Blue silver: A very sensitive colloidal Coomassie G‐250 staining for proteome analysis

化学 银染 色谱法 染色 考马斯亮蓝 磷酸 质谱法 十二烷基硫酸钠 污渍 等电聚焦 检出限 凝胶电泳 核化学 生物化学 有机化学 医学 分子生物学 病理 生物
作者
Giovanni Candiano,Maurizio Bruschi,Luca Musante,Laura Santucci,Gian Marco Ghiggeri,Barbara Carnemolla,Paola Orecchia,Luciano Zardi,Pier Giorgio Righetti
出处
期刊:Electrophoresis [Wiley]
卷期号:25 (9): 1327-1333 被引量:1918
标识
DOI:10.1002/elps.200305844
摘要

Abstract A modified Neuhoff's colloidal Coomassie Blue G‐250 stain is reported, dubbed “blue silver” on account of its considerably higher sensitivity, approaching the one of conventional silver staining. The main modifications, as compared to Neuhoff's protocol, were: a 20% increment in dye concentration (from 0.1% up to 0.12%) and a much higher level of phosphoric acid in the recipe (from 2% up to 10%). The “blue silver” exhibits a much faster dye uptake (80% during the first hour of coloration, vs. none with a commercial preparation from Sigma). Even at equilibrium (24 h staining), the “blue silver” exhibits a much higher sensitivity than all other recipes, approaching (but lower than) the one of the classical silver stain. Measurements of stain sensitivity after sodium dodecyl sulfate‐polyacrylamide gel electrophoresis (SDS‐PAGE) of bovine serum albumin (BSA) gave a detection limit (signal‐to‐noise ratio > 3) of 1 ng in a single zone. The somewhat lower sensitivity of “blue silver” as compared to classical silvering protocols in the presence of aldehydes is amply compensated for by its full compatibility with mass spectrometry of eluted polypeptide chains, after a two‐dimensional map analysis, thus confirming that no dye is covalently bound (or permanently modifies) to any residue in the proteinaceous material. It is believed that the higher level of phosphoric acid in the recipe, thus its lower final pH, helps in protonating the last dissociated residues of Asp and Glu in the polypeptide coils, thus greatly favoring ionic anchoring of dye molecules to the protein moiety. Such a binding, though, must be followed by considerable hydrophobic association with the aromatic and hydrophobic residues along the polypeptide backbone.
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