【摘要】 用膜蛋白分离试剂盒提取巨噬细胞膜蛋白,然后用SDS-聚丙烯酰氨凝胶电泳进行分离。将每个泳道平均切成8份,合并两个泳道同样位置的胶条,分别进行胶内酶解。酶解得到的多肽经脱盐后进入毛细管反相柱进行反相分离,分离后的肽段直接进入电喷离子源质谱仪进行一级和二级质谱分析。质谱数据用SEQUEST软件对小鼠IPI蛋白数据库进行检索,得到一个含有1000多种蛋白的名单,其中包括458种经GOA注释的膜蛋白。对膜蛋白部分进一步分析发现,其中包括CD11b、TNF-a、F4/80、CD14、CD18、CD86、CD44、CD16、Toll样受体等已知表达在巨噬细胞表面的蛋白分子,还包括另外13种CD分子和18种Ras相关GTPase,除了这些已知蛋白之外,还鉴定出若干新蛋白分子,为进一步深入研究巨噬细胞生物学功能提供了目标分子。更多还原

【Abstract】 Macrophages are involved in many important biological processes and membrane proteins are the key effector molecules for their functions. However, membrane proteins are difficult to analyze by 2-DE based method because of their intrinsic tendency to self-aggregate during the first dimension separation (IEF). To circumvent the obstacle hampering membrane protein analysis, we combined one-dimensional SDS-PAGE with capillary liquid chromatography-tandem mass spectrometry (LC-MS/MS). Using this technique, we identified 458 GO annotated membrane proteins with extremely high confidence, including most known markers of peritoneal macrophages (e.g., CD11b, F4/80, CD14, CD18, CD86, CD44, CD16 and Toll-like receptor). Thirteen other CD antigens and 18 Ras-related small GTPase were also identified. In addition to those known macrophage membrane proteins, a significant number of novel proteins have also been identified. This research provides a valuable data set of macrophage membrane proteins, thus allowing for more comprehensive study of membrane proteins and a better understanding of the function mechanisms of macrophages in many biological processes.更多还原