The Open Proteomics Journal




(Discontinued)

ISSN: 1875-0397 ― Volume 7, 2014

Widespread Occurrence of Non-Enzymatic Deamidations of Asparagine Residues in Yersinia pestis Proteins Resulting from Alkaline pH Membrane Extraction Conditions


The Open Proteomics Journal , 2008, 1: 106-115

Moo-Jin Suh, Hamid Alami, David J. Clark, Prashanth P. Parmar, Jeffrey M. Robinson, Shih-Ting Huang, Robert D. Fleischmann, Scott N. Peterson , Rembert Pieper

J. Craig Venter Institute, 9704 Medical Center Drive, Rockville, MD 20850, USA.

Electronic publication date 5/11/2008
[DOI: 10.2174/1875039700801010106]




Abstract:

Extraction of crude membrane fractions with alkaline solutions, such as 100-200 mM Na2CO3 (pH ~11), is often used to solubilize peripheral membrane proteins. Integral membrane proteins are largely retained in membrane pellets. We applied this method to the fractionation of membrane proteins of the plague bacterium Yersinia pestis. Extensive horizontal spot trains were observed in 2-DE gels. The pI values of the most basic spots part of such protein spot trains usually matched the computationally predicted pI values. Regular patterns of decreasing spot pI values and in silico analysis with the software ProMoST suggested ‘n-1’ deamidations of asparagine (N) and/or glutamine (Q) side chains for ‘n’ observed spots of a protein in a given spot train. MALDI-MS analysis confirmed the occurrence of deamidations, particularly in N side chains part of NG dipeptide motifs. In more than ten cases, tandem MS data for tryptic peptides provided strong evidence for deamidations, with y- and b-ion series increased by 1 Da following N-to-D substitutions. Horizontal spot trains in 2-DE gels were rare when alkaline extraction was omitted during membrane protein sample preparation. This study strongly supports the notion that exposure to alkaline pH solutions is a dominant cause of extensive N and Q side chain deamidations in proteins during sample preparation of membrane extracts. The modifications are of non-enzymatic nature and not physiologically relevant. Therefore, quantitative spot differences within spot trains in differential protein display experiments following the aforementioned sample preparation steps need to be interpreted cautiously.


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