Figure 3
Figure 3. eTAFH mutations impair HEB binding. (A) ITC measurements of the binding of HEB peptide to wild-type and mutant eTAFH domains. In each panel, the top portion is the raw data, and the bottom portion is a plot of the binding corrected for dilution enthalpy (squares indicate experimental data; line, fit to a one-site binding model). The average N (stoichiometry) and Kd from 2 independent experiments (± SD) for each protein are shown in the box. The stoichiometry was fixed to 1 to fit the F332A mutant data. (B) Overlay of 15N-1H HSQC spectra of wild-type eTAFH domain (red) and the F277A mutant (blue). Most peaks in the F277A mutant are absent or shifted, indicating the structure is disrupted.

eTAFH mutations impair HEB binding. (A) ITC measurements of the binding of HEB peptide to wild-type and mutant eTAFH domains. In each panel, the top portion is the raw data, and the bottom portion is a plot of the binding corrected for dilution enthalpy (squares indicate experimental data; line, fit to a one-site binding model). The average N (stoichiometry) and Kd from 2 independent experiments (± SD) for each protein are shown in the box. The stoichiometry was fixed to 1 to fit the F332A mutant data. (B) Overlay of 15N-1H HSQC spectra of wild-type eTAFH domain (red) and the F277A mutant (blue). Most peaks in the F277A mutant are absent or shifted, indicating the structure is disrupted.

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