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Endothelial cell differentiation CMO library processing

This repository contains the commands used to reconstruct per-channel GEX and CMO FASTQs from the mixed 10x multiome / CMO 5 timepoints sequencing data.

Summary of the steps:

  1. Concatenate the FASTQs
  2. Separate CMO from GEX with splitcode
  3. Trim CMO R1 file
  4. Quantify CMO tags per barcode using the kite workflow from kb

10X Genomics multi-ome 5 timepoints:

README.md

10X Genomics multi-ome 15 timepoints:

README.md

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Reproducible analysis code for endothelial differentiation 10x Multiome CMO experiments across timepoints

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