three month animal, severe degenerative changes were seen in

histological sections (Figure 19). The epithelial attachment and most

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of the periodontal ligament were absent and replaced by a well differen­

tiated stratified squamous epithelium with rete pegs, basal layer,

prickle cell layer, and parakeratosis. Furcation and interproximal al­

veolar bone was virtually completely absent and a chronic inflammatory

infiltrate was seen in the subepithelial tissues. Neither Hertwig's

epithelial root sheath nor any evidence of dentin resorption were seen

at the root apex. The root canals were devoid of contents and the epith­

elial sling was noticed surrounding the wide open apical foramen and con­

tinuing along the sinus tract.

All of the six month infected-only teeth were exfoliated and heal­

ing of the sockets was complete. No histological evidence of apical

closure or apical calcification was seen at any time in the infected­

only teeth during this entire study.

INFECTED JU~D ACIDIC-TREATED TEETH

One maxillary and one mandibular premolar in each animal, which

served as the infected and acidic-treated teeth, were infected with

~· faecalis for one week following pulp extirpation before an acidic

paste (pH=3) was inserted into the root canal and surrounding periapi­

cal tissue for the duration of the study.

Table III lists the average periapical tissue pH values at various

intervals during this study. The average initial periapical tissue pH

of the acidic-treated teeth in each animal ranged from 7.03 to 7.20 with

an overall average of .7.12. The average periapical tissue pH of these

teeth in each animal after one week of infection ranged from 6.33 to 6.76

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with an overall average of 6.50. The average periapical tissue pH at

the time of sacrifice ranged from 6.92 to 7.12 in the individual animals

with an overall average of 7.01.

Clinical results (Table IV) showed that all of the acidic~treated

teeth had a mobility of two or greater after the first week of infection

to the end of the experiment. Three out of four of the acidic-treated

teeth were exfoliated in the six month animals while the rest of the

animals still retained these teeth at the time of sacrifice (Table V).

Draining sinus tracts were present in eight of the sixteen acidic-treated

teeth after one week of infection, and in five out of thirteen so treated

teeth at the time of sacrifice (Table IV).

Radiographic results (Table I) showed that all acidic-treated teeth

had periapical and bifurcation radiolucent lesions present after one week

of infection through to the end of the study. These lesions did not

noticeably increase in size after one more \veek as seen in the one week

animal at sacrifice (Table VII). However, all other radiolucent lesions

in the remaining animals did increase in size as the post-operative sacri­

fice interval increased. There was no radiographic evidence of apical

closure in any of the acidic-treated teeth (Table I).

Histological evaluation of the acidic-treated teeth in the one week

animal revealed severe degenerative changes (Figure 20). No evidence of

vital or necrotic pulp tissue was seen in the root canal, but the remains

of the acidic paste could be seen as a faint pink amorphous mass in some

sections. Viable epithelial attachment and periodontal ligament remained

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~ !

55

on the interproximal root surfaces of maxillary teeth but more severe

destruction was seen in mandibular teeth. Furcation alveolar bone was

nearly completely absent and severe loss of periapical bone was evident.

A sling of proliferating epithelial tissue three to five cells thick was

present in areas where the periodontal membrane was missing and the sub-

epithelial tissues had a severe acute inflammatory infiltrate consisting

mainly of polymorphonuclear leukocytes and occasional mononuclear cells.

The surrounding alveolar bone was seen to be resorpin~ on the side of

the periapical lesion and bone deposition was evident on the non-lesion

side.

In the one month animals, the loss of the periodontal attachment

apparatus was far more severe. One of the mandibular teeth which had

no periodontal ligament and was completely surrounded by a sling of epith-

lium was obviously ready to exfoliate. The remaining acidic-treated teeth

had only isolated areas of viable periodontal ligament attachment (Figure

22) and no evidence of an epithelial attachment. A well differentiated

epithelial sling surrounded most of the teeth and rete pegs and basal

and prickle cell layers were seen in these stratified epithelial bands.

Furcation alveolar bone was absent and only isolated spicules of inter-

proximal bone remained. The root canals were devoid of any tissue con-

tents but a collection of extravasated red blood cells was seen in the

apical region of one root and the remains of the acidic paste could be

seen as a faint pink amorphous mass in some of the roots. Small frag-

ments of the temporary filling material were also seen in some of the

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canals. No evidence of Hertwig's sheath or dentin resorption was seen.

There was a mild chronic inflammatory reaction seen in the subepithelial

tissues around the roots which consisted of lymphocytes, plasma cells,

and macrophages dispersed among the newly forming dense fibrous connec­

tive tissue. The surrounding alveolar bone showed evidence of apposi­

tion and resorption since osteoclasts and osteoblasts were seen on the

lesion side of the cribriform plate.

In the three month animal, severe degenerative changes were seen

in histological sections of the acidic-treated teeth. The epithelial

attachment and nearly all of the periodontal ligament were absent and

replaced by a stratified squamous epithelial sling with rete pegs, ba-

sal and prickle cell layers, and parakeratin on the surface. Furcation

and periapical alveolar bone were nearly absent and there was a moderate

chronic inflammatory cellular infiltrate in the developing lamina propria.

There was some amorphous appearing paste remnants in the root canals but

Hertwig's sheath and dentin resorption were not seen. One tooth had ex­

tensive epithelial proliferation around the apex with an adjacent cyst­

like area (Figures 23 and 24).

Only one of the four acidic-treated teeth remained in the six month

animals (Figure 25). This tooth had no epithelial attachment and only

one isolated area of periodontal attachment remained which indicated this

tooth would soon be exfoliated. There were no tissue remnants left in

the root canal but remnants of the amorphous acidic paste could be seen

in some sections. Root resorption or evidence of Hertwig's sheath were

not seen. The tooth was surrounded by a well differentiated stratified

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squamous epithelial sling and there was a severe chronic inflammatory

infiltrate in the subepithelial tissues 1vhich consisted mainly of lym­

phocytes, but plasma cells and macrophages were also present. Furcation

and interproximal alveolar bone were absent while the periapical alveolar

bone showed signs of osteoblasts laying down new bone.

No histological evidence of apical closure or calcification was

seen at any time in the acidic-treated during this study.

INFECTED AND BASIC-TREATED TEETH

One maxillary and one mandibular premolar in each animal, which

served as the infected and basic-treated teeth, were infected with S.

faecalis for one week following pulp extirpation before an alkaline

paste (pH 11) was inserted into the root canal for the duration of the

study.

Table III lists the average periapical tissue pH values at various

intervals during this study. The average initial periapical tissue pH

of the basic-treated teeth in each animal ranged from 7.03 to 7.15 with

an overall average of 7.11. The average periapical tissue pH of these

teeth in each animal after one week of infection ranged from 6.30 to 6.68

with an overall average of 6.48. The average periapical tissue pH at

the time of sacrifice ranged from 6.93 to 7.10 in the individual animals

with an overall average of 7.02.

Clinical findings (Table IV) revealed that all of the basic­

treated teeth had a mobility of two or greater after the first week of

infection to the end of the experiment. One out of two basic-treated

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teeth in the one month animal and three out of four basic-treated teeth

in the six month animals were exfoliated while the rest of the animals

retained these teeth at the time of sacrifice (Table V). Draining sinus

tracts were present in ten out of sixteen basic-treated teeth after one

week of infection, and in four out of eight so treated teeth at the time

of sacrifice (Table IV).

Radiographic results (Table I) showed that all basic-treated teeth

had periapical and bifurcation radiolucent lesions present after one

week of infection to the end of the study. These lesions did not notice­

ably increase in size after one more week as seen in the one week animal

at sacrifice (Table VII). However, all other radiolucent lesions in the

remaining animals did increase in size as the postoperative sacrifice

interval increased. There was no evidence of apical closure in any of

the basic-treated teeth (Table I).

58

Histological evaluation of the basic-treated teeth in the one week

animal revealed severe degenerative changes (Figure 26). No evidence of

vital or necrotic pulp tissue was seen in the root canal, nor was Hertwig's

epithelial root sheath or root resorption demonstrable at the root apex.

Viable periodontal ligament, alveolar bone and epithelial attachment were

present on the mesial interproximal root surface, but a chronic draining

sinus tract was seen along the distal interproximal root surface. Fur­

cation alveolar bone was nearly absent and a proliferating sling of epith­

elium surrounded the root surfaces that lacked periodontal membrane (Fig­

ure 27). Periapical alveolar bone showed signs of osteoblastic activity

but this deposition was on the nonlesion side. The subepithelial tissues

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contained a moderate acute inflammatory infiltrate consisting mainly of

polymorphonuclear leukocytes, but some lymphocytes, plasma cells, macro­

phages, and fibroblasts were present.

In the one month animals, one of the four basic-treated teeth had

exfoliated. Complete healing of the socket areas was evident but an un­

usual finding of an embedded piece of dentin was seen in the lamina

propria (Figure 28). There was no evidence of inflammation around this

dentin which indicated it was well tolerated by the animal. The rest of

the basic-treated teeth exhibited severe loss of the periodontal attach­

ment apparatus. The epithelial attachment was absent with only some of

the interproximal areas of periodontal ligament remaining (Figure 29).

59

A well differentiated epithelial sling surrounded most of the root sur­

faces and a chronic round cell infiltrate was present in the subepithelial

tissues. In one root canal, there was an evagination of the well differ­

entiated epithelium into the apical foramen while small pieces of tempo­

rary filling material could be seen in the root canal and surrounding

tissues (Figure 30). Another root apex showed evidence of cementum and

dentin resorption but no evidence of Hertwig's sheath was seen (Figure 31).

In the three month animals, severe degenerative changes were seen

in histological sections of the basic-treated teeth (Figure 32). The

epithelial attachment and most of the periodontal ligament were absent

and replaced by a stratified squamous epithelial sling with rete pegs,

basal and prickle cell layers, and parakeratin (Figure 33). Furcation

and periradicular alveolar bone were nearly absent and there was a mod­

erate inflammatory infiltrate and hyperemia in the subepithelial tissues.

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60

There was some amorphous basic paste remnants in the canals, but Hertwig's

sheath and dentin resorption were not present.

Only one of the four basic-treated teeth remained in the six month

animals. Although this tooth was lost during histological preparation,

the tissue sections clearly showed the severe degenerative tissue changes

present in the tooth socket (Figure 34). No evidence of any connective

tissue attachment could be seen which indicated this tooth would have ex-

foliated soon. The socket was surrounded by a well differentiated stra-

tified squamous epithelium. A severe chronic inflammatory cellular in-

filtrate was seen in the subepithelial tissues and furcation and inter-

proximal alveolar bone were absent.

