Publication:
Comparative whole-genome sequence analysis of Mycobacterium tuberculosis isolated from pulmonary tuberculosis and tuberculous lymphadenitis patients in Northwest Ethiopia

dc.contributor.authorMekonnen, Daniel
dc.contributor.authorMunshea, Abaineh
dc.contributor.authorNibret, Endalkachew
dc.contributor.authorAdnew, Bethlehem
dc.contributor.authorHerrera-León, Silvia
dc.contributor.authorAmor Aramendia, Aranzazu
dc.contributor.authorBenito, Agustin
dc.contributor.authorAbascal, Estefanía
dc.contributor.authorJacqueline Forget, Camille
dc.contributor.authorAseffa, Abraham
dc.contributor.authorHerrera-Leon, Laura
dc.contributor.funderBahir Dar University (Etiopía)es_ES
dc.contributor.funderAmhara National Regional State Public Health Institute (Etiopía)es_ES
dc.contributor.funderInstituto de Salud Carlos IIIes_ES
dc.date.accessioned2023-08-25T09:27:00Z
dc.date.available2023-08-25T09:27:00Z
dc.date.issued2023-06
dc.description.abstractBackground: Tuberculosis (TB), caused by the Mycobacterium tuberculosis complex (MTBC), is a chronic infectious disease with both pulmonary and extrapulmonary forms. This study set out to investigate and compare the genomic diversity and transmission dynamics of Mycobacterium tuberculosis (Mtb) isolates obtained from tuberculous lymphadenitis (TBLN) and pulmonary TB (PTB) cases in Northwest Ethiopia. Methods: A facility-based cross-sectional study was conducted using two groups of samples collected between February 2021 and June 2022 (Group 1) and between June 2020 and June 2022 (Group 2) in Northwest Ethiopia. Deoxyribonucleic acid (DNA) was extracted from 200 heat-inactivated Mtb isolates. Whole-genome sequencing (WGS) was performed from 161 isolates having ≥1 ng DNA/μl using Illumina NovaSeq 6000 technology. Results: From the total 161 isolates sequenced, 146 Mtb isolates were successfully genotyped into three lineages (L) and 18 sub-lineages. The Euro-American (EA, L4) lineage was the prevailing (n = 100; 68.5%) followed by Central Asian (CAS, L3, n = 43; 25.3%) and then L7 (n = 3; 2.05%). The L4.2.2.ETH sub-lineage accounted for 19.9%, while Haarlem estimated at 13.7%. The phylogenetic tree revealed distinct Mtb clusters between PTB and TBLN isolates even though there was no difference at lineages and sub-lineages levels. The clustering rate (CR) and recent transmission index (RTI) for PTB were 30 and 15%, respectively. Similarly, the CR and RTI for TBLN were 31.1 and 18 %, respectively. Conclusion and recommendations: PTB and TBLN isolates showed no Mtb lineages and sub-lineages difference. However, at the threshold of five allelic distances, Mtb isolates obtained from PTB and TBLN form distinct complexes in the phylogenetic tree, which indicates the presence of Mtb genomic variation among the two clinical forms. The high rate of clustering and RTI among TBLN implied that TBLN was likely the result of recent transmission and/or reactivation from short latency. Hence, the high incidence rate of TBLN in the Amhara region could be the result of Mtb genomic diversity and rapid clinical progression from primary infection and/or short latency. To validate this conclusion, a similar community-based study with a large sample size and better sampling technique is highly desirable. Additionally, analysis of genomic variants other than phylogenetic informative regions could give insightful information. Combined analysis of the host and the pathogen genome (GXG) together with environmental (GxGxE) factors could give comprehensive co-evolutionary information.es_ES
dc.description.peerreviewedes_ES
dc.description.sponsorshipThe sample collection was funded by the Institute of Biotechnology, Bahir Dar University through the EN mega project. The Mtb culture and identification-related lab supply were supported by Amhara Public Health Institute, Bahir Dar Ethiopia. The whole-genome sequencing (WGS) and publication fee was covered by the National Center of Microbiology, Institute of Carlos III, Madrid, Spain. International Federation for Clinical Chemistry (IFCC) gave financial support to DM through the IFCC Professional Scientific Exchange Programme (PSEP) for 3-month WGS laboratory work.es_ES
dc.format.page1211267es_ES
dc.format.volume14es_ES
dc.identifier.citationFront Microbiol. 2023 Jun 30;14:1211267.es_ES
dc.identifier.doi10.3389/fmicb.2023.1211267es_ES
dc.identifier.issn1664-302Xes_ES
dc.identifier.journalFrontiers in microbiologyes_ES
dc.identifier.pubmedID37455714es_ES
dc.identifier.urihttp://hdl.handle.net/20.500.12105/16344
dc.language.isoenges_ES
dc.publisherFrontiers Mediaes_ES
dc.relation.publisherversionhttps://doi.org/10.3389/fmicb.2023.1211267es_ES
dc.repisalud.centroISCIII::Centro Nacional de Microbiologíaes_ES
dc.repisalud.centroISCIII::Centro Nacional de Medicina Tropicales_ES
dc.repisalud.institucionISCIIIes_ES
dc.rights.accessRightsopen accesses_ES
dc.rights.licenseAtribución 4.0 Internacional*
dc.rights.urihttp://creativecommons.org/licenses/by/4.0/*
dc.subjectMycobacterium tuberculosises_ES
dc.subjectTuberculous lymphadenitises_ES
dc.subjectPulmonary tuberculosises_ES
dc.subjectWhole-genome sequencinges_ES
dc.subjectEthiopiaes_ES
dc.titleComparative whole-genome sequence analysis of Mycobacterium tuberculosis isolated from pulmonary tuberculosis and tuberculous lymphadenitis patients in Northwest Ethiopiaes_ES
dc.typeresearch articlees_ES
dc.type.hasVersionVoRes_ES
dspace.entity.typePublication
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relation.isAuthorOfPublication07d1c759-cc3a-470f-8811-a5264c9a08dd
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relation.isAuthorOfPublication9bbbbb77-bd32-466c-820b-44bdad635fc4
relation.isAuthorOfPublication.latestForDiscovery82a8967d-0949-402d-a319-43330521cad3

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