Zinc binding of a Cys2His2-type zinc finger protein is enhanced by the interaction with DNA

Author:

Hajdu BálintORCID,Hunyadi-Gulyás ÉvaORCID,Kato Kohsuke,Kawaguchi AtsushiORCID,Nagata KyosukeORCID,Gyurcsik BélaORCID

Abstract

Abstract Zinc finger proteins specifically recognize DNA sequences and, therefore, play a crucial role in living organisms. In this study the Zn(II)-, and DNA-binding of 1MEY#, an artificial zinc finger protein consisting of three finger units was characterized by multiple methods. Fluorimetric, circular dichroism and isothermal calorimetric titrations were applied to determine the accurate stability constant of a zinc finger protein. Assuming that all three zinc finger subunits behave identically, the obtained thermodynamic data for the Zn(II) binding were ΔHbinding site =  − (23.5 − 28.0) kcal/mol (depending on the applied protonation state of the cysteines) and logβpH 7.4 = 12.2 ± 0.1, being similar to those of the CP1 consensus zinc finger peptide. The specific DNA binding of the protein can be characterized by logβpH 7.4 = 8.20 ± 0.08, which is comparable to the affinity of the natural zinc finger proteins (Sp1, WT1, TFIIIA) toward DNA. This value is ~ 1.9 logβ’ unit higher than those determined for semi- or nonspecific DNA binding. Competitive circular dichroism and electrophoretic mobility shift measurements revealed that the conditional stability constant characteristic for Zn(II) binding of 1MEY# protein increased by 3.4 orders of magnitude in the presence of its target DNA sequence. Graphical abstract

Funder

EU Horizon 2020

Hungarian National Research, Development and Innovation Office

University of Szeged

Publisher

Springer Science and Business Media LLC

Subject

Inorganic Chemistry,Biochemistry

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