Quantitative trait loci affecting phenotypic variation in the vacuolated lens mouse mutant, a multigenic mouse model of neural tube defects

doi:10.1152/physiolgenomics.90260.2008

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Physiol. Genomics 35: 296-304, 2008. First published September 16, 2008; doi:10.1152/physiolgenomics.90260.2008
1094-8341/08 $8.00

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Received 30 May 2008; accepted in final form 28 August 2008.
Physiological Genomics 35:296-304 (2008)
1094-8341/08 $8.00 © 2008 American Physiological Society

Quantitative trait loci affecting phenotypic variation in the vacuolated lens mouse mutant, a multigenic mouse model of neural tube defects

Ron Korstanje ¹^,*, Jigar Desai ³^,*, Gloria Lazar ³, Benjamin King ¹, Jarod Rollins ¹, Melissa Spurr ¹, Jamie Joseph ³, Sindhuja Kadambi ³, Yang Li ², Allison Cherry ¹, Paul G. Matteson ³, Beverly Paigen ¹ and James H. Millonig ³^,4^,5

¹ Jackson Laboratory, Bar Harbor, Maine
² Groningen Bioinformatics Centre, Groningen Biomolecular Sciences and Biotechnology Institute, Haren, The Netherlands
³ Center for Advanced Biotechnology and Medicine, UMDNJ-Robert Wood Johnson Medical School, Piscataway, New Jersey
⁴ Department of Neuroscience and Cell Biology, UMDNJ-Robert Wood Johnson Medical School, Piscataway, New Jersey
⁵ Department of Genetics, Rutgers University, Piscataway, New Jersey

The vacuolated lens (vl) mouse mutant arose spontaneously onthe C3H/HeSn background and exhibits neural tube defects (NTDs),congenital cataract, and occasionally a white belly spot. Wepreviously reported that 1) the vl phenotypes are due to a mutationin an orphan G protein-coupled receptor (GPCR), Gpr161; 2) thepenetrance of the vl NTD and cataract phenotypes are affectedby genetic background, allowing three unlinked quantitativetrait loci (QTL) to be mapped (modifiers of vacuolated lens,Modvl1-3); and 3) phenotype-based bioinformatics followed bygenetic and molecular analysis identified a lens-specific transcriptionfactor that contributes to the cataract-modifying effect ofModvl3. We now extend this analysis in three ways. First, usingthe Gpr161 mutation to unequivocally identify mutant adultsand embryos, we determined that $~$ 50% of vl/vl NTD-affected embryosdie during development. Second, the MOLF/Ei genetic backgroundsuppresses this embryonic lethality but increases the incidenceof the adult belly spot phenotype. Additional QTL analysis wasperformed, and two novel modifiers were mapped [Modvl4, logarithmof odds ratio (LOD) 4.4; Modvl5, LOD 5.0]. Third, phenotype-basedbioinformatics identified candidate genes for these modifiersincluding two GPCRs that cause NTD or skin/pigmentation defects(Modvl4: Frizzled homolog 6; Modvl5: Melanocortin 5 receptor).Because GPCRs form oligomeric complexes, these genes were resequencedand nonsynonymous coding variants were identified. Bioinformaticsand protein modeling suggest that these variants may be functional.Our studies further establish vl as a multigenic mouse modelfor NTDs and identify additional QTL that interact with Gpr161to regulate neurulation.

quantitative trait locus analysis; Gpr161; Frizzled homolog 6; Melanocortin 5 receptor