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Volume 29, Number 5—May 2023
Research Letter

Presence of Burkholderia pseudomallei in Soil, Nigeria, 2019

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Author affiliations: Amsterdam UMC location University of Amsterdam, Amsterdam, the Netherlands (J. Savelkoel, D.W. Notermans, S. Matamoros, W.J. Wiersinga, E. Birnie); Lagos University Teaching Hospital, Lagos, Nigeria (R.O. Oladele, R.F. Peters, J.O. Makinwa, A.S. Akanmu); College of Medicine University of Lagos, Lagos, Nigeria (R.O. Oladele, A.S. Akanmu); Ebonyi State University, Abakaliki, Nigeria (C.K. Ojide); Alex Ekwueme Federal University Teaching Hospital, Abakaliki, Nigeria (C.K. Ojide, U.S. Unigwe); National Institute for Public Health and the Environment (RIVM), Bilthoven, the Netherlands (D.W. Notermans, M.C. de Vries, M.A.E. Sunter); Federal Medical Centre, Abuja, Nigeria (N. Abdullahi); University of Nigeria Teaching Hospital, Enugu, Nigeria (U.S. Unigwe)

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Abstract

Melioidosis, caused by the soil-dwelling bacterium Burkholderia pseudomallei, is predicted to be endemic in Nigeria but is only occasionally reported. This report documents the systematic identification of the presence of B. pseudomallei and B. thailandensis in the soil across multiple states in Nigeria.

The gram-negative, soil-dwelling bacterium Burkholderia pseudomallei is the causative agent of melioidosis, which is an important cause of lethal community-acquired sepsis throughout the tropics (1). Melioidosis is predicted to be endemic in Nigeria, a country with the highest estimated annual incidence, mortality, and disease burden in Africa, partly explained by its suitable environment and large population (24). Clinical evidence of melioidosis in Nigeria is scarce and based only on traveler-associated cases in the United Kingdom and reports from Nigeria presuming the presence of B. pseudomallei (47). This study was a collaborative effort prompted by the African Melioidosis Workshop in Lagos, Nigeria (4); our goal was to determine the environmental presence of B. pseudomallei in Nigeria. Ethics approval was obtained from the National Health Research Ethics Committee of Nigeria (approval no. NHREC/01/01/2007-26/03/2019).

We performed an environmental soil sampling study based on consensus guidelines for the identification of B. pseudomallei (8). We consulted local residents and maps to select sites associated with the occurrence of B. pseudomallei, as we have done previously (9). Using a fixed interval grid and samples taken 5 meters apart, we collected 100 soil samples per site across 8 sites in Nigeria during the rainy season in April–May 2019 (Table; Appendix). We collected a total of 800 samples in the northwestern state Kebbi, southwestern state Ogun, and southeastern states Ebonyi and Enugu. We collected soil at a depth of 65 cm and processed 10 g of soil within 7 days to enable selective enriched culture (8,10). We screened isolates by using colony morphology and, if results were suspect, used matrix-assisted laser desorption/ionization-time of flight mass spectrometry (MALDI Biotyper Compass v4.1 and Compass Library v10; Bruker Daltonics, https://www.bruker.com). We subjected all presumptive B. pseudomallei isolates to real-time multiplex PCR and performed whole-genome sequencing on 9 B. pseudomallei isolates and 3 B. thailandensis isolates by using the NextSeq 500/550 platform (Illumina, https://www.illumina.com) (Appendix). We then included the same B. pseudomallei isolates in our phylogenetic comparison and used them for antimicrobial susceptibility testing (Appendix). Sequences for the samples in this study are available on the European Nucleotide Archive database (project number PRJEB54705, sample accession nos. ERS12451640–51; https://www.ebi.ac.uk/ena/browser/home).

By using the methods described, we isolated B. pseudomallei from 58 (7.3%) of 800 samples in 5 (62.5%) of the 8 sampling sites (Table; Appendix). We observed the highest positivity in the southeastern states, with rates as high as 38% in Ebonyi and 14% in Enugu. We also isolated the nonpathogenic B. thailandensis from 193 (24.1%) of 800 samples in 4 (50%) of the 8 sampling sites. Antimicrobial susceptibility of the B. pseudomallei isolates displayed overall sensitivity against antibiotic agents commonly used for the treatment of melioidosis, such as ceftazidime, meropenem, and trimethoprim/sulfamethoxazole (Appendix).

