4.7 Article

Sequestration to lipid droplets promotes histone availability by preventing turnover of excess histones

Journal

DEVELOPMENT
Volume 148, Issue 15, Pages -

Publisher

COMPANY BIOLOGISTS LTD
DOI: 10.1242/dev.199381

Keywords

Histones; Protein sequestration; Lipid droplets; Drosophila oogenesis; Protein turnover; Proteasome

Funding

  1. National Institutes of Health [RO1 GM102155]
  2. Deutsche Forschungsgemeinschaft [INST 208/760-1FUGG]

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The study reveals how histones H2B, H2A, and H2Av accumulate on lipid droplets in Drosophila embryos and the crucial role of lipid droplets in this process. Lipid droplets in nurse cells facilitate the transport of histones to the oocyte, ensuring the storage of histones for cellular function and development.
Because both dearth and overabundance of histones result in cellular defects, histone synthesis and demand are typically tightly coupled. In Drosophila embryos, histones H2B, H2A and H2Av accumulate on lipid droplets (LDs), which are cytoplasmic fat storage organelles. Without LD binding, maternally provided H2B, H2A and H2Av are absent; however, how LDs ensure histone storage is unclear. Using quantitative imaging, we uncover when during oogenesis these histones accumulate, and which step of accumulation is LD dependent. LDs originate in nurse cells (NCs) and are transported to the oocyte. Although H2Av accumulates on LDs in NCs, the majority of the final H2Av pool is synthesized in oocytes. LDs promote intercellular transport of the histone anchor Jabba and thus its presence in the ooplasm. Ooplasmic Jabba then prevents H2Av degradation, safeguarding the H2Av stockpile. Our findings provide insight into the mechanism for establishing histone stores during Drosophila oogenesis and shed light on the function of LDs as protein-sequestration sites.

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