A catalyst don’t appear in the overall stoichiometry of the reaction it catalyzes, but it must appear in at least one of the elementary reactions in the mechanism for the catalyzed reaction. 142-25-6, Name is N1,N1,N2-Trimethylethane-1,2-diamine, molecular formula is C5H14N2. In an article, author is Zheng, Qiangang,once mentioned of 142-25-6, Quality Control of N1,N1,N2-Trimethylethane-1,2-diamine.
Effect of an Imposed Contact on Secondary Structure in the Denatured State of Yeast Iso-1-cytochrome c
There is considerable evidence that long-range interactions stabilize residual protein structure under denaturing conditions. However, evaluation of the effect of a specific contact on structure in the denatured state has been difficult. Iso-1-cytochrome c variants with a Lys54 -> His mutation form a particularly stable His-heme loop in the denatured state, suggestive of loop-induced residual structure. We have used multidimensional nuclear magnetic resonance methods to assign H-1 and N-15 backbone amide and C-13 backbone and side chain chemical shifts in the denatured state of iso-1-cytochrome c carrying the Lys54 -> His mutation in 3 and 6 M guanidine hydrochloride and at both pH 6.4, where the His54-heme loop is formed, and pH 3.6, where the His54-heme loop is broken. Using the secondary structure propensity score, with the 6 M guanidine hydrochloride chemical shift data as a random coil reference state for data collected in 3 M guanidine hydrochloride, we found residual helical structure in the denatured state for the 60s helix and the C-terminal helix, but not in the N-terminal helix in the presence or absence of the His54-heme loop. Non-native helical structure is observed in two regions that form Omega-loops in the native state. There is more residual helical structure in the C-terminal helix at pH 6.4 when the loop is formed. Loop formation also appears to stabilize helical structure near His54, consistent with induction of helical structure observed when His heme bonds form in heme-peptide model systems. The results are discussed in the context of the folding mechanism of cytochrome c.
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