R (version 4.0 or higher) and RStudio (recommended).
If you work with next-generation sequencing (NGS) data, particularly RNA-seq, you know the nightmare of batch effects. You run your experiment, get your counts, but when you cluster the samples, they separate by date of extraction or sequencing run rather than by treatment group. sequator download
The object svobj$sv contains your new "Sequnator" variables. Add these to your DESeq2 design formula. Do not manually adjust the counts. Instead, include the surrogate variables in your statistical model: R (version 4
April 14, 2026 | Category: Bioinformatics Tools The object svobj$sv contains your new "Sequnator" variables
# Install BiocManager (if you don't have it) if (!require("BiocManager", quietly = TRUE)) install.packages("BiocManager") BiocManager::install("sva") Load the library library(sva)
# In R terminal: BiocManager::install("sva") library(sva) ?sva Now go fix those batch effects. Have a different tool called "Sequnator" in mind? If you meant a specific Windows GUI for sequence alignment, leave a comment below. But 90% of researchers searching this term actually need SVA.