| Literature DB >> 30595536 |
Weimin Zhang1, Xuedi Zhang2, Zhaoyu Xue2, Yijie Li3, Qing Ma3, Xiangle Ren2, Jiaying Zhang2, Songhua Yang2, Lijuan Yang2, Menghua Wu2, Mengda Ren2, Rongwen Xi4, Zheng Wu5, Ji-Long Liu5, Erika Matunis3, Junbiao Dai6, Guanjun Gao7.
Abstract
Replication-dependent histone genes often reside in tandemly arrayed gene clusters, hindering systematic loss-of-function analyses. Here, we used CRISPR/Cas9 and the attP/attB double-integration system to alter numbers and sequences of histone genes in their original genomic context in Drosophila melanogaster. As few as 8 copies of the histone gene unit supported embryo development and adult viability, whereas flies with 20 copies were indistinguishable from wild-types. By hierarchical assembly, 40 alanine-substitution mutations (covering all known modified residues in histones H3 and H4) were introduced and characterized. Mutations at multiple residues compromised viability, fertility, and DNA-damage responses. In particular, H4K16 was necessary for expression of male X-linked genes, male viability, and maintenance of ovarian germline stem cells, whereas H3K27 was essential for late embryogenesis. Simplified mosaic analysis showed that H3R26 is required for H3K27 trimethylation. We have developed a powerful strategy and valuable reagents to systematically probe histone functions in D. melanogaster.Entities:
Keywords: CRISPR/Cas9; Drosophila; FLP-FRT; H4K16; attB-attP; dosage effects; histone mutant library; mosaic system
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Year: 2018 PMID: 30595536 PMCID: PMC6595499 DOI: 10.1016/j.devcel.2018.11.047
Source DB: PubMed Journal: Dev Cell ISSN: 1534-5807 Impact factor: 12.270