D'Hertog Wannes, Overbergh Lut, Lage Kasper, Ferreira Gabriela Bonfim, Maris Michael, Gysemans Conny, Flamez Daisy, Cardozo Alessandra Kupper, Van den Bergh Gert, Schoofs Liliane, Arckens Lut, Moreau Yves, Hansen Daniel Aaen, Eizirik Decio Laks, Waelkens Ettienne, Mathieu Chantal
Laboratory for Experimental Medicine and Endocrinology, University Hospital Gasthuisberg, Catholic University of Leuven, Herestraat 49, box 902, B-3000 Leuven, Belgium.
Mol Cell Proteomics. 2007 Dec;6(12):2180-99. doi: 10.1074/mcp.M700085-MCP200. Epub 2007 Oct 5.
Cytokines released by islet-infiltrating immune cells play a crucial role in beta-cell dysfunction and apoptotic cell death in the pathogenesis of type 1 diabetes and after islet transplantation. RNA studies revealed complex pathways of genes being activated or suppressed during this beta-cell attack. The aim of the present study was to analyze protein changes in insulin-producing INS-1E cells exposed to inflammatory cytokines in vitro using two-dimensional DIGE. Within two different pH ranges we observed 2214 +/- 164 (pH 4-7) and 1641 +/- 73 (pH 6-9) spots. Analysis at three different time points (1, 4, and 24 h of cytokine exposure) revealed that the major changes were taking place only after 24 h. At this time point 158 proteins were altered in expression (4.1%, n = 4, p < or = 0.01) by a combination of interleukin-1beta and interferon-gamma, whereas only 42 and 23 proteins were altered by either of the cytokines alone, giving rise to 199 distinct differentially expressed spots. Identification of 141 of these by MALDI-TOF/TOF revealed proteins playing a role in insulin secretion, cytoskeleton organization, and protein and RNA metabolism as well as proteins associated with endoplasmic reticulum and oxidative stress/defense. We investigated the interactions of these proteins and discovered a significant interaction network (p < 1.27e-05) containing 42 of the identified proteins. This network analysis suggests that proteins of different pathways act coordinately in a beta-cell dysfunction/apoptotic beta-cell death interactome. In addition the data suggest a central role for chaperones and proteins playing a role in RNA metabolism. As many of these identified proteins are regulated at the protein level or undergo post-translational modifications, a proteomics approach, as performed in this study, is required to provide adequate insight into the mechanisms leading to beta-cell dysfunction and apoptosis. The present findings may open new avenues for the understanding and prevention of beta-cell loss in type 1 diabetes.
胰岛浸润免疫细胞释放的细胞因子在1型糖尿病发病机制以及胰岛移植后β细胞功能障碍和凋亡性细胞死亡中起关键作用。RNA研究揭示了在这种β细胞攻击过程中基因被激活或抑制的复杂途径。本研究的目的是使用二维差异凝胶电泳分析体外暴露于炎性细胞因子的胰岛素分泌细胞系INS-1E中的蛋白质变化。在两个不同的pH范围内,我们观察到2214±164个(pH 4 - 7)和1641±73个(pH 6 - 9)蛋白点。在三个不同时间点(细胞因子暴露1、4和24小时)进行分析,结果显示主要变化仅在24小时后发生。在这个时间点,白细胞介素-1β和干扰素-γ共同作用使158种蛋白质的表达发生改变(4.1%,n = 4,p≤0.01),而单独使用其中任何一种细胞因子时,分别只有42种和23种蛋白质的表达发生改变,从而产生了199个不同的差异表达蛋白点。通过基质辅助激光解吸电离飞行时间串联质谱(MALDI-TOF/TOF)对其中141个蛋白点进行鉴定,发现这些蛋白质在胰岛素分泌、细胞骨架组织、蛋白质和RNA代谢以及与内质网和氧化应激/防御相关的过程中发挥作用。我们研究了这些蛋白质之间的相互作用,发现了一个包含42个已鉴定蛋白质的显著相互作用网络(p < 1.27e - 05)。该网络分析表明,不同途径的蛋白质在β细胞功能障碍/凋亡性β细胞死亡相互作用组中协同发挥作用。此外,数据表明伴侣蛋白和在RNA代谢中起作用的蛋白质发挥着核心作用。由于许多这些已鉴定的蛋白质在蛋白质水平受到调控或经历翻译后修饰,因此需要像本研究中所采用的蛋白质组学方法,以充分了解导致β细胞功能障碍和凋亡的机制。本研究结果可能为理解和预防1型糖尿病中β细胞丢失开辟新途径。
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