TRANSFER OF PROTEIN FROM ELECTROPHORETIC BANDS INTO MASS SPECTROMETRY BY DIRECT ELECTROELUTION
     
Andreas Chrambach, Ph.D., Principal Investigator
Sergey Radko, Ph.D., Contractor
Zsuzsa Buzás, Ph.D., Contractor
Alfred Yergey, Ph.D., Collaborator, LCMB
Nancy Vieira, M.S., Collaborator, LCMB
Marcella Chiari, Ph.D., Collaborator, Institute of Molecular Recognition Chemistry, CNR, Milan, Italy
Marina Cretich, Ph.D., Collaborator, Institute of Molecular Recognition Chemistry, CNR, Milan, Italy
Huang-Tung Chang, Ph.D., Collaborator, National Taiwan University, Taipei, Taiwan
Andreas Chrambach
 

The Section on Macromolecular Analysis is attempting to upgrade the common practice of gel electrophoresis by undertaking the following projects: the development of theory and computer programs for deriving information from mobility regarding physical properties of analytes and polymer networks and for predicting resolution, resolution of presently unresolved or poorly resolved analyte types such as subcellular-sized particles and the size- and charge-isomeric forms of peptides and their complexes, the development of detergent and miniaturized gel methods suitable for native membrane proteins and their complexes of a low level of occurrence, and the development of automated analytic and preparative gel electrophoresis methods.

A significant portion of current biological research focuses on an account of the cellular proteins responsible for the activities and functions of the cell. One aspect of that research, designated proteomics, is working, by means of mass spectrometry, toward the identification of proteins on the basis of their mass. Conventional practice calls for separating the mixture of proteins in the cellular extract of interest by two-dimensional gel electrophoresis and detecting the proteins as "spots" by specific staining methods. The spot of interest is then excised from the gel, the gel slice is dehydrated and reswollen in the presence of the proteolytic enzyme trypsin, and the tryptic peptides derived from the protein are eluted from the gel slice for measurement of their mass by mass spectrometry. The mass of the peptides is then compared with that of aminoacid sequences in databases stored in computer memory and derived from the corresponding DNA sequence. Such identification therefore depends on a previous genetic analysis of the cellular material in question.

Our laboratory developed an alternative procedure for collecting protein identified as a gel band (or spot); it replaces band excision with direct electroelution of the intact protein by placing electrodes across the band at a direction orthogonal to that of electrophoretic migration in the separating gel (Figure 10). The alternative procedure offers several advantages over conventional practice. First, it is applicable to those cases in which no earlier DNA sequence analysis has been performed and for which, therefore, no sequence exists in the database. Second, even where a sequence has been determined, the procedure adds the mass of the intact protein to that of its constituent peptides for purposes of identification. Third, it allows for electrofocusing (IEF) and critical re-electrophoresis analysis of the eluate before mass spectrometry. Fourth, it avoids the presence of gel during tryptic digestion, thus increasing the rate of digestion and avoiding adsorption of protein, peptides, and enzyme. Fifth, it appears more adaptable than an excision procedure to automation of sequential spot elution. We were able to verify the first three advantages while the last two remain hypothetical. The primary potential importance of such an approach, compared with conventional practice, lies in the fact that the electroelution of the intact protein, when applied to Immobiline IEF gel strips of high load capacity, allows for an accumulation of large protein loads for a subsequent two-dimensional electrophoretic separation with a number of narrow pH gradients in the first dimension and subsequent peptide analysis of the bands. The alternative approach will allow for a significant increase in the number of proteins detected by two-dimensional gel electrophoresis, which currently yields only 10 to 20 percent of proteins, i.e., those that are most abundant. Of further interest for the future of proteomics is the fact that we have achieved a direct electroelution of a native protein from a nondetergent gel. This finding foreshadows the possibility of identifying those post-translationally modified proteins that on SDS-PAGE migrate together.

Figure 10

Figure 10

Apparatus for a direct orthogonal electroelution of gel electrophoretic protein bands.

Sequential electroelution of protein bands on the two-dimensional gels remains to be solved. A possible solution may be to polymerize on a net, which is permeable to the orthogonally directed current of electroelution. A suitable net support has been designed and constructed. We intend to position the gel by moving the net support under micromanipulator control, thereby preventing gel stretching as we move sequentially from spot to spot. Once a suitable frame for the net-supported gel is constructed, the positioning of the net will have to be interfaced with the image analysis system to arrive at a computer-controlled automated protein elution method without any gel sectioning.
 

