Transcriptional induction kinetics from the promoters of the catabolic pathways of TOL plasmid pWW0 of Pseudomonas putida for metabolism of aromatics.

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J Bacteriol. 1994 May; 176(9): 2517-2524

Transcriptional induction kinetics from the promoters of the catabolic pathways of TOL plasmid pWW0 of Pseudomonas putida for metabolism of aromatics.

S Marqués, A Holtel, K N Timmis and J L Ramos

Departamento de Bioquímica, Biología Molecular y Celular de Plantas, CSIC-Estación Experimental del Zaidín, Granada, Spain.

ABSTRACT

We determined, under several growth conditions, the kineticsof mRNA synthesis from the four Pseudomonas putida pWW0 plasmidpromoters involved in degradation of xylenes and methylbenzylalcohols via toluates. Transcription by XylS of the meta-cleavagepathway operon promoter (Pm) for the metabolism of alkylbenzoateswas stimulated immediately after the addition of an effector,both in Luria-Bertani (LB) medium and in minimal medium. Activationof the sigma 54-dependent upper-pathway operon promoter (Pu)and the xylS gene promoter (Ps) by effector-activated XylR wasdependent on the growth medium used: on minimal medium, activationof transcription from Pu and Ps occurred immediately after theaddition of a XylR effector; in contrast, activation appearedonly after several hours when cells were growing on LB medium.When Pm was induced through the physiological overexpressionof XylS, mediated by XylR when this regulator was activatedby upper-pathway effectors, the kinetics of transcription fromPm was similar to that of Pu and Ps: maximum values were reachedafter delays of several hours in rich medium and after severalminutes in minimal medium. The delay in the induction of transcriptionof sigma 54-dependent promoters reflects catabolite inhibitionexerted by LB components, since the addition of yeast extracts,Casamino Acids, or several combinations of amino acids dramaticallyinhibited the synthesis of XylR-controlled sigma 54-dependentpromoters. Expression from xylR gene tandem promoters occurredindependently of the growth medium used.

J Bacteriol. 1994 May; 176(9): 2517-2524

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