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Originally posted by icenzano March 28, 2024
Hello everyone! I am starting with multi-omics analysis and I need to analyze our three 10x multi-omics datasets with ArchR. However, I am not sure about the correct order to follow. If I have multiple samples, which is the correct approach?
Should I integrate RNA samples and ATAC samples separately using Harmony (or any other batch correction method) and then combine/integrate both omics layers using the batch corrected dimension coming from each omic?
Or, should I integrate both omics layers first and then correct the batch effect coming from having three samples using Harmony (or any other batch correction method) within the combined dimension?
Thank you.
The text was updated successfully, but these errors were encountered:
Hi @icenzano! Thanks for using ArchR! Lately, it has been very challenging for me to keep up with maintenance of this package and all of my other
responsibilities as a PI. I have not been responding to issue posts and I have not been pushing updates to the software. We are actively searching to hire
a computational biologist to continue to develop and maintain ArchR and related tools. If you know someone who might be a good fit, please let us know!
In the meantime, your issue will likely go without a reply. Most issues with ArchR right not relate to compatibility. Try reverting to R 4.1 and Bioconductor 3.15.
Newer versions of Seurat and Matrix also are causing issues. Sorry for not being able to provide active support for this package at this time.
Discussed in #2141
Originally posted by icenzano March 28, 2024
Hello everyone! I am starting with multi-omics analysis and I need to analyze our three 10x multi-omics datasets with ArchR. However, I am not sure about the correct order to follow. If I have multiple samples, which is the correct approach?
Thank you.
The text was updated successfully, but these errors were encountered: