Literature DB >> 12089047

Site-specific recombination-based genetic system for reporting transient or low-level gene expression.

N Carol Casavant1, Gwyn A Beattie, Gregory J Phillips, Larry J Halverson.   

Abstract

We report here the construction, characterization, and application of a plasmid-based genetic system that reports the expression of a target promoter by effecting an irreversible, heritable change in a bacterial cell. This system confers strong repression of the reporter gene gfp in the absence of target promoter expression and utilizes the site-specific recombination machinery of bacteriophage P22 to trigger high-level reporter gene expression in the original cell and its progeny after target gene induction. We demonstrate the effectiveness of this genetic system by tailoring it to indicate the availability of arabinose to the biological control agent Enterobacter cloacae JL1157 in culture and in the barley rhizosphere. The presence of bioavailable arabinose triggered the production of P22 excisionase and integrase from the reporter plasmid pAraLHB in JL1157, and this led to excision of the cI repressor gene, which is flanked by att sites, and the subsequent irreversible expression of gfp in the original cell and in its progeny. In culture, nearly 100% of an E. cloacae JL1157(pAraLHB) population expressed gfp after exposure to 6.5 to 65 microM arabinose for 3 h. We used this biosensor to demonstrate that arabinose was released from the seeds of several legumes and grass species during germination and from roots of barley seedlings grown hydroponically or in soil. When introduced into microcosms containing barley, the biosensor permitted the localization of arabinose along the roots. Arabinose was present near the root-seed junction and on the seminal roots but was not detected at the root tips. This recombination-based reporter system should be useful for monitoring bacterial exposure to transient or low levels of specific molecules directly in the environment.

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Year:  2002        PMID: 12089047      PMCID: PMC126813          DOI: 10.1128/AEM.68.7.3588-3596.2002

Source DB:  PubMed          Journal:  Appl Environ Microbiol        ISSN: 0099-2240            Impact factor:   4.792


  29 in total

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4.  Green fluorescent protein as a marker for gene expression.

Authors:  M Chalfie; Y Tu; G Euskirchen; W W Ward; D C Prasher
Journal:  Science       Date:  1994-02-11       Impact factor: 47.728

5.  Use of genetic recombination as a reporter of gene expression.

Authors:  A Camilli; D T Beattie; J J Mekalanos
Journal:  Proc Natl Acad Sci U S A       Date:  1994-03-29       Impact factor: 11.205

Review 6.  In vivo expression technology for selection of bacterial genes specifically induced in host tissues.

Authors:  J M Slauch; M J Mahan; J J Mekalanos
Journal:  Methods Enzymol       Date:  1994       Impact factor: 1.600

7.  Lambda replacement vectors carrying polylinker sequences.

Authors:  A M Frischauf; H Lehrach; A Poustka; N Murray
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8.  Use of recombinase gene fusions to identify Vibrio cholerae genes induced during infection.

Authors:  A Camilli; J J Mekalanos
Journal:  Mol Microbiol       Date:  1995-11       Impact factor: 3.501

9.  STRUCTURE AND BIOGENESIS OF THE CELL WALLS OF GRASSES.

Authors:  Nicholas C. Carpita
Journal:  Annu Rev Plant Physiol Plant Mol Biol       Date:  1996-06

10.  Rapid, sensitive bioluminescent reporter technology for naphthalene exposure and biodegradation.

Authors:  J M King; P M Digrazia; B Applegate; R Burlage; J Sanseverino; P Dunbar; F Larimer; G S Sayler
Journal:  Science       Date:  1990-08-17       Impact factor: 47.728

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  1 in total

1.  Arabinose and protocatechuate catabolism genes are important for growth of Rhizobium leguminosarum biovar viciae in the pea rhizosphere.

Authors:  Paula Garcia-Fraile; Jonathan C Seaman; Ramakrishnan Karunakaran; Anne Edwards; Philip S Poole; J Allan Downie
Journal:  Plant Soil       Date:  2015-01-30       Impact factor: 4.192

  1 in total

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