Your search keyword '"Agouti Signaling Protein"' showing total 20 results

1. Characterization of Japanese Quail yellow as a Genomic Deletion Upstream of the Avian Homolog of the Mammalian ASIP (agouti) Gene

Author

Shin'ichi Ito, David Gourichon, Miho Inoue-Murayama, Nicola J. Nadeau, Sarah A Follett, Terry Burke, Nicholas I. Mundy, Francis Minvielle, Department of Zoology, University of Cambridge [UK] (CAM), Génétique et Diversité Animales (GEDANIM), Institut National de la Recherche Agronomique (INRA)-AgroParisTech, Faculty of applied Biological Sciences, Gifu University, Pôle d'Expérimentation Avicole de Tours (UE PEAT), Institut National de la Recherche Agronomique (INRA), Department of Animal and Plant Sciences, and University of Sheffield [Sheffield]

Subjects

Male, 0106 biological sciences, Gene isoform, animal structures, [SDV]Life Sciences [q-bio], Molecular Sequence Data, Locus (genetics), Coturnix, SLC24A5, Investigations, 010603 evolutionary biology, 01 natural sciences, 03 medical and health sciences, biology.animal, Genetics, Animals, Coding region, [INFO]Computer Science [cs], Gene, Crosses, Genetic, Sequence Deletion, 030304 developmental biology, Mammals, 0303 health sciences, biology, Wild type, JAPANESE QUAIL, ASIP GENE, PIGMENTATION, Feathers, biology.organism_classification, Molecular biology, Quail, Mutation, biology.protein, Agouti Signaling Protein, RNA, Female, 5' Untranslated Regions, Chickens

Abstract

ASIP is an important pigmentation gene responsible for dorsoventral and hair-cycle-specific melanin-based color patterning in mammals. We report some of the first evidence that the avian ASIP gene has a role in pigmentation. We have characterized the genetic basis of the homozygous lethal Japanese quail yellow mutation as a >90-kb deletion upstream of ASIP. This deletion encompasses almost the entire coding sequence of two upstream loci, RALY and EIF2B, and places ASIP expression under control of the RALY promoter, leading to the presence of a novel transcript. ASIP mRNA expression was upregulated in many tissues in yellow compared to wild type but was not universal, and consistent differences were not observed among skins of yellow and wild-type quail. In a microarray analysis on developing feather buds, the locus with the largest downregulation in yellow quail was SLC24A5, implying that it is regulated by ASIP. Finally, we document the presence of ventral skin-specific isoforms of ASIP mRNA in both wild-type quails and chickens. Overall, there are remarkable similarities between yellow in quail and lethal yellow in mouse, which involve a deletion in a similar genomic position. The presence of ventral-specific ASIP expression in birds shows that this feature is conserved across vertebrates.

Published

2008

2. Linkage and Segregation Analysis of Black and Brindle Coat Color in Domestic Dogs

Author

Gregory S. Barsh, Rory J. Todhunter, Leigh Anne Clark, Sheila M. Schmutz, Julie A. Kerns, Michael Olivier, George Lust, Keith E. Murphy, Edward J. Cargill, Sophie I. Candille, and T. G. Berryere

Subjects

Coat, Genetic Linkage, Locus (genetics), Investigations, Biology, Chromosomes, Dogs, Genetic linkage, Chromosome Segregation, Genetics, Animals, Melanocyte-Stimulating Hormones, Allele, Hair Color, Gene, Alleles, Pigmentation, Chromosome Mapping, Epistasis, Genetic, Agouti Signaling Protein, Intercellular Signaling Peptides and Proteins, Epistasis, Melanocortin, Receptor, Melanocortin, Type 1, Melanocortin 1 receptor

Abstract

Mutations of pigment type switching have provided basic insight into melanocortin physiology and evolutionary adaptation. In all vertebrates that have been studied to date, two key genes, Agouti and Melanocortin 1 receptor (Mc1r), encode a ligand-receptor system that controls the switch between synthesis of red–yellow pheomelanin vs. black–brown eumelanin. However, in domestic dogs, historical studies based on pedigree and segregation analysis have suggested that the pigment type-switching system is more complicated and fundamentally different from other mammals. Using a genomewide linkage scan on a Labrador × greyhound cross segregating for black, yellow, and brindle coat colors, we demonstrate that pigment type switching is controlled by an additional gene, the K locus. Our results reveal three alleles with a dominance order of black (KB) > brindle (kbr) > yellow (ky), whose genetic map position on dog chromosome 16 is distinct from the predicted location of other pigmentation genes. Interaction studies reveal that Mc1r is epistatic to variation at Agouti or K and that the epistatic relationship between Agouti and K depends on the alleles being tested. These findings suggest a molecular model for a new component of the melanocortin signaling pathway and reveal how coat-color patterns and pigmentary diversity have been shaped by recent selection.

