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26S蛋白酶体的两个新型调节亚基p28(Nas6p)和p40.5(Nas7p)的cDNA克隆及功能分析

cDNA cloning and functional analysis of p28 (Nas6p) and p40.5 (Nas7p), two novel regulatory subunits of the 26S proteasome.

作者信息

Hori T, Kato S, Saeki M, DeMartino G N, Slaughter C A, Takeuchi J, Toh-e A, Tanaka K

机构信息

The Tokyo Metropolitan Institute of Medical Science, and CREST, Japan Science and Technology Corporation (JST), 3-18-22 Honkomagome, Bunkyo-ku, Tokyo 113-8613, Japan.

出版信息

Gene. 1998 Aug 17;216(1):113-22. doi: 10.1016/s0378-1119(98)00309-6.

Abstract

We employed cDNA cloning to deduce the complete primary structures of p28 and p40.5, two novel subunits of PA700 (also called 19S complex), a 700 kDa multisubunit regulatory complex of the human 26S proteasome. These polypeptides consisted of 226 and 376 amino acids with calculated molecular masses of 24428 Da and 42945 Da, and isoelectric points of 5. 68 and 5.46, respectively. Intriguingly, p28 contained five conserved motifs known as 'ankyrin repeats', implying that this subunit may contribute to interaction of the 26S proteasome with other protein(s). Computer-assisted homology analysis revealed high sequence similarities of p28 and p40.5 with yeast proteins, termed Nas6p and Nas7p (non-ATPase subunits 6 and 7), respectively, whose functions are as yet unknown. Disruption of these yeast genes, NAS6 and NAS7, had no effect on cell viability, indicating that neither of the two subunits is essential for proliferation of yeast cells. However, the NAS7, but not NAS6, disruptant cells caused high sensitivity to heat stress, being unable to proliferate at 37 degreesC.

摘要

我们采用cDNA克隆技术来推导p28和p40.5的完整一级结构,这两个蛋白是PA700(也称为19S复合物)的新型亚基,PA700是人类26S蛋白酶体的一种700 kDa多亚基调节复合物。这些多肽分别由226和376个氨基酸组成,计算分子量分别为24428 Da和42945 Da,等电点分别为5.68和5.46。有趣的是,p28包含五个被称为“锚蛋白重复序列”的保守基序,这意味着该亚基可能有助于26S蛋白酶体与其他蛋白质的相互作用。计算机辅助同源性分析显示,p28和p40.5与酵母蛋白分别具有高度的序列相似性,这两种酵母蛋白分别称为Nas6p和Nas7p(非ATP酶亚基6和7),其功能尚不清楚。破坏这些酵母基因NAS6和NAS7对细胞活力没有影响,这表明这两个亚基都不是酵母细胞增殖所必需的。然而,NAS7基因敲除细胞(而非NAS6基因敲除细胞)对热应激高度敏感,在37℃下无法增殖。

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