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CHROMATOGRAPHIC TECHNIQUES
     FOR THE ESTIMATION OF PLANT
             HORMONES




Chithra Rajagopal
INTRODUCTION

   Chromatography : Greek word chroma [color] + grafein [to
    write]
   The collective term for a family of laboratory techniques for the
    separation of mixtures.
   Russian botanist Mikhail Semyonovich Tsvet -invented the first
    chromatography technique in 1900 during his research on
    chlorophyll.
   He used a liquid-adsorption column containing calcium
    carbonate to separate plant pigments.
Chromatogram
Chromatography (Common terms)




Solute     Solvent   Stationary phase   Analyte   Mobile phase
Chromatography (Common terms) contd.



                         Effluent
          Chromatogram                       Immobilized
                             Chromatograph   phase

Bonded
                                                     Retention
phase
                                                     time
Chromatography




      Preparative                        Analytical


Separate the components         Operates with smaller
of a mixture for further use    amounts of material and
(And is thus a form of          seeks to measure the relative
purification)                   proportions of analytes in a
                                mixture.
Chromatography theory
   Components of a mixture may be interacting with the stationary
    phase based on charge (ion-ion-interactions, ion-dipole-
    interactions), van der Waals' forces, relative solubility or
    adsorption (hydrophobic interactions, specific affinity).
Chromatographic Techniques




Techniques by             Techniques by             Techniques by
chromatographic           physical state of         separation
bed shape                 mobile phase              mechanism



                                              Ion
Column                   GC                   exchange              Affinity
         Paper                        LC
                                                   Size exclusion
Major Plant Hormones




AUXINS   CYTOKININS GIBBERLLINS      ABA   ETHYLENE
PROBLEMS IN PLANT HORMONE ESTIMATION

   Efficiency in extraction of the plant tissue is considerably low.

   Although extractable hormones may be released from tissues
    relatively quickly ,it is not possible to determine how much of the
    hormone pool has been recovered.
                                                       (Sundberg,1990)
   Even for immunoassays, sample preparation accounts for a large
    proportion of the time and effort expended in performing an
    analysis.
                                                         (Hedden,1993)
LATEST TECHNIQUES


   HPLC- High Pressure Liquid Chromatography

   LC/MS- Liquid Chromatography/Mass Spectrometry

   GC/MS- Gas Chromatography/Mass Spectrometry
HPLC
Principle of HPLC
   Forces the analyte through a column of the stationary phase by
    pumping a liquid (mobile phase) at high pressure through the
    column.
   The sample to be analyzed is introduced in small volume to the
    stream of mobile phase and is retarded by specific chemical or
    physical interactions with the stationary phase as it traverses the
    length of the column.
   The use of pressure increases the linear velocity giving the
    components less time to diffuse within the column, leading to
    improved resolution in the resulting chromatogram.
    Common solvents methanol and acetonitrile.
HPLC Overview


                                                         Polychrom           Computer
                                                   (Diode Array) Detector   Workstation




                                    Variable
                   Solvent       UV/Vis Detector
HPLC Solvent   Delivery System
 Reservoirs




                                                          Rheodyne
                                                           Injector

                                                            HPLC
                                                           Column
%A %B %C    Flow Rate     Pressure                 to column
             {H2O} {MeOH} (mL/min)      (atmos.)
                                                                             load

  Ready
                                                                             inject

                                                               Rheodyne
                                                                Injector
Varian 9010 Solvent Delivery System            to injector



                                      through pump




                                                                                Column
   through                                           C
    pulse
  dampener
                               A              B

                                                             from solvent           to
                               Ternary Pump                    reservoir         detector
LC/GC- MS
             LC/GC- MS


   Coupling of liquid chromatography (LC) or gas chromatography
    (GC) separations to a mass spectrometer provides physical
    separation of metabolites, introducing different compounds into
    the mass spectrometer at different times.

   Separation of metabolites from interfering substances allows for
    improved quantitative accuracy.

