Stability of Mutant Type II Dihydrofolate Reductase Proteins in SuppressorStrains

摘要

In the course of study of a (Glu-58 to Gln-58) mutant type II dihydrofolatereductase (DHFR), it was found that the altered DHFR was poorly produced in vivo. Investigations with several common laboratory Escherichia coli strains including htpR and lon strains bearing plasmids expressing the Gln-58 DHFR indicated a correlation of rapid degradation with the presence of a sup phenotype. The sup strain MCl061(p3) was transformed with a series of plasmids containing the Gln-58 DHFR gene with and without an additional supF gene, and expression levels were compared. The supF constructs exhibited little accumulation of the Gln-58 DHFR, while reasonable levels were found in the sup cases. Experiments with extracts of plasmid-free sup and sup strains showed rapid degradation by certain strains compared to MC1061(p3) and this degradation was not dependent upon ATP. In another route to increasing the stability of labile DHFR derivatives, mutagenesis of a strain bearing a N-terminally shortened Gln-58 DHFR was performed. Selection and analysis of a trimethoprim-resistant stable mutant showed that this DHFR gene contained a triple repeat of leu-pro-ser in the enzymatically non-essential N-terminal portion of the protein.