Protein Folding
Idea: in this experiment we investigate protein (un)folding
by chemical denaturation of human serum albumin using tryptophan as an intrinsic fluorescent reporter
Biophysics Lab Course, Institute of Biophysics, Îçҹ̽»¨
The folding equilibrium of the plasmaprotein HSA (Human Serum Albumin) is characterized from the fluorescence of a tryptophan residue at position 214.
Successive addition of the denaturant GdmCl leads to an increasing spectral shift of Trp-214 fluorescence, which allows to quantify the increasing fraction of unfolded protein.
The free energy change between folded and unfolded state is determined for two different pH-values by extrapolation to zero denaturant concentration.
Biophysics Lab Course: Gene expression | Bioinformatics | Protein labelling | Protein crystallization | Protein folding | Stopped-flow kinetics | Single-molecule fluorescence | Fluorescence lifetime | Ligand binding | Fluorescence correlation spectroscopy (FCS) | Lipid monolayers | Ion channels | Live cell imaging | Superresolution microscopy | Optical tweezers | AFM
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Master of Science in Biophysics
Contact: Prof. Dr. Jens Michaelis, Dr. Carlheinz Röcker, Institute of Biophysics
