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- Description:c-Myc-Tag Magnetic IP/Co-IP Kit
- Size:40 reactions
- Environmentally Preferable:
- Cat. No.:PI88844
- Supplier no.:88844
Magnetic c-Myc-Tag IP/Co-IP kit contains specific immunoaffinity magnetic beads and reagents to perform immunoprecipitation assays of c-Myc fusion proteins or co-IP experiments using c-Myc-tagged bait proteins.
- Specific magnetic beads - covalently immobilized high-quality anti-c-Myc monoclonal antibody enables high yields of immunoprecipitation products
- Low non-specific binding - stable, pre-blocked beads and specific antibody minimize off-target binding
- Trouble-free elution - low-pH elution buffer ensures recovery of c-Myc-tagged protein interaction complexes without antibody leaching contamination
- Convenient and fast - complete kit and easy-to-follow instructions provide optimized protocols to perform IP or Co-IP experiment in approximately 1 hour
- Versatile - magnetic beads are compatible with manual and automated magnetic separation workflows
Unlike traditional IP procedures based on capture with Protein A/G beads, this kit uses magnetic beads containing pre-immobilized anti-c-Myc antibody. These anti-c-Myc magnetic beads ensure specific binding of c-Myc tagged protein complexes from biological samples. Because the antibody is covalently attached to the beads, IP-targets are easily eluted and recovered without antibody contamination.
The c-Myc peptide (EQKLISEEDL) derived from the C-terminus region of human c-Myc protein is one of several fusion protein tags used for recombinant protein expression. The Pierce c-Myc Magnetic IP/Co-IP Kit uses a specific, high-affinity immobilized antibody (clone 9E10) for rapid immunoprecipitation of c-Myc tagged fusion proteins from bacterial and mammalian cell lysates, as well as from lysates prepared with the Pierce Human in vitro Translation Kits. The beads are incubated with a cell lysate containing c-Myc tagged protein, the fusion protein is captured, and the beads are subsequently washed and then eluted using low-pH elution buffer or non-reducing sample buffer. The protocol and buffers have been optimized for both IP and co-IP reactions, enriching for specific protein interaction complexes in the eluted samples. Anti-c-Myc antibody can be used to detect c-Myc tagged protein by western blot analysis.