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Researchers rely on ELISA to detect and measure antigens in samples because of its robust nature, high degree of sensitivity, and ease of performance. However, it is possible to run into certain issues that cause ELISA-based experiments to produce inaccurate or irreproducible results. Accuracy is the degree of closeness between the obtained experimental value and the accepted true value under the experimental conditions. Reproducibility is the amount of variation between different samples within the same run of an assay or the variation between different assays performed on multiple days or by different researchers. 

The two primary factors that impact accuracy and reproducibility are non-specific binding and cross-reaction. Non-specific binding (NSB) occurs when substances other than the target reagents absorb into the plate, causing high background noise or false signals. Adding a blocking buffer is a crucial step for saturating the unoccupied wells of the plate and preventing NSB. Cross-reaction refers to any unexpected interactions between an antibody and non-specific analytes and is common among indirect ELISAs when the enzyme-labeled secondary antibody or an enzyme-labeled avidin against the detection antibody reduces the selectivity of the assay. 

Here are some of the most common ELISA issues experienced by researchers, alongside their potential causes and corresponding solutions:

Weak or Low Signal Intensity

Excessive Signal Intensity

High Background Noise

Poor Linearity or Dynamic Range of the Standard Curve

A captured antibody that does not bind to the plate can also result in weak/low signal intensity and poor standard curves. This can occur when the antibody lacks sufficient binding affinity towards the target. If you are coating a plate yourself rather than purchasing a kit with a pre-coated plate, make sure you are using a plate specifically designed for ELISA, not a tissue culture plate. Confirm correct preparation and incubation time for coating and blocking. 

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