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使用胺反应性等压标记试剂和串联质谱法对人成纤维细胞的四种不同生长状态进行同步蛋白质组分析。

Simultaneous proteomic profiling of four different growth states of human fibroblasts, using amine-reactive isobaric tagging reagents and tandem mass spectrometry.

作者信息

Cong Yu-Sheng, Fan Ellen, Wang Eugenia

机构信息

Department of Microbiology and Immunology, University of Louisville School of Medicine, 580 South Preston Street, Louisville, KY 40292, United States.

出版信息

Mech Ageing Dev. 2006 Apr;127(4):332-43. doi: 10.1016/j.mad.2005.12.005. Epub 2006 Jan 23.

DOI:10.1016/j.mad.2005.12.005
PMID:16434083
Abstract

In general, permanent growth arrest due to exhaustive cell replication can be induced prematurely by either stress or overexpression of selected oncogenes. In an attempt to examine key proteins involved in achieving premature senescence, and how they differ from those in serially passaged, replicatively exhausted cells, we used a novel proteomic profiling approach, isobaric tagging for relative and absolute quantitation (iTRAQ), to perform simultaneous four-way comparison of replicatively senescent fibroblasts, oxidatively stressed prematurely senescent fibroblasts, and their young replicating and quiescent counterparts. Two hundred and forty proteins were identified and quantified simultaneously; data analysis reveals: (1) groups of proteins whose expressions are uniformly either up- or down-regulated in all three growth arrest states; (2) signature proteins which may serve as candidate proteomic markers to differentiate the quiescent state from permanent growth arrest by either exhaustive replication or stress induction and (3) that while oxidative stress-induced, prematurely senescent fibroblasts morphologically resemble their replicatively exhausted counterparts, they exhibit different protein expression patterns. Results from simultaneous proteomic profiling were validated by Western blotting for selected proteins: collagen type I, HSP90 and vimentin. In conclusion, this report shows that iTRAQ proteomic profiling is a powerful technique for globally mapping protein signatures for different culture growth states.

摘要

一般来说,应激或特定癌基因的过表达可过早诱导因细胞复制耗尽而导致的永久性生长停滞。为了研究参与实现过早衰老的关键蛋白质,以及它们与连续传代、复制耗尽的细胞中的蛋白质有何不同,我们使用了一种新型蛋白质组学分析方法,即相对和绝对定量的等压标记(iTRAQ),对复制性衰老的成纤维细胞、氧化应激过早衰老的成纤维细胞及其年轻的增殖和静止对应细胞进行同时四路比较。同时鉴定和定量了240种蛋白质;数据分析显示:(1)在所有三种生长停滞状态下表达均一致上调或下调的蛋白质组;(2)可作为候选蛋白质组学标记物的特征蛋白,用于通过复制耗尽或应激诱导区分静止状态与永久性生长停滞;(3)虽然氧化应激诱导的过早衰老的成纤维细胞在形态上类似于其复制耗尽的对应细胞,但它们表现出不同的蛋白质表达模式。通过对选定蛋白质(I型胶原蛋白、热休克蛋白90和波形蛋白)进行蛋白质印迹法验证了同时蛋白质组学分析的结果。总之,本报告表明,iTRAQ蛋白质组学分析是一种强大的技术,可用于全面绘制不同培养生长状态下的蛋白质特征图谱。

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