DnaK recognize extended peptide stretches with some specific preferences in sequence. Dnak bound to the fusion protein is an indication that you have accessible peptide unfolded regions, that may belong to your protein or to the fusion protein (it is probable the peptide junction between the fusion and your protein if you are using a fusion protein approach). Some specific protease recognition sites (i.e thrombin) are prone to strongly bound DnaK.

However, is your protein properly folded? You sould probably need to check this first. DnaK in addition to proteolysis during E. coli protein expression is a good indication of a miss-folded / unfolded protein.

I cannot answer question 2.

Thank you Eduardo. I tested another vector "pProExhta" with trc promoter and Tev protease site, the degradation level decreased but the chaperone DnaK expression was high . I tried to remove it with 5mM MgATP and 20% glycerol in washing buffer but still co-purified. but the question now what is th effective approach to remove the DnaK? by the ion exchange?

btw, the lysis buffer is 50mM tris-SO4, 300mM NaCl, 4% sucrose, 20% glycerol, 3mM MgCl2 20mM imidazol.

thank you in advance

To improve DnaK removal we included unfolded E. coli proteins in the washing buffer. In this way the exchange of Dnak between your protein and the E. coli proteins favor the chaperone removal. Take a glance to our paper: http://www.sciencedirect.com/science/article/pii/S1046592802000244. or send me your email address and a send you back a copy of this work.

Eduardo

Thank you again Eduardo. I know your paper, it is very interesting. but i remembered that the ATP washing with or without unfolded proteins causes removing of DnaK, is it right?

anyway, I will try this too. another question please, do you think addition of detergents like Titron x-100 can enhance the removal of dnaK?

thank you