# Integrating RPA-LFD and TaqMan qPCR for Rapid On-Site Screening and Accurate Laboratory Identification of Coilia brachygnathus and Coilia nasus in the Yangtze River

**Authors:** Yu Lin, Suyan Wang, Min Zhang, Na Wang, Hongli Jing, Jizhou Lv, Shaoqiang Wu

PMC · DOI: 10.3390/foods14203484 · Foods · 2025-10-13

## TL;DR

This paper introduces a new method combining two DNA tests to accurately and quickly identify two fish species in the Yangtze River.

## Contribution

The novel integration of RPA-LFD for rapid screening and TaqMan qPCR for precise genotyping of Coilia brachygnathus and Coilia nasus.

## Key findings

- RPA-LFD assays enabled visual detection of species within 10 minutes at 37°C with high sensitivity.
- TaqMan qPCR accurately distinguished the two species with 100% concordance in validation tests.
- The dual method combines portability for field use with high accuracy for lab confirmation.

## Abstract

Accurate differentiation between Coilia brachygnathus and Coilia nasus is imperative for the effective management of fisheries, the conservation of aquatic ecosystems, and the mitigation of commercial fraud. Current morphological identification remains challenging due to their high morphological similarity—particularly for processed samples—while conventional molecular methods often lack the speed or specificity required for field applications or high-throughput screening. In this study, a novel integrated approach was developed and validated, combining TaqMan quantitative real-time PCR (qPCR). for precise genotyping of C. brachygnathus and C. nasus with Recombinase Polymerase Amplification coupled with Lateral Flow Dipstick (RPA-LFD) for rapid on-site screening. First, species-specific RPA-LFD assays were designed to target the mitochondrial COI gene sequence. This enabled visual detection within 10 min at 37 °C, with a sensitivity of 102 copies/μL, and required no complex equipment. A dual TaqMan MGB qPCR assay was further developed by validating stable differentiating SNPs (chr21:3798155, C/T) between C. brachygnathus and C. nasus, using FAM/VIC dual-labeled MGB probes. Results showed that this assay could distinguish the two species in a single tube: for C. brachygnathus, Ct values in the FAM channel were significantly earlier than those in the VIC channel (ΔCt ≥ 1), with a FAM detection limit of 125 copies/reaction; for C. nasus, only VIC channel amplification was observed, with a detection limit as low as 12.5 copies/reaction. Validation with 171 known tissue samples demonstrated 100% concordance with expected species identities. This integrated approach effectively combines the high accuracy and quantitative capacity of TaqMan qPCR for confirmatory laboratory genotyping with the speed, simplicity, and portability of RPA-LFD for initial field or point-of-need screening. This reliable, efficient, and user-friendly technique provides a powerful tool for resource management, biodiversity monitoring, and ensuring the authenticity of high-quality C. brachygnathus and C. nasus.

## Linked entities

- **Genes:** COX1 (cytochrome c oxidase subunit I) [NCBI Gene 4512]
- **Species:** Coilia brachygnathus (taxon 411919), Coilia nasus (taxon 365059)

## Full-text entities

- **Chemicals:** MGB (-)
- **Species:** Coilia nasus (estuarine tapertail anchovy, species) [taxon 365059], Coilia brachygnathus (Yangtse grenadier anchovy, species) [taxon 411919]

## Full text

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## Figures

9 figures with captions in the complete paper: https://tomesphere.com/paper/PMC12564251/full.md

## References

45 references — full list in the complete paper: https://tomesphere.com/paper/PMC12564251/full.md

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Source: https://tomesphere.com/paper/PMC12564251