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随机繁殖的叙利亚仓鼠对麻疹病毒感染靶细胞的细胞介导细胞毒性。

Cell-mediated cytotoxicity toward measles virus-infected target cells in randomly bred Syrian hamsters.

作者信息

Cremer N E, O'Keefe B, Hagens S J, Diggs J

出版信息

Infect Immun. 1982 Nov;38(2):580-7. doi: 10.1128/iai.38.2.580-587.1982.

Abstract

Cell-mediated cytotoxicity (CMC) toward measles virus-infected cells was studied by a (51)Cr release assay with spleen cells from hamsters inoculated with measles virus (strain Lec) or control antigen and with spleen cells from normal hamsters. Spleen cells from measles virus-inoculated hamsters showed greater CMC toward infected than toward noninfected target cells (designated specific CMC). Specific CMC was maximal 7 days after virus inoculation and was declining by 9 to 10 days. Effector cells were present in a nonadherent cell population. Specific CMC was reduced after treatments of effector cells with antithymocyte serum plus complement. The decrease in cytotoxicity was greater toward infected target cells than toward noninfected target cells. Treatment of infected target cells with antimeasles serum did not increase specific CMC by effector cells from the majority of virus-inoculated hamsters. CMC toward infected target cells by normal spleen cells (natural killer cells) or spleen cells from hamsters inoculated with control antigen was approximately the same as, or more often less than, CMC toward noninfected target cells. Natural killer cells were present in a nonadherent cell population. Treatment of natural killer cells with antithymocyte serum plus complement caused a similar decrease in cytotoxicity toward both infected and noninfected target cells. This study demonstrated virus-specific cellular cytotoxicity of effector spleen cells from measles virus-inoculated hamsters. Although the data were compatible with T cells as the source of effector cells in the virus-specific CMC, definitive identification could not be made. Additional membrane markers for better characterization of hamster lymphocyte subpopulations are required.

摘要

采用铬(51)释放试验,以接种麻疹病毒(Lec株)或对照抗原的仓鼠脾细胞以及正常仓鼠脾细胞,研究了对麻疹病毒感染细胞的细胞介导细胞毒性(CMC)。接种麻疹病毒的仓鼠脾细胞对感染靶细胞的CMC大于对未感染靶细胞的CMC(称为特异性CMC)。特异性CMC在病毒接种后7天达到最大值,9至10天时下降。效应细胞存在于非贴壁细胞群体中。用抗胸腺细胞血清加补体处理效应细胞后,特异性CMC降低。对感染靶细胞的细胞毒性降低幅度大于对未感染靶细胞的降低幅度。用抗麻疹血清处理感染靶细胞,大多数接种病毒的仓鼠的效应细胞并未增加特异性CMC。正常脾细胞(自然杀伤细胞)或接种对照抗原的仓鼠脾细胞对感染靶细胞的CMC与对未感染靶细胞的CMC大致相同,或更常见的是低于对未感染靶细胞的CMC。自然杀伤细胞存在于非贴壁细胞群体中。用抗胸腺细胞血清加补体处理自然杀伤细胞,对感染和未感染靶细胞的细胞毒性均有类似程度的降低。本研究证明了接种麻疹病毒的仓鼠效应脾细胞具有病毒特异性细胞毒性。尽管数据与T细胞作为病毒特异性CMC中效应细胞来源相符,但无法做出明确鉴定。需要更多的膜标记物来更好地表征仓鼠淋巴细胞亚群。

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