I am currently working on purifying a phosphoprotein of approx. 25 kDa in length and a pI of 6. In order to purify the phosphoprotein using FPLC, we used a Gallium (III) HiTrap column by GE and an Äkta purifier. Our protein is in a 0.5M NaCl, 50mM Tris pH 6 buffer, while elution is done using a 0.5M Sodium phosphate pH 6 buffer.

Our issue is this: After the first elution, we are unable to re-use the column, either because the phosphate sticks to the immobilized Gallium, or because the elution causes all our Gallium to be washed out alongside it. Since Gallium in solution is colorless, it's hard to tell whether or not the Gallium is still present, and because it is a costly metal, stripping and recharging the column after each purification is also not an option for us.

I have looked far and wide to see what I should do to figure out whether the column can be reused, but so far I've had no luck.

More Michael Adams's questions See All
Similar questions and discussions