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Dear,
I am trying your software on my own dataset. I have around 29000 cells in which in total around 16000 genes are detected. Moreover, there are 65 genes that are perturbed. What is the best way to determine the prior parameters for fit0? In my last execution I used prior_beta_s = 20 (and the others as specified in the vignette), but I still have a lot of genes with lsfr equal to 0, which makes it hard to identify the real impact..
Thank you in advance!
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