   Applications of GC/MS include drug detection, fire investigation,
    environmental analysis, explosives investigation, proteomics and
    identification of unknown samples.
LC/GC- MS
GC-MS
Working

   The molecules take different amounts of time (retention time) to
    come out of the gas chromatograph

    Allows the mass spectrometer downstream to capture, ionize,
    and detect the molecules separately.

    The mass spectrometer breaks each molecule into ionized
    fragments and detecting the fragments using their mass to
    charge ratio.
Mass Spectrometry
Reports On Different Types Of Estimation Of Plant
                   Hormones
Indole-3-acetic Acid Levels of Plant Tissue as Determined
by a new High Performance Liquid Chromatographic
Method                               (Philip et al, 1977)

   A method for the analysis of lndole-3-acetic acid (IAA) in plant
    extracts based on high performance liquid chromatography
    separation of IAA on a miroparticulate strong anion exchange
    column
   And quantitation with two selective detectors: an electrochemical,
    carbon paste amperometrc detector and/or a fluorescence
    detector.
A Rapid Method for the Extraction and Analysis of Abscisic
Acid from Plant Tissue( Kerry et al, 1980)



    The method makes use of silica Sep-pak prepacked cartridges.
    The ABA extracts are loaded on to the Sep-pak cartridges which
     are then washed with a series of solvents resulting in the removal
     of pigments and other unwanted compounds.
    The ABA is then eluted from the cartridge and the levels of this
     hormone are estimated by gas chromatography.
Headspace Gas Chromatographic Determination of
Ethylene Oxide in Air          (Binetti et al, 1986)
                               (
   Add 10 ml di-methyl acetamide(DMA)
   Keep for 1 hr
   Submit to GC determination
   The peak areas in the headspace chromatograms of the
    standard solutions are plotted against the corresponding ETO
    concentration in order to obtain the calibration curve.
Introduction

   Common purification procedures such as column
    chromatography, solid phase extraction (SPE), liquid–liquid
    extraction, etc. are employed for plant hormone purification
     – Require significant amounts of solvent, time and labor
   IAA and ABA exhibit many similar chemical properties
     – Relatively hydrophobic compounds containing a carboxylic
        group
     – common chromatographic techniques very often end up in
        the same fraction

   2D HPLC system obtain very pure separate fractions of IAA and
    ABA and quantify these compounds with much higher reliability.
Materials and methods used

   Chemicals and materials:-
     – Unlabelled IAA and ABA
     – Radioactive IAA and ABA
     – Deuterated ABA
     – 1-Methyl-3-nitro-1-nitrosoguanidine (MNNG, 97%)
     – HPLC grade methanol and acetonitrile
     – Formic acid and Ammonium hydroxide
Recoveries of standard IAA and ABA
2-D HPLC set up
Results and discussion
  – In the First dimension the sample was loaded into silica-
    cyanopropyl column.

  – When run in reversed-phase mode the polar sorbent of this
    column allows the elution of IAA and ABA with relatively low
    proportion of organic solvent.

  – Low concentration of organic solvent in the segment applied
    to the second dimension allowed concentrating IAA and ABA
    on the more hydrophobic column (silica-C18) used in the
    second dimension,
Contd.
   IAA and ABA were well retained and separated in the second
    HPLC dimension with capacity factor higher than 2 and resolution
     4.

   Relatively high throughput since the injection-to-injection cycle
    time is less than 30 min

   The results show that quantification by 2D-HPLC with on-line UV
    (ABA) and FLD (IAA) detection are statistically identical (with
    95% confidence) to the ones measured by GC–MS
   Includes an extraction with acetone/water/acetic acid (80:19:1, v/
    v), evaporation of the extracts and finally injection into the liquid
    chromatography-electro spray ionization tandem mass
    spectrometry (LC–ESI–MS–MS) system in multiple reaction
    monitoring (MRM) mode.

   The objective of this work has been to show the applicability of
    the method to quantify the endogenous content of ABA in
    Arabidopsis thaliana leaves at three different degrees of water
    stress.
LC-MS Optimization
   An LC column of 50 mm length used to analysis a high number of
    samples.

