DNA Methylation Analysis – Olympia Oyster Whole Genome BSseq Bismark Pipeline Comparison

Ran Bismark using our high performance computing (HPC) node, Mox, with two different bowtie2 settings:

  1. Default settings

  2. –score_min L,0,-0.6

The second setting is a bit less stringent than the default settings and should result in a higher percentage of reads mapping. However, not entirely sure what the actual implications will be (if any) for interpreting the resulting data.

Input data was previously trimmed per Bismark’s recommendation for Illumina TruSeq libraries (TrimGalore! 5′ 10bp):

List of input files and Bismark configurations can be seen in the SLURM scripts:

RESULTS

Output folders:

3 comments

  1. Pingback: Transcriptome Alignment & Bedgraph – Olympia oyster transcriptome with Olurida_v080 genome assembly | Sam's Notebook
  2. Pingback: Sam’s Notebook: DNA Methylation Analysis – Olympia Oyster Whole Genome BSseq Bismark Pipeline MethylKit Comparison | Roberts Lab
  3. Pingback: DNA Methylation Analysis – Olympia Oyster Whole Genome BSseq Bismark Pipeline MethylKit Comparison | Sam's Notebook

Leave a Reply

Your email address will not be published. Required fields are marked *


e.g. 0000-0002-7299-680X

You may use these HTML tags and attributes: <a href="" title=""> <abbr title=""> <acronym title=""> <b> <blockquote cite=""> <cite> <code> <del datetime=""> <em> <i> <q cite=""> <strike> <strong>