Defective germline reprogramming rewires the spermatogonial transcriptome.
Lina VasiliauskaitėRebecca V BerrensIvayla IvanovaClaudia CarrieriWolf ReikAnton J EnrightDònal O' CarrollPublished in: Nature structural & molecular biology (2018)
Defective germline reprogramming in Piwil4 (Miwi2)- and Dnmt3l-deficient mice results in the failure to reestablish transposon silencing, meiotic arrest and progressive loss of spermatogonia. Here we sought to understand the molecular basis for this spermatogonial dysfunction. Through a combination of imaging, conditional genetics and transcriptome analysis, we demonstrate that germ cell elimination in the respective mutants arises as a result of defective de novo genome methylation during reprogramming rather than because of a function for the respective factors within spermatogonia. In both Miwi2-/- and Dnmt3l-/- spermatogonia, the intracisternal-A particle (IAP) family of endogenous retroviruses is derepressed, but, in contrast to meiotic cells, DNA damage is not observed. Instead, we find that unmethylated IAP promoters rewire the spermatogonial transcriptome by driving expression of neighboring genes. Finally, spermatogonial numbers, proliferation and differentiation are altered in Miwi2-/- and Dnmt3l-/- mice. In summary, defective reprogramming deregulates the spermatogonial transcriptome and may underlie spermatogonial dysfunction.
Keyphrases
- genome wide
- dna methylation
- dna damage
- oxidative stress
- gene expression
- rna seq
- dna repair
- single cell
- germ cell
- induced apoptosis
- multiple sclerosis
- poor prognosis
- magnetic resonance
- high resolution
- signaling pathway
- type diabetes
- metabolic syndrome
- endoplasmic reticulum stress
- cell cycle arrest
- high fat diet induced
- transcription factor
- binding protein
- photodynamic therapy