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在内质网应激时,HacA依赖的转录开关从翻译阻滞中释放hacA mRNA。

HacA-dependent transcriptional switch releases hacA mRNA from a translational block upon endoplasmic reticulum stress.

作者信息

Mulder Harm J, Nikolaev Igor

机构信息

Genencor, Danisco, Archimedesweg 30, 2333 CN Leiden, The Netherlands.

出版信息

Eukaryot Cell. 2009 Apr;8(4):665-75. doi: 10.1128/EC.00131-08. Epub 2009 Jan 30.

Abstract

Activation of the unfolded protein response (UPR) in eukaryotes involves the splicing of an unconventional intron from the mRNA encoding the transcriptional activator of the pathway. In Saccharomyces cerevisiae a 252-nucleotide (nt) unconventional intron is spliced out of the transcript of HAC1, changing the 3' end of the HAC1 open reading frame and relieving the transcript from a translational block in a single step. The translational block is caused by the base pairing of part of the unconventional intron with the 5'-untranslated region (5'UTR). In Aspergillus niger and other aspergilli, the unconventional intron in hacA mRNA is only 20 nt long. Since this intron is part of a stable stem-loop structure, base pairing with the 5'UTR, in contrast to the case with yeast HAC1, is not possible. However, analysis of the hacA mRNA revealed a GC-rich inverted repeat (18 base pairings). Upon the activation of the UPR, the 5'UTR of hacA mRNA is truncated by 230 nt, removing the left part of this inverted repeat. This implies a similar release of a translational block as in the case of S. cerevisiae HAC1 but in two steps. The mechanism behind the 5' truncation, which does not take place in either yeast HAC1 or mammalian xbp1 mRNA, has been hitherto unknown. Here we show that during secretion stress in A. niger, hacA transcription starts from a new start site closer to the ATG, relieving the transcript from translational attenuation. This transcriptional switch is mediated by HacA itself and the unfolded protein response element 2 (UPRE2) in the hacA promoter.

摘要

真核生物中未折叠蛋白反应(UPR)的激活涉及从不编码该途径转录激活因子的mRNA中剪接出一个非常规内含子。在酿酒酵母中,一个252个核苷酸(nt)的非常规内含子从HAC1的转录本中被剪接出来,改变了HAC1开放阅读框的3'末端,并在一步中解除了转录本的翻译阻断。这种翻译阻断是由非常规内含子的一部分与5'-非翻译区(5'UTR)的碱基配对引起的。在黑曲霉和其他曲霉菌中,hacA mRNA中的非常规内含子只有20 nt长。由于这个内含子是一个稳定的茎环结构的一部分,与酵母HAC1的情况相反,它与5'UTR的碱基配对是不可能的。然而,对hacA mRNA的分析揭示了一个富含GC的反向重复序列(18个碱基对)。在UPR激活后,hacA mRNA的5'UTR被截断230 nt,去除了这个反向重复序列的左半部分。这意味着与酿酒酵母HAC1的情况类似,但分两步解除翻译阻断。5'截断背后的机制,在酵母HAC1或哺乳动物xbp1 mRNA中都不会发生,迄今为止尚不清楚。在这里,我们表明在黑曲霉的分泌应激过程中,hacA转录从一个更靠近ATG的新起始位点开始,解除了转录本的翻译衰减。这种转录开关是由HacA本身和hacA启动子中的未折叠蛋白反应元件2(UPRE2)介导的。

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