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首页> 外文期刊>Transplantation: Official Journal of the Transplantation Society >Porcine endogenous retrovirus encodes xenoantigens involved in porcine cellular xenograft rejection by mice.
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Porcine endogenous retrovirus encodes xenoantigens involved in porcine cellular xenograft rejection by mice.

机译:猪内源性逆转录病毒编码与小鼠的猪细胞异种移植排斥有关的异种抗原。

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摘要

BACKGROUND: Identification of the antigens that stimulate transplant rejection can help develop graft-specific antirejection strategies. The xenoantigens recognized during rejection of porcine cellular xenografts have not been clearly defined, but it has been assumed that major histocompatibility complex (MHC) xenoantigens are involved. METHODS: The role of porcine endogenous retrovirus (PERV) as a source of xenoantigens was examined. The authors used morphometry to compare the kinetics of swine leukocyte antigen (SLA) pig thyroid xenograft rejection in control mice and mice immunized with PERV PK15 cells (porcine kidney epithelial cells), PERV SLA pig peripheral blood lymphocytes (PBL), PERV virions purified from PK15 cells, and PERV or PERV A pseudotypes produced from infected human 293 cells. The tempo of rejection for cellular xenografts of PERV A pseudotype-producing human 293 cells, uninfected human 293 cells, and PK15 cells in PERV-preimmunized and control mice was also compared. RESULTS: Mice immunized with PK15 cells rejected pig thyroid xenografts significantly faster at day 5 than control mice and mice immunized with pig PBL. This correlated with the amount of PERV RNA and virions produced, but not with the amount of SLA class I MHC expressed by PK15 cells. Immunization of mice with PERV virions purified from porcine PK15 cells and with PERV virions or PERV A pseudotypes produced by human 293 cells also induced accelerated xenograft rejection by 5 days. Accelerated rejection induced by virus pretreatment was CD4 T-cell dependent and restricted to PERV-expressing cellular xenografts of porcine or nonporcine origin. CONCLUSIONS: PERV acts as a significant source of xenoantigens that target porcine cellular xenografts for rejection.
机译:背景:鉴定刺激移植排斥的抗原可以帮助开发特定于移植物的抗排斥策略。猪细胞异种移植排斥过程中识别的异种抗原尚未明确定义,但已假定涉及主要的组织相容性复合物(MHC)异种抗原。方法:检查猪内源性逆转录病毒(PERV)作为异种抗原来源的作用。作者使用形态计量学比较了对照小鼠和用PERV PK15细胞(猪肾上皮细胞),PERV SLA猪外周血淋巴细胞(PBL),从中纯化的PERV病毒颗粒免疫的小鼠中猪白细胞抗原(SLA)猪甲状腺异种移植排斥反应的动力学。 PK15细胞以及从感染的人293细胞产生的PERV或PERV A假型。还比较了PERV预免疫和对照小鼠中PERV A假型产生的人293细胞,未感染的人293细胞和PK15细胞的异种移植排斥反应的速度。结果:在第5天,用PK15细胞免疫的小鼠排斥猪甲状腺异种移植的速度明显快于对照小鼠和用猪PBL免疫的小鼠。这与产生的PERV RNA和病毒粒子的数量有关,但与PK15细胞表达的SLA I类MHC的数量无关。用从猪PK15细胞纯化的PERV病毒体和PERV病毒体或PERV A免疫小鼠,人293细胞产生的假型也诱导异种移植排斥反应加速5天。病毒预处理诱导的加速排斥反应是CD4 T细胞依赖性的,并仅限于猪或非猪源性PERV表达细胞异种移植。结论:PERV是靶向猪细胞异种移植排斥反应的异种抗原的重要来源。

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