Hi everyone,
Recently I am helping someone to obtain 2 proteins (both are glycohydrolases) from a Hydra species by using Expi293 suspension cells via secretion. He had tried once and they'd become inclusion bodies through E. coli; therefore, we are working on this.
Instead of generating proteins, cells were dying gradually after transfection. At the time of harvest, we got both completely opaque cultures. Since the genetic distances from cnidarians, either to procaryotes or to mammals, are absurdly far, the success rates of getting properly-folded proteins are somewhat of a mystery. For instance, GFP originally from jellyfish is a widespread tool for various purposes.
This time I have to examine the cell viability, but in 2 weeks, since I need to unfreeze the cells with a small passage number afresh and prepare sufficient materials to start with. Also, he'll take some to check the expressions in every part of the culture. If it's not working, what are alternatives? Like using adherent type instead, or another model systems?
Our vector is pEXPR-IBA42.
Thank you for having great patience with the question.