MICRONUCLEUS ASSAY

Kanazawa, BEMS 2007

Maria Rosaria Scarfì

CNR – IREA

Institute for Electromagnetic Sensing of Environment Naples, Italy

scarfi.mr@irea.cnr.it

IREA

MICRONUCLEIObservation of chromosomes and counting of

aberrations in metaphases is the most detailed analysis to measure chromosome damage

•Complexity and time consuming

•Confounding effects of artefactual loss of chromosomes from

metaphases

•Stimulated the development of a simpler method to

measure chromosome damage

FragmentsDicentricRing

Kanazawa, BEMS 2007

IREA

MICRONUCLEI

first described in the cytoplasm of erythocytes

small nuclei separated from the main nucleus

produced during nuclear division

contain chromosomes or chromosome fragments, derived from mitotic spindle

dysfunction or acentric fragments

Kanazawa, BEMS 2007

IREA

MICRONUCLEIMNi expressed in cells that have completed nuclear

division

ideally scored in the binucleated stage of the cell cycle

the assay cannot be applied efficiently or quantitatively in non-dividing cells

Kanazawa, BEMS 2007

IREA

X XX

X X X

X X X

X X X

Kanazawa, BEMS 2007

MICRONUCLEIIREA

Chromosome loss

Chromosome breakage

MICRONUCLEI

a need to develop a method that within a cell population could distinguish between cells that are not dividing and cells that are undergoing mitosis

because of the uncertainty of the fate of MNi following more than one nuclear division it is important to identify cells that have completed one nuclear division only

Kanazawa, BEMS 2007

IREA

CBMN ASSAYSeveral methods have been proposed

CITOKINESIS BLOCK METHOD

successfully introduced in many laboratories all over the world

versatility, simplicity and lack of effects on base-line genetic damage

Provides an index of both chromosome loss and chromosome breakage

monitoring exposed population

identifying mutagen-sensitive individuals

in vitro studiesKanazawa, BEMS 2007

IREA

CBMN ASSAY

mitosis

+Cyt-B

-Cyt-B

CITOKINESIS BLOCK METHOD (1985)

Cytochalasin-B (inhibitor of cytokinesis)once divided cells are binucleates

S.B. Carter, 1967

M.Fenech & A.Morley (1985)

Kanazawa, BEMS 2007

IREA

CBMN ASSAY

S phaseanaphase

Cyt-B

Kanazawa, BEMS 2007

IREA

CBMN ASSAY - method

72 hours

t=0 t=44h

Start culture (PHA)

+ Cyt-B

harvest

in human peripheral blood lymphocytes

cultures with whole blood or separate lymphocytes(culture medium and growth factors i.e. FCS and L-

G)

Kanazawa, BEMS 2007

IREA

CBMN ASSAY

Escaped block or

slow proliferation

more than one

nuclear division

Kanazawa, BEMS 2007

IREA

CBMN ASSAY

Mononucleated cells with MN  damage accumulated before cultivation of the cells (spontaneous)

Binucleated cells with MN   spontaneous damage + damage expressed

during cultivation (treatment)

MN must be counted only

in binucleated cells

Kanazawa, BEMS 2007

IREA

CBMN ASSAY

Experimental procedure in use in our Lab

Kanazawa, BEMS 2007

IREA

In the following, the experimental

procedures currently in use in our lab to

perform the CBMN assay in human

lymphocytes and in several cell lines are

shown.

The protocol for lymphocyte separation starting from a buffy coat obtained by the transfusion unit of a hospital is shown.The buffy coat is transferred in a sterile tube and diluted (1:2) in culture medium, gently mixed and stratified on a density gradient solution in a ratio of 2 to 1 for lymphocytes isolation.

CBMN assay is applied on both isolated and whole blood lymphocytes.

Experimental procedure in use at IREA Lab

confined at the interface between density gradient solution and the culture medium. A portion of medium is discarded and cells can be collected.After two washing steps in sterile PBS solution, cells are stained with Trypan blue and counted with a haemocytometric chamber to seed the required number of cells for each culture.

Experimental procedure in use at IREA Lab

Following a centrifugation at 2100 rpm for 30 minutes, lymphocytes are

RPMI, FCS, L-Glutamine and PHA, as mitogen, to stimulate lymphocytes to enter cell cycle. In the case of whole blood cultures, heparinized blood, collected by venipuncture, is directly diluted in complete medium, according to standard procedures. In both cases, samples are located for 44 h in a CO2 incubator, then Cytochalasin-B is added.

