Mahoganoid polypeptides, and related compositions and methods

[0003] Throughout this application, various references are cited. Disclosure of these references in their entirety is hereby incorporated by reference into this application to more fully describe the state of the art to which this invention pertains.

BACKGROUND OF THE INVENTION

[0004] Molecular cloning of the five extant monogenic forms of rodent obesity identified critical molecules in the pathways regulating energy homeostasis in animals and human (1). The agouti (a) gene encodes a 131 amino acid peptide, agouti signaling protein (ASP) that is normally secreted only in the follicular cells of the dermal papilla of the skin (2-4). Mutations of agouti (e.g. Ay and Avy) that cause ectopic overexpression of ASP in the hypothalamus and skin, result in a pleiotropic syndrome that includes increased lean and adipose tissue, yellow pelage (coat), hyperinsulinemia, hyperphagia, and hyperglycemia (3-5). ASP antagonizes the binding of alpha-melanocortin stimulating hormone (α-MSH) to the melanocortin 1 receptor (MC1R) causing melanogenesis to switch from the production of black/brown pigment (eumelanin) to a yellow/red pigment (pheomelanin) (FIG. 1) (2). In the hypothalamus, agouti related protein (AgRP) is the natural antagonist of MC3R and MC4R. AgRP also acts as an inverse agonist at MC4R in both human and mouse (6, 7). In Ay mice, ectopically produced ASP competes with α-MSH for binding to MC3R and MC4R, resulting in hyperphagia, increased body fat, and disordered insulin homeostasis (8).

[0005] Two other mutations, mahogany (Atrnmg, Chr 2) and mahoganoid (md, Chr 16), affect coat color and body weight. Both mutations are unique in their ability to suppress the obesity and darken the coat (umbrous effect) caused by mutations resulting in the ectopic overexpression of ASP. There are three reported alleles of mahogany: Atrnmg, Atrnmg-L, and Atrnmg-3J that are coisogenic on mouse strains LDJ/Le, C3H/HeJ, and C3HeB/FeJ, respectively (9, 10). Atrnmg and Atrnmg-L are each the result of ˜5kb retrovirus insertions in introns 26 and 27, respectively, that disrupt the splicing of Atrn. Atrnmg-3J has a 5-bp deletion at nucleotide 2,809 introducing a stop codon that results in a severely truncated protein. Attractin (Atrn) encodes a single-pass transmembrane ˜210 kDa protein containing 3 epidermal growth factor (EGF) domains, two laminin-like EGF repeats, a CUB domain, two plexin-like repeats, a C-type lectin and seven consecutive Kelch repeats (9, 10). The predicted structure of ATRN suggests that it functions as a receptor or receptor-like protein. The Atrnmg mutation does not suppress the obese phenotype of Mc4r null mice, or that of several monogenic obese models (Leprdb, Lepob, tub, Cpefat) (9, 10), but does suppress diet-induced obesity (10). Homozygosity for LDJ/Le Atrnmg backcrossed for 6-8 generations onto a C57BL/6J background suppresses Ay-induced weight gain by increasing basal metabolic rate (11). In animals doubly mutant for mg and Ay, food intake is not reduced relative to controls (+/+ Ay/a and mg/mg a/a), but body weight is reduced due to higher metabolic rate (11). Mahogany mice are not hyperphagic on a C3H/HeJ background (12). Homozygous Atrnmg animals develop abnormal myelination and vacuolization throughout the brain and spinal cord in association with severe tremors and flaccid paresis (13). The tremors may account for the increased metabolic rate. The neuropathological changes characteristic of Atrnmg animals, and the specificity of binding of ASP but not AgRP to ATRN (14), make it unlikely that ATRN plays a specific role in hypothalamic control of energy homeostasis aside from its effects on muscle motor activity.

[0006] Md has effects on coat color and obesity in Ay mice that are analogous to Atrnmg. The md mutation originally arose spontaneously in the C3H/HeJ strain at Jackson Laboratory in the early 1960s. Subsequently, four additional spontaneous mutations (md2J, md4J, md5J, and md6J) have been documented at this locus [http://www.informatics.jax.org/searches/allele_report .cgi?_Marker_key=11177]. Like Atrnmg, mahoganoid darkens the back, ears, and tail of nonalbino mice (15, 16). This darkening effect is described as an “umbrous” coat. Md suppresses Ay-induced yellow pigmentation and Ay-induced obesity in a gene dose-dependent manner (17). Similar to Atrnmg on the C57BL/6J background, homozygosity for md on the C3H/HeJ background causes hyperphagia (11). The ability of md to induce hyperphagia suggests that the md gene product has effects on energy homeostasis distinct from epistatic effects in the context of overexpression of ASP (Ay). Genetic studies have positioned md, functionally, at the same level or upstream of MC1R and downstream of ASP based on findings that the Mc1re mutation (extension, resulting in a yellow coat) suppressed the coat color effect of md, and that md suppressed both the yellow and obese phenotypes of Ay mice (17) (FIG. 1). Linkage analysis positioned md on chromosome 16, about 2 cM from the centromere (18, 19). Identification of md and its function could provide additional insight into the control of melanocortin signaling.

SUMMARY OF THE INVENTION

[0007] This invention provides an isolated mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity.

[0008] This invention also provides an isolated nucleic acid encoding a mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity.

[0009] This invention also provides a replicable vector comprising an isolated nucleic acid encoding a mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity.

[0010] This invention also provides an isolated nucleic acid that specifically hybridizes to mahoganoid polypeptide-encoding mRNA.

[0011] This invention also provides a host-vector system comprising a cell having therein a replicable vector comprising a nucleic acid encoding a mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity.

[0012] This invention also provides an antibody which specifically binds to an isolated mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity.

[0013] This invention also provides a composition of matter comprising an isolated nucleic acid encoding a mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity and a pharmaceutically acceptable carrier.

[0014] This invention also provides a composition of matter comprising an isolated mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity and a pharmaceutically acceptable carrier.

[0015] This invention also provides a composition of matter comprising an isolated nucleic acid that specifically hybridizes to mahoganoid polypeptide-encoding mRNA and a pharmaceutically acceptable carrier.

[0016] This invention also provides a method for decreasing the amount of mahoganoid polypeptide in a cell comprising contacting the cell with an agent that specifically inhibits mahoganoid polypeptide expression in the cell, thereby decreasing the amount of mahoganoid polypeptide in the cell.

[0017] This invention also provides a method for decreasing the amount of mahoganoid polypeptide in a subject's cells comprising administering to the subject an agent that specifically inhibits mahoganoid polypeptide expression in a cell, thereby decreasing the amount of mahoganoid polypeptide in the subject's cells.

[0018] This invention also provides a method for treating an overweight subject comprising administering to the subject a therapeutically effective amount of an agent that specifically inhibits mahoganoid polypeptide expression in a cell, thereby treating the subject.

[0019] This invention also provides a method for inhibiting the onset of weight gain in a subject comprising administering to the subject a prophylactically effective amount of an agent that specifically inhibits mahoganoid polypeptide expression in a cell, thereby inhibiting the onset of weight gain in the subject.

[0020] This invention also provides an article of manufacture comprising a packaging material having therein an agent that specifically inhibits mahoganoid polypeptide expression in a cell, and a label indicating a use for the agent in treating an overweight subject and/or inhibiting the onset of weight gain in a subject.

[0021] This invention also provides a method for determining whether an agent decreases mahoganoid polypeptide expression in a cell, which method comprises the steps of

[0022] (a) contacting the cell with the agent under suitable conditions;

[0023] (b) determining the amount of mahoganoid polypeptide expression in the cell after a suitable period of time; and

[0024] (c) comparing the amount of mahoganoid polypeptide expression determined in step (b) with the amount of mahoganoid polypeptide expression in a cell in the absence of the agent, whereby a lower amount of mahoganoid polypeptide expression in the cell contacted with the agent, relative to the amount of expression in the absence of the agent, indicates that the agent decreases mahoganoid polypeptide expression in the cell.

[0025] This invention also provides a method for determining whether an agent inhibits the ubiquitin ligase activity of mahoganoid polypeptide, which method comprises the steps of

[0026] (a) contacting mahoganoid polypeptide and ubiquitin with the agent under conditions which would permit mahoganoid polypeptide ubiquitin ligase activity in the absence of the agent;

[0027] (b) determining the amount of ubiquitin ligated after a suitable period of time; and

[0028] (c) comparing the amount of ligated ubiquitin determined in step (b) with the amount of ligated ubiquitin in the absence of the agent, whereby a lower amount of ligated ubiquitin in the presence of the agent, relative to the amount of ligated ubiquitin in the absence of the agent, indicates that the agent inhibits the ubiquitin ligase activity of mahoganoid polypeptide.

[0029] This invention also provides a method for increasing the amount of mahoganoid polypeptide in a cell comprising contacting the cell with an agent that specifically increases mahoganoid polypeptide expression in the cell, thereby increasing the amount of mahoganoid polypeptide in the cell.

[0030] This invention also provides a method for increasing the amount of mahoganoid polypeptide in a subject comprising administering to the subject an agent that specifically increases mahoganoid polypeptide expression in a cell, thereby increasing the amount of mahoganoid polypeptide in the subject.

[0031] This invention also provides a method for treating an underweight subject comprising administering to the subject a therapeutically effective amount of an agent that specifically increases mahoganoid polypeptide expression in a cell, thereby treating the subject.

