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Topography of a vacuolar-type H+-translocating ATPase: chromaffin-granule membrane ATPase I

机译:液泡型H +易位ATPase的形貌:嗜铬粒细胞膜ATPase I

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pProteins exposed on the cytoplasmic face of isolated chromaffin granules were labelled by lactoperoxidase-catalysed radioiodination and by non-enzymic biotinylation. Granule membranes were then prepared, and the H+-translocating ATPase isolated by fractionation with Triton X-114. The labelling of individual ATPase subunits was assessed by polyacrylamide-gel electrophoresis, followed by autoradiography or by blotting and decoration with 125I-labelled streptavidin. Subunits of 72, 57 and kDa were strongly labelled, and could be removed from the membrane at pH 11: they are therefore extrinsic proteins. The 120 kDa subunit was also labelled, but it was not solubilized at pH 11. Photolabelling with a hydrophobic probe indicated that this subunit penetrates the bilayer, and enzymic degradation studies showed the presence of N-linked oligosaccharides; this subunit therefore spans the chromaffin-granule membrane. Labelling of the 17 kDa subunit occurred predominantly on the extracytoplasmic (matrix) face of the granule membrane. These results are consistent with this V-type ATPase having a structure that is generally similar to that of mitochondrial (F-type) ATPases, although the attachment of the 120 kDa subunit may be asymmetrical./p
机译:通过乳过氧化物酶催化的放射性碘标记和非酶生物素化标记标记分离的嗜铬粒细胞颗粒细胞质表面上暴露的蛋白质。然后制备颗粒膜,并通过Triton X-114分级分离H +-易位ATP酶。通过聚丙烯酰胺凝胶电泳,放射自显影或印迹和125 I标记的链霉亲和素修饰来评估单个ATPase亚基的标记。 72、57和kDa的亚基被强烈标记,可以在pH 11时从膜上除去:因此它们是外在蛋白。 120 kDa亚基也被标记,但在pH 11时不溶解。用疏水探针进行光标记表明该亚基渗透了双层,酶促降解研究表明存在N-连接的寡糖。因此,该亚单位跨越了嗜铬粒细胞颗粒膜。 17 kDa亚基的标记主要发生在颗粒膜的胞质(基质)面上。这些结果与该V型ATP酶的结构基本一致,尽管其120 kDa亚基的附着可能是不对称的,但该结构通常类似于线粒体(F型)ATP酶。

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