Published

2007

3. Genetic Studies of the Mouse Mutations mahogany and mahoganoid

Author

M. M. Carrasquillo, Donald B. Galbraith, Kimberly A. Miller, Teresa M. Gunn, Gregory S. Barsh, and M. L. Lamoreux

Subjects

Male, Mutant, Investigations, Biology, Melanocyte, medicine.disease_cause, Mice, Adrenocorticotropic Hormone, Genetics, medicine, Animals, Obesity, Hair Color, Receptor, Gene, Crosses, Genetic, Melanins, Mice, Inbred C3H, Mutation, integumentary system, Receptors, Melanocortin, digestive, oral, and skin physiology, Proteins, Mice, Mutant Strains, Mice, Inbred C57BL, Phenotype, medicine.anatomical_structure, Receptors, Corticotropin, alpha-MSH, Protein Biosynthesis, Agouti Signaling Protein, Intercellular Signaling Peptides and Proteins, Female, Ectopic expression, Signal transduction, Melanocortin, hormones, hormone substitutes, and hormone antagonists, Signal Transduction

Abstract

The mouse mutations mahogany (mg) and mahoganoid (md) are negative modifiers of the Agouti coat color gene, which encodes a paracrine signaling molecule that induces a switch in melanin synthesis from eumelanin to pheomelanin. Animals mutant for md or mg synthesize very little or no pheomelanin depending on Agouti gene background. The Agouti protein is normally expressed in the skin and acts as an antagonist of the melanocyte receptor for α-MSH (Mc1r); however, ectopic expression of Agouti causes obesity, possibly by antagonizing melanocortin receptors expressed in the brain. To investigate where md and mg lie in a genetic pathway with regard to Agouti and Mc1r signaling, we determined the effects of these mutations in animals that carried either a loss-of-function Mc1r mutation (recessive yellow, Mc1re) or a gain-of-function Agouti mutation (lethal yellow, Ay). We found that the Mc1re mutation suppressed the effects of md and mg, but that md and mg suppressed the effects of Ay on both coat color and obesity. Plasma levels of α-MSH and of ACTH were unaffected by md or mg. These results suggest that md and mg interfere directly with Agouti signaling, possibly at the level of protein production or receptor regulation.

Published

1997

4. Coupled Site-Directed Mutagenesis/Transgenesis Identifies Important Functional Domains of the Mouse Agouti Protein

Author

Neal G. Copeland, Takuro Nakamura, Bryn Eagleson, William L. Perry, Nancy A. Jenkins, Carolyn M. Hustad, Lisa Secrest, and Deborah A. Swing

Subjects

Male, Signal peptide, Glycosylation, Transgene, Molecular Sequence Data, Mice, Transgenic, Investigations, Biology, Mice, chemistry.chemical_compound, Genetics, Animals, Humans, Amino Acid Sequence, Cysteine, Obesity, RNA, Messenger, Transgenes, Binding site, Hair Color, Site-directed mutagenesis, Receptor, Peptide sequence, Binding Sites, integumentary system, digestive, oral, and skin physiology, Proteins, Mice, Inbred C57BL, chemistry, Mice, Inbred DBA, Mutagenesis, Site-Directed, Agouti Signaling Protein, Intercellular Signaling Peptides and Proteins, Female, Asparagine, Melanocortin, hormones, hormone substitutes, and hormone antagonists

Abstract

The agouti locus encodes a novel paracrine signaling molecule containing a signal sequence, an N-linked glycosylation site, a central lysine-rich basic domain, and a C-terminal tail containing 10 cysteine (Cys) residues capable of forming five disulfide bonds. When overexpressed, agouti causes a number of pleiotropic effects including yellow coat and adult-onset obesity. Numerous studies suggest that agouti causes yellow coat color by antagonizing the binding of a-melanocyte-stimulating hormone (α-MSH) to the a-MSH-(melanocortin-1) receptor. With the goal of identifying functional domains of agouti important for its diverse biological activities, we have generated 14 agouti mutations by in vitro sitedirected mutagenesis and analyzed these mutations in transgenic mice for their effects on coat color and obesity. These studies demonstrate that the signal sequence, the N-linked glycosylation site, and the C-terminal Cys residues are important for full biological activity, while at least a portion of the lysine-rich basic domain is dispensable for normal function. They also show that the same functional domains of agouti important in coat color determination are important for inducing obesity, consistent with the hypothesis that agouti induces obesity by antagonizing melanocortin binding to other melanocortin receptors.