   Gradient was done in such a way that ABA elutes at approx 7 min for
    avoiding matrix interferences.

   A standard solution of ABA (1 ng µl-1 ) into the MS at 5µl min-1.

   MRM acquisition method was used for the quantification of extracts.
Results and Discussion

   The high specificity of the MRM acquisition mode allows us to
    obtain clean chromatograms (1 peak)from non-purified crude
    plant extracts, thus avoiding possible interferences to the
    analysis.

   The main contribution of this method is its speed and simplicity,
    allowing ABA to be determined in a few hours.

   solvents such as methanol/water/acetic acid (80:19:1, v/v) and
    acetone/ water/acetic acid have given consistent results and
    avoid the formation of ABA-Me
Introduction

 In this study the pH and polarity of the mobile phase were taken
into consideration to optimize the mobile phase for the
chromatographic separation of 3 important plant hormones: (ABA),
(IAA) and (GA3).

 GA3, IAA and ABA contain carboxylic groups and their retention
depends on the percentage of ionized and non-ionized species.

 The optimum pH of the mobile phase should be taken into account
to study the influence of pH on retention in LC.
Chromatographic procedure

   The mobile phases used:- Acetonitrile-water (26:74:30:70%; v/v)
   The chromatographic column equilibrated for each mobile condition
    with a time limit of 30 min.
   Column temperature :- 250 C
   Separation through Isocratic elution with a flow rate of 0.8 mL/ min.
   The standard solution of individual acid prepared in the mobile
    phase and chromatographed separately to determine the retention
    time for each acid.
   OD was measured at 208, 265, 280 nm for GA3, ABA and IAA.
Results and Discussion

   The mobile phase was adjusted to different pH values in order to
    select a suitable pH condition for chromatographic separation.
   Retention factor values, k, for the plant hormones studied were
    determined in ACN-water mixtures at 26% and 30% (v/v) of
    acetonitrile.
   Six pH values (4.0, 4.5, 5.0, 5.5, 6.0 and 7.0) were investigated
    for the mobile phase.
   The GA3, ABA and IAA content of 2 plant samples were
    determined in acetonitrile-water, 26% (v/v) containing 30 mM
    phosphoric acid at pH 4.00.
Chromatogram of the plant hormones
GC-MS ANIMATION




http://www.shsu.edu/~chm_tgc/sounds/flashfiles/GC-MS.swf
Chromatographic technique
Chromatographic technique
Chromatographic technique

