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鉴定出IRAP、TAB182和人类TRF1共有的但小鼠TRF1没有的端锚聚合酶结合基序。核有丝分裂器蛋白包含这个RXXPDG基序,并且是一种新的端锚聚合酶相互作用蛋白。

Identification of a tankyrase-binding motif shared by IRAP, TAB182, and human TRF1 but not mouse TRF1. NuMA contains this RXXPDG motif and is a novel tankyrase partner.

作者信息

Sbodio Juan I, Chi Nai-Wen

机构信息

Department of Medicine, University of California San Diego, La Jolla, California 92093-0673, USA.

出版信息

J Biol Chem. 2002 Aug 30;277(35):31887-92. doi: 10.1074/jbc.M203916200. Epub 2002 Jun 21.

Abstract

Tankyrase-1 and -2 are closely related poly(ADP-ribose) polymerases that use an ankyrin-repeat domain to bind diverse proteins, including TRF (telomere-repeat binding factor)-1, IRAP (insulin-responsive aminopeptidase), and TAB182 (182-kDa tankyrase-binding protein). TRF1 binding allows tankyrase to regulate telomere dynamics in human cells, whereas IRAP binding presumably allows tankyrase to regulate the targeting of IRAP. The mechanism by which tankyrase binds to diverse proteins has not been investigated. Herein we describe a novel RXXPDG motif shared by IRAP, TAB182, and human TRF1 that mediates their binding to tankyrases. Interestingly, mouse TRF1 lacks this motif and thus does not bind either tankyrase-1 or -2. Using the ankyrin domain of tankyrase as a bait in a yeast two-hybrid screen, we also found the RXXPDG motif in six candidate tankyrase partners, including the nuclear/mitotic apparatus protein (NuMA). We verified NuMA as an RXXPDG-mediated partner of tankyrase and suggest that this interaction contributes to the known colocalization of tankyrase and NuMA at mitotic spindle poles.

摘要

端锚聚合酶-1和-2是密切相关的聚(ADP-核糖)聚合酶,它们利用锚蛋白重复结构域结合多种蛋白质,包括端粒重复结合因子(TRF)-1、胰岛素反应性氨肽酶(IRAP)和182 kDa端锚聚合酶结合蛋白(TAB182)。TRF1的结合使端锚聚合酶能够调节人类细胞中的端粒动态,而IRAP的结合可能使端锚聚合酶能够调节IRAP的靶向作用。端锚聚合酶与多种蛋白质结合的机制尚未得到研究。在此,我们描述了IRAP、TAB182和人类TRF1共有的一个新的RXXPDG基序,该基序介导它们与端锚聚合酶的结合。有趣的是,小鼠TRF1缺乏这个基序,因此不与端锚聚合酶-1或-2结合。在酵母双杂交筛选中,以端锚聚合酶的锚蛋白结构域作为诱饵,我们还在六个候选端锚聚合酶伴侣中发现了RXXPDG基序,包括核/有丝分裂装置蛋白(NuMA)。我们证实NuMA是端锚聚合酶通过RXXPDG介导的伴侣,并表明这种相互作用促成了端锚聚合酶和NuMA在有丝分裂纺锤体极的已知共定位。

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