[0032] This invention also provides a method for inhibiting the onset of weight loss in a subject comprising administering to the subject a prophylactically effective amount of an agent that specifically increases mahoganoid polypeptide expression in a cell, thereby inhibiting the onset of weight loss in the subject.

[0033] This invention also provides an article of manufacture comprising a packaging material having therein an agent that specifically increases mahoganoid polypeptide expression in a cell, and a label indicating a use for the agent in treating an underweight subject and/or inhibiting the onset of weight loss in a subject.

[0034] This invention also provides a method for determining whether an agent increases mahoganoid polypeptide expression in a cell, which method comprises the steps of

[0035] (a) contacting the cell with the agent under suitable conditions;

[0036] (b) determining the amount of mahoganoid polypeptide expression in the cell after a suitable period of time; and

[0037] (c) comparing the amount of mahoganoid polypeptide expression determined in step (b) with the amount of mahoganoid polypeptide expression in a cell in the absence of the agent, whereby a higher amount of mahoganoid polypeptide expression in the cell contacted with the agent, relative to the amount of expression in the absence of the agent, indicates that the agent increases the amount of mahoganoid polypeptide expression in the cell.

[0038] Finally, this invention provides a method for determining whether an agent increases the ubiquitin ligase activity of mahoganoid polypeptide, which method comprises the steps of

[0039] (a) contacting mahoganoid polypeptide and ubiquitin with the agent under conditions which would permit mahoganoid polypeptide ubiquitin ligase activity in the absence of the agent;

[0040] (b) determining the amount of ligated ubiquitin after a suitable period of time; and

[0041] (c) comparing the amount of ligated ubiquitin determined in step (b) with the amount of ligated ubiquitin in the absence of the agent, whereby a higher amount of ligated ubiquitin in the presence of the agent, relative to the amount of ligated ubiquitin in the absence of the agent, indicates that the agent increases the ubiquitin ligase activity of mahoganoid polypeptide.

BRIEF DESCRIPTION OF THE FIGURES

[0042]

FIGS. 1A and 1B

[0043] Schematic of melanocortin signaling pathways, specifically melanocortin signaling in the hair follicle and hypothalamus. α-MSH is a melanocortin peptide that is cleaved from the pro-opiomelanocortin precursor (POMC). (A) α-MSH acts on MC1R resulting in an increase in cAMP to darken coat color. Agouti signaling protein (ASP) antagonizes α-MSH binding at MC1R resulting in pheomelanin synthesis. ATRN (mahogany) may function to down-regulate or desensitize MC1R or may be involved in ASP processing or binding to MC1R. (B) α-MSH activates MC4R to decrease food intake and increase energy expenditure. AgRP competes with α-MSH for binding at MC4R/MC3R resulting in increased food intake. Ay mice ectopically over-produce ASP, interfering with α-MSH signaling at MC4R/MC3R and resulting in an obese phenotype due to increased food intake.

[0044]

FIG. 2

[0045] Coat colors. C57BL/6J +/+ Ay/a and C57BL/6J +/+ a/a mice have yellow and black pelage, respectively. Homozygosity for md results in a darkened pelage in Agouti (A/?) animals, whereas heterozygous md/+ animals have normal agouti (alternate black, yellow banding) pelage. Colors are not shown in the Figure.

[0046]

FIG. 3

[0047] Genetic map of region of proximal Chr. 16 containing md. Map is based on 149 progeny of a B6.C3H-md-A md/md, A/?×B6.C3H-md-A md/+, A/? cross. The congenic C3H/HeJ interval is indicated. Genotype at md is inferred by coat color. md/md A/? animals are umbrous (mahoganoid), md/+ A/? are agouti.

[0048] FIGS. 4A-4C

[0049] Genetic and physical maps of md minimal interval. (A) Genetic map of proximal chromosome 16. Distances between markers indicated in centiMorgans. (B) Mouse genomic clones spanning the minimal interval containing md. Distances indicated are in megabases. (C) Locations of all transcripts (identified by accession number) and predicted genes (all mCGs). Riken full-length cDNA AK011747 is the Mahoganoid transcript (2010 bp).

[0050] FIGS. 5A-5C

[0051] PCR amplification and Southern blot analyses of md alleles. (A) PCR amplification of exon 12 from genomic DNA from all md alleles produces a ˜0.5 kb fragment except for md2J. (B) Southern blot of Pst I digest of md allelic series (md, md2J, md4J, md5J, md6J) genomic DNA probed with part of exon 12 and its 5′ intronic region. The md2J revealed a new fragment of 0.7 kb and a lack of fragment 1.4 kb corresponding to exon 12 whereas md showed a loss of 1.1 kb fragment and a novel 0.6 kb fragment corresponding to the intronic region 5′ of exon 12. md4J, md5J and md6J showed fragments of similar size to the C3H/HeJ +/+ control. (C) Southern blot of Hind III digest of md allelic series probed with cDNA for exons 2-9 shows novel restriction site in md5J.

[0052]

FIG. 6

[0053] Restriction map and location/nature of mahoganoid mutations. (top) Restriction map of normal fragment sizes. (bottom) md, md2J, and md5J mutations are all due to retroviral insertions. md5J and md are due to ˜5 kb insertion located in the intronic region 3′ of exon 2 and 5′ of exon 12, respectively. md2J is due to ˜8 kb insertion within exon 12. Fragment sizes shown above the inserted sequences represent the sizes from the new restriction sites located within retrovirus insertion to the normal restriction site in the direction of the arrow. RF indicates the location of the RING Finger domain located in exon 10. GenBank numbers for md with retrovirus insertions are indicated in parentheses adjacent to new sequences. IAP denotes mouse retrovirus-like repetitive intracisternal type A particle. Sequences in bold are normal sequences. The inserted sequences are underlined.

[0054]

FIGS. 7A and 7B

[0055] Northern Blots. (A) mahoganoid 3.9kb transcript is expressed in all tissues tested. A 5.2 kb transcript is also seen in brain, kidneys, and liver. Only kidney showed a faint transcript of 1.9 Kb. (B) The retrovirus insertion in md and md2J produces several aberrantly sized transcripts: 5.9 kb/5.5 kb/4.1 kb/2.2 kb in md and 12.0 kb/3.6 kb in md2J.

[0056]

FIG. 8

[0057] Mahoganoid protein (BAB27816). 494 amino acids containing a C3HC4 RING finger domain (underlined). Amino acid comparison of md RING domain with Smart00184 (c-Cbl) and other proteins that have E3 ubiquitin-protein ligase activity (33), suggesting a general function of this domain. Human (KIAA0544), D. melanogaster (AAF48305), C. elegans (CAA94116) homologs of mouse mahoganoid have the conserved C3HC4 RING finger. Conserved amino acids are bold. * indicates the conserved cysteine and histidine residues found in all C3HC4 RING finger domains (34).

[0058]

FIG. 9

[0059] Three potential models for Mahoganoid biological effects. Mahoganoid may decrease signaling through MC1R or MC3R/MC4R by increasing expression or activity of an inverse agonist of MC1R or MC3R/MC4R; influencing the physical proximity or binding of ASP and AgRP to their receptors by influencing binding of ATRN to ASP; and decreasing the availability of α-MSH to its receptors through sequestration or turnover of α-MSH.

DETAILED DESCRIPTION OF THE INVENTION

Definitions

[0060] As used in this application, except as otherwise expressly provided herein, each of the following terms shall have the meaning set forth below.

[0061] “Administering” shall mean delivering in a manner which is effected or performed using any of the various methods and delivery systems known to those skilled in the art. Administering can be performed, for example, topically, intravenously, pericardially, orally, via implant, transmucosally, transdermally, intramuscularly, subcutaneously, intraperitoneally, intrathecally, intralymphatically, intralesionally, or epidurally. Administering can also be performed, for example, once, a plurality of times, and/or over one or more extended periods.

[0062] “Agent” shall mean any chemical entity, including, without limitation, a glycomer, a protein, an antibody, a lectin, a nucleic acid, a small molecule, and any combination thereof.

[0063] “Antibody” includes, by way of example, both naturally occurring antibodies (e.g., IgG, IgM, IgE and IgA) and non-naturally occurring antibodies. The term “antibody” also includes polyclonal and monoclonal antibodies, and antigen-binding fragments thereof (e.g., antigen-binding portions). Furthermore, the term “antibody” includes chimeric antibodies, wholly synthetic antibodies, human and humanized antibodies, and antigen-binding fragments thereof.

[0064] “Host cells” include, but are not limited to, bacterial cells, yeast cells, fungal cells, insect cells, and mammalian cells. Mammalian cells can be transfected by methods well-known in the art such as calcium phosphate precipitation, electroporation and microinjection.

[0065] “Increasing the ubiquitin ligase activity” of mahoganoid polypeptide includes, without limitation, increasing the rate at which such ligase activity occurs and/or altering the reaction equilibrium thereof so as to increase the amount of ligated ubiquitin once equilibrium is reached.

[0066] “Inhibiting the ubiquitin ligase activity” of mahoganoid polypeptide includes, without limitation, reducing the rate at which such ligase activity occurs and/or altering the reaction equilibrium thereof so as to reduce the amount of ligated ubiquitin once equilibrium is reached.

[0067] “Inhibiting the onset” of a disorder shall mean either lessening the likelihood of the disorder's onset, or preventing the onset of the disorder entirely. In the preferred embodiment, inhibiting the onset of a disorder means preventing its onset entirely.

