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抗原受体触发的细胞毒性T淋巴细胞激活的生化研究的机制、功能及免疫药理学意义

Mechanistic, functional and immunopharmacological implications of biochemical studies of antigen receptor-triggered cytolytic T-lymphocyte activation.

作者信息

Sitkovsky M V

机构信息

Laboratory of Immunology, National Institute of Allergy and Infectious Diseases, Bethesda, Maryland 20892.

出版信息

Immunol Rev. 1988 Mar;103:127-60. doi: 10.1111/j.1600-065x.1988.tb00754.x.

DOI:10.1111/j.1600-065x.1988.tb00754.x
PMID:3134292
Abstract

Biochemical events that follow the engagement of cytotoxic T lymphocytes (CTL) with an Ag-bearing target cell (TC) or triggering by the crosslinking of the Ag-receptor (TcR) by immobilized anti-TcR mAb were studied using cloned CTL and a novel CTL activation assay. The approach described here was undertaken to shed light on the molecular mechanisms of "ON", "STOP" and "OFF" signalling that allow CTL to be activated, kill TC and disengage from the target cell after delivery of the "lethal hit" and then to proceed with the destruction of the next Ag-bearing target encountered. Biochemical studies of TcR-regulated and TcR-triggered constitutive exocytosis in CTL provided a detailed description of the molecular requirements for this important phenomenon in T lymphocytes and provided an alternative CTL activation assay; this assay measures the TcR-dependent response in the absence of a TC. These studies also helped to envision CTLs screening activities as a cycle of engagements-disengagements with the TC, where every surrounding cell is treated by the CTL as a potential Ag-bearing TC. Both constitutive and regulated exocytosis in CTL are triggered through a transmembrane signalling pathway which involves protein kinase C and extracellular Ca2+ that, most likely, is translocated through Ca2+ channels. This is followed by the involvement of calmodulin (CaM)-binding proteins, e.g., calcineurin, a CaM-dependent phosphatase, which was shown to be a major CaM-binding protein in murine lymphocytes. Unexpectedly, these biochemical studies demonstrated that the granule exocytosis model of CTL-mediated cytotoxicity cannot account for the mechanism of target cell lysis by CTL, at least in in vitro conditions in the absence of extracellular Ca2+. These results indicate the existence of an extracellular Ca2+-independent, TcR-regulated CTL response and raise the possibility that second messenger(s) other than Ca2+ and/or products of phosphoinositide turnover are involved in T-cell lysis. Predominance of "non-lethal" engagements between some CTL and TC, revealed during time-lapse cinematographic studies, together with comparative studies of TcR-regulated exocytosis of granules and of constitutive exocytosis of gamma-interferon, suggested that TC destruction by CTL may not be their only or even their most important function in vivo. It is possible that CTL, triggered by Ag recognition to exocytose storage granules and to synthesize and constitutively exocytose macrophage-activating factors, in turn promote tumor destruction by macrophages.(ABSTRACT TRUNCATED AT 400 WORDS)

摘要

利用克隆的细胞毒性T淋巴细胞(CTL)和一种新型的CTL激活测定法,研究了CTL与携带抗原的靶细胞(TC)结合后或通过固定化抗TcR单克隆抗体使抗原受体(TcR)交联触发后的生化事件。采用此处所述方法是为了阐明“开启”“停止”和“关闭”信号传导的分子机制,这些机制使CTL能够被激活、杀死TC,并在传递“致命一击”后与靶细胞脱离,然后继续破坏下一个遇到的携带抗原的靶细胞。对CTL中TcR调节的和TcR触发的组成型胞吐作用的生化研究,详细描述了T淋巴细胞中这一重要现象的分子要求,并提供了另一种CTL激活测定法;该测定法在没有TC的情况下测量TcR依赖性反应。这些研究还有助于将CTL的筛选活动设想为与TC的结合-脱离循环;在这个循环中CTL会将周围的每个细胞都视为潜在的携带抗原的TC。CTL中的组成型和调节型胞吐作用都是通过一个跨膜信号通路触发的,该通路涉及蛋白激酶C和细胞外Ca2+,Ca2+很可能是通过Ca2+通道转运进去;接下来是钙调蛋白(CaM)结合蛋白的参与,例如钙调神经磷酸酶,一种CaM依赖性磷酸酶,已被证明是小鼠淋巴细胞中主要的CaM结合蛋白。出乎意料的是,这些生化研究表明,CTL介导的细胞毒性的颗粒胞吐作用模型无法解释CTL在体外无细胞外Ca2+条件下裂解靶细胞的机制。这些结果表明存在一种不依赖细胞外Ca2+、受TcR调节CT的L反应,并增加了除Ca2+和/或磷脂酰肌醇代谢产物之外的第二信使参与T细胞裂解作用的可能性。在延时电影摄影研究中发现,一些CTL与TC之间存在“非致命”结合,同时对颗粒的TcR调节型胞吐作用和γ干扰素的组成型胞吐作用进行比较研究,结果表明CTL对TC的破坏可能不是其在体内唯一的甚至最重要的功能。有可能CTL在被抗原识别后,通过胞吐储存颗粒以及合成并组成型胞吐巨噬细胞激活因子,进而促进巨噬细胞对肿瘤的破坏作用。(摘要截选至400字)

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