PUBLICATIONS

  1. Buzas Z, Chang HT, Vieira NE, Yergey AL, Stastna M, Chrambach A. Direct vertical electroelution of protein from a PhastSystem band for mass spectrometric identification at the level of a few picomoles. Proteomics 2001;1:691-698.
  2. Buzas Z, Li T, Chrambach A. Horizontal gel electrophoresis of SDS-proteins on the PhastSystem with an at least 25-fold increased protein load volume. Anal Biochem 2001;292:161-163.
  3. Chang HT, Yergey AL, Chrambach A. Electroelution of proteins from bands in gel electrophoresis without gel sectioning for the purpose of protein transfer into mass spectrometry: elements of a new procedure. Electrophoresis 2001;22:394-398.
  4. Chiari M, Cretich M, Stastna M, Radko SP, Chrambach A. Rapid capillary coating by epoxy-poly-(dimethylacrylamide): performance in capillary zone electrophoresis of protein and polystyrene carboxylate. Electrophoresis 2001;22:656-659.
  5. Chrambach A, Chrambach A, Brining SK. Gel electrophoretic distinction between Congo Red nonreactive beta-amyloid (1-42) and beta-amyloid (1-40). Electrophoresis 2000;21:760-761.
  6. Chrambach A, Radko SP. Size-dependent retardation and resolution by electrophoresis of rigid, submicron-sized particles, using buffered solutions in presence of polymers: a review of recent work from the authors' laboratory. Electrophoresis. 2000;21:259-265.
  7. Gianazza E, Sirtori CR, Castiglioni S, Eberini I, Chrambach A, Rondanini A, Vecchio G. Interactions between carbonic anhydrase and its inhibitors revealed by gel electrophoresis and circular dichroism. Electrophoresis 2000;21:1435-1445.
  8. Gombocz E, Chrambach A, Yefimov S, Yergey AL. Electroelution of nonfluorescent stacked proteins detected by fluorescence optics from gel electrophoretic bands for transfer into mass spectrometry. Electrophoresis 2000;21:846-849.
  9. Li Y-M, Chrambach A. Gel electrophoretic isolation in the hundred microgram range of recombinant SDS-syntaxin from sea urchin egg cortical vesicles. Prep Biochem Biotechnol 2001;31:369-387.
  10. Radko SP, Stastna M, Chrambach A. Capillary zone electrophoresis of sub-micron-sized particles in electrolyte solutions of various ionic strengths: size-dependent electrophoretic migration and separation efficiency. Electrophoresis 2000;21:3583-3592.
  11. Radko SP, Stastna M, Chrambach A. Relation of peakwidth to polydispersity of liposome preparations subjected to capillary zone electrophoresis. J Chromatogr B Biomed Sci Appl 2001;761:69-75.
  12. Radko SP, Stastna M, Chrambach A. Size-dependent electrophoretic migration and separation of liposomes by capillary zone electrophoresis in electrolyte solutions of various ionic strengths. Anal Chem 2000;72:5955-5960.
  13. Stastna M, Radko SP, Chrambach A. Discrimination between peak spreading in capillary zone electrophoresis of proteins due to interaction with the capillary wall and due to protein microheterogeneity. Electrophoresis 2001;22:66-70.
  14. Stastna M, Radko SP, Chrambach A. Separation efficiency in protein zone electrophoresis performed in capillaries of different diameters. Electrophoresis 2000;21:985-992.
  15. Yefimov S, Sjomeling C, Yergey AL, Chrambach A. Stacking of unlabeled sodium dodecyl sulfate-proteins within a fluorimetrically detected moving boundary, electroelution and mass spectrometric identification. Electrophoresis 2001;22:999-1003.
  16. Yefimov S, Sjomeling C, Yergey AL, Li T, Chrambach A. Recovery of sodium dodecyl sulfate-proteins from gel electrophoretic bands in a single electroelution step for mass spectrometric analysis. Anal Biochem 2000;284:288-295.
  17. Yefimov S, Yergey AL, Chrambach A. Sequential electroelution and mass spectroscopic identification of intact sodium dodecyl sulfate-proteins labeled with 5(6)-carboxyfluorescein-N-hydroxysuccinimide ester. Electrophoresis 2001;22:2881-2887.
  18. Yefimov S, Yergey AL, Chrambach A. Transfer of SDS-proteins from gel electrophoretic zones into mass spectrometry, using electroelution of the band into buffer without sectioning of the gel. J Biochem Biophys Methods 2000;42:65-78.