[0068] “Isolated”, as used herein, with respect to a particular polypeptide or nucleic acid, includes, without limitation, being in a milieu having a reduced amount of other polypeptides or nucleic acids, respectively. In one embodiment, an isolated polypeptide or nucleic acid is free of other polypeptides or nucleic acids, respectively. In another embodiment, an isolated subject polypeptide or nucleic acid is in a milieu containing other polypeptides or nucleic acids, respectively, in a total amount which does not exceed the amount of the subject polypeptide or nucleic acid, respectively.

[0069] “Mahoganoid polypeptide” and “mahoganoid protein” are used equivalently herein, and are characterized, inter alia, by having ubiquitin ligase activity. Mahoganoid polypeptide is exemplified by the human and mouse polypeptides having the sequences set forth in FIG. 8. Mahoganoid polypeptide, also referred to as “MD”, is encoded by the mahoganoid gene, also referred to as “md”, and includes all allelic variants thereof. The mahoganoid polypeptide-encoding gene is also referred to as “Mahogunin”, “Mgn” and “MGN”, and the mahoganoid polypeptide is also referred to as “MGN.” On certain occasions, the term “mahoganoid” is used in the Experimental Details to refer to mutant mahoganoid genes and/or polypeptides. As used herein, a “mutant” mahoganoid polypeptide is a non-wild type mahoganoid polypeptide correlative with, for example, a change in coat color, body weight and/or brain anatomy and function. Except for this mutant-related usage in the Experimental Details, the meaning of which is clear from its context, mahoganoid polypeptide shall have the meaning as otherwise set forth in this application.

[0070] “Mammalian cells” include, without limitation, normal, abnormal and transformed mammalian cells, and are exemplified by neurons, epithelial cells, muscle cells, blood cells, immune cells, stem cells, osteocytes, endothelial cells and blast cells.

[0071] “Mammalian polypeptide” means a polypeptide originating from a mammalian cell.

[0072] The term “nucleic acid” refers to a polymer of deoxyribonucleotides and/or ribonucleotides. The deoxyribonucleotides and ribonucleotides can be naturally occurring or synthetic analogues thereof.

[0073] “Overweight subject” includes, without limitation, a subject whose weight exceeds the ideal weight for that subject by more than 20%. In one embodiment, the subject's weight exceeds the ideal weight by 50%, 100% or 200%.

[0074] “Pharmaceutically acceptable carriers” are well known to those skilled in the art and include, but are not limited to, 0.01-0.1 M and preferably 0.05 M phosphate buffer or 0.8% saline. Additionally, such pharmaceutically acceptable carriers can be aqueous or non-aqueous solutions, suspensions, and emulsions. Examples of non-aqueous solvents are propylene glycol, polyethylene glycol, vegetable oils such as olive oil, and injectable organic esters such as ethyl oleate. Aqueous carriers include water, alcoholic/aqueous solutions, emulsions and suspensions, including saline and buffered media. Parenteral vehicles include sodium chloride solution, Ringer's dextrose, dextrose and sodium chloride, lactated Ringer's and fixed oils. Intravenous vehicles include fluid and nutrient replenishers, electrolyte replenishers such as those based on Ringer's dextrose, and the like. Preservatives and other additives may also be present, such as, for example, antimicrobials, antioxidants, chelating agents, inert gases, and the like.

[0075] The terms “polypeptide” and “protein” are used interchangeably herein, and each means a polymer of amino acid residues. The amino acid residues can be naturally occurring or chemical analogues thereof. Polypeptides and proteins can also include modifications such as glycosylation, lipid attachment, sulfation, hydroxylation, and ADP-ribosylation.

[0076] “Prophylactically effective amount” means an amount sufficient to inhibit the onset of a disorder in a subject. Simple titration experiments can readily be performed by one of ordinary skill to determine such amount.

[0077] “Specifically bind” shall mean that, with respect to the binding of an antibody to its antigen, the antibody binds to the antigen with a greater affinity than that with which it binds to most other antigens. In the preferred embodiment, the antibody binds to the antigen with a greater affinity than that with which it binds to all other antigens.

[0078] “Specifically hybridize” to a nucleic acid shall mean, with respect to a first nucleic acid, that the first nucleic acid hybridizes to a second nucleic acid with greater affinity than to any other nucleic acid.

[0079] “Specifically inhibit” the expression of a protein shall mean to inhibit that protein's expression (a) more than the expression of any other protein, or (b) more than the expression of all but 10 or fewer other proteins.

[0080] As used herein, “subject” means any animal or artificially modified animal, such as a mammal or a bird, including, without limitation, a cow, a horse, a sheep, a pig, a dog, a cat, a rodent such as a mouse or rat, a chicken and a primate. In the preferred embodiment, the subject is a human.

[0081] “Suitable conditions” shall have a meaning dependent on the context in which this term is used. That is, when used in connection with contacting an agent to a cell, this term shall mean conditions that permit an agent capable of doing so to enter a cell and perform its intended function. In one embodiment, the term “suitable conditions” as used herein means physiological conditions.

[0082] “Therapeutically effective amount” means an amount sufficient to treat a subject. A person of ordinary skill in the art can perform simple titration experiments to determine such amount.

[0083] “Treating” means either slowing, stopping or reversing the progression of a disorder. As used herein, “treating” also means the amelioration of symptoms associated with the disorder.

[0084] “Underweight subject” includes, without limitation, a subject whose ideal weight exceeds his actual weight by more than 20%.

[0085] “Vector” shall mean any nucleic acid vector known in the art. Such vectors include, but are not limited to, plasmid vectors, cosmid vectors, and bacteriophage vectors. For example, one class of vectors utilizes DNA elements which are derived from animal viruses such as bovine papilloma virus, polyoma virus, adenovirus, vaccinia virus, baculovirus, retroviruses (RSV, MMTV, or MOMLV), Semliki Forest virus, SV40 virus or lentiviruses.

EMBODIMENTS OF THE INVENTION

[0086] This invention provides an isolated mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity. In one embodiment, the polypeptide is a mammalian polypeptide. In another embodiment, the polypeptide is a human polypeptide. In another embodiment, the polypeptide is a murine polypeptide.

[0087] This invention also provides an isolated nucleic acid encoding a mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity. In one embodiment, the nucleic acid is DNA. In another embodiment, the nucleic acid is genomic DNA. In another embodiment, the nucleic acid is cDNA. In a further embodiment, the nucleic acid is RNA.

[0088] In another embodiment of the invention, the nucleic acid is labeled with a detectable marker, such as a radioactive, a colorimetric, a luminescent or a fluorescent label.

[0089] This invention also provides a replicable vector comprising an isolated nucleic acid encoding a mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity. In further embodiments, the vector can be a plasmid, a cosmid, YAC or a λ phage.

[0090] This invention also provides an isolated nucleic acid that specifically hybridizes to mahoganoid polypeptide-encoding mRNA. In one embodiment, the nucleic acid is at least 15 nucleotides in length. In another embodiment, the nucleic acid is selected from the group consisting of an RNAi molecule, an antisense RNA molecule, a ribozyme and a DNAzyme.

[0091] This invention also provides a host-vector system comprising a cell having therein a replicable vector comprising a nucleic acid encoding a mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity. In one embodiment, the cell is a eukaryotic cell. In further embodiment, the cell is a mammalian cell. In another embodiment, the cell is a bacterial cell.

[0092] This invention also provides an antibody which specifically binds to an isolated mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity. In one embodiment, the antibody is labeled with a detectable moiety, such as a radioisotope, an enzyme, a fluorogenic material, a chemiluminescent material or an electrochemical material.

[0093] This invention also provides a composition of matter comprising an isolated nucleic acid encoding a mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity and a pharmaceutically acceptable carrier.

[0094] This invention also provides a composition of matter comprising an isolated mahoganoid polypeptide, or a portion thereof having ubiquitin ligase activity and a pharmaceutically acceptable carrier.

[0095] This invention also provides a composition of matter comprising an isolated nucleic acid that specifically hybridizes to mahoganoid polypeptide-encoding mRNA and a pharmaceutically acceptable carrier.

[0096] This invention also provides a method for decreasing the amount of mahoganoid polypeptide in a cell comprising contacting the cell with an agent that specifically inhibits mahoganoid polypeptide expression in the cell, thereby decreasing the amount of mahoganoid polypeptide in the cell. In one embodiment, the cell is a mammalian cell. In a further embodiment, the cell is a mouse cell. In further embodiment, the cell is a human cell. In another embodiment, the cell is a neuron. In a further embodiment, the agent is the instant anti-sense nucleic acid.

[0097] This invention also provides a method for decreasing the amount of mahoganoid polypeptide in a subject's cells comprising administering to the subject an agent that specifically inhibits mahoganoid polypeptide expression in a cell, thereby decreasing the amount of mahoganoid polypeptide in the subject's cells. In one embodiment, the subject is a mammal. In a further embodiment, the subject is a mouse. In a further embodiment, the subject is a human. In a further embodiment, the agent is the instant anti-sense nucleic acid.

[0098] This invention also provides a method for treating an overweight subject comprising administering to the subject a therapeutically effective amount of an agent that specifically inhibits mahoganoid polypeptide expression in a cell, thereby treating the subject. In a further embodiment, the agent is the instant anti-sense nucleic acid.

[0099] This invention also provides a method for inhibiting the onset of weight gain in a subject comprising administering to the subject a prophylactically effective amount of an agent that specifically inhibits mahoganoid polypeptide expression in a cell, thereby inhibiting the onset of weight gain in the subject. In a further embodiment, the agent is the instant anti-sense nucleic acid.

