Long-read sequencing across the C9orf72 'GGGGCC' repeat expansion: Implications for clinical use and genetic discovery efforts in human disease

Mark T.W. Ebbert; Stefan L. Farrugia; Jonathon P. Sens; Karen Jansen-West; Tania F. Gendron; Mercedes Prudencio; Ian J. McLaughlin; Brett Bowman; Matthew Seetin; Mariely Dejesus-Hernandez; Jazmyne Jackson; Patricia H. Brown; Dennis W. Dickson; Marka Van Blitterswijk; Rosa Rademakers; Leonard Petrucelli; John D. Fryer

doi:10.1186/s13024-018-0274-4

Long-read sequencing across the C9orf72 'GGGGCC' repeat expansion: Implications for clinical use and genetic discovery efforts in human disease

Mark T.W. Ebbert
, Stefan L. Farrugia
, Jonathon P. Sens
, Karen Jansen-West
, Tania F. Gendron
, Mercedes Prudencio
, Ian J. McLaughlin
, Brett Bowman
, Matthew Seetin
, Mariely Dejesus-Hernandez
, Jazmyne Jackson
, Patricia H. Brown
, Dennis W. Dickson
, Marka Van Blitterswijk
, Rosa Rademakers
, Leonard Petrucelli
, John D. Fryer

Research output: Contribution to journal › Article › peer-review

99 Scopus citations

Abstract

Background: Many neurodegenerative diseases are caused by nucleotide repeat expansions, but most expansions, like the C9orf72 'GGGGCC' (G₄C₂) repeat that causes approximately 5-7% of all amyotrophic lateral sclerosis (ALS) and frontotemporal dementia (FTD) cases, are too long to sequence using short-read sequencing technologies. It is unclear whether long-read sequencing technologies can traverse these long, challenging repeat expansions. Here, we demonstrate that two long-read sequencing technologies, Pacific Biosciences' (PacBio) and Oxford Nanopore Technologies' (ONT), can sequence through disease-causing repeats cloned into plasmids, including the FTD/ALS-causing G₄C₂ repeat expansion. We also report the first long-read sequencing data characterizing the C9orf72 G₄C₂ repeat expansion at the nucleotide level in two symptomatic expansion carriers using PacBio whole-genome sequencing and a no-amplification (No-Amp) targeted approach based on CRISPR/Cas9. Results: Both the PacBio and ONT platforms successfully sequenced through the repeat expansions in plasmids. Throughput on the MinION was a challenge for whole-genome sequencing; we were unable to attain reads covering the human C9orf72 repeat expansion using 15 flow cells. We obtained 8× coverage across the C9orf72 locus using the PacBio Sequel, accurately reporting the unexpanded allele at eight repeats, and reading through the entire expansion with 1324 repeats (7941 nucleotides). Using the No-Amp targeted approach, we attained > 800× coverage and were able to identify the unexpanded allele, closely estimate expansion size, and assess nucleotide content in a single experiment. We estimate the individual's repeat region was > 99% G₄C₂ content, though we cannot rule out small interruptions. Conclusions: Our findings indicate that long-read sequencing is well suited to characterizing known repeat expansions, and for discovering new disease-causing, disease-modifying, or risk-modifying repeat expansions that have gone undetected with conventional short-read sequencing. The PacBio No-Amp targeted approach may have future potential in clinical and genetic counseling environments. Larger and deeper long-read sequencing studies in C9orf72 expansion carriers will be important to determine heterogeneity and whether the repeats are interrupted by non-G₄C₂ content, potentially mitigating or modifying disease course or age of onset, as interruptions are known to do in other repeat-expansion disorders. These results have broad implications across all diseases where the genetic etiology remains unclear.

Original language	English
Article number	46
Journal	Molecular Neurodegeneration
Volume	13
Issue number	1
DOIs	https://doi.org/10.1186/s13024-018-0274-4
State	Published - Aug 21 2018

Bibliographical note

Publisher Copyright:
© 2018 The Author(s).

