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作 者:陈献华[1] 李静[1] 林万敏[1] 吴琨[1] 徐平[1]
机构地区:[1]复旦大学生命科学院基因生理学研究室,上海200433
出 处:《实验生物学报》2004年第2期109-117,共9页Acta Biologiae Experimentalis Sinica
基 金:国家自然科学基金(No.30070242)
摘 要:体外(in vitro)生化研究已证明哺乳动物Tra2蛋白是前体mRNA剪接的重要调控因子,但是,对该蛋白在in vivo条件下的剪接功能,尤其是在神经特异性基因剪接中的功能及其细胞特异性,目前所知甚少。本文采用in vivo分析模型,在COS-1和PFSK两种不同类型的细胞中,研究了两个神经特异性基因(GluR-B,SMN2)剪接的细胞特异性,同时分析了Tra2β1在这两个基因剪接中的功能及其细胞特异性。结果表明,在研究的两种细胞中,GluR-B和SMN2“小基因”的剪接均具有明显的细胞特异性;而Tra2β1蛋白的过量表达在这两种不同的细胞中对“小基因”的剪接有显著的相同倾向的调节作用,提示Tra2β1蛋白对该两个基因剪接的调节作用可能没有细胞特异性。The in vitro studies have shown that Tra2β1 proteins are important regulators in the alternative pre-mRNA splicing in mammalians. To date, the knowledge regarding the in vivo function of Tra2β1 proteins, especially the function in regulating the splicing of neural-specific genes and the cell-type specificity of the functions is very limited. In the present study, the cell-type specific splicing of two neural-specific genes (GluR-B and SMN2), and the function of Tra2β1 proteins in regulation of the splicing were studied in two types of cells (COS-1 and PFSK-1) using in vivo splicing models. The results showed that the splicing of GluR-B and SMN2 minigenes is cell-type specific, while Tra2β1 proteins regulate the splicing of the minigenes in both cell lines in a similar pattern. It indicates that the Tra2β1 -regulated splicing of GluR-B and SMN2 minigenes regulated by Tra2β1 is not cell-type specific.
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