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一种DNA解旋酶对非天然底物的解旋作用。

Unwinding of unnatural substrates by a DNA helicase.

作者信息

Tackett A J, Morris P D, Dennis R, Goodwin T E, Raney K D

机构信息

Department of Biochemistry and Molecular Biology, University of Arkansas for Medical Sciences, Little Rock, Arkansas 72205, USA.

出版信息

Biochemistry. 2001 Jan 16;40(2):543-8. doi: 10.1021/bi002122+.

Abstract

Helicases separate double-stranded DNA into single-stranded DNA intermediates that are required during replication and recombination. These enzymes are believed to transduce free energy available from ATPase activity to unwind the duplex and translocate along the nucleic acid lattice. The nature of enzyme-substrate interactions between helicases and duplex DNA substrates has not been well-defined. Most helicases require a single-stranded DNA overhang adjacent to duplex DNA in order to initiate unwinding. The strand containing the overhang is referred to as the loading strand whereas the complementary strand is referred to as the displaced strand. We have investigated the interactions between a DNA helicase and the DNA substrate by replacing the displaced strand with a nucleic acid mimic, peptide nucleic acid (PNA). PNA is capable of forming duplex structures with DNA according to Watson-Crick base pairing rules, but contains a N-(2-aminoethyl)glycine backbone in place of the deoxyribose phosphates. The PNA-DNA hybrids had higher melting temperatures than their DNA-DNA counterparts. Dda helicase, from bacteriophage T4, was able to unwind the DNA-PNA substrates at similar rates as DNA-DNA substrates. The results indicate that the rate-limiting step for unwinding is relatively insensitive to the chemical nature of the displaced strand and the thermal stability of oligonucleotide substrates.

摘要

解旋酶将双链DNA分离成复制和重组过程中所需的单链DNA中间体。据信,这些酶可将ATP酶活性产生的自由能转化,以解开双链并沿核酸晶格移位。解旋酶与双链DNA底物之间的酶-底物相互作用的性质尚未明确界定。大多数解旋酶需要双链DNA旁有一个单链DNA突出端,以便启动解旋。含有突出端的链称为加载链,而互补链称为置换链。我们通过用核酸类似物肽核酸(PNA)取代置换链,研究了DNA解旋酶与DNA底物之间的相互作用。PNA能够根据沃森-克里克碱基配对规则与DNA形成双链结构,但含有N-(2-氨基乙基)甘氨酸主链来替代脱氧核糖磷酸。PNA-DNA杂交体的解链温度高于其DNA-DNA对应物。来自噬菌体T4的Dda解旋酶能够以与DNA-DNA底物相似的速率解开DNA-PNA底物。结果表明,解旋的限速步骤对置换链的化学性质和寡核苷酸底物的热稳定性相对不敏感。

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