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| Recombinant Protein Forum Recombinant Protein Forum. Discuss purification, expression, and isolation of recombinant and cloned proteins here. |
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| Hey all, i am currently working with a his-tagged protein of about 45KDa. The protein has absolutely no solubility problem after overexpression from a pUC in 293 cells. Column Binding Info: This protein does not bind to Ni-NTA. With denaturation by 8M urea it binds to a certain extent in Ni-NTA. ![]() For almost always the damn protein goes into the flow-through for any column you put it in. I have tried DEAE, Ni-NTA, CM-Sepharose, and other columns with various pH ranges (8, 8.8, and pH 6.4 for CM Sepharose as well since the proteins theoretical pI is 10.02). I confirmed this with western blot and anti-His antibodies in all the results. any ideas??? ![]() thnx |
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| I'd try tagging the opposite terminus to see if that end is more exposed. Edited to add: Or -- have you tried binding in batch rather than on the column? It can give the protein more opportunity to bind. Or another thing -- you could try a cobalt resin rather than the nickel. Last edited by kmunson779; 02-26-2008 at 02:27 PM. |
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