[0100] This invention also provides an article of manufacture comprising a packaging material having therein an agent that specifically inhibits mahoganoid polypeptide expression in a cell, and a label indicating a use for the agent in treating an overweight subject and/or inhibiting the onset of weight gain in a subject.

[0101] This invention also provides a method for determining whether an agent decreases mahoganoid polypeptide expression in a cell, which method comprises the steps of

[0102] (a) contacting the cell with the agent under suitable conditions;

[0103] (b) determining the amount of mahoganoid polypeptide expression in the cell after a suitable period of time; and

[0104] (c) comparing the amount of mahoganoid polypeptide expression determined in step (b) with the amount of mahoganoid polypeptide expression in a cell in the absence of the agent, whereby a lower amount of mahoganoid polypeptide expression in the cell contacted with the agent, relative to the amount of expression in the absence of the agent, indicates that the agent decreases mahoganoid polypeptide expression in the cell.

[0105] This invention also provides a method for determining whether an agent inhibits the ubiquitin ligase activity of mahoganoid polypeptide, which method comprises the steps of

[0106] (a) contacting mahoganoid polypeptide and ubiquitin with the agent under conditions which would permit mahoganoid polypeptide ubiquitin ligase activity in the absence of the agent;

[0107] (b) determining the amount of ubiquitin ligated after a suitable period of time; and

[0108] (c) comparing the amount of ligated ubiquitin determined in step (b) with the amount of ligated ubiquitin in the absence of the agent, whereby a lower amount of ligated ubiquitin in the presence of the agent, relative to the amount of ligated ubiquitin in the absence of the agent, indicates that the agent inhibits the ubiquitin ligase activity of mahoganoid polypeptide.

[0109] In one embodiment, a suitable period of time is within 4 days. In a second embodiment, a suitable period of time is within 2 days. In another embodiment, a suitable period of time is within 1 day. In further embodiments, a suitable period of time is within 12 hours or 6 hours.

[0110] This invention also provides a method for increasing the amount of mahoganoid polypeptide in a cell comprising contacting the cell with an agent that specifically increases mahoganoid polypeptide expression in the cell, thereby increasing the amount of mahoganoid polypeptide in the cell. In one embodiment, the cell is a mammalian cell. In a further embodiment, the cell is a mouse cell. In further embodiment, the cell is a human cell. In another embodiment, the cell is a neuron. In a further embodiment, the agent is the instant polypeptide or nucleic acid encoding same.

[0111] This invention also provides a method for increasing the amount of mahoganoid polypeptide in a subject comprising administering to the subject an agent that specifically increases mahoganoid polypeptide expression in a cell, thereby increasing the amount of mahoganoid polypeptide in the subject. In one embodiment, the subject is a mammal. In a further embodiment, the subject is a mouse. In further embodiment, the subject is a human. In a further embodiment, the agent is the instant polypeptide or nucleic acid encoding same.

[0112] This invention also provides a method for treating an underweight subject comprising administering to the subject a therapeutically effective amount of an agent that specifically increases mahoganoid polypeptide expression in a cell, thereby treating the subject. In a further embodiment, the agent is the instant polypeptide or nucleic acid encoding same.

[0113] This invention also provides a method for inhibiting the onset of weight loss in a subject comprising administering to the subject a prophylactically effective amount of an agent that specifically increases mahoganoid polypeptide expression in a cell, thereby inhibiting the onset of weight loss in the subject. In a further embodiment, the agent is the instant polypeptide or nucleic acid encoding same.

[0114] This invention also provides an article of manufacture comprising a packaging material having therein an agent that specifically increases mahoganoid polypeptide expression in a cell, and a label indicating a use for the agent in treating an underweight subject and/or inhibiting the onset of weight loss in a subject.

[0115] This invention also provides a method for determining whether an agent increases mahoganoid polypeptide expression in a cell, which method comprises the steps of

[0116] (a) contacting the cell with the agent under suitable conditions;

[0117] (b) determining the amount of mahoganoid polypeptide expression in the cell after a suitable period of time; and

[0118] (c) comparing the amount of mahoganoid polypeptide expression determined in step (b) with the amount of mahoganoid polypeptide expression in a cell in the absence of the agent, whereby a higher amount of mahoganoid polypeptide expression in the cell contacted with the agent, relative to the amount of expression in the absence of the agent, indicates that the agent increases the amount of mahoganoid polypeptide expression in the cell.

[0119] This invention also provides a method for determining whether an agent increases the ubiquitin ligase activity of mahoganoid polypeptide, which method comprises the steps of

[0120] (a) contacting mahoganoid polypeptide and ubiquitin with the agent under conditions which would permit mahoganoid polypeptide ubiquitin ligase activity in the absence of the agent;

[0121] (b) determining the amount of ligated ubiquitin after a suitable period of time; and

[0122] (c) comparing the amount of ligated ubiquitin determined in step (b) with the amount of ligated ubiquitin in the absence of the agent, whereby a higher amount of ligated ubiquitin in the presence of the agent, relative to the amount of ligated ubiquitin in the absence of the agent, indicates that the agent increases the ubiquitin ligase activity of mahoganoid polypeptide.

[0123] This invention also provides a method for treating a subject suffering from spongiform degeneration (40) comprising administering to the subject a therapeutically effective amount of an agent that specifically increases mahoganoid polypeptide expression in a cell, thereby treating the subject.

[0124] Finally, this invention provides an article of manufacture comprising a packaging material having therein an agent that specifically increases mahoganoid polypeptide expression in a cell, and a label indicating a use for the agent in treating a subject suffering from spongiform degeneration.

[0125] Determining a therapeutically or prophylactically effective amount of the instant polypeptide and nucleic acids can be done based on animal data using routine computational methods. In one embodiment, the therapeutically or prophylactically effective amount contains between about 0.1 mg and about 1 g of nucleic acid or polypeptide, as applicable. In another embodiment, the effective amount contains between about 1 mg and about 100 mg of nucleic acid or polypeptide, as applicable. In a further embodiment, the effective amount contains between about 10 mg and about 50 mg of the nucleic acid or polypeptide, as applicable.

[0126] This invention will be better understood from the Experimental Details that follow. However, one skilled in the art will readily appreciate that the specific methods and results discussed are merely illustrative of the invention as described more fully in the claims which follow thereafter.

Experimental Details

[0127] Synopsis

[0128] Here we report the positional cloning of the mouse mahoganoid through a combination of genetic mapping and bioinformatics approaches.

[0129] Methods

[0130] Animals. N7F14 B6.C3H-md-A (md/md and md/+) mice were obtained from the Jackson Laboratory (Bar Harbor, Me.). The coat color effect of the mutation is easiest to detect on an agouti (A) coat (FIG. 2); hence these animals have been selected and bred for phenotypes at 2 loci on different chromosomes (md and A). Progeny for genetic mapping of the region around md were generated by mating md/md A/?×md/+ A/? animals of this congenic strain. The fact that this line was maintained by coat color selection offered the opportunity to map, and reduce by meiotic recombination, the C3H genetic interval containing the md locus. Mice were housed in a barrier facility under pathogen-free conditions with a 12 hour light/dark cycle. Mice were weaned at 21 days and were then given ad libitum access to 9% kcal fat Picolab Rodent Chow 20 (Purina Mills, Richmond, Ind.) or to 45% kcal fat D12451 (Research Diets, Inc., New Brunswick, N.J.). Mice were fasted for 2 hours prior to sacrifice by CO2 asphyxiation at 105-120 days of age. Weight and nasoanal body length were measured. The kidneys were removed and immediately frozen at −80° C. for subsequent isolation of genomic DNA. Other mice used were: B6.V-Lepob (N30), B6.Cg-Ay (N66), C57BL/6J (F217), C3H/HeJ (F243), and C3H/HeJ-md2J (N2). All were obtained from the Jackson Laboratory.

[0131] Microsatellite Genotyping. Genomic DNA was made from tail tips clipped at weaning using QIAamp Tissue Kit (Qiagen Inc, Valencia, Calif.). Mice were genotyped for Whitehead Institute microsatellites in the region of md (http://www-genome.wi.mit.edu/cgi-bin/mouse/gmap) by polymerase chain reaction (PCR) amplification. D16Mit182, D16Mit107, D16Mit154, D16Mit130, D16Mit129, D16Mit54, D16Mit159, D16Mit122, and D16Mit81 were scored using primers obtained from Research Genetics (Huntsville, Ala.). PCR conditions consisted of 40 cycles of denaturation at 94° C. for 30 sec, annealing at 55° C. for 30 sec, and extension at 72° C. for 45 sec. PCR fragments were resolved on 6% denaturing polyacrylamide gels.

[0132] Genetic and Physical Mapping. One hundred forty-nine progeny of an N7F14 B6.C3H-md/md A/?×N7F14 B6.C3H-md/+ A/? cross were used for genetic mapping of mahoganoid. Homozygosity for md was scored by observation of coat color (FIG. 2). Homozygosity for md results in a darkening of the agouti coat color (umbrous); md/+ mice have an agouti coat color. Initially, the congenic C3H interval containing md was defined by scoring congenic B6.C3H-md/md A/? mice with microsatellite markers on proximal chromosome 16 for B6 and C3H alleles. Next, all 149 progeny were scored for D16Mit182, D16Mit107, D16Mit154, D16Mit130, D16Mit129, D16Mit54, D16Mit159, D16Mit122, and D16Mit81 to identify recombinant md/md animals with B6/C3H heterozygous genotypes and md/+ animals with C3H/C3H homozygous genotypes. Once the minimal genetic interval was defined, all expressed sequence tags (ESTs) within the interval were obtained from the Whitehead radiation hybrid (RH) map (http://www-genome.wi.mit.edu/mouse_rh/rh_maps/Chr16.txt). Mouse and corresponding human genomic clones were identified through nBlast of ESTs and mouse microsatellite markers to online sources (http://www.ncbi.nlm.nih.gov, http://www.celera.com, http://www.genome.ucsc.edu, http://www. ensembl.org, and http://www.informatics.jax.org). Mouse genomic clones were used to search these databases to construct a complete 2.5 Mb contig of mouse BAC clones [http://genomics.roswellpark.org/cgi-bin/mouse/markers.cgi? chr=16] spanning the minimal interval containing md. All transcripts in the interval were identified using Celera and NCBI databases.

