After developing the ELISA plate, wells show no color change or very faint signal that is barely above background, even for positive controls or high-concentration standards.
Common Causes
1Reagents added in incorrect order or prepared improperly (e.g. wrong dilution factors, expired reconstituted standard)
2Primary or secondary antibody concentration too low, or incubation time insufficient
3Capture antibody or antigen failed to bind to plate (wrong plate type, coating time <4 h at room temperature)
4Capture and detection antibodies recognize the same epitope in sandwich ELISA
5Sodium azide present in buffers or antibody storage solution (inhibits HRP activity)
6Sample analyte concentration below detection range or masked by sample matrix components
Solutions
1Repeat experiment following exact protocol order; centrifuge lyophilized standard before reconstitution
2Increase antibody concentration via titration or extend incubation to overnight at 4°C
3Use ELISA-validated plates (not tissue culture plates); extend coating to overnight at 4°C
4Verify antibodies recognize distinct epitopes; use validated matched antibody pairs
5Remove sodium azide: increase washing steps or use azide-free buffers
6Perform serial dilutions starting with concentrated sample; spike samples with known antigen to test for interference