Sequence analysis and bacterial production of the anti-c- myc antibody 9E10: the V H domain has an extended CDR-H3 and exhibits unusual solubility

Abstract

The cDNAs for the two variable domains of the antibody 9E10 were cloned from the hybridoma cell line. A chimeric 9E10 F ab fragment was produced in E. coli under control of the tightly controlled tetracycline promoter. The functional F ab fragment was isolated in a single step via a His 6-tag, which also served for its recognition by a nickel chelate-alkaline phosphatase conjugate. Thus, the recombinant F ab fragment permitted the immunochemical detection of the myc tag in a sandwich ELISA. The dissociation constant for the interaction with the myc tag peptide was determined as 80±5 nM by fluorescence titration. In an attempt to produce the smaller 9E10 F v fragment it was found that its V H domain alone can be readily isolated from E. coli as a soluble protein. This unusual behaviour may be explained by the 18 amino acid-long CDR-H3 and could be of value in the design of `single domain' antibodies.