[0133] Sequence Analysis of Positional Candidate Genes. To screen for mutations in the coding sequences of the transcripts and predicted genes mapping to the minimal contig, each of the exons was amplified from genomic DNA by PCR followed by amplicon purification by QIAquick Gel Extraction Kit (Qiagen Inc, Valencia, Calif.) and bidirectional fluorescent dideoxy termination sequencing (20). This process was prioritized so that the known transcripts were screened before the predicted genes. Sequences from C3H/HeJ +/+ and C3H/HeJ md2J/md2J [coisogenic on C3H/HeJ] were compared using Sequencher software 4.0.5 (Gene Codes Corp, Ann Arbor, Mich.).

[0134] Southern Blot Analysis. Genomic DNA of affected md, md2J, md4J, md5J, and md6J obtained from the Jackson Laboratory was analyzed by Southern blot analysis (21) using restriction enzymes Pst I, EcoR I, Hind III, Sau3AI, Msp I, and Bgl II (Roche, Ridgefield, Conn.). Restriction fragments were separated by electrophoresis on 0.7% agarose gels, transferred by capillary action to a nylon membrane (Schleicher & Schuell Inc., Keene, N.H.), prehybridized (Ultrahyb; Ambion Inc., Woodward, Tex.), and hybridized using a random-primed 32P-labeled C3H/HeJ genomic PCR-amplified fragment prepared using the following primers: Probe 1, F: 5′-GATGGGGCTTGAGTCCTTAGA-3′, R: 5′-CCTCAGCCCAGCACTTTCTCT-3′ flanking exon 12 of Riken full-length cDNA AK011747 (shown by mutation analysis to contain the md gene, see below); and Probe 2, F: 5′-GGCAGGTGGGAACAGATGAGT-3′, R: 5′-CCGTCCGAGATGCCTGAGTAG-3′, spanning the intronic region between exon 11 and exon 12. Two cDNA probes (Probes 3 and 4) spanning, respectively, exons 2-9 and exons 3-13 of AK011747, were prepared from pooled C57BL/6J cDNA obtained from liver, kidneys, lungs, spleen, brain, adipose, pancreas, and heart cDNA using the following primers: Probe 3, F: 5′-TTGACACTCCCCATCCTGAAG-3′, R: 5′-TCCTGGTTGTTCTTGTTCTCG-3′, and Probe 4, F: 5′-CCAGTTTCCCTATGTCACCCC-3′, R: 5′-ATGGATGGGGAATGATGGAGA-3′. The blots were washed in 1×SSC/0.1% SDS twice for 10 minutes at room temperature and twice for 30 minutes at 64° C. and exposed to X-ray film (RX-B; Denville, Metuchen, N.J.) at −80° C. for 48 hrs.

[0135] Northern Blot Analysis. Northern blots of liver, heart, kidney, lung, skin, skeletal muscle, adipose, and brain tissue were performed using standard techniques (21). Total RNA was extracted using a commercial kit (Trizol; Invitrogen, Carlsbad, Calif.) and size fractionated on a 1% agarose formaldehyde gel. Blot handling was as for Southern blots. Only probe 4 was used for Northern hybridizations.

[0136] Real time RT-PCR. RNA was extracted from flash-frozen, freshly dissected whole organs using a commercial kit (Trizol; Invitrogen, Carlsbad, Calif.) and purified using RNeasy Mini kits (Qiagen Inc., Valencia, Calif.). cDNA was then made using SuperScript First-Strand Synthesis System for RT-PCR (Invitrogen, Carlsbad, Calif.) with 50 ng of random hexamers for each mg of total RNA. A negative control for cDNA was made in an identical manner without adding the SuperScript II RT to each tube. cDNA was diluted five-fold prior to use. A LightCycler (Roche, Mannheim, Germany) was used to quantify expression levels with 20 μl reactions consisting of 2 μl diluted cDNA, 16 μl FastStart DNA Master SYBR Green I mix (Roche, Mannheim, Germany) and 2 μl of primers (F: 5′-TGTCTCCCATCTCCTTCAGCC-3′; R: 5′-CTGTGTCTTGCCCTTCTGTAG-3′) spanning exon 11-12 of Riken cDNA AK011747. Each sample was run in triplicate with one negative control. β-actin (F: 5′-ATCGCTGCGCTGGTCGTC-3′; R: 5′-GCTCTGGGCCTCGTCACC-3′) was used to normalize expression levels. Only one product was seen on the melting curves, so fluorescent acquisition was set at the extension stage. Relative expression levels were found by comparing expression levels in each organ to the level found in +/+ C57BL/6J mice in the same organ (22). PCR fragments were resolved on 2% agarose gel.

[0137] Generating Restriction Maps of md Genomic Sequence. Ensembl gene ENSMUSG00000022517, containing the complete genomic sequence of md, was identified through nBlast of transcript AK011747 into genomic DNA database Ensembl (Ensembl, Cambridge, United Kingdom). The genomic sequence obtained was used as a control template in creating the restriction map for the md. Sequencher software 4.0.5 (Gene Codes Corp, Ann Arbor, Mich.) was used on both the normal and inserted retroviral sequences to determine the restriction sites and fragment sizes for specific restriction enzymes.

[0138] Neuropathology. Fifteen week old C3H.B6 md/md A/? and C57BL/6J +/+ male and female mice were sacrificed by CO2 asphyxiation, and the whole brain fixed overnight in 3.7% paraformaldehyde in phosphate buffered saline. One year old C3H.B6 md/md A/? male and female mice were also examined. Serial paraffin sections including cortex, hippocampus, pons, thalamus, cerebellum, brain stem, midbrain and hypothalamus were cut and stained with hematoxylin and eosin (23). These sections were examined by light microscopy by Dr. James Goldman (Department of Pathology, Columbia University).

[0139] Body Weight and Length. To assess the effects of md on energy homeostasis, at sacrifice at 105-120 days, body weight and nasoanal length were measured in male and female md/+ and md/md animals that had ingested 9% or 45% kcal fat diets since weaning at about 21 days of age.

[0140] Results

[0141] By genotyping congenic B6.C3H-md/md A/? mice for microsatellite genetic markers polymorphic between C57BL/6J and C3H/HeJ, the maximal congenic C3H/HeJ interval was determined to extend approximately 6.9 cM from the centromere to D16Mit181 (FIG. 3). Genetic mapping of 149 progeny of a B6.C3H-md/+ A/?×B6.C3H-md/md A/? intercross, in which genotype for md was assigned by coat color, identified a double recombination event in the C3H congenic interval between markers D16Mit122/D16Mit159 distally and markers D16Mit54/D16Mit129 proximally. Similarly, there was a single md/md mouse with a recombination between D16Mit54/D16Mit129 and D16Mit130/D16Mit154/D16Mit107/D16Mit182, narrowing the interval containing md to a region of approximately 4.0 cM proximal to D16Mit54/D16Mit129 (FIG. 3).

[0142] Using sequence databases at NCBI, Celera, Ensembl, Jackson Laboratory, and UCSC (see Methods for URL information), all mouse genomic clones in the 2.5 Mb interval containing md proximal to D16Mit129 and D16Mit54 were identified (FIG. 4). Twenty-nine transcripts and 39 computationally-predicted genes (24) were identified. Using nBlast, transcripts were compared against the Ensembl mouse cDNA database to obtain genomic sequences with exon predictions. These genes were then systematically analyzed as indicated below. The coding regions of 27 of the 29 known transcripts, excluding X94084 and AK004765, were systematically sequenced in md2J and coisogenic C3H/HeJ +/+ animals. By virtue of the disruptions described below in md2J and other members of the mahoganoid allelic series, Riken cDNA AK011747 was implicated as the mahoganoid transcript. md2J, an 8 kb retroviral insertion within exon 12. Each of the predicted coding sequences of ESTs, known genes, and computationally predicted genes in the minimum physical interval for mahoganoid were amplified from genomic DNA of an mu2J/md2J mouse and a co-isogenic non mutant animal using intronic primers flanking the known or predicted exons in the interval. For the Riken cDNA clone AK011747, all exons except exon 12 were amplified from both the md2J/md2J and C3H/HeJ +/+. For exon 12, the normal 589 bp C3H/HeJ allele could be amplified in the +/+ as well as all of the md alleles except md2J (FIG. 5A). PCR amplification and subsequent bidirectional sequencing of predicted coding exons 2-16 from homozygous affected md, md2J, md4J, md5J and md6J mice demonstrated normal genomic sequence. Southern blot analysis of md2J/md2J animals restricted with Pst I, using probe 2, that contained part of exon 12 and its 5′ intronic region, showed a novel 0.7 kb fragment in the md2J/md2J animal compared with a 1.4 kb fragment corresponding to exon 12 in the C3H/HeJ co-isogenic +/+ control and in mahoganoid alleles (md, md4J, md5J, md6J) (FIG. 5B). The region of probe 2 containing part of exon 12 and its 5′ intronic region was then amplified and sequenced from genomic DNA and demonstrated an ˜8 kb insertion in exon 12 of md2J (data not shown). The fragment was shown by sequence analysis to be a retroviral insertion (GenBank: AF532997, AF532998) containing a Pst I restriction site (FIG. 6).