No histological evidence of apical closure or calcification was

seen at any time in the basic-treated teeth during this study.

SUHHARY OF pH RESULTS

Table VI lists the average periapical tissue pH values at various

intervals during the experiment. Initial normal periapical tissue pH

ranged from 7.09 to 7.13 with an average pH=7.11. Following one week of

infection with ~· faecalis, the periapical tissue pH dropped to a range

of 6.33 to 6.62 with an average pH=6.49. At the time of sacrifice, the

periapical tissue pH had increased to a range of 6.89 to 7.16 with an

average pH=7.03.

Degrees of Sums of Mean F Value Source Freedom Squares Squares

Variance in pH between dogs 5 0.02 0.004 0.03 P>.S

Variance in pH within dogs 12 1.49 0.124

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61

This analysis of variance table shows that there was no statisti-

cally significant variation in response between or within animals at a

specific time interval during the experiment (P>.5). That is, each

animal responded in the same manner during a specific operative ses-

sion in this study.

Degrees of Sums of He an F Value Source Freedom Squares Squares

Variance in pH bet\veen time intervals 2 1.40 0.7 95.9 P<.Ol Variance in pH within time intervals 15 0.11 0.007

This analysis of variance table shows that there was a statistically

significant difference in periapical tissue pH at the various operative

sessions during this study. Using the K distribution, these significant

differences were determined. The periapical tissue pH after one week of

infection is significantly lower than the initial normal periapical tissue

pH (P<.Ol). That is, the pH of acutely inflamed periapical tissue was

significantly lower than the pH of normal periapical tissue in dogs. Fur-

thermore, the periapical tissue pH at sacrifice was significantly higher

than the periapical tissue pH after one week of infection (P<.Ol). Hence,

the pH of chronically inflamed periapical tissue was significantly higher

than the pH of acutely inflamed periapical tissue in dogs. However, there

was not a statistically significant difference in tissue pH bet~veen

chronically inflamed and normal periapical tissue in dogs (P>.05).

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CHAPTER V

DISCUSSION

Root end induction procedures have become a valuable addition to

the modern endodontic practice. In the literature review, numerous

clinical and animal studies were cited that have attempted to clarify

our understanding of the apexification process and to increase the suc­

cess rate of this treatment regimen. Although calcium hydroxide pastes

have become the most widely used agents to induce apexification, the use

of a blood clot, polyantibiotic and iodoform pastes, resorbable trical­

cium phosphate ceramic, and collagen-calcium phosphate gel have yielded

similarly successful results.

In order to further clarify the underlying reparative mechanism of

apexification, this study was undertaken in an attempt to delineate the

effects of the pH of the intracanal paste on the hard tissue repair which

occurs at the apices of pulpless immature teeth with periapical involve­

ment. The results, at first glance, were very discouraging since hard

tissue repair did not occur in any of the experimental teeth, most probably

as a result of overwhelming infection and tissue damage. Houever, one must

reflect upon Spallanzani's dictum as cited by Naidorf (149):

"If I set out to prove something, I am no real scientist.

I have to learn to follow where the facts lead me; I have

to learn to whip my prejudices."

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The following analysis of the experimental design 'vill delineate the sig­

nificant findings of this study as well as to suggest improvements for

future investigations.

SUMMARY OF THE OVERALL CLINICAL AND HISTOLOGICAL RESULTS

The results of this study indicated that the presence or absence of

a treatment paste did not induce root end closure. However, no conclu­

sions could be drawn concerning the effects of the pH of the intracanal

treatment paste on the apexification process due to the overwhelming

infection and tissue damage seen in the experimental teeth.

Tables IV and V summarize the clinical findings at various inter­

vals during this experiment. There were approximately equal numbers of

exfoliated teeth, draining sinus tracts, and mobile teeth in each of the

acidic, basic, and infected groups throughout this study. Hence, the

presence or absence of a paste in the root canal did not in itself affect

the number of exfoliated teeth, draining sinus tracts, or the mobility of

the experimental teeth in this study. However, the number of exfoliated

teeth and severity of tooth mobility did increase as the postoperative

interval increased.

Tables I and VII summarize the radiographic findings at various in­

tervals during this experiment. There was no radiographic evidence of

apical closure in any of the experimental teeth in this study. Periapical

and bifurcation radiolucent lesions were seen in all experimental teeth

and the size of these lesions increased as the postoperative sacrifice

interval increased, regardless of the type of paste used in the canal.

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Hence, the presence or absence of a paste neither induced apical closure

nor affected the growth of periapical or bifurcation radiolucent lesions

in this study.

Clinical results revealed that all experimental teeth suffered

64

severe degenerative changes regardless of the presence or absence of a

treatment paste in the root canal. The one week animal had lost consider­

able periodontal ligament support for these teeth and an epithelial sling

was beginning to form around the roots. Although no definitive conclu­

sions could be made, the origin of this epithelium was from cellular pro­

liferation of either the epithelial attachment at the gingival opening of

the sinus tract or the epithelial rests of }1alassez in the periodontal

ligament. After the loss of the periodontal ligament attachment to the

root surface, the epithelium grew into this area as a protective mechanism

to prevent further injury to the underlying periodontal tissues. Neither

vital nor necrotic tissue was seen in the root canals and neither Hertwig's

sheath nor evidence of root resorption was evident at the root apex.

An acute inflammatory cellular infiltrate of polymorphonuclear leukocytes

was present in the subepithelial tissues and severe loss of furcation bone

was seen.

As the postoperative interval increased, the degenerative changes

became more severe with increasing loss of the periodontal attachment ap­

paratus. The epithelial sling surrounding the root surfaces became more

organized and displayed rete pegs, basal and prickle cell layers, and a

surface of parakeratin. The subepithelial cellular inflammatory

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infiltrate became chronic in nature and consisted of lymphocytes, plasma

cells, and macrophages scattered among the dense fibrous connective tis­

sue of the developing lamina propria.

65

One could dedu'ce from these results that as the postoperative in­

terval increased, all experimental teeth would eventually be exfoliated

due to the infection and tissue damage. The observed degenerative changes

were similar in all experimental teeth and hence did not depend on the

presence or absence of a treatment paste in the root canal.

INTRACANAL pH CONCEPT

Table VI discloses the average periapical tissue pH at various in­

tervals in the experiment. Initial normal periapical tissue pH ranged

from 7.09 to 7.13 in the individual animals with an overall average of

7.11. Following one week of infection with 2· faecalis, the periapical

tissue pH dropped to a range of 6.33 to 6.62 with an overall average of

6.49. This result verifies lfenkin's (104) hypothesis that the normal

tissue pH will become acidic during the acute inflammatory process. At

the time of sacrifice, the periapical tissue pH had risen to a range of

6.89 to 7.16 with an average of 7.03. This result verifies Henkin's (104)

hypothesis that the pH of chronic inflammation will rise and may become

slightly alkaline. The pH of periapical tissues at the time of sacrifice

was independent of the presence of a paste in this study since the overall

average pH was 7.03 while the average pH of the infected-only teeth was

7.04, the acidic-treated teeth was 7.01 and the basic-treated teeth was

7.02. Hence the insertion of an acidic or basic paste had no effect on

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the periapical tissue pH at sacrifice.

This study did show that healthy periapical tissue pH in dogs aver­

aged 7.1 which is in agreement with the results of Wolpert,~ al., (141),

on mongrel dogs. Following one week of pulpal infection with S. faecalis

(human origin), the average periapical tissue pH dropped to 6.5. An

analysis of variance of the experimental results showed that each animal

responded in the same manner and that this decrease in periapical tissue

66

pH was statistically significant at the one per cent level of probability.

From one week to six months later, the average periapical tissue pH

increased to 7.03. An analysis of variance of the experimental results

showed that each animal responded in the same manner and that this increase

in periapical tissue pH was statistically significant at the one percent

level of probablility.

Menkin (140) created a severe inflammatory response in the pleural

cavity of dogs by injecting irritants. He reported that the exudate became

more acidic as inflammation progressed. However, when the pH increased,

the animal tended to improve and the outlook was more favorable.

It is not clear which part of the calcium hydroxide molecule exerts

the active effect on pulp, dentin, and periapical tissues. Sciaky and

Pisanti (92) and Pisanti and Sciaky (93) have shown, using labelled cal­

cium ions, that the calcium used in the formation of the dentin bridge

over a healing pulp capping is not contributed by the calcium hydroxide

medicament placed over the pulp, but rather comes from the circulating

serum calcium. Laws (150) found that the pH of calcium hydroxide from a

treated pulpotomy was 7.4 and he attributed this decrease in the normal

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pH of 12.5 of the calcium hydroxide material to be due to dilution by the

surrounding tissue fluids. However, Tronstad, ~ al., (148), found that

the pH of calcium hydroxide in the root canals of immature monkey's teeth

maintained a high pH which was greater than 12.2 during observation

periods up to thirteen months. Their results on the pH changes in imma­

ture teeth are shown in diagramatic form on page 68.

It is conceivable that the mode of action of calcium hydroxide may

be related to the alkaline pH of the treatment paste. It is possible

67

that calcium hydroxide may change the environment of the periapical tis­

sues to a more alkaline pH which is more conductive to healing. This

increase in pH by the hydroxide ions could inhibit the action of acid

hydrolases released by polymorphonuclear leukocytes and osteoclasts which

function best in a slightly acidic pH. Raisz (151), studying fetal rat

bone resorption stimulated by parathyroid hormone in tissue culture, found

that increasing the pH to 7.6 inhibited osteoclastic bone resorption sig­

nificantly. In an acidic pH, acid hydrolases cause a demineralization of

the mineral components of tissues. However, a rise in tissue pH would

be unfavorable for osteoclastic acid hydrolase activity. Furthermore, an

alkaline pH and the presence of calcium ions may activate alkaline phos­

phatase which has been proposed to play an important role in hard tissue

formation as stated by Tronstad, et al., (148).

Binnie and Rowe (134) found that calcium hydroxide, when used as a

root canal filling material, was particularly useful in an infected en­

vironment. Cvec (18), studying apexification of teeth \vith periapical

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pH CHANGES IN DENTAL TISSUES*

pH 8.0-10.0

pH 8.0-10.0

pH 8.0-10.0

pH 11.1-12-2

pH > 12.2

CROSS SECTION LONGITUDINAL SECTION

*from Tronstad, ~ al.,: pH changes in dental tissues following root canal filling with calcium hydroxide after induced pulp necrosis in replanted and non-replanted teeth. An experimental study in monkeys. In publication.

