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C1q可诱导小鼠成纤维细胞的趋化作用以及与胞质Ca2+增加相关的钾离子电导激活。

C1q induces chemotaxis and K+ conductance activation coupled to increased cytosolic Ca2+ in mouse fibroblasts.

作者信息

Oiki S, Okada Y

机构信息

Department of Physiology, Kyoto University Faculty of Medicine, Japan.

出版信息

J Immunol. 1988 Nov 1;141(9):3177-85.

PMID:3262684
Abstract

Cultured mouse fibroblasts (L cells) respond to whole C with a slow hyperpolarization. Among the C components tested, C1q was found to be most effective. In contrast, the cell did not respond to C1, in which the collagen-like region of the C1q molecule is masked. The C1q-induced hyperpolarizing response was inhibited by collagen or C1q-specific antisera. Human diploid skin fibroblasts (Flow 1,000 cells) also exhibited similar membrane potential changes in response to whole C or C1q. After repeated applications of C1q, the cell membrane became unresponsive (desensitized). The treatment of L cells with pronase E inhibited the C1q-induced response, whereas the response to ATP, which is known to interact to its own receptor, was still preserved. The reversal potential of C responses was close to the K+ equilibrium potential. The hyperpolarizing response was inhibited by a blocker of Ca2+-activated K+ channels in fibroblasts (quinine), by deprivation of extracellular Ca2+ or by a Ca2+ channel blocker (nifedipine). By means of Ca2+-selective microelectrodes, the cytosolic free Ca2+ concentration was found to increase from 126 to 206 nM upon stimulation of L cells with C1q. Using an agarose-well method, L cells were observed to migrate predominantly toward C1q or whole C. It is concluded that the fibroblasts have the C1q receptor sensitive to pronase E and that activation of C1q receptors gives rise to Ca2+ influx, triggering an increase in the cytosolic free Ca2+ ions, which in turn induces a hyperpolarizing response as a result of the stimulation of Ca2+-activated K+ channels and initiates chemotaxis to C1q.

摘要

培养的小鼠成纤维细胞(L细胞)对完整的补体C会产生缓慢的超极化反应。在所测试的补体C成分中,发现C1q最为有效。相比之下,细胞对C1无反应,因为C1中C1q分子的胶原样区域被掩盖了。C1q诱导的超极化反应被胶原蛋白或C1q特异性抗血清所抑制。人二倍体皮肤成纤维细胞(Flow 1,000细胞)对完整的补体C或C1q也表现出类似的膜电位变化。重复应用C1q后,细胞膜变得无反应(脱敏)。用链霉蛋白酶E处理L细胞可抑制C1q诱导的反应,而对已知与其自身受体相互作用的ATP的反应仍得以保留。补体C反应的反转电位接近钾离子平衡电位。成纤维细胞中钙激活钾通道的阻滞剂(奎宁)、细胞外钙的剥夺或钙通道阻滞剂(硝苯地平)均可抑制超极化反应。通过钙选择性微电极发现,用C1q刺激L细胞后,胞质游离钙浓度从126 nM增加到206 nM。使用琼脂糖孔法观察到L细胞主要向C1q或完整的补体C迁移。结论是,成纤维细胞具有对链霉蛋白酶E敏感的C1q受体,C1q受体的激活导致钙内流,引发胞质游离钙离子增加,进而由于钙激活钾通道的刺激诱导超极化反应,并启动对C1q的趋化作用。

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