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Hi,
I am looking into analyzing differential alternative splicing after a treatment. I have 2 conditions (control and treatment) and 4 biological replicates on each. I have on average 75 million pairs of 100bp per sample.
I am trying to use MATS do do this. I seem to have MATS working as per the test run. Although I could use my fastq files, I already have my reads mapped and wanted to use bam files, which were not generated by tophat and it is not working. Anyone knows what can be causing the problem? what does MATS expect from the bam fields?
Also, since I have to rent nodes form a cluster, what is the RAM required for MATS to do the analysis in mammalian size genomes with this number of replicates (my fastq files are ~17GB each, my bam files are ~9GB). For how long should I expect them to run?
thanks
Lucia
I am looking into analyzing differential alternative splicing after a treatment. I have 2 conditions (control and treatment) and 4 biological replicates on each. I have on average 75 million pairs of 100bp per sample.
I am trying to use MATS do do this. I seem to have MATS working as per the test run. Although I could use my fastq files, I already have my reads mapped and wanted to use bam files, which were not generated by tophat and it is not working. Anyone knows what can be causing the problem? what does MATS expect from the bam fields?
Also, since I have to rent nodes form a cluster, what is the RAM required for MATS to do the analysis in mammalian size genomes with this number of replicates (my fastq files are ~17GB each, my bam files are ~9GB). For how long should I expect them to run?
thanks
Lucia
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