68

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r pathosis, presumed that calcium hydroxide per~ was acting as a long­

lasting antimicrobial agent. Matsumiya and Kitamura (94) filled ex­

perimentally infected root canals in dogs with a calcium hydroxide paste

and found that bacteria living in the periapical tissues disappeared as

healing progressed. They concluded that calcium hydroxide has anti­

bacterial action in dental tissues. The result is not surprising since

most microorganisms will not survive in a highly alkaline environment.

Calcium hydroxide has been shown to induce ectopic calcification in

rat connective tissue in studies by Mitchell and Shankwalker (90), Yo­

shiki and Mori (145), and Binnie and Mitchell (152). Yoshiki and Mori

(145) carried out a histochemical survey of enzymes present in the tissues

surrounding the implant of calcium hydroxide and found they were similar

to enzymes associated with normal calcification. They suggested the high

hydroxide ion concentration may be the factor that induces calcification.

When one considers that all pastes used in successful apexification

procedures have an alkaline pH, one may conclude that the pH of the in­

tracanal treatment paste may conceivably play a role in the apexifica­

tion process and will warrant further investigation in future studies.

THE DOG AS AN EXPERIMENTAL ANIMAL

The choice of an animal model for apexification research has been

a subject of controversy. It is neither possible to histologically ex­

amine the response of human tissue beyond the apex of treated teeth nor

feasible to obtain adequate pre- and postoperative experimental controls.

These difficulties preclude the use of humans for basic research.

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70

The monkey has been chosen as the experimental animal in a number

of studies because of its evolutionary and anatomical resemblance to man.

The use of an animal species closely related to man would permit a more

convincing extrapolation of the experimental results to actual clinical

practice as stated by Steiner and Van Hassel (120). However, the recu-

perative power of the monkey is greater than man. Citrome (116) pointed

out that primate pulpal tissue is very resistant to the damaging effects

of oral contamination and that despite the existence of severe inflam-

matory disease, the periapical tissues of the monkey still permit hard

tissue repair in the form of dentin, cementum, and bone. He stated that

all materials tested in the monkey have been successful, but not so in

the dog. The high cost of obtaining and boarding monkeys may be a further

deterrent to their use as an animal model (153).

On the other hand, the canine species has been found to bear a

closer similarity in healing processes when compared to man. In 1932 Orban

(154) stated that canine dental tissues are more sensitive to any kind of

injury than human teeth due to the greater permeability of dentin and ce-

mentum. He concluded that if treatment was successful in the far more

sensitive dog, it could be expected to be satisfactory in humans.

Hill (155) in 1932 reported that dental granulomas could be pro-

duced more quickly and easily in dogs than humans. He felt this was due

to the difficulty in removing all the organic debris in the apical arbor-

ization of canals and large multiple apical foramina. He noted that den-

tal granulomas produced in dogs were histologically similar to those

found in humans.

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r 71

Ostby (64), Vojinovic (82), Hatsumiya and Kitamura (94), and Gott-

lieb, et al., (156) found close similarities in healing processes between -- . dogs and humans. Torneck and Tulananda (132) in 1969 stated that al-

though the basic periapical tissue response to injury was similar in dogs

and human beings, the greater degree of hard tissue resorption seen in

dogs could be due to accumulation of pus and inflammatory exudate which

occurred about the orifices of the numerous apical accessory canals.

They reported that no evidence of repair was seen '"here pus accumulated

or the inflammatory exudate was intense.

In 1971 Barker and Lockett (157), evaluating the mandibular pre-

molars of dogs for endodontic experimentation, concluded that canine tis-

sue is more sensitive to injury and experiences greater difficulty in

healing than humans due to the protected sites for microorganisms in the

apical canal arborizations. They stated that dogs' premolar teeth are an

ideal model for endodontic research.

In 1975 Mazukelli (158) commented that the periapical tissue re-

sponse after endodontic treatment of dogs' teeth would be similar to that

\vhich would occur in humans after similar therapy.

In 1977 England and Best (71) reported that dogs appear to be much

more resistant to injury than humans since apical closure was seen in

teeth whose pulpal tissue was exposed to saliva. Hmv-ever, examination of

the published photomicrographs revealed that the pulpal tissue in the

root canals appeared normal which may indicate that pulpal trauma and in-

fection was not very severe. In light of the unusual results of this

study, another study of similar design would lend credence to their

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r '

72

conclusions.

In 1977 Citrome (116) concluded that the dog is a more sensitive

animal than the monkey for apexification studies and hence the appro-

priate animal model for such experiments.

Based on the conclusions of these investigators, the beagle dog

was selected as the experimental animal for this study. As a result of

the overwhelming tissue damage seen in the experimental teeth, one must

agree that indeed the dog is very sensitive to tissue injury and infec-

tion as reported by most investigators.

The age of the animal and the degree of apical closure of the ex-

perimental teeth when the project begins must be carefully considered in

future studies. The eruption of the experimental teeth was closely ob-

served and the operative procedures began three weeks after eruption.

Experimental hindsight revealed that there was still a substantial number

of control teeth with widely divergent apices five weeks later as seen in

the animals sacrificed one month after operative procedures were completed.

If this study had been started at this later stage of tooth development,

the more fully developed teeth and further maturity of the animals may

have sho~vn more resistance to the devastating tissue injury which occurred

in this experiment. Perhaps the immaturity and underdevelopment of these

dogs may have been a major reason for the failure of any hard tissue de-

position to occur at the apices of the experimental teeth.

THE USE OF STREPTOCOCCUS FAECALIS

In 1943 Hayes (159) cultured the root canals of 340 teeth and

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r microscopically studied the bacteria. Of the 211 teeth which exhibited

positive cultures, ninety-five contained a pure culture of some species

of streptococcus.

Teeth 1;.1ith root canals that were unexposed to the oral environment

were studied for the presence of bacteria by Bro\vn and Rudolph (160) in

1957. They found that streptococci, diptheroids and micrococci were the

most frequently isolated organisms, and that mixed infections were preva­

lent. They discovered that the bacterial flora of unexposed canals var­

ied from that of exposed canals.

Blechman (161) in 1957 reported that alpha and gamma hemolytic

streptococci and Staphylococcus albus were the organisms most frequently

isolated from root canals. Approximately eighty per cent of isolated

cultures contained streptococci while forty-eight per cent of these were

pure cultures.

In 1958 Leavitt, Naidorf and Shugaevsky (162), using Trypticase Soy

broth and agar, studied the bacterial flora of root canals. They indica­

ted that streptococci were the largest single group of organisms present.

In 1960 Shovelton and Sidaway (163) cultured and subcultured the

root canals of 147 teeth and reported that alpha hemolytic streptococci

were the most prevalent microorganisms. Engstrom and Frostell (164)

noted that streptococci were present in the majority of teeth with posi­

tive cultures that had non-vital pulps and intact pulp cavities.

The Streptococcus faecalis organism, which is not an overt pathogen

and is generally considered to be an opportunistic organism, has been

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implicated as a significant pulpal pathogen. In 1959 Gran (165) studied

the microflora of root canals and stated that the streptococci were the

most difficult bacteria to eradicate. He reported that the enterococci

organisms, for example~· faecalis, Here very insensitive organisms and

were resistant to many antibiotics.

In 1959 Winkler and van Amerongen (166) commented on the bacterio­

logic results from 4,000 root canal cultures taken prior to and after

endodontic treatment. From the 1,141 positive cultures, fifty-one per

cent were streptococci in pure culture and alpha hemolytic ~· faecalis

74

was the most common isolate. This organism, which was isolated more fre­

quently in subsequent than initial cultures from teeth with necrotic pulps,

tended to persist in root canals once established. S. faecalis and its

variant ~· liquefaciens caused clinical infections which were very diffi­

cult to eliminate and hence they should be considered potentially patho­

genic for the dental pulp.

In 1961 Crawford and Shankle (167), comparing the bacterial flora

of root canals which were open to those closed to oral contamination, found

that non-beta hemolytic streptococci predominated in both environments.

They reported that enterobacteria were among the most common microorganisms

retrieved from the initial culture of a tooth left open to the oral en­

vironment.

In 1964 Engstrom (168) studied the significance of enterococci in

endodontic therapy. He found that the first antiseptic treatment failed

to eradicate the organisms from the root canal of sixty-five per cent of

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r the teeth infected with enterococci, ~· faecalis being the usual isolate.

This compared to the figure of 39.5 per cent for teeth infected 1vith

other varieties of microoreanisms. He concluded that pulpal infections

with enterococci were a treatment problem since the infections were

harder to eliminate and would require a longer treatment period.

In 1969 Torneck (169) isolated a high proportion of enterococci

and staphylococci from acutely infected dental pulps. He noted the pre­

sence of enterococci in cultures taken from the canals of teeth with a

history of previous endodontic therapy.

In 1971 Barker and Lockett (157) concluded that S. viridans was

an ideal microorganism for the infection of mandibular premolars in dog_s.

They reported that it will incite a chronic to subacute periapical re­

sponse without danger of acute exacerbation, while apical granulomas T~Jill

be visible radiographic.ally within two or three months. They stated that

a nutrient broth culture, Hhich had been incubated for tvJenty-four hours

following transfer of a standard innoculum from a stock ·culture, would

be suitable for animal experimentation.

Mazukelli (158), in dogs, and Felder (170), in monkeys, innocu­

lated dental pulps with pure cultures of ~· faecalis which induced radio­

graphically visible periapical pathosis within three to four months.

Based on these studies, ~· faecalis was chosen for infection of the

dogs' root canals in this study. This organism, having verified its

virulence as a significant pulpal pathogen in dogs by Mazukelli (158),

was obtained in pure culture from the Microbiology Department of Loyola

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University. Although the specific source of this organism could not be

determined, it was likely a hospital isolate of a non-oral human infec-

tion. The significance of this ill-suited choice will be discussed

after one considers that the periapical lesions of bacterial etiology are

the result of the number of invading organisms, the virulence of the

organism, and the intrinsic ability of the host to combat infection.

Zeldow and Ingle (171) stated that the relationship of this triad of

factors could be expressed by the equation:

Severity of the disease state Number x Virulence Host Resistance

Steiner and Van Hassel (120) explained that the experimental procedure

and animal model being examined should be tested under the most unfavor-

able situations likely to be encountered clinically. In this manner, the

validity of the effectiveness of a treatment regimen as determined in

an animal model would be reinforced for use in a human clinical situa-

tion. A major reason for the extreme tissue damage seen in this study

76

may have been related to the use of a human non-oral strain of S. faecalis.

