Monitoring RAYT activity by surface plasmon resonance biosensor

被引:0
|
作者
Markéta Bocková
Tomáš Špringer
Iva Nečasová
Jaroslav Nunvar
Bohdan Schneider
Jiří Homola
机构
[1] Institute of Photonics and Electronics AS CR,
[2] v. v. i.,undefined
[3] Institute of Biotechnology AS CR,undefined
[4] v. v. i.,undefined
来源
Analytical and Bioanalytical Chemistry | 2015年 / 407卷
关键词
Surface plasmon resonance; REP-associated tyrosine transposase; Biosensor;
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中图分类号
学科分类号
摘要
The process of DNA transposition involves the binding, cleavage, and recombination of specific DNA segments (transposable elements, TE) and is catalyzed by special enzymes encoded by the TE transposases. REP-associated tyrosine transposases (RAYTs) are a class of Y1 nucleases related to the IS200/IS605 transposases associated with a bacterial TE known as repetitive extragenic palindrome elements (REPs). Although RAYT has been subject of numerous studies, where DNA binding and cleavage by RAYT have been confirmed for Escherichia coli, the molecular mechanism of DNA insertion has not been fully understood. In this work, it is demonstrated that surface plasmon resonance (SPR) biosensor technology combined with a system of DNA hairpin probes (mimicking the natural REP sequence) and short oligonucleotides (ONs) can provide a rapid and real-time platform for monitoring and quantification of RAYT activity. We utilized RAYT from E. coli (strain MG1655) as a model system, where we evaluated its activity towards both a natural REP sequence as well as REP sequences having modifications targeting specific features of the DNA crucial for the DNA binding and cleavage. The characteristics of the RAYT-DNA interaction obtained by means of the SPR approach were compared with the results of SDS-PAGE analysis.
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页码:3985 / 3993
页数:8
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