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首页> 外文期刊>Nucleic Acids Research >Unwinding of nucleic acids by HCV NS3 helicase is sensitive to the structure of the duplex.
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Unwinding of nucleic acids by HCV NS3 helicase is sensitive to the structure of the duplex.

机译:HCV NS3解旋酶解开核酸对双链体的结构敏感。

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Hepatitis C virus (HCV) helicase, non-structural protein 3 (NS3), is proposed to aid in HCV genome replication and is considered a target for inhibition of HCV. In order to investigate the substrate requirements for nucleic acid unwinding by NS3, substrates were prepared by annealing a 30mer oligonucleotide to a 15mer. The resulting 15 bp duplex contained a single-stranded DNA overhang of 15 nt referred to as the bound strand. Other substrates were prepared in which the 15mer DNA was replaced by a strand of peptide nucleic acid (PNA). The PNA-DNA substrate was unwound by NS3, but the observed rate of strand separation was at least 25-fold slower than for the equivalent DNA-DNA substrate. Binding of NS3 to the PNA-DNA substrate was similar to the DNA-DNA substrate, due to the fact that NS3 initially binds to the single-stranded overhang, which was identical in each substrate. A PNA-RNA substrate was not unwound by NS3 under similar conditions. In contrast, morpholino-DNA and phosphorothioate-DNA substrates were utilized as efficiently by NS3 as DNA-DNA substrates. These results indicate that the PNA-DNA and PNA-RNA heteroduplexes adopt structures that are unfavorable for unwinding by NS3, suggesting that the unwinding activity of NS3 is sensitive to the structure of the duplex.
机译:丙型肝炎病毒(HCV)解旋酶,非结构蛋白3(NS3),被提议来帮助HCV基因组复制,并被认为是抑制HCV的靶标。为了研究NS3解链核酸的底物要求,通过将30mer寡核苷酸退火至15mer来制备底物。所得的15 bp双链体包含15 nt的单链DNA突出端,称为结合链。制备了其他底物,其中的15聚体DNA被肽核酸(PNA)链替代。 NS3可以解开PNA-DNA底物,但是观察到的链分离速率比等效的DNA-DNA底物至少慢25倍。 NS3与PNA-DNA底物的结合与DNA-DNA底物相似,这是因为NS3最初与单链突出端结合,这一点在每个底物中都是相同的。在类似条件下,NS3不会解开PNA-RNA底物。相比之下,吗啉代DNA和硫代磷酸酯DNA底物被NS3有效地利用为DNA-DNA底物。这些结果表明,PNA-DNA和PNA-RNA异源双链体具有不利于NS3解链的结构,这表明NS3的解链活性对双链体的结构敏感。

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