Weeks-old C57BL/6J mice. The y axis is truncated from

September 4, 2017

Weeks-old C57BL/6J mice. The y axis is truncated from 2?0 . doi:10.1371/journal.pone.0056955.gGGN Regulates Embryogenesis and Meiotic DSB RepairFigure 3. GGN haploinsufficiency resulted in compromised meiotic DSB repair. (A) qRT-PCR analysis and (B) GGN1 immunoblotting showed a reduction of Ggn transcripts and GGN1 protein in the Ggn+/2 spermatocytes compared to that of Ggn+/+. (C) RAD51 foci in pachytene spermatocytes from the Ggn+/+ (wild-type) and Ggn+/2 (heterozygous knockout) mice. DSBs were visualised with a RAD51 BIBS39 antibody (shown in red), and stage of meiosis was marked with a SYCP3 antibody (shown in green). (D) RAD51 foci count per pachytene cell. RAD51 foci were counted from a total of 50 randomly selected pachytene spermatocytes from each of a total of 7 Ggn+/+ and 7 Ggn+/2 mice. Data are shown as mean 6 S.E.M. doi:10.1371/journal.pone.0056955.gA Potential Role for GGN in DNA Repair during Mitosis in Early Embryonic DevelopmentThe embryonic lethality of the Ggn2/2 embryos is similar to that of mice lacking critical regulators of the DSB repair pathway, RAD51 [28], BRCA1 and BRCA2 [29], and ATR [30]. Several studies have demonstrated that the FA and BRCA pathways corporate DNA MedChemExpress CASIN damage response and repair during mitotic cell division [31]. Mitotic errors in FA patients are common [32?4] and may be a consequence of unresolved DNA damage caused in the preceding S-phase. The FA pathway also plays a direct role in M-phase, where it prevents chromatid breakage resulting from unresolved sites of DNA crosslinking in the previous S-phase [34]. Moreover, it has been shown that double knockdown of BRCCand it binding partner BRCC45 compromised G2/M checkpoint in response to ionizing radiation-induced DNA damage [17]. These findings strongly support the critical role for the FA and BRCA pathways in DNA damage response and cell cycle progression in mitotic cells. The death of the vast majority of Ggn2/2 embryos prior to morulae formation and an absence by the blastocyst stage suggest that only a few rounds of mitotic divisions occurred prior to cell death. These observations raise the possibility that the Ggn2/2 embryos were incapable of repairing DNA breaks that occurred during early mitotic divisions and in turn may lead genome instability and cell death. Further investigations to define role for GGN in mitotic DNA repair during early embryonic development and in response to DNAGGN Regulates Embryogenesis and Meiotic DSB Repairdamaging agents is required to delineate the mechanistic of action GGN plays in DNA repair. In summary, we have shown that GGN is essential for the survival of pre-implantation embryos. The Ggn knockout mouse model described herein is unique and affects a relatively poorly understood aspect of pre-implantation embryo development. Identification of the pathway(s) through which the GGN protein acts should provide a better understanding of the biology of early embryo development. Data also suggests that in the postnatal testis GGN plays a role in DSB repair during meiosis.amplify the 39 region of exons 2 and 59region of exon 3 of the Ggn1 transcript (NM_182694.2). This region is 100 identical to Ggn2 (AF538033.1) and Ggn3 (NM_182696.2) transcripts. To verify haploinsufficiency, spermatocytes were purified from Ggn+/+ and Ggn+/2 adult testes (10 weeks-old) using the Staput method as previously described [37]. qRT-PCR was performed as described above. Data obtained from the Ggn+/+ spermatocytes was set to 100 .Immunoprec.Weeks-old C57BL/6J mice. The y axis is truncated from 2?0 . doi:10.1371/journal.pone.0056955.gGGN Regulates Embryogenesis and Meiotic DSB RepairFigure 3. GGN haploinsufficiency resulted in compromised meiotic DSB repair. (A) qRT-PCR analysis and (B) GGN1 immunoblotting showed a reduction of Ggn transcripts and GGN1 protein in the Ggn+/2 spermatocytes compared to that of Ggn+/+. (C) RAD51 foci in pachytene spermatocytes from the Ggn+/+ (wild-type) and Ggn+/2 (heterozygous knockout) mice. DSBs were visualised with a RAD51 antibody (shown in red), and stage of meiosis was marked with a SYCP3 antibody (shown in green). (D) RAD51 foci count per pachytene cell. RAD51 foci were counted from a total of 50 randomly selected pachytene spermatocytes from each of a total of 7 Ggn+/+ and 7 Ggn+/2 mice. Data are shown as mean 6 S.E.M. doi:10.1371/journal.pone.0056955.gA Potential Role for GGN in DNA Repair during Mitosis in Early Embryonic DevelopmentThe embryonic lethality of the Ggn2/2 embryos is similar to that of mice lacking critical regulators of the DSB repair pathway, RAD51 [28], BRCA1 and BRCA2 [29], and ATR [30]. Several studies have demonstrated that the FA and BRCA pathways corporate DNA damage response and repair during mitotic cell division [31]. Mitotic errors in FA patients are common [32?4] and may be a consequence of unresolved DNA damage caused in the preceding S-phase. The FA pathway also plays a direct role in M-phase, where it prevents chromatid breakage resulting from unresolved sites of DNA crosslinking in the previous S-phase [34]. Moreover, it has been shown that double knockdown of BRCCand it binding partner BRCC45 compromised G2/M checkpoint in response to ionizing radiation-induced DNA damage [17]. These findings strongly support the critical role for the FA and BRCA pathways in DNA damage response and cell cycle progression in mitotic cells. The death of the vast majority of Ggn2/2 embryos prior to morulae formation and an absence by the blastocyst stage suggest that only a few rounds of mitotic divisions occurred prior to cell death. These observations raise the possibility that the Ggn2/2 embryos were incapable of repairing DNA breaks that occurred during early mitotic divisions and in turn may lead genome instability and cell death. Further investigations to define role for GGN in mitotic DNA repair during early embryonic development and in response to DNAGGN Regulates Embryogenesis and Meiotic DSB Repairdamaging agents is required to delineate the mechanistic of action GGN plays in DNA repair. In summary, we have shown that GGN is essential for the survival of pre-implantation embryos. The Ggn knockout mouse model described herein is unique and affects a relatively poorly understood aspect of pre-implantation embryo development. Identification of the pathway(s) through which the GGN protein acts should provide a better understanding of the biology of early embryo development. Data also suggests that in the postnatal testis GGN plays a role in DSB repair during meiosis.amplify the 39 region of exons 2 and 59region of exon 3 of the Ggn1 transcript (NM_182694.2). This region is 100 identical to Ggn2 (AF538033.1) and Ggn3 (NM_182696.2) transcripts. To verify haploinsufficiency, spermatocytes were purified from Ggn+/+ and Ggn+/2 adult testes (10 weeks-old) using the Staput method as previously described [37]. qRT-PCR was performed as described above. Data obtained from the Ggn+/+ spermatocytes was set to 100 .Immunoprec.