Question

Current standards for batch correction and gene expression correction?

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5.1 years ago

rshoobs ▴ 10

I am interested in running batch effect correction on my gene expression data and am looking into what the current standards are. Previously I used PEER to correct for batch effects but it is almost a decade old and does not seem to be supported on R 3.5. What are people currently using for batch effect correction?

RNA-Seq • 1.6k views

ADD COMMENT • link updated 5.1 years ago by GouthamAtla 12k • written 5.1 years ago by rshoobs ▴ 10

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RNAseq or Array?

Is it known which samples belong to which batches?

ADD REPLY • link 5.1 years ago by i.sudbery 20k

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RNASeq and the batches are not known

ADD REPLY • link 5.1 years ago by rshoobs ▴ 10

score 3 · Answer 1 · 2019-10-29

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5.1 years ago

i.sudbery 20k

If its RNAseq - if the batch/sample mapping is known, we include it in the design for differential expression, or if not doing differential expression, we either apply limma::voom or DESeq2::rLog and then use limma::removeBatchEffects().

ADD COMMENT • link 5.1 years ago by i.sudbery 20k

score 2 · Answer 2 · 2019-10-29

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5.1 years ago

swbarnes2 14k

Depends what you are doing. For differential gene expression, you can just include batch in the design, and that's enough. For other applications, you might try ComBat or RUVSeq

ADD COMMENT • link 5.1 years ago by swbarnes2 14k

score 2 · Answer 3 · 2019-10-29

If you don't know batches, may be RUVSeq helps but it depends on non-differential gene expression to estimate surrogate variables. PCA regression performs well. Its included not in sva package as sva_network function. Plot the PCs and see how many PCs to regress out. sva also has function to estimate the no. of PCs to regress out (num.sv) but from my experience it often overestimates number of PCs.