Experimental procedure in use at IREA Lab

Isolated lymphocytes are seeded in complete culture medium composed by

After 72 h of growth, cultures are harvested and slides prepared.

Procedure to make up slides from whole blood cultures:

a)Collection of 1 ml culture

b)Centrifugation at 3000 rpm for 1 minute

c)Red cells break (lysis buffer for 7 minutes)

d)3 washing steps e)Hypotonic

treatment (15 min).

Experimental procedure in use at IREA Lab

cytospinned for 7 min. Slides are air dried, fixed and stained in a Giemsa solution.Stained cells are confined in a spot on the slides and a coverslip is used to preserve the sample for microscope screening.The procedure described for whole blood cultures is also applied for isolated lymphocyte and cell line cultures, except for the lysis step, due to the absence of erythrocytes.

Experimental procedure in use at IREA Lab

Slides are prepared by using a cytospin. Cells in hypotonic solution are

Solutions requested to harvest cells

- Lysis buffer: EDTA disodium salt 0.1 mM; NH4 Cl 155

mM; KHCO3 10 mM

- Wash medium: RPMI medium +2% FBS

- Hypotonic solution: wash medium + distilled water (1:4)

- Fixation: 80% methanol in distilled water

- Staining: 5% Giemsa in phosphate buffer pH 6.8

Experimental procedure in use at IREA Lab

Advantagesvery sensitive and simple indicator of chromosome damage,

which also provides information on cell cycle progression

less time-consuming respect to chromosomal aberrations

Biomarker of effect: relevant for risk assessment of cancer

Scoring performed relatively easily

Applied on different cell types relevant for human biomonitoring: lymphocytes, fibroblasts and exfoliated

epithelial cells

Increased statistical power

DisadvantagesNo information on the type of chromosomal aberration

CBMN ASSAY

Kanazawa, BEMS 2007

IREA

CBMN ASSAY – HUMN projectInternational Collaborative Project

on MN Frequency in Human Population (HUMN)

34 laboratories in 21 countries participate to the Project

Coordinator: Dr. M. Fenech at CSIROto compare the baseline MN frequency from different labs and among different populations

to compare different techniques to define a standard protocol

to evaluate the suitability of MN as biomarker of risk for diseases such as cancerhttp://www.csiro.au/index.asp?type=activity&id=HUMN

Kanazawa, BEMS 2007

launched in 1997 because of world-wide interest in the MN method to assess environmental effects on chromosome damage in blood and epithelial tissues in

human populations

IREA

Kanazawa, BEMS 2007

IREACBMN ASSAY – HUMN project

Factors influencing MN frequencyAge, sex, life style (smoking, alcohol consumption, diet), drugs, X-rays

Criteria for slides scoringnumber of cells and morphological criteria

Recommendations for performing the MN assay on several cell typeslymphocytes, primary cells and cell lines

Kanazawa, BEMS 2007

Main results of the HUMN project

IREACBMN ASSAY – HUMN project

CBMN ASSAY: scoring criteria

Kanazawa, BEMS 2007

IREA

CBMN ASSAY: scoring criteria

Well stained cellsUndamaged cytoplasmic

membrane

main nuclei of similar dimension

No more than 6 MN per cell

MN with same colour of main nuclei

MN morphologically similar to nuclei and no larger than 1/3 of

the main nucleus

Samples in duplicate

1000 binucleated cells/sample

Kanazawa, BEMS 2007

IREA

Nucleoplasmic bridges(dicentric

chromosomes)

Necrotic cells (vacuolated cytoplasm

and fragmented nucleus)

Apoptotic cells (condensed chromatin)

Kanazawa, BEMS 2007

IREA CBMN ASSAY: scoring criteria

by scoring the number of nuclei in 500 cells

a) cytokinesis-block proliferation index (CBPI)mean number of cell cycles per cell

CBPI = ([M1 + 2M2 + 3(M3 + M4)]) / NIndex of cell kinetics

b) binucleate cell index (BCI)% cells in first mitosis

BCI = Binucleated Cells/NIndex of cytotoxicity

Kanazawa, BEMS 2007

IREA CBMN ASSAY: scoring criteria

CBMN ASSAY – Other cell types

Kanazawa, BEMS 2007

IREA

CB-Method adapted to other primary cell types or cell lines

To assess the cell cycle duration to define the right time for Cyt-B addition (first cell

cycle) and for cell harvest (prior to the second mitosis)

To determine the concentration of Cyt-B to block the maximum number of dividing cells

To use cell types with low and stable background frequency of MN (30/1000 CB

cells)to guarantee the sensitivity of the assay to detect

genotoxic effectsKanazawa, BEMS 2007

IREA CBMN ASSAY – Other cell types

Kanazawa, BEMS 2007

IREA CBMN ASSAY – cancer risk

IREA

Kanazawa, BEMS 2007

6718 subjects from of 10 countries, screened in20 labs for MN frequency between 1980 and 2002

selected from the database of the HUMN project and followed up for cancer incidence or mortality.

