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自然杀伤细胞/大颗粒淋巴细胞在病毒复制部位的聚集与趋化作用。

Accumulation and chemotaxis of natural killer/large granular lymphocytes at sites of virus replication.

作者信息

Natuk R J, Welsh R M

出版信息

J Immunol. 1987 Feb 1;138(3):877-83.

PMID:3027167
Abstract

A model for monitoring the accumulation of natural killer cell/large granular lymphocytes (NK/LGL) at a site of virus replication was studied by using mice infected i.p. with either lymphocytic choriomeningitis virus (LCMV), murine cytomegalovirus (MCMV), mouse hepatitis virus (MHV), Pichinde virus, or vaccinia virus. An i.p. but not i.v. infection resulted in a localized increase in NK/LGL cell number (a fourfold to greater than 20-fold increase) and augmentation (a 10- to 20-fold increase) of NK cell activity associated with virus-induced peritoneal exudate cell (PEC) populations. An increase in NK/LGL cell number was detected as early as 12 hr postinfection (p.i.) and peaked at 3 days p.i. with MHV. The initial LGL recruited into the peritoneal cavity at 1 to 3 days p.i. were nonadherent to plastic and were demonstrated to have an NK cell phenotype: asialo GM1+, Thy-1.2 +/-, Lyt-2.2-, and J11d-. The peak number of LGL appeared at 7 days after infection with the NK cell-resistant virus, LCMV. This LGL population had been previously demonstrated to contain cytotoxic T lymphocyte/LGL (CTL/LGL) as well as NK/LGL. During an MHV infection the number of LGL decreased between days 3 and 7 p.i., suggesting that the second wave of CTL/LGL was absent. These findings may explain the absence of a good MHV-CTL model. Virus-induced, activated NK/LGL responded to chemotactic signals by migrating in a unidirectional manner across two 5-microns pore size polycarbonate filters during 7 hr in vitro chemotaxis assays. Wash-out fluid obtained from the peritoneal cavity contained chemotactic activity for NK/LGL as well as for other cell types. We conclude that production and/or release of chemotactic factors at sites of virus replication are at least partially responsible for the accumulation of NK/LGL at these sites.

摘要

通过使用经腹腔注射感染淋巴细胞性脉络丛脑膜炎病毒(LCMV)、鼠巨细胞病毒(MCMV)、小鼠肝炎病毒(MHV)、皮钦德病毒或痘苗病毒的小鼠,研究了一种监测自然杀伤细胞/大颗粒淋巴细胞(NK/LGL)在病毒复制部位蓄积的模型。经腹腔而非静脉感染导致NK/LGL细胞数量局部增加(增加四倍至超过二十倍),并使与病毒诱导的腹腔渗出细胞(PEC)群体相关的NK细胞活性增强(增加十至二十倍)。早在感染后12小时(p.i.)就检测到NK/LGL细胞数量增加,感染MHV时在感染后3天达到峰值。在感染后1至3天募集到腹腔的初始LGL不黏附于塑料,且被证明具有NK细胞表型:无唾液酸GM1 +、Thy-1.2 +/ -、Lyt-2.2 -和J11d -。感染NK细胞抗性病毒LCMV后7天出现LGL的峰值数量。此前已证明该LGL群体包含细胞毒性T淋巴细胞/LGL(CTL/LGL)以及NK/LGL。在MHV感染期间,感染后3至7天LGL数量减少,表明不存在第二波CTL/LGL。这些发现可能解释了缺乏良好的MHV-CTL模型的原因。在体外趋化性测定的7小时内,病毒诱导的活化NK/LGL通过以单向方式穿过两个5微米孔径的聚碳酸酯滤膜对趋化信号作出反应。从腹腔获得的洗脱液含有对NK/LGL以及其他细胞类型的趋化活性。我们得出结论,病毒复制部位趋化因子的产生和/或释放至少部分负责NK/LGL在这些部位的蓄积。

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