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去腺苷酸化的机制与调控:非洲爪蟾PARN的鉴定与表征

The mechanism and regulation of deadenylation: identification and characterization of Xenopus PARN.

作者信息

Copeland P R, Wormington M

机构信息

Department of Biology, University of Virginia, Charlottesville 22903, USA.

出版信息

RNA. 2001 Jun;7(6):875-86. doi: 10.1017/s1355838201010020.

Abstract

In Xenopus oocytes, the deadenylation of a specific class of maternal mRNAs results in their translational repression. Here we report the purification, characterization, and molecular cloning of the Xenopus poly(A) ribonuclease (xPARN). xPARN copurifies with two polypeptides of 62 kDa and 74 kDa, and we provide evidence that the 62-kDa protein is a proteolytic product of the 74-kDa protein. We have isolated the full-length xPARN cDNA, which contains the tripartite exonuclease domain conserved among RNase D family members, a putative RNA recognition motif, and a domain found in minichromosome maintenance proteins. Characterization of the xPARN enzyme shows that it is a poly(A)-specific 3' exonuclease but does not require an A residue at the 3' end. However, the addition of 25 nonadenylate residues at the 3' terminus, or a 3' terminal phosphate is inhibitory. Western analysis shows that xPARN is expressed throughout early development, suggesting that it may participate in the translational silencing and destabilization of maternal mRNAs during both oocyte maturation and embryogenesis. In addition, microinjection experiments demonstrate that xPARN can be activated in the oocyte nucleus in the absence of cytoplasmic components and that nuclear export of deadenylated RNA is impeded. Based on the poly(A) binding activity of xPARN in the absence of catalysis, a model for substrate specificity is proposed.

摘要

在非洲爪蟾卵母细胞中,一类特定的母源mRNA的去腺苷酸化导致其翻译抑制。在此,我们报告了非洲爪蟾聚(A)核糖核酸酶(xPARN)的纯化、特性鉴定及分子克隆。xPARN与62 kDa和74 kDa的两种多肽共同纯化,并且我们提供证据表明62 kDa的蛋白质是74 kDa蛋白质的蛋白水解产物。我们分离出了全长的xPARN cDNA,其包含在核糖核酸酶D家族成员中保守的三联体外切核酸酶结构域、一个推定的RNA识别基序以及在微型染色体维持蛋白中发现的一个结构域。对xPARN酶的特性鉴定表明它是一种聚(A)特异性3'外切核酸酶,但不需要3'端有A残基。然而,在3'末端添加25个非腺苷酸残基或一个3'末端磷酸是有抑制作用的。蛋白质免疫印迹分析表明xPARN在整个早期发育过程中都有表达,这表明它可能在卵母细胞成熟和胚胎发生过程中参与母源mRNA的翻译沉默和去稳定化。此外,显微注射实验表明,在没有细胞质成分的情况下,xPARN可以在卵母细胞核中被激活,并且去腺苷酸化RNA的核输出受到阻碍。基于xPARN在无催化情况下的聚(A)结合活性,提出了一个底物特异性模型。

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