Does anyone know if RPKM normalization and quantile normalization of RNA-seq read counts can or should be combined?
For normalization of paired-end reads in RNA-seq, is it accurate to normalize the raw read counts using the quantile method, then following that calculate the RPKM value for each transcript using the quantile normalized values?
It seems that RPKM normalization using the total millions of mapped reads is somewhat redundant with an initial quantile normalization of read counts. Are these two methods mutually exclusive or should they be combined? Any recommendations?
thanks!
For normalization of paired-end reads in RNA-seq, is it accurate to normalize the raw read counts using the quantile method, then following that calculate the RPKM value for each transcript using the quantile normalized values?
It seems that RPKM normalization using the total millions of mapped reads is somewhat redundant with an initial quantile normalization of read counts. Are these two methods mutually exclusive or should they be combined? Any recommendations?
thanks!
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