Published

1996

5. Opposite Orientations of an Inverted Duplication and Allelic Variation at the Mouse agouti Locus

Author

Gregory S. Barsh, Yanru Chen, and David M. J. Duhl

Subjects

Male, Genotype, Molecular Sequence Data, Locus (genetics), Investigations, Biology, Mice, Exon, Inbred strain, Genetics, Animals, Gene conversion, Allele, Alleles, Southern blot, Base Sequence, Haplotype, Genetic Variation, Proteins, DNA, Exons, Molecular biology, Multigene Family, Agouti Signaling Protein, Intercellular Signaling Peptides and Proteins, Female, Homologous recombination, Microsatellite Repeats

Abstract

The mouse agouti protein is a paracrine signaling molecule that causes yellow pigment synthesis. A pale ventral coloration distinguishes the light-bellied agouti (AW) from the agouti (A) allele, and is caused by expression of ventral-specific mRNA isoforms with a unique 5′ untranslated exon. Molecular cloning demonstrates this ventral-specific exon lies within a 3.1-kb element that is duplicated in the opposite orientation 15-kb upstream to produce an interrupted palindrome and that similarity between the duplicated elements has been maintained by gene conversion. Orientation of the palindrome is reversed in A compared to AW, which suggests that mutation from one allele to the other is caused by intrachromosomal homologous recombination mediated by sequences within the duplicated elements. Analysis of 15 inbred strains of laboratory and wild-derived mice with Southern hybridization probes and closely linked microsatellite markers suggests six haplotype groups: one typical for most strains that carry AW (129/SvJ, LP/J, CE/J, CAST/Ei), one typical for most strains that carry A (Balb/cJ, CBA/J, FVB/N, PERA/Rk, RBB/Dn); and four that are atypical (MOLC/Rk, MOLG/Dn, PERA/Ei, PERC/Ei, SPRET/Ei, RBA/Dn). Our results suggest a model for molecular evolution of the agouti locus in which homologous recombination can produce a reversible switch in allelic identity.

Published

1996

6. A transgenic mouse assay for agouti protein activity

Author

Carolyn M. Hustad, William L. Perry, Nancy A. Jenkins, Neal G. Copeland, and Deborah A. Swing

Subjects

Male, Genetically modified mouse, DNA, Complementary, Recombinant Fusion Proteins, Molecular Sequence Data, Mice, Transgenic, Investigations, Biology, Mice, Black hair, Genetics, medicine, Animals, Humans, Point Mutation, Obesity, Allele, Hair Color, Promoter Regions, Genetic, Gene, Regulation of gene expression, Mice, Inbred C3H, Base Sequence, integumentary system, Point mutation, digestive, oral, and skin physiology, Proteins, Hair follicle, Phenotype, Molecular biology, Actins, Mice, Mutant Strains, Mice, Inbred C57BL, medicine.anatomical_structure, Gene Expression Regulation, Genes, Mice, Inbred DBA, Protein Biosynthesis, Agouti Signaling Protein, Intercellular Signaling Peptides and Proteins, Female, Genes, Lethal, hormones, hormone substitutes, and hormone antagonists

Abstract

The mouse agouti gene encodes an 131 amino acid paracrine signaling molecule that instructs hair follicle melanocytes to switch from making black to yellow pigment. Expression of agouti during the middle part of the hair growth cycle in wild-type mice produces a yellow band on an otherwise black hair. The ubiquitous unregulated expression of agouti in mice carrying dominant yellow alleles is associated with pleiotropic effects including increased yellow pigment in the coat, obesity, diabetes and increased tumor susceptibility. Agouti shows no significant homology to known genes, and the molecular analysis of agouti alleles has shed little new light on the important functional elements of the agouti protein. In this paper, we show that agouti expression driven by the human beta-ACTIN promoter produces obese yellow transgenic mice and that this can be used as an assay for agouti activity. We used this assay to evaluate a point mutation associated with the a16H allele within the region encoding agouti's putative signal sequence and our results suggest that this mutation is sufficient to cause the a16H phenotype. Thus, in vitro mutagenesis followed by the generation of transgenic mice should allow us to identify important functional elements of the agouti protein.

Published

1995

7. Genetic instability at the agouti locus of the mouse (Mus musculus). I. Increased reverse mutation frequency to the Aw allele in A/a heterozygotes

Author

Jack Favor, Angelika Neuhäuser-Klaus, and Rodica Sandulache

Subjects

Male, Heterozygote, DNA Mutational Analysis, Reversion, Locus (genetics), Investigations, Biology, Chromosomal crossover, Mice, Genetics, Animals, Crossing Over, Genetic, Allele, Gene, Alleles, Mice, Inbred C3H, integumentary system, Models, Genetic, digestive, oral, and skin physiology, Proteins, Heterozygote advantage, Molecular biology, Mice, Mutant Strains, Mice, Inbred C57BL, Mice, Inbred DBA, Mutagenesis, Genetic marker, Ethylnitrosourea, Agouti Signaling Protein, Intercellular Signaling Peptides and Proteins, Female, Restriction fragment length polymorphism, Polymorphism, Restriction Fragment Length

Abstract

We have compiled the reverse mutation rate data to the white bellied agouti (Aw) allele in heterozygous A/a mice and shown it to be increased by a factor of at least 350 in comparison to the reverse mutation rate in homozygous a/a mice. Employing tightly linked flanking restriction fragment length polymorphism DNA markers, we have shown that reversion to Aw is associated with crossing over in the vicinity of the agouti locus. The non-agouti (a) allele has been recently shown to contain an 11-kb insert within the first intron of the agouti gene. Together with our present results, these observations suggest possible mechanisms to explain the reversion events.

