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6.8 years ago
Shaurya Jauhari
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50
In context to the aforementioned statement, is that to say that my analysis is egregious hitherto.
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In cuffdiff significant value (yes or no) defined by q_value cut off. Do you have replicates ? if you don't have replicates there is no meaning of p or q value.
You mean it would therefore be pointless to analyze data using this pipeline if I don't have replicates, or will the data not be very reliable? And if the data cannot be analyzed without replicates, would it be OK for me to use the different fastq files (paired-end reads) as replicates, as both the fragments would map to the same reference genome (I understand that not all paired-end reads will have fragments mapping to the same gene)?
Hi,
I am not telling that it is pointless to use cuffdiff if you don't have replicates. If you don't have replicates there is no meaning of p value or q value. Read this to know more about p value and how to calculate it for diff expressed genes. You have to be more stringent to get your differentially expressed genes if you don't have replicates. (for e.g fold change >= 2 , minimum fpkm/rpkm 10 or some arbitrary cutoff on number of reads mapped to particular gene.)
Replicates are there to check if biology can be reproduced or not. By using r1 and r2 as replicates (which are not replicates in any sense) you are not checking biology but something else (which I don't know)
You need to provide details such as command you used, and things you tried so far.