An automated small-scale protein expression and purification screening provides beneficial information for protein production
- 1 March 2004
- journal article
- Published by Springer Nature in Journal of Structural and Functional Genomics
- Vol. 5 (1/2) , 23-27
- https://doi.org/10.1023/b:jsfg.0000029195.73810.86
Abstract
One of the first key steps in structural genomics is high-throughput expression and rapid screening to select highly soluble proteins, the preferred candidates for crystal production. Here we describe the methodology used at the Berkeley Structural Genomics Center (BSGC) for automated parallel expression and small-scale purification of fusion proteins using a 96-well format. Our robotic method includes cell lysis, soluble fraction separation and purification with affinity resins. For detection of His-tagged proteins in the soluble fractions and after affinity resin elution, a dot-blot procedure with an anti-His-antibody is used. The expression level and molecular mass of recombinant proteins are checked by SDS-PAGE. With this approach, we are able to obtain beneficial information to be used for large-scale protein expression and purification.Keywords
This publication has 5 references indexed in Scilit:
- A global representation of the protein fold spaceProceedings of the National Academy of Sciences, 2003
- Protein expression systems for structural genomics and proteomicsCurrent Opinion in Chemical Biology, 2003
- High Throughput Methods for Gene Cloning and ExpressionProtein Expression and Purification, 2002
- Screening for Soluble Expression of Recombinant Proteins in a 96-Well FormatAnalytical Biochemistry, 2001
- IMMUNOCYTOCHEMICAL DEMONSTRATION OF HUMAN PROINSULIN CHIMERIC POLYPEPTIDE WITHIN CYTOPLASMIC INCLUSION-BODIES OF ESCHERICHIA-COLI1983