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Exon and intron sequences, respectively, repress and activate splicing of a fibroblast growth factor receptor 2 alternative exon.

机译:外显子和内含子序列分别阻遏和激活成纤维细胞生长因子受体2替代性外显子的剪接。

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摘要

Two alternative exons, BEK and K-SAM, code for part of the ligand binding site of fibroblast growth factor receptor 2. Splicing of these exons is mutually exclusive, and the choice between them is made in a tissue-specific manner. We identify here pre-mRNA sequences involved in controlling splicing of the K-SAM exon. The short K-SAM exon sequence 5'-TAGGGCAGGC-3' inhibits splicing of the exon. This inhibition can be overcome by mutating either the exon's 5' or 3' splice site to make it correspond more closely to the relevant consensus sequence. Two separate sequence elements in the intron immediately downstream of the K-SAM exon, one of which is a sequence rich in pyrimidines, are both needed for efficient K-SAM exon splicing. This is no longer the case if either the exon's 5' or 3' splice site is reinforced. Furthermore, if the exon inhibitory sequence is removed, the intron sequences are not required for splicing of the K-SAM exon in a cell line which normally splices this exon. At least three elements are thus involved in controlling splicing of the K-SAM exon: suboptimal 5' and 3' splice sites, an exon inhibitory sequence, and intron activating sequences.
机译:BEK和K-SAM这两个替代外显子编码成纤维细胞生长因子受体2的部分配体结合位点。这些外显子的拼接是互斥的,它们之间的选择以组织特异性方式进行。我们在这里确定了参与控制K-SAM外显子剪接的前mRNA序列。短的K-SAM外显子序列5'-TAGGGCAGGC-3'抑制外显子的剪接。可以通过突变外显子的5'或3'剪接位点使其与相应的共有序列更接近,来克服这种抑制作用。 K-SAM外显子紧接下游的内含子中有两个独立的序列元件,其中之一是富含嘧啶的序列,都需要有效的K-SAM外显子剪接。如果外显子的5'或3'拼接位点得到增强,则不再是这种情况。此外,如果去除了外显子抑制序列,则在正常剪接该外显子的细胞系中剪接K-SAM外显子不需要内含子序列。因此,至少三个元件参与控制K-SAM外显子的剪接:次佳的5'和3'剪接位点,外显子抑制序列和内含子激活序列。

著录项

  • 作者

    Del Gatto, F; Breathnach, R;

  • 作者单位
  • 年度 1995
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  • 原文格式 PDF
  • 正文语种 en
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