Cloning and genetic organization of the pca gene cluster from Acinetobacter calcoaceticus.

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J Bacteriol. 1987 July; 169(7): 3168-3174

Cloning and genetic organization of the pca gene cluster from Acinetobacter calcoaceticus.

R C Doten, K L Ngai, D J Mitchell and L N Ornston

ABSTRACT

The beta-ketoadipate pathway of Acinetobacter calcoaceticuscomprises two parallel metabolic branches. One branch, mediatedby six enzymes encoded by the cat genes, converts catechol tosuccinate and acetyl coenzyme A (acetyl-CoA); the other branch,catalyzed by products of the pca genes, converts protocatechuateto succinate and acetyl-CoA by six metabolic reactions analogousor identical to those of the catechol sequence. We used theexpression plasmid pUC18 to construct expression libraries ofDNA from an A. calcoaceticus mutant strain from which the catgenes had been deleted. Immunological screening with antiserumto the pcaE gene product, beta-ketoadipate:succinyl-CoA transferaseI, resulted in the isolation of a cloned 11-kilobase-pair (kbp)fragment which inducibly expressed all six pca genes under controlof the lac promoter on pUC18. The induced Escherichia coli cellsformed the six pca gene products at levels 10- to 30-fold higherthan found in fully induced A. calcoaceticus cultures, althoughprotocatechuate 3,4-dioxygenase (the iron-containing productof the pcaA gene) from the recombinant strain possessed a relativelylow turnover number. An E. coli culture expressing the clonedpca genes quantitatively converted protocatechuate to beta-ketoadipate;failure of the organism to metabolize the latter compound canbe most readily ascribed to relatively low pool levels of succinyl-CoA,a required substrate for beta-ketoadipate:succinyl-CoA transferase,in E. coli. The gene order and direction of transcription weredetermined to be pcACBDFE by identification of enzymes expressedin subclones, by using natural transformation to identify subclonescarrying DNA corresponding to dysfunctional alleles in mutantA. calcoaceticus strains, and by restriction mapping of boththe 11-kbp fragment and derivatives of the 11-kbp fragment containingTn5 in the pcaA, pcaB, pcaD, and pcaE genes. The fragment containingthe pca gene hybridized strongly and specifically to a previouslycloned fragment containing A. calcoaceticus cat genes.

J Bacteriol. 1987 July; 169(7): 3168-3174

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