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普遍表达的不均一核糖核蛋白F参与了神经特异性前体mRNA剪接事件。

The generally expressed hnRNP F is involved in a neural-specific pre-mRNA splicing event.

作者信息

Min H, Chan R C, Black D L

机构信息

Molecular Biology Institute, University of California at Los Angeles 90024-1662, USA.

出版信息

Genes Dev. 1995 Nov 1;9(21):2659-71. doi: 10.1101/gad.9.21.2659.

DOI:10.1101/gad.9.21.2659
PMID:7590243
Abstract

The proteins and RNA regulatory elements that control tissue-specific pre-mRNA splicing in mammalian cells are mostly unknown. In this study, a set of proteins is identified that binds to a splicing regulatory element downstream of the neuron specific c-src N1 exon. This complex of proteins bound specifically to a short RNA containing the regulatory sequence in neuronal extracts that splice the N1 exon. It was not seen in non-neuronal cell extracts that fail to splice this exon. UV-cross-linking experiments identified a neuron-specific 75-kD protein and several nontissue-specific proteins, including the 53-kD heterogeneous nuclear ribonucleoprotein F (hnRNP F), as components of this complex. Although present in both extracts, hnRNP F binds tightly to the RNA only in the neuronal extracts. A mutation in the regulatory RNA sequence, that inhibits N1 splicing in vivo, abolished formation of the neuron-specific complex and the binding of the neuron-specific 75-kD protein. Competition experiments in the two extracts show that the binding of the neuronal protein complex to the src pre-mRNA is required to activate N1 exon splicing in vitro. Antibody inhibition experiments indicate that the hnRNP F protein is a functional part of this complex. The assembly of regulatory complexes from both constitutive and specific proteins is likely to be a general feature of tissue-specific splicing regulation.

摘要

在哺乳动物细胞中,控制组织特异性前体mRNA剪接的蛋白质和RNA调控元件大多未知。在本研究中,鉴定出一组与神经元特异性c-src N1外显子下游的剪接调控元件结合的蛋白质。这种蛋白质复合物在剪接N1外显子的神经元提取物中特异性地结合到含有调控序列的短RNA上。在不能剪接该外显子的非神经元细胞提取物中未观察到这种复合物。紫外线交联实验确定了一种神经元特异性的75-kD蛋白质和几种非组织特异性蛋白质,包括53-kD异质性核核糖核蛋白F(hnRNP F),作为该复合物的组成成分。虽然在两种提取物中都存在,但hnRNP F仅在神经元提取物中紧密结合RNA。调控RNA序列中的一个突变,在体内抑制N1剪接,消除了神经元特异性复合物的形成以及神经元特异性75-kD蛋白质的结合。在两种提取物中的竞争实验表明,神经元蛋白质复合物与src前体mRNA的结合是体外激活N1外显子剪接所必需的。抗体抑制实验表明,hnRNP F蛋白是该复合物的功能组成部分。由组成型和特异性蛋白质组装调控复合物可能是组织特异性剪接调控的一个普遍特征。

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