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酿酒酵母热休克反应的定量分析。

Quantitative analysis of the heat shock response of Saccharomyces cerevisiae.

作者信息

Miller M J, Xuong N H, Geiduschek E P

出版信息

J Bacteriol. 1982 Jul;151(1):311-27. doi: 10.1128/jb.151.1.311-327.1982.

Abstract

Transient protein synthesis in Saccharomyces cerevisiae, after shift from 21-23 degrees C to 37 degrees C, was quantitatively analyzed. Pulse-labeled proteins were separated by two-dimensional gel electrophoresis, and autoradiograms of the gels were analyzed by a recently described method involving a computer-coupled film scanning system. In this way, the rate of incorporation of L-[35S]methionine into approximately 500 proteins was followed. The synthesis of more than 80 of these proteins was transiently induced at 37 degrees C, with about 20 being classified as major heat shock proteins (defined as those whose rate of labeling was increased at least eightfold at some time during the response). The synthesis of more than 300 of the proteins was transiently repressed at 37 degrees C, and several general temporal patterns of repression could be distinguished. The influence of temperature-sensitive mutations affecting RNA synthesis and transport on the heat shock response was also examined. A protein whose induction in response to heat shock has a post-transcriptional component could be identified. As previously pointed out, the heat shock repression of certain proteins is so rapid that it also must involve post-transcriptional effects.

摘要

对酿酒酵母从21 - 23摄氏度转移至37摄氏度后的瞬时蛋白质合成进行了定量分析。脉冲标记的蛋白质通过二维凝胶电泳进行分离,凝胶的放射自显影片通过一种最近描述的涉及计算机耦合胶片扫描系统的方法进行分析。通过这种方式,追踪了L - [³⁵S]甲硫氨酸掺入大约500种蛋白质的速率。其中80多种蛋白质的合成在37摄氏度时被瞬时诱导,约20种被归类为主要热休克蛋白(定义为在反应过程中的某个时间其标记速率至少增加八倍的那些蛋白)。300多种蛋白质的合成在37摄氏度时被瞬时抑制,并且可以区分出几种一般的抑制时间模式。还研究了影响RNA合成和转运的温度敏感突变对热休克反应的影响。可以鉴定出一种其对热休克的诱导具有转录后成分的蛋白质。如先前所指出的,某些蛋白质的热休克抑制非常迅速,以至于它也必定涉及转录后效应。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/17e2/220243/12b9368ee9aa/jbacter00254-0330-a.jpg

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