The extensive destruction of periapical tissues seen in these animals

after one week of infection is rarely seen in clinical situations. As

this strain of bacteria was too virulent for the resistance of the dog to

overcome, future research projects should consider the use of oral strains

of S. faecalis. These organisms could be obtained from the root canals

of human teeth with positive cultures. However, one must consider that

human strains of this microorganism may be more virulent than the bac-

terial flora normally found in the canine species. Perhaps a more

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logical choice would be the isolation of an indiginous strain of S.

faecalis from the dog's saliva for use in future studies.

The use of a standard innoculum of microorganisms in this study

ensured that a constant number of organisms was introduced into each ex­

perimental tooth. However, no attempt was made to analyze the bacterio­

logic status of the root canals. Ham,~ al., (73), reported that when

complete pulpal necrosis and extensive periapical destruction were pre­

sent, the likelihood of successful apexification results were lessened

if a negative culture could not be obtained. Future experimentation

should delay insertion of the treatment pastes until a negative culture

has been obtained. The use of a parenteral antibiotic to reduce sys­

temic disturbances should also be considered. As discussed previously,

the host resistance of the experimental animals may have been increased

if the study had begun at a later date when the animals were more mature.

One should also consider using non-infected experimental teeth, in addi­

tion to infected experimental teeth, to evaluate the effectiveness of

the treatment pastes. This method would simulate the clinical situation

of apexification of non-infected pulpless immature teeth.

USE OF VITAL DYE ~~RKERS

Histological evidence of hard tissue deposition at the apex of a

root canal can be visualized in a hematoxylin and eosin stained tissue

section. Unfortunately, one cannot be sure whether this deposition

occurred before, during, or after experimental pro~edures. This reali­

zation necessitates the use of a biological marker to label the tissue

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so that one can determine the sequence of hard tissue deposition.

Tomich (172) in 1968 reported that Procion Brilliant Red H-8BS

was an effective in vivo hard tissue marking agent ''"hich Has used safely

at a dosage of 100 mg./kg. of body weight in rats. Goland, ~ al., (173,

174), noted that the reactive Procion dyes formed very stable covalent

bonds and crosslinkages under physiological conditions in rats. These

dyes were retained in incremental lines and zones of growth in teeth and

bones, and these dyes were preserved in decalcification and preparation

of tissue sections. Prescott,~ al., (175), in 1968 showed that a

single dose of Procion Brilliant Red H-8BS given intraperitoneally to a

dog ,.,ould selectively stain bone, dentin and cementum being formed at

the time of administration. Sherman (176) used this dye to observe de­

position of cementum and alveolar bone apposition following intentional

replantation of teeth in dogs and monkeys. Ham,~ al., (73), used a

single injection of this dye to observe hard tissue deposition in an

apexification study using monkeys while Citrome (116) used multiple in­

jections of this dye to monitor hard tissue repair in an apexification

study using dogs.

Due to the extensive tissue damage which occurred in this study,

the use of a vital dye did not aid in the evaluation of the histological

results. However, the use of a biological marker to monitor calcific

repair after experimental procedures should not be neglected in future

studies. In this manner, one can objectively state that the calcific re­

pair occurred after the treatment was performed.

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CHAPTER VI

SUMMARY AND CONCLUSIONS

In an effort to delineate the role of pH in healing of developing

periapical lesions in immature teeth of dogs, the pulps of twenty-four

premolar teeth were extirpated in six young purebred beagle littermates.

Then a standardized innoculum of a pure culture of ~· faecalis was placed

in the root canal and the access cavities were sealed. Untreated pre­

molar teeth adjacent to the operated teeth served as controls. One week

later, the root canals of two-thirds of the experimental teeth received

endodontic canal enlargement, were irrigated and dried before the inser­

tion of either an acidic paste (pH=3) or a basic paste (pH~ll). These

teeth served as the acidic-treated and basic-treated teeth while the re­

maining experimental teeth served as infected-only teeth. The periapical

tissue pH in the region of the root apex was measured at various inter­

vals during the experiment using pH microelectrodes. Regular radiographic

and clinical observations of the experimental and control teeth were con­

ducted throughout the entire experiment. The animals were sacrificed at

four different postoperative intervals: one dog at one week, two dogs at

one month, one dog at three months, and two dogs at six months. The jaws

were removed at necropsy and following fixation, decalcification and his­

tologic preparation, the teeth and surrounding structures were evaluated

microscopically.

Under the conditions of this experiment, the following conclusions

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could be drawn:

a) S. faecalis is capable of producing pathologic

periapical lesions in dogs.

b) Hertwig's epithelial root sheath is destroyed

following pulpal extirpation, infection and

severe periapical inflammation.

c) In the presence of severe periapical tissue

inflammation, further root development will not

occur in immature teeth of dogs in response to

change in pH of periapical tissue.

Under the conditions of this experiment, the following impressions

could be drawn:

a) Young beagle dogs appear to be sensitive to severe

periapical tissue injury and infection.

b) The normal periapical tissue pH in dogs is 7.1. In

the presence of acute inflammation, the periapical

tissue pH of the beagle dogs in this study dropped

to approximately 6.5. As the inflammation became

chronic, the periapical tissue pH rose to about pH=7.

c) The use of a human isolate of S. faecalis for peri­

apical infection of young dogs' teeth may be too

virulent to allow healing of the periapical tissues.

The use of a strain of S. faecalis indiginous to the

canine species may be preferable in future studies

of this nature.

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CHAPTER VII

REFERENCES

(1) Weine, F.S.: Endodontic Therapy, 2nd ed .. C.V. Mosby Co., St. Louis, 1976, pp. 206, 429.

(2) Schour, I., Massler, M. and Brescia, N.J.: Development and growth of teeth. In Orban's Oral Histology And Embryology, 6th ed. Sicher, H., editor. C.V. Mosby Co., St. Louis, 1966, p. 18.

(3) Skillen, W.G.: A report on the formation of dentin and cementum relative to the structure of the root end. J. Nat. Dent. Assoc., 8 (1): 3, 1921.

(4) Orban, B.J.: Growth and movement of tooth germs and teeth. J. Am. Dent. Assoc., 15:1024, 1928.

(5) Diab, M.A. and Stallard, R.E.: A study of the relationship between epithelial root sheath and root development. J. Amer. Soc. Periodont., 3(1):10, 1965.

(6) Kenney, E.B. and Ramfjord, S.P.: tion of teeth in rhesus monkeys.

Cellular dynamics in root forma­J. Dent. Res., 48:114, 1969.

(7) Gottlieb, B.: Biology of cementum. J. Periodont., 13:13, 1942.

(8) Owens, P.D.A.: A light microscopic study of the development of the roots of premolar teeth in dogs. Arch. Oral Biol., 19:525, 1974.

(9) Friend, L.A.: Root canal morphology in incisor teeth in the 6-15 year old child. J. Brit. Endodont. Soc., 3:35, 1969.

(10) Bernick, S., Rutherford, R.L. and Rabinowitch, B.Z.: Microscopic studies of the teeth of a 6-year-old-boy. Anat. Rec., 105(2):235, 1949.

(11) Zeldow, L.L.: Endodontic treatment of vital and non-vital immature teeth. N.Y. State Dent. J., 33:327, 1967.

(12) Hallett, G.E.M. and Porteous, J.R.: Fractured incisors treated by vital pulpotomy. A report on 100 consecutive cases. Br. Dent. J., 115(7):279, 1963.

81

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r '

(13) Luks, S.: Observed effects of traumatic injuries upon anterior teeth. N.Y. State Dent. J., 28:65, 1962.

(14) Hargreaves, J.A.: The traumatized tooth. In Biology Of The Human Dental Pulp, Siskin, H., editor. C.V. Hosby Co., St. Louis, 1973, p. 407.

(15) Tegart, R.L.: Pulpectomy in young permanent incisors. J. Can. Dent. Assoc., 25:622, 1959.

(16) Seltzer, S., and Bender, I.B.: The Dental Pulp. Biologic Considerations In Dental Procedures, 2nd ed .. J.B. Lippincott Co., Philadelphia, 1975, p. 252.

(17) Vanek, P .H.: S. and Burns, p. 375.

Traumatic injuries. In Pathwavs Of The Pulp, Cohen, R.C., editors. C.V. Mosby Co., St. Louis, 1976,

(18) Cvek, H.: Treatment of non-vital permanent incisors with calcium hydroxide. I. Follow-up of periapical repair and apical closure of iromature roots. Odont. Revy, 23:27, 1972.

(19) Andreasen, J.O.: Traumatic Injuries Of The Teeth. C.V. Hosby Co., St. Louis, 1972, p. 81.

(20) Corpron, R.E. and Dmvson, J.: Pulpal therapy for the traumatized immature permanent anterior tooth. J. Nich. Dent. Assoc., 52:224, 1970.

(21) Bodenham, R.G.: The prognosis for vital pulpotomy of traumatized permanent incisors. Dent. Practit., 17(9):327, 1967.

(22) Dow, P.R. and Le\vis, T.H.: Pulp management for the immature frac­tured anterior tooth. J. Can. Dent. Assoc., 26:5, 1960.

(23) Krakow, A.A., Berk, H. and Gron, P.: Therapeutic induction of root formation in the exposed incompletely formed tooth \vith vital pulp. Oral Surg., 42(5):755, 1977.

(24) Laws, A.J.: Condensed calcium hydroxide root filling following partial pulpectomy. N.Z. Dent. J., 67:161, 1971.

(25) Bennett, D.T.: Traumatized anterior teeth. I. Assessing the injury and principles of treatment. Br. Dent. J., 115:309, 1963.

(26) Law, D.B.: Prevention and treatment of traumatized permanent anterior teeth. Dent. Clin. North Am., 9:615, 1961.

82

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(27) }fasterton, J.B.: Inherent healing potential of the dental pulp. Br. Dent. J., 120:430, 1966.

(28) Moodnick, R.M.: Clinical correlations of the development of the root apex and surrounding structures. Oral Surg., 16(5):600, 1963.

(29) Schroder, V. and Granath, L.E.: Early reaction of intact human teeth to calcium hydroxide following experimental pulpotomy and its significance to the development of hard tissue barrier. Odont. Revy, 22:379, 1971.

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Endodontic management of teeth with J. Hawaii Dent. Assoc., 7:13, 1974.

(31) Winter, G.B.: Endodontic therapy of traumatized teeth in children. Int. Dent. J., 27(3):252, 1977.

(32) Traintor, J.F.: Technic for root end closure: Apexification.

