| Literature DB >> 31793929 |
Gangyi Chen1, Rong Chen2, Sheng Ding1, Mei Li1, Jiayu Wang1, Jiawei Zou1, Feng Du1, Juan Dong1, Xin Cui1, Xin Huang1, Yun Deng2, Zhuo Tang1.
Abstract
Polymerase chain reaction (PCR) and isothermal amplification methods such as LAMP and RPA are widely used for genetic detection. However, there are some shortcomings of these methods such as dependence on thermocycler instruments for PCR, complexity of primer design, the possibility for nonspecific amplification in LAMP and complexity of components in RPA. We develop a novel isothermal DNA detection system named Recombinase Assisted Loop-mediated Amplification (RALA). Recombinase from Thermus thermophilus (TthRecA) was used to open target double-stranded DNA to initiate loop-mediated amplification under isothermal conditions, which simplified the primer design and circumvented pre-denaturation. A FRET sensor named ProofMan and a proofreading enzyme Pfu were introduced to produce fluorescence signals by cleaving the sensor from the 3' end. Consequently, sequence-specific detection based on the RALA system was achieved, and even a single nucleotide polymorphism (SNP) could be identified. By introducing additional loop primers, the fast RALA version can amplify 102 DNA targets in 30 minutes. In addition to high sensitivity and specificity, the flexibility of choosing different reporting sensors makes this method versatile in either quantitative or qualitative DNA detection.Entities:
Year: 2019 PMID: 31793929 DOI: 10.1039/c9an01701a
Source DB: PubMed Journal: Analyst ISSN: 0003-2654 Impact factor: 4.616