Developer Reagent【子货号:G653A,包装:1 x 10μl,,运保温度:–20°C】
HDAC-Glo™ 2 Buffer【子货号:G957A,包装:1 x 25ml,,运保温度:–20°C】
HDAC-Glo™ 2 Substrate【子货号:G958A,包装:1 x 10μl,,运保温度:–20°C】
Luciferin Detection Reagent【子货号:V859A,包装:1 x 1 each,,运保温度:–20°C】
描述:
The HDAC-Glo™ Class IIa and HDAC-Glo™ 2 Assays are single-reagent-addition, homogeneous, luminescent assays that measure the relative activity of histone deacetylase (HDAC) Class IIa and Class I enzyme 2, respectively, from cells, extracts or purified enzyme sources.
The assays use an acetylated, live-cell-permeant, luminogenic peptide substrate that can be deacetylated by HDAC activities. Deacetylation of the peptide aminoluciferin substrate is measured using a coupled enzymatic system in which a protease in the Developer Reagent cleaves the deacetylated peptide from the aminoluciferin substrate, releasing aminoluciferin, which is quantified in a reaction using Ultra-Glo™ Recombinant Luciferase (firefly). The signal from the assay reaction can be measured within 15–45 minutes after reagent addition with no sample manipulation. The HDAC-mediated luminescent signal is persistent, with a half-life of greater than 2 hours, allowing batch processing of multiwell plates.
Features - Benefits
Provide Relevant Insight into Compound Effects in Biological Setting:Make better decisions about your compound library early in drug screening.
Panel of Screening Tools Allows Comprehensive Screening of HDAC Activity:Easy detection of Class IIa or Isozyme 2 in the same, convenient platform.
Highly Sensitive:Feel confident because you can see more. Obtain a dynamic range 10- to 100-fold higher than comparable fluorescence methods.
Flexible Format:Determine inhibitor performance in both biochemical and predictive cell-based formats using viable cells or in vitro with cell extracts or purified recombinant enzymes.
Simple Measurement of Deacetylating Activities:Easy implementation from benchtop to screening with a single-reagent-addition, homogeneous, add-mix-measure protocol.
Fast Data Acquisition in as Little as 15 Minutes:Achieve maximum signal in as little as 15 minutes with persistent glow-type steady-state signal, making the protocol amenable to automation in high-throughput formats and compatible with luminometers without injectors.
Robust Detection:Minimize assay interference often encountered with fluorescent assays with robust, bioluminescence-based detection. This technology also allows you to multiplex with cell-health assays, offering more biologically relevant data within a predictive, cell-based context.
Applications
Determine HDAC inhibitor potency using purified enzymes, extracts or cells directly in culture plates.
Selectively profile HDAC inhibitors with purified enzymes.
Correlate HDAC inhibitor potency with cellular fate in same-well multiplexed viability assays.
Determine off-target HDAC effects of compounds.
Notes
Cat.# G9560 and G9590 are sufficient to perform 100 × 100µl assays in 96-well plates or 1,000 × 10µl biochemical-based assays in 384-well plates (500 × 20µl cell-based assays in 384-well plates).
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