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Preparation of Affinity Column制备亲和层析柱【UCSF】

2024-11-25 蛋白质技术 加入收藏
1.Add 222.2μl 1M MOPS,pH 7.5 to 2ml of 10mg of CREBtide (0.1M MOPS pH 7.5 final

1.Add 222.2μl 1M MOPS,pH 7.5 to 2ml of 10mg of CREBtide (0.1M MOPS pH 7.5 final concentration).

2.Read OD205,OD280 (using 0.1M MOPS buffer as blank)

3.Affigel-10 is stored frozen at < -70℃.Thaw at 4℃ for ~20min.

4.Filter 1-2ml 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.

9.Wash 2x500μl dH2O.

10.Collect eluate and save at -20℃.Read OD.

11.Wash column:

2x5ml cold PBS

1x5ml PBS/0.02% NaN3 (1μl NaN3 in5ml PBS)

12.Store at 4℃ upright in beaker in PBS/NaN3 parafilm.


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