Can someone guide me on how to get rid of imidazole adsorbed to Ni-NTA agarose beads so they might be reused. Thanks in advance.
0
2 replies to this topic
#1
mdsr
-
- Members
-
- 2 posts
member
0
Neutral
Neutral
Posted 12 January 2005 - 03:04 AM
Can someone guide me on how to get rid of imidazole adsorbed to Ni-NTA agarose beads so they might be reused. Thanks in advance.
#2
strial
-
- Active Members
-
- 9 posts
member
0
Neutral
Neutral
Posted 12 January 2005 - 08:05 AM
Download this PDF document :
http://www1.qiagen.c...IAexpressionist
You will find lots of informations about NiNTA purification system. And a protocol for Ni-NTA regeneration...
You can wash your resin with 0.5N NaOH 30min for rapid regeneration. And use the same resin for the same protein purification...
For information :
Handling :
Ni-NTA matrices are stable under a wide variety of conditions and need not be refrigerated,
except to inhibit growth of microorganisms for long-term storage. After use they should be
washed for 30 minutes with 0.5M NaOH. Ni-NTA matrices should be stored in
30% ethanol to inhibit microbial growth. The matrix can be stored for up to one week in
any of the denaturing buffers.
Reuse of Ni-NTA Resin
The reuse of Ni-NTA resin depends on the nature of the sample and should only be performed
with identical recombinant proteins. Based on the experience of Hoffmann-La Roche Ltd.
(Basel, Switzerland), who have purified more than 100 different proteins on Ni-NTA resin,
we recommend a maximum of 5 runs per column.
If the Ni-NTA Agarose changes from light blue to brownish-gray, the following regeneration
procedure is recommended.
Procedure:
1. Wash the column with 2 volumes of Regeneration Buffer (6 M GuHCl, 0.2 M acetic
acid).
2. Wash the column with 5 volumes of H2O.
3. Wash the column with 3 volumes of 2% SDS.
4. Wash the column with 1 volume of 25% EtOH.
5. Wash the column with 1 volume of 50% EtOH.
6. Wash the column with 1 volume of 75% EtOH.
7. Wash the column with 5 volumes of 100% EtOH.
8. Wash the column with 1 volume of 75% EtOH.
9. Wash the column with 1 volume of 50% EtOH.
10. Wash the column with 1 volume of 25% EtOH.
11. Wash the column with 1 volume of H2O.
12. Wash the column with 5 volumes of 100 mM EDTA, pH 8.0.
13. Wash the column with H2O.
14. Recharge the column with 2 volumes of 100 mM NiSO4.
15. Wash the column with 2 volumes of H2O.
16. Wash the column with 2 volumes of Regeneration Buffer.
17. Equilibrate with 2 volumes of a suitable buffer (e.g., Buffer A or
.
Good luck.
David.
http://www1.qiagen.c...IAexpressionist
You will find lots of informations about NiNTA purification system. And a protocol for Ni-NTA regeneration...
You can wash your resin with 0.5N NaOH 30min for rapid regeneration. And use the same resin for the same protein purification...
For information :
Handling :
Ni-NTA matrices are stable under a wide variety of conditions and need not be refrigerated,
except to inhibit growth of microorganisms for long-term storage. After use they should be
washed for 30 minutes with 0.5M NaOH. Ni-NTA matrices should be stored in
30% ethanol to inhibit microbial growth. The matrix can be stored for up to one week in
any of the denaturing buffers.
Reuse of Ni-NTA Resin
The reuse of Ni-NTA resin depends on the nature of the sample and should only be performed
with identical recombinant proteins. Based on the experience of Hoffmann-La Roche Ltd.
(Basel, Switzerland), who have purified more than 100 different proteins on Ni-NTA resin,
we recommend a maximum of 5 runs per column.
If the Ni-NTA Agarose changes from light blue to brownish-gray, the following regeneration
procedure is recommended.
Procedure:
1. Wash the column with 2 volumes of Regeneration Buffer (6 M GuHCl, 0.2 M acetic
acid).
2. Wash the column with 5 volumes of H2O.
3. Wash the column with 3 volumes of 2% SDS.
4. Wash the column with 1 volume of 25% EtOH.
5. Wash the column with 1 volume of 50% EtOH.
6. Wash the column with 1 volume of 75% EtOH.
7. Wash the column with 5 volumes of 100% EtOH.
8. Wash the column with 1 volume of 75% EtOH.
9. Wash the column with 1 volume of 50% EtOH.
10. Wash the column with 1 volume of 25% EtOH.
11. Wash the column with 1 volume of H2O.
12. Wash the column with 5 volumes of 100 mM EDTA, pH 8.0.
13. Wash the column with H2O.
14. Recharge the column with 2 volumes of 100 mM NiSO4.
15. Wash the column with 2 volumes of H2O.
16. Wash the column with 2 volumes of Regeneration Buffer.
17. Equilibrate with 2 volumes of a suitable buffer (e.g., Buffer A or
.Good luck.
David.
#3
wei_i
-
- Members
-
- 1 posts
member
0
Neutral
Neutral
Posted 02 February 2005 - 11:15 AM
Hi, so in my protocol it says that regeneration should be performed if the Ni-NTA agarose turns from light blue to brownish-gray.
Am I right to assume that if the agarose is still light blue, that I just need to wash my resin with 0.5N NaOH 30min for rapid regeneration, and then use it again?
Thanks for your help!
Am I right to assume that if the agarose is still light blue, that I just need to wash my resin with 0.5N NaOH 30min for rapid regeneration, and then use it again?
Thanks for your help!
