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上海玉博生物科技有限公司
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文献和实验.27. Column Buffers Make 500mls equivalent of base buffer: 10ml 1M Hepes pH 7.9 100ml 10% glycerol 5ml 10% NP40 (or 5.0ml 300mM Octyl glucoside) 200ml 0.5 EDTA ------- 115.2ml /5 = 23ml Base 1M KCl2.5M KCl dH20 for 0 KCL 46ml 0 0 154ml = 200
Preparation of Affinity Column
ml on nylon (0.22uM poresize),using Buchner funnel and vacuum.Do not allow beads to dry. 5.Wash bed with 3x2ml dH2O. 6.Scrape 0.5-1ml into 15ml microfuge tube. 7.Add 2.22ml CREBtide ligand solution to tube. Rock at 4℃ for 4hrs. 8.Transfer slurry to column
Preparation of Affinity Column制备亲和层析柱【UCSF】
and vacuum.Do not allow beads to dry. 5.Wash bed with 3x2ml dH2O. 6.Scrape 0.5-1ml into 15ml microfuge tube. 7.Add 2.22ml CREBtide ligand solution to tube. Rock at 4℃ for 4hrs. 8.Transfer slurry to column. 9.Wash 2x500μl dH2O. 10.Collect eluate
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