| Literature DB >> 34599906 |
Benjamin C Stark1, Yuanyuan Gao2, Diane S Sepich3, Lakyn Belk2, Matthew A Culver2, Bo Hu2, Marlene Mekel1, Wyndham Ferris3, Jimann Shin3, Lilianna Solnica-Krezel4, Fang Lin5, John A Cooper6.
Abstract
Cell migration is important during early animal embryogenesis. Cell migration and cell shape are controlled by actin assembly and dynamics, which depend on capping proteins, including the barbed-end heterodimeric actin capping protein (CP). CP activity can be regulated by capping-protein-interacting (CPI) motif proteins, including CARMIL (capping protein Arp2/3 myosin-I linker) family proteins. Previous studies of CARMIL3, one of the three highly conserved CARMIL genes in vertebrates, have largely been limited to cells in culture. Towards understanding CARMIL function during embryogenesis in vivo, we analyzed zebrafish lines carrying mutations of carmil3. Maternal-zygotic mutants showed impaired endodermal migration during gastrulation, along with defects in dorsal forerunner cell (DFC) cluster formation, which affected the morphogenesis of Kupffer's vesicle (KV). Mutant KVs were smaller, contained fewer cells and displayed decreased numbers of cilia, leading to defects in left/right (L/R) patterning with variable penetrance and expressivity. The penetrance and expressivity of the KV phenotype in carmil3 mutants correlated well with the L/R heart positioning defect at the end of embryogenesis. This in vivo animal study of CARMIL3 reveals its new role during morphogenesis of the vertebrate embryo. This role involves migration of endodermal cells and DFCs, along with subsequent morphogenesis of the KV and L/R asymmetry.Entities:
Keywords: Actin; Capping protein; Cell migration; Endoderm; Gastrulation; Kupffer's vesicle; Morphogenesis; Zebrafish
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Year: 2021 PMID: 34599906 PMCID: PMC8781030 DOI: 10.1016/j.ydbio.2021.09.008
Source DB: PubMed Journal: Dev Biol ISSN: 0012-1606 Impact factor: 3.582