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Instability of pUC19 in Escherichia coli transcription termination factor mutant, rho026.
Sozhamannan, S; Morris, J G; Stitt, B L.
Afiliación
  • Sozhamannan S; Department of Medicine, University of Maryland School of Medicine, Baltimore, Maryland, 21201, USA.ssozhama@umppal.ab.umd.edu
Plasmid ; 41(1): 63-9, 1999 Jan.
Article en En | MEDLINE | ID: mdl-9887307
ABSTRACT
The higher copy number of pUC19, compared to its parent plasmid pBR322, is known to be due to deletion of rop, also known as rom, and to an ori mutation that impedes RNAIRNAII interaction. pUC19, unlike pBR322, fails to transform E. coli rho mutant rho026 cells. Here we identify two features of pUC19 that contribute to this transformation defect. (1) The pUCori mutation is involved because replacing the pUCori with that of pBR322 restored transformation. (2) Transcription from the lac promoter in pUC19 is important, since deletion or inversion of the promoter or insertion of a transcription terminator (lambdat0) downstream of it restored transformation. Host RNase E activity is responsible for the transformation defect because introduction of an rne-1 allele into rho026 cells suppressed this defect, indicating that RNAI instability due to RNase E is aggravated in the rho026 strain. We suggest that in rho026 cells pUC19 RNAIRNAII interaction is more impeded than in rho+ cells and Rop/Rom may confer stability by protecting RNAI against RNase E activity because expression of a rom gene inserted into pUC19 restored transformation.
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Colección: 01-internacional Base de datos: MEDLINE Asunto principal: Plásmidos / Factor Rho / Escherichia coli / Mutación Tipo de estudio: Prognostic_studies Idioma: En Revista: Plasmid Año: 1999 Tipo del documento: Article
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Colección: 01-internacional Base de datos: MEDLINE Asunto principal: Plásmidos / Factor Rho / Escherichia coli / Mutación Tipo de estudio: Prognostic_studies Idioma: En Revista: Plasmid Año: 1999 Tipo del documento: Article