Published

1994

8. A domestic cat X chromosome linkage map and the sex-linked orange locus: mapping of orange, multiple origins and epistasis over nonagouti

Author

Melody E. Roelke, Eduardo Eizirik, Victor A. David, Steven S. Hannah, Anne Schmidt-Küntzel, Marilyn Menotti-Raymond, Alejandro A. Schäffer, James Kehler, Stephen J. O'Brien, and George W. Nelson

Subjects

Genetics, X Chromosome, Pseudoautosomal region, Quantitative Trait Loci, Chromosome Mapping, Locus (genetics), Epistasis, Genetic, Biology, Investigations, Evolution, Molecular, Centimorgan, Genetics, Population, Gene mapping, Genetic linkage, Evolutionary biology, Genetic marker, Cats, Agouti Signaling Protein, Animals, Hair Color, X chromosome, Sex linkage, Microsatellite Repeats

Abstract

A comprehensive genetic linkage map of the domestic cat X chromosome was generated with the goal of localizing the genomic position of the classic X-linked orange (O) locus. Microsatellite markers with an average spacing of 3 Mb were selected from sequence traces of the cat 1.9× whole genome sequence (WGS), including the pseudoautosomal region 1 (PAR1). Extreme variation in recombination rates (centimorgans per megabase) was observed along the X chromosome, ranging from a virtual absence of recombination events in a region estimated to be >30 Mb to recombination frequencies of 15.7 cM/Mb in a segment estimated to be

Published

2009

9. Genetics of Sex-linked yellow in the Syrian hamster

Author

Azita Alizadeh, Gregory S. Barsh, Lewis Z. Hong, Christopher B. Kaelin, Hermogenes Manuel, and Terje Raudsepp

Subjects

Male, X Chromosome, Genetic Linkage, Mutant, Population, Hamster, Investigations, behavioral disciplines and activities, Models, Biological, Genetic linkage, Cricetinae, Genetics, Animals, education, Hair Color, Gene, X chromosome, education.field_of_study, biology, Mesocricetus, Genetic Variation, Epistasis, Genetic, biology.organism_classification, Pedigree, Genetics, Population, Phenotype, Agouti Signaling Protein, Female, Receptor, Melanocortin, Type 1, Sex linkage

Abstract

Alternating patches of black and yellow pigment are a ubiquitous feature of mammalian color variation that contributes to camouflage, species recognition, and morphologic diversity. X-linked determinants of this pattern—recognized by variegation in females but not in males—have been described in the domestic cat as Orange, and in the Syrian hamster as Sex-linked yellow (Sly), but are curiously absent from other vertebrate species. Using a comparative genomic approach, we develop molecular markers and a linkage map for the euchromatic region of the Syrian hamster X chromosome that places Sly in a region homologous to the centromere-proximal region of human Xp. Comparison to analogous work carried out for Orange in domestic cats indicates, surprisingly, that the cat and hamster mutations lie in nonhomologous regions of the X chromosome. We also identify the molecular cause of recessively inherited black coat color in hamsters (historically referred to as nonagouti) as a Cys115Tyr mutation in the Agouti gene. Animals doubly mutant for Sly and nonagouti exhibit a Sly phenotype. Our results indicate that Sly represents a melanocortin pathway component that acts similarly to, but is genetically distinct from, Mc1r and that has implications for understanding both the evolutionary history and the mutational mechanisms of pigment-type switching.

Published

2009

10. Molecular and phenotypic analysis of 25 recessive, homozygous-viable alleles at the mouse agouti locus

Author

Rosalynn J. Miltenberger, Liane B. Russell, Edward J. Michaud, Kazumasa Wakamatsu, Shosuke Ito, and Richard P. Woychik

Subjects

Signal peptide, Male, Molecular Sequence Data, Locus (genetics), Genes, Recessive, Biology, Germline, Exon, Mice, Gene expression, Genetics, Animals, Amino Acid Sequence, Allele, Alleles, Melanins, Mice, Inbred C3H, integumentary system, Pigmentation, Proteins, Exons, Sequence Analysis, DNA, Phenotype, Molecular biology, Mice, Inbred C57BL, Mutation, Agouti Signaling Protein, Intercellular Signaling Peptides and Proteins, Female, Melanocortin, Hair, Research Article

Abstract

Agouti is a paracrine-acting, transient antagonist of melanocortin 1 receptors that specifies the subapical band of yellow on otherwise black hairs of the wild-type coat. To better understand both agouti structure/function and the germline damage caused by chemicals and radiation, an allelic series of 25 recessive, homozygous-viable agouti mutations generated in specific-locus tests were characterized. Visual inspection of fur, augmented by quantifiable chemical analysis of hair melanins, suggested four phenotypic categories (mild, moderate, umbrous-like, severe) for the 18 hypomorphs and a single category for the 7 amorphs (null). Molecular analysis indicated protein-coding alterations in 8 hypomorphs and 6 amorphs, with mild-moderate phenotypes correlating with signal peptide or basic domain mutations, and more devastating phenotypes resulting from C-terminal lesions. Ten hypomorphs and one null demonstrated wild-type coding potential, suggesting that they contain mutations elsewhere in the ≥125-kb agouti locus that either reduce the level or alter the temporal/spatial distribution of agouti transcripts. Beyond the notable contributions to the field of mouse germ cell mutagenesis, analysis of this allelic series illustrates that complete abrogation of agouti function in vivo occurs most often through protein-coding lesions, whereas partial loss of function occurs slightly more frequently at the level of gene expression control.

