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通过A⁺-C碱基对和假尿苷使tRNALys,3的反密码子茎环稳定。

Stabilization of the anticodon stem-loop of tRNALys,3 by an A+-C base-pair and by pseudouridine.

作者信息

Durant P C, Davis D R

机构信息

University of Utah, Salt Lake City, UT, 84112, USA.

出版信息

J Mol Biol. 1999 Jan 8;285(1):115-31. doi: 10.1006/jmbi.1998.2297.

Abstract

NMR spectroscopy was used to determine the solution structures of RNA oligonucleotides comprising the anticodon domain of tRNALys,3. The structural effects of the pseudouridine modification at position 39 were investigated and are well correlated with changes in thermodynamic parameters derived from temperature dependent UV measurements. The pseudouridine-containing hairpin is thermodynamically more stable than the unmodified hairpin by 5 degreesC, and this corresponds with increased base stacking on the 3' side of the tRNA anticodon loop. An A+38-C32 base-pair also forms at the base of the anticodon stem with an approximate pKa of 6 for A38. Formation of the A+-C base-pair increases the Tm of both pseudouridine modified and unmodified RNA hairpins by 5-6 degreesC, and decreases the DeltaG degrees for hairpin formation by 1 kcal/mol. Solution structures were determined for both psi39 and unmodified hairpins under limiting pH conditions at pH 5 and pH 7 to assess the structural effects of both psi modification and the additional A+-C base-pair on tRNALys,3 structure. The A+38-C32 base-pair strengthens the 31-39 base-pair, and induces formation of a dynamic U33-A37 base-pair that effectively reduces the normal seven nucleotide anticodon loop to a three nucleotide UUU loop. These undermodified tRNALys,3 anticodon loops are distinctly different from those seen for other tRNAs exemplified by tRNAPhe. The conformation of the tRNA loop has important implications for the role of nucleoside modification in codon-anticodon recognition and for utilization of tRNALys,3 by HIV-1 as the native reverse transcriptase primer.

摘要

核磁共振光谱法被用于确定包含tRNALys,3反密码子结构域的RNA寡核苷酸的溶液结构。研究了39位假尿苷修饰的结构效应,并且这些效应与从温度依赖性紫外测量得出的热力学参数变化密切相关。含假尿苷的发夹在热力学上比未修饰的发夹稳定5摄氏度,这与tRNA反密码子环3'侧碱基堆积增加相对应。在反密码子茎的底部还形成了一个A+38-C32碱基对,A38的近似pKa为6。A+-C碱基对的形成使假尿苷修饰和未修饰的RNA发夹的解链温度均升高5-6摄氏度,并使发夹形成的ΔG°降低1千卡/摩尔。在pH 5和pH 7的极限pH条件下,测定了psi39和未修饰发夹的溶液结构,以评估psi修饰和额外的A+-C碱基对对tRNALys,3结构的影响。A+38-C32碱基对加强了31-39碱基对,并诱导形成一个动态的U33-A37碱基对,有效地将正常的七核苷酸反密码子环减少为三核苷酸UUU环。这些修饰不足的tRNALys,3反密码子环比以tRNAPhe为代表的其他tRNA的反密码子环明显不同。tRNA环的构象对于核苷修饰在密码子-反密码子识别中的作用以及HIV-1将tRNALys,3用作天然逆转录酶引物的利用具有重要意义。

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