A sensitized mutagenesis screen identifies Gli3 as a modifier of Sox10 neurocristopathy

doi:10.1093/hmg/ddn110

Human Molecular Genetics Advance Access published online on April 7, 2008
Human Molecular Genetics, doi:10.1093/hmg/ddn110

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Published by Oxford University Press 2008

A sensitized mutagenesis screen identifies Gli3 as a modifier of Sox10 neurocristopathy

Ivana Matera¹^,2^,3, Dawn E. Watkins-Chow¹^,3, Stacie K. Loftus¹, Ling Hou¹, Arturo Incao¹, Debra L. Silver¹, Cecelia Rivas¹, Eugene C. Elliott¹, Laura L. Baxter¹ and William J. Pavan¹^,*

¹ Genetic Disease Research Branch, National Human Genome Research Institute, National Institutes of Health, Bethesda, MD 20892 ² Laboratorio di Genetica Molecolare, Instituto G. Gaslini, Genova, Italy

^* To whom correspondence should be addressed Address Correspondence to: Dr. William J. Pavan Bldg 49, Room 4A82 49 Convent Drive Mouse Embryology Section, Genetic Disease Research Branch National Human Genome Research Institute, National Institutes of Health Bethesda, MD 20892-4472 bpavan{at}mail.nih.gov phone: (301) 496-7584 fax: (301) 402-2170

Received January 25, 2008; Revised March 5, 2008; Accepted April 2, 2008

Haploinsufficiency for the transcription factor SOX10 is associatedwith the pigmentary deficiencies of Waardenburg syndrome (WS)and is modeled in Sox10 haploinsufficient mice (Sox10^LacZ^/+).As genetic background affects WS severity in both humans andmice, we established an N-ethyl-N-nitrosourea (ENU) mutagenesisscreen to identify modifiers that increase the phenotypic severityof Sox10^LacZ^/+ mice. Analysis of 230 pedigrees identified threemodifiers, named Modifier of Sox10 neurocristopathies (Mos1,Mos2, and Mos3). Linkage analysis confirmed their locationson mouse chromosomes 13, 4, and 3 respectively, within regionsdistinct from previously identified WS loci. Positional candidateanalysis of Mos1 identified a truncation mutation in a hedgehog-signalingmediator, GLI-Kruppel family member 3 (Gli3). Complementationtests using a second allele of Gli3 (Gli3^Xt-J) confirmed thata null mutation of Gli3 causes the increased hypopigmentationin Sox10^LacZ^/+; Gli3^Mos1^/+ double heterozygotes. Early melanoblastmarkers (Mitf, Sox10, Dct, and Si) are reduced in Gli3^Mos1^/Mos1embryos, indicating that loss of GLI3 signaling disrupts melanoblastspecification. In contrast, mice expressing only the GLI3 repressorhave normal melanoblast specification, indicating that the full-lengthGLI3 activator is not required for specification of neural crestto the melanocyte lineage. This study demonstrates the feasibilityof sensitized screens to identify disease modifier loci andimplicates GLI3 and other Hedgehog (HH) signaling componentsas modifiers of human neurocristopathies.

³ Both authors contributed equally to this manuscript

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