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通过适体/凝血酶复合物的催化激活实现DNA的荧光检测。

Fluorescence detection of DNA by the catalytic activation of an aptamer/thrombin complex.

作者信息

Pavlov Valeri, Shlyahovsky Bella, Willner Itamar

机构信息

Institute of Chemistry, The Farkas Center for Light-Induced Processes, The Hebrew University of Jerusalem, Jerusalem 91904, Israel.

出版信息

J Am Chem Soc. 2005 May 11;127(18):6522-3. doi: 10.1021/ja050678k.

Abstract

A conjugate consisting of a thrombin aptamer tethered to the thrombin, Th, with a sensing nucleic acid (1) is used for the optical detection of DNA. The thrombin/aptamer complex blocks the biocatalytic functions of Th. Hybridization of the analyte DNA (2) to the sensing nucleic acid 1 yields a rigid duplex that detaches the aptamer from Th, a process that activates the protein toward the hydrolysis of bis(p-tosyl-Gly-Pro-Arg)-R110 (3) to the rhodamine 110 fluorophore (4). The system allows the DNA sensing with a sensitivity limit of 1 x 10-8 M. The aptamer/Th conjugate is also immobilized on glass slides for the optical detection of DNA. The dissociation of the aptamer/Th complex upon hybridization and the subsequent dehybridization of the duplex and the regeneration of the catalytically inactive Th/aptamer complex duplicate machinery functions.

摘要

一种由与凝血酶(Th)相连的凝血酶适配体和传感核酸(1)组成的共轭物用于DNA的光学检测。凝血酶/适配体复合物会阻断Th的生物催化功能。分析物DNA(2)与传感核酸1杂交会产生一个刚性双链体,使适配体与Th分离,这一过程会激活该蛋白质对双(对甲苯磺酰甘氨酰-脯氨酰-精氨酸)-R110(3)水解生成罗丹明110荧光团(4)。该系统能够以1×10⁻⁸ M的灵敏度极限进行DNA传感。适配体/Th共轭物也固定在载玻片上用于DNA的光学检测。杂交时适配体/Th复合物的解离以及随后双链体的解杂交和催化无活性的Th/适配体复合物的再生重复了机械功能。

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