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The promoter region of the yeast KAR2 (BiP) gene contains a regulatory domain that responds to the presence of unfolded proteins in the endoplasmic reticulum.

机译:酵母KAR2(BiP)基因的启动子区域包含一个调节域该域响应内质网中未折叠蛋白的存在。

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摘要

The endoplasmic reticulum (ER) of eukaryotic cells contains an abundant 78,000-Da protein (BiP) that is involved in the translocation, folding, and assembly of secretory and transmembrane proteins. In the yeast Saccharomyces cerevisiae, as in mammalian cells, BiP mRNA is synthesized at a high basal rate and is further induced by the presence of increased amounts of unfolded proteins in the ER. However, unlike mammalian BiP, yeast BiP is also induced severalfold by heat shock, albeit in a transient fashion. To identify the regulatory sequences that respond to these stimuli in the yeast KAR2 gene that encodes BiP, we have cloned a 1.3-kb segment of DNA from the region upstream of the sequences coding for BiP and fused it to a reporter gene, the Escherichia coli beta-galactosidase gene. Analysis of a series of progressive 5' truncations as well as internal deletions of the upstream sequence showed that the information required for accurate transcriptional regulation of the KAR2 gene in S. cerevisiae is contained within a approximately 230-bp XhoI-DraI fragment (nucleotides -245 to -9) and that this fragment contains at least two cis-acting elements, one (heat shock element [HSE]) responding to heat shock and the other (unfolded protein response element [UPR]) responding to the presence of unfolded proteins in the ER. The HSE and UPR elements are functionally independent of each other but work additively for maximum induction of the yeast KAR2 gene. Lying between these two elements is a GC-rich region that is similar in sequence to the consensus element for binding of the mammalian transcription factor Sp1 and that is involved in the basal expression of the KAR2 gene. Finally, we provide evidence suggesting that yeast cells monitor the concentration of free BiP in the ER and adjust the level of transcription of the KAR2 gene accordingly; this effect is mediated via the UPR element in the KAR2 promoter.
机译:真核细胞的内质网(ER)包含丰富的78,000-Da蛋白(BiP),该蛋白参与分泌蛋白和跨膜蛋白的移位,折叠和组装。在酵母酿酒酵母中,如在哺乳动物细胞中一样,BiP mRNA以高基础速率合成,并且由于内质网中未折叠蛋白数量的增加而进一步被诱导。但是,与哺乳动物的BiP不同,酵母BiP也会被热激诱导数倍,尽管是短暂的。为了鉴定对编码BiP的酵母KAR2基因中的这些刺激有反应的调控序列,我们从编码BiP的序列上游区域克隆了一个1.3 kb的DNA片段,并将其融合到报告基因大肠杆菌中。 β-半乳糖苷酶基因。对一系列进行性5'截短以及上游序列内部缺失的分析表明,啤酒酵母中KAR2基因的准确转录调控所需的信息包含在大约230 bp的XhoI-DraI片段中(核苷酸- 245至-9),并且该片段至少包含两个顺式作用元件,一个(热激元件[HSE])响应热激,另一个(未折叠蛋白反应元件[UPR])响应未折叠蛋白的存在在急诊室。 HSE和UPR元件在功能上彼此独立,但可加在一起发挥作用,以最大程度地诱导酵母KAR2基因。位于这两个元件之间的是一个富含GC的区域,该区域的序列与结合哺乳动物转录因子Sp1的共有元件序列相似,并且参与了KAR2基因的基础表达。最后,我们提供的证据表明酵母细胞可监测ER中游离BiP的浓度并相应地调节KAR2基因的转录水平。这种作用是通过KAR2启动子中的UPR元件介导的。

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