Schwarz Katrin, Fiedler Tomas, Fischer Ralf-Jörg, Bahl Hubert
University of Rostock, Institute of Biological Sciences, Division of Microbiology, Rostock, Germany.
J Microbiol Methods. 2007 Feb;68(2):396-402. doi: 10.1016/j.mimet.2006.09.018. Epub 2006 Nov 13.
We report on the development of a Standard Operating Procedure (SOP) for extraction and handling of intra- and extracellular protein fractions of Clostridium acetobutylicum ATCC 824 for reproducible high quality two-dimensional gel electrophoresis (2-DE) analyses. Standardized cells from a phosphate-limited chemostat were used to evaluate different protein preparation methods. For the preparation of the secretome, a dialysis/ultrafiltration procedure resulted in higher protein yields and proved to be more reliable compared to different precipitation methods using TCA, DOC-TCA, acetone, and PEG 6000. Sonication was found to be the most efficient method among different tested techniques of cell disruption for the analysis of the intracellular proteome. Furthermore, the effect of protease inhibitors and sample storage conditions were tested for both intra- and extracellular protein samples. Significant changes in the protein pattern were observed depending on the addition of protease inhibitors. 2-DE gels with a pH gradient from 4 to 7 prepared according to the developed SOP contained at least 736 intracellular and 324 extracellular protein spots.
我们报告了一种标准操作程序(SOP)的开发,该程序用于提取和处理丙酮丁醇梭菌ATCC 824的细胞内和细胞外蛋白质组分,以进行可重复的高质量二维凝胶电泳(2-DE)分析。来自磷酸盐限制恒化器的标准化细胞用于评估不同的蛋白质制备方法。对于分泌蛋白质组的制备,与使用三氯乙酸(TCA)、十二烷基氧膦-三氯乙酸(DOC-TCA)、丙酮和聚乙二醇6000(PEG 6000)的不同沉淀方法相比,透析/超滤程序产生了更高的蛋白质产量,并且被证明更可靠。在用于细胞内蛋白质组分析的不同测试细胞破碎技术中,超声处理被发现是最有效的方法。此外,还针对细胞内和细胞外蛋白质样品测试了蛋白酶抑制剂和样品储存条件的影响。根据添加蛋白酶抑制剂的情况,观察到蛋白质图谱有显著变化。根据所开发的SOP制备的pH梯度为4至7的2-DE凝胶包含至少736个细胞内蛋白质斑点和324个细胞外蛋白质斑点。
