I generated a phage library against a specific peptide. After several rounds of panning, I do see an enrichment in specific phages but only 2 fold as compared to the BSA control. What is the best measure to check if panning has successfully worked? How does one normalizes the phage pools used for ELISA?
Thanks
Ruchi
Diogo Estêvão
Hi Ruchi,
I would say that a clear enrichment is observed when you see equal or more than 10 fold enrichment between your antigen condition and control
Good luck!
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