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Splicing factor SUP-12 and the molecular complexity of apparent cooperativity

机译:剪接因子SUP-12和表观协同性的分子复杂性

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摘要

The splicing factor SUP-12 from C. elegans, in combination with either ASD-1 or FOX-1 from the Fox-1 (RBFOX) family, is required for generating a muscle-specific isoform of the fibroblast growth factor receptor EGL-15. Biophysical techniques have revealed the sequence preference for the RNA Recognition Motif (RRM) domain from SUP-12 as well as the structural details of the RNA-bound complex. Detailed genetics have identified a requisite need for the presence of both SUP-12 and ASD-1/FOX-1 to regulate the alternative splicing event, prompting speculation of a cooperative mechanism between these proteins on binding RNA. In contrast, the interplay between SUP-12 and ASD-1 suggests that although the RRM domains from each protein are in direct contact on the egl-15 pre-mRNA, there is no simple contribution of binding cooperativity. Evidence for an independent binding mechanism by SUP-12 and ASD-1 will be discussed, including a model in which both positive and negative contributions are balanced during complex assembly. The ability to monitor tissue-specific alternative splicing in live nematodes will continue to provide a powerful method to test in vivo mechanistic models derived from atomic-level investigation.
机译:秀丽隐杆线虫的剪接因子SUP-12与Fox-1(RBFOX)家族的ASD-1或FOX-1结合在一起是生成成纤维细胞生长因子受体EGL-15的肌肉特异性同工型所必需的。生物物理技术已经揭示了来自SUP-12的RNA识别基序(RRM)域的序列偏好以及RNA结合复合物的结构细节。详细的遗传学已经确定了同时存在SUP-12和ASD-1 / FOX-1来调节选择性剪接事件的必要需求,从而促使人们推测这些蛋白质之间在结合RNA上的协同机制。相反,SUP-12和ASD-1之间的相互作用表明,尽管每种蛋白质的RRM结构域都直接与egl-15 pre-mRNA接触,但结合合作性并没有简单的贡献。将讨论由SUP-12和ASD-1建立独立结合机制的证据,包括一个模型,该模型在复杂组装过程中平衡了正负贡献。监视活线虫中组织特异性替代剪接的能力将继续提供强大的方法来测试源自原子水平研究的体内机制模型。

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