Published

2002

11. Linkage and segregation analysis of black and brindle coat color in domestic dogs.

Author

Kerns JA, Cargill EJ, Clark LA, Candille SI, Berryere TG, Olivier M, Lust G, Todhunter RJ, Schmutz SM, Murphy KE, and Barsh GS

Subjects

Agouti Signaling Protein, Alleles, Animals, Chromosome Mapping, Chromosomes, Dogs, Melanocyte-Stimulating Hormones antagonists & inhibitors, Pigmentation genetics, Chromosome Segregation, Epistasis, Genetic, Genetic Linkage, Hair Color genetics, Intercellular Signaling Peptides and Proteins genetics, Receptor, Melanocortin, Type 1 genetics

Abstract

Mutations of pigment type switching have provided basic insight into melanocortin physiology and evolutionary adaptation. In all vertebrates that have been studied to date, two key genes, Agouti and Melanocortin 1 receptor (Mc1r), encode a ligand-receptor system that controls the switch between synthesis of red-yellow pheomelanin vs. black-brown eumelanin. However, in domestic dogs, historical studies based on pedigree and segregation analysis have suggested that the pigment type-switching system is more complicated and fundamentally different from other mammals. Using a genomewide linkage scan on a Labrador x greyhound cross segregating for black, yellow, and brindle coat colors, we demonstrate that pigment type switching is controlled by an additional gene, the K locus. Our results reveal three alleles with a dominance order of black (K(B)) > brindle (k(br)) > yellow (k(y)), whose genetic map position on dog chromosome 16 is distinct from the predicted location of other pigmentation genes. Interaction studies reveal that Mc1r is epistatic to variation at Agouti or K and that the epistatic relationship between Agouti and K depends on the alleles being tested. These findings suggest a molecular model for a new component of the melanocortin signaling pathway and reveal how coat-color patterns and pigmentary diversity have been shaped by recent selection.

Published

2007

12. Molecular and phenotypic analysis of 25 recessive, homozygous-viable alleles at the mouse agouti locus.

Author

Miltenberger RJ, Wakamatsu K, Ito S, Woychik RP, Russell LB, and Michaud EJ

Subjects

Agouti Signaling Protein, Alleles, Amino Acid Sequence, Animals, Exons genetics, Female, Genes, Recessive physiology, Hair physiology, Male, Melanins genetics, Melanins physiology, Mice, Mice, Inbred C3H, Mice, Inbred C57BL, Molecular Sequence Data, Mutation, Phenotype, Pigmentation genetics, Proteins physiology, Sequence Analysis, DNA, Genes, Recessive genetics, Intercellular Signaling Peptides and Proteins, Proteins genetics

Abstract

Agouti is a paracrine-acting, transient antagonist of melanocortin 1 receptors that specifies the subapical band of yellow on otherwise black hairs of the wild-type coat. To better understand both agouti structure/function and the germline damage caused by chemicals and radiation, an allelic series of 25 recessive, homozygous-viable agouti mutations generated in specific-locus tests were characterized. Visual inspection of fur, augmented by quantifiable chemical analysis of hair melanins, suggested four phenotypic categories (mild, moderate, umbrous-like, severe) for the 18 hypomorphs and a single category for the 7 amorphs (null). Molecular analysis indicated protein-coding alterations in 8 hypomorphs and 6 amorphs, with mild-moderate phenotypes correlating with signal peptide or basic domain mutations, and more devastating phenotypes resulting from C-terminal lesions. Ten hypomorphs and one null demonstrated wild-type coding potential, suggesting that they contain mutations elsewhere in the > or = 125-kb agouti locus that either reduce the level or alter the temporal/spatial distribution of agouti transcripts. Beyond the notable contributions to the field of mouse germ cell mutagenesis, analysis of this allelic series illustrates that complete abrogation of agouti function in vivo occurs most often through protein-coding lesions, whereas partial loss of function occurs slightly more frequently at the level of gene expression control.

