High prevalence of spotted fever group rickettsiae in Amblyomma variegatum from Uganda and their identification using sizes of intergenic spacers

Ticks Tick Borne Dis. 2013 Dec;4(6):506-12. doi: 10.1016/j.ttbdis.2013.07.001. Epub 2013 Oct 26.

Abstract

The spotted fever group (SFG) rickettsiae are obligate intracellular bacteria transmitted by ticks that cause several tick-borne rickettsioses in humans worldwide. This study was intended to determine the prevalence of SFG rickettsiae in Amblyomma variegatum from 7 districts across Uganda. In addition to sequencing of gltA and ompA genes, identification of Rickettsia species based on the sizes of highly variable intergenic spacers, namely, dksA-xerC, mppA-purC, and rpmE-tRNA(fMet) was carried out. Application of multiplex PCR for simultaneous amplification of 3 spacers combined with capillary electrophoresis separation allowed simple, accurate, and high-throughput fragment sizing with considerable time and cost savings. Rickettsia genus-specific real-time PCR detected 136 positives out of 140 samples, giving an overall prevalence of 97.1%. Most samples (n=113) had a size combination of 225, 195, and 341 bp for dksA-xerC, mppA-purC, and rpmE-tRNA(fMet), respectively, which was identical to that of R. africae, a causative agent of African tick bite fever. In addition, several samples had size variants in either dksA-xerC or rpmE-tRNA(fMet). Nonetheless, the partial sequences of gltA and ompA genes of samples of all size combinations showed the greatest similarity to R. africae (99.3-100% for gltA and 98.1-100% for ompA). Given these results, it is highly possible that the tested ticks were infected with R. africae or closely related species. This is a first report on molecular genetic detection of R. africae and its high endemicity in Uganda. Clinicians in this country should be aware of this pathogen as a cause of non-malarial febrile illness. This study provided a starting point for the development of Rickettsia species identification based on the sizes of intergenic spacers. The procedure is simple, rapid, and cost-effective to perform; hence it might be particularly well suited for preliminary species identification in epidemiological investigations. The results may be more detailed and reliable when simultaneous sequencing analysis is performed.

Keywords: African tick bite fever; Amblyomma variegatum; Intergenic spacer; Rickettsia africae; Uganda; Zoonosis.

Publication types

  • Research Support, Non-U.S. Gov't

MeSH terms

  • Animals
  • Arachnid Vectors / microbiology*
  • Bacterial Proteins / genetics
  • Base Sequence
  • Cattle
  • Cattle Diseases / microbiology
  • Cattle Diseases / parasitology
  • Cattle Diseases / transmission*
  • DNA, Bacterial / chemistry
  • DNA, Bacterial / genetics
  • DNA, Intergenic / chemistry
  • DNA, Intergenic / genetics
  • Female
  • Ixodidae / microbiology*
  • Male
  • Molecular Sequence Data
  • Multiplex Polymerase Chain Reaction / veterinary
  • Prevalence
  • Real-Time Polymerase Chain Reaction / veterinary
  • Rickettsia / classification
  • Rickettsia / genetics
  • Rickettsia / isolation & purification*
  • Rickettsia Infections / epidemiology
  • Rickettsia Infections / transmission
  • Rickettsia Infections / veterinary
  • Sequence Analysis, DNA / veterinary
  • Tick Infestations / microbiology
  • Tick Infestations / parasitology
  • Tick Infestations / veterinary*
  • Tick-Borne Diseases / epidemiology
  • Tick-Borne Diseases / microbiology
  • Tick-Borne Diseases / veterinary*
  • Time Factors
  • Uganda / epidemiology
  • Zoonoses

Substances

  • Bacterial Proteins
  • DNA, Bacterial
  • DNA, Intergenic

Associated data

  • GENBANK/AB763400
  • GENBANK/AB763401
  • GENBANK/AB763402
  • GENBANK/AB763403
  • GENBANK/AB763404
  • GENBANK/AB763405
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