Advancing quantitative PCR with color cycle multiplex amplification

Author:

Chen Wei1ORCID,Zhang Kerou1ORCID,Huang Fei2,Zhao Lan3,Waldren George C1,Jiang Qi1,Chen Sherry X1,Wang Bonnie1,Guo Wei2,Zhang David Y1ORCID,Zhang Jinny X1ORCID

Affiliation:

1. Department of Innovation, NuProbe USA , Houston , TX  77054 , USA

2. Department of Laboratory Medicine, Zhongshan Hospital, Fudan University , Shanghai , Shanghai  200032 , China

3. Department of Respiratory Diseases, Shanghai Pulmonary Hospital, Tongji University School of Medicine , Shanghai , Shanghai  200433 , China

Abstract

Abstract Quantitative PCR (qPCR) is the gold standard for detection and quantitation of known DNA targets, but the scarcity of spectrally distinct fluorophores and filter sets limits the number of detectable targets. Here, we introduce color cycle multiplex amplification (CCMA) to significantly increase the number of detectable DNA targets in a single qPCR reaction using standard instrumentation. In CCMA, presence of one DNA target species results in a pre-programmed pattern of fluorescence increases. This pattern is distinguished by cycle thresholds (Cts) through rationally designed delays in amplification. For example, we design an assay wherein Staphylococcus aureus sequentially induces FAM, then Cy5.5, then ROX fluorescence increases with more than 3 cycles between each signal. CCMA offers notably higher potential for multiplexing because it uses fluorescence permutation rather than combination. With 4 distinct fluorescence colors, CCMA theoretically allows the detection of up to 136 distinct DNA target sequences using fluorescence permutation. Experimentally, we demonstrated a single-tube qPCR assay screening 21 sepsis-related bacterial DNA targets in samples of blood, sputum, pleural effusion and bronchoalveolar lavage fluid, with 89% clinical sensitivity and 100% clinical specificity, showing its potential as a powerful tool for advanced quantitative screening in molecular diagnostics.

Funder

NuProbe USA

Publisher

Oxford University Press (OUP)

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