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用于单核苷酸特异性DNA序列检测的模板金属催化

Templated metal catalysis for single nucleotide specific DNA sequence detection.

作者信息

Boll Iris, Krämer Roland, Brunner Jens, Mokhir Andriy

机构信息

Anorganisch-Chemisches Institut, Ruprecht-Karls-Universität Heidelberg, Im Neuenheimer Feld 270, 69120 Heidelberg, Germany.

出版信息

J Am Chem Soc. 2005 Jun 1;127(21):7849-56. doi: 10.1021/ja0503332.

Abstract

A catalytic DNA-templated reaction of hydrolysis of an ester group in an N-modified peptide nucleic acid, which is activated by a Cu2+ complex-PNA, has been discovered and optimized. Both the ester-containing PNA and the metal complex PNA bind neighboring sites on a template DNA. This brings the reacting groups (the ester and the Cu2+ complex) in proximity to each other and accelerates the hydrolysis of the ester approximately 500 times in comparison with its hydrolysis in the absence of the template. The hydrolysis reaction provides >10(2)-fold kinetic discrimination between DNAs that are different from each other at a single nucleotide position. Natural enzyme T4 DNA ligase is slightly less selective. On the basis of this reaction a fully homogeneous and sensitive assay for sequence-specific DNA detection has been developed (10 fmol DNA). Identification of one of four DNAs (variation at one position) can be done in a single experiment. Since the Cu2+ ion is tightly bound in an associate containing the ester PNA, the metal complex PNA, and the template DNA, application of this method in buffers containing other Cu2+-binding ligands, e.g., PCR buffer and physiological buffer, is possible.

摘要

已发现并优化了一种由铜离子配合物修饰的肽核酸(PNA)激活的、催化N-修饰肽核酸中酯基水解的DNA模板反应。含酯PNA和金属配合物PNA均与模板DNA上的相邻位点结合。这使反应基团(酯基和铜离子配合物)彼此靠近,与无模板时的水解相比,酯的水解速度加快了约500倍。水解反应在单核苷酸位置不同的DNA之间提供了大于10²倍的动力学区分。天然酶T4 DNA连接酶的选择性略低。基于该反应,已开发出一种用于序列特异性DNA检测的完全均相且灵敏的检测方法(10 fmol DNA)。在单个实验中即可鉴定四种DNA中的一种(一个位置的变异)。由于铜离子紧密结合在包含酯PNA、金属配合物PNA和模板DNA的复合物中,因此该方法可应用于含有其他铜离子结合配体的缓冲液中,例如PCR缓冲液和生理缓冲液。

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