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Former Name	STOCK a Tyrp1b Si/J    (Changed: 16-JUN-05 )
	STOCK a Tyrp1b si    (Changed: 15-DEC-04 )
Genes & Alleles	Si;   Sisi;   Tyrp1;   Tyrp1b;   a;

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Product Information

Strain Details

Type JAX® GEMM® Strain - Mutant Stock Additional information on JAX® GEMM® Strains. Species laboratory mouse Generation pF4p

Appearance
black with varying amounts of silver hairs
Related Genotype: a/a, Tyrp1^b/Tyrp1^b Si^si/Si^si or a/a Tyrp1^b/+, Si^si/Si^si

Strain Description
Several proteins have been characterized as being critical for melanogenesis, including tyrosinase and its related proteins tyrosinase related protein 1 and 2 (TRP-1 and TRP-2). The silver locus protein (SI) is also crucial to the normal melanogenic pathway and it is believed that the interactions of these, and probably other, proteins are necessary for proper melanin pigment production within melanocytes. Nonagouti mice (a/a) homozygous for the recessive si mutation display a range of coat color variations, including all black and all white. Also, single hairs can be both black and white as the tips contain no pigment while the base retains pigmentation. Black and white banding patterns in individual hairs is also observed. It is noted that similar si/si hair color variation is also seen on the agouti background. Young a/a mice typically have black hairs, with some silver/grey hair present on the head, behind the ears and around the posterior. The hair generally becomes progressively lighter with age, with the males displaying more silvering than the females. The silver mutation causes a graying of hair because the follicular melanocytes become dysfunctional and eventually die. Variations in the silvering of the coat color reflect an overall reduction in the number or total lack of melanocytic pigment granules. The loss of these melanocytes, in fact, co-localizes with hypopigmented hair follicles. Also, reduced viability of si/si melanocytes is observed in vitro where these cultured cells exhibit very slow growth rates and have a reduced life span compared to similarly prepared wild type melanocytes.

Functionally, two general activities have been linked to GP87. First, this protein has been reported to be a stabilizing structural matrix glycoprotein in cultured B16 murine melanoma cells as the carboxy-terminus contains an epitope that is recognized by the anti-melanosomal matrix protein antibody alpha-MX. The protein is exclusively restricted to the melanosomal compartment itself as shown by Western blotting of sub-cellular fractions, but is not detected in coated vesicles that shuttle tyrosinase-related proteins to melanosomes. Therefore, the trafficking of the silver protein is distinct. The predicted protein product of GP87 contains a single potential transmembrane domain but based on detergent solubility studies, the protein is likely to be loosely associated with the melanosomal matrix, or contained near the inner aspects of the organelle membrane, or even free in the space between the matrix and membrane. This is in contrast to the subcellular localization of TRP-1 and TRP-2, which are known integral membrane proteins. GP87 is rapidly synthesized and delivered to the melanosomes. Soon after, the protein is processed to lose its C-terminus, as shown through specific reactivity by using a peptide that recognizes this epitope (alpha PEP13). It is not clear what function this post-translational step plays in the normal melanosome but by acting as a structural component, the silver protein could restrict melanogenesis to the appropriate intracellular compartment and 1) protect the cells from toxic melanogenic metabolites such as 5,6-dihydroxyindole and/or 2) stabilize melanin metabolites such as dihydroxyindoles and indolequinones. The silver protein has also been proposed to have an enzymatic role in catalyzing melanin formation through the polymerization of 5,6-dihydroxyindole-2-carboxylic acid (DHICA). Melanin synthesis via the enzymatic conversion of DHICA was found to be mediated by the silver protein through an immunopurification assay conducted on extracts from cultured Cloudman S91 mouse melanoma cells.

Based on primary sequence analysis, the protein product of the si allele is predicted to be mistargeted within melanocytes. Direct evidence for this comes from melan-Si cells (Tyrp1^b/+ Si^si/Si^si). These si/si cells express the mutant protein abnormally outside of the melanosome/pre-melanosome in the soluble fraction where the protein appears degraded or in aggregates. The mutant silver protein, therefore, is misrouted within si/si melanosomes. Interestingly, tyrosinase also is not normally localized within the melan-Si cells. Disrupted protein distribution in the silver mutant melanosomes likely results in a lack of the formation of functional melanogenic complexes containing GP87, tyrosinase and TRPs. While it is not clear what leads to si/si melanocyte death, it could be due to cytotoxic events induced by the mutation that causes the release of toxic melanin precursors. The chemical properties of melanins found in Si hair pigment granules were quantified by high-performance liquid chromatography and spectrophotometric assays measuring levels of pyrrole-2,3,5-tricarboxylic acid (PTCA), aminohydroxyphenylalanine (AHP), spectrophotometric eumelanin (SE), spectrophotometric pheomelanin (SP) and alkali-soluble melanins. The chemical properties of silver hair-derived melanins are similar to brown and light hair melanins but as expected, the total melanin content is much lower compared to black hair melanins (reduced by one-fifth to one-tenth). Chemical characterization of the pigment forms found in silver melanins revealed a partial suppression of eumelanogenesis similar to that seen in the brown hair locus mutants (encoding tyrosinase-related protein 1).