Published

2002

13. Molecular and phenotypic analysis of Attractin mutant mice.

Author

Gunn TM, Inui T, Kitada K, Ito S, Wakamatsu K, He L, Bouley DM, Serikawa T, and Barsh GS

Subjects

Age Factors, Agouti Signaling Protein, Alleles, Animals, Base Sequence, Blotting, Southern, Body Weight genetics, Brain metabolism, Central Nervous System metabolism, DNA, Complementary metabolism, Genotype, Homozygote, Melanins chemistry, Mice, Mice, Inbred C3H, Molecular Sequence Data, Phenotype, Pigmentation genetics, Proteins genetics, Proteins physiology, RNA, Messenger metabolism, Time Factors, Intercellular Signaling Peptides and Proteins, Membrane Proteins genetics, Membrane Proteins physiology, Mutation

Abstract

Mutations of the mouse Attractin (Atrn; formerly mahogany) gene were originally recognized because they suppress Agouti pigment type switching. More recently, effects independent of Agouti have been recognized: mice homozygous for the Atrn(mg-3J) allele are resistant to diet-induced obesity and also develop abnormal myelination and vacuolation in the central nervous system. To better understand the pathophysiology and relationship of these pleiotropic effects, we further characterized the molecular abnormalities responsible for two additional Atrn alleles, Atrn(mg) and Atrn(mg-L), and examined in parallel the phenotypes of homozygous and compound heterozygous animals. We find that the three alleles have similar effects on pigmentation and neurodegeneration, with a relative severity of Atrn(mg-3J) > Atrn(mg) > Atrn(mg-L), which also corresponds to the effects of the three alleles on levels of normal Atrn mRNA. Animals homozygous for Atrn(mg-3J) or Atrn(mg), but not Atrn(mg-L), show reduced body weight, reduced adiposity, and increased locomotor activity, all in the presence of normal food intake. These results confirm that the mechanism responsible for the neuropathological alteration is a loss--rather than gain--of function, indicate that abnormal body weight in Atrn mutant mice is caused by a central process leading to increased energy expenditure, and demonstrate that pigmentation is more sensitive to levels of Atrn mRNA than are nonpigmentary phenotypes.

Published

2001

14. Genetic studies of the mouse mutations mahogany and mahoganoid.

Author

Miller KA, Gunn TM, Carrasquillo MM, Lamoreux ML, Galbraith DB, and Barsh GS

Subjects

Adrenocorticotropic Hormone blood, Agouti Signaling Protein, Animals, Crosses, Genetic, Female, Hair Color physiology, Male, Melanins biosynthesis, Melanins genetics, Mice, Mice, Inbred C3H, Mice, Inbred C57BL, Mice, Mutant Strains, Obesity genetics, Obesity metabolism, Phenotype, Protein Biosynthesis, Proteins genetics, Receptors, Corticotropin antagonists & inhibitors, Receptors, Melanocortin, Signal Transduction, alpha-MSH blood, Hair Color genetics, Intercellular Signaling Peptides and Proteins, Mutation

Abstract

The mouse mutations mahogany (mg) and mahoganoid (md) are negative modifiers of the Agouti coat color gene, which encodes a paracrine signaling molecule that induces a swithc in melanin synthesis from eumelanin to pheomelanin. Animals mutant for md or mg synthesize very little or no pheomelanin depending on Agouti gene background. The Agouti protein is normally expressed in the skin and acts as an antagonist of the melanocyte receptor for alpha-MSH (Mc1r); however, ectopic expression of Agouti causes obesity, possibly by antagonizing melanocortin receptors expressed in the brain. To investigate where md and mg lie in a genetic pathway with regard to Agouti and Mc1r signaling, we determined the effects of these mutations in animals that carried either a loss-of-function Mc1r mutation (recessive yellow, Mc1re) or a gain-of-function Agouti mutation (lethal yellow, Ay). We found that the Mc1re mutation suppressed the effects of md and mg, but that md and mg suppressed the effects of Ay on both coat color and obesity. Plasma levels of alpha-MSH and of ACTH were unaffected by md or mg. These results suggest that md and mg interfere directly with Agouti signaling, possibly at the level of protein production or receptor regulation.

Published

1997

15. Opposite orientations of an inverted duplication and allelic variation at the mouse agouti locus.

Author

Chen Y, Duhl DM, and Barsh GS

Subjects

Agouti Signaling Protein, Animals, Base Sequence, DNA, Exons, Female, Genotype, Male, Mice, Molecular Sequence Data, Multigene Family, Alleles, Genetic Variation, Intercellular Signaling Peptides and Proteins, Microsatellite Repeats, Proteins genetics

Abstract

The mouse agouti protein is a paracrine signaling molecule that causes yellow pigment synthesis. A pale ventral coloration distinguishes the light-bellied agouti (AW) from the agouti (A) allele, and is caused by expression of ventral-specific mRNA isoforms with a unique 5' untranslated exon. Molecular cloning demonstrates this ventral-specific exon lies within a 3.1-kb element that is duplicated in the opposite orientation 15-kb upstream to produce an interrupted palindrome and that similarity between the duplicated elements has been maintained by gene conversion. Orientation of the palindrome is reversed in A compared to AW, which suggests that mutation from one allele to the other is caused by intrachromosomal homologous recombination mediated by sequences within the duplicated elements. Analysis of 15 inbred strains of laboratory and wild-derived mice with Southern hybridization probes and closely linked microsatellite markers suggests six haplotype groups: one typical for most strains that carry AW (129/SvJ, LP/J, CE/J, CAST/Ei), one typical for most strains that carry A (Balb/cJ, CBA/J, FVB/N, PERA/Rk, RBB/Dn); and four that are atypical (MOLC/Rk, MOLG/Dn, PERA/Ei, PERC/Ei, SPRET/Ei, RBA/Dn). Our results suggest a model for molecular evolution of the agouti locus in which homologous recombination can produce a reversible switch in allelic identity.

