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Filtering bisulfite fastq files #63
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Hi Alex, That is a huge amount of memory and I'm surprised it isn't working. I don't remember FastQ Screen making core.#### files either. Perhaps they are generated by Bowtie2 or Bismark. What is the file size of this pilot dataset? Does FastQ Screen work without using the --tag command? That command would be: fastq_screen --conf fastq_screen.conf --bisulfite --outdir tagged_data $datapath/*.gz Best, |
Hi Steven, Thanks so much for your quick reply! The dataset I'm working with is 542GB, there are 88 files and each file is between 4-10 GB. FastQ-Screen works fine without --tag - the job finished successfully in under 15 hours and only needed 15GB memory. In contrast when I include tag I am using 150GB memory and it takes 168 hours to process just over 50% of the data. I've noticed with some more tests that these core files were produced for a job where I had requested less memory and the job was near the limit of the requested memory (99.75%) but not for another job where I requested more memory and memory usage was lower (97.42%). I'm running this in snakemake so I can easily see which files were incomplete when the job timed out on the HPC, but have also tried running this outside snakemake in a batch job. I will keep digging but let me know if you have any suggestions. How many cores/threads would you usually suggest for a dataset my size? Also, just to double check - I'm trying to filter out the controls (puc19 and lambda) from my sheep reads. In my conf file I only have the sheep, puc19 and lambda databases as I assumed I would later be filtering out reads from the tagged file that match puc19 or lambda but not sheep. Am I assuming correctly or do I not need to include the sheep database in my conf file and only puc19 and lambda? Just thought I would check as perhaps this would help speed it up a bit. Thanks a lot, |
Hi Alex, It's hard for me to assess what is causing this. FastQ Screen silently tags every read as part of normal processing, so I'm not sure why this is causing a problem. Just a simple suggestion - have your tried processing the files sequentially rather than parallelising (say, just use 8 threads). Maybe the parallelisation is not working as expected for some reason. Yes, you could try tagging with puc19 and lambda. That is all you need to remove reads. I hope that helps. All the best, |
Hello,
I'm trying to run FastQ-Screen on bisulfite data on sheep. I've managed to run FastQ-Screen successfully before as a QC check on the data (on 80GB memory), but am having trouble with memory now (currently trying 150GB memory) that I am trying to create a tag file to filter out controls (puc19 and lambda) which were spiked in with my samples to test for bisulfite conversion efficiency. I am running this on a HPC and have noticed that a number of 'core.#####' files are created in the directory which seems to be ~23GB each and I wonder if this is related to the problem. I never noticed these files before when running fastq-screen without --tag (or on any other jobs on the HPC) - are these files created by FastQ-Screen and are they needed? If you have any advice on how to reduce the memory needed for the job that would be really appreciated - I am currently only working on a pilot dataset and will be working with a much larger dataset in the future.
The code I'm using is:
fastq_screen --tag --conf fastq_screen.conf --bisulfite --outdir tagged_data $datapath/*.gz
Thanks so much in advance,
Alex
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