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枯草芽孢杆菌 RNA 聚合酶的动态蛋白质伙伴关系。

The dynamic protein partnership of RNA polymerase in Bacillus subtilis.

机构信息

INRA,UMR 1319 Micalis, Jouy-en-Josas, France.

出版信息

Proteomics. 2011 Aug;11(15):2992-3001. doi: 10.1002/pmic.201000790. Epub 2011 Jun 28.

Abstract

In prokaryotes, transcription results from the activity of a 400 kDa RNA polymerase (RNAP) protein complex composed of at least five subunits (2α, β, β', ω). To ensure adequate responses to changing environmental cues, RNAP activity is tightly controlled by means of interacting regulatory proteins. Here, we report the affinity-purification of the Bacillus subtilis RNAP complexes from cells in different growth states and stress conditions, and the quantitative assessment by mass spectrometry of the dynamic changes in the composition of the RNAP complex. The stoichiometry of RNA polymerase was determined by a comparison of two mass spectrometry-based quantification methods: a label-based and a label-free method. The validated label-free method was then used to quantify the proteins associated with RNAP. The levels of sigma factors bound to RNAP varied during growth and exposure to stress. Elongation factors, helicases such as HelD and PcrA, and novel unknown proteins were also associated with RNAP complexes. The content in 6S RNAs of purified RNAP complexes increased at the onset of the stationary phase. These quantitative variations in the protein and RNA composition of the RNAP complexes well correlate with the known physiology of B. subtilis cells under different conditions.

摘要

在原核生物中,转录是由一个由至少五个亚基(2α、β、β'、ω)组成的 400 kDa RNA 聚合酶(RNAP)蛋白复合物的活性所产生的。为了确保对不断变化的环境线索做出充分的反应,RNAP 活性通过相互作用的调节蛋白来进行严格的控制。在这里,我们报告了从不同生长状态和应激条件下的细胞中亲和纯化枯草芽孢杆菌 RNAP 复合物的情况,并通过质谱法对 RNAP 复合物组成的动态变化进行了定量评估。通过比较两种基于质谱的定量方法:标记法和无标记法,确定了 RNA 聚合酶的化学计量。用经过验证的无标记方法来定量与 RNAP 相关的蛋白质。与 RNAP 结合的 sigma 因子的水平在生长和应激暴露过程中发生变化。延伸因子、解旋酶(如 HelD 和 PcrA)和新的未知蛋白也与 RNAP 复合物有关。在静止期开始时,纯化的 RNAP 复合物中的 6S RNA 含量增加。这些与已知的不同条件下枯草芽孢杆菌细胞生理学相关的 RNAP 复合物中蛋白质和 RNA 组成的定量变化。

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