Päivi Pihkala scite author profile

Improved ways to cleave peptide chains at engineered sites easily and specifically would form useful tools for biochemical research. Uses of such methods include the activation or inactivation of enzymes or the removal of tags for enhancement of recombinant protein expression or tags used for purification of recombinant proteins. In this work we show by gel electrophoresis and mass spectroscopy that salts of Co(II) and Cu(II) can be used to cleave fusion proteins specifically at sites where sequences of His residues have been introduced by protein engineering. The His residues could be either consecutive or spaced with other amino acids in between. The cleavage reaction required the presence of low concentrations of ascorbate and in the case of Cu(II) also hydrogen peroxide. The amount of metal ions required for cleavage was very low; in the case of Cu(II) only one to two molar equivalents of Cu(II) to protein was required. In the case of Co(II), 10 molar equivalents gave optimal cleavage. The reaction occurred within minutes, at a wide pH range, and efficiently at temperatures ranging from 0°C to 70°C. The work described here can also have implications for understanding protein stability in vitro and in vivo.

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An antigen-mediated selection system for mammalian cells that produce glycosylated single-chain Fv

Pihkala

Kawahara

Ueda

et al. 2004

Biochemical and Biophysical Research Communications

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Päivi Pihkala

Immunologic Activity in the Small Intestinal Mucosa of Pediatric Patients With Type 1 Diabetes

Cleavage of recombinant proteins at poly‐His sequences by Co(II) and Cu(II)

An antigen-mediated selection system for mammalian cells that produce glycosylated single-chain Fv

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