Assays for mechanistic investigations of protein/histone acetyltransferases

Protein/histone acetyltransferases (PATs/HATs) have been implicated in a number of cellular functions including gene regulation, DNA synthesis, and repair. This paper reviews methods that can be used to quantitatively determine the activity and ultimately the catalytic/kinetic mechanism of PAT/HATs...

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Veröffentlicht in:Methods (San Diego, Calif.) Calif.), 2005-08, Vol.36 (4), p.321-331
Hauptverfasser: Berndsen, Christopher E., Denu, John M.
Format: Artikel
Sprache:eng
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Zusammenfassung:Protein/histone acetyltransferases (PATs/HATs) have been implicated in a number of cellular functions including gene regulation, DNA synthesis, and repair. This paper reviews methods that can be used to quantitatively determine the activity and ultimately the catalytic/kinetic mechanism of PAT/HATs in vitro. Two methods will be described in detail. The first method is a filter-binding assay that measures the transfer of radiolabeled acetate from acetyl-CoA to protein. The second method is a continuous, spectroscopic, enzyme-coupled assay that links the PAT/HAT reaction to the reduction of NAD + by pyruvate or α-ketoglutarate dehydrogenase. Both methods are highly applicable in determining steady-state reaction rates, and obtaining the kinetic constants V max, K m, and V/ K from substrate saturation curves. We describe a new application of the filter-binding assay to determine the kinetic parameters for HATs using low concentrations of nucleosomal substrates.
ISSN:1046-2023
1095-9130
DOI:10.1016/j.ymeth.2005.03.002