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Chromatographic Methods: Basics AdvancedChromatographic Methods: Basics, Advanced HPLC Methods
Lecture of Seema Mishra in the advanced course “Bioinorganic Chemistry & Biophysics of Plants” 2012
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Chromatography: Basics
Chromatography a physical method for the separation of mixtureg p y p y pbased on the concept of partition coefficient
Chromatography involves two phasesChromatography involves two phasesMobile phase: a liquid/ gas which caries the mixture to be separated Stationary phase: through which the mixture is carried by mobile Phase it can be solid/ liquidPhase, it can be solid/ liquid
Separations are carried out based on differences in physical andCh i l ti f tit t f i t hChemical properties of constituents of a mixture such assize, shape, mass, charge, boiling point, polarity or chemical affinity
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Chromatography: Terminology
Chromatogram: The visual output of theChromatogram: The visual output of the chromatograph
Retention time: The characteristic timeRetention time: The characteristic time a particular analyte takes to pass throughthe system i.e. from column inlet to the
k ipeak maxima
Peak height: The distance between thepeak maximum and the base line
Peak width: The distance between each side of a peak measured at certain height of the peakof the peak
x-axis= the time and y-axis = a signal
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Chromatography: principle/TheoryChromatography: principle/Theory
the solutes will elute in order of their increasing distribution coefficients with respect to the stationary phase
Plate theory: column is considered to be divided into a number of plates
N = 5 55* t 2/ w ½2N = 5.55 tR / w ½
equilibrium must exist in each plateXs = KXm
(Xm) ; concentration of solute in the mobile phase ( m) ; p(Xs) ; concentration of solute in the stationary phase(K); distribution coefficient of the solute between the two
phases with reference to the stationary phasephases with reference to the stationary phase
K X /XK = Xs/Xm
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Chromatography: principle/TheoryChromatography: principle/Theory
the change of mass of solute (dm) in plate (p) will be
d = (X X )dVdm = (Xm(p-1) - Xm(p))dV
At equilibrium dm = vsdXs(p) + vmdXm(p)
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Chromatography: principle/Theoryg p y p p y
X = X e-v vn / n !Xm(n) = X0 . e v / n !
Basic elution curve equation it shows that if (n= no. of theoretical plates) is large, the function tends to the Gaussian function.
Vr = Vm + KVSVr = Vm KVS
The retention volume depends solely on the distribution coefficient and the volumes of the two phases that are present in the columnthe two phases that are present in the column.
K(A) < > K(B) or VS(A) < > VS(B)
The separation of two solutes depends exclusively on the magnitude of their distribution coefficients (K(A)) and (K(B)) and the amount of stationary phase available to them, (V(A)) and (V )and (V(B)).
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ChromatographyElution mode
Isocratic elution : The composition of the mobilephase kept constant through out elution
Isocratic elution
Gradient elution : The composition of the mobile phasevaried during elutionvaried during elution
Linear gradient Linear gradient
% B
Linear gradient
Step gradient Step gradient Step gradient
min
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Chromatographyg p yElution mode
PAH analysis through HPLCy g
I ti l ti
Gradient elution
Isocratic elution
ACN/H2OACN/H O 70/30 ACN/H2O0-5 50/505-20 100/0
ACN/H2O 70/30
20-30 100/0
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Chromatography: TypesChromatography: TypesBased on shape of chromatography (stationary phase)
Paper chromatography:Paper chromatography: - A paper serves as stationary phase - Separating and identifying mixtures by colour
Thin layer chromatography: - Thin layer of silica gel, alumina or cellulose adsorbed on an inert substrateadsorbed on an inert substrate
Column chromatography: Th t ti h i k d i l- The stationary phase is packed in a column
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Chromatography: Typesg p y ypBased on physical state of mobile phase
Gas chromatography: -Mobile phase is gas like Hep g
Applications: Analytical chemistry, petrochemical environmental monitoringpetrochemical, environmental monitoring
Not good for bimolecules e.g. protein due to high heatheat
Liquid chromatography : Mobile phase is liquid
e.g. high performance liquid chromatogrephy g g p q g p y
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Hi h f li id h t hChromatography: Types
High performance liquid chromatography
Optimized for rapid high resolution separations-Very high efficiency HPLC columns with inert packing materials- Fine particle packing (5µm) providing larger surface for interaction- HPLC high pressure pumps with very constant flow (6000-10000 psi) -Unique high accuracy, low dispersion, HPLC sample valvesUnique high accuracy, low dispersion, HPLC sample valves
(sub µl - few µl )- Extremely precise gradient mixers (optional).
