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编码锌指蛋白CCCH类成员的两个酵母基因的克隆与特性分析:锌指介导的细胞生长损伤

Cloning and characterization of two yeast genes encoding members of the CCCH class of zinc finger proteins: zinc finger-mediated impairment of cell growth.

作者信息

Thompson M J, Lai W S, Taylor G A, Blackshear P J

机构信息

Howard Hughes Medical Institute Laboratories, Duke University Medical Center, Durham, NC 27710, USA.

出版信息

Gene. 1996 Oct 3;174(2):225-33. doi: 10.1016/0378-1119(96)00084-4.

Abstract

Members of the CCCH zinc finger (Zf) protein family have in common two or more repeats of a novel Zf motif consisting of Cys and His residues in the form Cx8Cx5Cx3H [where x is a variable amino acid (aa)]. We used a degenerate polymerase chain reaction (PCR) strategy to clone members of this gene family from Saccharomyces cerevisiae. The deduced aa sequences encoded by these genes, designated CTH1 and CTH2, share 46% overall identity and 59% similarity, largely due to the two highly conserved Zf domains. We found readily detectable expression of a 1.4-kb mRNA encoding Cth1p. The 1.1-kb mRNA encoding Cth2p was barely detectable under normal growth conditions; however, disruption of CTH1 resulted in at least a threefold increase in CTH2 mRNA accumulation. No change in phenotype was detected following disruption of CTH1 and CTH2, either singly or together. In contrast, overexpression of the CTH genes or one of the related mammalian genes, tris-tetraprolin (TTP), caused delayed entry of cell cultures into exponential growth, and a decrease in final cell density. Removal of the Zf domain of Cth1p by truncation or deletion completely reversed this slow growth phenotype, indicating that it was mediated through this highly conserved structural motif.

摘要

CCCH锌指(Zf)蛋白家族的成员具有一个由Cys和His残基组成的新型Zf基序的两个或更多重复序列,其形式为Cx8Cx5Cx3H [其中x是可变氨基酸(aa)]。我们使用简并聚合酶链反应(PCR)策略从酿酒酵母中克隆该基因家族的成员。这些基因编码的推导氨基酸序列,命名为CTH1和CTH2,总体上具有46%的同一性和59%的相似性,这主要归因于两个高度保守的Zf结构域。我们发现很容易检测到编码Cth1p 的1.4 kb mRNA的表达。在正常生长条件下,编码Cth2p的1.1 kb mRNA几乎检测不到;然而,CTH1的破坏导致CTH2 mRNA积累至少增加三倍。单独或一起破坏CTH1和CTH2后,未检测到表型变化。相比之下,CTH基因或相关哺乳动物基因之一三磷酸四脯氨酸(TTP)的过表达导致细胞培养物进入指数生长的延迟以及最终细胞密度的降低。通过截短或缺失去除Cth1p的Zf结构域完全逆转了这种缓慢生长表型,表明它是通过这个高度保守的结构基序介导的。

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