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酵母TRP4基因中的一个单点突变会影响mRNA 3'末端加工的效率,并改变聚腺苷酸化位点的选择。

A single point mutation in the yeast TRP4 gene affects efficiency of mRNA 3' end processing and alters selection of the poly(A) site.

作者信息

Düvel K, Egli C M, Braus G H

机构信息

Institute of Microbiology and Genetics, Georg-August-University, Grisebachstrasse 8, D-37077 Göttingen, Germany.

出版信息

Nucleic Acids Res. 1999 Mar 1;27(5):1289-95. doi: 10.1093/nar/27.5.1289.

Abstract

The yeast TRP4 mRNA 3' end formation element is a bidirectional element which functions in both orien-tations in an artificial in vivo test system. In this study, the role of 3' end formation was analysed in the context of the entire TRP4 gene. The 3' untranslated region (3'UTR) of TRP4 was altered and changes were analysed for their influence on TRP4 gene expression. The 3'UTR in reverse orientation was fully functional and did not affect TRP4 gene expression. Exchanging the TRP4 3'UTR by the bidirectional ARO4 or the unidirectional GCN4 3' end formation element allowed efficient gene expression. Deletion of the entire TRP4 3'UTR resulted in 70% reduction of TRP4 mRNA and 50% reduced specific Trp4 enzyme activity in comparison to wild-type. A single point mutation within the TRP4 3'UTR caused the same effect on gene expression. This point mutation did not only affect the efficiency of 3' end formation, but also produced new poly(A) sites which were situated upstream of the wild-type poly(A) sites. Therefore this sequence motif in the TRP4 3'UTR acts simultaneously as both an efficiency and positioning element.

摘要

酵母TRP4 mRNA 3'端形成元件是一种双向元件,在人工体内测试系统中,无论其处于何种方向均能发挥作用。在本研究中,我们在整个TRP4基因的背景下分析了3'端形成的作用。改变了TRP4的3'非翻译区(3'UTR),并分析了这些变化对TRP4基因表达的影响。反向的3'UTR功能完全正常,且不影响TRP4基因表达。用双向的ARO4或单向的GCN4 3'端形成元件替换TRP4的3'UTR,可实现高效的基因表达。与野生型相比,删除整个TRP4 3'UTR导致TRP4 mRNA减少70%,Trp4酶的比活性降低50%。TRP4 3'UTR内的一个单点突变对基因表达产生了相同的影响。该点突变不仅影响3'端形成的效率,还产生了位于野生型聚腺苷酸化位点上游的新聚腺苷酸化位点。因此,TRP4 3'UTR中的这个序列基序同时作为效率元件和定位元件发挥作用。

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