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首页> 外文期刊>Endocrinology >Delineating biological pathways unique to embryonic stem cell-derived insulin-producing cell lines from their noninsulin-producing progenitor cell lines.
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Delineating biological pathways unique to embryonic stem cell-derived insulin-producing cell lines from their noninsulin-producing progenitor cell lines.

机译:从其非胰岛素产生祖细胞中描绘出胚胎干细胞衍生的胰岛素产生细胞系所特有的生物途径。

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To identify unique biochemical pathways in embryonic stem cell-derived insulin-producing cells as potential therapeutic targets to prevent or delay beta-cell dysfunction or death in diabetic patients, comparative genome-wide gene expression studies of recently derived mouse insulin-producing cell lines and their progenitor cell lines were performed using microarray technology. Differentially expressed genes were functionally clustered to identify important biochemical pathways in these insulin-producing cell lines. Biochemical or cellular assays were then performed to assess the relevance of these pathways to the biology of these cells. A total of 185 genes were highly expressed in the insulin-producing cell lines, and computational analysis predicted the pentose phosphate pathway (PPP), clathrin-mediated endocytosis, and the peroxisome proliferator-activated receptor (PPAR) signaling pathway as important pathways in these cell lines. Insulin-producing ERoSHK cells were more resistant to hydrogen peroxide (H(2)O(2))-induced oxidative stress. Inhibition of PPP by dehydroepiandrosterone and 6-aminonicotinamide abrogated this H(2)O(2) resistance with a concomitant decrease in PPP activity as measured by 3-(4,5-dimethylthiazol-2-yl)-2,5-diphenyl tetrazolium bromide (MTT) assay. Clathrin-mediated endocytosis, which is essential in maintaining membrane homeostasis in secreting cells, was up-regulated by glucose in ERoSHK but not in their progenitor ERoSH cells. Its inhibition by chlorpromazine at high glucose concentration was toxic to the cells. Troglitazone, a PPARG agonist, up-regulated expression of Ins1 and Ins2 but not Glut2. Gene expression analysis has identified the PPP, clathrin-mediated endocytosis, and the PPAR signaling pathway as the major delineating pathways in these insulin-producing cell lines, and their biological relevance was confirmed by biochemical and cellular assays.
机译:为了确定源自胚胎干细胞的胰岛素产生细胞中独特的生化途径作为预防或延迟糖尿病患者β细胞功能障碍或死亡的潜在治疗靶标,对最近衍生的小鼠胰岛素产生细胞系和全基因组基因表达进行了比较研究。他们的祖细胞系使用微阵列技术进行。在这些产生胰岛素的细胞系中,差异表达的基因在功能上进行了聚类以鉴定重要的生化途径。然后进行生化或细胞测定以评估这些途径与这些细胞生物学的相关性。共有185个基因在胰岛素产生细胞系中高度表达,并且计算分析预测,戊糖磷酸途径(PPP),网格蛋白介导的内吞作用和过氧化物酶体增殖物激活受体(PPAR)信号途径是这些途径中的重要途径。细胞系。胰岛素生产的ERoSHK细胞对过氧化氢(H(2)O(2))诱导的氧化应激更有抵抗力。脱氢表雄酮和6-氨基烟酰胺对PPP的抑制废除了这种H(2)O(2)的耐药性,同时伴随着3-(4,5-二甲基噻唑-2-基)-2,5-二苯基四唑鎓测定的PPP活性下降溴化物(MTT)分析。网格蛋白介导的内吞作用是维持分泌细胞膜稳态的关键,它在ERoSHK中被葡萄糖上调,但在其祖细胞ERoSH中并未被葡萄糖上调。在高葡萄糖浓度下,氯丙嗪对其抑制作用对细胞有毒。曲格列酮(PPARG激动剂)可上调Ins1和Ins2的表达,但不上调Glut2的表达。基因表达分析已确定PPP,网格蛋白介导的内吞作用和PPAR信号传导途径是这些产生胰岛素的细胞系的主要描绘途径,并且它们的生物学相关性已通过生化和细胞分析证实。

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