Altered germline cyst and oocyte differentiation inTex14mutant mice reveal a new mechanism underlying female reproductive life-span

AbstractIn adult mammalian females, primordial follicles that form in the fetal/neonatal ovary are the only source to sustain adult ovarian function. Our previous studies revealed that during oocyte differentiation and primordial follicle formation in mouse fetal ovaries, primary oocytes form via gaining cytoplasm and organelles from sister germ cells that are connected to them by intercellular bridges within germline cysts. To better understand the role of intercellular bridges in oocyte differentiation, we analyzed mutant females lackingtestis-expressed 14 (Tex14), a gene involved in cytokinesis and bridge formation. InTex14-/-fetal ovaries, germ cells divide to form a reduced number of cysts in which sister germ cells are still connected via syncytia or fragmented cell membranes, rather than normal intercellular bridges. Compared with wildtype cysts,Tex14-/-cysts fragment at a higher frequency and produce a greatly reduced number of primary oocytes with highly precocious cytoplasmic enrichment and enlarged volume. By contrast,Tex14+/-germline cysts are less fragmented and generate primary oocytes that are smaller than wild type. Interestingly, enlargedTex14-/-primary oocytes are much more stable than wild type oocytes and more efficiently sustain folliculogenesis, whereas undersizedTex14+/-primary oocytes turn over at an accelerated rate. Our observations directly link the nature of fetal germ cell connectivity to cytoplasmic enrichment during oocyte differentiation and to oocyte developmental potential in the adult ovary. Our results imply that the duration of adult ovarian function is strongly influenced by the number of primary oocytes acquiring highly enriched cytoplasm during oocyte differentiation in fetal ovaries, rather than just by the size of the primordial follicle pool.