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course-card Image adapted from https://doi.org/10.3389/fgene.2011.00106

University of Hawaiʻi at Mānoa WGBS Module


Contents

Overview

This module will show you how to run a whole genome bisulfite sequencing (WGBS) data analysis workflow on Google Cloud Platform (GCP). In addition to the overview given in this README you will find four Jupyter notebooks that help you understand the basics of the workflow to running large dataset using Google Batch in the cloud. To use this module, clone the parent repository, git clone https://github.com/NIGMS/DNA-Methylation-Sequencing-Analysis-with-WGBS.git and then navigate to the directory for this project. You will then see the following notebooks in your environment:

  • Introduction of DNA methylation (tutorial_0-introduction.pdf): more background of DNA methylation and WGBS data analysis.

  • Notebook 1 (tutorial_1-bismark.ipynb): using the Bismark workflow to extract the methylation percentage at each position from the raw FASTQ sequences. This tutorial will use a small example to walk through the process step by step. (Running time: ~50 mins)

  • Notebook 2 (tutorial_2-metilene.ipynb): using metilene to identify differential methylated regions (DMRs) from the methylation profiles generated from Notebook 1. This workflow requests at least two samples. (Running time: < 3 mins)

  • Notebook 3 (tutorial_3-methylseq1.ipynb): run the existing workflow methylseq developed by nf-core. This workflow is built using Nextflow, and is highly automated and portable.
    (Running time: ~50 mins)

  • Notebook 4 (tutorial_4-methylseq2.ipynb): run the nf-core/methylseq workflow using Google Batch, which enables the workflows to use highly scalable and compliant infrastructure in the Google Cloud Platform. (Running time: ~3 hrs)

This whole module will only cost you about $2.00 to run, assuming you tear down all resources upon completion.

Watch this Introduction Video to learn more about the module.

workflow diagram

Background

As one of the most abundant and well-studied epigenetic modifications, DNA methylation plays an essential role in normal cell development and has various effects on transcription, genome stability, and DNA packaging within cells.

  • DNA Methylation refers to the addition of a methyl (CH3) group to the 5th carbon on a cytosine ring giving rise to 5-methylcytosine (5mC). The whole process is mediated by DNA methyltransferases (DNMTs): dna methylation
  • DNA methylation primarily happens at CpG sites, where a cytosine is followed by a guanine in the 5’-3’ direction (5’-Cytosine-phosphate-Guanine-3’). And DNA regions have a high frequency of CpG sites are called CpG island. Methylation can also occur at CHG and CHH sites, where "H" is A, C, or T.
  • Function. DNA methylation effects on transcriptional regulation differ depending on the location of the CpG site (intragenic vs. promoter region vs enhancer). For example, there are extensive differences in DNA methylation patterning between normal and cancer cells across the entire genome. And this change in distribution collectively causes a suppression of tumor suppressor genes and concomitant increase in the expression of oncogenes, which drive tumorigenesis (Skvortsova K, et al. 2019).

To measure DNA methylation, WGBS was developed with the next-generation sequencing technologies (NGS) and bisulfited-based technologies. The basic steps of WGBS include DNA extraction, bisulfite conversion, library preparation, sequencing, and bioinformatics analysis.

  • A bisulfite treatment converts cytosines into uracils, but leaves methylated cytosines unchanged: bisulfite treatment
  • Subsequently, methylation can be measured at single base pair resolution by quantifying the C-C positions reference-bisulfite treatment (methylated site) versus the positions that changed C-T reference-bisulfite treatment (unmethylated site).
  • In this learning module, our focus is to process and analyze the sequencing data generated from WGBS experiments. The major steps include quality control, alignment, methylation calling and differentially methylated region detection. We'll introduce two workflows and show how to run them on GCP, with detailed explanation how each step works in these workflows.

Before Starting

These tutorials were designed to be used on Google Cloud Platforms (GCP), with the aim of requiring nothing but the files within this GitHub repository. However, you do need to set up your Google account to access GCP and the Vertex AI Workbench to use the notebooks. The steps you need before getting started:

  • Set up a Google Cloud account
  • Create a project
  • Enable billing
  • Enable APIs (Compute Engine API, Cloud Storage API, Google Batch)
  • Create a Nextflow service account (only needed for tutorial 4)
  • Create a Cloud Storage bucket (details)

More detailed instructions of the above steps can be found here. Or you can also refer to NIH Cloud Lab README for more instructions.

Getting Started

This repository contains several notebook files which serve as bioinformatics WGBS workflow tutorials. To view these notebooks on GCP, the following steps will guide you through setting up a virtual machine on Google Cloud Platform, downloading our tutorial files, and running those files.

Optional: Creating a Nextflow Service Account

If you are using Nextflow outside of NIH CloudLab you must set up a service account and add your service account to your notebook permissions before creating the notebook. Follow section 2 of the accompanying How To document for instructions. If you are executing this tutorial with an NIH CloudLab account your default Compute Engine service account will have all required IAM roles to run the nextflow portion.

Creating a user managed notebook

Follow the steps highlighted here to create a new user-managed notebook in Vertex AI. Follow steps 1-8 and be especially careful to enable idle shutdown as highlighted in step 7. For this module you should select Debian 11 and Python 3 in the Environment tab in step 5. In step 6 in the Machine type tab, select n1-standard-4 from the dropdown box.

