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富含脯氨酸外显子的差异剪接插入将αNAC转化为肌肉特异性转录因子。

Differential splicing-in of a proline-rich exon converts alphaNAC into a muscle-specific transcription factor.

作者信息

Yotov W V, St-Arnaud R

机构信息

Genetics Unit, Shriners Hospital, Montréal, Québec, Canada.

出版信息

Genes Dev. 1996 Jul 15;10(14):1763-72. doi: 10.1101/gad.10.14.1763.

DOI:10.1101/gad.10.14.1763
PMID:8698236
Abstract

NAC (nascent polypeptide-associated complex) was recently purified as an alpha/beta heterodimeric complex binding the newly synthesized polypeptide chains as they emerge from the ribosome. We have identified, cloned, and characterized a muscle-specific isoform of alphaNAC. The 7.0-kb mRNA arises from differential splicing-in of a 6.0 kb-exon giving rise to a proline-rich isoform that we termed skNAC. The skNAC protein was specifically expressed in differentiated myotubes but not in myoblasts. We have identified a specific DNA binding site for skNAC and shown that it can activate transcription through that element. The murine myoglobin promoter contains three putative skNAC-binding sites. skNAC was shown to activate transcription from the myoglobin promoter, and site-specific mutation of the skNAC response elements abrogated skNAC-dependent activation. We also examined the role of the NAC isoforms in the myogenic program. Whereas overexpression of alphaNAC prevented C2C12 differentiation and myotube fusion, the overexpression of skNAC in C2C12 myoblasts led to early fusion of the cells into gigantic myosacs, suggesting that skNAC may be involved in normal differentiation along the myogenic lineage and in the regulation of myoblast fusion. Our data demonstrate that differential splicing converts alphaNAC into a tissue-specific DNA-binding activator and suggest that this regulation may be an important event in the proper control of gene expression during myogenic differentiation.

摘要

新生多肽相关复合体(NAC)最近被纯化出来,它是一种α/β异二聚体复合物,能在新合成的多肽链从核糖体中出现时与之结合。我们已经鉴定、克隆并表征了αNAC的一种肌肉特异性同工型。7.0 kb的mRNA源自一个6.0 kb外显子的差异剪接插入,产生了一种富含脯氨酸的同工型,我们将其命名为skNAC。skNAC蛋白在分化的肌管中特异性表达,而在成肌细胞中不表达。我们已经鉴定出skNAC的一个特定DNA结合位点,并表明它可以通过该元件激活转录。小鼠肌红蛋白启动子包含三个假定的skNAC结合位点。研究表明,skNAC可激活肌红蛋白启动子的转录,skNAC反应元件的位点特异性突变可消除skNAC依赖性激活。我们还研究了NAC同工型在成肌程序中的作用。虽然αNAC的过表达阻止了C2C12细胞的分化和肌管融合,但skNAC在C2C12成肌细胞中的过表达导致细胞早期融合形成巨大的肌囊,这表明skNAC可能参与了成肌谱系的正常分化以及成肌细胞融合的调控。我们的数据表明,差异剪接将αNAC转化为一种组织特异性的DNA结合激活剂,并表明这种调控可能是成肌分化过程中基因表达正确控制的一个重要事件。

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