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Search Purification (Commentary)

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EC Number Purification (Commentary) Reference
Display the word mapDisplay the reaction diagram Show all sequences 2.7.1.158- 660942, 662093
Display the word mapDisplay the reaction diagram Show all sequences 2.7.1.158a glutathione affinity column is used to capture intact GST-ZmIPK1. The purified GST-ZmIPK1 fusion is cleaved with thrombin and further purified by a sequential affinity and ion-exchange chromatography. ZmIPK1 protein is eluted at 0.1 M NaCl on a high resolution Mono Q column with an estimated purity of 95%. Identity of the purified protein is confirmed via trypsin digestion followed by matrix-assisted laser deposition/ionization (MALDI) time-of-flight mass spectrometry analysis and comparison of the MALDI fingerprint to the amino acid sequences deduced from ZmIPK1. 676634
Display the word mapDisplay the reaction diagram Show all sequences 2.7.1.158by batch-elution from Ni-NTA affinity resin, Analysis by SDS-PAGE gel and Western Blot using an anti-His antibody. Purity of protein is >98% estimated by SDS-PAGE. 686761
Display the word mapDisplay the reaction diagram Show all sequences 2.7.1.158expression in Escherichia coli 676634
Display the word mapDisplay the reaction diagram Show all sequences 2.7.1.158glutathione agarose bead chromatography 737654
Display the word mapDisplay the reaction diagram Show all sequences 2.7.1.158Ni-NTA bead chromatography 738589
Display the word mapDisplay the reaction diagram Show all sequences 2.7.1.158recombinant 661020, 662106, 662117, 662336
Display the word mapDisplay the reaction diagram Show all sequences 2.7.1.158recombinant enzyme 760534
Display the word mapDisplay the reaction diagram Show all sequences 2.7.1.158recombinant His-tagged enzyme from Escherichia coli strain BL21 (Lys) DE3 by nickel affinity chromatography 760326
Display the word mapDisplay the reaction diagram Show all sequences 2.7.1.158recombinant LSLt-tagged enzyme from Escherichia coli strain BL21 Star (DE3) by heparin affinity chromatography and gel filtration followed by tag cleavage with TEV protease and again heparin affinity chromatography and gel filtration. The recombinant GST-tagged enzyme from Sf21 insect cells is purified by glutathione affinity chromatography and tag cleavage with PreScission protease, followed by heparin affinity chromatography and gel filtration 762323
Results 1 - 10 of 11 > >>