Hi,
Why don't you try adding GST/MBP tags first? This is a easy quick test.
We have a nice fusion (MBP) vector for e.coli expression if you want.
Grant
From: Sutapa Chakrabarti <[log in to unmask]<mailto:[log in to unmask] BERLIN.DE>>
Reply-To: Sutapa Chakrabarti <[log in to unmask]<mailto:[log in to unmask] BERLIN.DE>>
Date: Monday 3 April 2017 08:49
To: "[log in to unmask]<mailto:[log in to unmask] >" <[log in to unmask]<mailto:[log in to unmask] >>
Subject: [ccp4bb] Using a codon-optimised gene to improve protein solubility
Dear All,
We're trying to express and purify a 1000 residue long protein and have run into the problem that it is completely insoluble when expressed in E.coli and is not expressed at all in insect cells. The usual tricks for improving solubility in E.coli, such as addition of GST/MBP tags, optimising expression media and induction conditions and use of different cell strains, have not led to any improvement.
We are now looking into ordering a codon-optimised synthetic gene for this protein and are trying to decide whether it would be worthwhile to codon-optimise for expression in E.coli (given that the protein was expressed but not soluble) or if we should attempt baculovirus expression again with a gene that has been codon-optimised for insect cells.
My question is:
has anyone observed an improvement in the solubility of their target protein using a codon optimised gene?
I know of several instances where the use of a codon-optimised gene has led to expression where the native gene sequence did not but am unable to find any references for improvement in solubility. Since codon optimisation significantly alters the translation rate of a gene, I believe this should affect solubility as well; but I'd like to know what the community thinks/has observed before I order an exorbitantly priced gene!
Thank you in advance,
Sutapa
--
Sutapa Chakrabarti, Ph.D.
Institute of Chemistry and Biochemistry
Freie Universität Berlin
Takustr. 6
14195 Berlin
Germany
Phone: +49-(0)30-83875094