首页> 美国卫生研究院文献>Proceedings of the National Academy of Sciences of the United States of America >Strand breakage by the DNA untwisting enzyme results in covalent attachment of the enzyme to DNA.
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Strand breakage by the DNA untwisting enzyme results in covalent attachment of the enzyme to DNA.

机译:DNA解捻酶造成的链断裂导致酶与DNA共价连接。

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摘要

Strands of DNA that have been broken by the DNA untwisting enzyme exhibit a reduced buoyant density in alkaline CsCl due to bound protein. A covalent linkage between the DNA and the enzyme was indicated by the stability of the complex in alkali (pH greaterthan 12.7), in 7 M guanidine-HCl, and at 90 degrees in 1% Sarkosyl for 5 min. The single-strand breaks generated by the enzyme are resistant to exonuclease III, indicating that the protein is attached to one of the ends of the broken strands. The free end of the broken strand bears a 5'-hydroxyl group, indicating attachment of the protein to the 3'-phosphoryl terminus. A nucleotide-peptide linkage involving a phosphoamide bond is unlikely since the complex is resistant to 3.5 M hydroxylamine at pH 4.75.
机译:被DNA解捻酶断裂的DNA链由于结合了蛋白质而在碱性CsCl中的浮力密度降低。 DNA和酶之间的共价键由复合物在碱(pH大于12.7),在7 M盐酸胍中和在90度的1%Sarkosyl中5分钟的稳定性表明。该酶产生的单链断裂对核酸外切酶III具有抗性,表明该蛋白质附着在断裂链的末端之一上。断裂链的自由端带有一个5'-羟基,表明该蛋白质与3'-磷酰基末端连接。涉及磷酰胺键的核苷酸-肽键是不可能的,因为该复合物在pH 4.75下对3.5 M羟胺具有抗性。

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