2007
DOI: 10.1016/j.pep.2007.04.013
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A combined approach to improving large-scale production of tobacco etch virus protease

Abstract: Tobacco etch virus NIa proteinase (TEV protease) is an important tool for the removal of fusion tags from recombinant proteins. Production of TEV protease in E. coli has been hampered by insolubility and addressed by many different strategies. However, the best previous results and newer approaches for protein expression have not been combined to test whether further improvements are possible.Here we use a quantitative, high throughput assay for TEV protease activity in cell lysates to evaluate the efficacy of… Show more

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Cited by 247 publications
(261 citation statements)
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“…The eluted fractions that were found to contain homogeneous DFTR via SDS-PAGE were pooled and concentrated using an Amicon ultracentrifugal filter, 3-kDa molecular mass cutoff (EMD Millipore, Bedford, MA). The NH 2 -terminal His 6 tag of the purified protein was cleaved by incubation at 4°C with recombinant His 6 -TEV (recombinant TEV-protease carrying a His 6 tag) (78), at an Mj-DFTR to protease ratio of 20:1 under overnight dialysis against a solution containing Tris-Cl buffer, pH 8.0, NaCl, and DTT at final concentrations of 50, 200, and 5 mM, respectively. DTT was then removed by three more rounds of dialysis against the same solution but without DTT and containing a higher final concentration of NaCl (400 mM).…”
Section: Methodsmentioning
confidence: 99%
“…The eluted fractions that were found to contain homogeneous DFTR via SDS-PAGE were pooled and concentrated using an Amicon ultracentrifugal filter, 3-kDa molecular mass cutoff (EMD Millipore, Bedford, MA). The NH 2 -terminal His 6 tag of the purified protein was cleaved by incubation at 4°C with recombinant His 6 -TEV (recombinant TEV-protease carrying a His 6 tag) (78), at an Mj-DFTR to protease ratio of 20:1 under overnight dialysis against a solution containing Tris-Cl buffer, pH 8.0, NaCl, and DTT at final concentrations of 50, 200, and 5 mM, respectively. DTT was then removed by three more rounds of dialysis against the same solution but without DTT and containing a higher final concentration of NaCl (400 mM).…”
Section: Methodsmentioning
confidence: 99%
“…pNIC28-BSA4 was a generous gift from Professor Opher Gileadi, University of Oxford, and pMHT238⌬ was from Professor Brian G. Fox, University of Wisconsin. The His-tagged and C-terminally truncated TEV protease encoded in pMHT238⌬ was expressed and purified essentially as described before (31). Primers were from Thermo Fischer Scientific; Phusion High-Fidelity PCR master mix was from Finnzymes, and Exonuclease I was from Fermentas.…”
Section: General-b Anthracis Sterne 7700 (Pxo1mentioning
confidence: 99%
“…The column was washed with the lysis buffer, and the protein was subsequently eluted using a gradient of imidazole in the buffer. Appropriate protein fractions were pooled and dialyzed at 4°C in the presence of rTEV protease (25) to remove the N-terminal His 6 tag. The His 6 -tagged rTEV protease, encoded in a pProEX HTa expression vector, was produced earlier from E. coli Rosetta TM (DE3)pLysS cells (Novagen), as described previously (25).…”
Section: Pcr Amplification and Cloning-mentioning
confidence: 99%
“…Appropriate protein fractions were pooled and dialyzed at 4°C in the presence of rTEV protease (25) to remove the N-terminal His 6 tag. The His 6 -tagged rTEV protease, encoded in a pProEX HTa expression vector, was produced earlier from E. coli Rosetta TM (DE3)pLysS cells (Novagen), as described previously (25). After overnight incubation of the purified FbiB proteins with rTEV protease, a subtractive immobilized metal affinity chromatography step was performed to remove the cleaved protein from uncut protein and rTEV protease.…”
Section: Pcr Amplification and Cloning-mentioning
confidence: 99%