Published

1996

16. Coupled site-directed mutagenesis/transgenesis identifies important functional domains of the mouse agouti protein.

Author

Perry WL, Nakamura T, Swing DA, Secrest L, Eagleson B, Hustad CM, Copeland NG, and Jenkins NA

Subjects

Agouti Signaling Protein, Amino Acid Sequence, Animals, Asparagine, Binding Sites, Cysteine, Female, Humans, Male, Mice, Mice, Inbred C57BL, Mice, Inbred DBA, Mice, Transgenic, Molecular Sequence Data, Mutagenesis, Site-Directed, RNA, Messenger, Transgenes, Hair Color genetics, Intercellular Signaling Peptides and Proteins, Obesity genetics, Proteins genetics

Abstract

The agouti locus encodes a novel paracrine signaling molecule containing a signal sequence, an N-linked glycosylation site, a central lysine-rich basic domain, and a C-terminal tail containing 10 cysteine (Cys) residues capable of forming five disulfide bonds. When overexpressed, agouti causes a number of pleiotropic effects including yellow coat and adult-onset obesity. Numerous studies suggest that agouti causes yellow coat color by antagonizing the binding of alpha-melanocyte-stimulating hormone (alpha-MSH) to the alpha-MSH-(Melanocortin-1) receptor. With the goal of identifying functional domains of agouti important for its diverse biological activities, we have generated 14 agouti mutations by in vitro site-directed mutagenesis and analyzed these mutations in transgenic mice for their effects on coat color and obesity. These studies demonstrate that the signal sequence, the N-linked glycosylation site, and the C-terminal Cys residues are important for full biological activity, while at least a portion of the lysine-rich basic domain is dispensable for normal function. They also show that the same functional domains of agouti important to coat color determination are important for inducing obesity, consistent with the hypothesis that agouti induces obesity by antagonizing melanocortin binding to other melanocortin receptors.

Published

1996

17. Molecular basis of the pleiotropic phenotype of mice carrying the hypervariable yellow (Ahvy) mutation at the agouti locus.

Author

Argeson AC, Nelson KK, and Siracusa LD

Subjects

Agouti Signaling Protein, Animals, Base Sequence, Blotting, Southern, DNA Primers, Dinucleoside Phosphates metabolism, Exons, Female, Male, Methylation, Mice, Mice, Inbred C3H, Molecular Sequence Data, Mutagenesis, Insertional, Phenotype, RNA, Messenger, Sequence Homology, Nucleic Acid, Gene Expression Regulation, Genes, Intracisternal A-Particle, Hair Color genetics, Intercellular Signaling Peptides and Proteins, Proteins genetics

Abstract

The murine agouti locus regulates a switch in pigment synthesis between eumelanin (black/brown pigment) and phaeomelanin (yellow/red pigment) by hair bulb melanocytes. We recently described a spontaneous mutation, hypervariable yellow (Ahvy) and demonstrated that Ahvy is responsible for the largest range of phenotypes yet identified at the agouti locus, producing mice that are obese with yellow coats to mice that are of normal weight with black coats. Here, we show that agouti expression is altered both temporally and spatially in Ahvy mutants. Agouti expression levels are positively correlated with the degree of yellow pigmentation in individual Ahvy mice, consistent with results from other dominant yellow agouti mutations. Sequencing of 5' RACE and genomic PCR products revealed that Ahvy resulted from the integration of an intracisternal A particle (IAP) in an antisense orientation within the 5' untranslated agouti exon 1C. This retrovirus-like element is responsible for deregulating agouti expression in Ahvy mice; agouti expression is correlated with the methylation state of CpG residues in the IAP long terminal repeat as well as in host genomic DNA. In addition, the data suggest that the variable phenotype of Ahvy offspring is influenced in part by the phenotype of their Ahvy female parent.

