BioTechniques (Feb 2006)

Direct production and purification of T7 phage display cloned proteins selected and analyzed on microarrays

  • James E. Nowak,
  • Madhumita Chatterjee,
  • Saroj Mohapatra,
  • Sylvia C. Dryden,
  • Michael A. Tainsky

DOI
https://doi.org/10.2144/000112099
Journal volume & issue
Vol. 40, no. 2
pp. 220 – 227

Abstract

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Phage display technology has emerged into a powerful tool for identifying proteins with specific binding properties. This technology adds amino acid sequences to the carboxy terminus of a phage capsid protein, thus generating a fusion protein displayed on the surface of the phage. Here, we have developed a high-throughput strategy to synthesize purified protein that solves many of the problems associated with crude phage lysates. Phage DNA was used as a template for a nested PCR that added the T7 promoter, ribosome binding site, and a His6-tag. The PCR product was then used as a template for in vitro transcription/translation. The resulting His6-tagged recombinant protein was then purified by nickel affinity chromatography. The functionality of the purified protein was verified using protein microarray analysis.