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I have a relatively large bulk RNA seq dataset (~ 1300 samples, from ~70 experiments) that I'd like to correct for significant batch effects. Is it valid/possible to apply BERMUDA to my dataset? Instead of clustering cells of patients, I'd just cluster patients to remove batch effects. Is this valid?
The text was updated successfully, but these errors were encountered:
While the use of domain adaptation in BERMUDA does not specifically restrict to single-cell data, the whole workflow of BERMUDA also depends on Seurat and Metaneighbor, which are designed for single-cell data. We also only applied BERMUDA in single-cell data in our paper. Therefore, I would suggest using the batch correction method designed for bulk data for your dataset.
I have a relatively large bulk RNA seq dataset (~ 1300 samples, from ~70 experiments) that I'd like to correct for significant batch effects. Is it valid/possible to apply BERMUDA to my dataset? Instead of clustering cells of patients, I'd just cluster patients to remove batch effects. Is this valid?
The text was updated successfully, but these errors were encountered: