A zebrafish sox9 gene required for cartilage morphogenesis

Author:

Yan Yi-Lin1,Miller Craig T.1,Nissen Robert2,Singer Amy1,Liu Dong1,Kirn Anette3,Draper Bruce14,Willoughby John1,Morcos Paul A.5,Amsterdam Adam2,Chung Bon-chu6,Westerfield Monte1,Haffter Pascal3,Hopkins Nancy2,Kimmel Charles1,Postlethwait John H.1

Affiliation:

1. Institute of Neuroscience, University of Oregon, Eugene, OR 97403, USA

2. Center for Cancer Research, Department of Biology, Massachusetts Institute of Technology, 40 Ames Street, E17-341, Cambridge, MA 02139, USA

3. MPI für Entwicklungsbiologie, Spemannstr. 35/III, D-72076 Tübingen,Germany

4. Division of Basic Science, Fred Hutchinson Cancer Research Center, B2-152,1100 Fairview Ave. N., Seattle, WA 98109-1024, USA

5. Gene Tools, LLC, One Summerton Way, Philomath, OR 97370, USA

6. Institute of Molecular Biology, Academia Sinica, Nankang, Taipei, Taiwan ROC

Abstract

The molecular genetic mechanisms of cartilage construction are incompletely understood. Zebrafish embryos homozygous for jellyfish (jef)mutations show craniofacial defects and lack cartilage elements of the neurocranium, pharyngeal arches, and pectoral girdle similar to humans with campomelic dysplasia. We show that two alleles of jef contain mutations in sox9a, one of two zebrafish orthologs of the human transcription factor SOX9. A mutation induced by ethyl nitrosourea changed a conserved nucleotide at a splice junction and severely reduced splicing of sox9a transcript. A retrovirus insertion intosox9a disrupted its DNA-binding domain. Inhibiting splicing of thesox9a transcript in wild-type embryos with splice site-directed morpholino antisense oligonucleotides produced a phenotype like jefmutant larvae, and caused sox9a transcript to accumulate in the nucleus; this accumulation can serve as an assay for the efficacy of a morpholino independent of phenotype. RNase-protection assays showed that in morpholino-injected animals, the percent of splicing inhibition decreased from 80% at 28 hours post fertilization to 45% by 4 days. Homozygous mutant embryos had greatly reduced quantities of col2a1 message, the major collagen of cartilage. Analysis of dlx2 expression showed that neural crest specification and migration was normal in jef (sox9a)embryos. Confocal images of living embryos stained with BODIPY-ceramide revealed at single-cell resolution the formation of precartilage condensations in mutant embryos. Besides the lack of overt cartilage differentiation,pharyngeal arch condensations in jef (sox9a) mutants lacked three specific morphogenetic behaviors: the stacking of chondrocytes into orderly arrays, the individuation of pharyngeal cartilage organs and the proper shaping of individual cartilages. Despite the severe reduction of cartilages, analysis of titin expression showed normal muscle patterning in jef (sox9a) mutants. Likewise, calcein labeling revealed that early bone formation was largely unaffected injef (sox9a) mutants. These studies show that jef(sox9a) is essential for both morphogenesis of condensations and overt cartilage differentiation.

Publisher

The Company of Biologists

Subject

Developmental Biology,Molecular Biology

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