LINE-1 retrotransposon activation intrinsic to interneuron development

Author:

Bodea Gabriela O.,Ferreiro Maria E.,Sanchez-Luque Francisco J.,Botto Juan M.,Rasmussen Jay,Rahman Muhammed A.,Fenlon Laura R.,Gubert Carolina,Gerdes Patricia,Bodea Liviu-Gabriel,Ajjikuttira Prabha,Kozulin Peter,Billon Victor,Morell Santiago,Kempen Marie-Jeanne H.C.,Love Chloe J.,Palmer Lucy M.,Ewing Adam D.,Jhaveri Dhanisha J.,Richardson Sandra R.,Hannan Anthony J.,Faulkner Geoffrey J.ORCID

Abstract

Transposable elements (TEs) are a reservoir of new transcription factor binding sites for protein-coding genes1–3. Developmental programs that activate TE-derived regulatory elements could, in principle, manifest in lineage-specific TE mobility. While somatic LINE-1 (L1) retrotransposon insertions have been detected in human neurons4–6, the impact of L1 insertions on neurodevelopmental gene regulation, and whether L1 mobility is restricted to certain neuronal lineages, is unknown. Here, we reveal programmed L1 activation by SOX6, a transcription factor critical for parvalbumin (PV+) interneuron development7–9. PV+ neurons harbor unmethylated and euchromatic L1 promoters, express L1 mRNA, and permit L1 transgene mobilization in vivo. Elevated L1 expression in adult dentate gyrus PV+ neurons is however attenuated by environmental enrichment. Nanopore sequencing of PV+ neurons identifies unmethylated L1 loci providing alternative promoters to core PV+ neuron genes, such as CAPS2. These data depict SOX6-mediated L1 activation as an ingrained component of the mammalian PV+ neuron developmental program.

Publisher

Cold Spring Harbor Laboratory

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