ABSTRACT
Due to a resurgence of flea-borne rickettsioses in Orange County, California, we investigated the etiologies of rickettsial infections of Ctenocephalides felis, the predominant fleas species obtained from opossums (Didelphis virginiana) and domestic cats (Felis catus), collected from case exposure sites and other areas in Orange County. In addition, we assessed the prevalence of IgG antibodies against spotted fever group (SFGR) and typhus group (TGR) rickettsiae in opossum sera. Of the 597 flea specimens collected from opossums and cats, 37.2% tested positive for Rickettsia. PCR and sequencing of rickettsial genes obtained from C. felis flea DNA preparations revealed the presence of R. typhi (1.3%), R. felis (28.0%) and R. felis-like organisms (7.5%). Sera from opossums contained TGR-specific (40.84%), but not SFGR-specific antibodies. The detection of R. felis and R. typhi in the C. felis fleas in Orange County highlights the potential risk for human infection with either of these pathogens, and underscores the need for further investigations incorporating specimens from humans, animal hosts, and invertebrate vectors in endemic areas. Such studies will be essential for establishing a link in the ongoing flea-borne rickettsioses outbreaks.
Subject(s)
Cats/parasitology , Ctenocephalides/microbiology , Flea Infestations/veterinary , Insect Vectors/microbiology , Opossums/parasitology , Rickettsia Infections/veterinary , Rickettsia/isolation & purification , Animals , California/epidemiology , Cats/blood , Cats/microbiology , Disease Outbreaks , Flea Infestations/complications , Humans , Immunoglobulin G/blood , Opossums/blood , Opossums/microbiology , Rickettsia Infections/blood , Rickettsia Infections/epidemiology , Rickettsia Infections/transmission , Rickettsia felis/isolation & purification , Rickettsia typhi/isolation & purificationABSTRACT
To increase knowledge of undifferentiated fevers in Kenya, we tested paired serum samples from febrile children in western Kenya for antibodies against pathogens increasingly recognized to cause febrile illness in Africa. Of patients assessed, 8.9%, 22.4%, 1.1%, and 3.6% had enhanced seroreactivity to Coxiella burnetii, spotted fever group rickettsiae, typhus group rickettsiae, and scrub typhus group orientiae, respectively.
Subject(s)
Q Fever/epidemiology , Rickettsia Infections/epidemiology , Scrub Typhus/epidemiology , Antibodies, Bacterial/blood , Antibodies, Bacterial/immunology , Child , Child, Preschool , Cross Reactions , Enzyme-Linked Immunosorbent Assay , Female , Fever/epidemiology , Fever/microbiology , History, 21st Century , Humans , Infant , Kenya/epidemiology , Male , Q Fever/diagnosis , Q Fever/history , Q Fever/microbiology , Rickettsia Infections/diagnosis , Rickettsia Infections/history , Rickettsia Infections/microbiology , Scrub Typhus/diagnosis , Scrub Typhus/history , Scrub Typhus/microbiology , SeasonsABSTRACT
Human infections with Rickettsia felis have been reported worldwide. Recent studies have revealed the presence of many closely related but unique rickettsiae, referred to as Rickettsia felis-like organisms (RFLO), identified in various arthropods. Due to the recent discovery of the lack of specificity of earlier R. felis-specific assays, there has become a need to develop a new generation of R. felis-specific molecular assays that will differentiate R. felis not only from other rickettsiae but more importantly from other members of the R. felis genogroup that may not be pathogenic to humans. This new generation of assays is essential for determining the true risk for flea-borne spotted fever (FBSF) by surveying arthropod vectors/hosts. Because of the lack of specificity of previous assays developed to detect R. felis infections, prior surveys may have overestimated the prevalence of R. felis in arthropod vectors and thus the perceived risk of FBSF. We have developed a specific quantitative real-time polymerase chain reaction (qPCR) assay to detect R. felis (RfelB). Specificity of the assay was determined by testing it with a panel of 17 related Rickettsia species and 12 nonrickettsial bacterial DNA preparations. The RfelB qPCR assay was positive for R. felis DNA and negative for all of the 17 related Rickettsia species and 12 nonrickettsia bacterial DNA preparations. The limit of detection of the RfelB qPCR assay was determined to be two copies (two genoequivalents) per microliter of R. felis target ompB fragment-containing plasmid. Validation of the RfelB qPCR assay was accomplished by testing 83 previously sequence-confirmed R. felis and RFLOs containing DNA preparations from human and flea samples collected from different geographical locations around the world. This assay will be useful for rapid detection, identification, and enumeration of R. felis, an emerging human pathogen of worldwide importance, from both clinical and environmental samples.