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Chromatographic technique

  • 1. CHROMATOGRAPHIC TECHNIQUES FOR THE ESTIMATION OF PLANT HORMONES Chithra Rajagopal
  • 2. INTRODUCTION  Chromatography : Greek word chroma [color] + grafein [to write]  The collective term for a family of laboratory techniques for the separation of mixtures.  Russian botanist Mikhail Semyonovich Tsvet -invented the first chromatography technique in 1900 during his research on chlorophyll.  He used a liquid-adsorption column containing calcium carbonate to separate plant pigments.
  • 3.
  • 5. Chromatography (Common terms) Solute Solvent Stationary phase Analyte Mobile phase
  • 6. Chromatography (Common terms) contd. Effluent Chromatogram Immobilized Chromatograph phase Bonded Retention phase time
  • 7. Chromatography Preparative Analytical Separate the components Operates with smaller of a mixture for further use amounts of material and (And is thus a form of seeks to measure the relative purification) proportions of analytes in a mixture.
  • 8. Chromatography theory  Components of a mixture may be interacting with the stationary phase based on charge (ion-ion-interactions, ion-dipole- interactions), van der Waals' forces, relative solubility or adsorption (hydrophobic interactions, specific affinity).
  • 9. Chromatographic Techniques Techniques by Techniques by Techniques by chromatographic physical state of separation bed shape mobile phase mechanism Ion Column GC exchange Affinity Paper LC Size exclusion
  • 10. Major Plant Hormones AUXINS CYTOKININS GIBBERLLINS ABA ETHYLENE
  • 11.
  • 12. PROBLEMS IN PLANT HORMONE ESTIMATION  Efficiency in extraction of the plant tissue is considerably low.  Although extractable hormones may be released from tissues relatively quickly ,it is not possible to determine how much of the hormone pool has been recovered. (Sundberg,1990)  Even for immunoassays, sample preparation accounts for a large proportion of the time and effort expended in performing an analysis. (Hedden,1993)
  • 13. LATEST TECHNIQUES  HPLC- High Pressure Liquid Chromatography  LC/MS- Liquid Chromatography/Mass Spectrometry  GC/MS- Gas Chromatography/Mass Spectrometry
  • 14. HPLC
  • 15. Principle of HPLC  Forces the analyte through a column of the stationary phase by pumping a liquid (mobile phase) at high pressure through the column.  The sample to be analyzed is introduced in small volume to the stream of mobile phase and is retarded by specific chemical or physical interactions with the stationary phase as it traverses the length of the column.  The use of pressure increases the linear velocity giving the components less time to diffuse within the column, leading to improved resolution in the resulting chromatogram.  Common solvents methanol and acetonitrile.
  • 16. HPLC Overview Polychrom Computer (Diode Array) Detector Workstation Variable Solvent UV/Vis Detector HPLC Solvent Delivery System Reservoirs Rheodyne Injector HPLC Column
  • 17. %A %B %C Flow Rate Pressure to column {H2O} {MeOH} (mL/min) (atmos.) load Ready inject Rheodyne Injector Varian 9010 Solvent Delivery System to injector through pump Column through C pulse dampener A B from solvent to Ternary Pump reservoir detector
  • 18. LC/GC- MS LC/GC- MS  Coupling of liquid chromatography (LC) or gas chromatography (GC) separations to a mass spectrometer provides physical separation of metabolites, introducing different compounds into the mass spectrometer at different times.  Separation of metabolites from interfering substances allows for improved quantitative accuracy.  Applications of GC/MS include drug detection, fire investigation, environmental analysis, explosives investigation, proteomics and identification of unknown samples.
  • 20. GC-MS
  • 21. Working  The molecules take different amounts of time (retention time) to come out of the gas chromatograph  Allows the mass spectrometer downstream to capture, ionize, and detect the molecules separately.  The mass spectrometer breaks each molecule into ionized fragments and detecting the fragments using their mass to charge ratio.
  • 23. Reports On Different Types Of Estimation Of Plant Hormones
  • 24. Indole-3-acetic Acid Levels of Plant Tissue as Determined by a new High Performance Liquid Chromatographic Method (Philip et al, 1977)  A method for the analysis of lndole-3-acetic acid (IAA) in plant extracts based on high performance liquid chromatography separation of IAA on a miroparticulate strong anion exchange column  And quantitation with two selective detectors: an electrochemical, carbon paste amperometrc detector and/or a fluorescence detector.
  • 25. A Rapid Method for the Extraction and Analysis of Abscisic Acid from Plant Tissue( Kerry et al, 1980)  The method makes use of silica Sep-pak prepacked cartridges.  The ABA extracts are loaded on to the Sep-pak cartridges which are then washed with a series of solvents resulting in the removal of pigments and other unwanted compounds.  The ABA is then eluted from the cartridge and the levels of this hormone are estimated by gas chromatography.
