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溶血磷脂酰丝氨酸通过对骨髓来源的肥大细胞、C6胶质瘤细胞和结肠癌细胞中Ki16425/VPC32183敏感的G蛋白偶联受体诱导钙信号传导。

Lysophosphatidylserine induces calcium signaling through Ki16425/VPC32183-sensitive GPCR in bone marrow-derived mast cells and in C6 glioma and colon cancer cells.

作者信息

Kim Kyeok, Kim Hyo-Lim, Lee Yun-Kyung, Han Mijin, Sacket Santosh J, Jo Ji-Yeong, Kim Yu-Lee, Im Dong-Soon

机构信息

Laboratory of Pharmacology, College of Pharmacy (BK21 Project), Pusan National University, San 30, Jang-Jun-dong, Geum-Jung-gu, Busan 609-735, Korea.

出版信息

Arch Pharm Res. 2008 Mar;31(3):310-7. doi: 10.1007/s12272-001-1157-x. Epub 2008 Apr 13.

DOI:10.1007/s12272-001-1157-x
PMID:18409043
Abstract

Lysophosphatidylserine (LPS) can be generated following phosphatidylserine-specific phospholipase A2 activation. The effects of LPS on cellular activities and the identities of its target molecules, however, have not been fully elucidated. In this study, we observed that LPS stimulated intracellular calcium increased in mouse bone marrow-derived mast cells (BMMC), and rat C6 glioma and human HCT116 colon cancer cells and compared the LPS-induced Ca2+ increases with the response by lysophosphatidic acid (LPA), a structurally related bioactive lysolipid. In order to test involvement of signaling molecules in the LPS-induced Ca2+ signaling, we used pertussis toxin (PTX), U73122, and 2-APB, which are specific inhibitors for G proteins, phospholipase C (PLC), and IP3 receptors, respectively. The increases due to LPS and LPA were inhibited by PTX, U-73122 and 2-APB, suggesting that both lipids stimulate calcium signaling via G proteins (Gi/o types), PLC activation, and subsequent IP3 production, although the sensitivity to pharmacological inhibitors varied from complete inhibition to partial inhibition depending on cell type and lysolipid. Furthermore, we observed that Ki16425 completely inhibited an LPS-induced Ca2+ response in three cell types, but that the effect of VPC32183 varied from complete inhibition in BMMC and C6 glioma cells to partial inhibition in HCT116 cells. Therefore, we conclude that LPS increases [Ca2+]i through Ki16425/VPC32183-sensitive G protein-coupled receptors (GPCR), G protein, PLC, and IP3 in mouse BMMC, rat C6, and human HCT116 cells.

摘要

溶血磷脂酰丝氨酸(LPS)可在磷脂酰丝氨酸特异性磷脂酶A2激活后产生。然而,LPS对细胞活性的影响及其靶分子的身份尚未完全阐明。在本研究中,我们观察到LPS刺激小鼠骨髓来源的肥大细胞(BMMC)、大鼠C6胶质瘤细胞和人HCT116结肠癌细胞内钙增加,并将LPS诱导的Ca2+增加与溶血磷脂酸(LPA,一种结构相关的生物活性溶血脂质)的反应进行了比较。为了测试信号分子是否参与LPS诱导的Ca2+信号传导,我们使用了百日咳毒素(PTX)、U73122和2-APB,它们分别是G蛋白、磷脂酶C(PLC)和IP3受体的特异性抑制剂。PTX、U-73122和2-APB抑制了LPS和LPA引起的增加,表明这两种脂质均通过G蛋白(Gi/o类型)、PLC激活和随后的IP3产生来刺激钙信号传导,尽管对药理抑制剂的敏感性因细胞类型和溶血脂质而异,从完全抑制到部分抑制不等。此外,我们观察到Ki16425完全抑制了三种细胞类型中LPS诱导的Ca2+反应,但VPC32183的作用在BMMC和C6胶质瘤细胞中为完全抑制,在HCT116细胞中为部分抑制。因此,我们得出结论,在小鼠BMMC、大鼠C6和人HCT116细胞中,LPS通过Ki16425/VPC32183敏感的G蛋白偶联受体(GPCR)、G蛋白、PLC和IP3增加[Ca2+]i。

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