Peptide Nucleic Acid Clamp‐Assisted Photothermal Multiplexed Digital PCR for Identifying SARS‐CoV‐2 Variants of Concern

Lexiang Zhang; Rokshana Parvin; Siyue Lin; Mingshuo Chen; Ruixuan Zheng; Qihui Fan; Fangfu Ye

doi:10.1002/advs.202306088

Advanced Science (Apr 2024)

Peptide Nucleic Acid Clamp‐Assisted Photothermal Multiplexed Digital PCR for Identifying SARS‐CoV‐2 Variants of Concern

Lexiang Zhang,
Rokshana Parvin,
Siyue Lin,
Mingshuo Chen,
Ruixuan Zheng,
Qihui Fan,
Fangfu Ye

Affiliations

Lexiang Zhang: Joint Centre of Translational Medicine the First Affiliated Hospital of Wenzhou Medical University Wenzhou Zhejiang 325035 China
Rokshana Parvin: Oujiang Laboratory (Zhejiang Lab for Regenerative Medicine, Vision and Brain Health); Wenzhou Institute University of Chinese Academy of Sciences Wenzhou 325000 China
Siyue Lin: Department of Biomedical Engineering Columbia University New York NY 10027 USA
Mingshuo Chen: Oujiang Laboratory (Zhejiang Lab for Regenerative Medicine, Vision and Brain Health); Wenzhou Institute University of Chinese Academy of Sciences Wenzhou 325000 China
Ruixuan Zheng: Joint Centre of Translational Medicine the First Affiliated Hospital of Wenzhou Medical University Wenzhou Zhejiang 325035 China
Qihui Fan: Beijing National Laboratory for Condensed Matter Physics Institute of Physics Chinese Academy of Sciences Beijing China 100190
Fangfu Ye: Joint Centre of Translational Medicine the First Affiliated Hospital of Wenzhou Medical University Wenzhou Zhejiang 325035 China

DOI: https://doi.org/10.1002/advs.202306088
Journal volume & issue: Vol. 11, no. 13
pp. n/a – n/a

Abstract

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Abstract The unprecedented demand for variants diagnosis in response to the COVID‐19 epidemic has brought the spotlight onto rapid and accurate detection assays for single nucleotide polymorphisms (SNPs) at multiple locations. However, it is still challenging to ensure simplicity, affordability, and compatibility with multiplexing. Here, a novel technique is presented that combines peptide nucleic acid (PNA) clamps and near‐infrared (NIR)‐driven digital polymerase chain reaction (dPCR) to identify the Omicron and Delta variants. This is achieved by simultaneously identifying highly conserved mutated signatures at codons 19, 614, and 655 of the spike protein gene. By microfluidically introducing graphene‐oxide‐nanocomposite into the assembled gelatin microcarriers, they achieved a rapid temperature ramping‐up rate and switchable gel‐to‐sol phase transformation synchronized with PCR activation under NIR irradiation. Two sets of duplex PCR reactions, each classifying respective PNA probes, are emulsified in parallel and illuminated together using a homemade vacuum‐based droplet generation device and a programmable NIR control module. This allowed for selective amplification of mutant sequences due to single‐base‐pair mismatch with PNA blockers. Sequence‐recognized bioreactions and fluorescent‐color scoring enabled quick identification of variants. This technique achieved a detection limit of 5,100 copies and a 5‐fold quantitative resolution, which is promising to unfold minor differences and dynamic changes.

Published in Advanced Science

ISSN: 2198-3844 (Online)
Publisher: Wiley
Country of publisher: Germany
LCC subjects: Science
Website: https://onlinelibrary.wiley.com/journal/21983844

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