Immunoprecipitation Controls IP Controls

By Ryan Hamnett, PhD

Immunoprecipitation (IP) is a technique that uses antibodies to enrich or purify a target protein from a complex biological sample. Controls are essential for confirming the accuracy, reliability and sensitivity of IPs, and can assist with troubleshooting in case of spurious results.

Control Type of control Description Purpose Notes
Supernatant controls Negative Run the supernatant from each main step on the gel and western blot (WB) Confirms that target protein has successfully been depleted and held (bound by antibody) at each stage Supernatants from all steps (pre-clearing, IP, washing, elution) can be kept for troubleshooting in case the expected band is not seen in the experimental lane
Bead only control Negative Run the IP as normal but in the absence of any antibody Identifies non-specific binding to the beads alone May not be necessary if performing an isotype control, which will also pick up non-specific binding to beads, but can help with troubleshooting
Isotype control Negative Run the IP as normal but replacing the antibody with an isotype control antibody Identifies non-specific binding to the antibody (e.g. to the Fc region) due to its isotype
Knockdown or knockout control Negative Run the full IP on a sample known not to express the target protein due to knockout or knockdown Confirms the specificity of the antibody Performing the IP on a sample known not to express the protein naturally (e.g. because it is a different tissue type) may also be sufficient
Input control Positive Run 1-10% of the starting lysate on the gel and WB 1) Demonstrates IP was successful: there should be a band in both the IP and input lanes

2) Indicates IP efficiency: comparing strengths of target bands in IP and input lanes

3) Indicates IP specificity: comparing strengths of non-specific bands

4) Indicates consistency of starting material amount
Typically run alongside every IP. Particularly important for co-IP
Positive lane control Positive Run purified recombinant target protein on the gel and WB Serves as a positive reference Running a sample known to express high levels of the protein naturally (e.g. from a different tissue type) may also be sufficient

Table 1:Key controls to run alongside an IP experiment.

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