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钙离子、肌醇三磷酸和环二磷酸腺苷核糖在介导绵羊晶状体细胞间钙离子信号传导中的作用。

Roles of Ca2+, inositol trisphosphate and cyclic ADP-ribose in mediating intercellular Ca2+ signaling in sheep lens cells.

作者信息

Churchill G C, Louis C F

机构信息

Department of Biochemistry, University of Minnesota, St. Paul, MN 55108, USA.

出版信息

J Cell Sci. 1998 May;111 ( Pt 9):1217-25. doi: 10.1242/jcs.111.9.1217.

DOI:10.1242/jcs.111.9.1217
PMID:9547298
Abstract

To further characterize how gap junction-dependent Ca2+ waves propagate between sheep lens cells, we examined the possible roles of inositol 1,4,5-trisphosphate (IP3), Ca2+ and cyclic ADP-ribose (cADPR) in mediating intercellular Ca2+ waves. Second messengers were microinjected into a single cell in a monolayer of sheep lens cells while monitoring cytosolic Ca2+ with fura-2 and fluorescence microscopy. All three compounds initiated intercellular Ca2+ waves, but more cells responded following the injection of either IP3 or cADPR than responded following the injection of Ca2+. When either IP3 or cADPR was co-injected with the Ca2+ chelator EGTA, cytosolic Ca2+ in the injected cell decreased but cytosolic Ca2+ in the adjacent cells increased, indicating that the intercellular messenger was IP3 or cADPR, rather than Ca2+. The phospholipase C inhibitor U73122 eliminated mechanically initiated intercellular Ca2+ waves, indicating that mechanical initiation probably requires IP3 production. In U73122-treated cells, injected IP3 initiated an intercellular Ca2+ wave in which the number of cells responding increased as the amount of IP3 injected increased, indicating that the distance traveled by the Ca2+ wave was dependent on cell-to-cell diffusion of IP3. In contrast, the ability of cADPR both to increase cytosolic Ca2+ in the injected cell and to initiate intercellular Ca2+ waves was greatly attenuated by U73122. In conclusion, Ca2+, IP3 and cADPR can all mediate intercellular Ca2+ waves by passing through gap junction channels, but both IP3 and cADPR are more effective intercellular messengers than Ca2+.

摘要

为了进一步明确缝隙连接依赖的Ca2+波在绵羊晶状体细胞间的传播方式,我们研究了肌醇1,4,5-三磷酸(IP3)、Ca2+和环ADP核糖(cADPR)在介导细胞间Ca2+波中的可能作用。将第二信使显微注射到单层绵羊晶状体细胞中的单个细胞内,同时用fura-2和荧光显微镜监测胞质Ca2+。所有这三种化合物均能引发细胞间Ca2+波,但注射IP3或cADPR后作出反应的细胞比注射Ca2+后作出反应的细胞更多。当IP3或cADPR与Ca2+螯合剂乙二醇双四乙酸(EGTA)共同注射时,注射细胞内的胞质Ca2+减少,但相邻细胞内的胞质Ca2+增加,这表明细胞间信使是IP3或cADPR,而非Ca2+。磷脂酶C抑制剂U73122消除了机械引发的细胞间Ca2+波,这表明机械引发可能需要IP3的产生。在经U73122处理的细胞中,注射的IP3引发了细胞间Ca2+波,其中作出反应的细胞数量随着IP3注射量的增加而增加,这表明Ca2+波传播的距离取决于IP3在细胞间的扩散。相反,U73122极大地减弱了cADPR增加注射细胞内胞质Ca2+以及引发细胞间Ca2+波的能力。总之,Ca2+、IP3和cADPR均可通过缝隙连接通道介导细胞间Ca2+波,但IP3和cADPR作为细胞间信使比Ca2+更有效。

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