(33)

J. Nebr. Dent. Assoc., 53:8, 1977.

Feldman, G., Solomon, C., Notaro, P. and Hoskowitz, E.: treatment of vital and non-vital teeth with open apices. State Dent. J., 39:277, 1973.

Endodontic N.Y.

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(36) Vojinovic, 0.: Induction of apical formation in immature teeth by different endodontic methods of treatment. Experimental patho­histological study. J. Oral Rehabil., 1:85, 1974.

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(38) Langeland, K., Dowden, W.E., Tronstad, L. and Langeland, L.K.: Human pulp changes of iatrogenic or1g1n. In Biology Of The Human Dental Pulp, Siskin, H., editor. C.V. Mosby Co., St. Louis, 1973, p. 122.

(39) Fischer, C.H.: Hard tissue formation of the pulp in relation to treatment of traumatic injuries. Int. Dent. J., 24:387, 1974.

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83

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r (41) Duell, R.C.: Conservative endodontic treatment of the open apex in

three dimensions. Dent. Clin. North A~., 17:125, 1973.

(42) Friend, L.A.: The root treatment of teeth with open bpices. Proc. Roy. Soc. Med., 59:1035, 1966.

(43) Friend, L.A.: The treatment of immature teeth with non-vital pulps. J. Brit. Endodont. Soc., 1:28, 1967.

(44) Dimashkieh, M.R.: The problem of the open apex- A new approach. Oxidized regenerated cellulose technique. J. Brit. Endodont. Soc., 10(1):9, 1977.

(45) Dimashkieh, M.R.: A method of using silver amalgam in routine endodontics, and its use in open apices. Brit. Dent. J., 138:298, 1975.

(46) Koenigs, J.F. and Brilliant, J.D.: Open apices: creating apical stop with a zinc-acetate-Grossman's cement mixture on a gutta-percha cone. J. Acad. Gen. Dent., 22:32, 1974.

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84

(48) Heling, B., Azas, B. and Goldstein, A: Traumatized permanent incisors in children. J. Brit. Endodont. Soc., 10(2):65, 1977.

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(50) Ellis, R.G. and Davey, K.W.: The Classification And Treatment Of Injuries To The Teeth Of Children. Year Book Medical Publishers, Chicago, 1970, p. 120.

(51) Grossman, L.I.: Endodontic Practice, 8th ed .. Lea and Febiger, Philadelphia, 1974, p. 282.

(52) Sommer, R.F., Ostrander, F.D. and Crowley, M.C.: Clinical Endo­dontics, 2nd ed .. W.B. Saunders Co., Philadelphia, 1962, pp. 221, 507.

(53) Boyle, P.E.: Kronfeld's Histopathology Of The Teeth And Their Surrounding Structures, 4th ed .. Lea and Febiger, Philadelphia, 1955, p. 239.

(54) Ingle, J.I.: Endodontics. Lea and Febiger, Philadelphia, 1965, p. 60.

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(55) Haxmen, H.A.: The expanding scope of endodontics. J. Hich. Dent. Assoc., 41:25-40, 1959.

(56) Ingle, J.I.: Obliterating the flaring apical foramen. D. Digest, 62:410, 1956.

(57) Patterson, S.S.: The endodontic management of the young permanent tooth. J. Dent. Child., 25:215, 1958.

(58) Frank, A.L.: Therapy for the divergent pulpless tooth by continued apical formation. J.Am. Dent. Assoc., 72:87, 1966.

(59) Luebke, R.G., Glick, D.H. and Ingle, J.I.: Indications and con­traindications for endodontic surgery. Oral Surg., 18(1):97, 1964.

(60) Cooke, C. and Rowbotham, T.C.: Root canal therapy in non-vital teeth with open apices. Brit. Dent. J., 108:147, 1960.

(61) Frank, A.L.: Endodontic endosseous implants and treatment of the wide open apex. Dent. Clin. North Am., 11:675, 1967.

(62) Levin, H.D.: Endodontic therapy of non-vital teeth with open apices. J. D.C. Dent. Soc., p. 11, 1976.

(63) Van Hassel, H.J. and Natkin, E.: Induction of root end closure. A case report. J. Dent. Child., 37:57, 1970.

(64) Ostby, B.N.: The role of the blood clot in endodontic therapy. An experimental histologic study. Acta. Odontol. Scand., 19:323, 1961.

(65) Ball, J.S.: Apical root formation in a non-vital immature permanent incisor. Report of a case. Brit. Dent. J., 116:166, 1964.

(66) Heithersay, G.S.: Stimulation of root formation in incompletely developed pulpless teeth. Oral Surg., 29:620, 1970.

(67) Hichanowicz, J.P. and Hichanm..ricz, A.E.: A conservative approach and procedure to fill an incompletely formed root using calcium hydroxide as an adjunct. J. Dent. Child., 32:42, 1967.

(68) Rule, D.C. and Winter, G.B.: Root growth and apical repair subse­quent to pulpal necrosis in children. Brit. Dent. J., 120:586, 1966.

(69) Cvek, M.: Treatment of non-vital permanent incisors with calcium hydroxide. IV. Periodontal healing and closure of the root canal in the coronal segment of teeth with intra-alveolar fracture and vital apical fragment. A follow up. Odont. Revy, 25:239, 1974.

85

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(70) Dyle~;.;ski, J.J.: Apical closure of non-vital teeth. Oral Surg., 32:82, 1971.

(71) England, M.G. and Best, E.: Noninduced apical closure in immature roots of dog's teeth. J. Endod., 3(11):411, 1977.

(72) Ham, J.W.: A study of induced apical closure in pulpless teeth with open apices. Thesis, Indiana University School of Dentistry, Indianapolis, Ind., 1969.

(73) Ham, J.W., Patterson, S.S. and Mitchell, D.F.: closure of immature pulpless teeth in monkeys. 1972.

Induced apical Oral Surg., 33:438,

(74) Holland, R., Souza, V. de and Russo, M. de C.: Healing process after root canal therapy in immature human teeth. Rev. Fac. Odontol. Aracatuba, 2:269, 1973.

(75) Gibson, A.C.L.: Continued root development after traumatic avulsion of partly formed permanent incisor. Brit. Dent. J., 126:356, 1969.

(76) Klein, S.H. and Levy, B.A.: Histologic evaluation of induced apical closure of a human pulpless tooth. Report of a case. Oral Surg., 38(6):954, 1974.

(77) Narang, R. and Wells, H.: Experimental osteogenesis in periapical areas -.;.;ith decalcified allogeneic bone matrix. Oral Surg., 35(1): 136' 1973.

(78) Nevins, A.J., Finkelstein, F., Borden, E.G. and Moodnick, R.: Formation of mineralized scar tissue induced by implants containing collagen-calcium phosphate gel. J. Endod., 1(9):303, 1975.

(79) Piekoff, M.D. and Trott, J.R.: Apexification: report of case. J. Endod., 2(6):182, 1976.

(80) Torneck, C.D., Smith, J.S. and Grindall, P.: Effects of endodontic procedures on developing incisor teeth. II. Effect of pulp injury and oral contamination. Oral Surg., 35(3):378, 1973.

(81) Urist, }f.R., Silverman, B.F., Buring, K., Dubuc, E.L. and Rosenberg, J.}f.: The bone induction principle. Clin. Orthoped., 53:243, 1973.

(82) Vojinovic, 0.: Influence of various endodontic methods of treatment upon the process of apical closure of immature pulpless human teeth and the structure of the newly formed calcified tissue in apical opening. J. Oral Rehabil., 4:335, 1977.

86

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(83) Applebaum, E.: Tissue changes at the apex following death of the pulp. Dent. Cosmos, 71:1106, 1929.

(84) Easlick, K.A.: Management of pulp exposure in the mixed dentition. J. Am. Dent. Assoc., 30:179, 1943.

(85) Johnson, M.: Experimental development of bone through apical fora­men. J. Am. Dent. Assoc., 32:443, 1945.

(86) Herbert, W.E.: Three cases of disturbance of calcification of a tooth and infection of the dental pulp following trauma. Dent. Practit., 9(7):176, 1959.

(87) Kaiser, H.J.: Apical closure of non-vital teeth with open apices using calcium hydroxide. Presented before the Am. Assoc. Endod., Washington, D.C. April, 1964.

(88) Crabb, H.S.M.: The basis of root canal therapy. Dent. Practit., 15(11):397, 1965.

(89) Bouchon, F.: Apex formation following treatment of necrotized immature permanent incisor. J. Dent. Child., 33:370, 1966.

(90) Mitchell, D.F. and Shankwalker, G.B.: Osteogenic potential of calcium hydroxide and other materials in soft tissue and bone wounds. J. Dent. Res., 37(6):1157, 1958.

(91) Mitchell, D.F. and Amos, E.R.: Reaction of connective tissue of rats to implanted dental materials. I.A.D.R., 35th General Meeting, Atlantic City, March, 1957, Preprinted abstracts, p. 59.

(92) Sciaky, I. and Pisanti, S.: Localization of calcium placed over amputated pulps in dog's teeth. J. Dent. Res., 39:1128, 1960.

(93) Pisanti, S. and Sciaky, I.: Origin of calcium in the repair wall after pulp exposure in the dog. J. Dent. Res., 43:641, 1964.

(94) ~Iatsumiya, S. and Kitamura, M.: Histo-pathological and histo­bacteriological studies of the relation between the condition of sterilization of the interior of the root canal and the healing process of periapical tissues in experimentally infected root canal treatment. Bull. Tokyo Dent. Coll., 1(1):1, 1960.

(95) Frank, A.L. and Weine, F.S.: Nonsurgical therapy for the perfora­tive defect of internal resorption. J. Am. Dent. Assoc., 87:863, 1973.

(96) Day, R.M: Calcium hydroxide in root canal therapy. A case report. Dent. Practit., 17(11):384, 1967.

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(97) Heithersay, G.S.: Calcium hydroxide in the treatment of pulpless teeth with associated pathology. J. Brit. Endodont. Soc., 8(2):74, 1975.

(98) Martin, D.M. and Crabb, H.S.M.: Calcium hydroxide in root canal therapy. A review. Brit. Dent. J., 142(9):277, 1977.

(99) Braham, R.L., Roberts, N.H. and Morris, H. E.: Hanagement of dental trauma in children and adolescents. J. Trauma, 17(11):857, 1977.

(100) Natkin, E.: Diagnosis and treatment of traumatic injuries and their sequellae. In Ingle's Endodontics. Lea and Febiger, Phila­delphia, 1965, p. 570.

