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使用定量质谱法描绘大肠杆菌核糖体生物发生图谱。

Characterization of the ribosome biogenesis landscape in E. coli using quantitative mass spectrometry.

机构信息

Department of Molecular Biology, The Scripps Research Institute, La Jolla, CA 92037, USA.

出版信息

J Mol Biol. 2013 Feb 22;425(4):767-79. doi: 10.1016/j.jmb.2012.11.040. Epub 2012 Dec 7.

Abstract

The ribosome is an essential and highly complex biological system in all living cells. A large body of literature on the assembly of the ribosome in vitro is available, but a clear picture of this process inside the cell has yet to emerge. Here, we directly characterized in vivo ribosome assembly intermediates and associated assembly factors from wild-type Escherichia coli cells using a general quantitative mass spectrometry (qMS) approach. The presence of distinct populations of ribosome assembly intermediates was verified using an in vivo stable isotope pulse-labeling approach, and their exact ribosomal protein contents were characterized against an isotopically labeled standard. The model-free clustering analysis of the resultant protein levels for the different ribosomal particles produced four 30S assembly groups that correlate very well with previous in vitro assembly studies of the small ribosomal subunit and six 50S assembly groups that clearly define an in vivo assembly landscape for the larger ribosomal subunit. In addition, de novo proteomics identified a total of 21 known and potentially new ribosome assembly factors co-localized with various ribosomal particles. These results represent new in vivo assembly maps of the E. coli 30S and 50S subunits, and the general qMS approach should prove to be a solid platform for future studies of ribosome biogenesis across a host of model organisms.

摘要

核糖体是所有活细胞中必不可少且高度复杂的生物系统。关于核糖体在体外组装的大量文献已经存在,但细胞内这一过程的清晰图景尚未出现。在这里,我们使用通用的定量质谱 (qMS) 方法直接从野生型大肠杆菌细胞中鉴定了体内核糖体组装中间体和相关组装因子。使用体内稳定同位素脉冲标记方法验证了核糖体组装中间体的存在,并用同位素标记的标准品对其确切的核糖体蛋白含量进行了表征。对不同核糖体颗粒产生的蛋白质水平进行无模型聚类分析,得到了四个 30S 组装组,它们与小核糖体亚基的体外组装研究非常吻合,还有六个 50S 组装组,它们明确定义了大核糖体亚基的体内组装图谱。此外,从头蛋白质组学共鉴定了总共 21 种已知和潜在的新核糖体组装因子,它们与各种核糖体颗粒共定位。这些结果代表了大肠杆菌 30S 和 50S 亚基的新体内组装图谱,通用的 qMS 方法应该成为未来在众多模式生物中研究核糖体生物发生的可靠平台。

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