Question

Removal of ERCC spike-in in RNA-Seq

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6.5 years ago

anu014 ▴ 190

Hello Biostars!

Can anyone tell me if is it necessary to remove spike-in sequences before aligning FASTQs to reference FASTA OR is it necessary to consider spike-in while normalizing in DEseq2 ? And if yes, how to handle spike-in in RNA-Seq? Can STAR or DEseq handle it somehow?

Please suggest me. Thank you :)

RNA-Seq Assembly alignment • 3.1k views

ADD COMMENT • link updated 10 months ago by Daniel ▴ 30 • written 6.5 years ago by anu014 ▴ 190

score 1 · Answer 1 · 2018-05-17

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6.5 years ago

Devon Ryan 104k

Presuming you mean ERCC spike-ins the best practice is to include them in the reference genome. However in practice not doing so has little if any effect, so we rarely bother. Unless you have a use-case that absolutely requires spike-ins, it's best to simply ignore them (i.e., do not use them in any way in your analysis).

ADD COMMENT • link 6.5 years ago by Devon Ryan 104k

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Hi @Devon . What if the data is single cell RNA-seq?

ADD REPLY • link 6.5 years ago by anu014 ▴ 190

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scRNA-seq can sometimes benefit from spike-ins. Just align to them and use them for computing scaling factors.

ADD REPLY • link 6.5 years ago by Devon Ryan 104k

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If I am not mistaken this answer is now outdated? It seems that more and more people are starting to only trust in data which has spike-in normalization, for all types of rna-seq.

ADD REPLY • link 10 months ago by Daniel ▴ 30