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嗜热古菌嗜热栖热放线菌的DNA聚合酶在发夹-线圈过渡状态下对串联重复DNA的延伸:原始简单DNA序列扩增模型

Elongation of tandem repetitive DNA by the DNA polymerase of the hyperthermophilic archaeon Thermococcus litoralis at a hairpin-coil transitional state: a model of amplification of a primordial simple DNA sequence.

作者信息

Ogata N, Miura T

机构信息

Taiko Pharmaceutical Company, Ltd., Suita, Osaka, Japan.

出版信息

Biochemistry. 2000 Nov 14;39(45):13993-4001. doi: 10.1021/bi0013243.

Abstract

DNA is replicated by DNA polymerase semiconservatively in many organisms. Accordingly, the replicated DNA does not become larger than the original DNA (template DNA), implying that replicative synthesis by DNA polymerase alone cannot explain the diversification of primordial simple DNA. We demonstrate that a single-stranded tandem repetitive oligodeoxyribonucleic acid (oligoDNA) composed of a palindromic or quasi-palindromic motif sequence and 25-50% GC content is elongated in vitro to more than 20,000 bases at 70-74 degrees C by the DNA polymerase of the hyperthermophilic archaeon Thermococcus litoralis without a bimolecular primer-template complex. The efficiency of elongation decreased when the palindromic structure of the oligoDNA was destroyed or when the GC content of the oligoDNA was outside the range of 25-50%. The thermal melting transition profile of the oligoDNA, as observed by ultraviolet spectroscopy, exhibited a biphasic curve, reflecting a duplex-hairpin transition at 31-40 degrees C and a hairpin-coil transition at 70-77 degrees C. The optimal reaction temperature for the elongation, for instance, of oligoDNA (AGATATCT)(6) (72 degrees C) was very close to its hairpin-coil transition melting temperature (70.4 degrees C), but was markedly higher than the temperature at which duplex oligoDNA can exist stably (<35.9 degrees C). These results suggest that a hairpin-based "intramolecular primer-template structure" is formed transiently in the oligoDNA, and it is elongated by the DNA polymerase to long DNA through repeated cycles of folding and melting of the hairpin structure. We discuss the implication of this phenomenon, "hairpin elongation", from the standpoint of potential amplification of simple DNA sequences during the evolution of the genome.

摘要

在许多生物体中,DNA由DNA聚合酶以半保留方式进行复制。因此,复制后的DNA不会比原始DNA(模板DNA)更大,这意味着仅靠DNA聚合酶进行的复制性合成无法解释原始简单DNA的多样化。我们证明,由回文或准回文基序序列组成且GC含量为25 - 50%的单链串联重复寡脱氧核糖核酸(oligoDNA),在70 - 74摄氏度下,无需双分子引物 - 模板复合物,就能被嗜热古菌嗜热栖热袍菌的DNA聚合酶在体外延长至超过20,000个碱基。当oligoDNA的回文结构被破坏或其GC含量超出25 - 50%范围时,延长效率会降低。通过紫外光谱观察到的oligoDNA的热熔解转变曲线呈现双相曲线,反映了在31 - 40摄氏度时的双链 - 发夹转变以及在70 - 77摄氏度时的发夹 - 线圈转变。例如,oligoDNA(AGATATCT)(6)延长的最佳反应温度(72摄氏度)非常接近其发夹 - 线圈转变熔解温度(70.4摄氏度),但明显高于双链oligoDNA能够稳定存在的温度(<35.9摄氏度)。这些结果表明,在oligoDNA中会瞬时形成基于发夹的“分子内引物 - 模板结构”,并且它会通过DNA聚合酶对发夹结构的反复折叠和熔解循环延长为长DNA。我们从基因组进化过程中简单DNA序列潜在扩增的角度讨论了这种“发夹延长”现象的意义。

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