Locus-level L1 DNA methylation profiling reveals the epigenetic and transcriptional interplay between L1s and their integration sites

Sophie Lanciano; Claude Philippe; Arpita Sarkar; David Pratella; Cécilia Domrane; Aurélien J. Doucet; Dominic van Essen; Simona Saccani; Laure Ferry; Pierre Antoine Defossez; Gael Cristofari

doi:10.1016/j.xgen.2024.100498

Locus-level L1 DNA methylation profiling reveals the epigenetic and transcriptional interplay between L1s and their integration sites

Sophie Lanciano
, Claude Philippe
, Arpita Sarkar
, David Pratella
, Cécilia Domrane
, Aurélien J. Doucet
, Dominic van Essen
, Simona Saccani
, Laure Ferry
, Pierre Antoine Defossez
, Gael Cristofari

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

Abstract

Long interspersed element 1 (L1) retrotransposons are implicated in human disease and evolution. Their global activity is repressed by DNA methylation, but deciphering the regulation of individual copies has been challenging. Here, we combine short- and long-read sequencing to unveil L1 methylation heterogeneity across cell types, families, and individual loci and elucidate key principles involved. We find that the youngest primate L1 families are specifically hypomethylated in pluripotent stem cells and the placenta but not in most tumors. Locally, intronic L1 methylation is intimately associated with gene transcription. Conversely, the L1 methylation state can propagate to the proximal region up to 300 bp. This phenomenon is accompanied by the binding of specific transcription factors, which drive the expression of L1 and chimeric transcripts. Finally, L1 hypomethylation alone is typically insufficient to trigger L1 expression due to redundant silencing pathways. Our results illuminate the epigenetic and transcriptional interplay between retrotransposons and their host genome.

Original language	English
Article number	100498
Journal	Cell Genomics
Volume	4
Issue number	2
DOIs	https://doi.org/10.1016/j.xgen.2024.100498
Publication status	Published - 14 Feb 2024
Externally published	Yes

Keywords

5-methyl-cytosine
ESR1
LINE-1
Nanopore
YY1
chromatin
estrogen receptor
nuclear receptor
transposable elements
transposon

UN SDGs

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

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10.1016/j.xgen.2024.100498

Cite this

Lanciano, S., Philippe, C., Sarkar, A., Pratella, D., Domrane, C., Doucet, A. J., van Essen, D., Saccani, S., Ferry, L., Defossez, P. A., & Cristofari, G. (2024). Locus-level L1 DNA methylation profiling reveals the epigenetic and transcriptional interplay between L1s and their integration sites. Cell Genomics, 4(2), Article 100498. https://doi.org/10.1016/j.xgen.2024.100498

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title = "Locus-level L1 DNA methylation profiling reveals the epigenetic and transcriptional interplay between L1s and their integration sites",

abstract = "Long interspersed element 1 (L1) retrotransposons are implicated in human disease and evolution. Their global activity is repressed by DNA methylation, but deciphering the regulation of individual copies has been challenging. Here, we combine short- and long-read sequencing to unveil L1 methylation heterogeneity across cell types, families, and individual loci and elucidate key principles involved. We find that the youngest primate L1 families are specifically hypomethylated in pluripotent stem cells and the placenta but not in most tumors. Locally, intronic L1 methylation is intimately associated with gene transcription. Conversely, the L1 methylation state can propagate to the proximal region up to 300 bp. This phenomenon is accompanied by the binding of specific transcription factors, which drive the expression of L1 and chimeric transcripts. Finally, L1 hypomethylation alone is typically insufficient to trigger L1 expression due to redundant silencing pathways. Our results illuminate the epigenetic and transcriptional interplay between retrotransposons and their host genome.",

keywords = "5-methyl-cytosine, ESR1, LINE-1, Nanopore, YY1, chromatin, estrogen receptor, nuclear receptor, transposable elements, transposon",

author = "Sophie Lanciano and Claude Philippe and Arpita Sarkar and David Pratella and C{\'e}cilia Domrane and Doucet, \{Aur{\'e}lien J.\} and \{van Essen\}, Dominic and Simona Saccani and Laure Ferry and Defossez, \{Pierre Antoine\} and Gael Cristofari",

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year = "2024",

month = feb,

day = "14",

doi = "10.1016/j.xgen.2024.100498",

language = "English",

volume = "4",

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T1 - Locus-level L1 DNA methylation profiling reveals the epigenetic and transcriptional interplay between L1s and their integration sites

AU - Lanciano, Sophie

AU - Philippe, Claude

AU - Sarkar, Arpita

AU - Pratella, David

AU - Domrane, Cécilia

AU - Doucet, Aurélien J.

AU - van Essen, Dominic

AU - Saccani, Simona

AU - Ferry, Laure

AU - Defossez, Pierre Antoine

AU - Cristofari, Gael

PY - 2024/2/14

Y1 - 2024/2/14

N2 - Long interspersed element 1 (L1) retrotransposons are implicated in human disease and evolution. Their global activity is repressed by DNA methylation, but deciphering the regulation of individual copies has been challenging. Here, we combine short- and long-read sequencing to unveil L1 methylation heterogeneity across cell types, families, and individual loci and elucidate key principles involved. We find that the youngest primate L1 families are specifically hypomethylated in pluripotent stem cells and the placenta but not in most tumors. Locally, intronic L1 methylation is intimately associated with gene transcription. Conversely, the L1 methylation state can propagate to the proximal region up to 300 bp. This phenomenon is accompanied by the binding of specific transcription factors, which drive the expression of L1 and chimeric transcripts. Finally, L1 hypomethylation alone is typically insufficient to trigger L1 expression due to redundant silencing pathways. Our results illuminate the epigenetic and transcriptional interplay between retrotransposons and their host genome.

AB - Long interspersed element 1 (L1) retrotransposons are implicated in human disease and evolution. Their global activity is repressed by DNA methylation, but deciphering the regulation of individual copies has been challenging. Here, we combine short- and long-read sequencing to unveil L1 methylation heterogeneity across cell types, families, and individual loci and elucidate key principles involved. We find that the youngest primate L1 families are specifically hypomethylated in pluripotent stem cells and the placenta but not in most tumors. Locally, intronic L1 methylation is intimately associated with gene transcription. Conversely, the L1 methylation state can propagate to the proximal region up to 300 bp. This phenomenon is accompanied by the binding of specific transcription factors, which drive the expression of L1 and chimeric transcripts. Finally, L1 hypomethylation alone is typically insufficient to trigger L1 expression due to redundant silencing pathways. Our results illuminate the epigenetic and transcriptional interplay between retrotransposons and their host genome.

KW - 5-methyl-cytosine

KW - ESR1

KW - LINE-1

KW - Nanopore

KW - YY1

KW - chromatin

KW - estrogen receptor

KW - nuclear receptor

KW - transposable elements

KW - transposon

U2 - 10.1016/j.xgen.2024.100498

DO - 10.1016/j.xgen.2024.100498

M3 - Article

AN - SCOPUS:85185345026

SN - 2666-979X

VL - 4

JO - Cell Genomics

JF - Cell Genomics

IS - 2

M1 - 100498

ER -

Locus-level L1 DNA methylation profiling reveals the epigenetic and transcriptional interplay between L1s and their integration sites

Abstract

Keywords

UN SDGs

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