Published

1996

18. Molecular genetic characterization of six recessive viable alleles of the mouse agouti locus.

Author

Hustad CM, Perry WL, Siracusa LD, Rasberry C, Cobb L, Cattanach BM, Kovatch R, Copeland NG, and Jenkins NA

Subjects

Agouti Signaling Protein, Animals, Base Sequence, Chromosome Inversion, Chromosome Mapping, DNA genetics, Gene Expression Regulation, Hair Color genetics, Lung Diseases, Interstitial genetics, Lymphoproliferative Disorders genetics, Male, Melanins biosynthesis, Mice, Mice, Inbred C3H, Mice, Inbred C57BL, Molecular Sequence Data, Mutagenesis, Phenotype, RNA, Messenger genetics, Transcription, Genetic, Alleles, Genes, Recessive, Intercellular Signaling Peptides and Proteins, Mice, Mutant Strains genetics, Proteins genetics

Abstract

The agouti locus on mouse chromosome 2 encodes a secreted cysteine-rich protein of 131 amino acids that acts as a molecular switch to instruct the melanocyte to make either yellow pigment (phaeomelanin) or black pigment (eumelanin). Mutations that up-regulate agouti expression are dominant to those causing decreased expression and result in yellow coat color. Other associated effects are obesity, diabetes, and increased susceptibility to tumors. To try to define important functional domains of the agouti protein, we have analyzed the molecular defects present in a series of recessive viable agouti mutations. In total, six alleles (amJ, au, ada, a16H, a18H, ae) were examined at both the RNA and DNA level. Two of the alleles, a16H and ae, result from mutations in the agouti coding region. Four alleles (amJ, au, a18H, and ada) appear to represent regulatory mutations that down-regulate agouti expression. Interestingly, one of these mutations, a18H, also appears to cause an immunological defect in the homozygous condition. This immunological defect is somewhat analogous to that observed in motheaten (me) mutant mice. Short and long-range restriction enzyme analyses of homozygous a18H DNA are consistent with the hypothesis that a18H results from a paracentric inversion where one end of the inversion maps in the 5' regulatory region of agouti and the other end in or near a gene that is required for normal immunological function. Cloning the breakpoints of this putative inversion should allow us to identify the gene that confers this interesting immunological disorder.

Published

1995

19. A transgenic mouse assay for agouti protein activity.

Author

Perry WL, Hustad CM, Swing DA, Jenkins NA, and Copeland NG

Subjects

Actins genetics, Agouti Signaling Protein, Animals, Base Sequence, DNA, Complementary genetics, Female, Gene Expression Regulation, Genes, Genes, Lethal, Hair Color genetics, Humans, Male, Mice, Mice, Inbred C3H, Mice, Inbred C57BL, Mice, Inbred DBA, Mice, Mutant Strains, Mice, Transgenic, Molecular Sequence Data, Obesity genetics, Phenotype, Point Mutation, Promoter Regions, Genetic, Protein Biosynthesis, Proteins genetics, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins genetics, Intercellular Signaling Peptides and Proteins, Proteins analysis

Abstract

The mouse agouti gene encodes an 131 amino acid paracrine signaling molecule that instructs hair follicle melanocytes to switch from making black to yellow pigment. Expression of agouti during the middle part of the hair growth cycle in wild-type mice produces a yellow band on an otherwise black hair. The ubiquitous unregulated expression of agouti in mice carrying dominant yellow alleles is associated with pleiotropic effects including increased yellow pigment in the coat, obesity, diabetes and increased tumor susceptibility. Agouti shows no significant homology to known genes, and the molecular analysis of agouti alleles has shed little new light on the important functional elements of the agouti protein. In this paper, we show that agouti expression driven by the human beta-ACTIN promoter produces obese yellow transgenic mice and that this can be used as an assay for agouti activity. We used this assay to evaluate a point mutation associated with the a16H allele within the region encoding agouti's putative signal sequence and our results suggest that this mutation is sufficient to cause the a16H phenotype. Thus, in vitro mutagenesis followed by the generation of transgenic mice should allow us to identify important functional elements of the agouti protein.

Published

1995

20. Genetic instability at the agouti locus of the mouse (Mus musculus). I. Increased reverse mutation frequency to the Aw allele in A/a heterozygotes.

Author

Sandulache R, Neuhäuser-Klaus A, and Favor J

Subjects

Agouti Signaling Protein, Animals, Crossing Over, Genetic, DNA Mutational Analysis, Ethylnitrosourea, Female, Heterozygote, Male, Mice, Inbred C3H, Mice, Inbred C57BL, Mice, Inbred DBA, Mice, Mutant Strains genetics, Models, Genetic, Mutagenesis, Polymorphism, Restriction Fragment Length, Alleles, Intercellular Signaling Peptides and Proteins, Mice genetics, Proteins genetics

Abstract

We have compiled the reverse mutation rate data to the white bellied agouti (Aw) allele in heterozygous A/a mice and shown it to be increased by a factor of at least 350 in comparison to the reverse mutation rate in homozygous a/a mice. Employing tightly linked flanking restriction fragment length polymorphism DNA markers, we have shown that reversion to Aw is associated with crossing over in the vicinity of the agouti locus. The non-agouti (a) allele has been recently shown to contain an 11-kb insert within the first intron of the agouti gene. Together with our present results, these observations suggest possible mechanisms to explain the reversion events.

Published

1994