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Inhibitory Effects of Nitric Oxide and Gamma Interferon on In Vitro and In Vivo Replication of Mareks Disease Virus

机译:一氧化氮和γ干扰素对马立克氏病病毒体外和体内复制的抑制作用

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摘要

The replication of Marek's disease herpesvirus (MDV) and herpesvirus of turkeys (HVT) in chicken embryo fibroblast (CEF) cultures was inhibited by the addition of S-nitroso-N-acetylpenicillamine, a nitric oxide (NO)-generating compound, in a dose-dependent manner. Treatment of CEF culture, prepared from 11-day-old embryos, with recombinant chicken gamma interferon (rChIFN-γ) and lipopolysaccharide (LPS) resulted in production of NO which was suppressed by the addition of NG-monomethyl l-arginine (NMMA), an inhibitor of inducible NO synthase (iNOS). Incubation of CEF cultures for 72 h prior to treatment with rChIFN-γ plus LPS was required for optimal NO production. Significant differences in NO production were observed in CEF derived from MDV-resistant N2a (major histocompatibility complex [MHC], B21B21) and MDV-susceptible S13 (MHC, B13B13) and P2a (MHC, B19B19) chickens. N2a-derived CEF produced NO earlier and at higher levels than CEF from the other two lines. The lowest production of NO was detected in P2a-derived CEF. NO production in chicken splenocyte cultures followed a similar pattern, with the highest levels of NO produced in cultures from N2a chickens and the lowest levels produced in cultures from P2a chickens. Replication of MDV and HVT was significantly inhibited in CEF cultures treated with rChIFN-γ plus LPS and producing NO. The addition of NMMA to CEF treated with rChIFN-γ plus LPS reduced the inhibition. MDV infection of chickens treated with S-methylisothiourea, an inhibitor of iNOS, resulted in increased virus load compared to nontreated chickens. These results suggest that NO may play an important role in control of MDV replication in vivo.
机译:在鸡胚成纤维细胞(CEF)培养物中,马立克氏病疱疹病毒(MDV)和火鸡疱疹病毒(HVT)的复制受到S-亚硝基-N-乙酰青霉胺(一氧化氮(NO)生成)的添加的抑制。剂量依赖性。用重组鸡γ干扰素(rChIFN-γ)和脂多糖(LPS)处理从11日龄胚胎制备的CEF培养物,导致NO的产生,其通过添加N G 得到抑制-单甲基1-精氨酸(NMMA),诱导型NO合酶(iNOS)的抑制剂。为了获得最佳的NO生成,需要在用rChIFN-γ加LPS处理之前将CEF培养物孵育72小时。在耐MDV的N2a(主要组织相容性复合物[MHC],B 21 B 21 )和MDV易感性S13(MHC, B 13 B 13 )和P2a(MHC,B 19 B 19 )鸡。 N2a衍生的CEF产生NO的时间要早​​于其他两个品系的CEF。在源自P2a的CEF中检测到最低的NO产生。鸡脾细胞培养物中的NO产生遵循类似的模式,其中N2a鸡的培养物中NO含量最高,而P2a鸡的培养物中NO含量最低。在用rChIFN-γ加LPS处理的CEF培养物中,MDV和HVT的复制被显着抑制,并产生NO。在用rChIFN-γ加LPS处理的CEF中添加NMMA可降低抑制作用。与未处理的鸡相比,用iNOS抑制剂S-甲基异硫脲处理的鸡MDV感染导致病毒载量增加。这些结果表明NO可能在体内控制MDV复制中起重要作用。

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