High sensitivity low dispersion HPLC detectors- High sensitivity low dispersion HPLC detectors
A li tiApplicationsquality control, process control, forensic analysis, environmentalmonitoring and clinical testing
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Chromatography: TypesHigh performance liquid chromatography
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Chromatography: TypesHigh performance liquid chromatography
Normal phase (NP-HPLC): Polar stationary phase e.g. silica Non polar mobile phase e.g. Toluene Polar interactionNon polar Polarp
Reverse phase (RP-HPLC): Non polar stationary phase e.g. C18Reverse phase (RP HPLC): Non polar stationary phase e.g. C18Polar mobile phase such as waterHydrophobic interactionPolar Non polarPolar Non polar
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Chromatography: TypesHydrophilic interaction chromatography (HILIC-HPLC)
-A kind of partition chromatography - solute equilibrate between a liquid stationary phase and eluent-Separation based on polar differencesSeparation based on polar differences-Can separate acid, base and neutral molecule in single chromatogram -Good for separation of very polar compounds such as amino acids, glycopeptides oligonucleotides and highly polar natural productsglycopeptides, oligonucleotides, and highly polar natural products
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Ion exchange chromatographyChromatography: TypesIon exchange chromatography
Principle: highly charged proteins bind stronger to the column material, so that they elute at higher salt concentrations in the buffer than less charged proteins
From: www.ucl.ac.uk/~ucbcdab/enzpur/ionX.htm
foto of phycobiliprotein purification in the lab of H. Küpper on a MonoQ anion exchange column
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Ion pair chromatographyChromatography: Types
Ion pair chromatography
- Ion Pair Chromatography is a method for improving the separation of charged analytesg p y p g p g y-The ion pair reagents comprise of an alkyl chain with an ionizable terminus
Advantages over ion exchange
- Simple preparation of buffers- Wide choice of carbon chain lengths for i d t ti d tiimproved retention and separation
- Significantly reduced separation time-Simultaneous separation of both ionizedand nonionized solutes
- Highly reproducible results- Improved peak shapep p p
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i l i h t hChromatography: Types
size exclusion chromatography
Principle: Small proteins can enter more of the pores in the column material than large proteins, so that small proteins migrate slower
From: elchem.kaist.ac.kr From: http://en.wikipedia.org/wiki
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Chromatography: Types
The higher-affinity solutes are preferentially
Displacement chromatographyg y p y
retained near the head of the column, withthe lower-affinity solutes moving fartherdownstream each making pure zonesdownstream each making pure zones
A displacer having higher affinity than Sample components will push otherSample components will push other Components downstream making a displacement train
Advantage:Comparatively more material can be p yseparated High-retention conditions can achieved without gradient operationwithout gradient operation
Disadvantage:Overlap of zone may occurOverlap of zone may occur Difficulty in interpretation on chromatogramColumn regeneration
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Affinity chromatographyChromatography: TypesAffinity chromatography
Based on a highly specific interaction between analyte and stationary phase
dolly.biochem.arizona.edu/.../methods.html foto of TcHMA4 purification in the lab of H. Küpper on an IMAC column
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Chromatography: TypesS i l t h iSpecial techniques
Fast protein liquid chromatographyFast protein liquid chromatography-Also called as fast performance liquid chromatographyOften used for protein purification- Often used for protein purification
- Operates at low pressure typically less than 5 bar- flow rate is relatively high, typically 1-5 ml/min.-Relatively low cost-Pressure is not a limitation
Supercritical fluid chromatography(SFC)- Mobile phase is carbon dioxide-To separate thermally labile moleculesTo separate thermally labile molecules- Separation of chiral coumpounds
Chiral column chromatography:- Chiral stationary phase
F ti f ti- For separation of enantiomers
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Chromatography: TypesSpecial techniquesSpecial techniques
Two-dimensional chromatography:-Two columns with different physicochemical properties are used- Increased peak capacity
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Hyphenated techniquesHyphenated Techniques combine
chromatographic and spectral methods tol it th d t f b thexploit the advantages of both.
Chromatography - Produces pure or nearly pure fractions of chemical components in a mixturecomponents in a mixture.
Spectroscopy – Produces selective information for identification using p py gstandards or library spectra.
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Hyphenated techniquesyp q
LC-Absorbance data
James K Hardy and The University of Akron http://ull chemistry uakron edu/chemsep/hyphen/James K. Hardy and The University of Akron http://ull.chemistry.uakron.edu/chemsep/hyphen/
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Hyphenated techniquesHyphenated techniquesLiquid chromatography- mass spectrometry (LC-MS)
ESI-MS HPLC
QTOF-MS
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Hyphenated techniquesyp qHPLC-ICP-MS
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Inductively Coupled Plasma Mass Spectrometry (ICP-MS)
argongas
From: Perkin Elmer teaching file (top); LC-ICP-MS experiment at UFZ Leipzig (bottom)
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Hyphenated techniquesHPLC-ICP-MS
S i ti f A i Pl t t t th h RP HPLC (C18) l d t ICP MS
1
Speciation of As in Plant extract through RP-HPLC (C18) coupled to ICP-MS
9
76
10
23 54
11 14138 12 15
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Hyphenated techniquesHPLC-ICP-MS-ESI-MS
(II)
(II)
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Hyphenated techniquesHPLC-ESI-MS-ICP-MS
ESI MSICP-MS ESI-MS HPLC
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Hyphenated techniquesHPLC ESI MS ICP MSHPLC-ESI-MS-ICP-MS
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Hyphenated techniquesHPLC-ESI-MS-MS
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Analytical LabUFZ, LeipzigUFZ, Leipzig
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Analytical LabUFZ LeipzigUFZ, Leipzig
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The slides can be downloaded from the workgroup hhomepage
ni konstan de Department of Biolog Workgro ps Küpper labwww.uni-konstanz.de Department of Biology Workgroups Küpper lab,
or directlyy
http://www.uni-konstanz.de/FuF/Bio/kuepper/Homepage/AG_Kuepper_Homepage.html