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ELISA (R&D Guide) severe

Poor Dynamic Range Between Signal and Background

Symptom
The difference between maximum signal (high standards) and background (blank wells) is compressed, typically less than 5-fold, making it difficult to distinguish between samples of different concentrations.
Common Causes
  1. 1 HRP-conjugate concentration too low or detection antibody too dilute
  2. 2 Substrate incubation time insufficient for colorimetric development
  3. 3 Plate reader using incorrect wavelength (wrong filter for chromogen or fluorochrome)
  4. 4 Capture antibody did not bind well to plate (tissue culture plate used or coated in protein-containing buffer)
  5. 5 Standard curve dilutions calculated incorrectly
Solutions
  1. 1 Check and optimize HRP-conjugate and detection antibody dilutions through titration
  2. 2 Extend substrate incubation time (typically 15-30 min for TMB until blue color develops)
  3. 3 Verify plate reader wavelength matches protocol specification (e.g. 450 nm for TMB, 405 nm stop)
  4. 4 Use ELISA-validated plates; dilute capture antibody/antigen in PBS without additional protein (no BSA/serum)
  5. 5 Recalculate and prepare fresh standard curve; verify serial dilution accuracy
Related Video (2)
Bilibili (China-Accessible Mirrors) ★ 85
How to Run an R&D Systems Quantikine ELISA
"Complete R&D Systems Quantikine ELISA workflow demonstration with troubleshooting guidance directly addresses detection antibody and HRP-conjugate optimization issues"
Bilibili (China-Accessible Mirrors) ★ 78
DuoSet ELISA — Sandwich ELISA Hands-on Protocol (Bio-Techne)
"Hands-on DuoSet sandwich ELISA protocol explicitly covers capture/detection antibody steps and substrate development critical for optimizing signal-to-background ratio"
Source: rndsystems.com ↗
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