Method development for DNA methylation on a single cell level...comparison between these two cell...
Transcript of Method development for DNA methylation on a single cell level...comparison between these two cell...
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Method development for DNA methylation on a single cell level
The project is carried out in TATAA Biocenter, Gothenburg, Sweden/ Secondment at Babraham institute , Cambridge
Dr. Bentolhoda Fereydouni, Marie curie Postdoctoral research fellow
Presented in final Epitrain meeting , University College London, 16th January 2017
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Outline
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- Introduction
- Aims of the study
- Reduced representation bisulfite sequencing (RRBS)
- Bismark software and data analysis
- Summary & Discussion
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What is Epigenetics?
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From The Cell Biology of Stem Cells (2010)
1) histone modification
2) DNA methylation
- Is the study of heritable changes in gene expression (on or off the genes) that does not involve changes to the underlying DNA sequence
- A change in phenotype without a change in genotype
Introduction
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Epigenetic inheritance as a form of Lamarckism
Lamarckism (or Lamarckian inheritance) is the idea that an organism can pass on characteristics that it has acquired during its lifetime to its offspring .
Lamarckism has continued as studies in the field of epigenetics have highlighted the possible inheritance of behavioral traits acquired by the previous generation.
(1744–1829)
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Effects of environmental factors
Epigenetic marks play important roles in defining different cell types in the body and can be influenced by environmental and nutritional factors.
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DNA Methylation
Cytosine 5-methyl Cytosine
DNA methyl-transferases
DNA-demethylase(s)?TETs?
Passive demethylation?
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- symmetric CG context
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Silencing of gene expressionTissue differentiation and embryonic development
Faults in correct DNA methylation may result in- early development failure- epigenetic syndromes- cancer
Regulation by DNA methylation
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DNA methylation is reset during reprogramming
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http://www.cell.com/cms/attachment/2002984389/2011335745/gr1.jpg
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Hypermethylation of CpGs leads to cancer
http://www.ks.uiuc.edu/Research/methylation/normal_cancer_cell.png
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Measuring DNA methylation by Bisulfite-sequencing
Image by Illumina
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Unmethylated cytosine produce uracil in DNA
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- Establish a method to evaluate methylation profiles in singlecell material
- Gel-free RRBS protocol and try to reduce the number ofpurification steps
- Using computational and statistical method for detecting andanalyzing covered CpG sites at the single cell level
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Aims of the Study
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Reduced representation bisulfite sequencing (RRBS)
- is an efficient and high-throughput technique used to analyze the genome-wide methylation profiles on a single nucleotide level.
- This technique combines restriction enzymes and bisulfite sequencing in orderto enrich for the areas of the genome that have a high CpG content.
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Five steps in the standard RRBS method
1- Genomic DNA purification
2- Restriction enzyme digestion -cuts at CCGG sites. This enriches for CpG rich regions of the genome
3- End repair and dA tailing
4- Adapter ligation
5- Bisulfite conversion
All the five steps into a single-tube reaction
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Artificial methylation calls in RRBS libraries
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C genomic cytosineC unmethylated cytosine
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The final RRBS libraries were prepared with fragment analyzer and the concentration and size distribution were checked with Pico green/ Nanodrop.
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The Fragment Analyzer results of two RRBS libraries
Typical DNA size distribution in RRBS libraries ranges from 150 to
350 bp with visible peaks corresponding to MspI fragments
33 pg hgDNA 6.6 pg hgDNA
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The Fragment Analyzer results of two human tomour RRBS libraries
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The Fragment Analyzer results of two human Oocyte RRBS libraries
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BS-Seq Analysis Workflow
SequencingProcessing
pipeline
Methylation
Analysis
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Explore and
understand
data
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Illumina platforms
HiSeq 2500 2000Mreads/run400 Gb/run 2x1002x125 bp
Miseq15-22Mreads/run4,5-13,2 Gb/run2x300
NextSeq500400 Mreads/run120 Gb/run 2x1502x150
Production power Flexible power Focused power
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BS-Seq Analysis Workflow
QC Trimming Mapping
Methylation
extractionMapped QCAnalysis
23Taken from Babraham institute bioinformatics home page
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Data analysis for RRBS dataBioinformatic analysis methods for DNA methylation profiling data with bioinformatic tools Bismark program adapter trimming with Trim Galore.
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What is Bismark?
- Is a set of tools for the time-efficient analysis of Bisulfite-Seq (BS-Seq) data.
- Performs alignments of bisulfite-treated reads to a reference genome and cytosine methylation calls at the same time.
- is written in Perl and is run from the command line.
- Bisulfite-treated reads are mapped using the short read aligner Bowtie .
