G12/13和Gq以一种依赖于Rho而非Rho激酶的方式介导S1P2诱导的血管平滑肌中Rac抑制和迁移。

G12/13 and Gq mediate S1P2-induced inhibition of Rac and migration in vascular smooth muscle in a manner dependent on Rho but not Rho kinase.

作者信息

Takashima Shin-Ichiro, Sugimoto Naotoshi, Takuwa Noriko, Okamoto Yasuo, Yoshioka Kazuaki, Takamura Masayuki, Takata Shigeo, Kaneko Shuichi, Takuwa Yoh

机构信息

Department of Physiology, Graduate School of Medical Sciences, Kanazawa University, 13-1 Takara-machi, Kanazawa, Ishikawa 920-8640, Japan.

出版信息

Cardiovasc Res. 2008 Sep 1;79(4):689-97. doi: 10.1093/cvr/cvn118. Epub 2008 May 14.

DOI:10.1093/cvr/cvn118

PMID:18480127

Abstract

AIMS

The lysophospholipid mediator sphingosine-1-phosphate (S1P) activates G protein-coupled receptors (GPCRs) to induce potent inhibition of platelet-derived growth factor (PDGF)-induced Rac activation and, thereby, chemotaxis in rat vascular smooth muscle cells (VSMCs). We explored the heterotrimeric G protein and the downstream mechanism that mediated S1P inhibition of Rac and cell migration in VSMCs.

METHODS AND RESULTS

S1P inhibition of PDGF-induced cell migration and Rac activation in VSMCs was abolished by the selective S1P(2) receptor antagonist JTE-013. The C-terminal peptides of Galpha subunits (Galpha-CTs) act as specific inhibitors of respective G protein-GPCR coupling. Adenovirus-mediated expression of Galpha(12)-CT, Galpha(13)-CT, and Galpha(q)-CT, but not that of Galpha(s)-CT or LacZ or pertussis toxin treatment, abrogated S1P inhibition of PDGF-induced Rac activation and migration, indicating that both G(12/13) and G(q) classes are necessary for the S1P inhibition. The expression of Galpha(q)-CT as well as Galpha(12)-CT and Galpha(13)-CT also abolished S1P-induced Rho stimulation. C3 toxin, but not a Rho kinase inhibitor or a dominant negative form of Rho kinase, abolished S1P inhibition of PDGF-induced Rac activation and cell migration. The angiotensin II receptor AT(1), which robustly couples to G(q), did not mediate either Rho activation or inhibition of PDGF-induced Rac activation or migration, suggesting that activation of G(q) alone was not sufficient for Rho activation and resultant Rac inhibition. However, the AT(1) receptor fused to Galpha(12) was able to induce not only Rho stimulation but also inhibition of PDGF-induced Rac activation and migration. Phospholipase C inhibition did not affect S1P-induced Rho activation, and protein kinase C activation by a phorbol ester did not mimic S1P action, suggesting that S1P inhibition of migration or Rac was not dependent on the phospholipase C pathway.

CONCLUSION

These observations together suggest that S1P(2) mediates inhibition of Rac and migration through the coordinated action of G(12/13) and G(q) for Rho activation in VSMCs.

摘要

目的

溶血磷脂介质1-磷酸鞘氨醇（S1P）激活G蛋白偶联受体（GPCRs），从而有效抑制血小板衍生生长因子（PDGF）诱导的大鼠血管平滑肌细胞（VSMCs）中的Rac激活及趋化作用。我们探究了异源三聚体G蛋白及介导S1P对VSMCs中Rac抑制和细胞迁移的下游机制。

方法与结果

选择性S1P(2)受体拮抗剂JTE-013消除了S1P对VSMCs中PDGF诱导的细胞迁移和Rac激活的抑制作用。Gα亚基的C末端肽（Gα-CTs）作为各自G蛋白-GPCR偶联的特异性抑制剂。腺病毒介导的Gα(12)-CT、Gα(13)-CT和Gα(q)-CT的表达，但不是Gα(s)-CT、LacZ的表达或百日咳毒素处理，消除了S1P对PDGF诱导的Rac激活和迁移的抑制作用，表明G(12/13)和G(q)类别对于S1P抑制作用均是必需的。Gα(q)-CT以及Gα(12)-CT和Gα(13)-CT的表达也消除了S1P诱导的Rho激活。C3毒素，但不是Rho激酶抑制剂或Rho激酶的显性负性形式，消除了S1P对PDGF诱导的Rac激活和细胞迁移的抑制作用。与G(q)强烈偶联的血管紧张素II受体AT(1)，既不介导Rho激活，也不介导对PDGF诱导的Rac激活或迁移的抑制作用，这表明单独激活G(q)不足以激活Rho并导致Rac抑制。然而，与Gα(12)融合的AT(1)受体不仅能够诱导Rho激活，还能抑制PDGF诱导的Rac激活和迁移。磷脂酶C抑制不影响S1P诱导的Rho激活，佛波酯激活蛋白激酶C也不能模拟S1P的作用，这表明S1P对迁移或Rac的抑制不依赖于磷脂酶C途径。