Input: Raw or QC'ed methylation data?

[Jannobold]

Hey guys,
thank you for this fantastic implementation of PC-based epigenetic clocks.

I wonder if I should use raw methylation data (just "beta <- rawmet / (rawmet+rawume+100)") or QC'ed data (e.g. filter out CpGs aligning to SNPs or to multiple locations in the genome)?

Best wishes
Jan