Guidelines for whole genome bisulphite sequencing of intact and FFPET DNA on the Illumina HiSeq X Ten

Shalima S Nair; Phuc-Loi Luu; Wenjia Qu; Madhavi Maddugoda; Lily Huschtscha; Roger Reddel; Georgia Chenevix-Trench; Martina Toso; James G Kench; Lisa G Horvath; Vanessa M Hayes; Phillip D Stricker; Timothy P Hughes; Deborah L White; John E J Rasko; Justin J-L Wong; Susan J Clark

doi:10.1186/s13072-018-0194-0

Guidelines for whole genome bisulphite sequencing of intact and FFPET DNA on the Illumina HiSeq X Ten

Epigenetics Chromatin. 2018 May 28;11(1):24. doi: 10.1186/s13072-018-0194-0.

Authors

Shalima S Nair^{1

2}, Phuc-Loi Luu^{1

2}, Wenjia Qu¹, Madhavi Maddugoda^{1

2}, Lily Huschtscha³, Roger Reddel³, Georgia Chenevix-Trench⁴, Martina Toso⁴, James G Kench^{5

6}, Lisa G Horvath^{6

7

8}, Vanessa M Hayes^{1

2

6}, Phillip D Stricker⁹, Timothy P Hughes^{10

11

12

13}, Deborah L White^{10

11

14

15}, John E J Rasko^{16

17

18}, Justin J-L Wong^{16

17

19}, Susan J Clark^{20

21

22}

Affiliations

¹ Genomics and Epigenetics Division, Garvan Institute of Medical Research, Darlinghurst, NSW, 2010, Australia.
² St Vincent's Clinical School, UNSW, Sydney, NSW, 2010, Australia.
³ Cancer Research Unit, Children's Medical Research Institute, University of Sydney, Westmead, NSW, 2145, Australia.
⁴ QIMR Berghofer, Brisbane, QLD, 4006, Australia.
⁵ Department of Tissue Pathology and Diagnostic Oncology, Royal Prince Alfred Hospital, Camperdown, NSW, Australia.
⁶ Central Clinical School, Sydney Medical School, University of Sydney, Camperdown, NSW, Australia.
⁷ Clinical Prostate Cancer Research, The Kinghorn Cancer Centre, Garvan Institute of Medical Research, Darlinghurst, NSW, Australia.
⁸ Chris O'Brien Lifehouse, Camperdown, NSW, Australia.
⁹ Department of Urology, St. Vincent's Hospital, Darlinghurst, NSW, Australia.
¹⁰ Cancer Theme, South Australian Health and Medical Research Institute, Adelaide, SA, Australia.
¹¹ Australian Leukaemia and Lymphoma Group, Melbourne, Australia.
¹² Discipline of Medicine, University of Adelaide, Adelaide, SA, Australia.
¹³ Department of Haematology, SA Pathology, Adelaide, SA, Australia.
¹⁴ Faculty of Health Science and Faculty of Science, University of Adelaide, Adelaide, SA, Australia.
¹⁵ Australian Genomic Health Alliance, Melbourne, Australia.
¹⁶ Gene and Stem Cell Therapy Program, Centenary Institute, University of Sydney, Camperdown, NSW, 2050, Australia.
¹⁷ Sydney Medical School, University of Sydney, Sydney, NSW, 2006, Australia.
¹⁸ Cell and Molecular Therapies, Royal Prince Alfred Hospital, Camperdown, 2050, Australia.
¹⁹ Gene Regulation in Cancer Laboratory, Centenary Institute, University of Sydney, Camperdown, NSW, 2050, Australia.
²⁰ Genomics and Epigenetics Division, Garvan Institute of Medical Research, Darlinghurst, NSW, 2010, Australia. s.clark@garvan.org.au.
²¹ St Vincent's Clinical School, UNSW, Sydney, NSW, 2010, Australia. s.clark@garvan.org.au.
²² Epigenetics Research Program, The Garvan Institute of Medical Research, 384 Victoria St, Darlinghurst, Sydney, NSW, 2010, Australia. s.clark@garvan.org.au.

Abstract

Background: Comprehensive genome-wide DNA methylation profiling is critical to gain insights into epigenetic reprogramming during development and disease processes. Among the different genome-wide DNA methylation technologies, whole genome bisulphite sequencing (WGBS) is considered the gold standard for assaying genome-wide DNA methylation at single base resolution. However, the high sequencing cost to achieve the optimal depth of coverage limits its application in both basic and clinical research. To achieve 15× coverage of the human methylome, using WGBS, requires approximately three lanes of 100-bp-paired-end Illumina HiSeq 2500 sequencing. It is important, therefore, for advances in sequencing technologies to be developed to enable cost-effective high-coverage sequencing.

Results: In this study, we provide an optimised WGBS methodology, from library preparation to sequencing and data processing, to enable 16-20× genome-wide coverage per single lane of HiSeq X Ten, HCS 3.3.76. To process and analyse the data, we developed a WGBS pipeline (METH10X) that is fast and can call SNPs. We performed WGBS on both high-quality intact DNA and degraded DNA from formalin-fixed paraffin-embedded tissue. First, we compared different library preparation methods on the HiSeq 2500 platform to identify the best method for sequencing on the HiSeq X Ten. Second, we optimised the PhiX and genome spike-ins to achieve higher quality and coverage of WGBS data on the HiSeq X Ten. Third, we performed integrated whole genome sequencing (WGS) and WGBS of the same DNA sample in a single lane of HiSeq X Ten to improve data output. Finally, we compared methylation data from the HiSeq 2500 and HiSeq X Ten and found high concordance (Pearson r > 0.9×).

Conclusions: Together we provide a systematic, efficient and complete approach to perform and analyse WGBS on the HiSeq X Ten. Our protocol allows for large-scale WGBS studies at reasonable processing time and cost on the HiSeq X Ten platform.

Keywords: DNA methylation; Epigenetics; HiSeq X Ten; HiSeq 2500; SNP; Whole genome bisulphite sequencing.

Publication types

Comparative Study
Research Support, Non-U.S. Gov't

MeSH terms

CpG Islands
DNA / analysis*
DNA / chemistry
DNA Methylation*
Epigenomics
Gene Library
Genome, Human
Guidelines as Topic
High-Throughput Nucleotide Sequencing / methods*
Humans
Male
Software
Sulfites / chemistry*
Whole Genome Sequencing / methods*

Substances

Sulfites
DNA
hydrogen sulfite

Abstract

Publication types

MeSH terms

Substances

Grants and funding