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Molecular detection of Rickettsia felis and Candidatus Rickettsia Asemboensis in fleas from human habitats, Asembo, Kenya

dc.contributor.authorJiang, Ju
dc.contributor.authorMaina, Alice N.
dc.contributor.authorKnobel, Darryn L.
dc.contributor.authorCleaveland, Sarah
dc.contributor.authorLaudisoit, Anne
dc.contributor.authorWamburu, Kabura
dc.contributor.authorOgola, Eric
dc.contributor.authorParola, Philippe
dc.contributor.authorBreiman, Robert F.
dc.contributor.authorNjenga, Kariuki M.
dc.contributor.authorRichards, Allen L.
dc.date.accessioned2018-11-21T12:12:28Z
dc.date.available2018-11-21T12:12:28Z
dc.date.issued2013
dc.identifier.uri10.1089/vbz.2012.1123
dc.identifier.urihttp://ir.jooust.ac.ke:8080/xmlui/handle/123456789/2947
dc.description.abstractThe flea-borne rickettsioses murine typhus (Rickettsia typhi) and flea-borne spotted fever (FBSF) (Rickettsia felis) are febrile diseases distributed among humans worldwide. Murine typhus has been known to be endemic to Kenya since the 1950s, but FBSF was only recently documented in northeastern (2010) and western (2012) Kenya. To characterize the potential exposure of humans in Kenya to flea-borne rickettsioses, a total of 330 fleas (134 pools) including 5 species (Xenopsylla cheopis, Ctenocephalides felis, Ctenocephalides canis, Pulex irritans, and Echidnophaga gallinacea) were collected from domestic and peridomestic animals and from human dwellings within Asembo, western Kenya. DNA was extracted from the 134 pooled flea samples and 89 (66.4%) pools tested positively for rickettsial DNA by 2 genus-specific quantitative real-time PCR (qPCR) assays based upon the citrate synthase (gltA) and 17-kD antigen genes and the Rfelis qPCR assay. Sequences from the 17-kD antigen gene, the outer membrane protein (omp)B, and 2 R. felis plasmid genes (pRF and pRFd) of 12 selected rickettsiapositive samples revealed a unique Rickettsia sp. (n = 11) and R. felis (n = 1). Depiction of the new rickettsia by multilocus sequence typing (MLST) targeting the 16S rRNA (rrs), 17-kD antigen gene, gltA, ompA, ompB, and surface cell antigen 4 (sca4), shows that it is most closely related to R. felis but genetically dissimilar enough to be considered a separate species provisionally named Candidatus Rickettsia asemboensis. Subsequently, 81 of the 134 (60.4%) flea pools tested positively for Candidatus Rickettsia asemboensis by a newly developed agentspecific qPCR assay, Rasemb. R. felis was identified in 9 of the 134 (6.7%) flea pools, and R. typhi the causative agent of murine typhus was not detected in any of 78 rickettsia-positive pools assessed using a species-specific qPCR assay, Rtyph. Two pools were found to contain both R. felis and Candidatus Rickettsia asemboensis DNA and 1 pool contained an agent, which is potentially new.en_US
dc.description.sponsorshipGlobal Emerging Infections Surveillance and Response Systemen_US
dc.language.isoenen_US
dc.publisherMary Ann Liebert, Inc.en_US
dc.subjectRickettsiaen_US
dc.subjectFleasen_US
dc.subjectPCRen_US
dc.subjectMultilocus sequence typingen_US
dc.subjectMultilocus sequence typingen_US
dc.subjectSurveillanceen_US
dc.titleMolecular detection of Rickettsia felis and Candidatus Rickettsia Asemboensis in fleas from human habitats, Asembo, Kenyaen_US
dc.typeArticleen_US


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