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突触质膜外表面的ATP结合蛋白:通过光亲和标记进行鉴定

ATP-binding proteins on the external surface of synaptic plasma membranes: identification by photoaffinity labeling.

作者信息

Nagy A K, Shuster T A

机构信息

Department of Neurology, UCLA School of Medicine, USA.

出版信息

J Neurochem. 1995 Oct;65(4):1849-58. doi: 10.1046/j.1471-4159.1995.65041849.x.

DOI:10.1046/j.1471-4159.1995.65041849.x
PMID:7561884
Abstract

8-Azidoadenosine triphosphate labeled in the alpha or gamma position with 32P was used as a photoaffinity reagent for identifying ATP binding sites on the external surface of intact rat brain synaptosomes. As revealed by autoradiography of sodium dodecyl sulfate-polyacrylamide gel electrophoretic patterns. UV irradiation of intact synaptosomes in the presence of the above radioactive compounds at 5-10 microM resulted in the formation of several major radioactive conjugates with approximate molecular masses of 29, 45/46, 58, and 93 kDa. Minor bands of 20, 39, 52/54, 82/84, 120, and 140 kDa were also consistently labeled in these experiments. The possibility that labeling of these proteins was due to the presence of contaminating subcellular particles or intrasynaptosomal proteins was excluded. The major 8-azidoadenosine [alpha-32P]triphosphate-labeled protein complex of approximately 45/46 kDa was resolved into several subbands that are labeled differently depending on the type of divalent cations added to the photoaffinity reaction. In the presence of magnesium only, the major labeled band appeared at 45 kDa. With calcium, two additional subbands (43 and 46 kDa) could be distinguished. In the presence of 1 mM EDTA, a band at 44 kDa was labeled within this ATP-binding complex. The labeling pattern of the subbands of this 45/46-kDa complex is consistent with these bands being extracellular ATP-binding proteins on the surface of the synaptosome.

摘要

用α或γ位标记有32P的8-叠氮三磷酸腺苷作为光亲和试剂,用于鉴定完整大鼠脑突触体外表的ATP结合位点。通过十二烷基硫酸钠-聚丙烯酰胺凝胶电泳图谱的放射自显影显示。在5-10 microM的上述放射性化合物存在下,对完整突触体进行紫外线照射,导致形成几种主要的放射性缀合物,其近似分子量为29、45/46、58和93 kDa。在这些实验中,20、39、52/54、82/84、120和140 kDa的次要条带也一直被标记。这些蛋白质的标记是由于污染的亚细胞颗粒或突触体内蛋白质的存在这种可能性被排除。大约45/46 kDa的主要8-叠氮腺苷[α-32P]三磷酸标记的蛋白质复合物被解析为几个亚条带,根据添加到光亲和反应中的二价阳离子类型,这些亚条带的标记方式不同。仅在镁存在下,主要标记条带出现在45 kDa处。有钙时,可以区分另外两个亚条带(43和46 kDa)。在1 mM EDTA存在下,该ATP结合复合物中出现一条44 kDa的条带被标记。这个45/46-kDa复合物亚条带的标记模式与这些条带是突触体表面的细胞外ATP结合蛋白一致。

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