The EpiQuik™ Global Acetyl Histone H3-K36 Quantification Kit (Colorimetric) is a convenient package of tools that allows the experimenter to specifically measure global acetylation of histone H3-K36 colorimterically, using a variety of mammalian cells (human, mouse, etc.) including fresh and frozen tissues, and cultured adherent and suspension cells. The kit has the following advantages:
Background InformationAcetylation of histones, including histone H3, has been involved in the regulation of chromatin structure and recruitment of transcription factors to the gene promoters. Histone acetyltransferases (HATs) and histone deacetylases (HDACs) play a critical role in control of histone H3 acetylation at multiple sites. Acetylation of histone H3 at lysine 36 (H3-K36) is a conserved modification, which functions in transcription. Acetylation of histone H3-K36 is tightly involved in the cell cycle regulation, cell proliferation, and apoptosis. An imbalance in the equilibrium of histone H3 acetylation, including K36 acetylation, has been associated with cancer progression. Histone H3- K36 acetylation may be increased by inhibition of HDACs and decreased by HAT inhibition. Thus, quantitative detection of global acetyl histone H3-K36 would provide useful information for better understanding epigenetic regulation of gene activation, and for developing HAT or HDACtargeted drugs. The EpiQuik™ Global Acetyl Histone H3-K36 Quantification Kit (Colorimetric) provides a tool for measuring global acetylation of histone H3-K36.
Principle & ProcedureThis kit is designed for measuring global histone H3-K36 acetylation. In an assay with this kit, the acetyl histone H3 at lysine 36 is captured to the strip wells coated with an anti-acetyl H3-K36 antibody. The captured acetyl histone H3-K36 can then be detected with a labeled detection antibody followed by a color development reagent. The ratio of acetyl H3-K36 is proportional to the intensity of absorbance. The absolute amount of acetyl H3-K36 can be quantified by comparing to the standard control.
Starting MaterialsInput material should be purified histone extracts. In general, the input amount should be from 50 ng to 200 ng per well of histone extracts.