A K-light chain from a Fab expression system was truncated by the insertion of a stop codon in the gene sequence to produce a variable light (V-L) single domain antibody (dAb). Here, we describe the expression of dAb in the periplasm of Escherichia coli through fermentation in a defined media. Immunoglobulin binding domains from peptostreptococcal protein L (PpL) have been shown to bind specifically to K-light chains. We have produced recombinant PpL, at high yield, and this was used to custom-produce PpL-Sepharose affinity columns. Here, we show that the affinity purification of V-L dAb by this method is simple and efficient with no apparent loss in protein at any stage. The truncated dAb protein product was confirmed by electrospray mass spectrometry and N-terminal sequencing. When analyzed by SDS-PAGE it was shown to be over 95% pure and produced at yields of 35-65 mg/L of culture medium. The dAb protein produced was shown by NMR and CD to be a folded P-sheet domain. This domain is bound by PpL with a Kd of similar to 50 nM as determined by stopped-flow fluorimetry. (c) 2006 Elsevier Inc. All rights reserved.