Home Failure Case Library Wrong Instrument Settings for Detection Wavelength
ELISA (Signal Problems) moderate

Wrong Instrument Settings for Detection Wavelength

Symptom
No signal or very low signal readings from plate reader despite visible color development or expected fluorescence. Signal does not correlate with visual observations.
Common Causes
  1. 1 Plate reader absorbance wavelength does not match substrate (e.g., TMB requires 450 nm, OPD requires 490 nm)
  2. 2 Excitation/emission filters are incorrect for the fluorophore used
  3. 3 Detection mode is set to wrong method (e.g., endpoint instead of kinetic)
  4. 4 Reference wavelength setting interferes with signal measurement
Solutions
  1. 1 Verify correct absorbance wavelength: TMB at 450 nm, ABTS at 405 nm, OPD at 490 nm
  2. 2 Confirm fluorescence excitation/emission match fluorophore specifications exactly
  3. 3 Use kinetic reading mode for slow-developing colorimetric reactions to capture signal development over time
  4. 4 Check reference wavelength is appropriate (typically 540-650 nm for colorimetric assays)
Related Video (3)
Bilibili (China-Accessible Mirrors) ★ 85
Thermo Fisher Microplate Reader Software Operation
"Directly addresses microplate reader software operation and instrument control, which is essential for understanding and correcting wavelength settings that caused the detection failure."
Bilibili (China-Accessible Mirrors) ★ 78
DuoSet ELISA — Sandwich ELISA Hands-on Protocol (Bio-Techne)
"Explicitly demonstrates plate reading at 450 nm for sandwich ELISA, providing concrete example of correct wavelength selection for TMB substrate detection."
Bilibili (China-Accessible Mirrors) ★ 72
How to Run an R&D Systems Quantikine ELISA
"Complete R&D Systems Quantikine ELISA workflow with troubleshooting guidance provides context for identifying and resolving detection signal problems."
Source: abcam.com ↗
← Back to all cases