PARP (Poly ADP-Ribose Polymerase) proteins are a large family of 17 members that catalyze the ADP-ribosylation of proteins and, for PARP1 and PARP2, of DNA. PARPs are part of a network of 150 proteins involved in the DNA damage response, which constantly scan and repair DNA to maintain genome integrity. The PARP proteins are involved in a wide range of biological functions: DNA repair, chromatin remodeling, mitotic spindle assembly, regulation of RNA turnover, regulation of gene expression, apoptosis, and more.
Accelerate your drug discovery and development projects using PARP or PARPtrap™ screening services. We offer the largest PARP proteins panel on the market, allowing you to compare efficacy across our entire PARP family.
Our team of experts, using our in-house developed biochemical assay kits, will:
Screen for PARP inhibitors from large compound libraries, measured by ELISA, AlphaLISA®, or Fluorescence Polarization assays
Screen for PARG inhibitors
Compare potency with IC50 screens
Answer your questions and guide your project in a timely manner
Deliver detailed results promptly and on time
Enzymatic Activity by ELISA
ELISA: Histone proteins are coated on a plate. Biotin-labeled NAD+ is added with the PARP enzyme. PARP-mediated ribosylation activity is detected by adding Streptavidin-HRP (horseradish peroxidase), which binds to the newly formed ribosylation branch, and a chemiluminescent or colorimetric HRP substrate.
Enzymatic Activity by AlphaLISA®
AlphaLISA® Assay: a PARP enzyme is incubated with biotinylated histone substrate and NAD+ for an hour. An ADP-ribose binding reagent is added with an acceptor bead, then a streptavidin-conjugated donor bead is added. Excitation of the donor bead results in excitation of the acceptor bead and light emission. This is a homogeneous assay.
PARP Trapping
Fluorescence Polarization Assay: The assay uses fluorescent DNA probes that emit differently polarized light depending on PARP binding. Addition of a PARP inhibitor prevents ribosylation and results in the trapping of PARP onto the fluorescent oligonucleotide duplex, which increases the Fluorescence Polarization signal in a dose dependent manner. This is a homogeneous assay.
Molecular Degradation Optimization
AlphaLISA® Assay: A degrader of interest interacts with both PARP and CRBN, bringing them in proximity. PARP-GST is recognized by the GSH donor bead, while CRBN-FLAG binds to anti-FLAG conjugated to the acceptor bead. Excitation of the donor bead results in excitation of the acceptor bead and light emission. This is a homogeneous assay.
Available Service Assays
Chemiluminescent Assays*:
| PARG | PARP1 | PARP2 | PARP3 | PARP4 | PARP5A (TNKS1) | PARP5B (TNKS2) | PARP6 | |
| PARP7 | PARP8 | PARP10 | PARP11 | PARP12 | PARP14 | PARP15 | PARP16 | |
*
NOTE: As of April 2022, these protocols have been re-optimized for performance. Previous versions of this protocol are available upon request.
Colorimetric Assays:
| PARP1 | PARP2 | PARP5A (TNKS1) | PARP5B (TNKS2) |
Homogenous Assays:
| PARP1 | PARP2 | PARP3 | PARP5A (TNKS1) | PARP5B (TNKS2) | PARP11 |
PARPTrap™ Assays:
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