[0143] md5J, a 5 kb retroviral insertion in the intron 3′ of exon 2. Southern blot analysis of md5J DNA restricted with HindIII (but not PstI, EcoRI, BglII, or Sau3AI), and probed with a cDNA corresponding to exons 2-9, demonstrated a different restriction pattern than the C3H/HeJ co-isogenic +/+ control and the other md alleles (FIG. 5C). The md5J DNA showed loss of an 8.8 kb fragment corresponding to the region of exons 2-4 and introduction of new 5.2 kb and 4.0 kb fragments. Similar results were obtained with a cDNA probe spanning exons 3-5 (data not shown). PCR amplification of genomic md5J DNA corresponding to the intronic region between exon 2 and exon 3 demonstrated a fragment ˜5 kb larger than the C3H/HeJ co-isogenic +/+ control (data not shown). Sequence analysis showed that md5J is a retroviral insertion (GenBank: AF532995, AF532996) of ˜5 kb in the intronic region 3′ of exon 2 (FIG. 6).

[0144] md, a 5kb retroviral insertion in the intron between exons 11-12. Southern blot analysis of a PstI digest of md using probe 2 demonstrated a missing fragment of 1.1 kb and the presence of a new fragment of 0.6 kb corresponding to the intronic region 5′ of exon 12 (FIG. 5B). PCR amplification in md genomic DNA of the intron between exons 11 and 12 demonstrated a fragment ˜5 kb larger than the C3H/HeJ co-isogenic +/+, suggesting that the md mutation is due to an insertion in this intron (data not shown). Sequence analysis of the PCR-amplified genomic DNA between exons 11 and 12 showed an inserted retroviral sequence (GenBank: AF532993, AF532994) within the intron (FIG. 6).

[0145] The insertions are intracisternal type A particle elements. Comparison of the 5′ and 3′ regions of the insertions detected in md, md2J, and md5J with GenBank entries revealed that the insertion is a mouse retrovirus-like repetitive intracisternal type A particle (IAP) element matching GenBank X04120. The IAP seen in the mahoganoid mutations reported here is similar to the element reported in mahogany (Atrnmg and Atrnmg-L) (12). The integrated IAP elements associated with the md mutations were flanked in all instances with canonical long terminal repeat (LTR) sequences that are frequently observed in contiguous to retroviral IAP insertions (25).

[0146] Expression of mahoganoid alleles. Northern blot analysis, using probe 5 that spans exons 3-13 containing the RING (really interesting new gene) finger domain in exon 10, demonstrated a 3.9 kb mahoganoid transcript expressed in kidney, brain, heart, spleen, lung, skin, skeletal muscle, and adipose tissue in B6.V-Lepop, B6.Cg- Ay, and C57BL/6J +/+ mice (FIG. 7A). An additional transcript of 5.2 kb was also seen in the kidney, brain, and liver; and a transcript of 1.9 kb in the kidney of C57BL/6J +/+, B6.V-Lepob, and B6.Cg- Ay mice (FIG. 7A). Both were at lower levels of expression than the 3.9 kb transcript. Expression levels of the 3.9 kb and 5.2 kb transcripts were 10- to 20-fold lower in the md/md and md2J/md2J animals. Additionally, several aberrantly sized transcripts of 5.9, 5.5, 4.1, and 2.2 kb were observed in md/md animals, and 12.0 kb and 3.6 kb transcripts in md2J/md2J (FIG. 7B). The aberrantly sized transcripts were not sequenced.

[0147] Using NCBI and Ensembl databases, KIAA0544 was identified as the human homolog of md. Like md, KIAA0544 is predicted to have 17 exons with a RING finger domain located in exon 10. NCBI Aceview analysis (http://www.ncbi.nih.gov/IEB/Research/Acembly/av.cgi?db=28&1=Hs16—10709—29—1_t16_Hs16—10709—29—2—5347.a) of KIAA0544 showed that the human homolog of md is defined by 139 sequences from 129 cDNA clones and produces, by alternative splicing, 6 mRNAs of variant a, 4.1 kb; variant b, 3.9 kb; variant c, 5.2 kb; variant d, 1.9 kb; variant e, 2.4 kb; and variant f, 2.2 kb. Using probe 4, which spans exons 3-13, only md transcripts of 3.9 kb, 5.2 kb, and 1.9 kb were detected in Northern blots. These transcripts are similar in size to human transcripts b, c, and d. The human 5.2 kb transcript is alternatively spliced to incorporate an additional 66-bp exon between exons 11 and 12 of the 3.9 kb transcript as well as to use an alternative splice site for the final exon. Further blast analysis of md transcript AK011747 in the TIGR Mouse (Mus musculus) gene index (MGI) (http://www.tigr.org/tigr-scripts/tgi/tc_report.pl?species=mouse&tc=TC457132) identified mouse EST TC457132 that corresponds to the human 5.2 kb transcript. An expression profile of KIAA0544 in 14 different tissues (heart, brain, placenta, lung, liver, skeletal muscle, kidney, pancreas, spleen, thymus, prostate, testis, ovary, and small intestine) generated by RT-PCR, indicates that the human homolog has a similar expression pattern as mahoganoid in the mouse (26).

[0148] By quantitative RT-PCR using primers spanning exons 11-12, mahoganoid expression levels relative to actin were found to be similar in the brain and kidney among genetically obese Lepop/Lepop and Ay/+ mice and C57BL/6J +/+ controls (Table 1).

1TABLE 1Expression levels of mahoganoid by quantitative RT-PCRRelative Expression LevelKidneysBrainB6.V-Lepob0.7601.15B6.Cg-Ay0.9931.10C57BL/6J11B6.C3H-md-A0.09500.0501C3H/HeJ md2J0.05980.0144

[0149] However, mahoganoid expression in the brain of md/md and md2J/md2J animals relative to actin was 5% and 1% of that of C57BL/6J +/+ controls (Table 1). The probe spanning exons 11-12 detects both the 3.9 kb and 5.2 kb transcripts. The quantitative RT-PCR results are consistent with the very low expression levels for these transcripts seen in the Northern blots of md and md2J RNA.

[0150] Mahoganoid does not suppress obesity related to a high fat diet. The dose-dependent effect of md in diminishing the obesity of Ay mice is striking and clear (17). The effect of this mutation on body composition in circumstances in which the gene is not in epistatic apposition to an obesity mutation is reportedly more subtle (17). We examined this issue by estimating the mouse equivalent of the body mass index (BMI; weight in grams/nasoanal length in cm2) (27) in progeny of the N7F14 B6.C3H-md-A md/md×md/+ intercross used for mapping and minimizing the C3H interval containing the md locus. The progeny were fed from the time of weaning at about 21 days with mouse chow containing either 9% or 45% Kcal fat. Body weight and nasoanal length were measured every 2 weeks and the animals were sacrificed at about 115 days when weight and nasoanal length were measured. BMI was used as a surrogate measure for adiposity (27). As expected, animals fed 45% Kcal as fat were heavier and had higher BMI than those fed 9% fat. However, no effect of md genotype was seen on body weight or BMI of animals fed either the 9% or 45% Kcal fat chow (Table 2).

2TABLE 2BMI* and Weight in progeny of the N7F14 B6.C3H-md-A md/md ×md/+ intercross on 9% or 45% fat diet [mean value (SD)]BMIWeight (gm)Age (days)N 9% fat dietFemalemd/+.276 (.019)24.8 (2.7)108.1 (1.8)15md/md.276 (.029)24.8 (3.0)107.9 (1.5)15Malemd/+.329 (.026)33.7 (1.9)109.2 (1.9)21md/md.322 (.024)33.9 (2.1)107.7 (0.9)2245% fat dietFemalemd/+.344 (.046)30.1 (5.6)114.1 (2.1) 8md/md.325 (.042)29.0 (5.2)113.8 (2.2)16Malemd/+.402 (.040)40.6 (4.0)114.6 (1.6)14md/md.391 (.050)39.8 (4.9)114.0 (1.1)13*Weight (grams)/naso-anal length (cm2)

[0151] No significant diet-by-genotype interaction was seen for either BMI or body weight by ANOVA (Table 3).

3TABLE 3ANOVA for effects of md on body weight and BMI ANOVA fordiet and genotype effectsEffectFp-valueDependentSex72.06<0.0001BMI223.30<0.0001WeightDiet (9% or 45% fat)10.340.002BMI0.340.56WeightGenotype at md0.940.34BMI0.050.83WeightSex/Diet (interaction)0.950.33BMI1.730.19WeightSex/Genotype (interaction)0.120.73BMI0.530.47WeightDiet/Genotype (interaction)0.960.33BMI1.180.28WeightSex/Diet/Genotype (interaction)0.150.70BMI0.070.79Weight

[0152] It is important to note that we looked only at md/+ and md/md animals in this analysis because these were the only genotypes issuing from the md/+×md/md mapping cross.

