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
1HRP-conjugate concentration too low or detection antibody too dilute
2Substrate incubation time insufficient for colorimetric development
3Plate reader using incorrect wavelength (wrong filter for chromogen or fluorochrome)
4Capture antibody did not bind well to plate (tissue culture plate used or coated in protein-containing buffer)
5Standard curve dilutions calculated incorrectly
Solutions
1Check and optimize HRP-conjugate and detection antibody dilutions through titration
2Extend substrate incubation time (typically 15-30 min for TMB until blue color develops)