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ChIP (PCR Amplification Problems) severe

No DNA Amplification in ChIP Samples

Symptom
No PCR product is detected in ChIP samples by qPCR or gel electrophoresis. Ct values fail to appear or remain above threshold, and no visible bands are observed on gels.
Common Causes
  1. 1 Primers are non-functional or degraded
  2. 2 Insufficient ChIP DNA input due to poor immunoprecipitation efficiency
  3. 3 DNA degradation during ChIP or storage
  4. 4 PCR inhibitors carried over from ChIP buffers or beads
  5. 5 Incorrect primer design targeting wrong genomic region
Solutions
  1. 1 Include standard/input DNA control to confirm primers are working properly
  2. 2 Test primers on known positive control DNA (e.g. 10% input chromatin)
  3. 3 Verify DNA concentration using Qubit or spectrophotometry; ensure sufficient template
  4. 4 Dilute ChIP eluate (e.g. 1:5 or 1:10) to reduce potential PCR inhibitors
  5. 5 Check primer sequences and validate genomic coordinates match target site
  6. 6 Use fresh primer aliquots; avoid repeated freeze-thaw cycles
Related Video (3)
YouTube (Curated Tutorials) ★ 85
The Features Of A Good qPCR Primer Pair
"Directly addresses primer pair design and validation—the core issue in this failure case of non-functional or degraded primers."
Bilibili (China-Accessible Mirrors) ★ 78
ChIP-Seq: Chromatin Immunoprecipitation Principles & Protocol
"Comprehensive ChIP protocol walkthrough provides experimental context and proper execution guidance to prevent upstream errors affecting PCR amplification."
Bilibili (China-Accessible Mirrors) ★ 72
qPCR Primer Design: NCBI Screencast Tutorial
"Step-by-step NCBI primer design tutorial helps researchers validate and design functional primers before use in ChIP-qPCR workflows."
Source: abcam.com ↗
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