Bio-Rad Profinity IMAC Resins User Manual
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Section 13
Sample Preparation-Size Spin-Column
Purification of His-Tagged Proteins Using
Denaturing Conditions
Materials
Reagent
•
Binding buffer (urea-based)
–
50 mM sodium phosphate (NaH
2
PO
4
)
–
300 mM NaCl
–
5 mM imidazole
–
Up to 8 M urea
Adjust to pH 8.0.
•
Wash buffer
–
50 mM sodium phosphate (NaH
2
PO
4
)
–
300 mM NaCl
–
10 mM imidazole
–
Up to 8 M urea
Adjust to pH 8.0.
•
Elution buffer
–
50 mM sodium phosphate (NaH
2
PO
4
)
–
300 mM NaCl (pH 6.8 or higher)
–
250 mM imidazole
–
Up to 8 M urea
Adjust to pH 8.0.
•
Optimized wash buffer (optional, see Section 10)
A wash buffer containing slightly less imidazole than necessary to elute
the target protein may be used to increase the stringency of the wash
step. Refer to Section 10, Medium-Pressure Column Purification — Using
an Imidazole Gradient to Determine Optimal Purification of His-Tagged
Proteins.
Once the concentration of imidazole in the wash step is determined using
medium-pressure column chromatography, a stepwise elution step may
be carried out as indicated in this protocol.
Equipment
•
Sample preparation sized IMAC spin column (as prepared in Section 5)
(for example, Micro Bio-Spin column
™
, catalog #732-6204)
•
Plasticware, 2 ml capped, and 2 ml capless tubes
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