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Nmd2p与Upf1p之间的相互作用对于酵母中无义介导的mRNA降解途径的活性是必需的,但对于其显性负性抑制作用则不是必需的。

Interaction between Nmd2p and Upf1p is required for activity but not for dominant-negative inhibition of the nonsense-mediated mRNA decay pathway in yeast.

作者信息

He F, Brown A H, Jacobson A

机构信息

Department of Molecular Genetics and Microbiology, University of Massachusetts Medical School, Worcester 01655-0122, USA.

出版信息

RNA. 1996 Feb;2(2):153-70.

Abstract

Rapid turnover of nonsense-containing mRNAs in the yeast Saccharomyces cerevisiae is dependent on the products of the UPF1 (Upf1p), NMD2/UPF2 (Nmd2p) and UPF3 (Upf3p) genes. Mutations in each of these genes lead to the selective stabilization of mRNAs containing early nonsense mutations without affecting the decay rates of most other mRNAs. NMD2 was recently identified in a two-hybrid screen as a gene that encodes a Upf1p-interacting protein. To identify the amino acids essential to this interaction, we used two-hybrid analysis as well as missense, nonsense, and deletion mutants of NMD2, and mapped the Upf1p-interacting domain of Nmd2p to a 157-amino acid segment at its C-terminus. Mutations in this domain that disrupt interaction with Upf1p also disrupt nonsense-mediated mRNA decay. A dominant-negative deletion allele of NMD2 identified previously includes the Upf1p-interacting domain. However, mutations in the Upf1p-interacting domain do not affect dominant-negative inhibition of mRNA decay caused by this allele, suggesting interaction with yet another factor. These results, and the observation that deletion of a putative nuclear localization signal and a putative transmembrane domain also inactivate nonsense-mediated mRNA decay, suggest that Nmd2p may contain as many as four important functional domains.

摘要

酿酒酵母中含无义密码子的信使核糖核酸(mRNA)的快速周转依赖于UPF1(Upf1p)、NMD2/UPF2(Nmd2p)和UPF3(Upf3p)基因的产物。这些基因中的每一个发生突变都会导致含有早期无义突变的mRNA被选择性稳定,而不会影响大多数其他mRNA的降解速率。NMD2最近在双杂交筛选中被鉴定为一个编码与Upf1p相互作用蛋白的基因。为了确定这种相互作用所必需的氨基酸,我们使用了双杂交分析以及NMD2的错义、无义及缺失突变体,并将Nmd2p与Upf1p相互作用的结构域定位到其C末端的一个157个氨基酸的片段上。该结构域中破坏与Upf1p相互作用的突变也会破坏无义介导的mRNA降解。先前鉴定的NMD2的一个显性负性缺失等位基因包含与Upf1p相互作用的结构域。然而,与Upf1p相互作用结构域中的突变并不影响由该等位基因引起的mRNA降解的显性负性抑制,这表明它与另一个因子相互作用。这些结果,以及观察到删除一个假定的核定位信号和一个假定的跨膜结构域也会使无义介导的mRNA降解失活,表明Nmd2p可能包含多达四个重要的功能结构域。

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