Bio-Rad Nuvia™ IMAC Resin User Manual

18 Nuvia IMAC Ni-Charged Resin

2. Equipment

• IMAC column (as prepared in Section 4)

3. Biological Sample

• Clarified lysate
The binding capacity of the Nuvia

™

IMAC resin is ~40 mg

histidine-tagged protein per ml resin. Larger amounts of
protein will require use of a larger column.

4. Additional Materials

• Medium-pressure chromatography system (such as

Bio-Rad’s BioLogic

™

or NGC

™

system)

• Equipment for determining total protein concentration

within the lysate

Method
1. Equilibrate the column with at least 5 column volumes of

binding buffer.

2. Add or dilute sample in binding buffer and load onto the

column using a desired flow rate.
The choice of binding buffer will vary based on the properties
of the sample to be purified. Sodium or potassium phosphate
is recommended as a general starting buffer; for example,
50 mM sodium phosphate, 300 mM NaCl, 5 mM imidazole,
pH 8.0. Binding of histidine-tagged protein on the Nuvia IMAC
resin is optimal in the pH range of 7–8.
The column may be run at flow rates up to 500 cm/hr. Higher
binding of histidine-tagged proteins will be achieved at lower
flow rates. Average binding capacity of the Nuvia IMAC resin is
approximately 40 mg histidine-tagged protein/ml resin.

3. Collect fractions.

These fractions represent unbound proteins.

4. Wash the resin with at least 5 column volumes of wash buffer

to remove unbound sample.
Wash out remaining unbound solutes. Repeat wash steps as
necessary for the A

280

to be at or near baseline.