Hello Everyone,
http://www.gelifesci...em_handbook.pdf
We are trying to understand a plasmid we were sent, and my knowledge of cloning is out of date. The plasmid consists of the phosphatase of interest (of known sequence) cloned into a vector designed to make glutathione S-transferase (GST) fusion proteins, namely pGEX-4T-1, and there is a site for thrombin cleavage. After the Arg-Gly thrombin site are six nucleotides that would express a serene and a proline residue. The next nucleotides begin a restriction site for EcoRI, GAATTC. The paper we are following indicates that EcoRI and XhoI were the enzymes used to clone the gene of interest.
"Collectively, the pGEX vectors provide all three translational reading frames beginning with the EcoRI restriction site (Fig 1.1). pGEX-1λT, pGEX-6P-1, pGEX-4T-1, and pGEX-5X-1 can directly accept and express cDNA inserts isolated from λgt11 libraries." Based upon this passage from the handbook above, I would offer a guess that the phosphatase gene was cloned out of λgt11, but I don't know this with certainty. What I don't know is what lies between the EcoRI site and the beginning of the phosphatase gene. Is there any way to make an intelligent guess about this? is there any resource that describes cloning from lambda-gt11 into pGEX-4T-1?
We have the mass of the fusion protein, and we would like to compare the predicted versus the theoretical mass to verify the existence of the thrombin cleavage site. Thanks for any help or suggestions.
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Topic: cloning into a pGEX vector (Read 3796 times)