首页> 美国卫生研究院文献>The EMBO Journal >Evidence for a Prp24 binding site in U6 snRNA and in a putative intermediate in the annealing of U6 and U4 snRNAs.
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Evidence for a Prp24 binding site in U6 snRNA and in a putative intermediate in the annealing of U6 and U4 snRNAs.

机译:在U6和U4 snRNA退火中,在U6 snRNA和推定的中间体中存在Prp24结合位点的证据。

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摘要

A mutation (U4-G14C) that destabilizes the base-pairing interaction between U4 and U6 snRNAs causes the accumulation of a novel complex containing U4, U6 and Prp24, a protein with RNA binding motifs. An analysis of suppressors of this cold-sensitive mutant led to the hypothesis that this complex is normally a transient intermediate in the annealing of U4 and U6. It was proposed that Prp24 must be released to form a fully base-paired U4/U6 snRNP. By using a chemical probing method we have tested the prediction that nucleotides A40-C43 in U6 mediate the binding of Prp24. Consistent with the location of recessive suppressors in U6, we find that residues A40-C43 are protected from chemical modification in U4/U6 complexes from the U4-G14C mutant but not from the wild-type or suppressor strains carrying mutations in U6 or PRP24. Furthermore, we find that base-pairing is substantially disrupted in the mutant complexes. Notably, the base-paired structure is restored in recessive suppressors despite the presence of a mismatched base-pair at the U4-G14C site. Our results support the model that Prp24 binds to U6 to promote its association with U4, but must dissociate to allow complete annealing.
机译:使U4和U6 snRNA之间的碱基配对相互作用不稳定的突变(U4-G14C)导致含有U4,U6和Prp24(一种具有RNA结合基序的蛋白质)的新型复合物的积累。对这种冷敏突变体的抑制子的分析导致了这样的假设,即该复合物通常是U4和U6退火中的瞬时中间体。提出必须释放Prp24以形成完全碱基配对的U4 / U6 snRNP。通过使用化学探测方法,我们测试了U6中核苷酸A40-C43介导Prp24结合的预测。与U6中隐性抑制子的位置一致,我们发现残基A40-C43受到保护,不受U4-G14C突变体的U4 / U6复合物中的化学修饰,但不受野生型或携带U6或PRP24突变的抑制株的化学修饰。此外,我们发现碱基对在突变体复合物中被破坏了。值得注意的是,尽管在U4-G14C位点存在不匹配的碱基对,但在隐性抑制子中碱基对的结构得以恢复。我们的结果支持Prp24与U6结合以促进其与U4缔合的模型,但必须解离以允许完全退火。

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