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Expression of an epitope-tagged virulence protein in Rickettsia parkeri using transposon insertion.


ABSTRACT: Despite recent advances in our ability to genetically manipulate Rickettsia, little has been done to employ genetic tools to study the expression and localization of Rickettsia virulence proteins. Using a mariner-based Himar1 transposition system, we expressed an epitope-tagged variant of the actin polymerizing protein RickA under the control of its native promoter in Rickettsia parkeri, allowing the detection of RickA using commercially-available antibodies. Native RickA and epitope-tagged RickA exhibited similar levels of expression and were specifically localized to bacteria. To further facilitate protein expression in Rickettsia, we also developed a plasmid for Rickettsia insertion and expression (pRIE), containing a variant Himar1 transposon with enhanced flexibility for gene insertion, and used it to generate R. parkeri strains expressing diverse fluorescent proteins. Expression of epitope-tagged proteins in Rickettsia will expand our ability to assess the regulation and function of important virulence factors.

SUBMITTER: Welch MD 

PROVIDER: S-EPMC3356282 | biostudies-literature | 2012

REPOSITORIES: biostudies-literature

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Expression of an epitope-tagged virulence protein in Rickettsia parkeri using transposon insertion.

Welch Matthew D MD   Reed Shawna C O SC   Lamason Rebecca L RL   Serio Alisa W AW  

PloS one 20120518 5


Despite recent advances in our ability to genetically manipulate Rickettsia, little has been done to employ genetic tools to study the expression and localization of Rickettsia virulence proteins. Using a mariner-based Himar1 transposition system, we expressed an epitope-tagged variant of the actin polymerizing protein RickA under the control of its native promoter in Rickettsia parkeri, allowing the detection of RickA using commercially-available antibodies. Native RickA and epitope-tagged Rick  ...[more]

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