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Problems in recombinant protein expression - Problems in recombinant protein expression (Apr/20/2011 )

Hi all,

I cloned a bacterial surface protein without N-terminal signal peptide in pET15b vector and expressed in BL21 host. After induction at 37 degrees celsius, I just boiled the cell pellet of a positive clone in sample buffer for 8 min, centrifuged for 10 min and loaded onto 12% SDS gel. I could not able to see any expressed protein. Then, I purified the expressed protein after induction at 37 degrees celsius using metal affinity resin specific for His-tag. The purified protein was mixed with sample buffer, boiled for 8 min, centrifuged for 5 min and loaded onto 12% SDS gel. Then also, I could not able to see any expressed protein. Later, instead of IPTG, I used auto-induction kit also. But, there is no change in outcome. What could be the reason and how to get over expression?

-vels-

Try express using a milder condition: 25 C or below... lesser IPTG concentration, and longer time of expression. See if it helps....

-adrian kohsf-

Thank you and I will try that. Please suggest me any other changes to be made for conditions of expression.

-vels-

vels on Thu Apr 21 17:31:55 2011 said:


Thank you and I will try that. Please suggest me any other changes to be made for conditions of expression.


I tried overnight expression at 23 degress Celsius. Still, it did not express the protein. Please suggest me in this regard.

-vels-

what about cell growth? ...do you measured OD every hour after induction?

Do your cells stop growing? ...is it possible that the cells die after induction?

At what OD you induce your recombinant culture?

Regards,
p

-pDNA-

wait a minute... do you do western blot to confirm the expression?

-adrian kohsf-