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牛视紫红质转导蛋白(一种来自光感受器细胞的可溶性磷蛋白)的氨基酸序列和互补DNA序列。

Amino acid and cDNA sequence of bovine phosducin, a soluble phosphoprotein from photoreceptor cells.

作者信息

Lee R H, Fowler A, McGinnis J F, Lolley R N, Craft C M

机构信息

Department of Anatomy and Cell Biology, UCLA School of Medicine 90024.

出版信息

J Biol Chem. 1990 Sep 15;265(26):15867-73.

PMID:2203790
Abstract

Vertebrate photoreceptor cells contain a soluble phosphoprotein, phosducin, which complexes with the beta, gamma subunits of the GTP-binding protein, transducin. Light-induced changes in cyclic nucleotide levels modulate the phosphorylation of phosducin by protein kinase A. The complete amino acid sequence of purified phosducin from bovine retinas was determined by Edman degradation from overlapping polypeptides derived from enzymatic digestion by trypsin and Staphylococcus aureus V8 protease or from chemical degradation by cyanogen bromide. Excluding the unidentified group which blocks the NH2 terminus, phosducin contains 245 amino acids with a calculated molecular weight of 28,185 and isoelectric point of pH 4.5. Phosducin is enriched with acidic and sulfur-containing amino acids, having 32 glutamic acid, 16 aspartic acid, 9 methionine, and 5 cysteine residues. It also contains 24 serine and 8 threonine residues, of which only serine 73 is located within a consensus phosphorylation sequence (-RKMS(P)QV-) for cyclic nucleotide-dependent protein kinase. Secondary structure analysis predicts the presence of 62% alpha-helix, 22% beta-sheet, and 16% random coil, with eight turns. Computer-aided searches of protein data banks revealed no apparent homology to any sequenced protein except that coded by a MEKA cDNA clone (Kuo, C-H., Akiyama, M., and Miki, N. (1989) Mol. Brain Res. 6, 1-10) which deviates from the confirmed phosducin sequence in the last 15 amino acids. Sequence analysis of a cDNA clone for bovine retinal phosducin confirmed that the MEKA clone deviation resulted from an unidentified cDNA guanosine nucleotide, a shifted reading frame and a premature stop codon.

摘要

脊椎动物的光感受器细胞含有一种可溶性磷蛋白——视紫红质转导蛋白,它与GTP结合蛋白转导素的β、γ亚基结合。环核苷酸水平的光诱导变化通过蛋白激酶A调节视紫红质转导蛋白的磷酸化。通过对胰蛋白酶和金黄色葡萄球菌V8蛋白酶酶解产生的重叠多肽或溴化氰化学降解产生的多肽进行埃德曼降解,确定了从牛视网膜中纯化的视紫红质转导蛋白的完整氨基酸序列。除了阻断NH2末端的未鉴定基团外,视紫红质转导蛋白含有245个氨基酸,计算分子量为28,185,等电点为pH 4.5。视紫红质转导蛋白富含酸性和含硫氨基酸,有32个谷氨酸、16个天冬氨酸、9个甲硫氨酸和5个半胱氨酸残基。它还含有24个丝氨酸和8个苏氨酸残基,其中只有丝氨酸73位于环核苷酸依赖性蛋白激酶的共有磷酸化序列(-RKMS(P)QV-)内。二级结构分析预测存在62%的α-螺旋、22%的β-折叠和16%的无规卷曲,有八圈。对蛋白质数据库的计算机辅助搜索显示,除了由MEKA cDNA克隆编码的蛋白质外,与任何已测序蛋白质都没有明显的同源性(郭,C-H.,秋山,M.,和三木,N.(1989年)《分子脑研究》6,1-10),该克隆在最后15个氨基酸上与已确认的视紫红质转导蛋白序列不同。牛视网膜视紫红质转导蛋白cDNA克隆的序列分析证实,MEKA克隆的差异是由一个未鉴定的cDNA鸟苷酸、阅读框移位和一个提前终止密码子导致的。

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