Targeted culture-independent sequencing identifies emergence of macrolide-resistant Bordetella pertussis in Australia

百日咳博德特菌 微生物学 生物 病毒学 遗传学 细菌
作者
Winkie Fong,Rebecca J. Rockett,Kingsley King-Gee Tam,Trang Nguyen,Eby Sim,Enoch Tay,C. J. E. Suster,Jessica E. Agius,Shona Chandra,A. Watt,David Speers,Maryza Graham,Thomas Tran,Chuan Kok Lim,Michael C. Wehrhahn,Andrew N. Ginn,Darcy Gray,Jennifer Robson,Indya Gardner,Rodney McDougall
出处
期刊:Cold Spring Harbor Laboratory - medRxiv
标识
DOI:10.1101/2024.12.19.24319368
摘要

Bordetella pertussis continues to circulate globally despite wide-spread vaccination, with an emergent international epidemic in 2024. The resurgence of disease is confounded by the emergence of pertactin-deficient, macrolide-resistant B. pertussis (MRBP) strains in Asia and Europe, which are under-recognised using traditional diagnostic and surveillance methods. This study addressed these gaps by applying a probe-capture hybridisation technique, which enables targeted culture-independent sequencing of genomes (tNGS) directly from respiratory specimens. Seven co-circulating lineages of B. pertussis were identified in Australia, including two associated with MRBP. Eight epidemiologically unrelated and geographically dispersed cases of MRBP in Australia with a A2037G mutation in all three copies of 23S rRNA were documented, three of which were confirmed by phenotypic testing and sequencing of corresponding isolates. The estimated rate of MRBP among B. pertussis PCR positive cases was 4.4%. This study demonstrated the value of tNGS based on target enrichment and probe capture sets designed for respiratory pathogens for public health laboratory surveillance of pertussis. This approach can improve the resolution and completeness of B. pertussis surveillance given the increasing diversity and vaccine evasion capability of this pathogen.
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