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首页> 外文期刊>Genetics: A Periodical Record of Investigations Bearing on Heredity and Variation >Genetic Interactions With CLF1 Identify Additional Pre-mRNA Splicing Factors and a Link Between Activators of Yeast Vesicular Transport and Splicing
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Genetic Interactions With CLF1 Identify Additional Pre-mRNA Splicing Factors and a Link Between Activators of Yeast Vesicular Transport and Splicing

机译:与CLF1的遗传相互作用确定了额外的前mRNA剪接因子以及酵母囊泡运输和剪接激活剂之间的联系。

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Clf1 is a conserved spliceosome assembly factor composed predominately of TPR repeats. Here we show that the TPR elements are not functionally equivalent, with the amino terminus of Clf1 being especially sensitive to change. Deletion and add-back experiments reveal that the splicing defect associated with TPR removal results from the loss of TPR-specific sequence information. Twelve mutants were found that show synthetic growth defects when combined with an allele that lacks TPR2 ( i.e., clf1 Δ 2 ). The identified genes encode the Mud2, Ntc20, Prp16, Prp17, Prp19, Prp22, and Syf2 splicing factors and four proteins without established contribution to splicing (Bud13, Cet1, Cwc2, and Rds3). Each s ynthetic l ethal with clf1 Δ 2 ( slc ) mutant is splicing defective in a wild-type CLF1 background. In addition to the splicing factors, SSD1, BTS1 , and BET4 were identified as dosage suppressors of clf1 Δ 2 or selected slc mutants. These results support Clf1 function through multiple stages of the spliceosome cycle, identify additional genes that promote cellular mRNA maturation, and reveal a link between Rab/Ras GTPase activation and the process of pre-mRNA splicing.
机译:Clf1是一个保守的剪接体组装因子,主要由TPR重复序列组成。在这里,我们显示TPR元件在功能上不相同,而Clf1的氨基末端对变化特别敏感。删除和回加实验表明,与TPR去除相关的剪接缺陷是由TPR特异性序列信息的丢失引起的。发现有十二个突变体与缺乏TPR2(即​​clf1Δ2)的等位基因结合时显示出合成的生长缺陷。鉴定出的基因编码Mud2,Ntc20,Prp16,Prp17,Prp19,Prp22和Syf2剪接因子以及四种对剪接没有贡献的蛋白质(Bud13,Cet1,Cwc2和Rds3)。每个带有clf1Δ2(slc)突变体的合成蛋白在野生型CLF1背景中均剪接有缺陷。除剪接因子外,SSD1,BTS1和BET4还被确定为clf1Δ2或选定的slc突变体的剂量抑制剂。这些结果在剪接体循环的多个阶段支持Clf1功能,鉴定促进细胞mRNA成熟的其他基因,并揭示Rab / Ras GTPase活化与mRNA前剪接过程之间的联系。

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