IMPROVED N-TERMINAL PROCESSING OF RECOMBINANT PROTEINS SYNTHESIZED IN ESCHERICHIA-COLI

Preparations of rNMfA (recombinant histone A from Methanothermus fervidus) synthesized in E. coli by the heterologous expression of the hmfA gene were found to contain a mixture of rHMfA molecules, similar to 40% that retained the N-terminal formyl-methionyl residue (f-met-rNMfA), similar to 50% that lacked the formyl moiety but retained the methionyl residue (met-rHMfA), and only similar to 10% that had lost both components of the protein synthesis initiating amino acid residue and therefore had the same N-terminal sequence as native HMfA molecules synthesized in Mt, fervidus, Expression of the hmfA gene in E, coli cells grown in the presence of trimethoprim and thymidine, coupled with the concurrent over-expression of a methionine aminopeptidase-encoding map gene, has been shown to overcome this N-terminal heterogeneity problem and to result in rHMfA preparations in which > 85% of the molecules have the fully processed, native N-terminal sequence, This procedure should be generally useful for ensuring N-terminal processing of recombinant proteins synthesized in E. coli.