Author:
He Wen-Xia,Wu Min,Liu Zhen,Li Zhi,Wang Yang,Zhou Jian,Yu Peng,Zhang Xiao-Juan,Zhou Li,Gui Jian-Fang
Abstract
Stem–loop binding protein (SLBP) is required for replication-dependent histone mRNA metabolism in mammals. Zebrafish possesses two slbps, and slbp1 is necessary for retinal neurogenesis. However, the detailed expression and function of slbp2 in zebrafish are still unknown. In this study, we first identified zebrafish slbp2 as an oocyte-specific maternal factor and then generated a maternal-zygotic slbp2 F3 homozygous mutant (MZslbp2Δ4−/−) using CRISPR/Cas9. The depletion of maternal Slbp2 disrupted early nuclear cleavage, which resulted in developmental arrest at the MBT stage. The developmental defects could be rescued in slbp2 transgenic MZslbp2Δ4−/− embryos. However, homozygous mutant MZslbp1Δ1−/− developed normally, indicating slbp1 is dispensable for zebrafish early embryogenesis. Through comparative proteome and transcriptome profiling between WT and MZslbp2Δ4−/− embryos, we identified many differentially expressed proteins and genes. In comparison with those in WT embryos, four replication-dependent histones, including H2a, H2b, H3, and H4, all reduced their expression, while histone variant h2afx significantly increased in MZslbp2Δ4−/− embryos at the 256-cell stage and high stage. Zebrafish Slbp2 can bind histone mRNA stem–loop in vitro, and the defects of MZslbp2Δ4−/− embryos can be partially rescued by overexpression of H2b. The current data indicate that maternal Slbp2 plays a pivotal role in the storage of replication-dependent histone mRNAs and proteins during zebrafish oogenesis.
Funder
Key Program of Frontier Sciences of the Chinese Academy of Sciences
Strategic Priority Research Program of the Chinese Academy of Sciences
Earmarked Fund for Modern Agro-industry Technology Research System
Autonomous Project of the State Key Laboratory of Freshwater Ecology and Biotechnology
Publisher
Cold Spring Harbor Laboratory
Cited by
16 articles.
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