A high-throughput assay shows that DNase-I binds actin monomers and polymers with similar affinity |
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| Authors: | Morrison Scott S Dawson John F |
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| Affiliation: | Department of Molecular and Cellular Biology, University of Guelph, Guelph, Ontario N1G 2W1, Canada. |
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| Abstract: | Previous conflicting reports suggest that DNase-I binds F-actin with either equal or drastically different K(D) values compared to G-actin. We developed a high-throughput DNase-I inhibition assay to determine the K(D) of DNase-I for F-actin. We confirmed that phalloidin-stabilized F-actin is protected from depolymerization by DNase-I and that the critical concentration at the pointed end of phalloidin-F-actin is 45.5+/-13.9 nM. We found that DNase-I inhibition by actin follows ultrasensitive mechanics. Using varying lengths of gelsolin-capped phalloidin-F-actin, we concluded that the affinities of DNase-I for G- and the pointed end subunits of F-actin are almost indistinguishable, such that DNase-I may not distinguish between G- and F-actin conformations. |
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| Keywords: | Actin DNase-I Phalloidin Gelsolin Actin binding proteins Ultrasensitivity Critical concentration Dissociation constant |
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