  • 26. Headspace Gas Chromatographic Determination of Ethylene Oxide in Air (Binetti et al, 1986) (
  • 27. Add 10 ml di-methyl acetamide(DMA)  Keep for 1 hr  Submit to GC determination  The peak areas in the headspace chromatograms of the standard solutions are plotted against the corresponding ETO concentration in order to obtain the calibration curve.
  • 28.
  • 29.
  • 30. Introduction  Common purification procedures such as column chromatography, solid phase extraction (SPE), liquid–liquid extraction, etc. are employed for plant hormone purification – Require significant amounts of solvent, time and labor  IAA and ABA exhibit many similar chemical properties – Relatively hydrophobic compounds containing a carboxylic group – common chromatographic techniques very often end up in the same fraction  2D HPLC system obtain very pure separate fractions of IAA and ABA and quantify these compounds with much higher reliability.
  • 31. Materials and methods used  Chemicals and materials:- – Unlabelled IAA and ABA – Radioactive IAA and ABA – Deuterated ABA – 1-Methyl-3-nitro-1-nitrosoguanidine (MNNG, 97%) – HPLC grade methanol and acetonitrile – Formic acid and Ammonium hydroxide
  • 32. Recoveries of standard IAA and ABA
  • 34. Results and discussion – In the First dimension the sample was loaded into silica- cyanopropyl column. – When run in reversed-phase mode the polar sorbent of this column allows the elution of IAA and ABA with relatively low proportion of organic solvent. – Low concentration of organic solvent in the segment applied to the second dimension allowed concentrating IAA and ABA on the more hydrophobic column (silica-C18) used in the second dimension,
  • 35. Contd.  IAA and ABA were well retained and separated in the second HPLC dimension with capacity factor higher than 2 and resolution 4.  Relatively high throughput since the injection-to-injection cycle time is less than 30 min  The results show that quantification by 2D-HPLC with on-line UV (ABA) and FLD (IAA) detection are statistically identical (with 95% confidence) to the ones measured by GC–MS
  • 36.
  • 37. Includes an extraction with acetone/water/acetic acid (80:19:1, v/ v), evaporation of the extracts and finally injection into the liquid chromatography-electro spray ionization tandem mass spectrometry (LC–ESI–MS–MS) system in multiple reaction monitoring (MRM) mode.  The objective of this work has been to show the applicability of the method to quantify the endogenous content of ABA in Arabidopsis thaliana leaves at three different degrees of water stress.
  • 38. LC-MS Optimization  An LC column of 50 mm length used to analysis a high number of samples.  Gradient was done in such a way that ABA elutes at approx 7 min for avoiding matrix interferences.  A standard solution of ABA (1 ng µl-1 ) into the MS at 5µl min-1.  MRM acquisition method was used for the quantification of extracts.
  • 39. Results and Discussion  The high specificity of the MRM acquisition mode allows us to obtain clean chromatograms (1 peak)from non-purified crude plant extracts, thus avoiding possible interferences to the analysis.  The main contribution of this method is its speed and simplicity, allowing ABA to be determined in a few hours.  solvents such as methanol/water/acetic acid (80:19:1, v/v) and acetone/ water/acetic acid have given consistent results and avoid the formation of ABA-Me
  • 40.
  • 41.
  • 42. Introduction  In this study the pH and polarity of the mobile phase were taken into consideration to optimize the mobile phase for the chromatographic separation of 3 important plant hormones: (ABA), (IAA) and (GA3).  GA3, IAA and ABA contain carboxylic groups and their retention depends on the percentage of ionized and non-ionized species.  The optimum pH of the mobile phase should be taken into account to study the influence of pH on retention in LC.
  • 43. Chromatographic procedure  The mobile phases used:- Acetonitrile-water (26:74:30:70%; v/v)  The chromatographic column equilibrated for each mobile condition with a time limit of 30 min.  Column temperature :- 250 C  Separation through Isocratic elution with a flow rate of 0.8 mL/ min.  The standard solution of individual acid prepared in the mobile phase and chromatographed separately to determine the retention time for each acid.  OD was measured at 208, 265, 280 nm for GA3, ABA and IAA.
  • 44. Results and Discussion  The mobile phase was adjusted to different pH values in order to select a suitable pH condition for chromatographic separation.  Retention factor values, k, for the plant hormones studied were determined in ACN-water mixtures at 26% and 30% (v/v) of acetonitrile.  Six pH values (4.0, 4.5, 5.0, 5.5, 6.0 and 7.0) were investigated for the mobile phase.  The GA3, ABA and IAA content of 2 plant samples were determined in acetonitrile-water, 26% (v/v) containing 30 mM phosphoric acid at pH 4.00.
  • 45. Chromatogram of the plant hormones