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核因子TDP - 43和SR蛋白促进体外和体内CFTR基因第9外显子跳跃。

Nuclear factor TDP-43 and SR proteins promote in vitro and in vivo CFTR exon 9 skipping.

作者信息

Buratti E, Dörk T, Zuccato E, Pagani F, Romano M, Baralle F E

机构信息

International Centre for Genetic Engineering and Biotechnology (ICGEB), Padriciano 99, 34012 Trieste, Italy.

出版信息

EMBO J. 2001 Apr 2;20(7):1774-84. doi: 10.1093/emboj/20.7.1774.

Abstract

Alternative splicing of human cystic fibrosis transmembrane conductance regulator (CFTR) exon 9 is regulated by a combination of cis-acting elements distributed through the exon and both flanking introns (IVS8 and IVS9). Several studies have identified in the IVS8 intron 3' splice site a regulatory element that is composed of a polymorphic (TG)m(T)n repeated sequence. At present, no cellular factors have been identified that recognize this element. We have identified TDP-43, a nuclear protein not previously described to bind RNA, as the factor binding specifically to the (TG)m sequence. Transient TDP-43 overexpression in Hep3B cells results in an increase in exon 9 skipping. This effect is more pronounced with concomitant overexpression of SR proteins. Antisense inhibition of endogenous TDP-43 expression results in increased inclusion of exon 9, providing a new therapeutic target to correct aberrant splicing of exon 9 in CF patients. The clinical and biological relevance of this finding in vivo is demonstrated by our characterization of a CF patient carrying a TG10T9(DeltaF508)/TG13T3(wt) genotype leading to a disease-causing high proportion of exon 9 skipping.

摘要

人类囊性纤维化跨膜传导调节因子(CFTR)外显子9的可变剪接受分布于该外显子及其两侧内含子(IVS8和IVS9)中的顺式作用元件组合调控。多项研究在IVS8内含子的3'剪接位点鉴定出一个由多态性(TG)m(T)n重复序列组成的调控元件。目前,尚未鉴定出识别该元件的细胞因子。我们已鉴定出TDP - 43,一种此前未被描述为可结合RNA的核蛋白,作为特异性结合(TG)m序列的因子。在Hep3B细胞中瞬时过表达TDP - 43会导致外显子9跳跃增加。伴随SR蛋白的过表达,这种效应更为明显。对内源性TDP - 43表达进行反义抑制会导致外显子9的包含增加,为纠正CF患者中外显子9的异常剪接提供了一个新的治疗靶点。我们对一名携带TG10T9(ΔF508)/TG13T3(野生型)基因型的CF患者进行了表征,该基因型导致致病的高比例外显子9跳跃,从而证明了这一发现在体内的临床和生物学相关性。

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