跳转至内容
Merck
  • Efficient site specific removal of a C-terminal FLAG fusion from a Fab' using copper(II) ion catalysed protein cleavage.

Efficient site specific removal of a C-terminal FLAG fusion from a Fab' using copper(II) ion catalysed protein cleavage.

Protein engineering (1999-04-09)
D P Humphreys, B J Smith, L M King, S M West, D G Reeks, P E Stephens
摘要

The peptide sequence (N)DKTH(C) was investigated as a site for efficient, specific cleavage of a fusion protein by cupric ions using a humanised gamma1 Fab' as a model protein. The native upper hinge (N)DKTH(C) sequence was mutated to create a site resistant to cleavage by cupric ions and a (N)DKTH(C) sequence introduced between the hinge and a C-terminal FLAG peptide. Incubation of Fab' with Cu2+ at 62 degrees C at alkaline pHs resulted in removal of the FLAG peptide with efficiencies of up to 86%. Cleavage conditions did not detrimentally affect the Fab' protein. Use of the (N)DKTH(C) sequence along with cupric ions may provide a cost-effective method for large scale proteolytic cleavage of fusion proteins.

材料
货号
品牌
产品描述

Sigma-Aldrich
大鼠单克隆抗-FLAG® 抗体, clone 6F7, purified from hybridoma cell culture
Sigma-Aldrich
抗-FLAG®-过氧化物酶抗体(兔), IgG fraction of antiserum