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艰难梭菌毒素 B 对巨噬细胞中 GPCR 刺激的 Ca2+反应有差异影响:Rho 和 PLA2 的作用独立。

Clostridium difficile toxin B differentially affects GPCR-stimulated Ca2+ responses in macrophages: independent roles for Rho and PLA2.

机构信息

Alliance for Cellular Signaling at Northern California Institute for Research and Education, VA Medical Center, San Francisco, California, USA.

出版信息

J Leukoc Biol. 2010 Jun;87(6):1041-57. doi: 10.1189/jlb.1108708. Epub 2010 Mar 3.

Abstract

Clostridium difficile toxins cause acute colitis by disrupting the enterocyte barrier and promoting inflammation. ToxB from C. difficile inactivates Rho family GTPases and causes release of cytokines and eicosanoids by macrophages. We studied the effects of ToxB on GPCR signaling in murine RAW264.7 macrophages and found that ToxB elevated Ca(2+) responses to Galphai-linked receptors, including the C5aR, but reduced responses to Galphaq-linked receptors, including the UDP receptors. Other Rho inhibitors also reduced UDP Ca(2+) responses, but they did not affect C5a responses, suggesting that ToxB inhibited UDP responses by inhibiting Rho but enhanced C5a responses by other mechanisms. By using PLCbeta isoform-deficient BMDM, we found that ToxB inhibited Ca(2+) signaling through PLCbeta4 but enhanced signaling through PLCbeta3. Effects of ToxB on GPCR Ca(2+) responses correlated with GPCR use of PLCbeta3 versus PLCbeta4. ToxB inhibited UDP Ca(2+) signaling without reducing InsP3 production or the sensitivity of cellular Ca(2+) stores to exogenous InsP3, suggesting that ToxB impairs UDP signaling at the level of InsP3/Ca(2+)coupling. In contrast, ToxB elevated InsP3 production by C5a, and the enhancement of Ca(2+) signaling by C5a was prevented by inhibition of PLA(2) or 5-LOX but not COX, implicating LTs but not prostanoids in the mechanism. In sum, ToxB has opposing, independently regulated effects on Ca(2+) signaling by different GPCR-linked PLCbeta isoforms in macrophages.

摘要

艰难梭菌毒素通过破坏肠上皮细胞屏障并促进炎症来引起急性结肠炎。艰难梭菌的 ToxB 使 Rho 家族 GTP 酶失活,并导致巨噬细胞释放细胞因子和类二十烷酸。我们研究了 ToxB 对小鼠 RAW264.7 巨噬细胞中 GPCR 信号的影响,发现 ToxB 增强了与 Galphai 连接的受体(包括 C5aR)的 Ca(2+)反应,但降低了与 Galphaq 连接的受体(包括 UDP 受体)的反应。其他 Rho 抑制剂也降低了 UDP Ca(2+)反应,但它们不影响 C5a 反应,这表明 ToxB 通过抑制 Rho 抑制 UDP 反应,但通过其他机制增强 C5a 反应。通过使用 PLCbeta 同工型缺陷的 BMDM,我们发现 ToxB 通过 PLCbeta4 抑制 Ca(2+)信号,但通过 PLCbeta3 增强信号。ToxB 对 GPCR Ca(2+)反应的影响与 GPCR 使用 PLCbeta3 与 PLCbeta4 相关。ToxB 抑制 UDP Ca(2+)信号而不降低 InsP3 的产生或细胞 Ca(2+)库对外部 InsP3 的敏感性,表明 ToxB 在 InsP3/Ca(2+)偶联水平上损害 UDP 信号。相比之下,ToxB 通过 C5a 升高 InsP3 的产生,并且通过 PLA(2)或 5-LOX 但不是 COX 抑制 C5a 增强的 Ca(2+)信号,提示 LTs 而不是前列腺素在该机制中起作用。总之,ToxB 在巨噬细胞中对不同与 GPCR 相关的 PLCbeta 同工型的 Ca(2+)信号具有相反的、独立调节的影响。

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