Literature DB >> 9820957

Understanding the mechanism of the zinc-ion stains of biomacromolecules in electrophoresis gels: generalization of the reverse-staining technique.

C Fernandez-Patron1, L Castellanos-Serra, E Hardy, M Guerra, E Estevez, E Mehl, R W Frank.   

Abstract

We have recently shown that a few nanograms of protein separated by electrophoresis in sodium dodecyl sulfate-polyacrylamide gels can be detected by reverse-staining, exploiting the precipitation reaction between zinc(II) and imidazole. Modifications of this method have also been generated to detect gel-isolated nucleic acids and bacterial glycolipids. Because there is no recourse to chemical modifiers, the reverse-staining technique has been valuable when micropreparing these biomacromolecules for later use or characterization. The mechanism underlying the reverse-staining effect, however, remains incompletely understood and this has prevented a further generalization of the technique. Here, we have conducted physicochemical experiments and identified zinc imidazolate (ZnIm2) as the main component of the precipitate that forms along the surface of zinc-imidazole reverse-stained gels. Many staining effects observed when gels containing electrophoretically separated biopolymers are subjected to zinc-imidazole stains have been rationalized. The reverse-staining method has been vastly generalized, now allowing the detection of proteins and glycolipids as well as complexes of these macromolecules in native gels. We demonstrate the application of the reverse-staining technique in situations where Coomassie blue or silver staining was inappropriate or failed to produce detection of the species of interest. The present generalization of the reverse-staining method facilitated the characterization of biomacromolecular interaction partners in mixtures of bacterial glycolipids and human tears.

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Year:  1998        PMID: 9820957     DOI: 10.1002/elps.1150191407

Source DB:  PubMed          Journal:  Electrophoresis        ISSN: 0173-0835            Impact factor:   3.535


  5 in total

Review 1.  Proteomics for protein expression profiling in neuroscience.

Authors:  Willard M Freeman; Scott E Hemby
Journal:  Neurochem Res       Date:  2004-06       Impact factor: 3.996

2.  Quantitative proteomics: assessing the spectrum of in-gel protein detection methods.

Authors:  Victoria J Gauci; Elise P Wright; Jens R Coorssen
Journal:  J Chem Biol       Date:  2010-06-19

3.  Differences between the Molecular Mechanisms Underlying Ruptured and Non-Ruptured Carotid Plaques, and the Significance of ABCA1.

Authors:  Sung Hyuk Heo; Eun-Hye Lee; Hyun-Hee Park; Bum Joon Kim; Hyo Chul Youn; Young Seo Kim; Hyun Young Kim; Seong-Ho Koh; Dae-Il Chang
Journal:  J Stroke       Date:  2018-01-31       Impact factor: 6.967

4.  Identification of fibrinogen as a natural inhibitor of MMP-2.

Authors:  Hassan Sarker; Eugenio Hardy; Ayman Haimour; Walter P Maksymowych; Lorenzo D Botto; Carlos Fernandez-Patron
Journal:  Sci Rep       Date:  2019-03-13       Impact factor: 4.379

5.  Improved coomassie blue dye-based fast staining protocol for proteins separated by SDS-PAGE.

Authors:  Pavel Májek; Zuzana Riedelová-Reicheltová; Klára Pecánková; Jan E Dyr
Journal:  PLoS One       Date:  2013-11-21       Impact factor: 3.240

  5 in total

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