ChemistryOpen (Jun 2025)

Measuring the Thermal Unfolding of Lysozyme: A Critical Comparison of Differential Scanning Fluorimetry and Differential Scanning Calorimetry

  • Weronika Malicka,
  • Yueyue Dai,
  • Andreas Herrmann,
  • Rainer Haag,
  • Matthias Ballauff,
  • Marina Pigaleva,
  • Thomas Risse,
  • Daniel Lauster,
  • Iman Asakereh,
  • Mazdak Khajehpour

DOI
https://doi.org/10.1002/open.202400340
Journal volume & issue
Vol. 14, no. 6
pp. n/a – n/a

Abstract

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Abstract The thermal unfolding of lysozyme in aqueous solution has been analyzed by (nano) differential scanning fluorimetry (nanoDSF) and differential scanning calorimetry (DSC). In addition, dynamic light scattering (DLS) acquired in parallel to the DSF measurements, was used to confirm that the change in hydrodynamic radius upon unfolding is rather small (RH,f =1.75 nm in the folded state; and RH,u=1.91 nm in the unfolded state). NanoDSF measurements were evaluated to characterize the folding/unfolding transition within the classical two‐state folding model. The temperature of unfolding (Tm) is found to be the most robust quantity. The unfolding enthalpy ΔHu and the change of specific heat were also obtained and errors in the range of 5–10 % and 30–50 % were determined, respectively. A comparison of thermodynamic parameters from nanoDSF and DSC measurements provides evidence for an increasing unfolding enthalpy ΔHu with protein concentration. A comparison with data from literature suggests that a weak association in the folded state can lead to the observed change of the unfolding enthalpy. For Δcp significantly higher values is deduced from the analysis of temperature dependent nanoDSF measurements (10 kJ/(K mol)) as compare to DSC (3–5 kJ/(K mol)).