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Identification of a receptor-independent activator of G protein signaling (AGS8) in ischemic heart and its interaction with Gβγ

机译:缺血性心脏中G蛋白信号传导的受体非依赖性激活剂(AGS8)的鉴定及其与Gβγ的相互作用

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As part of a broader effort to identify postreceptor signal regulators involved in specific diseases or organ adaptation, we used an expression cloning system in Saccharomyces cerevisiae to screen cDNA libraries from rat ischemic myocardium, human heart, and a prostate leiomyosarcoma for entities that activated G protein signaling in the absence of a G protein coupled receptor. We report the characterization of activator of G protein signaling (AGS) 8 (KIAA1866), isolated from a rat heart model of repetitive transient ischemia. AGS8 mRNA was induced in response to ventricular ischemia but not by tachycardia, hypertrophy, or failure. Hypoxia induced AGS8 mRNA in isolated adult ventricular cardiomyocytes but not in rat aortic smooth muscle cells, endothelial cells, or cardiac fibroblasts, suggesting a myocyte-specific adaptation mechanism involving remodeling of G protein signaling pathways. The bioactivity of AGS8 in the yeast-based assay was independent of guanine nucleotide exchange by Gα, suggesting an impact on subunit interactions. Subsequent studies indicated that AGS8 interacts directly with Gβγ and this occurs in a manner that apparently does not alter the regulation of the effector PLC-β_2 by Gβγ. Mechanistically, AGS8 appears to promote G protein signaling by a previously unrecognized mechanism that involves direct interaction with Gβγ.
机译:为了更广泛地确定参与特定疾病或器官适应的受体后信号调节剂,我们在酿酒酵母中使用了表达克隆系统,从大鼠缺血性心肌,人心脏和前列腺平滑肌肉瘤中筛选了激活G蛋白的实体的cDNA文库。 G蛋白偶联受体不存在时的信号转导。我们报告了从重复性短暂性脑缺血的大鼠心脏模型分离的G蛋白信号转导(AGS)8(KIAA1866)激活剂的表征。 AGS8 mRNA是对心室缺血的反应诱导的,而不是由心动过速,肥大或衰竭引起的。缺氧诱导离体成年大鼠心室心肌细胞中的AGS8 mRNA,但不影响大鼠主动脉平滑肌细胞,内皮细胞或心脏成纤维细胞中的AGS8 mRNA,这提示了涉及G蛋白信号通路重塑的心肌特异性适应机制。在基于酵母的分析中,AGS8的生物活性与Gα的鸟嘌呤核苷酸交换无关,这表明对亚基相互作用的影响。随后的研究表明,AGS8直接与Gβγ相互作用,并且这种发生方式显然不会改变Gβγ对效应子PLC-β_2的调节。从机理上讲,AGS8似乎是通过一种以前无法识别的机制促进G蛋白信号传导,该机制涉及与Gβγ的直接相互作用。

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