(101) Steiner, J.C., Dow, P.R. and Cathey, G.M.: Inducing root end closure of non-vital permanent teeth. J. Dent. Child., 35:47, 1968.

(102) Van Hassel, H.F. and Natkin, E.: Induction of foraminal closure. J. Can. Dent. Assoc., 35:606, 1969.

(103) Heithersay, G.S.: Periapical repair following conservative endo­dontic therapy. Aust. Dent. J., 15:511, 1970.

(104) Simpson, S. T. : through trauma.

Treatment of the open apex - pulp involvement Case reports. Aust. Dent. J., 15:392, 1970.

(105) Bimstein, E. and Fuks, A.B.: Biological closure of open apices of non-vital teeth following calcium hydroxide root filling. Israel J. Dent. Med., 25(3):3, 1976.

(106) Kennedy, G.D.C., HcLundie, A.C. and Day, R.M.: its role in a simplified endodontic technique. 1967.

Calcium hydroxide -Dent. Mag., 84:51,

(107) ~valkoff-Hess: Lehrbuch der konservierenden zhanheilkunde, Leipzig: Barth., 1954, p. 266. Cited in Day, R.M.: Calcium hydroxide in root canal therapy. A case report. Dent. Practit., 17(11):384, 1967.

(108) Wechsler, S.M., Fishelberg, G., Opderbeck, W.R., LoMonaco, C.J., Skribner, J.E. and Shovlin, F.E.: Apexification: a valuable and effective clinical procedure. J. Acad. Gen. Dent., 26(5):40, 1978.

(109) Cvec, H., Hollender, L. and Nord, C.E.: Treatment of non-vital permanent incisors with calcium hydroxide. Odontol. Revy, 27(2):93 1976.

(110) Herforth, V.A. and Strasburg, M.: (Therapy of chronic apical perio­dontitis in traumatically injured front teeth \vith ongoing root growth). Dtsch. Zahnarztl. Z., 32:453, 1977.

88

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(111) Kreter, V.F. and Emmer, H.: (Apical filling with hard tissues in teeth of young persons after loss of vitality of the pulp). Dtsch. Zahnarztl. Z., 29:902, 1974.

(112) Roberts, S.C. and Brilliant, J.D.: Tricalcium phosphate as an adjunct to apical closure in pulpless permanent teeth. J. Endod., 1(8):263, 1975.

(113) Nevins, A., Wrobel, W., Valachovic, R. and Finkelstein, F.: Hard tissue induction into pulpless open-apex teeth using collagen-calcium phosphate gel. J. Endod., 3(11):431, 1977.

(114) Barker, B.W.C. and Mayne, J.R.: Some unusual cases of apexifica­tion subsequent to trauma. Oral Surg., 39(1):144, 1975.

89

(115) Shusterman, S., Meller, S.M. and Kane, J.: Reimplantation of trau­matically avulsed immature incisor: report of case. J. Dent. Child., 43:49, 1976.

(116) Citrome, G.P.: A comparative study of tooth apexification in the dog. Thesis, North~vestern University, Chicago, Il., 1977.

(117) Cvec, M. and Sundstrom, B.: Treatment of non-vital permanent in­cisors with calcium hydroxide. V. Histologic appearance of ro­entgenographically demonstrable apical closure of immature roots. Odont. Revy, 25:379, 1974.

(118) Holland, R., Mello, W.de and Nery, M.J.: Reaction of human peri­apical tissue to pulp extirpation and immediate root canal filling with calcium hydroxide. J. Endod., 3(2):63, 1977.

(119) Weinstein, R. and Goldman, M.: adult teeth of monkeys with use 43 (4): 627' 1977.

Apical hard-tissue deposition in of calcium hydroxide. Oral Surg.,

(120) Steiner, J.C. and Van Hassel, H.J.: Experimental root apexifica­tion in primates. Oral Surg., 31:409, 1971.

(121) Spedding, R.H., Mitchell, D.F. and HcDonald, R.E.: Formocresol and calcium hydroxide therapy. J. Dent. Res., 44(5):1023, 1965.

(122) Torneck, C.D., Smith, J.S. and Grindall, R.: Biologic effects of endodontic procedures on developing incisor teeth. III. Effect of debridement and disinfection procedures in the treatment of experi­mentally induced pulp and periapical disease. Oral Surg., 35(4):532, 1973.

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(123) Torneck, C.D., Smith, J.S. and Grindall, R.: Effect of endodontic procedures on developing incisor teeth. IV. Effect of debridement procedures and calcium hydroxide-camphorated parachlorophenol paste in the treatment of experimentally induced pulp and periapical dis­ease. Oral Surg., 35(4):541, 1973.

(124) ~1yers, W.C. and Fountain, S.B.: Dental pulp regeneration aided by blood and blood substitutes after experimentally induced periapical infection. Oral Surg., 37(3):441, 1974.

(125) Koenigs, J.F., Heller, A.L., Brilliant, J.D., Melfi, R.C. and Driskell, T.D.: Induced apical closure of permanent teeth in adult primates using a resorbable form of tricalcium phosphate ceramic. J.Endod., 1(3):102, 1975.

(126) Driskell, D., Hassler, C.R., Tennery, V.J., McCoy, L.R. and Clarke, W.J.: Calcium phosphate resorbable ceramics: a potential alterna­tive to bone grafting. J. Dent. Res., 52:123, 1973.

(127) Nevins, A.J., Finkelstein, F., Borden, B.G. and Laporta, R.: Re­vitalization of pulpless open apex teeth in rhesus monkeys using collagen-calcium phosphate gel. J. Ended., 2(6):159, 1976.

(128) Donlon, W.: Immune neutrality of calf-skin collagen gel used to stimulate revitalization in pulpless open-apex teeth of rhesus monkeys. J. Dent. Res., 56(6):670, 1977.

(129) Nevins, A.J., Finkelstein, F., Laporta, R. and Borden, B.G.: In­duction of hard tissue into pulpless open-apex teeth using collagen­calcium phosphate gel. J. Ended., 4(3):76, 1978.

(130) Heide, S. and Kerekes, K.: (Endodontic treatment of immature perm­anent incisors. A histological study of apical hard tissue formation following root filling with calcium hydroxide). Nor Tannlaegeforen Tid, 87(9):426, 1977.

(131) Camp, J.H.: Continued apical development of pulpless permanent teeth following endodontic therapy. Thesis, Indiana University School of Dentistry, Indianapolis, Ind., 1968.

(132) Torneck, C.D. and Tulananda, N.: cementum to experimental abscess 28(3):404, 1969.

Reaction of alveolar bone and formation in the dog. Oral Surg.,

(133) Holland, R., DeSouza, V., Tagliavini, R.L. and Milanezi, L.A.: Healing process of teeth with open apices: histological study. Bull. Tokyo Dent. Call., 12:333, 1971.

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(134) Binnie, W.H. and Rowe, A.H.R.: A histological study of the peri­apical tissues of incompletely formed pulpless teeth filled with calcium hydroxide. J. Dent. Res., 52(5):1110, 1973.

(135) Binnie, W.H. and Rowe, A.H.R.: The incidence of epithelial rests, proliferations and apical periodontal cysts following root canal treatment in young dogs. Brit. Dent. J., 137:56, 1974.

(136) Hager, T.F.: The effects of beta phase tricalcium phosphate on the pulp and periapical supporting apparatus in dogs. Thesis, Northwestern University, Chicago, Il., 1975.

(137) Vojinovic, 0. and Srnie, E.: Induction of apical formation by the use of calcium hydroxide and iodoform-Chlumsky paste in the endo­dontic treatment of immature teeth. J. Brit. Endodont. Soc., 8(1):16, 1975.

(138) White, A., Handler, P. and Smith, E.L.: Principles Of Biochemistry, 5th ed .. McGraw Hill Book Co., New York, 1973, p. 98.

(139) Gardiner, H.S. and Flemister, S.C.: The Principles of General Biology, 2nd ed .. The Macmillan Co., New York, 1967, p. 27.

(140) Henkin, V.: Biochemical Mechanisms In Inflammation, 2nd ed .. Chas. A. Thomas, Springfield, Il., 1956, p. 66.

91

(141) Wolpert, P.W., Noller, K., Shaughnessy, D., Houchin, D.N., Baccari, M.E. and Miller, F.A.: Tissue pH: a new clinical tool. Arch. Surg., 101:309, 1970.

(142) Glinz, W. and Clodius, 1.: Measurement of tissue pH for predicting viability in pedicle flaps: experimental studies in pigs. Brit. J. Plast. Surg., 25:111, 1972.

(143) Goldstein, J.: Antibiotics as related to endodontic therapy. J. Endod., 4(5):135, 1978.

(144) Bellanti, J.A.: Immunology II. W.B. Saunders Co., Philadelphia, 1978, p. 29.

(145) Yoshiki, S. and Mori, N.: Enzyme histochemistry on the tissue reaction to calcium hydroxide. Bull. Tokyo Dent. Coll., 2(1):32, 1961.

(146) Frankl, S.N.: Pulp therapy in endodontics. In Biology Of The Human Dental Pulp, Siskin, M., editor. C.V. Mosby Co., St. Louis, 1973, p. 355.

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(147) Tronstad, L.: The use of calcium hydroxide in endodontic therapy. J. Endod., 2(11):356, Abstr., 1976.

(148) Tronstad, L., Andreasen, J.O., Hasselgren, G., Kristersson, L. and Riis, I.: pH changes in dental tissues following root canal filling with calcium hydroxide after induced pulp necrosis in replanted and non-replanted teeth. An experimental study in monkeys. In publi­cation.

(149) Naidorf, I.J.: Inflammation and infection of pulp and periapical tissues. In Biology Of The Human Dental Pulp, Siskin, M., editor. C.V. ~osby Co., St. Louis, 1973, p. 391.

(150) Laws, A.J.: Calcium hydroxide as a possible root filling material. N.Z. Dent. J., 58:274, 1962.

(151) Raisz, L.: Bone resorption in tissue culture: factors influencing the response to parathyroid hormone. J. Clin. Invest., 44(1):103, 1965.

(152) Binnie, W.H. and Mitchell, D.F.: Induced calcification in the sub­dermal tissues of the rat. J. Dent. Res., 52:1087, 1973.

(153) Torabinejad, M. and Bakland, L.K.: An animal model for the study of immunopathogenesis of periapical lesions. J. Endod., 4(9):273, 1978.

(154) Orban, B.: The problem of root canal treatment. J. Am. Dent. Assoc., 19:1384, 1932.