Funding

This work was supported by the PhRMA Foundation [RSGTMT17 to M.E.]; the Ed and Ethel Moore Alzheimer’s Disease Research Program of Florida Department of Health [8AZ10 to M.E. and 6AZ06 to J.F.]; the National Institutes of Health [NS094137 to J.F., AG047327 to J.F, AG049992 to J.F., R21NS099631 to M.v.B., R35NS097261 to R.R., R35NS097273 to L.P., R21NS084528 to L.P., P01NS084974 to L.P., P01NS099114 to L.P., R01NS088689 to L.P., R01NS093865 to L.P.]; Department of Defense [ALSRP AL130125 to L.P.]; Mayo Clinic Foundation (L.P. and J.F.); Mayo Clinic Center for Individualized Medicine (L.P. and J.F.); Amyotrophic Lateral Sclerosis Association (M.E., M.P., M.V.B., L.P.); Robert Packard Center for ALS Research at Johns Hopkins (M.V.B., L.P.) Target ALS (L.P.); Association for Frontotemporal Degeneration (L.P.); GHR Foundation (J.F.); and the Mayo Clinic Gerstner Family Career Development Award (J.F.).

Funders	Funder number
Ed and Ethel Moore Alzheimer’s Disease Research Program of Florida Department of Health	6AZ06, 8AZ10
GHR Foundation
National Institutes of Health (NIH)	R21NS099631, R01NS093865, P01NS099114, R01NS088689, NS094137, R21NS084528, R35NS097261, P01NS084974, R35NS097273, AG047327
U.S. Department of Defense	ALSRP AL130125
National Institute on Aging	R03AG049992
Mayo Clinic Rochester
Hennepin Faculty Associates Amyotrophic Lateral Sclerosis Association Certified ALS Center
Pharmaceutical Research and Manufacturers of America Foundation	RSGTMT17
Association for Frontotemporal Degeneration
Robert Packard Center for ALS Research, Johns Hopkins University

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

SDG 3 Good Health and Well-being

Keywords

Amyotrophic lateral sclerosis (ALS)
C9orf72
Frontotemporal dementia (FTD)
GGGGCC
Genetics
Long-read sequencing
Oxford Nanopore Technologies MinION
PacBio RS II and Sequel
Repeat expansion disorders
Structural mutations

ASJC Scopus subject areas

Molecular Biology
Clinical Neurology
Cellular and Molecular Neuroscience

Access to Document

10.1186/s13024-018-0274-4

Cite this

Ebbert, M. T. W., Farrugia, S. L., Sens, J. P., Jansen-West, K., Gendron, T. F., Prudencio, M., McLaughlin, I. J., Bowman, B., Seetin, M., Dejesus-Hernandez, M., Jackson, J., Brown, P. H., Dickson, D. W., Van Blitterswijk, M., Rademakers, R., Petrucelli, L., & Fryer, J. D. (2018). Long-read sequencing across the C9orf72 'GGGGCC' repeat expansion: Implications for clinical use and genetic discovery efforts in human disease. Molecular Neurodegeneration, 13(1), Article 46. https://doi.org/10.1186/s13024-018-0274-4

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title = "Long-read sequencing across the C9orf72 'GGGGCC' repeat expansion: Implications for clinical use and genetic discovery efforts in human disease",

abstract = "Background: Many neurodegenerative diseases are caused by nucleotide repeat expansions, but most expansions, like the C9orf72 'GGGGCC' (G4C2) repeat that causes approximately 5-7\% of all amyotrophic lateral sclerosis (ALS) and frontotemporal dementia (FTD) cases, are too long to sequence using short-read sequencing technologies. It is unclear whether long-read sequencing technologies can traverse these long, challenging repeat expansions. Here, we demonstrate that two long-read sequencing technologies, Pacific Biosciences' (PacBio) and Oxford Nanopore Technologies' (ONT), can sequence through disease-causing repeats cloned into plasmids, including the FTD/ALS-causing G4C2 repeat expansion. We also report the first long-read sequencing data characterizing the C9orf72 G4C2 repeat expansion at the nucleotide level in two symptomatic expansion carriers using PacBio whole-genome sequencing and a no-amplification (No-Amp) targeted approach based on CRISPR/Cas9. Results: Both the PacBio and ONT platforms successfully sequenced through the repeat expansions in plasmids. Throughput on the MinION was a challenge for whole-genome sequencing; we were unable to attain reads covering the human C9orf72 repeat expansion using 15 flow cells. We obtained 8× coverage across the C9orf72 locus using the PacBio Sequel, accurately reporting the unexpanded allele at eight repeats, and reading through the entire expansion with 1324 repeats (7941 nucleotides). Using the No-Amp targeted approach, we attained > 800× coverage and were able to identify the unexpanded allele, closely estimate expansion size, and assess nucleotide content in a single experiment. We estimate the individual's repeat region was > 99\% G4C2 content, though we cannot rule out small interruptions. Conclusions: Our findings indicate that long-read sequencing is well suited to characterizing known repeat expansions, and for discovering new disease-causing, disease-modifying, or risk-modifying repeat expansions that have gone undetected with conventional short-read sequencing. The PacBio No-Amp targeted approach may have future potential in clinical and genetic counseling environments. Larger and deeper long-read sequencing studies in C9orf72 expansion carriers will be important to determine heterogeneity and whether the repeats are interrupted by non-G4C2 content, potentially mitigating or modifying disease course or age of onset, as interruptions are known to do in other repeat-expansion disorders. These results have broad implications across all diseases where the genetic etiology remains unclear.",

