Improved protocol for Bst polymerase and reverse transcriptase production and application to a point-of-care diagnostics system

Bst 聚合酶和逆转录酶生产的改进方案及其在即时诊断系统中的应用

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作者:Lucas Rodrigo de Souza, Italo Esposti Poly da Silva, Gabriele Celis-Silva, Bruna Winkert Raddatz, Louise Matiê Imamura, Edson Yu Sin Kim, Gabriel Vieira Valderrama, Halanna de Paula Riedi, Sergio Renato Rogal Jr, Bernardo Montesanti Machado de Almeida, Marcus Vinícius Mazega Figueredo, Mario Henriqu

Abstract

The pandemic caused by severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2) has raised awareness in the scientific community about the importance of being prepared for sanitary emergencies. Many measures implemented during the COVID pandemic are now being expanded to other applications. In the field of molecular and immunological diagnostics, the need to massively test the population worldwide resulted in the application of a variety of methods to detect viral infection. Besides gold standard reverse transcription quantitative polymerase chain reaction (RT-qPCR), the use of reverse transcription loop-mediated isothermal amplification (RT-LAMP) arose as an alternative and sensitive method to amplify and detect viral genetic material. We have used openly available protocols and have improved the protein production of RT-LAMP enzymes Bst polymerase and HIV-reverse transcriptase. To optimize enzyme production, we tested different protein tags, and we shortened the protein purification protocol, resulting in reduced processing time and handling of the enzymes and, thus, preserved the protein activity with high purity. The enzymes showed significant stability at 4 °C and 25 °C, over 60 days, and were highly reliable when used as a one-step RT-LAMP reaction in a portable point-of-care device with clinical samples. The enzymes and the reaction setup can be further expanded to detect other infectious diseases agents.

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