(155) Hill, T.J.: Experimental dental granulomas in dogs. J. Am. Dent. Assoc., 19:1389, 1932.

(156) Gottlieb, B., Baron, S.L. and Cook, J.H.: Endodontia. Henry Kimpton, London, 1950.

(157) Barker, B.C.W. and Lockett, B.C.: Utilization of the mandibular premolars of the dog for endodontic research. Aust. Dent. J., 16:280, 1971.

(158) Mazukelli, R.J.: A study of host resistance of the periapical tis­sues of dogs when exposed to Streptococcus faecalis. Thesis, Loyola University, Maywood, Il., 1975.

(159) Hayes, R.L.: Clinical and bacteriologic study of 340 pulp involved cases. J. Dent. Res., 22:301, 1943.

(160) Brown, L.R. and Rudolph, C.B: Isolation and identification of micro­organisms from unexposed canals of pulp involved teeth. Oral Surg., 10:1094, 1957.

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(161) Blechman, H.: Bacteriology in endodontic treatment. North Am., 5:845, 1957.

Dent. Clin.

(162) Leavitt, J.M., Naidorf, I.J. and Shugaevsky, P.: The bacterial flora of root canals as disclosed by a culture medium for endodontics. Oral Surg., 11:302, 1958.

(163) Shovelton, D.S. and Sidaway, D.A.: Infection in root canals. Brit. Dent. J., 108:115, 1960.

(164) Engstrom, B. and Frostell, G.: Bacteriologic studies of the non­vital pulp in cases with intact pulp cavities. Acta. Odont. Scand., 19:23, 1961.

(165) Gran, J.A.: The bacteriology and pathology of the pulpless tooth. Aust. Dent. J., 4:241, 1959.

(166) Winkler, K.C. and Van Amerongen, J.: Bacteriologic results from 4,000 root canal cultures. Oral Surg., 12:857, 1959.

93

(167) Crawford, J.J. and Shankle, R.J.: Application of neT.ver methods to study the importance of root canal and oral microbiota in endodontics. Oral Surg., 14:1109, 1961.

(168) Engstrom, B.: The significance of enterococci in root canal treat­ment. Odont. Revy, 15:87, 1964.

(169) Torneck, C.D.: The role of microorganisms in endodontic disease. Alpha Omegan, p. 180, 1969.

(170) Felder, B.K.: The effect of decalcified allogeneic bone matrix on the healing of periapical lesions in the rhesus monkey. Thesis, Loyola University, Maywood, Il., 1978.

(171) Zeldow, B.J. and Ingle, J.I.: Correlation of the positive culture to the prognosis of endodontically treated teeth: a clinical study. J. Am. Dent. Assoc., 66:9, 1963.

(172) Tomich, C.E.: An evaluation of procion brilliant red H-8BS as an

(173)

in vivo hard tissue marking agent. Thesis, Indiana University School of Dentistry, Indianapolis, Ind., 1968.

Goland, P.O., Wolnak, B. and Williamson, R.: tooth and bone by the in vivo use of reactive dyes. I.A.D.R. Abstr-.-#134, p. 70, 1965.

Permanent stainings of procion and remazol

(174) Goland, P.P. and Grand, N.G.: Chloro-s-triazine as markers and fix­atives for the study of growth in teeth and bones. Am. J. Phys. Anthrop., 29:201, 1968.

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(175) Prescott, G.H., Mitchell, D.F. and Fahmy, H.: Procion dyes as matrix markers in growing bone and teeth. Am. J. Phys. Anthrop., 29:219, 1968.

(176) Sherman, P.: Intentional replantation of teeth in dogs and monkeys. J. Dent. Res., 47(6):1066, 1968.

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C!Lt\PTER VIII

TABLES AND FIGURES

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1 week I. animal A.S.

1 month I. animal A.S.

1 month I. animal A.S.

3 month I. animal A.S.

6 month I. animal A.S.

6 month I. animal A.S.

TABLE I

COMPARISON OF RADIOGRAPHIC FINDINGS AFTER ONE WEEK OF INFECTION AND AT SACRIFICE

CONTROL TEETH

Apical Closure Apical Closure N.E. Partial Complete N.E. E.

4 12 4 12

4 12 2 2 12

4 12 1 2 1 12

4 12 4 12

4 12 4 12

4 12 4 12

EXPERIHENTAL TEETH

Periapical Radiolucency Bifurcation Radiolucency N .E. <3mm. >3mm. N.E. <3mm. >3mm.

10 2 1 5 10 2 6

5 7 1 5 3 9:>'~ 6:>'~

3 9 2 4 1 11 6

6 6 4 2 12 2 4

4 8 5 1 12~~ 6:>'~

5 7 2 4 12* 6~~

LEGEND

I. - After one week infection with S. faecalis A.S. - At sacrifice N.E. - Not evident on radiograph

E. - Evident on radiograph * - Includes exfoliated teeth

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TABLE II

INDIVIDUAL PERIAPICAL TISSUE pH VALUES AT VARIOUS INTERVALS

DURING THE EXPERH1ENT

Initial Tissue pH pH After 1 Heek pH At Sacrifice of Infection

Animal Tooth Nesial Distal Mesial Distal Mesial Distal UR3 7.1 7.05 6.45 6.2 7.1 7.0 UL2 7.1 7.15 6.45 6.6 6.9 7.1

1 Week LR3 7.1 7.0 6.2 5.9 7.0 6.9 Dog LR2 7.1 7.2 6.9 7.1

LL2 7.1 7.1 6.85 6.6 7.1 7.0 LL3 7.15 7.1 6.8 7.3

Average 7.10 Average 6.41 Average 7.02 UR3 7.1 7.1 6.85 7.0 7.1 6.85 UL2 7.1 7.1 6.6 6.05 7.4 7.3

1 Honth LR3 7.1 7.2 6.6 6.3 7.1 7.1 Dog LR2 7.1 7.1 7.0 7.1

LL2 7.2 7.1 6.6 6.6 6.7 6.7 LL3 7.1 7.2 6.9 6.9

Average 7.13 Average 6.58 Average 7.03 UR3 7.1 7.1 6.6 6.3 7.0 6.95 UL2 7.2 7.1 6.85 6.85 E E

1 Honth LR3 7.05 7.2 6.6 6.45 6.9 6.95 Dog LR2 7.3 7.1 6.9 7.0

LL2 7.1 7.2 6.7 6.6 6.75 6.9 LL3 7.2 7.1 6.75 6.8

Average 7.15 Average 6.62 Average 6.89 UR3 7.3 7.2 6.2 5.9 7.1 6.85 UL2 7.1 7.0 6.6 6.7 7.1 6.95

3 Month LR3 7.2 6.8 6.7 6.45 7.2 7.2 Dog LR2 7.1 7.0 7.2 7.2

LL2 7.1 7.2 6.85 6.85 7.3 7.3 LL3 7.1 7.1 7.3 7.2

Average 7.09 Average 6.54 Average 7.16

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TABLE II (continued)

Initial Tissue pH pH After 1 Week pH At Sacrifice of Infection

Animal Tooth He sial Distal Mesial Distal Mesial Distal UR3 7.1 7.1 6.3 5.8 E E UL2 7.1 7.2 6.4 6.6 E E

6 Honth LR3 7.1 7.1 6.7 6.6 E E Dog LR2 7.2 7.1 E E

LL2 7.1 7.1 6.8 6.7 E E LL3 7.0 7.1 E E

Average 7.11 Average 6.48 UR3 6.9 7.0 5.9 6.0 E E UL2 7.1 7.1 6.7 6.4 E E

6 Honth LR3 7.2 7.2 6.3 6.0 7.1 7.2 Dog LR2 7.1 7.0 6.2 6.4 7.0 7.1

LL2 7.1 7.1 6.7 6.7 E E LL3 7.1 7.2 E E

Average 7.09 Average 6.33 Average 7.10

LEGEND

E - Exfoliated UR3 - Upper right third premolar UL2 - Upper left second premolar LR3 - Lower right third premolar LR2 - Lower right second premolar LL2 - Lower left second premolar LL3 - Low·er left third premolar

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TABLE III

AVERAGE PERIAPICAL TISSUE ~ VALUES AT VARIOUS TIHE

INTERVALS

I. One Week In f. Animal A.S.

I. One Honth In f. Animal A.S.

I. One Honth In f. Animal A.S.

I. Three Honth In f. Animal A.S.

I. Six Honth In f. Animal A.S.

I. Six Honth In f. Animal A.S.

I. Overall In f. Averages A.S.

DURING THE EXPERIHENT COHPARING THE

EFFECTS OF PASTE INSERTED

Acidic Paste Basic Paste Infected Only

7.10 6.53 7.04 7.13 6.76 6.92 7.13 6.55 6.93 7.20 6.45 7.12 7.10 6.40

7.03 6.33 7.05 7.12 6.50 7.01

7.08 7.14 6.30 7.01 7.00 7.13 7.15 6.37 7.03 6.98 7.14 7.17 6.68 6.93 6.88 7.03 7.05 6.61 7.10 7.21 7.13 7.10 6.58

7.15 7.10 6.35

7.15 7.11 7.12 6.48 7.02 7.04

LEGEND

I. - At beginning of the experiment Inf. -After one week infection with

S. faecalis A.S. -At sacrifice

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One Week Animal One Honth Animal One Honth Animal Three Honth Animal Six Month Animal Six Honth Animal

TABLE IV

COMPARISON OF CLINICAL FINDINGS AFTER ONE

WEEK OF INFECTION AND AT SACRIFICE

Number of Number of Exfoliated Draining Tooth Hobility Teeth Sinus Tracts

A. B. I. Total Normal Two Three

I. 1 2 3 4 2 A.S. 1 1 6 I. 1 1 2 4 1 5

A.S. 1 1 1 2 2 4* I. 2 2 2 6 1 5

A.S. 2 1 1 4 2 4 I. 1 1 1 3 4 2

A.S. 1 1 1 3 4 2 I. 1 2 2 5 6

A.S. 6 0 6* I. 2 2 1 5 6

A.S. 4 1 1 2 6>~

LEGEND

I. - After one week infection with S. faecalis A.S. - At sacrifice

A. - Acidic-treated teeth B. - Basic-treated teeth I. - Infected-only teeth * - Exfoliated teeth included

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One Week Animal One Honth Animal One Honth Animal Three Honth Animal Six Honth Animal Six Month Animal

Totals

TABLE V

CLINICAL FINDINGS AT TIHE OF SACRIFICE ----COHPARING EFFECTS

Number of Exfoliated Teeth

A. B. I.

1

2 2 2

1 1 2

3 4 4

OF PASTE INSERTED

Number of Teeth Number of Teeth With Draining With Hobility Sinus Tracts Two or Greater A. B. I. A. B.

