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Methylation of the ribosyl moiety at position 34 of selenocysteine tRNASerSec is governed by both primary and tertiary structure.

机译:硒代半胱氨酸tRNA Ser Sec的34位核糖基部分的甲基化由一级和三级结构控制。

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摘要

The selenocysteine (Sec) tRNA[Ser]Sec population in higher vertebrates consists of two major isoacceptors that differ from each other by a single nucleoside modification in the wobble position of the anticodon (position 34). One isoacceptor contains 5-methylcarboxymethyluridine (mcmU) in this position, whereas the other contains 5-methylcarboxymethyluridine-2'-O-methylribose (mcmUm). The other modifications in these tRNAs are N6-isopentenyladenosine (i6A), pseudouridine (psi), and 1-methyladenosine (m1A) at positions 37, 55, and 58, respectively. As methylation of the ribose at position 34 is influenced by the intracellular selenium status and the presence of this methyl group dramatically alters tertiary structure, we investigated the effect of the modifications at other positions as well as tertiary structure on its formation. Mutations were introduced within a synthetic gene encoded in an expression vector, transcripts generated and microinjected into Xenopus oocytes, and the resulting tRNA products analyzed for the presence of modified bases. The results suggest that efficient methylation of mcmU to yield mcmUm requires the prior formation of each modified base and an intact tertiary structure, whereas formation of modified bases at other positions, including mcmU, is not as stringently connected to precise primary and tertiary structure. These results, along with the observations that methylation of mcmU is enhanced in the presence of selenium and that this methyl group affects tertiary structure, further suggest that the mcmUm isoacceptor must have a role in selenoprotein synthesis different from that of the mcmU isoacceptor.
机译:高等脊椎动物中的硒代半胱氨酸(Sec)tRNA [Ser] Sec种群由两个主要的异受体组成,它们彼此之间的区别在于反密码子的摆动位置(位置34)存在单个核苷修饰。一个异位受体在该位置包含5-甲基羧甲基尿苷(mcmU),而另一个包含5-甲基羧甲基尿苷-2'-O-甲基核糖(mcmUm)。这些tRNA中的其他修饰分别是在位置37、55和58处的N6-异戊烯基腺苷(i6A),假尿苷(psi)和1-甲基腺苷(m1A)。由于34位核糖的甲基化受到细胞内硒状态的影响,并且此甲基的存在会显着改变三级结构,因此我们研究了其他位置修饰以及三级结构对其形成的影响。将突变引入表达载体中编码的合成基因中,生成转录本并将其显微注射到非洲爪蟾卵母细胞中,并分析所得tRNA产物中修饰碱基的存在。结果表明,mcmU的有效甲基化产生mcmUm需要事先形成每个修饰的碱基和完整的三级结构,而在其他位置(包括mcmU)形成修饰的碱基并不严格地连接到精确的一级和三级结构。这些结果,以及在硒的存在下mcmU的甲基化作用增强以及该甲基基团影响三级结构的观察结果,进一步表明,mcmUm异构体在硒蛋白合成中的作用必须不同于mcmU异构体。

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