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一种钙结合蛋白钙网蛋白与穿孔素(细胞毒性T细胞颗粒的一种成分)之间的相互作用。

Interaction between a Ca2+-binding protein calreticulin and perforin, a component of the cytotoxic T-cell granules.

作者信息

Andrin C, Pinkoski M J, Burns K, Atkinson E A, Krahenbuhl O, Hudig D, Fraser S A, Winkler U, Tschopp J, Opas M, Bleackley R C, Michalak M

机构信息

Molecular Biology of Membranes Research Group, University of Alberta, Edmonton, Canada.

出版信息

Biochemistry. 1998 Jul 21;37(29):10386-94. doi: 10.1021/bi980595z.

DOI:10.1021/bi980595z
PMID:9671507
Abstract

Calreticulin is a component of cytotoxic T-lymphocyte and NK lymphocyte granules. We report here that granule-associated calreticulin terminates with the KDEL endoplasmic reticulum retrieval amino acid sequence and somehow escapes the KDEL retrieval system. In perforin knock-out mice calreticulin is still targeted into the granules. Thus, calreticulin will traffic without perforin to cytotoxic granules. In the granules, calreticulin and perforin are associated as documented by (i) copurification of calreticulin with perforin but not with granzymes and (ii) immunoprecipitation of a calreticulin-perforin complex using specific antibodies. By using calreticulin affinity chromatography and protein ligand blotting we show that perforin binds to calreticulin in the absence of Ca2+ and the two proteins dissociate upon exposure to 0.1 mM or higher Ca2+ concentration. Perforin interacts strongly with the P-domain of calreticulin (the domain which has high Ca2+-binding affinity and chaperone function) as revealed by direct protein-protein interaction, ligand blotting, and the yeast two-hybrid techniques. Our results suggest that calreticulin may act as Ca2+-regulated chaperone for perforin. This action will serve to protect the CTL during biogenesis of granules and may also serve to regulate perforin lytic action after release.

摘要

钙网蛋白是细胞毒性T淋巴细胞和自然杀伤(NK)淋巴细胞颗粒的一个组成部分。我们在此报告,颗粒相关的钙网蛋白以KDEL内质网回收氨基酸序列结尾,并且不知何故逃脱了KDEL回收系统。在穿孔素基因敲除小鼠中,钙网蛋白仍被靶向进入颗粒。因此,钙网蛋白在没有穿孔素的情况下也会运输到细胞毒性颗粒中。在颗粒中,钙网蛋白和穿孔素相互关联,这一点通过以下方式得以证明:(i)钙网蛋白与穿孔素共纯化,但不与颗粒酶共纯化;(ii)使用特异性抗体对钙网蛋白-穿孔素复合物进行免疫沉淀。通过使用钙网蛋白亲和层析和蛋白质配体印迹法,我们发现穿孔素在没有Ca2+的情况下与钙网蛋白结合,并且在暴露于0.1 mM或更高Ca2+浓度时这两种蛋白质会解离。如直接蛋白质-蛋白质相互作用、配体印迹和酵母双杂交技术所揭示的,穿孔素与钙网蛋白的P结构域(具有高Ca2+结合亲和力和伴侣功能的结构域)强烈相互作用。我们的结果表明,钙网蛋白可能作为穿孔素的Ca2+调节伴侣发挥作用。这种作用将有助于在颗粒生物发生过程中保护细胞毒性T淋巴细胞(CTL),并且也可能有助于在释放后调节穿孔素的溶解作用。

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