My recombinant protein of 38 kDa has been expressed and it was in soluble fraction (with 10% glycerol, 0.5mM IPTG and 23 degree celcius). but the protein was not binding to the Ni-NTA column. I suspect the his tag might have occluded within the protein tertiary structure. How can i purify my protein without adding any denaturants such as urea or Gdn-HCl.

Thanks in advance.

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