Hello all,
I need to ask two questions. I am new to this area. I have my epic array data from 4 different cells with 2 replicates. I have to use Minfi package. I have loaded my idat data into the environment. I checked tens of workflows and all of them contained sample sheet. There is no sample sheet for my data. Should I create it somehow or should I start analyzing without the sample sheet? If I should create, how can I do it? And the second question is how will I handle with the replicates? I will continue with bump hunter and Limma for differential methylation. At what point the replicates should be merged, if they should be merged? Thanks in advance
> RGset
class: RGChannelSet
dim: 1105209 8
metadata(0):
assays(2): Green Red
rownames(1105209): 1600157 1600179 ... 99810982 99810990
rowData names(0):
colnames(8): 207716530101_R01C01 207716530101_R02C01 ... 207716530101_R07C01
207716530101_R08C01
colData names(14): X Date ... Basename filenames
Annotation
array: IlluminaHumanMethylationEPIC
annotation: ilm10b4.hg19
Thank you so much for the clarification. As you said the replicates are the cells from different plates. For instance, both R01C01 and R05C01 are SUP-B15 cell line grown in different plates, and R02C01 and R06C01 are from resistant cell line derived from SUP-B15. I want to use preprocessFunnorm for normalization, and then I want to find differentially methylated regions between the resistant and the sensitive cell lines using bumphunter. And then, I want to use Limma. How am I supposed to design the matrix?
You can use
model.matrix
to generate the design matrix. See examples in the 'limma User's Guide' or the vignette for theDMRcate
package.Thanks a lot for the help. You saved my day