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通过定量质谱法监测的稳定同位素脉冲追踪技术应用于大肠杆菌30S核糖体组装动力学研究。

Stable isotope pulse-chase monitored by quantitative mass spectrometry applied to E. coli 30S ribosome assembly kinetics.

作者信息

Bunner Anne E, Williamson James R

机构信息

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

出版信息

Methods. 2009 Oct;49(2):136-41. doi: 10.1016/j.ymeth.2009.06.002. Epub 2009 Jun 24.

Abstract

Stable isotope mass spectrometry has become a widespread tool in quantitative biology. Pulse-chase monitored by quantitative mass spectrometry (PC/QMS) is a recently developed stable isotope approach that provides a powerful means of studying the in vitro self-assembly kinetics of macromolecular complexes. This method has been applied to the Escherichia coli 30S ribosomal subunit, but could be applied to any stable self-assembling complex that can be reconstituted from its component parts and purified from a mixture of components and complex. The binding rates of 18 out of the 20 ribosomal proteins have been measured at several temperatures using PC/QMS. Here, PC/QMS experiments on 30S ribosomal subunit assembly are described, and the potential application of the method to other complexes is discussed. A variation on the PC/QMS experiment is introduced that enables measurement of kinetic cooperativity between proteins. In addition, several related approaches to stable isotope labeling and quantitative mass spectrometry data analysis are compared and contrasted.

摘要

稳定同位素质谱已成为定量生物学中广泛应用的工具。通过定量质谱监测的脉冲追踪(PC/QMS)是一种最近开发的稳定同位素方法,它为研究大分子复合物的体外自组装动力学提供了一种强大的手段。该方法已应用于大肠杆菌30S核糖体亚基,但可应用于任何能够从其组成部分重构并从组分和复合物混合物中纯化出来的稳定自组装复合物。使用PC/QMS在几个温度下测量了20种核糖体蛋白中18种的结合速率。本文描述了关于30S核糖体亚基组装的PC/QMS实验,并讨论了该方法在其他复合物中的潜在应用。引入了PC/QMS实验的一种变体,能够测量蛋白质之间的动力学协同性。此外,还对稳定同位素标记和定量质谱数据分析的几种相关方法进行了比较和对比。

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