BioTechniques (Jul 1999)

Purification of Proteins Fused to Either the Amino or Carboxy Terminus of the Mycobacterium xenopi Gyrase A Intein

  • Maurice W. Southworth,
  • Kensey Amaya,
  • Thomas C. Evans,
  • Ming-Qun Xu,
  • Francine B. Perler

DOI
https://doi.org/10.2144/99271st04
Journal volume & issue
Vol. 27, no. 1
pp. 110 – 120

Abstract

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The Mycobacterium xenopi gyrase A mini-intein has been engineered to yield a controllable N-terminal or C-terminal, single- splice-junction autocleavage element. When combined with an affinity tag, these modified mini-inteins can be used to purify target proteins after a single combined chromatography/cleavage step. Cleavage at the intein N terminus was induced with thiol reagents, while cleavage at the intein C terminus was induced by a temperature shift to 16°–25°C. Different preferences for the residue immediately preceding the intein were observed during thiol-induced, N-terminal splice-junction cleavage of the M. xenopi gyrase A mini-intein vs. the Saccharomyces cerevisiae vacuolar ATPase, subunit A (VMA) intein present in the IMPACTTM purification system. Furthermore, the M. xenopi gyrase A mini-intein Cterminal autocleavage vector allows isolation of polypeptides with N-terminal cysteine residues that are active in the Intein Mediated Protein Ligation method of protein semisynthesis.