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白细胞介素-1β诱导大鼠胰岛蛋白质表达变化的蛋白质组分析

Proteome analysis of interleukin-1beta--induced changes in protein expression in rat islets of Langerhans.

作者信息

Larsen P M, Fey S J, Larsen M R, Nawrocki A, Andersen H U, Kähler H, Heilmann C, Voss M C, Roepstorff P, Pociot F, Karlsen A E, Nerup J

机构信息

Center for Proteome Analysis, University of Southern Denmark, Odense.

出版信息

Diabetes. 2001 May;50(5):1056-63. doi: 10.2337/diabetes.50.5.1056.

DOI:10.2337/diabetes.50.5.1056
PMID:11334408
Abstract

The intracellular molecular events involved in the beta-cell death process are complex but poorly understood. Cytokines, e.g., interleukin (IL)-1beta, may play a crucial role in inducing this process. Protein synthesis is necessary for the deleterious effect of IL-1, and induction of both protective and deleterious proteins has been described. To characterize the rather complex pattern of islet protein expression in rat islets in response to IL-1, we have attempted to identify proteins of altered expression level after IL-1 exposure by 2D gel electrophoresis and mass spectrometry. Of 105 significantly changed (i.e., up- or downregulated or de novo-induced) protein spots, we obtained positive protein identification for 60 protein spots. The 60 identifications corresponded to 57 different proteins. Of these, 10 proteins were present in two to four spots, suggesting that posttranslatory modifications had occurred. In addition, 11 spots contained more than one protein. The proteins could be classified according to their function into the following groups: 1) energy transduction; 2) glycolytic pathway; 3) protein synthesis, chaperones, and protein folding; and 4) signal transduction, regulation, differentiation, and apoptosis. In conclusion, valuable information about the molecular mechanisms involved in cytokine-mediated beta-cell destruction was obtained by this approach.

摘要

β细胞死亡过程中涉及的细胞内分子事件很复杂,但了解甚少。细胞因子,如白细胞介素(IL)-1β,可能在诱导这一过程中起关键作用。蛋白质合成对于IL-1的有害作用是必需的,并且已经描述了保护性和有害性蛋白质的诱导。为了表征大鼠胰岛中响应IL-1的相当复杂的胰岛蛋白质表达模式,我们试图通过二维凝胶电泳和质谱法鉴定IL-1暴露后表达水平改变的蛋白质。在105个显著变化(即上调、下调或从头诱导)的蛋白质斑点中,我们对60个蛋白质斑点进行了阳性蛋白质鉴定。这60个鉴定对应于57种不同的蛋白质。其中,10种蛋白质存在于2至4个斑点中,表明发生了翻译后修饰。此外,11个斑点包含不止一种蛋白质。这些蛋白质可根据其功能分为以下几类:1)能量转导;2)糖酵解途径;3)蛋白质合成、伴侣蛋白和蛋白质折叠;4)信号转导、调节、分化和凋亡。总之,通过这种方法获得了关于细胞因子介导的β细胞破坏所涉及分子机制的有价值信息。

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