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9L大鼠胶质肉瘤细胞中Hsp90亚型差异翻译的调控机制

Control mechanisms of differential translation of Hsp90 isoforms in 9L rat gliosarcoma cells.

作者信息

Lo Chih-Wei, Chang Yuo-Sheng, Chao Chih-Chung, Chang Margaret Dah-Tsyr, Chang Kun-Che, Lai Yiu-Kay

机构信息

Department of Life Science, Institute of Biotechnology, National Tsing Hua University, Hsinchu 30013, Taiwan, ROC.

出版信息

J Cell Biochem. 2009 Jun 1;107(3):418-27. doi: 10.1002/jcb.22138.

Abstract

Although the differential expression of heat shcok proteins, Hsp90alpha and Hsp90beta was extensively studied in many kinds of cells, the post-transcriptional regulation of Hsp90 isoforms remains unclear. In control and GA-treated rat gliosarcoma cells, it has been reported that the translational efficiency of hsp90alpha is higher than hsp90beta. In this study, we present evidences identifying the roles for leaky scanning and 5'-UTR sequence in translational regulation of Hsp90beta. The result of in vitro transcription and translation (IVTT) experiment showed that hsp90alpha exhibited higher translation efficiency than hsp90beta. Sequence analysis revealed that there is an out-of-frame downstream AUG codon in hsp90beta gene. However, elimination of the downstream AUG by site-directly mutagenesis or introducing Kozak context sequence around the initiator AUG of hsp90beta open reading frame increased its translational efficiency, which indicated that leaky scanning might be a possible mechanism regulating hsp90beta. Furthermore, we also constructed a firefly luciferase reporter system to verify the effect of subsequent translation at the downstream out-of-frame AUG codon in 9L and A549 cells. Furthermore, it is believed that 5'-untranslated region (5'-UTR) also plays a significant role in translational control. We showed hsp90beta 5'-UTR gives rise to the reduction of the translation efficiency in IVTT experiment. Additionally, the reductive effect of hsp90beta 5'-UTR was further confirmed by luciferase reporter assay using truncated deletion analyses of 5'-UTR of hsp90beta. Our results support the hypothesis that ribosome leaky scanning mechanism and 5'-UTR sequence acts as negative regulators in hsp90beta mRNA.

摘要

尽管热休克蛋白Hsp90α和Hsp90β的差异表达在多种细胞中得到了广泛研究,但Hsp90亚型的转录后调控仍不清楚。在对照和GA处理的大鼠胶质肉瘤细胞中,据报道hsp90α的翻译效率高于hsp90β。在本研究中,我们提供了证据,确定了渗漏扫描和5'-UTR序列在Hsp90β翻译调控中的作用。体外转录和翻译(IVTT)实验结果表明hsp90α的翻译效率高于hsp90β。序列分析显示hsp90β基因中有一个框外下游AUG密码子。然而,通过定点诱变消除下游AUG或在hsp90β开放阅读框的起始AUG周围引入Kozak上下文序列可提高其翻译效率,这表明渗漏扫描可能是调节hsp90β的一种可能机制。此外,我们还构建了萤火虫荧光素酶报告系统,以验证9L和A549细胞中框外下游AUG密码子处后续翻译的效果。此外,人们认为5'-非翻译区(5'-UTR)在翻译控制中也起着重要作用。我们发现在IVTT实验中hsp90β 5'-UTR导致翻译效率降低。此外,通过对hsp90β 5'-UTR进行截短缺失分析的荧光素酶报告试验进一步证实了hsp90β 5'-UTR的还原作用。我们的结果支持核糖体渗漏扫描机制和5'-UTR序列作为hsp90β mRNA负调控因子的假设。

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