keywords = "Amyotrophic lateral sclerosis (ALS), C9orf72, Frontotemporal dementia (FTD), GGGGCC, Genetics, Long-read sequencing, Oxford Nanopore Technologies MinION, PacBio RS II and Sequel, Repeat expansion disorders, Structural mutations",

author = "Ebbert, \{Mark T.W.\} and Farrugia, \{Stefan L.\} and Sens, \{Jonathon P.\} and Karen Jansen-West and Gendron, \{Tania F.\} and Mercedes Prudencio and McLaughlin, \{Ian J.\} and Brett Bowman and Matthew Seetin and Mariely Dejesus-Hernandez and Jazmyne Jackson and Brown, \{Patricia H.\} and Dickson, \{Dennis W.\} and \{Van Blitterswijk\}, Marka and Rosa Rademakers and Leonard Petrucelli and Fryer, \{John D.\}",

note = "Publisher Copyright: {\textcopyright} 2018 The Author(s).",

year = "2018",

month = aug,

day = "21",

doi = "10.1186/s13024-018-0274-4",

language = "English",

volume = "13",

number = "1",

}

Ebbert, MTW, Farrugia, SL, Sens, JP, Jansen-West, K, Gendron, TF, Prudencio, M, McLaughlin, IJ, Bowman, B, Seetin, M, Dejesus-Hernandez, M, Jackson, J, Brown, PH, Dickson, DW, Van Blitterswijk, M, Rademakers, R, Petrucelli, L & Fryer, JD 2018, 'Long-read sequencing across the C9orf72 'GGGGCC' repeat expansion: Implications for clinical use and genetic discovery efforts in human disease', Molecular Neurodegeneration, vol. 13, no. 1, 46. https://doi.org/10.1186/s13024-018-0274-4

TY - JOUR

T1 - Long-read sequencing across the C9orf72 'GGGGCC' repeat expansion

T2 - Implications for clinical use and genetic discovery efforts in human disease

AU - Ebbert, Mark T.W.

AU - Farrugia, Stefan L.

AU - Sens, Jonathon P.

AU - Jansen-West, Karen

AU - Gendron, Tania F.

AU - Prudencio, Mercedes

AU - McLaughlin, Ian J.

AU - Bowman, Brett

AU - Seetin, Matthew

AU - Dejesus-Hernandez, Mariely

AU - Jackson, Jazmyne

AU - Brown, Patricia H.

AU - Dickson, Dennis W.

AU - Van Blitterswijk, Marka

AU - Rademakers, Rosa

AU - Petrucelli, Leonard

AU - Fryer, John D.

PY - 2018/8/21

Y1 - 2018/8/21

N2 - Background: Many neurodegenerative diseases are caused by nucleotide repeat expansions, but most expansions, like the C9orf72 'GGGGCC' (G4C2) repeat that causes approximately 5-7% of all amyotrophic lateral sclerosis (ALS) and frontotemporal dementia (FTD) cases, are too long to sequence using short-read sequencing technologies. It is unclear whether long-read sequencing technologies can traverse these long, challenging repeat expansions. Here, we demonstrate that two long-read sequencing technologies, Pacific Biosciences' (PacBio) and Oxford Nanopore Technologies' (ONT), can sequence through disease-causing repeats cloned into plasmids, including the FTD/ALS-causing G4C2 repeat expansion. We also report the first long-read sequencing data characterizing the C9orf72 G4C2 repeat expansion at the nucleotide level in two symptomatic expansion carriers using PacBio whole-genome sequencing and a no-amplification (No-Amp) targeted approach based on CRISPR/Cas9. Results: Both the PacBio and ONT platforms successfully sequenced through the repeat expansions in plasmids. Throughput on the MinION was a challenge for whole-genome sequencing; we were unable to attain reads covering the human C9orf72 repeat expansion using 15 flow cells. We obtained 8× coverage across the C9orf72 locus using the PacBio Sequel, accurately reporting the unexpanded allele at eight repeats, and reading through the entire expansion with 1324 repeats (7941 nucleotides). Using the No-Amp targeted approach, we attained > 800× coverage and were able to identify the unexpanded allele, closely estimate expansion size, and assess nucleotide content in a single experiment. We estimate the individual's repeat region was > 99% G4C2 content, though we cannot rule out small interruptions. Conclusions: Our findings indicate that long-read sequencing is well suited to characterizing known repeat expansions, and for discovering new disease-causing, disease-modifying, or risk-modifying repeat expansions that have gone undetected with conventional short-read sequencing. The PacBio No-Amp targeted approach may have future potential in clinical and genetic counseling environments. Larger and deeper long-read sequencing studies in C9orf72 expansion carriers will be important to determine heterogeneity and whether the repeats are interrupted by non-G4C2 content, potentially mitigating or modifying disease course or age of onset, as interruptions are known to do in other repeat-expansion disorders. These results have broad implications across all diseases where the genetic etiology remains unclear.