Download the tutorials

To clone this repository, use the Git command git clone https://github.com/NIGMS/MethylSeqUH.git in the dropdown menu option in Jupyter notebook. Please make sure you only enter the link for the repository that you want to clone. There are other bioinformatics related learning modules available in the NIGMS Repository.

This should download our repository, and the tutorial files inside, into a folder called MethylSeqUH. Double-click this folder now. Inside you will find all our tutorial files, which you can double-click and run.

Running Tutorial Files

All our tutorial workflows are in Jupyter notebook format. To run these notebooks (.ipynb) you need only to double-click the tutorial files and this will open the Jupyter file in Jupyter notebook. From here you can run each section, or 'cell', of the code, one by one, by pushing the 'Play' button on the above menu.

Some 'cells' of code take longer for the computer to process than others. You will know a cell is running when a cell has an asterisk next to it [*]. When the cell finishes running, that asterisk will be replaced with a number which represents the order that cell was run in.

You can now explore the tutorials by running the code in each, from top to bottom. Look at the Overview section for a short description of each tutorial.

Stopping Your Virtual Machine

When you are finished running code, you can turn off your virtual machine to prevent unneeded billing or resource use by checking your notebook and clicking the Stop button.

Software Requirements

In this module, you will need access to a Jupyter notebook in GCP Vertex AI environment. The environment settings are listed here:

  • Environment : Python 3 (with Intel® MKL)
  • Environment version :M97
  • IPython :7.33.0
  • ipykernel :6.16.0
  • jupyter_client :7.3.5
  • jupyter_core :4.11.1
  • jupyter_server :1.19.1
  • jupyterlab :3.4.7
  • nbclient :0.6.8
  • nbconvert :7.0.0
  • nbformat :5.6.1
  • notebook :6.4.12
  • traitlets :5.4.0

For Notebook 1 and 2, you can install all necessary requirements using the instructions in Notebook 1, and the detailed software versions used in this tutorial (Oct, 2022) are listed here:

  • conda 22.9.0 (pre-installed)
  • mamba 0.27.0
  • bedtools v2.30.0
  • FastQC v0.11.9
  • Bismark v0.23.1
  • samtools 1.15.1
  • htslib 1.16
  • trim_galore 0.6.7
  • Cutadapt 4.1
  • metilene 0.2-8
  • MultiQC v1.13
  • Python 3.7.12

For Notebook 3 and 4, you will need to install Java and Nextflow in your notebook. Other software listed are included in the nfcore/methylseq pipeline, installation is not required, since they will be downloaded along with the pipeline.

  • openjdk 17.0.3-internal
  • Nextflow v22.04.5
  • nf-core/methylseq v1.6.1
  • Bismark genomePrep v0.23.0
  • FastQC v0.11.9
  • Cutadapt v3.4
  • Trim Galore! v0.6.6
  • Bismark v0.23.0
  • Bismark Deduplication v0.23.0
  • Bismark methXtract v0.23.0
  • Bismark Report v0.23.0
  • Bismark Summary v0.22.4
  • Samtools v1.11
  • BWA v0.7.17-r1188
  • bwa-meth v0.2.2
  • Picard MarkDuplicates v1.6.1
  • MethylDackel v0.5.2 (using HTSlib version 1.11)
  • Qualimap v2.2.2-dev
  • Preseq v2.0.3
  • MultiQC v1.10.1
  • HISAT2 v2.2.1

Architecture Design

technical infrastructure diagram

Data

Example dataset 1: used in Notebook 1,2 and 3, was created by the snakePipes WGBS pipeline from paper: Habibi, Ehsan, et al. Cell stem cell 13.3 (2013): 360-369. There were four samples in this example dataset, two kinase inhibitors (2i) enables derivation of mouse embryonic stem cells (ESCs) vs. conventional ESCs maintained in serum. To streamline the tutorials the dataset were down sampled to only keep the reads from mouse genome chr6:4000000-6000000 and was stored in a Google Cloud Storage Bucket. Accordingly, the reference genome (.fasta file) from mouse GRCm39 chromosome 6 can be downloaded from NCBI or Ensemble websites, and was also stored in the same bucket.

Example dataset 2: used in Notebook 4. It was originally downloaded from the SRA database using the accession numbers SRR306435 and SRR033942. The data was from Molaro, Antoine, et al. Cell 146.6 (2011): 1029-1041 and Laurent, Louise, et al. " Genome research 20.3 (2010): 320-331. The studies profiled the methylomes of human and chimp sperm as a basis for comparison to methylation patterns of embryonic stem cells (ESCs). We use one sample from human sperm and one sample from ESCs as examples to demonstrate how to download these published datasets from SRA and process them using nf-core/methylseq in the Google Life Sciences API.

Funding

Funded by NIH/NIGMS P20GM103466.

License for Data

Text and materials are licensed under a Creative Commons CC-BY-NC-SA license. The license allows you to copy, remix and redistribute any of our publicly available materials, under the condition that you attribute the work (details in the license) and do not make profits from it. More information is available here.

Creative commons license

This work is licensed under a Creative Commons Attribution-NonCommercial-ShareAlike 4.0 International License

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