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鹌鹑Pax-6(Pax-QNR)亚型的核定位信号、DNA结合及反式激活特性

Nuclear localization signals, DNA binding, and transactivation properties of quail Pax-6 (Pax-QNR) isoforms.

作者信息

Carrière C, Plaza S, Caboche J, Dozier C, Bailly M, Martin P, Saule S

机构信息

Centre National de la Recherche Scientifique, EP 56, Institut Pasteur de Lille, France.

出版信息

Cell Growth Differ. 1995 Dec;6(12):1531-40.

PMID:9019158
Abstract

We reported previously the characterization of Pax-QNR/Pax-6 products expressed in the avian neuroretina. Five proteins (48, 46, 43, 33, and 32 kDa) were characterized, among which the 33 and 32 kDa proteins are devoid of the paired domain. In contrast to the 48-kDa (containing an alternative paired exon 4a) and 46-kDa proteins exclusively located in the nucleus, the 43- (in which the paired exon 5 is spliced out), 33-, and 32-kDa proteins were also found in the cytoplasmic compartment. We report the identification of two nuclear targeting sequences: the basic LKRKLQR region (amino acids 206-212) located in the NH2 terminus of the homeodomain used by the p43 and 33/32 kDa proteins; and the paired exon 5 sequence. A case of human aniridia, where arginine 208 of LKRKLQR is mutated into a tryptophan, has been reported recently. We introduced this mutation into the Pax-QNR p46, p43, and p33/32 proteins. No effect on the nuclear localization or in transactivation potential of the proteins could be observed. Among the several Pax-QNR isoforms characterized, only p46 exhibited DNA-binding and transactivating properties on the Pax-QNR promoter. Deletions of parts of the protein showed that the Pax-6 transactivation domain is located in the carboxyl terminus of the protein.

摘要

我们之前报道了在鸟类神经视网膜中表达的Pax-QNR/Pax-6产物的特征。鉴定出了五种蛋白质(48、46、43、33和32 kDa),其中33 kDa和32 kDa的蛋白质缺乏配对结构域。与仅定位于细胞核中的48 kDa(包含可变配对外显子4a)和46 kDa蛋白质不同,43 kDa(其中配对外显子5被剪接掉)、33 kDa和32 kDa的蛋白质也存在于细胞质部分。我们报道了两个核定位序列的鉴定:位于p43以及33/32 kDa蛋白质所使用的同源结构域NH2末端的碱性LKRKLQR区域(氨基酸206 - 212);以及配对外显子5序列。最近报道了一例人类无虹膜病例,其中LKRKLQR的精氨酸208突变为色氨酸。我们将此突变引入Pax-QNR的p46、p43和p33/32蛋白质中。未观察到对蛋白质的核定位或反式激活潜能有影响。在所鉴定的几种Pax-QNR异构体中,只有p46对Pax-QNR启动子具有DNA结合和反式激活特性。蛋白质部分区域的缺失表明Pax-6反式激活结构域位于蛋白质的羧基末端。

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