CHARACTERIZATION OF THE PYRB GENE OF SERRATIA MARCESCENS AND HYBRID GENE FORMATION WITH THE PYRB GENE OF ESCHERICHIA COLI, LEADING TO THE PRODUCTION OF CHIMERIC ATCASES

The ATCase from Escherichia coli has been the subject of extensive physical, biochemical and genetic studies. The exact natures of the intrasubunit and intersubunit interactions responsible for enzymatic function are still not completely defined. While many residues have been implicated from chemical modification studies as participating in substrate binding, heterotropic interactions or homotropic interactions, x-ray crystallographic studies have suggested that some of these amino acids may not be directly involved. Site-directed mutagenesis of the genes that encode the subunits of ATCase can potentially define more directly residues that are involved in structural and functional roles of the enzyme, although it is hardly feasible to replace all the residues of ATCase with all other possible amino acid residues.;While most chimeric constructs exhibit the effector responses characteristic of the regulatory subunits present, the C;The nucleotide and deduced amino acid sequences of the catalytic polypeptide of ATCase from the enteric bacterium Serratia marcescens HY will be investigated. The polypeptide contains 305 amino acids, as compared to 310 in the corresponding polypeptide from E. coli, and 40 amino acid differences from the E. coli polypeptide. Hybrid pyrB genes have been constructed from portions of the pyrB genes of E. coli and S. marcescens, producing hybrid catalytic polypeptides which have been utilized to produce chimeric holoenzymes. These constructs implicate the equatorial domain of the catalytic polypeptide of S. marcescens as responsible for some of the altered characteristics seen in these hybrid and chimeric ATCases.