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Re-refinement of the spliceosomal U4 snRNP core-domain structure

机译:细化U4 snRNP核心域结构的重新完善。

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摘要

The core domain of small nuclear ribonucleoprotein (snRNP), comprised of a ring of seven paralogous proteins bound around a single-stranded RNA sequence, functions as the assembly nucleus in the maturation of U1, U2, U4 and U5 spliceosomal snRNPs. The structure of the human U4 snRNP core domain was initially solved at 3.6 Å resolution by experimental phasing using data with tetartohedral twinning. Molecular replacement from this model followed by density modification using untwinned data recently led to a structure of the minimal U1 snRNP at 3.3 Å resolution. With the latter structure providing a search model for molecular replacement, the U4 core-domain structure has now been re-refined. The U4 Sm site-sequence AAUUUUU has been shown to bind to the seven Sm proteins SmF–SmE–SmG–SmD3–SmB–SmD1–SmD2 in an identical manner as the U1 Sm-site sequence AAUUUGU, except in SmD1 where the bound U replaces G. The progression from the initial to the re-refined structure exemplifies a tortuous route to accuracy: where well diffracting crystals of complex assemblies are initially unavailable, the early model errors are rectified by exploiting preliminary interpretations in further experiments involving homologous structures. New insights are obtained from the more accurate model.
机译:小核糖核蛋白(snRNP)的核心结构域由围绕单链RNA序列结合的七个旁源蛋白的环组成,在U1,U2,U4和U5剪接snRNPs成熟中起装配核的作用。人四联体snRNP核心结构域的结构最初是通过四相四面体孪晶数据通过实验定相以3.6Å分辨率解决的。从该模型进行分子置换,然后使用未保存的数据进行密度修改,最近导致了在3.3Å分辨率下最小的U1 snRNP的结构。借助后者的结构提供了分子替代的搜索模型,U4核心结构域结构现已得到重新完善。已显示,U4 Sm位点序列AAUUUUU以与U1 Sm位点序列AAUUUGU相同的方式与七种Sm蛋白SmF–SmE–SmG–SmD3–SmB–SmD1–SmD2结合,但在SmD1中结合的U从最初的结构转变为精确的结构代表了通往准确性的曲折道路:在最初无法获得复杂组装的良好衍射晶体的情况下,可以通过在涉及同源结构的进一步实验中利用初步解释来纠正早期的模型错误。从更准确的模型中可以获得新的见解。

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