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Examination of Rickettsial Host Range for Shuttle Vectors Based on dnaA and parA Genes from the pRM Plasmid of Rickettsia monacensis.
Burkhardt, Nicole Y; Price, Lisa D; Wang, Xin-Ru; Heu, Chan C; Baldridge, Gerald D; Munderloh, Ulrike G; Kurtti, Timothy J.
  • Burkhardt NY; University of Minnesotagrid.17635.36, Department of Entomology, Saint Paul, Minnesota, USA.
  • Price LD; University of Minnesotagrid.17635.36, Department of Entomology, Saint Paul, Minnesota, USA.
  • Wang XR; University of Minnesotagrid.17635.36, Department of Entomology, Saint Paul, Minnesota, USA.
  • Heu CC; University of Minnesotagrid.17635.36, Department of Entomology, Saint Paul, Minnesota, USA.
  • Baldridge GD; University of Minnesotagrid.17635.36, Department of Entomology, Saint Paul, Minnesota, USA.
  • Munderloh UG; University of Minnesotagrid.17635.36, Department of Entomology, Saint Paul, Minnesota, USA.
  • Kurtti TJ; University of Minnesotagrid.17635.36, Department of Entomology, Saint Paul, Minnesota, USA.
Appl Environ Microbiol ; 88(7): e0021022, 2022 04 12.
Article en En | MEDLINE | ID: mdl-35323021
The genus Rickettsia encompasses a diverse group of obligate intracellular bacteria that are highly virulent disease agents of mankind as well as symbionts of arthropods. Native plasmids of Rickettsia amblyommatis (AaR/SC) have been used as models to construct shuttle vectors for genetic manipulation of several Rickettsia species. Here, we report on the isolation of the complete plasmid (pRM658B) from Rickettsia monacensis IrR/Munich mutant Rmona658B and the construction of shuttle vectors based on pRM. To identify regions essential for replication, we made vectors containing the dnaA and parA genes of pRM with various portions of the region surrounding these genes and a selection reporter cassette conferring resistance to spectinomycin and expression of green fluorescent protein. Rickettsia amblyommatis (AaR/SC), R. monacensis (IrR/Munich), Rickettsia bellii (RML 369-C), Rickettsia parkeri (Tate's Hell), and Rickettsia montanensis (M5/6) were successfully transformed with shuttle vectors containing pRM parA and dnaA. PCR assays targeting pRM regions not included in the vectors revealed that native pRM was retained in R. monacensis transformants. Determination of native pRM copy number using a plasmid-carried gene (RM_p5) in comparison to chromosomally carried gltA indicated reduced copy numbers in R. monacensis transformants. In transformed R. monacensis strains, native pRM and shuttle vectors with homologous parA and dnaA formed native plasmid-shuttle vector complexes. These studies provide insight on the maintenance of plasmids and shuttle vectors in rickettsiae. IMPORTANCERickettsia spp. are found in a diverse array of organisms, from ticks, mites, and fleas to leeches and insects. Many are not pathogenic, but others, such as Rickettsia rickettsii and Rickettsia prowazeckii, can cause severe illness or death. Plasmids are found in a large percentage of nonpathogenic rickettsiae, but not in species that cause severe disease. Studying these plasmids can reveal their role in the biology of these bacteria, as well as the molecular mechanism whereby they are maintained and replicate in rickettsiae. Here, we describe a new series of shuttle plasmids for the transformation of rickettsiae based on parA and dnaA sequences of plasmid pRM from Rickettsia monacensis. These shuttle vectors support transformation of diverse rickettsiae, including the native host of pRM, and are useful for investigating genetic determinants that govern rickettsial virulence or their ability to function as symbionts.
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Texto completo: 1 Banco de datos: MEDLINE Asunto principal: Rickettsia / Especificidad del Huésped Idioma: En Año: 2022 Tipo del documento: Article

Texto completo: 1 Banco de datos: MEDLINE Asunto principal: Rickettsia / Especificidad del Huésped Idioma: En Año: 2022 Tipo del documento: Article