Kawahara T, Yanagi H, Yura T, Mori K
HSP Research Institute, Kyoto Research Park, Japan.
Mol Biol Cell. 1997 Oct;8(10):1845-62. doi: 10.1091/mbc.8.10.1845.
An intracellular signaling from the endoplasmic reticulum (ER) to the nucleus, called the unfolded protein response (UPR), is activated when unfolded proteins are accumulated in the ER under a variety of stress conditions ("ER stress"). We and others recently identified Hac1p/Ern4p as a transcription factor responsible for the UPR in Saccharomyces cerevisiae. It was further reported that Hac1p (238 aa) is detected only in ER-stressed cells, and its expression is mediated by unconventional splicing of HAC1 precursor mRNA. The splicing replaces the C-terminal portion of Hac1p; it was proposed that precursor mRNA is also translated but the putative product of 230 aa is rapidly degraded by the ubiquitin-proteasome pathway. We have identified and characterized the same regulated splicing and confirmed its essential features. Contrary to the above proposal, however, we find that the 238-aa product of mature mRNA and the 230-aa-type protein tested are highly unstable with little of no difference in stability. Furthermore, we demonstrate that the absence of Hac1p in unstressed cells is due to the lack of translation of precursor mRNA. We conclude that Hac1p is synthesized as the result of ER stress-induced mRNA splicing, leading to activation of the UPR.
在内质网(ER)与细胞核之间存在一种细胞内信号传导,称为未折叠蛋白反应(UPR),当未折叠蛋白在各种应激条件下(“内质网应激”)在内质网中积累时,该反应被激活。我们和其他研究人员最近鉴定出Hac1p/Ern4p是酿酒酵母中负责UPR的转录因子。进一步报道称,仅在内质网应激的细胞中才能检测到Hac1p(238个氨基酸),其表达是由HAC1前体mRNA的非常规剪接介导的。这种剪接替换了Hac1p的C末端部分;有人提出前体mRNA也会被翻译,但推测的230个氨基酸的产物会被泛素-蛋白酶体途径迅速降解。我们已经鉴定并表征了相同的调控剪接,并证实了其基本特征。然而,与上述提议相反,我们发现成熟mRNA的238个氨基酸的产物和测试的230个氨基酸类型的蛋白质高度不稳定,稳定性几乎没有差异。此外,我们证明在未受应激的细胞中不存在Hac1p是由于前体mRNA缺乏翻译。我们得出结论,Hac1p是内质网应激诱导的mRNA剪接的结果,导致UPR的激活。
