Dolor-Amino acid dehydrogenase of Escherichia coli K12: Positive selection of mutants defective in enzyme activity and localization of the structural gene

A method for the positive selection of dadA mutants defective in D-amino acid dehydrogenase has been devised, It consists in isolating mutants resistant to fi-chloro-D-alanine and screening for mutant colony color on a special agar medium. All 70 Escheriehia coti Kt2 dadA mutants isolated either by this method or by other selection procedures map at a locus which is near to hemA and closely linked with dadR. Since some of the dadA mutants are thermosensitive in D-methionine utilization in vivo and have thermolabile D-amino acid dehydrogenase in vitro, it is proposed that the dadA gene codes for the enzyme structure. The broad substrate specificity, apparent membrane localization, inducibility by alanine, and repressibility by glucose strongly suggest that the u-amino acid dehydrogenase coded by the dadA gene is a species variant of the enzyme described under the same name in Salmonella typhimurium. It may be identical or homologous with the enzymes described under the names alaninase, D-alanine oxidase or D-alanine dehydrogenase in E. coli K12 or B.