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小鼠泛素结合酶mUBC9与E2A转录因子相互作用。

The mUBC9 murine ubiquitin conjugating enzyme interacts with the E2A transcription factors.

作者信息

Loveys D A, Streiff M B, Schaefer T S, Kato G J

机构信息

Division of Pediatric Hematology, The Johns Hopkins University School of Medicine, Baltimore, MD 21205, USA.

出版信息

Gene. 1997 Nov 12;201(1-2):169-77. doi: 10.1016/s0378-1119(97)00444-7.

Abstract

The ubiquitin-mediated degradation of cellular proteins requires the sequential activity of E1, E2 and, in some cases, E3 enzymes. Using the yeast two-hybrid system, we have cloned 1.0- and 2.5-kb cDNAs encoding the identical murine E2, or ubiquitin conjugating enzyme by virtue of its interaction with the E2A transcription factor. This cDNA encodes the 158-amino-acid protein, mUBC9, which has considerable sequence homology to UBC9 from Saccharomyces cerevisiae and HUS5 from Schizosaccharomyces pombe and is identical to the human UBC9 protein. HUS5 is essential for DNA damage repair, whereas UBC9 is necessary for G2/M progression. The human protein has been shown to correct the UBC9 defect in yeast. Antisera raised against bacterially expressed mUBC9 fusion protein recognize a murine cellular protein of approximately 18 kDa, corresponding to the predicted mobility. Unlike E2A, the mUBC9 protein level is not regulated by serum growth factors. The activity of the apparent homologues UBC9 and HUS5 suggests that mUBC9 may be involved in the degradation of key nuclear proteins that regulate cell cycle progression.

摘要

细胞蛋白质的泛素介导降解需要E1、E2以及某些情况下E3酶的顺序活性。利用酵母双杂交系统,我们克隆了1.0 kb和2.5 kb的cDNA,它们编码相同的鼠E2,即泛素结合酶,这是基于其与E2A转录因子的相互作用。该cDNA编码158个氨基酸的蛋白质mUBC9,它与酿酒酵母的UBC9和粟酒裂殖酵母的HUS5有相当程度的序列同源性,并且与人UBC9蛋白相同。HUS5对DNA损伤修复至关重要,而UBC9对G2/M期进程是必需的。已证明人蛋白可纠正酵母中的UBC9缺陷。针对细菌表达的mUBC9融合蛋白产生的抗血清识别一种约18 kDa的鼠细胞蛋白,与预测的迁移率相符。与E2A不同,mUBC9蛋白水平不受血清生长因子调节。明显的同源物UBC9和HUS5的活性表明mUBC9可能参与调节细胞周期进程的关键核蛋白的降解。

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