IPS-1基因缺失突变体对IFN-β诱生作用及抗HSV-1病毒作用的影响

目的：初步研究缺失300—444位氨基酸突变体△IPS-1对IFN-β诱生作用及抗HSV-1病毒作用的影响，进而确定该部位对IPS-1发挥正常功能的作用。方法：通过重叠延伸PCR法获得缺失300～444位氨基酸的△IPS-1，构建突变重组质粒pEF—BOS—FLAG—△IPS-1，并经酶切及测序鉴定。采用磷酸钙体外转染HEK293T真核细胞。经Western blot检测蛋白的表达；ELISA检测细胞上清中IFN—β分泌量；HSV-1病毒感染分别转染了pEF—BOS—FLAG／IPS-1、pEF—BOS—FLAG／△IPS-1质粒的HEK293T细胞，空斑检测各转染细胞组不同时间段细胞上清的病毒滴度。结果：成功构建了缺失300～444位氨基酸的IPS-1基因重组真核表达载体pEF—BOS—FLAG／△IPS-1；与转染pEF—BOS—FLAG／IPS-1质粒组相比转染了pEF—BOS—FLAG／△IPS-1的细胞在不同时间段其上清中IFN—β分泌量有一定量的减少；空斑测定结果表明转染了pEF—BOS—FLAG／△IPS-1质粒组细胞中病毒滴度明显高于pEF—BOS-FLAG／IPS-1质粒组。结论：△IPS-1与IPS-1相比能使HEK293T细胞IFN—β分泌量明显减少，△IPS-1不能完全抑制HSV-1感染细胞产生的细胞病变效应，该突变体抗HSV-1病毒作用有一定程度的减弱。

IPS-1基因缺失突变体真核表达载体的构建与鉴定

目的构建干扰素8启动刺激因子1（IPS-1）的300～444位氨基酸缺失突变体重组质粒，并初步鉴定。方法通过重叠延伸PCR法获得缺失300～444位氨基酸的突变体△IPS-1，构建缺失突变体重组质粒pEF—BOS—FLAG-△IPS-1，并经XbaI及claI双酶切及测序鉴定。结果双酶切缺失突变体重组质粒pEF—BOS—nAG-△1PS—l后，琼脂糖凝胶电泳可见1250bp附近的片段。DNA测序结果做BLAsT分析，显示重组质粒含有1266bp的目的基因片段，读码框正确，无碱基错配和移码突变。结论成功构建了缺失300～444位氨基酸的IPS-1基因重组真核表达载体pEF—BOS—nAG-△IPS-1。

The interaction between the helicase DHX33 and IPS-1 as a novel pathway to sense double-stranded RNA and RNA viruses in myeloid dendritic cells

In eukaryotes, there are at least 60 members of the DExD/H helicase family, many of which are able to sense viral nucleic acids. By screening all known family members, we identified the helicase DHX33 as a novel double-stranded RNA （dsRNA） sensor in myeloid dendritic cells （mDCs）. The knockdown of DHX33 using small heteroduplex RNA （shRNA） blocked the ability of mDCs to produce type I interferon （IFN） in response to poly hC and reovirus. The HELICc domain of DHX33 was shown to bind poly hC. The interaction between DHX33 and IPS-1 is mediated by the HELICc region of DHX33 and the C-terminal domain of IPS-1 （also referred to MAVS and VISA）. The inhibition of DHX33 expression by RNA interference blocked the poly hC-induced activation of MAP kinases, NF-KB and IRF3. The interaction between the helicase DHX33 and IPS-1 was independent of RIG-I/MDA5 and may be a novel pathway for sensing poly I-C and RNA viruses in mDCs.

MDA5与抗病毒感染信号转导

MDA5是胞内模式识别受体,能够识别入侵病毒RNA链,主要在非髓系细胞系中发挥抗病毒作用。MDA5包括3个功能区域:CARD、DExD/H以及无功能RD。CARD与DExD/H分别发挥信号传递与ATP水解功能,无功能RD主要使MDA5基于病毒5'-ppp末端不同识别单股正链RNA病毒中的EMCV;MDA5能通过CARD结构域与线粒体结合的接头蛋白IPS-1相互作用,激活转录因子IRF-3/IRF-7,诱导其核转位促进β干扰素的表达,从而启动固有免疫应答。此外,还可以通过FADD依赖途径产生NF-κB,调控炎症反应因子表达。本文综述MDA5在结构、识别病毒及其信号转导等方面的研究新进展。