Part:BBa_K5036052

this figure illustrates the structure of TEV cleavage site (TCS(Q,G)) .

This section details the amino acid sequences of four tags attached to the N-terminus of proteins. Each tag contains six histidine residues, highlighted for easy identification. Additionally, the TEV protease cleavage site (ENLYFQ/G) is bolded for the TEV1 and TEV2 tags. It's important to note that the His-S and TEV2 tags have an extra four amino acids (SAND) at the C-terminus, compared to the other two tags.

This section examines the analysis of expression and solubility of proteins with four different His-tags. The boxes indicate the expected size of the protein produced. (A) The mouse protein USF1 was produced at high levels from E. coli when the His-L, His-S, and TEV1 tags were present, but no protein was produced when the TEV2 tag was used. The protein remained dissolved when the His-L and His-S tags were used, but the protein formed clumps when the TEV1 tag was used. (B) The mouse latexin protein was produced at high levels with all four tags, but the protein only remained dissolved when the His-L or His-S tag was present. The presence of the TEV cleavage site (in TEV1 and TEV2 tags) resulted in insoluble proteins.

This figure confirmed that this TCS(Q.L) sequence was the most appropriate for our conditions with a ΔG of -9.3 kcal mol-1 between the two domains of the TEV and the TCS(Q.L). While the TCS(Q.L) mutant form scored ΔG of -9.0 kcal mol-1 for Q6G. On the other hand, TCS(Q.G) scored ΔG of -10.2 kcal mol-1 while its mutant form E1D scored ΔG of -10.1 kcal mol-1. .