Ultrasensitive Uracil-DNA Glycosylase Activity Assay and Its Inhibitor Screening Based on Primer Remodeling Jointly via Repair Enzyme and Polymerase

The development of isothermal nucleic acid amplification techniques has great significance for highly sensitive biosensing in modern biology and biomedicine. A facile and robust exponential rolling circle amplification (RCA) strategy is proposed based on primer-remodeling amplification jointly via a...

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Veröffentlicht in:	Langmuir : the ACS journal of surfaces and colloids. - 1992. - 38(2022), 12 vom: 29. März, Seite 3868-3875
1. Verfasser:	Wang, Yu (VerfasserIn)
Weitere Verfasser:	Sun, Wenyu, Wang, Jingfeng, Wang, Xu, Xu, Yicheng, Guo, Yuanzhen, Wang, Yeru, Zhang, Manru, Jiang, Long, Liu, Su, Huang, Jiadong
Format:	Online-Aufsatz
Sprache:	English
Veröffentlicht:	2022
Zugriff auf das übergeordnete Werk:	Langmuir : the ACS journal of surfaces and colloids
Schlagworte:	Journal Article Research Support, Non-U.S. Gov't Fluorescent Dyes alpha-Fetoproteins Uracil-DNA Glycosidase EC 3.2.2.-


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100	1		\|a Wang, Yu \|e verfasserin \|4 aut
245	1	0	\|a Ultrasensitive Uracil-DNA Glycosylase Activity Assay and Its Inhibitor Screening Based on Primer Remodeling Jointly via Repair Enzyme and Polymerase
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520			\|a The development of isothermal nucleic acid amplification techniques has great significance for highly sensitive biosensing in modern biology and biomedicine. A facile and robust exponential rolling circle amplification (RCA) strategy is proposed based on primer-remodeling amplification jointly via a repair enzyme and polymerase, and uracil-DNA glycosylase (UDG) is selected as a model analyte. Two kinds of complexes, complex I and complex II, are preprepared by hybridizing a circular template (CT) with a uracil-containing hairpin probe and tetrahydrofuran abasic site mimic (AP site)-embedded fluorescence-quenched probe (AFP), respectively. The target UDG specifically binds to complex I, resulting in the generation of an AP site, followed by cleavage via endonuclease IV (Endo IV) and the successive trimming of unmatched 3' terminus via phi29 DNA polymerase, thus producing a useable primer-CT complex that actuates the primary RCA. Then, numerous complex II anneal with the first-generation RCA product (RP), generating a complex II-RP assembly containing AP sites within the DNA duplex. With the aid of Endo IV and phi29, AFP, as a pre-primer in complex II, is converted into a mature primer to initiate additional rounds of RCA. So, countless AFPs are cleaved, releasing remarkably strong fluorescent signals. The biosensor is demonstrated to enable rapid and accurate detection of the UDG activity with an improved detection limit as low as 4.7 × 10-5 U·mL-1. Moreover, this biosensor is successfully applied for UDG inhibitor screening and complicated biological samples analysis. Compared to the previous exponential RCA methods, our proposed strategy offers additional advantages, including excellent stability, optional design of CT, and simplified operating steps. Therefore, this proposed strategy may create a useful and practical platform for ultrasensitive detection of low levels of analytes in clinical diagnosis and fundamental biomedicine research
650		4	\|a Journal Article
650		4	\|a Research Support, Non-U.S. Gov't
650		7	\|a Fluorescent Dyes \|2 NLM
650		7	\|a alpha-Fetoproteins \|2 NLM
650		7	\|a Uracil-DNA Glycosidase \|2 NLM
650		7	\|a EC 3.2.2.- \|2 NLM
700	1		\|a Sun, Wenyu \|e verfasserin \|4 aut
700	1		\|a Wang, Jingfeng \|e verfasserin \|4 aut
700	1		\|a Wang, Xu \|e verfasserin \|4 aut
700	1		\|a Xu, Yicheng \|e verfasserin \|4 aut
700	1		\|a Guo, Yuanzhen \|e verfasserin \|4 aut
700	1		\|a Wang, Yeru \|e verfasserin \|4 aut
700	1		\|a Zhang, Manru \|e verfasserin \|4 aut
700	1		\|a Jiang, Long \|e verfasserin \|4 aut
700	1		\|a Liu, Su \|e verfasserin \|4 aut
700	1		\|a Huang, Jiadong \|e verfasserin \|4 aut
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773	1	8	\|g volume:38 \|g year:2022 \|g number:12 \|g day:29 \|g month:03 \|g pages:3868-3875
856	4	0	\|u http://dx.doi.org/10.1021/acs.langmuir.2c00115 \|3 Volltext
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