Sirtuin activity assays

Sirtuin activity assays

Sirtuin activity assays are experimental methods used to measure the enzymatic activity of sirtuins, a family of NAD+-dependent deacetylases and deacylases. These enzymes are key regulators of chromatin structure, metabolism, stress responses, and aging-related pathways. Because sirtuins act on both histone and non-histone substrates, activity assays are widely applied in epigenetics, cell biology, and drug discovery.

Principle of the Assay

Most sirtuin activity assays are based on detecting deacetylation or deacylation of synthetic peptide substrates. The reaction requires NAD+, which is consumed during catalysis and represents a defining biochemical feature of sirtuin enzymes. Depending on the assay format, detection can be fluorescent, colorimetric, luminescent, or mass spectrometry-based.

Assay Formats

Sirtuin activity can be measured using direct enzymatic assays, coupled assay systems, or antibody-based detection methods. Fluorescence-based assays are widely used due to their sensitivity and compatibility with high-throughput screening platforms. Luminescent and colorimetric formats are also commonly applied, particularly in inhibitor screening and comparative enzyme activity studies.

Biological Targets

The assay can be designed to evaluate different sirtuin isoforms, including SIRT1, SIRT2, SIRT3, SIRT5, and others. Each isoform exhibits distinct substrate preferences and subcellular localization, resulting in specific biological functions. Careful selection of substrates and assay conditions is therefore critical for accurate interpretation of enzymatic activity.

Applications in Research

Sirtuin activity assays are used in studies of aging, metabolism, neurobiology, cancer biology, and inflammatory signaling. They are also essential tools for evaluating small-molecule activators and inhibitors that modulate sirtuin function. In basic research, these assays help elucidate how cellular conditions such as nutrient availability and oxidative stress influence protein deacetylation dynamics.

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