Embryonic alcohol exposure disrupts the ubiquitin-proteasome system
Olivia Weeks, Bess M. Miller, Brian J. Pepe-Mooney, Isaac M. Oderberg, Scott H. Freeburg, Colton J. Smith, Trista E. North, Wolfram Goessling
Olivia Weeks, Bess M. Miller, Brian J. Pepe-Mooney, Isaac M. Oderberg, Scott H. Freeburg, Colton J. Smith, Trista E. North, Wolfram Goessling
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Embryonic alcohol exposure disrupts the ubiquitin-proteasome system

Abstract

Ethanol (EtOH) is a commonly encountered teratogen that can disrupt organ development and lead to fetal alcohol spectrum disorders (FASDs); many mechanisms of developmental toxicity are unknown. Here, we used transcriptomic analysis in an established zebrafish model of embryonic alcohol exposure (EAE) to identify the ubiquitin-proteasome system (UPS) as a critical target of EtOH during development. Surprisingly, EAE alters 20S, 19S, and 11S proteasome gene expression and increases ubiquitylated protein load. EtOH and its metabolite acetaldehyde decrease proteasomal peptidase activity in a cell type–specific manner. Proteasome 20S subunit β 1 (psmb1hi2939Tg) and proteasome 26S subunit, ATPase 6 (psmc6hi3593Tg), genetic KOs define the developmental impact of decreased proteasome function. Importantly, loss of psmb1 or psmc6 results in widespread developmental abnormalities resembling EAE phenotypes, including growth restriction, abnormal craniofacial structure, neurodevelopmental defects, and failed hepatopancreas maturation. Furthermore, pharmacologic inhibition of chymotrypsin-like proteasome activity potentiates the teratogenic effects of EAE on craniofacial structure, the nervous system, and the endoderm. Our studies identify the proteasome as a target of EtOH exposure and signify that UPS disruptions contribute to craniofacial, neurological, and endodermal phenotypes in FASDs.

Authors

Olivia Weeks, Bess M. Miller, Brian J. Pepe-Mooney, Isaac M. Oderberg, Scott H. Freeburg, Colton J. Smith, Trista E. North, Wolfram Goessling

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Figure 1

RNA-Seq identifies the ubiquitin proteasome system as a target of embryonic alcohol exposure.

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RNA-Seq identifies the ubiquitin proteasome system as a target of embryo...
(A) Schematic of RNA-Seq performed on 7 dpf whole-larval extracts following 0% or 1% EtOH exposure (12 hpf–5 dpf). (B) Heatmap of significantly dysregulated genes (Padj < 0.05; n = 1,603). (C) GOrilla GSEA identifies GO components enriched in the dysregulated gene set. (D) Heatmap of genes involved in proteasome-mediated, ubiquitin-dependent protein catabolism. Following EAE, these genes were significantly upregulated relative to controls. (E) ISH for psmb1 following 0% or 1% EtOH exposure (12–96 hpf). At 96 hpf, psmb1 expression is increased in the liver (black arrow) and intestine (white star). Scale bars: 100 μm. (F) Overview of the protocol for treatment and isolation of GFP+ hepatocytes via FACS sorting at 120 hpf. (G) ef1α-normalized qPCR of proteasome-related genes in GFP+ hepatocytes sorted by FACS (*P ≤ 0.05, **P ≤ 0.01, 2-sided t test; n = 5 per column). Data represent mean ± SEM.