To standardize for the inter-laboratory variability subjects were classified according to the percentiles of MN distribution within each laboratory as low, medium or high frequency.

CBMN ASSAY – cancer risk

IREA

Kanazawa, BEMS 2007

A significant increase of all cancers incidence was found for the groups with medium and high MN frequency The same groups also showed a decreased cancer-freesurvival.

This association was present in all national cohorts and for all major cancer sites, especially urogenital and gastro-intestinal cancers

The results provide preliminary evidence that MN frequency in PBL is a predictive biomarker of cancer risk within a population of healthy subjects.

CBMN ASSAY – cancer risk

CBMN ASSAY – centromeric staining

Kanazawa, BEMS 2007

IREA

.

.

The combination of the micronucleus assay with staining techniques of the centromeric region of the chromosomes allows discrimination between micronuclei containing a whole chromosome (centromere positive micronucleus) and an acentric chromosome fragment (centromere negative micronucleus)

It is possible by using

– Abs that bind to kinetochore proteins assembled at the centromeric regions (not specific for single

chromosomes) CREST

– probes that are specific for centromeric DNA FISH

CREST assayImmunofluorescence

staining with antibodies anti-kinetochore

Centromeres of MN can be immunologically visualized with

antikinetochore Ab from scleroderma patients of the CREST subtype (calcinosis,

Raynaud phenomenon, esophageal dismotility,

sclerodactily and telangiectasia)

CREST serum contains antibody to a specific protein of the kinetochore region of

chromosomesKanazawa, BEMS 2007

IREACBMN ASSAY – CREST

staining

Kanazawa, BEMS 2007

IREACBMN ASSAY – FISH

pan-centromeric probes - not specific for single chromosomes

chromosome-specific centromeric probes

FISH techniquefluorescence in situ

hybridisation with a DNA probe specific to the centromeric

regions

Kanazawa, BEMS 2007

FISH using pan-centromeric probe

IREACBMN ASSAY – FISH

Chung et al., Mutation Res. 516, 49–56 (2002)

a) one red and two green signals in each sister nucleus and two red signals in one of four MN b) same nuclei counter-stained with DAPI

FISH using chromosome-specific centromeric probes

CBMN ASSAY – FISH

Kanazawa, BEMS 2007

aneuploidy in CB-lymphocytes with MN

a b

Chromosome 7

Chromosome 8

IREA

Information on:

Genotoxicitychromosome loss (clastogenic events)chromosome breakage (aneugenic events)dicentric chromosomes (nucleoplasmic bridges)

Cytotoxicityapoptotic cellsnecrotic cellscell cycle kinetics (CBPI)% of binucleated cells (BCI)Kanazawa, BEMS 2007

IREA CBMN ASSAY

erythroblast matureerythrocytes

Differentiation process from the erythroblast to the mature erythrocyte

ExpulsionOf the nucleus

Type I Type II Type III Type VI

RETICULOCYTES

Micronucleus assay

Kanazawa, BEMS 2007

IREA MN ASSAY in erythrocytes

In vivo MN test in mammalian erythrocytes

Micronucleus in a type I reticulocyte AO

stained

Kanazawa, BEMS 2007

IREA

The frequency of MN in reticulocytes and erythrocytes increases in response to a

genotoxic treatment

MN ASSAY in erythrocytes

As the average life-span is much longer than immature erythocytes, MN assay is reliable when chronic, but not acute, treatments are performed

Advantage - blood can be obtained by tail venupuncture without sacrifying animals (multiple

sample collection)

Largely employed since 1991

Vijayalaxmi, Obe G Radiat Res. 162: 481-96 (2004)

Vijayalaxmi and G.Obe Bioelectromagnetics 26: 412-430 (2005)

Moulder et al., Int J Radiat Biol 81: 189-203 (2005)

Verschaeve L, Toxicol Appl Pharmacol. 207: 336-41 (2005)

IREA

Kanazawa, BEMS 2007

MN ASSAY in BEMS research