Dissection of the protein G B1 domain binding site for human IgG Fc fragment

DAVID J. SLOAN; HOMME W. HELLINGA

doi:10.1110/ps.8.8.1643

Abstract

The contribution to the free energy of binding of each of the residues forming the binding site for a human IgG Fc fragment on the surface of the B1 domain of protein G was determined by alanine-scanning mutagenesis. The interface between these two proteins is atypical in that it is smaller than usual, polar in character, and involves two well-defined “knobs-into-holes” interactions. The bulk of the free energy of binding is contributed by three central residues, which make hydrogen bonds across the interface. Of these, the most critical interaction is formed by Glu27, which acts as a charged knob on the surface of the B1 domain, inserting into a polar hole on the Fc fragment. A single alanine mutation of this residue virtually abolishes stable complex formation. Formation of a stable interface between these two proteins is therefore dominated by a small, polar “hot spot.”

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Dissection of the protein G B1 domain binding site for human IgG Fc fragment

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Dissection of the protein G B1 domain binding site for human IgG Fc fragment

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