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核糖体蛋白 S19 C 端在 C5a 受体介导的 Gi 蛋白依赖性人肥大细胞 HMC-1 细胞中 p38MAP 激酶的替代激活中的作用。

The role of the ribosomal protein S19 C-terminus in Gi protein-dependent alternative activation of p38 MAP kinase via the C5a receptor in HMC-1 cells.

机构信息

Department of Molecular Pathology, Kumamoto University Graduate School, Japan.

出版信息

Apoptosis. 2010 Aug;15(8):966-81. doi: 10.1007/s10495-010-0511-y.

DOI:10.1007/s10495-010-0511-y
PMID:20473571
Abstract

We have demonstrated that an alternative C5a receptor (C5aR) ligand, the homodimer of ribosomal protein S19 (RP S19), contains a unique C-terminus (I(134)-H(145)) that is distinct from the moieties involved in the C5a-C5aR interaction. To examine the role of I(134)-H(145) in the ligand-C5aR interaction, we connected this peptide to the C-terminus of C5a (C5a/RP S19) and found that it endowed the second binding moiety of RP S19 (L(131)DR) with a relatively higher binding affinity to the C5aR on a human mast cell line, HMC-1. In contrast to the C5aR, the second C5aR C5L2 worked as a decoy receptor. As a result, the mitogen-activated protein kinase (MAPK) downstream of the Gi protein exchanged extracellular-signal regulated kinase for p38MAPK. This alternative p38MAPK activation could be pharmacologically suppressed not only by the downregulation of phosphoinositide 3-kinase (PI3K) by LY294002, but also by the over-activation of protein kinase C by phorbol 12-myristate 13-acetate. The activation was reproduced upon C5a-C5aR interaction by a simultaneous suppression of PI3K and phospholipase C with LY294002 and U73122 at low concentrations. Moreover, p38MAPK phosphorylation upstream of the pertussis toxin-dependent extracellular Ca(2+) entry was also suppressed by high concentrations of MgCl(2), which blocks melastatin-type transient receptor potential Ca(2+) channels (TRPMs). The active conformation of C5aR upon the ligation by C5a, at least on HMC-1 cells, is changed by the additional interaction of the I(134)-H(145) peptide, which seems to guide the alternative activation of p38MAPK. This activation is then amplified by a novel positive feedback loop between p38MAPK and TRPM.

摘要

我们已经证明,一种替代 C5a 受体(C5aR)配体,核糖体蛋白 S19(RP S19)的同源二聚体,含有一个独特的 C 末端(I(134)-H(145)),与参与 C5a-C5aR 相互作用的部分不同。为了研究 I(134)-H(145)在配体-C5aR 相互作用中的作用,我们将该肽连接到 C5a 的 C 末端(C5a/RP S19)上,并发现它赋予 RP S19 的第二个结合基序(L(131)DR)对人肥大细胞系 HMC-1 上的 C5aR 具有相对较高的结合亲和力。与 C5aR 相反,第二个 C5aR C5L2 作为诱饵受体起作用。结果,Gi 蛋白下游的丝裂原激活蛋白激酶(MAPK)将细胞外信号调节激酶交换为 p38MAPK。这种替代的 p38MAPK 激活不仅可以通过 LY294002 下调磷酯酰肌醇 3-激酶(PI3K)来抑制,还可以通过佛波醇 12-肉豆蔻酸 13-醋酸酯过度激活蛋白激酶 C 来抑制。通过在低浓度下同时用 LY294002 和 U73122 抑制 PI3K 和磷脂酶 C,可以在 C5a-C5aR 相互作用时再现这种激活。此外,高浓度的 MgCl2(阻断 melastatin 型瞬时受体电位 Ca2+通道(TRPM))也抑制了百日咳毒素依赖性细胞外 Ca2+进入上游的 p38MAPK 磷酸化。至少在 HMC-1 细胞上,C5a 配体结合后 C5aR 的活性构象通过 I(134)-H(145)肽的额外相互作用发生改变,这似乎引导了 p38MAPK 的替代激活。这种激活然后通过 p38MAPK 和 TRPM 之间的新的正反馈环放大。

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