1

1

1

1

4

2 2

1 1 2 2

1 2 2 2>'<

1 1 2 2

21~ 27\

1 2* 2i~

3 5 12* 12*

LEGEND

A. - Acidic-treated teeth B. - Basic-treated teeth I. - Infected-only teeth

I.

2

2

2

2

2>'<

z,';

12*

* Exfoliated teeth included

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One Week Animal One Month Animal One Honth Animal Three Honth Animal Six Honth Animal Six Honth Animal

Average

TABLE VI

AVERAGE PERIAPICAL TISSUE ~ VALUES OF THE

EXPERIMENTAL TEETH AT VARIOUS TIME INTERVALS

DURING THE EXPERIMENT

Initial Normal Tissue pH

pH After One pH at Sacrifice Week of Infection

7.10 6.41 7.02

7.13 6.58 7.03

7.15 6.62 6.89

7.09 6.53 7.16

7.11 6.48

7.09 6.33 7.10

7.11 6.49 7.03

102

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TABLE VII

RADIOGRAPHIC FINDINGS AT TIME OF SACRIFICE ----COMPARING EFFECTS OF PASTE INSERTED

ACIDIC PASTE BASIC PASTE INFECTED ONLY Lesion Size Smaller Same Larger Smaller Same Larger Smaller Same Larger

One Week 2 2 2 Animal One Month Animal 2 2 2 One Month Animal 2 2''' 2 Three Month Animal 2 2 2 Six Honth Animal z;~ 2* 21<

Six Month Animal z,~ 2''' 2*

Total 0 2 10* 0 2 10>'< 0 2 10>'<

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Figure 1: Typical preoperative radiographic survey. Note the wide open apices of the premolar teeth. Second premolar (2), third pre­molar (3).

Figure 2: Typical radiographic survey after one week of infection with Streptococcus faecalis. Acidic-treated tooth (A), basic-treated tooth (B), infected-only tooth (I), control tooth (C). Note the small periapical radio­lucent lesions and larger bifurcation radio­lucent lesions.

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Figure 3: Radiographic survey of one week animal at sacrifice. Acidic-treated tooth (A), basic-treated tooth (B), infected-only tooth (I), control tooth (C). Periapical radiolucent lesions are continuous with bifurcation radiolucent lesions.

Figure 4: Radiographic survey of one month animal at sacrifice. Acidic-treated tooth (A), basic-treated tooth (B), infected-only tooth (I), control tooth (C). Note severe bifurcation and periapical radio­lucent lesions.

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3

4

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Figure 5: Radiographic survey of three month animal at sacrifice. Acidic-treated tooth (A), basic-treated tooth (B), infected-only tooth (I), control tooth (C). Note severe radiolucent lesions present in upper left and lower right quadrants.

Figure 6: Radiographic survey of six month animal at sacrifice. Note that only one acidic­treated tooth (A) and one basic-treated tooth (B) remain and very little support­ing bone is evident.

]

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5

6

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Figure 7: Apex of control tooth in one >veek animal. Dental pulp (P), odontoblastic layer (0), dentin (D), Hertwig's epithelial root sheath (H), periodontal ligament (1), nerve (N), alveolar bone (B). (Hematoxylin and eosin stain, original magnification X25).

Figure 8: Furcation area of control tooth in one week animal. Dental pulp (P), dentin (D), perio­dontal ligament (1), alveolar bone (B). (Hematoxylin and eosin stain, original mag­nification X25).

llo

;. j

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p

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Figure 9: Interproximal gingival sulcus area in one week animal. Note the normal gingival attach­ment (G) adjacent to the control tooth (C) while the adjacent acidic-treated tooth (A) appears to have a deepened gingival sulcus due to the plane of section. (Hematoxylin and eosin stain, original magnification X25).

Figure 10: Apex of control tooth in one month animal. Note some blood vessel congestion (C) in the dental pulp and nerve (N) in periapical tissue. (Hematoxylin and eosin stain, orig­inal magnification X40).

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Figure 11: Apex of control tooth in three month animal. Note the completed root development and the apical arborization of the root canal in cementum. Dentin (D), cementum (C). (Hema­toxylin and eosin stain, original magnifi­cation X40).

Figure 12: Apex of control tooth in six month animal. Note that apical development is complete and the apical arborization of the root canal in cemen­tum is clearly seen. Dental pulp (P), dentin (D), cementum (G) maxillary sinus (S), perio­dontal ligament (L). Pulp fixation is poor and separation artifacts (A) can be seen. (Hematoxylin and eosin stain, original magnification X25).

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c

D

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Figure 13: Apex of infected-only tooth in one week animal. Note loss of alveolar bone, epithelial sling at apex (E), and temporary filling material in root canal (F). (Hematoxylin and eosin stain, original magnification X25).

Figure 14: Higher magnification of periapical tissue in Figure 13 showing acute inflammatory cellular infiltrate consisting mainly of polymor­phonuclear leukocytes (arrmvs). (Hematoxylin and eosin stain, original magnification X250).

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Figure 15: Periapical alveolar bone around infected-only tooth in one week animal. Note bone deposi­tion and osteoblasts (arrows) on the non­lesion side. (Hematoxylin and eosin stain, original magnification X40).

Figure 16: Apex of infected-only tooth in one month animal. Note well differentiated epithelial sling (E) around apex and probable puncture site (M) of microelectrode. (Hematoxylin and eosin stain, original magnification X40).

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: Figure 17: Higher magnification of periapical tissue in Figure 16 showing chronic inflammatory cellular infiltrate of lymphocytes, plasma cells, and macrophages. (Hematoxylin and eosin stain, original magnification X250).

Figure 18: Furcation area of infected-only tooth in one month animal. Note complete loss of furcation alveolar bone and periodontal ligament and their replacement by epithe­lium (E) with a severe subepithelial chronic inflammatory response. Pulp chamber (P), bi­furcation area (B), dentin (D). (Hematoxylin and eosin stain, original magnification X40).

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Figure 19: Apex of infected-only tooth in 3 month animal. Note the absence of periodontal ligament sup­port, epithelial sling (E), and focus of pus (P) in the sinus tract. (Hematoxylin and eosin stain, original magnification X40).

Figure 20: Apex of acidic-treated tooth in one week animal. Note the epithelial sling (E), sinus tract (S), and remnants of the acidic paste (P). (Hema­toxylin and eosin stain, original magnification X40).

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p

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Figure 21: Apex of acidic-treated tooth in one month animal. Note the well differentiated epithe­lium (E) in the apical region and remnants of the acidic-paste (A) in the root canal. (Hematoxylin and eosin stain, original mag­nification X40).

Figure 22: Isolated periodontal ligament attachment (L) of an acidic-treated tooth in one month animal. (Hematoxylin and eosin stain, orig­inal magnification X40).

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Figure 23: Apex of acidic-treated tooth in three month animal. Note the epithelial proliferation in the periapical region. (Hematoxylin and eosin stain, original magnification X25).

Figure 24: Periodontal cyst-like area adjacent to root apex seen in Figure 23. Note the well de­marcated cyst-like area (C) lined by epithe­lium and a chronic inflammatory infiltrate. (Hematoxylin and eosin stain, original mag­nification X25).

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: '

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Figure 25: Apex of acidic-treated tooth in six month animal. Note the lack of any periodontal ligament support and the severe subepithe­lial chronic inflammatory infiltrate. (Hem­atoxylin and eosin stain, original magni­fication X40).

Figure 26: Apex of basic-treated tooth in one week animal. Note the epithelial sling (E), sinus tract (S), and acute inflammatory response (A) in the periapical tissues. (Hematoxylin and eosin stain, original magnification X40).

12:

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Figure 27: Proliferating epithelium (E) is adjacent to an acute focus of pus (P) in a sinus tract of a basic-treated tooth in one week animal. Note the epithelial rests of Malassez (11). (Hematoxylin and eosin stain, original magnification X40).

Figure 28: Embedded piece of dentin in lamina propria of 1 month animal. Note the absence of in­flammation around the embedded piece of dentin (D) and temporary filling material (F). (Hematoxylin and eosin stain, original magnification X25).

1~

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Figure 29: Isolated periodontal ligament attachment of a basic-treated tooth in one month animal. Note the degenerating epithelial attachment (A) and proliferating epithelium (E). (Hematoxylin and eosin stain, original mag­nification X40).

Figure 30: Apex of basic-treated tooth in one month animal. Note epithelial sling evagination (E) into the apical region of the root canal. (Hematoxylin and eosin stain, orig­inal magnification X40).

13:

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Figure 31: Apex of basic-treated tooth in one month animal. Note dentin and cementum resorption (R) in the apical region. (Hematoxylin and eosin stain, original magnification X40).

Figure 32: Apex of basic-treated tooth in three month animal. Note extensive epithelial prolifer­ation (E), probable puncture site of micro­electrode (M), and basic paste (B), blood clot (C), and temporary filling remnants (F) in the root canal. (Hematoxylin and eosin stain, original magnification X40).

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Figure 33: Well differentiated epithelial sling of a basic-treated tooth in three month animal. The rete pegs (R) and basal and prickle cell (P) layers are evident. (Hematoxylin and eosin stain, original magnification X40).

Figure 34: Remaining socket of basic-treated tooth in six month animal. Note the remaining tooth structure was lost in preparation and a severe subepithelial chronic inflammatory response is present. (Hematoxylin and eosin stain, original magnification X40).

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APPROVAL SHEET

. This .thesis submitted by James E. McCormick, D.M.D., has been read and appr~ved by the following committee:

Franklin S. Weine, D.D.S., M.S.D. Professor and Director of Graduate Studies Department of Endodontics Loyola University School of Dentistry

Joseph D. Maggio, D.D.S. Clinical Assistant Professor Department of Endodontics Loyola University School of Dentistry

Hal D. McReynolds, Ph.D. Associate Professor Department of Histology Loyola University School of Dentistry

Ioannis S. Scarpa, Ph.D. Assistant Professor and Chairman Department of Biochemistry Loyola University School of Dentistry

The final copies have been examined by the director of the thesis and the signature which appears below verifies the fact that any necessary changes have been incorporated and that the thesis is now given final approval by the above committee with reference to content, form, and mechanical accuracy.

The thesis is therefore accepted in partial fulfillment of the require­ments for the degree of Master of Science.

Franklin S. Weine, D.D.S., M.S.D.

Signature of Advisor