Enhanced Preprints

Post-fertilization transcription initiation in an ancestral LTR retrotransposon drives lineage-specific genomic imprinting of ZDBF2

  1. Hisato Kobayashi author has email address
  2. Tatsushi Igaki
  3. Soichiro Kumamoto
  4. Keisuke Tanaka
  5. Tomoya Takashima
  6. Shunsuke Suzuki
  7. Masaaki Hayashi
  8. Marilyn B. Renfree
  9. Manabu Kawahara
  10. Shun Saito
  11. Toshihiro Kobayashi
  12. Hiroshi Nagashima
  13. Hitomi Matsunari
  14. Kazuaki Nakano
  15. Ayuko Uchikura
  16. Hiroshi Kiyonari
  17. Mari Kaneko
  18. Hiroo Imai
  19. Kazuhiko Nakabayashi
  20. Matthew C. Lorincz
  21. Kazuki Kurimoto
  1. Department of Embryology, Nara Medical University, Kashihara, Nara 634-0813, Japan
  2. Department of Chemistry and Biochemistry, School of Advanced Science and Engineering, Waseda University, Shinjuku, Tokyo 169-8555, Japan
  3. Division of Cancer and Senescence Biology, Cancer Research Institute, Institute for Frontier Science Initiative, Kanazawa University, Kanazawa, Ishikawa 920-1192, Japan
  4. Department of Informatics, Tokyo University of Information Sciences, Wakaba, Chiba 265-8501, Japan
  5. NODAI Genome Research Center, Tokyo University of Agriculture, Setagaya, Tokyo 156-8502, Japan
  6. Department of Agriculture, Graduate School of Science and Technology, Shinshu University, Nagano 399-4598, Japan
  7. School of BioSciences, University of Melbourne, Melbourne, Victoria 3010, Australia
  8. Laboratory of Animal Genetics and Reproduction, Research Faculty of Agriculture, Hokkaido University, Sapporo, Hokkaido 060-8589, Japan
  9. Division of Mammalian Embryology, Center for Stem Cell Biology and Regenerative Medicine, The Institute of Medical Science, University of Tokyo, Minato, Tokyo 108-8639, Japan
  10. Center for Genetic Analysis of Behavior, National Institute for Physiological Sciences, Okazaki, Aichi 444-8787, Japan
  11. Meiji University International Institute for Bio-Resource Research, Kawasaki 214-8571, Japan
  12. Laboratory for Animal Resources and Genetic Engineering, RIKEN Center for Biosystems Dynamics Research, Kobe, Hyogo 650-0047, Japan
  13. Molecular Biology Section, Center for the Evolutionary Origins of Human Behavior, Kyoto University, Inuyama, Aichi 484-8506 Japan
  14. Division of Developmental Genomics, Research Institute, National Center for Child Health and Development, Setagaya, Tokyo 157-8535, Japan
  15. Life Sciences Institute, Department of Medical Genetics, University of British Columbia, Vancouver, British Columbia V6T 1Z3, Canada

Peer review process

Not revised: This Reviewed Preprint includes the authors’ original preprint (without revision), an eLife assessment, and public reviews.

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Editors

  • Reviewing Editor
    Thomas Gingeras
    Cold Spring Harbor Laboratory, Cold Spring Harbor, United States of America
  • Senior Editor
    Claude Desplan
    New York University, New York, United States of America

Reviewer #1 (Public Review):

Summary:
The study tests the conservation of imprinting of the ZBDF2 locus across mammals. ZDBF2 is known to be imprinted in mice, humans, and rats. The locus has a unique mechanism of imprinting: although imprinting is conferred by a germline DMR methylated in oocytes, the DMR is upstream to ZDBF2 (at GPR1) and monoallelic methylation of the gDMR does not persist beyond early developmental stages. Instead, a lncRNA (GPR1-AS, also known as Liz in mouse) initiating at the gDMR is expressed transiently in embryos and sets up a secondary DMR (by mechanisms not fully elucidated) that then confers monoallelic expression of ZDBF2 in somatic tissues.