[0153] Absence of a neurological phenotype in md/md mice. Md/md animals are neurologically normal at 15 weeks and at 1 year of age, without obvious tremor or movement disorder. Gross and microscopic examination of the midbrain, cerebellum, pons, hippocampus, hypothalamus, thalamus, cortex and brainstem demonstrated normal anatomy with no evidence of vacuolization or dysmyelination as is observed in the mahogany mouse (data not shown).

[0154] Mahoganoid encodes a 494 amino acid protein containing a C3HC4 RING domain from amino acids 240-278 (FIG. 8). The human homologue, KIAA0544 (http://www.ncbi.nlm.nih.gov/LocusLink/LocRpt.cgi?l=76564), maps to 16p13.3 and is 81% identical in amino acid sequence. The RING finger domain of KIAA0544 is 99% identical to mahoganoid C3HC4 RING domain. There are homologous genes in D. melanogaster and C. elegans with 43% and 37% identity of amino acids, respectively, that include the highly conserved C3HC4 RING domains (FIG. 8).

[0155] Discussion

[0156] Coat color mutations in mice have provided unique insights into the molecular physiology of melanocortin-related control of coat color and energy homeostasis in mice and other mammals (28). Remarkably similar (sometimes identical) pathways/molecules are involved in these disparate phenotypes. G-protein-coupled melanocortin receptors (MC1R in skin, MC3R and MC4R in brain) mediate the effects of the physiologic ligand, α-MSH, and antagonists, ASP and AgRP (FIG. 1). Binding of a MSH to MC1R in the hair follicle, or to MC3R and MC4R in the hypothalamus, increases intracellular cAMP and increases the production of eumelanin in the hair follicle or decreases food intake by effects in the hypothalamus. Conversely, antagonism of MC1R by ASP in the hair follicle, or of MC4R by AgRP in the hypothalamus, produces increased pheomelanin in the hair follicle and increased food intake by effects in the hypothalamus. Constitutive overexpression of ASP in the Ay mouse outside of the hair follicle best demonstrates the analogies between the two pathways since the yellow coat color of these mice is due to ASP antagonism of MC1R and the increased weight and adiposity is due to ASP antagonism of MC3R and MC4R in the hypothalamus (28). Other genes, such as mahogany and mahoganoid, modulate the activity of this pathway in skin and the brain (17). Here we present evidence that the mahoganoid allelic series is due to mutations in a RING finger protein whose function is unknown but that has a strong impact on the melanocortin signaling. Mutations in the mahoganoid allelic series (md, md2J and md5J) are due to large retroviral insertions that disrupt the expression of md. Retroviral insertions have been shown to affect gene expression in other coat color mutations such as dilute (29), agouti (2), and mahogany (10). Tissue expression data indicate that md is ubiquitously expressed with highest expression in the brain and kidney. Expression of normal mahoganoid transcripts is greatly reduced in md/md and md2J/md2J mice in all tissues examined by both Northern blot analysis and quantitative RT-PCR. The ability to identify md was greatly expedited by the availability of near complete human and mouse genomic sequence and annotation.

[0157] Mutations of md in mice act as suppressors of obesity and yellow coat color that are associated with constitutive overexpression of Asp in the Ay mouse, but do not alter the yellow coat color phenotype of Mc1re deficient mice (extension mutants) (17). Genetically, mutations in md are epistatic to Ay and Mc1re is epistatic to md, suggesting that mahoganoid is functionally distal to ASP and proximal to MC1R (FIG. 1). The epistatic relationship appears to be similar in the hair follicle and the hypothalamus since mahoganoid is able to suppress both the yellow coat color phenotype induced by constitutive ASP antagonism of MC1R as well as to suppress the obesity induced by ASP antagonism of MC3R and MC4R (17). Furthermore, these mutations of mahoganoid appear to be loss-of-function alleles because the phenotypes of the various alleles are all similar, and because mutations in the md and md2J alleles result in loss of normal gene expression in all tissues examined (FIG. 7). On the basis of similarities between the ASP/MC1R and AgRP/MC3R/MC4R pathways, we suggest that the normal mahoganoid allele acts through a similar mechanism in the hair follicle and hypothalamus, decreasing signaling through MC1R and MC3R/MC4R to produce increased pheomelanin production and increased body weight, respectively.

[0158] Both mg and md show epistatic effects on Ay coat color and adiposity. Mahogany and mahoganoid have similar effects on coat color, but it is not yet clear if the mechanisms by which they confer their effects on body mass are similar. When expressed on an agouti (A/A or A/a) coat, mahogany mice have darker coat color than md (17). Mahogany fully suppresses Ay obesity, while md rescues about 80% of the Ay obesity phenotype (1). Atrnmg/Atrnmg mice are leaner than +/+ mice of the same strain and have approximately 20% higher levels of energy expenditure by indirect calorimetry, possibly secondary to the muscle tremors attributable to the associated spongy degeneration in the central nervous system (14). The effects of mg and md on body weight in non-obese animals are much more subtle. Barsh reported that female A/A md/md animals fed standard lab chow were heavier than md/+ or +/+ animals at 12-40 weeks (17); we did not see this effect in our ˜115 day old male and female animals fed 9% or 45% fat chow (Table 2). Atrnmg is due to deficiency of attractin, a transmembrane protein with binding specificity for ASP but not AgRP. Attractin is thought to act by localizing ASP to MC1R (10). Atrnmg specifically and fully suppresses obesity due to widespread overexpression of Asp in the Ay mouse, possibly by virtue of loss of the ability to keep ASP in proximity to MC3R/MC4R in the hypothalamus and/or by virtue of the tremors caused by neurodegeneration (14). In comparison, mahoganoid mice (MD allele) have no obvious neurological, behavioral, gross or microscopic central nervous system anatomic phenotype. However, other alleles of mahoganoid (e.g. mdnc) have been shown to have neurologic and neuroanatomic phenotype (40). The quantity of Atrn expression in the various mg alleles parallels the effects of the mg alleles on pigmentation and neurodegeneration, with the Atrnmg-3J allele showing the lowest Atrn expression and having the most significant effects on coat color and neurodegeneration, while the Atrnmg-L allele conversely shows the highest Atrn expression and mildest phenotype (12).

[0159] The primary impact of mahoganoid on energy homeostasis is apparently via the melanocortin-signaling pathway(s) in the brain. This effect is clearest when amplified by overexpressing ASP in the brain (as in the Ay animal). This situation is reminiscent of what is seen in the neuropeptide Y (Npy) knockout mouse, where despite a profound effect of the protein on food intake and energy metabolism, knockout of the gene does not have much effect on food intake or body composition of the knockout animal (30). However, Npy−/− substantially reduces the obesity of Lepob/Lepop mice (30). Additional studies of energy intake, energy expenditure and body composition will be required to assess the effects of md on energy homeostasis.

[0160] Mahoganoid is a ubiquitously expressed protein with a C3HC4 RING finger domain that is similar to the RING finger domain of the proto-oncogene c-Cbl. The RING finger, an evolutionarily conserved cysteine/histidine residue containing motif, Cys-X2-Cys-X9-39-Cys-X1-3-His-X2-3-Cys/His-X2-Cys-X4-48-Cys-X2-Cys (31), identified in more than 200 proteins, is a small zinc-binding domain often found in subunits of multiprotein complexes (32). The RING finger binds two zinc atoms in a unique “cross-brace” system. RING fingers are located close to amino or carboxyl termini of proteins and may be associated with other domains to form larger conserved motifs like the RING finger-B box-a-helical coiled-coil (RBCC) motif (31). The RING domain is a common structural element in a superfamily of E3 ubiquitin ligase complexes: e.g., SCF (Skp1-Cdc53/CUL1-F-box protein) family, APC (anaphase-promoting complex) family, c-Cbl and MDM2 proto-oncogene, and members of the IAP family of antiapoptotic proteins (33). Based on protein sequence homology to E3 RING domain ubiquitin ligases, mahoganoid may itself function as an E3 ubiquitin ligase (34).

[0161] Ubiquitylation involves conjugation of proteins with the highly conserved 76-amino acid protein, ubiquitin. The process targets proteins for degradation in the proteosome, vacuoles, or lysosomes, or regulates cellular processes through translational control, protein kinase activation, or transcriptional regulation (35, 36). The specificity of the ubiquitylation process is conferred by the E3 ubiquitin ligase, of which there are many (36). Ubiquitylation has been implicated in the regulation of myriad cellular processes including cell cycling, apoptosis, cellular differentiation, DNA repair, and stress responses. Inherited loss-of-function mutations in other E3 ubiquitin ligase genes have been implicated in juvenile Parkinson disease, Angelman syndrome, breast and ovarian cancer susceptibility (BRCA1), and von Hippel Lindau disease (37). Ubiquitylation proceeds through a three-step process, involving ubiquitin-activating (E1), ubiquitin-conjugating (E2), and ubiquitin-ligating (E3) enzymes. The E3 enzymes mediate the transfer of ubiquitin from the E2 to the substrate, and thereby confer substrate specificity (34).

[0162] The mahoganoid protein may decrease signaling through MC1R and MC3R/MC4R by increasing expression or activity of an inverse agonist of MC1R and MC3R/MC4R, influencing the physical proximity or binding of ASP and AgRP to their receptors by influencing binding of ATRN to ASP or by decreasing the amount of α-MSH available to MC1R or MC3R/MC4R through sequestration or turnover of α-MSH (FIG. 9). If mahoganoid is an E3 ligase, identification of the targets of mahoganoid ubiquitylation should define additional components of this system. In this context, it should be noted that knockout mice lacking E3 ubiquitin ligase UBR1 activity have decreased body weight due to reduction in both skeletal muscle and adipose tissues (38). This phenotype supports a role for the E3 ligase in regulating body mass and composition.

