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磷脂酶C-γ1是肝细胞中储存操纵性Ca2+通道激活所必需的。

Phospholipase C-gamma1 is required for the activation of store-operated Ca2+ channels in liver cells.

作者信息

Litjens Tom, Nguyen Than, Castro Joel, Aromataris Edoardo C, Jones Lynette, Barritt Greg J, Rychkov Grigori Y

机构信息

School of Molecular and Biomedical Science, University of Adelaide, Adelaide, South Australia 5005, Australia.

出版信息

Biochem J. 2007 Jul 15;405(2):269-76. doi: 10.1042/BJ20061762.

Abstract

Repetitive hormone-induced changes in concentration of free cytoplasmic Ca2+ in hepatocytes require Ca2+ entry through receptor-activated Ca2+ channels and SOCs (store-operated Ca2+ channels). SOCs are activated by a decrease in Ca2+ concentration in the intracellular Ca2+ stores, but the molecular components and mechanisms are not well understood. Some studies with other cell types suggest that PLC-gamma (phospholipase C-gamma) is involved in the activation of receptor-activated Ca2+ channels and/or SOCs, independently of PLC-gamma-mediated generation of IP3 (inositol 1,4,5-trisphosphate). The nature of the Ca2+ channels regulated by PLC-gamma has not been defined clearly. The aim of the present study was to determine if PLC-gamma is required for the activation of SOCs in liver cells. Transfection of H4IIE cells derived from rat hepatocytes with siRNA (short interfering RNA) targeted to PLC-gamma1 caused a reduction (by approx. 70%) in the PLC-gamma1 protein expression, with maximal effect at 72-96 h. This was associated with a decrease (by approx. 60%) in the amplitude of the I(SOC) (store-operated Ca2+ current) developed in response to intracellular perfusion with either IP(3) or thapsigargin. Knockdown of STIM1 (stromal interaction molecule type 1) by siRNA also resulted in a significant reduction (approx. 80% at 72 h post-transfection) of the I(SOC) amplitude. Immunoprecipitation of PLC-gamma1 and STIM1, however, suggested that under the experimental conditions these proteins do not interact with each other. It is concluded that the PLC-gamma1 protein, independently of IP3 generation and STIM1, is required to couple endoplasmic reticulum Ca2+ release to the activation of SOCs in the plasma membrane of H4IIE liver cells.

摘要

激素诱导的肝细胞中游离细胞质Ca2+浓度的重复性变化需要Ca2+通过受体激活的Ca2+通道和SOCs(储存-操作性Ca2+通道)进入细胞。SOCs由细胞内Ca2+储存中Ca2+浓度的降低激活,但其分子成分和机制尚未完全清楚。一些针对其他细胞类型的研究表明,磷脂酶C-γ(PLC-γ)参与受体激活的Ca2+通道和/或SOCs的激活,独立于PLC-γ介导的肌醇1,4,5-三磷酸(IP3)的生成。由PLC-γ调节的Ca2+通道的性质尚未明确界定。本研究的目的是确定PLC-γ是否是肝细胞中SOCs激活所必需的。用靶向PLC-γ1的小干扰RNA(siRNA)转染源自大鼠肝细胞的H4IIE细胞,导致PLC-γ1蛋白表达降低(约70%),在72-96小时达到最大效应。这与在用IP(3)或毒胡萝卜素进行细胞内灌注后产生的储存-操作性Ca2+电流(I(SOC))幅度降低(约60%)相关。用siRNA敲低基质相互作用分子1型(STIM1)也导致I(SOC)幅度显著降低(转染后72小时约80%)。然而,PLC-γ1和STIM1的免疫沉淀表明,在实验条件下这些蛋白不相互作用。得出的结论是,PLC-γ1蛋白独立于IP3生成和STIM1,是将内质网Ca2+释放与H4IIE肝细胞质膜中SOCs的激活相偶联所必需的。

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