In this study, the authors first interrogate existing placental RNA-seq datasets from multiple mammalian species, and detect GPR1-AS1 candidate transcripts in humans, baboons, macaques and mice, but not in about a dozen other mammals. Because of the varying depth, quality, and nature of these RNA-seq libraries, the ability to definitely detect the GPR1-AS1 lncRNA is not guaranteed; therefore, they generate their own deep, directional RNA-seq data from tissues/embryos from five species, finding evidence of GPR1-AS in rabbits and chimpanzees, but not bovine animals, pigs or opossums. From these surveys, the authors conclude that the lncRNA is present only in Euarchontoglires mammals. To test the association between GPR1-AS and ZDBF2 imprinting, they perform RT-PCR and sequencing in tissue from wallabies and cattle, finding biallelic expression of ZDBF2 in these species that also lack a detected GPR1-AS transcript. From inspection of the genomic location of the GPR1-AS first exon, the authors identify an overlap with a solo LTR of the MER21C retrotransposon family in those species in which the lncRNA is observed, except for some rodents, including mice. However, they do detect a degree of homology (46%) to the MER21C consensus at the first exon on Liz in mouse. Finally, the authors explore public RNA-seq datasets to show that GPR1-AS is expression transiently during human preimplantation development, an expression dynamic that would be consistent with the induction of monoallelic methylation of a somatic DMR at ZDBF2 and consequent monoallelic expression.

Strengths:
-The analysis uncovers a novel mechanism by which a retrotransposon-derived LTR may be involved in genomic imprinting.
-The genomic analysis is very well executed.
-New directional and deeply-sequenced RNA-seq datasets from the placenta or the trophectoderm of five mammalian species and marsupial embryos, that will be of value to the community.

Weaknesses:
Although the genomic analysis is very strong, the study remains entirely correlative. All of the data are descriptive, and much of the analysis is performed on RNA-seq and other datasets from the public domain; a small amount of primary data is generated by the authors.
Evidence that the residual LTR in mouse is functionally relevant for Liz lncRNA expression is lacking.

Reviewer #2 (Public Review):

Summary:
This work concerns the evolution of ZDBF2 imprinting in mammalian species via initiation of GPR1 antisense (AS) transcription from a lineage-specific long-terminal repeat (LTR) retrotransposon. It extends previous work describing the mechanism of ZDBF2 imprinting in mice and humans by demonstrating conservation of GPR1-AS transcripts in rabbits and non-human primates. By identifying the origin of GPR1-AS transcription as the LTR MER21C, the authors claim to account for how imprinting evolved in these species but not in those lacking the MER21C insertion. This illustrates the principle of LTR co-option as a means of evolving new gene regulatory mechanisms, specifically to achieve parent-of-origin allele specific expression (i.e., imprinting). Examples of this phenomenon have been described previously, but usually involve initiation of transcription during gametogenesis rather than post-fertilization, as in this work. The findings of this paper are therefore relevant to biologists studying imprinted genes or interested more generally in the evolution of gene regulatory mechanisms.

Strengths:
(1) The authors convincingly demonstrate the existence of GPR1-AS orthologs in specific mammalian lineages using deeply sequenced, stranded, and paired-end RNA-seq libraries collected from diverse mammalian species.

Weaknesses:
(1) The authors do not directly demonstrate imprinting of the ZDBF2 locus in rabbits and non-human primates, which would greatly strengthen their model linking ZDBF2 imprinting to transcription from MER21C.

(2) Experimental evidence linking GPR1-AS transcription to ZDBF2 imprinting in rabbits and non-human primates is currently lacking. Consideration should be given to the challenges associated with studying non-model species and manipulating repeat sequences, which may explain the absence of experimental evidence in this case. Further, this mechanism is established in humans and mice, so the authors' model is arguably sufficiently supported merely by the existence of GPR1-AS orthologs in other mammalian lineages.

Reviewer #3 (Public Review):

Summary:
Kobayashi et al identify MER21C as a common promoter of GPR1-AS/Liz in Euarchontoglires, which establishes a somatic DMR that controls ZFDB2 imprinting. In mice, MER21C appears to have diverged significantly from its primate counterparts and is no longer annotated as such.

Strengths:
The authors used high-quality cross-species RNA-seq data to characterise GPR1-AS-like transcripts, which included generating new data in five different species. The association between MER21C/B elements and the promoter of GPR1-AS in most species is clear and convincing. The expression pattern of MER21C/B elements overall further supports their role in enabling correct temporal expression of GPR1-AS during embryonic development.

Weaknesses:
A deeper comparison of syntenic regions to the GPR1-AS promoter could be performed to provide a clearer picture of how the MER21C/B element evolved. The use of alternative TE annotation software may also be helpful. These analyses would be particularly useful to drive home the conclusion that the mouse (Liz) promoter is derived from the same insertion.

  1. Howard Hughes Medical Institute
  2. Wellcome Trust
  3. Max-Planck-Gesellschaft
  4. Knut and Alice Wallenberg Foundation