Bio-Rad Foresight™ Chromatography Columns, Prepacked User Manual

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Materials and Methods
1. Preparation of stock solutions:

Loading buffer: 0.02 M Na Acetate, pH 4.5 was

adjusted to a conductivity of 5.0 mS/cm with 0.02 M

Na Acetate, 5 M NaCl, pH 4.5

Stock protein solution: human IgG from Cohn fraction

II+III (Sigma catalog #G4386-25G) was solubilized in

the loading buffer to a final concentration of

3.0 mg/ml. The stock solution was thereafter sterile

filtered.

2. Preparation of test solutions:

Loading buffer was added proportionally into test

tubes containing the stock protein solution to prepare

10 test solutions with a hIgG concentration ranging

from 0.25 to 3.0 mg/ml. The tubes were vortexed prior

to use. The total hIgG concentration was determined

as follows: 200 µl of each of the test solutions was

loaded to a 96-well plate to determine its absorbance

at 280 nm. Next, the protein concentration was

calculated using the Lambert-Beer law with a fixed

mass extinction coefficient of 1.4 ml/mg/cm.

3. Generation of adsorption isotherm data using

Foresight chromatography media filter plate:

A 96-well plate containing Nuvia

™

cPrime

™

, a mixed-

mode resin was used. The sequence of steps was as

follows:

a) Apply 300 µl of loading buffer to each designated

well. Apply vacuum to drain the loading buffer.

Repeat twice.

b) Apply 300 µl of test solution to each designated

well. Secure the plate to microplate mixer and

agitate at 1100 rpm for one hr. Longer incubation

time may be required to reach equilibrium.

A conservative incubation time of 4–6 hr is

recommended for a broad range of buffer

conditions and target molecules.