I was measuring lyophylized bovine thrombin (purchased form Sigma Aldrich, http://www.sigmaaldrich.com/catalog/product/sigma/t4648 : composition | Protein, 40-60%, Lyophilized powder containing sodium chloride and Tris-HCl, pH 7.0.) Raman spectrum and found out a strange (as I see it) thing. According to PDB X-ray structure (for example, 1uvs and 1ppb(human)) the 4 disulfide bonds in thrombin have ggg (cys168-cys182 and cys122-cys1) and tgg (cys42-cys58 and cys191-cys220) conformations. But in the measured Raman spectrum I could define peaks on all three frequences, commonly assosiated with different conformations of SS-bonds (~510, 525 & 540(!) cm-1), what indicates the presence of tgt conformation in lyophylized state. Is it possible, that there is such differ between X-ray structure and lyophylized powder?
P.S. I checked, this is not the contribution of Tris-HCl buffer.