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大鼠胰岛蛋白的二维凝胶电泳。L-精氨酸耗竭和烟酰胺可减轻白细胞介素1β诱导的蛋白表达变化。

Two-dimensional gel electrophoresis of rat islet proteins. Interleukin 1 beta-induced changes in protein expression are reduced by L-arginine depletion and nicotinamide.

作者信息

Andersen H U, Larsen P M, Fey S J, Karlsen A E, Mandrup-Poulsen T, Nerup J

机构信息

Steno Diabetes Center, Gentofte, Denmark.

出版信息

Diabetes. 1995 Apr;44(4):400-7. doi: 10.2337/diab.44.4.400.

DOI:10.2337/diab.44.4.400
PMID:7698507
Abstract

Interleukin (IL)-1 beta-mediated damage to beta-cells in isolated islets of Langerhans depends upon de novo synthesis of proteins that have not been fully identified. Further, IL-1 beta-induced and tumor necrosis factor alpha-induced islet damage partly depends on the intracellular production of the nitric oxide (NO) radical. IL-1 beta has also been reported to induce the synthesis of cellular defense proteins, e.g., heme-oxygenase and heat shock proteins 70 and 90. Nicotinamide, while in itself inactive, inhibited IL-1 beta-induced NO production in a time- and dose-dependent manner. To enable the identification of IL-1 beta-induced proteins with possible protective and deleterious effects, we characterized the effects of IL-1 beta, nicotinamide, and NO synthesis inhibition by L-arginine depletion on rat islet protein expression detected by high-resolution two-dimensional gel electrophoresis. More than 1,600 proteins were reproducibly detected in control rat islets. Incubation with IL-1 beta-, nicotinamide-, or L-arginine-depleted control medium upregulated 29, 3, and 1 protein, respectively, and downregulated 4, 0, and 1 protein, respectively. Addition of nicotinamide and L-arginine depletion reduced the upregulation of 16 and 20 IL-1 beta-induced proteins, respectively. The identity of these proteins is under study. The demonstrated changes in protein expression caused by IL-1 beta +/- nicotinamide and L-arginine depletion may form the basis for identification of proteins with possible protective and deleterious roles in the initial beta-cell destruction in insulin-dependent diabetes mellitus.

摘要

白细胞介素(IL)-1β介导的对分离的胰岛β细胞的损伤取决于尚未完全鉴定的蛋白质的从头合成。此外,IL-1β诱导的和肿瘤坏死因子α诱导的胰岛损伤部分取决于一氧化氮(NO)自由基的细胞内产生。据报道,IL-1β还可诱导细胞防御蛋白的合成,例如血红素加氧酶以及热休克蛋白70和90。烟酰胺本身无活性,但能以时间和剂量依赖的方式抑制IL-1β诱导的NO产生。为了能够鉴定出具有可能的保护和有害作用的IL-1β诱导蛋白,我们通过高分辨率二维凝胶电泳检测了IL-1β、烟酰胺以及通过耗竭L-精氨酸抑制NO合成对大鼠胰岛蛋白表达的影响。在对照大鼠胰岛中可重复检测到1600多种蛋白质。用IL-1β、烟酰胺或耗竭L-精氨酸的对照培养基孵育分别上调了29、3和1种蛋白质,分别下调了4、0和1种蛋白质。添加烟酰胺和耗竭L-精氨酸分别减少了16种和20种IL-1β诱导蛋白的上调。这些蛋白质的身份正在研究中。由IL-1β±烟酰胺和耗竭L-精氨酸所导致的已证实的蛋白质表达变化可能为鉴定在胰岛素依赖型糖尿病初始β细胞破坏中具有可能的保护和有害作用的蛋白质奠定基础。

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