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一种新型的G蛋白β亚基Gbeta5特异性地在脊椎动物视网膜中表达。

A novel form of the G protein beta subunit Gbeta5 is specifically expressed in the vertebrate retina.

作者信息

Watson A J, Aragay A M, Slepak V Z, Simon M I

机构信息

Division of Biology, 147-75, California Institute of Technology, Pasadena, California 91125, USA.

出版信息

J Biol Chem. 1996 Nov 8;271(45):28154-60. doi: 10.1074/jbc.271.45.28154.

Abstract

The G protein beta subunit, Gbeta5, is predominantly expressed in the central nervous system. In rodent brain, Gbeta5 is expressed as a protein with an apparent molecular mass of 39,000 daltons (39 kDa). We have identified an additional Gbeta5 immunoreactive protein of apparent size 44 kDa in the vertebrate retina. Molecular cloning and sequencing of polymerase chain reaction products revealed that the cDNA encoding the larger species of Gbeta5 (Gbeta5L) was identical to the shorter form with the addition of 126 base pairs of 5' DNA sequence potentially encoding an in-frame 42-amino acid extension. Sequencing of mouse Gbeta5 genomic clones demonstrated that the 126-base pair of retinal-specific coding material is derived from a hitherto undetected 5' exon. During sucrose density gradient fractionation of bovine retinas, the 44-kDa Gbeta5L protein co-purified with rod outer segment membranes. Incubation of rod outer segment membranes with the nonhydrolyzable guanine nucleotide, GTPgammaS (guanosine 5'-3-O-(thio)triphosphate), which released the Gbeta subunit of transducin (Gbeta1), failed to remove Gbeta5L. The 39-kDa Gbeta5 protein displayed differential association with retinal and brain membranes. In the retina, Gbeta5 was present as a soluble protein and was undetectable in the membrane fraction, whereas in the brain approximately 70% of Gbeta5 was associated with cellular membranes. In transient COS-7 cell expression experiments, Gbeta5L formed functional Gbetagamma dimers and Galphabetagamma heterotrimers, and activated phosphoinositide-specific phospholipase Cbeta2 in a manner indistinguishable from the 39-kDa Gbeta5 protein. The cloning of the retinal-specific Gbeta5L cDNA suggests the existence of potentially novel G protein-mediated signaling cascades in photoreception.

摘要

G蛋白β亚基Gβ5主要在中枢神经系统中表达。在啮齿动物大脑中,Gβ5以一种表观分子量为39,000道尔顿(39 kDa)的蛋白质形式表达。我们在脊椎动物视网膜中鉴定出了另一种表观大小为44 kDa的Gβ5免疫反应性蛋白。聚合酶链反应产物的分子克隆和测序显示,编码较大形式Gβ5(Gβ5L)的cDNA与较短形式相同,但增加了126个碱基对的5' DNA序列,该序列可能编码一个框内的42个氨基酸延伸。小鼠Gβ5基因组克隆的测序表明,视网膜特异性编码材料的126个碱基对来自一个迄今未检测到的5' 外显子。在牛视网膜的蔗糖密度梯度分级分离过程中,44 kDa的Gβ5L蛋白与视杆细胞外段膜共纯化。用不可水解的鸟嘌呤核苷酸GTPγS(鸟苷5'-3-O-(硫代)三磷酸)孵育视杆细胞外段膜,该核苷酸可释放转导素的Gβ亚基(Gβ1),但未能去除Gβ5L。39 kDa的Gβ5蛋白与视网膜和脑膜的结合存在差异。在视网膜中,Gβ5以可溶性蛋白形式存在,在膜部分中未检测到,而在大脑中,约70%的Gβ5与细胞膜相关。在瞬时COS-7细胞表达实验中,Gβ5L形成功能性的Gβγ二聚体和Gαβγ三聚体,并以与39 kDa的Gβ5蛋白无法区分的方式激活磷脂酰肌醇特异性磷脂酶Cβ2。视网膜特异性Gβ5L cDNA的克隆表明在光感受器中可能存在新的G蛋白介导的信号级联反应。

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