Cloning and characterization of a gene whose product is a trans-activator of anthrax toxin synthesis.

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J Bacteriol. 1993 September; 175(17): 5329-5338

research-article

Cloning and characterization of a gene whose product is a trans-activator of anthrax toxin synthesis.

I Uchida, J M Hornung, C B Thorne, K R Klimpel and S H Leppla

Laboratory of Microbial Ecology, National Institute of Dental Research, Bethesda, Maryland 20892.

ABSTRACT

The 184-kb Bacillus anthracis plasmid pXO1, which is requiredfor virulence, contains three genes encoding the protein componentsof anthrax toxin, cya (edema factor gene), lef (lethal factorgene), and pag (protective antigen gene). Expression of thethree proteins is induced by bicarbonate or serum. Using a pag-lacZtranscriptional construct to measure pag promoter activity,we cloned in Bacillus subtilis a gene (atxA) whose product actsin trans to stimulate anthrax toxin expression. Deletion analysislocated atxA on a 2.0-kb fragment between cya and pag. DNA sequencingidentified one open reading frame encoding 476 amino acids witha predicted M(r) of 55,673, in good agreement with the valueof 53 kDa obtained by in vitro transcription-translation analysis.The cloned atxA gene complemented previously characterized Tn917insertion mutants UM23 tp29 and UM23 tp32 (J. M. Hornung andC. B. Thorne, Abstr. 91st Gen. Meet. Am. Soc. Microbiol. 1991,abstr. D-121, p. 98), which are deficient in synthesis of allthree toxin proteins. These results demonstrate that the atxAproduct activates not only transcription of pag but also thatof cya and lef. beta-Galactosidase synthesis from the pag-lacZtranscriptional fusion construct introduced into an insertionmutant (UM23 tp62) which does not require bicarbonate for toxinsynthesis indicated that additional regulatory genes other thanatxA play a role in the induction of anthrax toxin gene expressionby bicarbonate.

J Bacteriol. 1993 September; 175(17): 5329-5338

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