AB - Background: Many neurodegenerative diseases are caused by nucleotide repeat expansions, but most expansions, like the C9orf72 'GGGGCC' (G4C2) repeat that causes approximately 5-7% of all amyotrophic lateral sclerosis (ALS) and frontotemporal dementia (FTD) cases, are too long to sequence using short-read sequencing technologies. It is unclear whether long-read sequencing technologies can traverse these long, challenging repeat expansions. Here, we demonstrate that two long-read sequencing technologies, Pacific Biosciences' (PacBio) and Oxford Nanopore Technologies' (ONT), can sequence through disease-causing repeats cloned into plasmids, including the FTD/ALS-causing G4C2 repeat expansion. We also report the first long-read sequencing data characterizing the C9orf72 G4C2 repeat expansion at the nucleotide level in two symptomatic expansion carriers using PacBio whole-genome sequencing and a no-amplification (No-Amp) targeted approach based on CRISPR/Cas9. Results: Both the PacBio and ONT platforms successfully sequenced through the repeat expansions in plasmids. Throughput on the MinION was a challenge for whole-genome sequencing; we were unable to attain reads covering the human C9orf72 repeat expansion using 15 flow cells. We obtained 8× coverage across the C9orf72 locus using the PacBio Sequel, accurately reporting the unexpanded allele at eight repeats, and reading through the entire expansion with 1324 repeats (7941 nucleotides). Using the No-Amp targeted approach, we attained > 800× coverage and were able to identify the unexpanded allele, closely estimate expansion size, and assess nucleotide content in a single experiment. We estimate the individual's repeat region was > 99% G4C2 content, though we cannot rule out small interruptions. Conclusions: Our findings indicate that long-read sequencing is well suited to characterizing known repeat expansions, and for discovering new disease-causing, disease-modifying, or risk-modifying repeat expansions that have gone undetected with conventional short-read sequencing. The PacBio No-Amp targeted approach may have future potential in clinical and genetic counseling environments. Larger and deeper long-read sequencing studies in C9orf72 expansion carriers will be important to determine heterogeneity and whether the repeats are interrupted by non-G4C2 content, potentially mitigating or modifying disease course or age of onset, as interruptions are known to do in other repeat-expansion disorders. These results have broad implications across all diseases where the genetic etiology remains unclear.

KW - Amyotrophic lateral sclerosis (ALS)

KW - C9orf72

KW - Frontotemporal dementia (FTD)

KW - GGGGCC

KW - Genetics

KW - Long-read sequencing

KW - Oxford Nanopore Technologies MinION

KW - PacBio RS II and Sequel

KW - Repeat expansion disorders

KW - Structural mutations

UR - https://www.scopus.com/pages/publications/85052156507

UR - https://www.scopus.com/pages/publications/85052156507#tab=citedBy

U2 - 10.1186/s13024-018-0274-4

DO - 10.1186/s13024-018-0274-4

M3 - Article

C2 - 30126445

AN - SCOPUS:85052156507

SN - 1750-1326

VL - 13

JO - Molecular Neurodegeneration

JF - Molecular Neurodegeneration

IS - 1

M1 - 46

ER -

Long-read sequencing across the C9orf72 'GGGGCC' repeat expansion: Implications for clinical use and genetic discovery efforts in human disease

Abstract

Bibliographical note

Funding

UN SDGs

Keywords

ASJC Scopus subject areas

Access to Document

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