Assessing Different PCR Master Mixes for Ultrarapid DNA Amplification: Important Analytical Parameters

Author:

Brukner Ivan1ORCID,Paliouras Miltiadis2ORCID,Trifiro Mark12,Bohbot Marc3,Shamir Daniel3,Kirk Andrew G.4

Affiliation:

1. Lady Davis Institute for Medical Research, Jewish General Hospital, Montreal, QC H3T 1E2, Canada

2. Department of Medicine, McGill University, Montreal, QC H3G 2M1, Canada

3. Nexless Healthcare, 1315 Chem. Canora, Mont-Royal, Montreal, QC H3P 2J5, Canada

4. Department of Electrical and Computer Engineering, McGill University, Montreal, QC H3A 0E9, Canada

Abstract

The basic principles of ultrafast plasmonic PCR have been promulgated in the scientific and technological literature for over a decade. Yet, its everyday diagnostic utility remains unvalidated in pre-clinical and clinical settings. Although the impressive speed of plasmonic PCR reaction is well-documented, implementing this process into a device form compatible with routine diagnostic tasks has been challenging. Here, we show that combining careful system engineering and process control with innovative and specific PCR biochemistry makes it possible to routinely achieve a sensitive and robust “10 min” PCR assay in a compact and lightweight system. The critical analytical parameters of PCR reactions are discussed in the current instrument setting.

Funder

Canadian Institutes for Health Research

MEDTEQ (Project 17-G), Natural Sciences and Engineering Research Council (NSERC)-Alliance

Jewish General Hospital Foundation on behalf of Sophie Desmarais

Nexless Healthcare

Solis Biodyne

Publisher

MDPI AG

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