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Metal ion catalysis during splicing of premessenger RNA

机译:信使RNA剪接过程中的金属离子催化

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The removal of intervening sequences from premessenger RNA is essential for the expression of most eukaryotic genes. The spliceosome ribonucleoprotein complex catalyses intron removal by two sequential phosphotransesterification reactions, but the catalytic mechanisms are unknown. It has been proposed that two divalent metal ions may mediate catalysis of both reaction steps, activating the 2'- or 3'-hydroxyl groups for nucleophilic attack and stabilizing the 3'-oxyanion leaving groups by direct coordination. Here we show that in splicing reactions with a precursor RNA containing a 3'-sulphur substitution at the 5' splice site, interaction between metal ion and leaving group is essential for catalysis of the first reaction step. This establishes that the spliceosome is a metalloenzyme and demonstrates a direct parallel with the catalytic strategy used by the self-splicing group I intron from Tetrahymena. In contrast, 3'-sulphur substitution at the 3' splice site provides no evidence for a metal ion-leaving group interaction in the second reaction step, suggesting that the two steps of splicing proceed by different catalytic mechanisms and therefore in distinct active sites.
机译:从前信使RNA中去除插入序列对于大多数真核基因的表达是必不可少的。剪接体核糖核蛋白复合物通过两个连续的磷酸酯交换反应催化内含子的去除,但是催化机理尚不清楚。已经提出,两个二价金属离子可介导两个反应步骤的催化,活化2'-或3'-羟基用于亲核攻击并通过直接配位稳定3'-氧阴离子离去基团。在这里,我们显示在与在5'剪接位点包含3'-硫取代的前体RNA进行剪接反应时,金属离子和离去基团之间的相互作用对于第一步反应的催化至关重要。这证明剪接体是金属酶,并证明与四膜虫的自剪接基团I内含子所使用的催化策略直接平行。相反,在3'剪接位点的3'-硫取代没有提供第二反应步骤中金属离子离去基团相互作用的证据,表明剪接的两个步骤通过不同的催化机理进行,因此在不同的活性位点进行。

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