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鸡骨骼肌中20S蛋白酶体的亚基结构与动力学

The subunit structure and dynamics of the 20S proteasome in chicken skeletal muscle.

作者信息

Hayter Julia R, Doherty Mary K, Whitehead Colin, McCormack Heather, Gaskell Simon J, Beynon Robert J

机构信息

Department of Veterinary Preclinical Sciences, University of Liverpool, Liverpool L69 7ZJ, United Kingdom.

出版信息

Mol Cell Proteomics. 2005 Sep;4(9):1370-81. doi: 10.1074/mcp.M400138-MCP200. Epub 2005 Jun 19.

DOI:10.1074/mcp.M400138-MCP200
PMID:15965267
Abstract

We have succeeded in purifying the 20S core proteasome particle from less than 1 g of skeletal muscle in a rapid process involving two chromatographic steps. The individual subunits were readily resolved by two-dimensional PAGE, and the identities of each of the 14 subunits were assigned by a combination of peptide mass fingerprinting and MS/MS/de novo sequencing. To assess the dynamics of proteasome biogenesis, chicks were fed a diet containing stable isotope-labeled valine, and the rate of incorporation of label into valine-containing peptides derived from each subunit was assessed by mass spectrometric analysis after two-dimensional separation. Peptides containing multiple valine residues from the 20S proteasome and other soluble muscle proteins were analyzed to yield the relative isotope abundance of the precursor pool, a piece of information that is essential for calculation of turnover parameters. The rates of synthesis of each subunit are rather similar, although there is evidence for high turnover subunits in both the alpha (nonproteolytic) and beta (proteolytic) rings. The variability in synthesis rate for the different subunits is consistent with a model in which some subunits are produced in excess, whereas others may be the rate-limiting factor in the concentration of 20S subunits in the cell. The ability to measure turnover rates of proteins on a proteome-wide scale in protein assemblies and in a complex organism provides a new dimension to the understanding of the dynamic proteome.

摘要

我们已成功地通过一个包含两个色谱步骤的快速过程,从不到1克的骨骼肌中纯化出20S核心蛋白酶体颗粒。通过二维聚丙烯酰胺凝胶电泳(2D-PAGE)很容易分离出各个亚基,并通过肽质量指纹图谱和串联质谱/从头测序相结合的方法确定了14个亚基中每个亚基的身份。为了评估蛋白酶体生物合成的动力学,给雏鸡喂食含有稳定同位素标记缬氨酸的饲料,并在二维分离后通过质谱分析评估标记掺入源自每个亚基的含缬氨酸肽中的速率。分析了来自20S蛋白酶体和其他可溶性肌肉蛋白的含有多个缬氨酸残基的肽,以得出前体池的相对同位素丰度,这是计算周转参数所必需的一条信息。每个亚基的合成速率相当相似,尽管有证据表明在α(非蛋白水解)环和β(蛋白水解)环中都存在高周转率的亚基。不同亚基合成速率的变异性与一种模型一致,在该模型中,一些亚基过量产生,而其他亚基可能是细胞中20S亚基浓度的限速因素。在蛋白质组装体和复杂生物体中在全蛋白质组范围内测量蛋白质周转速率的能力为理解动态蛋白质组提供了一个新的维度。

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