首页> 外文期刊>The Journal of biological chemistry >ATP Hydrolysis Enhances RNA Recognition and Antiviral Signal Transduction by the Innate Immune Sensor, Laboratory of Genetics and Physiology 2 (LGP2)
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ATP Hydrolysis Enhances RNA Recognition and Antiviral Signal Transduction by the Innate Immune Sensor, Laboratory of Genetics and Physiology 2 (LGP2)

机译:ATP水解增强了先天免疫传感器,遗传学和生理学实验室的RNA识别和抗病毒信号转导2(LGP2)

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摘要

Laboratory of genetics and physiology 2 (LGP2) is a member of the RIG-I-like receptor family of cytoplasmic pattern recognition receptors that detect molecular signatures of virus infection and initiate antiviral signal transduction cascades. The ATP hydrolysis activity of LGP2 is essential for antiviral signaling, but it has been unclear how the enzymatic properties of LGP2 regulate its biological response. Quantitative analysis of the dsRNA binding and enzymatic activities of LGP2 revealed high dsRNA-independent ATP hydrolysis activity. Biochemical assays and single-molecule analysis of LGP2 and mutant variants that dissociate basal from dsRNA-stimulated ATP hydrolysis demonstrate that LGP2 utilizes basal ATP hydrolysis to enhance and diversify its RNA recognition capacity, enabling the protein to associate with intrinsically poor substrates. This property is required for LGP2 to synergize with another RIG-I-like receptor, MDA5, to potentiate IFNβ transcription in vivo during infection with encephalomyocarditis virus or transfection with poly(I:C). These results demonstrate previously unrecognized properties of LGP2 ATP hydrolysis and RNA interaction and provide a mechanistic basis for a positive regulatory role for LGP2 in antiviral signaling.
机译:遗传学和生理学实验室2(LGP2)是细胞质图案识别受体的钻石-i样受体家族的成员,其检测病毒感染的分子签名,并引发抗病毒信号转导级联。 LGP2的ATP水解活性对于抗病毒信号传导至关重要,但目前尚不清楚LGP2的酶促性能调节其生物反应。 LGP2的DSRNA结合和酶活性的定量分析显示出高DSRNA无关的ATP水解活性。 LGP2和突变体变体的生化测定和单分子分析来自DSRNA刺激的ATP水解的基础分离,表明LGP2利用基础ATP水解以增强和多样化其RNA识别能力,使蛋白质能够与本质上差的基材相关联。 LGP2需要此属性与另一种钻井平台-I样受体MDA5和脑膜眼病毒感染或用聚(I:C)转染期间,在体内增强IFNβ转录。这些结果证明了先前未被识别的LGP2 ATP水解和RNA相互作用的性能,并为抗病毒信号传导中LGP2的阳性调节作用提供机械基础。

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