Construction of a dual-tag system for gene expression, protein affinity purification and fusion protein processing

## Abstract The choline‐binding domain (ChoBD) of the carboxy‐terminal region of the __Streptococcus pneumoniae__ amidase LYTA (C‐LYTA) presents a strong affinity for tertiary amines. We report a method for single‐step purification of proteins expressed in the methylotrophic yeast __Pichia pastoris

encoding N-terminal-deleted regions of human progesterone receptor, in agreement with the observations that the cDNAs encoding progesterone receptor were detected by RT-PCR in the human ovary cDNA library, but not in the HeLa cell cDNA library. The ligandindependent colonies turned out to harbor cDN

## Abstract A multiple vector system for the intracellular high‐level production of affinity tagged recombinant proteins in __Bacillus megaterium__ was developed. The N‐ and C‐terminal fusion of a protein of interest to a Strep II and a His~6~‐tag is possible. Corresponding genes are expressed unde