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拟南芥不对称植物质体 ClpP/R 蛋白酶复合物的亚基计量、进化和功能意义。

Subunit stoichiometry, evolution, and functional implications of an asymmetric plant plastid ClpP/R protease complex in Arabidopsis.

机构信息

Department of Plant Biology, Cornell University, Ithaca, New York 14853, USA.

出版信息

Plant Cell. 2011 Jun;23(6):2348-61. doi: 10.1105/tpc.111.086454. Epub 2011 Jun 28.

DOI:10.1105/tpc.111.086454
PMID:21712416
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC3160023/
Abstract

The caseinolytic protease (Clp) protease system has been expanded in plant plastids compared with its prokaryotic progenitors. The plastid Clp core protease consists of five different proteolytic ClpP proteins and four different noncatalytic ClpR proteins, with each present in one or more copies and organized in two heptameric rings. We determined the exact subunit composition and stoichiometry for the intact core and each ring. The chloroplast ClpP/R protease was affinity purified from clpr4 and clpp3 Arabidopsis thaliana null mutants complemented with C-terminal StrepII-tagged versions of CLPR4 and CLPP3, respectively. The subunit stoichiometry was determined by mass spectrometry-based absolute quantification using stable isotope-labeled proteotypic peptides generated from a synthetic gene. One heptameric ring contained ClpP3,4,5,6 in a 1:2:3:1 ratio. The other ring contained ClpP1 and ClpR1,2,3,4 in a 3:1:1:1:1 ratio, resulting in only three catalytic sites. These ClpP1/R1-4 proteins are most closely related to the two subunits of the cyanobacterial P3/R complex and the identical P:R ratio suggests conserved adaptation. Furthermore, the plant-specific C-terminal extensions of the ClpP/R subunits were not proteolytically removed upon assembly, suggesting a regulatory role in Clp chaperone interaction. These results will now allow testing ClpP/R structure-function relationships using rationale design. The quantification workflow we have designed is applicable to other protein complexes.

摘要

与原核祖先相比,植物质体中的蛋白水解蛋白酶(Clp)蛋白酶系统已经得到扩展。质体 Clp 核心蛋白酶由五个不同的蛋白水解 ClpP 蛋白和四个不同的非催化 ClpR 蛋白组成,每个蛋白都有一个或多个拷贝,并组织在两个七聚体环中。我们确定了完整核心和每个环的精确亚基组成和化学计量。叶绿体 ClpP/R 蛋白酶是从 clpr4 和 clpp3 拟南芥 null 突变体中亲和纯化的,分别用 C 端带有 StrepII 标签的 CLPR4 和 CLPP3 互补。亚基化学计量是通过基于质谱的绝对定量确定的,使用从合成基因产生的稳定同位素标记的蛋白质肽段。一个七聚体环包含 ClpP3、4、5、6,比例为 1:2:3:1。另一个环包含 ClpP1 和 ClpR1、2、3、4,比例为 3:1:1:1:1,仅产生三个催化位点。这些 ClpP1/R1-4 蛋白与蓝细菌 P3/R 复合物的两个亚基最密切相关,相同的 P:R 比值表明了保守的适应。此外,组装过程中 ClpP/R 亚基的植物特异性 C 端延伸没有被蛋白水解去除,这表明它们在 Clp 伴侣相互作用中具有调节作用。这些结果现在将允许使用合理设计来测试 ClpP/R 的结构-功能关系。我们设计的定量工作流程适用于其他蛋白质复合物。

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