Figure

Phylogenetic tree of Burkholderia pseudomallei genomes from Nigeria (orange text) and additional genomes originating from Africa, all retrieved from the European Nucleotide Archive database. Tree generated by FastTree (http://www.microbesonline.org/fasttree) based on core single-nucleotide polymorphisms distance and visualized with iTOL (https://itol.embl.de). Colors indicate countries of origin. Asterisk indicates a previously sequenced, traveler-associated strain. Scale bar indicates number of nucleotide substitutions per site.

Figure. Phylogenetic tree of Burkholderia pseudomallei genomes from Nigeria (orange text) and additional genomes originating from Africa, all retrieved from the European Nucleotide Archive database. Tree generated by FastTree (...

We conducted phylogenetic analysis of our 9 sequenced B. pseudomallei isolates and 13 additional genomes originating from Africa, all retrieved from the European Nucleotide Archive database. The phylogenetic tree revealed a cluster of predominantly continental African origin that included all of the soil isolates from Nigeria and a cluster of strains derived mainly from the Indian Ocean region (Figure). Our B. pseudomallei isolates did not closely match the previously sequenced traveler-associated strain from Nigeria (ERR298772) (7): the genome differed by 8,370 to 9,431 core single-nucleotide polymorphisms. We speculated that the higher positivity in the southeastern states reflects the relatively high annual precipitation in southeastern Nigeria as compared with sampling sites in the northwestern and southwestern states (Appendix).

Adopting a culture-based approach, combined with matrix-assisted laser desorption/ionization-time of flight mass spectrometry, real-time PCR, and whole genome sequencing allowed us to identify the environmental presence of B. pseudomallei. Limitations of our study include possible sampling errors and false-negative samples because we relied on a culture-based approach instead of using an additional quantitative PCR on soil samples (9). Moreover, we did not collect soil samples in multiple seasons to investigate a seasonal pattern, nor did we collect water or air samples.

In conclusion, we documented the systematic confirmation of the environmental presence of B. pseudomallei and B. thailandensis across multiple states in Nigeria. We identified the highest B. pseudomallei positivity rates in the southeastern states Ebonyi and Enugu. Phylogenetic analysis clustered our B. pseudomallei isolates with previous genomes that originated mostly from continental Africa. Our results highlight the probability of unrecognized melioidosis in Nigeria and warrant the attention of health workers and public health officials. Improving capacity and increasing awareness, together with environmental, serologic, and disease surveillance, is needed to increase our understanding of the melioidosis burden within Nigeria.

Mr. Savelkoel is a researcher at the Center for Experimental and Molecular Medicine of Amsterdam UMC. His research interests include the global distribution and global health aspects of melioidosis.

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Acknowledgments

We thank all participants of the African Melioidosis Workshop in Lagos, Nigeria, and everyone who helped with the soil sampling. We also express our gratitude to Michelle B.S. Menig, Cornelia M. Prtenjaca Wolbers, Maaike J.C. van den Beld, and Frans A.G. Reubsaet for their expert technical assistance.

This work was supported by an Amsterdam UMC PhD Scholarship to Jelmer Savelkoel in 2021 and a research grant from the European Society of Clinical Microbiology and Infectious Diseases to Emma Birnie in 2018.

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References

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Cite This Article

DOI: 10.3201/eid2905.221138

Original Publication Date: April 11, 2023

1These first authors contributed equally to this article.

2These senior authors contributed equally to this article.

Table of Contents – Volume 29, Number 5—May 2023

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Jelmer Savelkoel, Amsterdam UMC location University of Amsterdam, Center for Experimental and Molecular Medicine, Meibergdreef 9, 1105 AZ, Room T1.0-234, Amsterdam, the Netherlands

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Page created: April 04, 2023
Page updated: April 21, 2023
Page reviewed: April 21, 2023
The conclusions, findings, and opinions expressed by authors contributing to this journal do not necessarily reflect the official position of the U.S. Department of Health and Human Services, the Public Health Service, the Centers for Disease Control and Prevention, or the authors' affiliated institutions. Use of trade names is for identification only and does not imply endorsement by any of the groups named above.
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