Thermodynamic investigations of proteins: II. Calorimetric study of lysozyme denaturation by guanidine hydrochloride

The stabilization of the folded conformation of lysozyme, arising from the binding of the inhibitor (NAG) against induced denaturation, is demonstrated from the 'H-nmr spectra of the enzyme. The nmr spectra reveal that the binding of the denaturant (GuHC1) to the enzyme is associbted with changes in

## Abstract The technique of intensity correlation light‐scattering spectroscopy has been used to accurately determine the extent of physical swelling of lysozyme, ribonuclease, and chymotrypsinogen produced by thermal denaturation. The change in hydrodynamic radius is deduced from direct measureme

## Abstract A three‐dimensional lattice model of protein designed to assimilate lysozyme is introduced. An attractive interaction is assumed to work between preassigned specific pairs of units, when they occupy the nearest‐nighbor lattice points. The behavior of this lattice lysozyme is studied by

## Abstract Chymotrypsinogen, nitrated chymotrypsinogen (two of the four tyrosyls nitrated), acetylated chymotrypsinogen (all amino groups blocked), and nitrated‐acetylated chymotrypsinogen were titrated as __f__(pH) in an isoperibolic calorimeter at 20°C. After appropriate correction and reduction