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首页> 外文OA文献 >IRF3 Inhibition by Rotavirus NSP1 Is Host Cell and Virus Strain Dependent but Independent of NSP1 Proteasomal Degradation▿
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IRF3 Inhibition by Rotavirus NSP1 Is Host Cell and Virus Strain Dependent but Independent of NSP1 Proteasomal Degradation▿

机译:轮状病毒NSP1对IRF3的抑制取决于宿主细胞和病毒株,但独立于NSP1蛋白酶体降解▿

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Rotavirus host range restriction forms a basis for strain attenuation although the underlying mechanisms are unclear. In mouse fibroblasts, the inability of rotavirus NSP1 to mediate interferon (IFN) regulatory factor 3 (IRF3) degradation correlates with IFN-dependent restricted replication of the bovine UK strain but not the mouse EW and simian RRV strains. We found that UK NSP1 is unable to degrade IRF3 when expressed in murine NIH 3T3 cells in contrast to the EW and RRV NSP1 proteins. Surprisingly, UK NSP1 expression led to IRF3 degradation in simian COS7 cells, indicating that IRF3 degradation by NSP1 is host cell dependent, a finding further supported using adenovirus-expressed NSP1 from NCDV bovine rotavirus. By expressing heterologous IRF3 proteins in complementary host cells, we found that IRF3 is the minimal host factor constraining NSP1 IRF3-degradative ability. NSP1-mediated IRF3 degradation was enhanced by transfection of double-stranded RNA (dsRNA) in a host cell-specific manner, and in IRF3-dependent positive regulatory domain III reporter assays, NSP1 inhibited IRF3 function in response to pathway activation by dsRNA, TBK-1, IRF3, or constitutively activated IRF3-5D. An interesting observation arising from these experiments is the ability of transiently expressed UK NSP1 to inhibit poly(I:C)-directed IRF3 activity in NIH 3T3 cells in the absence of detectable IRF3 degradation, an unexpected finding since UK virus infection was unable to block IFN secretion, and UK NSP1 expression did not result in suppression of IRF3-directed activation of the pathway. RRV and EW but not UK NSP1 was proteasomally degraded, requiring E1 ligase activity, although NSP1 degradation was not required for IRF3 degradation. Using a chimeric RRV NSP1 protein containing the carboxyl 100 residues derived from UK NSP1, we found that the RRV NSP1 carboxyl 100 residues are critical for its IRF3 inhibition in murine cells but are not essential for NSP1 degradation. Thus, NSP1's ability to degrade IRF3 is host cell dependent and is independent of NSP1 proteasomal degradation.
机译:轮状病毒宿主范围的限制形成了菌株减毒的基础,尽管其潜在机制尚不清楚。在小鼠成纤维细胞中,轮状病毒NSP1无法介导干扰素(IFN)调节因子3(IRF3)降解与牛UK株的IFN依赖性限制性复制有关,而与小鼠EW和猿猴RRV株无关。我们发现UK NSP1在鼠NIH 3T3细胞中表达时,与EW和RRV NSP1蛋白相反,不能降解IRF3。出乎意料的是,UK NSP1表达导致猿猴COS7细胞中IRF3降解,表明NSP1对IRF3的降解是宿主细胞依赖性的,这一发现进一步得到了使用来自NCDV牛轮状病毒的腺病毒表达的NSP1的支持。通过在互补宿主细胞中表达异源IRF3蛋白,我们发现IRF3是限制NSP1 IRF3降解能力的最小宿主因子。 NSP1介导的IRF3降解可通过以宿主细胞特异性方式转染双链RNA(dsRNA)来增强,并且在IRF3依赖性正调控域III报告基因检测中,NSP1响应dsRNA,TBK的途径激活而抑制IRF3功能。 -1,IRF3或组成性激活的IRF3-5D。这些实验引起的有趣观察是,在没有可检测到的IRF3降解的情况下,瞬时表达的UK NSP1抑制NIH 3T3细胞中由poly(I:C)定向的IRF3活性的能力,这是一个意外的发现,因为UK病毒感染无法阻断IFN的分泌和UK NSP1的表达均未导致抑制IRF3导向的途径的激活。尽管IRF3降解不需要NSP1降解,但RRV和EW而不是UK NSP1可以被蛋白酶降解,需要E1连接酶活性。使用包含衍生自UK NSP1的羧基100残基的嵌合RRV NSP1蛋白,我们发现RRV NSP1羧基100残基对其在鼠细胞中抑制IRF3至关重要,但对于NSP1降解不是必需的。因此,NSP1降解IRF3的能力取决于宿主细胞,并且独立于NSP1蛋白酶体降解。

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