Home Failure Case Library Buffer Components Inhibit Detection Enzyme
ELISA (Signal Problems) severe

Buffer Components Inhibit Detection Enzyme

Symptom
No or very weak signal despite correct antibody binding. Signal loss occurs after addition of detection reagent. Other wells using different buffers show normal signal.
Common Causes
  1. 1 Sodium azide (commonly 0.02-0.1% in antibody storage buffers) inhibits HRP enzyme activity
  2. 2 High concentration of reducing agents (e.g., DTT, β-mercaptoethanol) interferes with enzyme conjugates
  3. 3 Buffer pH is outside optimal range for enzyme activity (HRP optimal at pH 5.0-6.0)
  4. 4 Chelating agents (e.g., EDTA) remove metal ions required for enzyme function
Solutions
  1. 1 Remove sodium azide from all buffers used with HRP-conjugated antibodies; use alternative preservatives
  2. 2 Avoid buffers containing reducing agents or chelating agents during detection steps
  3. 3 Ensure detection buffer pH is within optimal range: pH 5.0-6.0 for HRP, pH 8.0-9.5 for alkaline phosphatase
  4. 4 Use manufacturer-recommended buffers or prepare fresh detection buffers without incompatible reagents
Related Video (2)
Bilibili (China-Accessible Mirrors) ★ 75
DuoSet ELISA — Sandwich ELISA Hands-on Protocol (Bio-Techne)
"Demonstrates complete sandwich ELISA workflow including substrate development and detection steps where HRP inhibition would manifest as signal loss"
Bilibili (China-Accessible Mirrors) ★ 72
How to Run an R&D Systems Quantikine ELISA
"R&D Systems Quantikine protocol with troubleshooting guidance relevant to diagnosing signal problems in detection enzyme phase"
Source: abcam.com ↗
← Back to all cases