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在哺乳动物细胞中,有丝分裂周期蛋白的蛋白水解作用从有丝分裂末期持续到S期开始。

The proteolysis of mitotic cyclins in mammalian cells persists from the end of mitosis until the onset of S phase.

作者信息

Brandeis M, Hunt T

机构信息

ICRF Clare Hall Laboratories, South Mimms, Herts, UK.

出版信息

EMBO J. 1996 Oct 1;15(19):5280-9.

Abstract

We have studied how the cell cycle-specific oscillations of mitotic B-type cyclins are generated in mouse fibroblasts. A reporter enzyme comprising the N-terminus of a B-type cyclin fused to bacterial chloramphenicol acetyl transferase (CAT) was degraded at the end of mitosis like endogenous cyclins. Point mutations in the destruction box of this construct completely abolished its mitotic instability. When the destructible reporter was driven by the cyclin B2 promoter, CAT activity mimicked the oscillations in the level of the endogenous cyclin B2. These oscillations were largely conserved when the reporter was transcribed constitutively from the SV40 promoter. Pulse-chase experiments or addition of the proteasome inhibitors lactacystin and ALLN showed that cyclin synthesis continued after the end of mitosis. The destruction box-specific degradation of cyclins normally ceases at the onset of S phase, and is active in fibroblasts arrested in G0 and in differentiated C2 myoblasts. We were able to reproduce this proteolysis in vitro in extracts of synchronized cells. Extracts of G1 cells degraded cyclin B1 whereas p27Kip1 was stable, in contrast, cyclin B1 remained stable and p27Kip1 was degraded in extracts of S phase cells.

摘要

我们研究了小鼠成纤维细胞中,有丝分裂B型细胞周期蛋白的细胞周期特异性振荡是如何产生的。一种由B型细胞周期蛋白的N端与细菌氯霉素乙酰转移酶(CAT)融合而成的报告酶,在有丝分裂末期像内源性细胞周期蛋白一样被降解。该构建体破坏框中的点突变完全消除了其有丝分裂不稳定性。当可降解的报告基因由细胞周期蛋白B2启动子驱动时,CAT活性模拟了内源性细胞周期蛋白B2水平的振荡。当报告基因由SV40启动子组成型转录时,这些振荡在很大程度上得以保留。脉冲追踪实验或添加蛋白酶体抑制剂乳胞素和ALLN表明,细胞周期蛋白的合成在有丝分裂结束后仍在继续。细胞周期蛋白的破坏框特异性降解通常在S期开始时停止,在G0期停滞的成纤维细胞和分化的C2成肌细胞中具有活性。我们能够在同步化细胞的提取物中体外重现这种蛋白水解过程。G1期细胞的提取物降解细胞周期蛋白B1,而p27Kip1是稳定的,相反,在S期细胞的提取物中,细胞周期蛋白B1保持稳定,而p27Kip1被降解。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/401c/452272/bb2411e47639/emboj00019-0162-a.jpg

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