Dadi H K, Morris R J
Eur J Biochem. 1984 Nov 2;144(3):617-28. doi: 10.1111/j.1432-1033.1984.tb08510.x.
The muscarinic cholinergic receptor present in synaptosomal membranes of rat brain was covalently labelled with the alkylating muscarinic antagonist, tritiated propylbenzilylcholine mustard. The labelled receptor was then solubilized in sodium deoxycholate and sodium dodecyl sulphate, and its migration in polyacrylamide gel electrophoresis and gel filtration in the presence of sodium dodecyl sulphate analysed. Provided both proteolysis and inter-chain disulphide bond formation were vigorously prevented, the receptor from rat forebrain (cerebral cortex plus caudate putamen) migrated, in sodium dodecyl sulphate/polyacrylamide gel electrophoresis, as a broad band of apparent Mr 66000-76000. Two dominantly labelled polypeptides, of apparent Mr 68000 and 73000, could be distinguished as the major components of this band. These multiple species seen in electrophoresis may reflect a structural diversity related to the different binding properties, and modes of action, of this receptor. In electrophoresis using discontinuous buffer systems the labelled receptor readily formed intermolecular disulphide bonds and so aggregated. In particular, if solubilized membranes were reduced with 2-mercaptoethanol, and reformation of disulphide bonds during electrophoresis not prevented, then formation of a dimeric species (apparent Mr 119000-128000) occurred. This probably explains previous reports in the literature of larger-Mr species seen in electrophoresis. During gel filtration, the receptor formed intra-chain disulphide bonds which produced conformational heterogeneity, leading to polydisperse migration. In addition, extensive proteolytic degradation of the receptor occurred due to a protease migrating slightly ahead of the receptor. Both effects were eliminated by alkylation of the solubilized membranes with iodoacetamide before gel filtration. Alkylated receptor migrated on Sephacryl S-300 in 0.5% sodium dodecyl sulphate with an equivalent Stokes' radius of 6.1 nm. This is identical to that of reduced ovalbumin, a molecule with an apparent Mr in gel electrophoresis of 43000. On a different gel matrix, TSK HW 55(S), the receptor migrated with a somewhat larger Stokes' radius, eluting just behind reduced bovine serum albumin (Stokes' radius 8.5 nm; apparent Mr in electrophoresis 67000). Thus the receptor appears to adsorb to the Sephacryl matrix, although even on the TSK gel the receptor eluted as a somewhat smaller protein than expected from its behaviour in gel electrophoresis. Solubilized, alkylated receptor, partly purified by gel filtration so that it was not degraded by endogenous proteases, was not cleaved by mild hydroxylamine treatment.(ABSTRACT TRUNCATED AT 400 WORDS)
大鼠脑突触体膜中的毒蕈碱型胆碱能受体用放射性标记的烷基化毒蕈碱拮抗剂——氚标记的丙基苯甲酰胆碱氮芥进行共价标记。然后将标记的受体溶解于脱氧胆酸钠和十二烷基硫酸钠中,并分析其在十二烷基硫酸钠存在下的聚丙烯酰胺凝胶电泳迁移情况以及凝胶过滤情况。只要能有力地防止蛋白水解和链间二硫键形成,大鼠前脑(大脑皮层加尾状核壳核)的受体在十二烷基硫酸钠/聚丙烯酰胺凝胶电泳中会迁移成一条表观分子量为66000 - 76000的宽带。在这条带中可分辨出两条主要标记多肽,表观分子量分别为68000和73000,它们是这条带的主要成分。电泳中出现的这些多种形式可能反映了与该受体不同结合特性及作用方式相关的结构多样性。在使用不连续缓冲系统的电泳中,标记的受体很容易形成分子间二硫键并聚集。特别是,如果用2 - 巯基乙醇还原溶解的膜,且不阻止电泳过程中二硫键的重新形成,就会形成二聚体形式(表观分子量为119000 - 128000)。这可能解释了文献中先前报道的电泳中出现的较大分子量形式。在凝胶过滤过程中,受体形成链内二硫键,导致构象异质性,从而产生多分散迁移。此外,由于一种蛋白酶迁移速度略快于受体,受体发生了广泛的蛋白水解降解。在凝胶过滤前用碘乙酰胺对溶解的膜进行烷基化处理,可消除这两种影响。烷基化受体在含0.5%十二烷基硫酸钠的Sephacryl S - 300上迁移,其斯托克斯半径相当于6.1 nm。这与还原的卵清蛋白相同,卵清蛋白在凝胶电泳中的表观分子量为43000。在另一种凝胶基质TSK HW 55(S)上,受体迁移时的斯托克斯半径稍大,在还原的牛血清白蛋白(斯托克斯半径8.5 nm;电泳中的表观分子量67000)之后洗脱。因此,受体似乎吸附在Sephacryl基质上,尽管即使在TSK凝胶上,受体洗脱时的蛋白分子量也比根据其在凝胶电泳中的行为预期的要小一些。通过凝胶过滤部分纯化的溶解、烷基化受体,使其不被内源性蛋白酶降解,经温和的羟胺处理后未被切割。(摘要截短至400字)
