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酵母UPF1基因的产物是含有提前翻译终止密码子的mRNA快速周转所必需的。

The product of the yeast UPF1 gene is required for rapid turnover of mRNAs containing a premature translational termination codon.

作者信息

Leeds P, Peltz S W, Jacobson A, Culbertson M R

机构信息

Laboratories of Genetics and Molecular Biology, University of Wisconsin, Madison 53706.

出版信息

Genes Dev. 1991 Dec;5(12A):2303-14. doi: 10.1101/gad.5.12a.2303.

Abstract

mRNA decay rates often increase when translation is terminated prematurely due to a frameshift or nonsense mutation. We have identified a yeast gene, UPF1, that codes for a trans-acting factor whose function is necessary for enhanced turnover of mRNAs containing a premature stop codon. In the absence of UPF1 function, frameshift or nonsense mutations in the HIS4 or LEU2 genes that normally cause rapid mRNA decay fail to have this effect. Instead, the mRNAs decay at rates similar to the corresponding wild-type mRNAs. The stabilization of frameshift or nonsense mRNAs observed in upf1- strains does not appear to result from enhanced readthrough of the termination signal. Loss of UPF1 function has no effect on the accumulation or stability of HIS4+ or LEU2+ mRNA, suggesting that the UPF1 product functions only in response to a premature termination signal. When we examined the accumulation and stability of other wild-type mRNAs in the presence or absence of UPF1, including MAT alpha 1, STE3, ACT1, PGK1, PAB1, and URA3 mRNAs, only the URA3 transcript was affected. On the basis of these and other results, the UPF1 product appears to participate in a previously uncharacterized pathway leading to the degradation of a limited class of yeast transcripts.

摘要

当由于移码突变或无义突变导致翻译提前终止时,mRNA的降解速率通常会增加。我们已经鉴定出一个酵母基因UPF1,它编码一种反式作用因子,其功能对于含有提前终止密码子的mRNA的增强周转是必需的。在缺乏UPF1功能的情况下,通常会导致mRNA快速降解的HIS4或LEU2基因中的移码突变或无义突变无法产生这种效果。相反,这些mRNA以与相应野生型mRNA相似的速率降解。在upf1-菌株中观察到的移码或无义mRNA的稳定化似乎不是由于终止信号的通读增强所致。UPF1功能的丧失对HIS4+或LEU2+ mRNA的积累或稳定性没有影响,这表明UPF1产物仅在响应提前终止信号时起作用。当我们在有或没有UPF1的情况下检查其他野生型mRNA的积累和稳定性时,包括MAT alpha 1、STE3、ACT1、PGK1、PAB1和URA3 mRNA,只有URA3转录本受到影响。基于这些及其他结果,UPF1产物似乎参与了一条以前未被描述的途径,该途径导致一类有限的酵母转录本的降解。

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