- Bowtie (http://bowtie-bio.sourceforge.net/index.shtml) or Bowtie 2 http://bowtie-bio.sourceforge.net/bowtie2 needs to be installed on computer.
Taken from Babraham institute bioinformatics home page
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Reference genomeFirst reference genome downloaded and place it in a genome folder.
Genomes can be obtained from the Ensembl(http://www.ensembl.org/info/data/ftp/index.html/) orNCBI website (ftp://ftp.ncbi.nih.gov/genomes/)
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Bismark workflow
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Quality Control shows : - Number of sequences
- Basecall qualities
- Base composition
- Potential contaminants
- Expected duplication rate
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www.bioinformatics.babraham.ac.uk/projects/fastqc/
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QC: Base Composition
OocytesTumour cells
-Typical BSSeq experiments in mammals tend to have an average cytosine content of ~1-2%throughout the entire sequence length
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Duplication rate(RRBS has high duplication rate)
Oocytes Tumour cells
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Removing adapter contamination
before trimming after trimming
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Summary Adapter/Quality Trimming
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Important to trim because failure to do so might result in:
Low mapping efficiency
Mis-alignments
Errors in methylation calls since adapters are methylated
Basecall errors tend toward 50% (C:mC)
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Methylation bias
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good opportunity to look at conversion efficiency
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Bismark run report- Summary of alignment parameters used.
- Number of sequences analyzed.
- Number of sequences with a unique best alignment (mapping efficiency).
- Statistics summarizing the bisulfite strand the unique best alignments came from.
- Number of cytosines analyzed.
- Number of methylated and unmethylated cytosines.
- Percentage methylation of cytosines in CpG, CHG or CHH context
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Summary& Discussion
-The advantage of the scRRBS method is, its applicability to subnanogram levelsof DNA as starting material, down to a single cell.
- Particularly useful when the starting materials are very limited and precious, such as mammalian early embryos and primordial germ cells.
- Enables the heterogeneity of DNA methylomes among individual cells to bestudied, which may have important roles in biological processes such as celldifferentiation, memory formation and oncogenesis.
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- Since RRBS is highly sensitive, this technique can be used to quickly look at aberrant methylation in cancer
- If samples from the patient's tumor and normal cells can be obtained, acomparison between these two cell types can be observed
- A profile of the overall methylation can be produced quite rapidly
- This technique can rapidly determine the overall methylation status of cancergenomes which is cost and time effective
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Seminars and Presentations 1. B. Fereydouni “Method development for DNA methylation on a single cell level” presented in EpiTrain Final meeting. University College London, London, UK, 16th January 2017.
2. B. Fereydouni, E.Hanson, A. Ståhlberg A and R. Sjöback “Gel-free reduced representation bisulfite sequencing for single cell DNA methylation profiling” The Biology of Genomes meeting,10 – 14 May 2016, Cold Spring Harbor Laboratory, New York, USA, Poster presentation.
3. B. Fereydouni “Method development for DNA methylation on a single cell level” presented in EpiTrain annual meeting. Epigenomics of Common Diseases conference and EpiTrain annual meeting, Wellcome Genome Campus, Hinxton, Cambridge, UK 6-9 November 2015.
4. B. Fereydouni “Find and establish a method to evaluate methylation profiles in single cell material?” Novel technologies in Epigenetics, Technology transfer and Entrepreneurship, EpiTrain annual meeting, IDIBELL, L’Hospitalet de Llobregat, Barcelona, Spain 15-16 October 2015.
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Courses - Multiplex PCR, 11th December 2015, TATAA Biocenter. Gothenburg, Sweden.
- Sample preparation and quality control, 10th December 2015, TATAA Biocenter. Gothenburg, Sweden.
- 2- Day NGS – Library construction and quality control, 26- 27th November 2015, TATAA Biocenter. Gothenburg, Sweden.
- Methods and applications for microRNA analysis, 9th October 2015, TATAA Biocenter. Gothenburg, Sweden.
Genotyping with qPCR, 8th October 2015, TATAA Biocenter. Gothenburg, Sweden.
- 2- Day Digital PCR- Application and analysis, 10-11th September 2015. TATAA Biocenter. Gothenburg, Sweden.
- 3- Day Hands-on qPCR, 7-9th September 2015. TATAA Biocenter, Gothenburg, Sweden
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Thank you
Dr. Ellen Hanson
Dr. Robert Sjöback
Dr. Gavin Kelsey
Dr. Felix Krueger
All my colleagues at TATAA biocenter
Professor Ståhlberg
Dr. Kirsten Ward
Professor Mikael Kubista
Professor Stephan Beck