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使用溴化氰裂解和传统双向电泳分析大于150 kDa的高分子量蛋白质。

Analysis of high molecular mass proteins larger than 150 kDa using cyanogen bromide cleavage and conventional 2-DE.

作者信息

Morla Aymeric, Poirier Florence, Pons Sylvie, Beaulieu Corinne, Charrier Jean-Philippe, Ataman-Onal Yasemin, Gléhen Olivier, Jolivet Michel, Choquet-Kastylevsky Geneviève

机构信息

Department of Biomarker' Research and Validation, bioMérieux, Marcy l'Etoile, France.

出版信息

Electrophoresis. 2008 Nov;29(20):4158-68. doi: 10.1002/elps.200800007.

Abstract

Proteomic approaches including high-resolution 2-DE are providing the tools needed to discover disease-associated biomarkers in complex biological samples. Although 2-DE is an extremely powerful approach to analyze the proteome, the separation of proteins with extreme molecular masses still remains an issue requiring improvement. Because high molecular mass (HMM) proteins larger than 150 kDa have already been observed to be differentially expressed in several pathologies such as cancer, we developed an original strategy to analyze this part of the proteome that is not easily separated by 2-DE in polyacrylamide gels. This strategy is based on the 2-DE separation of cyanogen bromide (CNBr) fragments of purified HMM protein fractions, and combines techniques including SEC fractionation, TCA precipitation, CNBr cleavage, 2-DE and MS analysis. The method was first tested on a model protein, the BSA. Preliminary results obtained using colonic tissues led to the identification of six HMM proteins with M(r) comprised between 163 and 533 kDa in their reduced state. These results demonstrated that our CNBr/2-DE approach should provide a powerful tool for identification of new biomarkers larger than 150 kDa.

摘要

包括高分辨率二维电泳(2-DE)在内的蛋白质组学方法,正在为在复杂生物样品中发现疾病相关生物标志物提供所需工具。尽管二维电泳是分析蛋白质组的一种极其强大的方法,但分离极端分子量的蛋白质仍然是一个需要改进的问题。由于已经观察到大于150 kDa的高分子量(HMM)蛋白质在癌症等几种病症中存在差异表达,我们开发了一种原创策略来分析蛋白质组中这部分不易在聚丙烯酰胺凝胶中通过二维电泳分离的蛋白质。该策略基于纯化的高分子量蛋白质组分的溴化氰(CNBr)片段的二维电泳分离,并结合了包括尺寸排阻色谱(SEC)分级分离、三氯乙酸(TCA)沉淀、CNBr裂解、二维电泳和质谱分析在内的技术。该方法首先在一种模型蛋白质——牛血清白蛋白(BSA)上进行了测试。使用结肠组织获得的初步结果导致鉴定出六种还原状态下分子量(M(r))介于163至533 kDa之间的高分子量蛋白质。这些结果表明,我们的CNBr/二维电泳方法应为鉴定大于150 kDa的新生物标志物提供一种强大的工具。

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