Home Failure Case Library No Signal in Co-IP Due to Stringent Lysis Buffer
Immunoprecipitation (CST Guide) severe

No Signal in Co-IP Due to Stringent Lysis Buffer

Symptom
No signal detected in co-immunoprecipitation experiment despite adequate protein expression confirmed by input lysate control. Western blot shows no target protein bands after IP.
Common Causes
  1. 1 RIPA Buffer (#9806) containing ionic detergent sodium deoxycholate disrupts protein-protein interactions
  2. 2 Kinase denaturation caused by denaturing buffer components incompatible with co-IP
  3. 3 Insufficient sonication leading to incomplete nuclear rupture and poor protein recovery
  4. 4 Membrane protein complexes disrupted by overly stringent detergent conditions
Solutions
  1. 1 Use Cell Lysis Buffer #9803 instead of RIPA Buffer for all IP and co-IP experiments
  2. 2 Perform adequate sonication to ensure nuclear rupture, DNA shearing, and maximal protein recovery without disrupting protein complexes
  3. 3 Include input lysate control to verify target protein expression and antibody functionality
  4. 4 Probe blot with antibody to IP protein to confirm successful pull-down of primary protein
Related Video (2)
Cell Signaling Technology ★ 85
Western Blotting Protocol
"Western blotting is the detection method used to visualize co-IP results; understanding proper technique is essential to troubleshoot signal loss"
Cell Signaling Technology ★ 78
How CUT&RUN Profiles Chromatin | Cell Signaling Technology
"CUT&RUN is explicitly presented as an alternative to chromatin immunoprecipitation, providing context on IP methodology and protein-chromatin interaction preservation strategies"
Source: cellsignal.com ↗
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