Full-length 16S rDNA sequencing based on Oxford Nanopore Technologies revealed the association between gut-pharyngeal microbiota and tuberculosis in cynomolgus macaques

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作者
Vorthon Sawaswong
Prangwalai Chanchaem
Pavit Klomkliew
Suwatchareeporn Rotcheewaphan
Suthirote Meesawat
Taratorn Kemthong
Mutchamon Kaewparuehaschai
Kirana Noradechanon
Monya Ekatat
Reka Kanitpun
Prapaporn Srilohasin
Saradee Warit
Angkana Chaiprasert
Suchinda Malaivijitnond
Sunchai Payungporn
机构
[1] Chulalongkorn University,Department of Biochemistry, Center of Excellence in Systems Microbiology, Faculty of Medicine
[2] Mahidol University,Department of Biochemistry, Faculty of Science
[3] Chulalongkorn University,Department of Microbiology, Faculty of Medicine
[4] Chulalongkorn University,National Primate Research Center of Thailand
[5] Chulalongkorn University,Department of Biology, Faculty of Science
[6] Wildlife Conservation Office,Office for Research, Faculty of Medicine Siriraj Hospital
[7] Department of National Parks Wildlife and Plant Conservation,Department of Microbiology, Faculty of Medicine Siriraj Hospital
[8] National Institute of Animal Health (NIAH),Industrial Tuberculosis Team, Industrial Medical Molecular Biotechnology Research Group, National Center for Genetic Engineering and Biotechnology
[9] Mahidol University,undefined
[10] Mahidol University,undefined
[11] National Science and Technology Development Agency,undefined
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关键词
Tuberculosis; Cynomolgus macaque; Gut-pharyngeal microbiome; Full-length 16S sequencing;
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摘要
Tuberculosis (TB) is an infectious disease caused by the Mycobacterium tuberculosis complex (Mtbc), which develops from asymptomatic latent TB to active stages. The microbiome was purposed as a potential factor affecting TB pathogenesis, but the study was limited. The present study explored the association between gut-pharyngeal microbiome and TB stages in cynomolgus macaques using the full-length 16S rDNA amplicon sequencing based on Oxford Nanopore Technologies. The total of 71 macaques was divided into TB (−) control, TB (+) latent and TB (+) active groups. The differential abundance analysis showed that Haemophilus hemolyticus was decreased, while Prevotella species were increased in the pharyngeal microbiome of TB (+) macaques. In addition, Eubacterium coprostanoligenes in the gut was enriched in TB (+) macaques. Alteration of these bacteria might affect immune regulation and TB severity, but details of mechanisms should be further explored and validated. In summary, microbiota may be associated with host immune regulation and affect TB progression. The findings suggested the potential mechanisms of host-microbes interaction, which may improve the understanding of the role of microbiota and help develop therapeutics for TB in the future.
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