Literature DB >> 27388326

Development and evaluation of a non-ribosomal random PCR and next-generation sequencing based assay for detection and sequencing of hand, foot and mouth disease pathogens.

Anh To Nguyen1, Thanh Tan Tran2, Van Minh Tu Hoang3, Ngoc My Nghiem4, Nhu Nguyen Truc Le2, Thanh Thi My Le4, Qui Tu Phan4, Khanh Huu Truong5, Nhan Nguyen Thanh Le5, Viet Lu Ho3, Viet Chau Do3, Tuan Manh Ha3, Hung Thanh Nguyen5, Chau Van Vinh Nguyen4, Guy Thwaites2,6, H Rogier van Doorn2,6, Tan Van Le2.   

Abstract

BACKGROUND: Hand, foot and mouth disease (HFMD) has become a major public health problem across the Asia-Pacific region, and is commonly caused by enterovirus A71 (EV-A71) and coxsackievirus A6 (CV-A6), CV-A10 and CV-A16. Generating pathogen whole-genome sequences is essential for understanding their evolutionary biology. The frequent replacements among EV serotypes and a limited numbers of available whole-genome sequences hinder the development of overlapping PCRs for whole-genome sequencing. We developed and evaluated a non-ribosomal random PCR (rPCR) and next-generation sequencing based assay for sequence-independent whole-genome amplification and sequencing of HFMD pathogens. A total of 16 EV-A71/CV-A6/CV-A10/CV-A16 PCR positive rectal/throat swabs (Cp values: 20.9-33.3) were used for assay evaluation.
RESULTS: Our assay evidently outperformed the conventional rPCR in terms of the total number of EV-A71 reads and the percentage of EV-A71 reads: 2.6 % (1275/50,000 reads) vs. 0.1 % (31/50,000) and 6 % (3008/50,000) vs. 0.9 % (433/50,000) for two samples with Cp values of 30 and 26, respectively. Additionally the assay could generate genome sequences with the percentages of coverage of 94-100 % of 4 different enterovirus serotypes in 73 % of the tested samples, representing the first whole-genome sequences of CV-A6/10/16 from Vietnam, and could assign correctly serotyping results in 100 % of 24 tested specimens. In all but three the obtained consensuses of two replicates from the same sample were 100 % identical, suggesting that our assay is highly reproducible.
CONCLUSIONS: In conclusion, we have successfully developed a non-ribosomal rPCR and next-generation sequencing based assay for sensitive detection and direct whole-genome sequencing of HFMD pathogens from clinical samples.

Entities:  

Keywords:  Enterovirus A; FR26RV-Endoh primer; Hand, foot and mouth disease; Next-generation sequencing; Random PCR

Mesh:

Year:  2016        PMID: 27388326      PMCID: PMC4937578          DOI: 10.1186/s12985-016-0580-9

Source DB:  PubMed          Journal:  Virol J        ISSN: 1743-422X            Impact factor:   4.099


  35 in total

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