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噻唑橙染料的分子工程:在生物测定中与核酸结合后荧光信号从通用型转变为特异性。

Molecular Engineering of Thiazole Orange Dye: Change of Fluorescent Signaling from Universal to Specific upon Binding with Nucleic Acids in Bioassay.

作者信息

Lu Yu-Jing, Deng Qiang, Hou Jin-Qiang, Hu Dong-Ping, Wang Zheng-Ya, Zhang Kun, Luyt Leonard G, Wong Wing-Leung, Chow Cheuk-Fai

机构信息

Institute of Natural Medicine and Green Chemistry, School of Chemical Engineering and Light Industry, Guangdong University of Technology , Guangzhou 510006, Peoples' Republic of China.

London Regional Cancer Program , 790 Commissioners Road East, London, Ontario N6A 4L6, Canada.

出版信息

ACS Chem Biol. 2016 Apr 15;11(4):1019-29. doi: 10.1021/acschembio.5b00987. Epub 2016 Jan 26.

Abstract

The universal fluorescent staining property of thiazole orange (TO) dye was adapted in order to be specific for G-quadruplex DNA structures, through the introduction of a styrene-like substituent at the ortho-position of the TO scaffold. This extraordinary outcome was determined from experimental studies and further explored through molecular docking studies. The molecular docking studies help understand how such a small substituent leads to remarkable fluorescent signal discrimination between G-quadruplex DNA and other types of nucleic acids. The results reveal that the modified dyes bind to the G-quadruplex or duplex DNA in a similar fashion as TO, but exhibit either enhanced or quenched fluorescent signal, which is determined by the spatial length and orientation of the substituent and has never been known. The new fluorescent dye modified with a p-(dimethylamino)styryl substituent offers 10-fold more selectivity toward telomeric G-quadruplexes than double-stranded DNA substrates. In addition, native PAGE experiments, FRET, CD analysis, and live cell imaging were also studied and demonstrated the potential applications of this class of thiazole-orange-based fluorescent probes in bioassays and cell imaging.

摘要

噻唑橙(TO)染料具有通用的荧光染色特性,通过在TO支架的邻位引入类似苯乙烯的取代基,使其对G-四链体DNA结构具有特异性。这一非凡的结果是通过实验研究确定的,并通过分子对接研究进一步探索。分子对接研究有助于理解这样一个小取代基如何导致G-四链体DNA与其他类型核酸之间显著的荧光信号差异。结果表明,修饰后的染料与G-四链体或双链DNA的结合方式与TO相似,但表现出增强或淬灭的荧光信号,这取决于取代基的空间长度和取向,这是前所未有的。用对-(二甲基氨基)苯乙烯基取代基修饰的新型荧光染料对端粒G-四链体的选择性比双链DNA底物高10倍。此外,还研究了天然PAGE实验、FRET、CD分析和活细胞成像,并证明了这类基于噻唑橙的荧光探针在生物测定和细胞成像中的潜在应用。

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