Adenine deaminase activity of the yicP gene product of Escherichia coli

During previous work on deriving inosine-producing mutants of Escherichia coli, we observed that an excess of adenine added to the culture medium was quickly converted to hypoxanthine. This phenomenon was still apparent after disruption of the known adenosine deaminase gene (add) on the E, coli chromosome, suggesting that, like Bacillus subtilis, E, coli has an adenine deaminase. As the yicP gene of E, coli shares about 35% identify with the B, subtilis adenine deaminase gene (ade), me cloned yicP from the E, coli genome and developed a strain that overexpressed its product. The enzyme was purified from a cell extract of E, coli harboring a plasmid containing the cloned yicP gene, and had significant adenine deaminase [EC 3.5.4.2] activity. It was deduced to be a homodimer, each subunit having a molecular mass of 60kDa, The enzyme required manganese ions as a cofactor, and adenine was its only substrate. Its optimum pH was 6.5-7.0 and its optimum temperature was 60 degreesC, The apparent K-m for adenine was 0.8 mM.