首页> 美国卫生研究院文献>Journal of Virology >Cytolytic T-lymphocyte responses to respiratory syncytial virus: effector cell phenotype and target proteins.
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Cytolytic T-lymphocyte responses to respiratory syncytial virus: effector cell phenotype and target proteins.

机译:对呼吸道合胞病毒的溶细胞性T淋巴细胞反应:效应细胞表型和靶蛋白。

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摘要

Cytolytic T-lymphocyte (CTL) activity specific for respiratory syncytial (RS) virus was investigated after intranasal infection of mice with RS virus, after intraperitoneal infection of mice with a recombinant vaccinia virus expressing the F glycoprotein, and after intramuscular vaccination of mice with Formalin-inactivated RS virus or a chimeric glycoprotein, FG, expressed from a recombinant baculovirus. Spleen cell cultures from mice previously infected with live RS virus or the F-protein recombinant vaccinia virus had significant CTL activity after one cycle of in vitro restimulation with RS virus, and lytic activity was derived from a major histocompatibility complex-restricted, Lyt2.2+ (CD8+) subset. CTL activity was not restimulated in spleen cells from mice that received either the Formalin-inactivated RS virus or the purified glycoprotein, FG. The protein target structures for recognition by murine CD8+ CTL were identified by using target cells infected with recombinant vaccinia viruses that individually express seven structural proteins of RS virus. Quantitation of cytolytic activity against cells expressing each target structure suggested that 22K was the major target protein for CD8+ CTL, equivalent to recognition of cells infected with RS virus, followed by intermediate recognition of F or N, slight recognition of P, and no recognition of G, SH, or M. Repeated stimulation of murine CTL with RS virus resulted in outgrowth of CD4+ CTL which, over time, became the exclusive subset in culture. Murine CD4+ CTL were highly cytolytic for RS virus-infected cells, but they did not recognize target cells infected with any of the recombinant vaccinia viruses expressing the seven RS virus structural proteins. Finally, the CTL response in peripheral blood mononuclear cells of adult human volunteers was investigated. The detection of significant levels of RS virus-specific cytolytic activity in these cells was dependent on at least two restimulations with RS virus in vitro, and cytolytic activity was derived primarily from the CD4+ subset.
机译:在小鼠鼻内感染RS病毒后,腹膜内感染表达F糖蛋白的牛痘病毒小鼠和肌肉注射福尔马林疫苗后,研究了呼吸道合胞(RS)病毒特异的细胞溶解性T淋巴细胞(CTL)活性重组杆状病毒表达的灭活的RS病毒或嵌合糖蛋白FG。经过一个周期的RS病毒体外再刺激后,先前感染了活RS病毒或F蛋白重组牛痘病毒的小鼠的脾细胞培养物具有显着的CTL活性,并且裂解活性源自主要的组织相容性复合物限制的Lyt2.2。 +(CD8 +)子集。在接受福尔马林灭活的RS病毒或纯化的糖蛋白FG的小鼠的脾脏细胞中,CTL活性未得到重新刺激。通过使用感染了重组牛痘病毒的靶细胞鉴定了可被鼠CD8 + CTL识别的蛋白质靶结构,重组牛痘病毒分别表达RS病毒的七个结构蛋白。对表达每种靶结构的细胞的细胞溶解活性的定量分析表明,22K是CD8 + CTL的主要靶蛋白,等同于识别受RS病毒感染的细胞,其次是对F或N的中等识别,对P的细微识别,对G,SH或M。用RS病毒反复刺激鼠CTL导致CD4 + CTL的生长,随着时间的流逝,CD4 + CTL成为培养物中的唯一子集。鼠CD4 + CTL对RS病毒感染的细胞具有高度的细胞溶解作用,但它们不能识别被表达7种RS病毒结构蛋白的重组牛痘病毒感染的靶细胞。最后,研究了成年志愿者的外周血单个核细胞中的CTL反应。在这些细胞中检测到显着水平的RS病毒特异性细胞溶解活性取决于至少两次体外RS病毒的再刺激,细胞溶解活性主要来源于CD4 +亚群。

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