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KIT FOR RECOMBINASE POLYMERASE AMPLIFICATION

机译:用于重组酶聚合酶扩增的试剂盒

摘要

This disclosure describes related novel methods for Recombinase-Polymerase Amplification (RPA) of a target DNA that exploit the properties of recombinase and related proteins, to invade double-stranded DNA with single stranded homologous DNA permitting sequence specific priming of DNA polymerase reactions. The disclosed methods have the advantage of not requiring thermocycling or thermophilic enzymes, thus offering easy and affordable implementation and portability relative to other amplification methods. Further disclosed are conditions to enable real-time monitoring of RPA reactions, methods to regulate RPA reactions using light and otherwise, methods to determine the nature of amplified species without a need for gel electrophoresis, methods to improve and optimize signal to noise ratios in RPA reactions, methods to optimize oligonucleotide primer function, methods to control carryover contamination, and methods to employ sequence-specific third 'specificity' probes. Further described are novel properties and approaches for use of probes monitored by light in dynamic recombination environments.
机译:本公开描述了用于靶DNA的重组酶-聚合酶扩增(RPA)的相关新方法,其利用重组酶和相关蛋白的性质,以单链同源DNA侵入双链DNA,从而允许DNA聚合酶反应的序列特异性引发。所公开的方法具有不需要热循环或嗜热酶的优点,因此相对于其他扩增方法提供了容易且负担得起的实施和便携性。进一步公开了能够实时监测RPA反应的条件,使用光调节RPA反应的方法等,无需凝胶电泳即可确定扩增物种的性质的方法,改善和优化RPA中信噪比的方法反应,优化寡核苷酸引物功能的方法,控制残留污染的方法以及采用序列特异性第三“特异性”探针的方法。进一步描述了在动态重组环境中使用由光监控的探针的新颖性质和方法。

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