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克隆性胰岛素瘤细胞系中葡萄糖反应性及一种ATP刺激的、不依赖钙的磷脂酶A2酶的表达

Glucose-responsitivity and expression of an ATP-stimulatable, Ca(2+)-independent phospholipase A2 enzyme in clonal insulinoma cell lines.

作者信息

Ramanadham S, Wolf M J, Li B, Bohrer A, Turk J

机构信息

Washington University School of Medicine, St. Louis, MO 63110, USA.

出版信息

Biochim Biophys Acta. 1997 Jan 21;1344(2):153-64. doi: 10.1016/s0005-2760(96)00139-7.

Abstract

We have previously reported that pancreatic islet beta-cells and clonal HIT insulinoma cells express an ATP-stimulatable Ca(2+)-independent phospholipase A2 (ASCI-PLA2) enzyme and that activation of this enzyme appears to participate in glucose-stimulated insulin secretion. To further examine this hypothesis, glucose-responsitivity and expression of ASCI-PLA2 activity in various insulinoma cell lines were examined. Secretagogue-stimulated insulin secretion was observed with beta TC6-f7 and early passage (EP)-beta TC6 cells. In contrast, RIN-m5f, beta TC3, and late passage (LP)-beta TC6 cells exhibited little secretagogue-induced secretion. A haloenollactone suicide substrate (HELSS) which inhibits ASCI-PLA2 activity ablated secretagogue-induced insulin secretion from beta TC6-f7 and EP-beta TC6 cells. All insulinoma cell lines studied expressed both cytosolic and membrane-associated Ca(2+)-independent PLA2 activities which were inhibited by HELSS. The cytosolic enzymatic activity in the glucose-responsive beta TC6-f7 and EP-beta TC6 cells was activated by ATP and protected against thermal denaturation by ATP, but this was not the case in the glucose-unresponsive RIN-m5f, beta TC3, or LP-beta TC6 cells. Comparison of the distribution of Ca(2+)-independent PLA2 activity revealed that membrane-associated activity was higher than cytosolic activity in beta TC6-f7 and EP-beta TC6 cells but not in RIN-m5f, beta TC3, or LP-beta TC6 cells. Insensitivity of cytosolic activity to ATP may prevent association of the PLA2 activity with membrane substrates and contribute to attenuated glucose-responsitivity in the RIN-m5f, beta TC3, or LP-beta TC6 cells. HIT insulinoma cells were also found to undergo a decline in both glucose-responsitivity and membrane-associated Ca(2+)-independent PLA2 activity upon serial passage in culture, and this was associated with a reduction in membrane content of arachidonate-containing phospholipids. These and previous results suggest that the ATP-stimulatable PLA2 enzyme may participate in glucose-induced insulin secretion.

摘要

我们之前曾报道,胰岛β细胞和克隆的HIT胰岛素瘤细胞表达一种ATP刺激的、不依赖钙离子的磷脂酶A2(ASCI-PLA2),且该酶的激活似乎参与了葡萄糖刺激的胰岛素分泌。为了进一步验证这一假说,我们检测了各种胰岛素瘤细胞系中ASCI-PLA2活性的葡萄糖反应性和表达情况。在βTC6-f7细胞和早期传代(EP)-βTC6细胞中观察到促分泌剂刺激的胰岛素分泌。相比之下,RIN-m5f细胞、βTC3细胞和晚期传代(LP)-βTC6细胞几乎没有促分泌剂诱导的分泌。一种抑制ASCI-PLA2活性的卤代烯醇内酯自杀底物(HELSS)消除了βTC6-f7细胞和EP-βTC6细胞中促分泌剂诱导的胰岛素分泌。所有研究的胰岛素瘤细胞系均表达胞质和膜相关的不依赖钙离子的PLA2活性,且均被HELSS抑制。葡萄糖反应性的βTC6-f7细胞和EP-βTC6细胞中的胞质酶活性被ATP激活,并被ATP保护免受热变性影响,但在葡萄糖无反应性的RIN-m5f细胞、βTC3细胞或LP-βTC6细胞中并非如此。对不依赖钙离子的PLA2活性分布的比较显示,膜相关活性在βTC6-f7细胞和EP-βTC6细胞中高于胞质活性,但在RIN-m5f细胞、βTC3细胞或LP-βTC6细胞中并非如此。胞质活性对ATP不敏感可能会阻止PLA2活性与膜底物结合,并导致RIN-m5f细胞、βTC3细胞或LP-βTC6细胞中葡萄糖反应性减弱。还发现HIT胰岛素瘤细胞在培养中连续传代后,葡萄糖反应性和膜相关的不依赖钙离子的PLA2活性均下降,这与含花生四烯酸磷脂的膜含量减少有关。这些结果以及之前的结果表明,ATP刺激的PLA2酶可能参与葡萄糖诱导的胰岛素分泌。

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