Tiscornia G, Mahadevan M S
Laboratory of Genetics, University of Wisconsin-Madison Medical School 53706, USA.
Mol Cell. 2000 Jun;5(6):959-67. doi: 10.1016/s1097-2765(00)80261-0.
The mechanism by which (CTG)n expansion in the 3' UTR of the DMPK gene causes myotonic dystrophy (DM) is unknown. We identified four RNA splicing factors--hnRNP C, U2AF (U2 auxiliary factor), PTB (polypyrimidine tract binding protein), and PSF (PTB associated splicing factor)--that bind to two short regions 3' of the (CUG)n, and found a novel 3' DMPK exon resulting in an mRNA lacking the repeats. We propose that the (CUG)n is an essential cis acting element for this splicing event. In contrast to (CUG)n containing mRNAs, the novel isoform is not retained in the nucleus in DM cells, resulting in imbalances in relative levels of cytoplasmic DMPK mRNA isoforms and a new dominant effect of the mutation on DMPK.
DMPK基因3'非翻译区的(CTG)n扩增导致强直性肌营养不良(DM)的机制尚不清楚。我们鉴定出四种RNA剪接因子——hnRNP C、U2AF(U2辅助因子)、PTB(多嘧啶序列结合蛋白)和PSF(PTB相关剪接因子),它们与(CUG)n下游的两个短区域结合,并发现了一个新的3' DMPK外显子,导致产生一种缺乏重复序列的mRNA。我们提出,(CUG)n是这一剪接事件的必需顺式作用元件。与含有(CUG)n的mRNA不同,这种新的异构体在DM细胞中不会保留在细胞核中,导致细胞质DMPK mRNA异构体的相对水平失衡,以及该突变对DMPK产生新的显性效应。
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