[0163] The human homolog of mahoganoid maps to 16p13.3. Loci for coronary heart disease, hypertension, and type 2 diabetes have been mapped to this region in Indo-Mauritians and Pondicherian families of Indian origin (39). These phenotypes could be related to allelic variation in mahoganoid. This possibility can now be tested by mutation analysis and association studies.

References

[0164] 1. Leibel, R. L., Chung, W. K. and Chua, S. C. J. (1997). The molecular genetics of rodent single gene obesities. J Biol Chem. 272:31937-31940.

[0165] 2. Bultman, S. J., Michaud, E. J. and Woychik, R. P. (1992). Molecular characterization of the mouse agouti locus. Cell 71:1195-1204.

[0166] 3. Miller, M. W., Duhl, D. M., Vrieling, H., Cordes, S. P., Ollmann, M. M., Winkes, B. M. and Barsch, G. S. (1993). Cloning of the mouse agouti gene predicts a secreted protein ubiquitously expressed in mice carrying the lethal yellow mutation. Genes Dev. 7:454-467.

[0167] 4. Michaud, E. J., Bultman, S. J., Klebig, M. L., van Bugt, M. J., Stubbs, L. J., Russell, L. B. and Woychik, R. P. (1994). A Molecular Model for the Genetic and Phenotypic Characteristics of the Mouse Lethal Yellow (Ay) Mutation. Proc Natl Acad Sci USA. 91:2562-2566.

[0168] 5. Wolff, G. L., Galbraith, D. B., Domon, O. E. and Row, J. M. (1978). Phaeomelanin synthesis and obesity in mice. Interaction of the viable yellow (Avy) and sombre (eso) mutations. J Hered. 69:295-298.

[0169] 6. Nijenhuis, W., Oosterom, J. and Adan, R. (2001). AgRP(83-132) acts as an inverse agonist on the human melanocortin-4 receptor. Molecular Endocrinology 15:164-171.

[0170] 7. Haskell-Luevano, C. and Monck, E. K. (2001). Agouti-related protein functions as an inverse agonist as a constitutively active brain melanocortin-4 receptor. Regulatory Peptides 99:1-7.

[0171] 8. Ollmann, M. M., Wilson, B. D.-, Yang, Y. K., Kerns, J. A., Chen, Y., Gantz, I. and Barsh, G. S. (1997). Antagonism of central melanocortin receptors in vitro and in vivo by agouti-related protein. Science 278:135-138.

[0172] 9. Nagle, D. L., McGrail, S. H., Vitale, J., Woolf, E. A., Dussault, B. J. J., DiRocco, L., Holmgren, L., Montagno, J., Bork, P., Huszar, D., et al. (1999). The mahogany protein is a receptor involved in suppression of obesity. Nature 398:148-152.

[0173] 10. Gunn, T. M., Miller, K. A., He, L., Hyman, R. W., Davis, R. W., Azarani, A., Schlossman, S. F., Duke-Cohan, J. S. and Barsh, G. S. (1999). The mouse mahogany locus encodes a transmembrane form of human attractin. Nature 398:152-156.

[0174] 11. Dinulescu, D. M., Fan, W., Boston, B. A., McCall, K., Lamoreux, M. L., Moore, K. J., Montagno, J. and Cone, R. D. (1998). Mahogany (mg) stimulates feeding and increases basal metabolic rate independent of its suppression of agouti. Proc Natl Acad Sci USA 95:12707-12712.

[0175] 12. Gunn, T., Inui, T., Kitada, K., Ito, K., Wakamtsu, K., He, L., Bouley, D. M., Serikawa, T. and Barsch, G. S. (2001). Molecular and phenotypic Analysis of Attractin Mutant mice. Genetics 158:1683-1695.

[0176] 13. Kuramoto, T., Kitada, K., Inui, I., Sasaki, Y. and Ito, K. (2001). Attractin/Mahogany/Zitter plays a critical role in myelination of the central nervous system. Proc Natl Acad Sci USA 98:559-564.

[0177] 14. He, L., Gunn, T. M., Bouley, D. M., Lu, X. Y., Watson, S. J., Schlossman, S. F., Duke-Cohan, J. S. and Barsh, G. S. (2001). A biochemical function for attractin in agouti-induced pigmentation and obesity. Nat Genet. 27:40-47.

[0178] 15. Lane, P. W. (1960). New mutants. Mouse News Lett. 22: 35.

[0179] 16. Lane, P. W. and Green, M. C. (1960). Mahogany, a recessive color mutation in linkage group V of the mouse. J. Hered. 51:228-230.

[0180] 17. Miller, K. A., Gunn, T. M., Carrasquillo, M. M., Lamoreux, M. L., Galbraith, D. B. and Barsh, G. S. (1997). Genetic studies of the mouse mutations mahogany and mahoganoid. Genetics. 146:1407-1415.

[0181] 18. Green, M. C. (1989). Genetic Variants and Strains of the Laboratory Mouse. Oxford, Oxford Unviersity Press.

[0182] 19. Roderick, T., Davisson, M. and Lane, P. (1976). Chromosome 16 and mahoganoid md. Mouse News Lett. 55:18.

[0183] 20. Chung, W. K., Power-Kehoe, L., Chua, M., Chu, F., Aronne, L., Huma, Z., Sothern, M., Udall, J. N., Kahle, B. and Leibel, R. L. (1997). Exonic and intronic sequence variation in the human leptin receptor gene (LEPR). Diabetes 46:1509-1511.

[0184] 21. Sambrook, J., Fritsch, E. F. and Maniatis, T. (1989). Molecular Cloning: A Laboratory Manual, Cold Spring Harbor Laboratory Press.

[0185] 22. Pfaffl, M. W., Georgieva, M. T., Georgiev, P. I., Ontsouka, E., Hageleit, M. and Blum, J. W. (2002). Real-time RT-PCR quantification of insulin-like growth factor (IGF)-1, IGF-1 receptor, IGF-2, IGF-2 receptor, insulin receptor, growth hormone receptor, IGF-binding proteins 1,2 and 3 in the bovine species. Domestic Animal Endocrinology 22:91-102.

[0186] 23. Roderick, T., Donahue, L., Samples, R., Kim, J. and Naggert, J. (2001). Mice with mutations in the mahogany gene atrn have cerebral spongiform changes. J Neuropathol Exp Neurol 60:724-730.

[0187] 24. Venter, J. C., Adams, M. D., Myers, E. W., Li, P. W., Mural, R. J., Sutton, G. G., Smith, H. O., Yandell, M., Evans, C. A., Holt, R. A., et al. (2001). The sequence of the human genome. Science 291:1304-1351.

[0188] 25. Lower, R. (1999). The pathogenic potential of endogenous retroviruses: facts and fantasies. Trends in Microbiology 7:350-356.

[0189] 26. Nagase, T., Ishikawa, K., Miyajima, N., Tanaka, A., Kotani, H., Nomura, N. and Ohara, O. (1998). Prediction of the coding sequences of unidentified human genes. IX. The complete sequences of 100 new cDNA clones from brain which can code for large proteins in vitro. DNA Research 5:31-39.

[0190] 27. Bahary, N., Siegel, D. A., Walsh, J., Zhang, Y., Leopold, L., Leibel, R. L., Proenca, R. and Friedman, J. M. (1993). Microdissection of proximal mouse chromosome 6: identification of RFLPs tightly linked to the ob mutation. Mammalian Genome 4:511-515.

[0191] 28. Yeo, G. S. H., Farooqi, I. S., Challis, B. G., Jackson, R. S. and O'Rahilly, S. (2000). The role of melanocortin signalling in the control of body weight: evidence from human and murine genetic models. QJM 93:7-14.

[0192] 29. Seperack, P. K., Mercer, J. A., Strobel, M. C., Copeland, N. G. and Jenkins, N. A. (1995). Retroviral sequences located within an intron of the dilute gene alter dilute expression in a tissue-specific manner. EMBO J 14:2326-2332.

[0193] 30. Palmiter, R. D., Erickson, J. C., Hollopeter, G., Baraban, S. C. and Schwartz, M. W. (1998). Life without Neuropeptide Y. Recent Prog Horm Res 53:163-199.

[0194] 31. Saurin, A. J., Borden, K. L. B., Boddy, M. N. and Freemont, P. S. (1996). Does this have a familiar RING? TIBS 21:208-214.

[0195] 32. Borden, K. and Freemont, P. S. (1996). The RING finger domain: a recent example of a sequence-structure family. Current Opinion Structure Biology 6:395-401.

[0196] 33. Zheng, N., Wang, P., Jeffrey, P. D. and Pavletich, N. P. (2000). Structure of a c-Cbl-UbcH7 Complex: RING domain function in ubiquitin-protein ligases. Cell 102:533-539.

[0197] 34. Joazeiro, C. A. and Weissman, A. M. (2000). RING finger proteins: mediators of ubiquitin ligase activity. Cell 102:549-552.

[0198] 35. Conaway, R. C., Brower, C. S. and Conaway, J. W. (2002). Emerging Roles of Ubiquitin in Transcription Regulation. Science 296:1254-1258.

Mahoganoid polypeptides, and related compositions and methods

Information

Publication Number

Date Filed

Date Published

Inventors

CPC

US Classifications

International Classifications

Abstract

Description

Claims

Parent Case Info

Government Interests

Provisional Applications (1)