Follicular melanocytes of silver mice are more susceptible to damage resulting from X-irradiation. Since human GP100 is an antigenic marker for a variety of human melanomas that can be recognized by CD8+ T lymphocytes, the silver mutant might serve as a model to experimentally test for potential immunotherapies. (Dunn and Thigpen, 1930; Spanakis et al., 1992; Ozeki et al., 1995; Lamoreux et al., 2001; Kwon et al., 1995; Martinez-Esparza et al., 1999; Zhou et al., 1994; Kobayashi et al., 1994; Solano et al., 2000; Chakraborty et al., 1996; Berson et al., 2001; Martinez-Esparza et al., 2000b; Cormier et al., 1998).

Strain Development
This "silver grey" stock was acquired by Dunn and Thigpen (Dunn and Thigpen 1930) in 1927 from a single pair of mice from the house mouse colony, where the mutation arose, maintained by English fancier William Turton. Silver (Dunn-MacDowell-Gowen) was subsequently maintained in LGW inbred mice at Iowa State University and was bred into the linkage stock carrying Pcdh15^av/Pcdh15^av, Si^si/Si^si, Tyrp1^b/+, a^e/a^e (RH Schaible, 1957). Pcdh15^av is a mutation that arose on the K strain in 1955 and linkage with the silver locus was demonstrated (RH Schaible, 1961); extreme non-agouti, a^e, appeared in mice descending from x-ray mutagenized male breeders of the S strain (Hollander and Gowen, 1956). In 1963, this "av" linkage stock was imported from RH Schaible to the Jackson Laboratory where mice were sibling mated for 14 generations. A single outcross to C57BL/10Gn occurred in 1968 and mice were sibling mating thereafter; Pcdh15^av has not been detected in this stock since the outcross. In 1979 at about F50, males from this strain (a/a, Tyrp1^b/Tyrp1^b, Si^si/Si^si) were outcrossed to female B6C3Fe-a/a F1 mice for frozen embryo storage. In 1987, B6C3Fe-a/a X STOCK a Tyrp1^b Si^si embryos were thawed and a live stock reconstituted. These mice were sibling mated [F1p] F3 through F5 to generate additional embryo stocks in 1988. Either of these sets of frozen stocks may be used to reconstitute this strain. Embryos are homozygous for both the silver mutation and a, and segregate for the Tyrp1^b allele.

Mammalian Phenotype Terms assigned by genotype The following phenotype information may relate to a genetic background differing from this JAX® Mice strain. Sisi/Sisi         Background Not Specified pigmentation phenotype irregular coat pigmentation (MGI Ref ID J:78801) random inviability of melanoblasts in hair follicles results in mice that are variegated for white, partially pigmented (gray) hairs, and fully pigmented hairs other pigment loci influence appearance: nonagouti mice display silvering more on the belly than on the back and become more silvery with age, with nonagouti and brown, mice display fewer white and partially white hairs, and with agouti the yellow band at the tip of hairs is not affected but the base of each hair is lightened creating a whiteish "underfur" and silvering decreases with age the merle pigment pattern is difficult to classify in different crosses reduced hair shaft melanin granule number (MGI Ref ID J:13051) the basis for variable silvering of the coat skin/coat/nails phenotype irregular coat pigmentation (MGI Ref ID J:78801) random inviability of melanoblasts in hair follicles results in mice that are variegated for white, partially pigmented (gray) hairs, and fully pigmented hairs other pigment loci influence appearance: nonagouti mice display silvering more on the belly than on the back and become more silvery with age, with nonagouti and brown, mice display fewer white and partially white hairs, and with agouti the yellow band at the tip of hairs is not affected but the base of each hair is lightened creating a whiteish "underfur" and silvering decreases with age the merle pigment pattern is difficult to classify in different crosses reduced hair shaft melanin granule number (MGI Ref ID J:13051) the basis for variable silvering of the coat homeostasis/metabolism phenotype *normal* homeostasis/metabolism phenotype (MGI Ref ID J:29151) no aberrant bleeding time after tail vein nick hematopoietic system phenotype *normal* hematopoietic system phenotype (MGI Ref ID J:29151) NORMAL: bleeding time is normal

Gene & Allele Details

Allele Symbol		Sisi
Allele Name		silver
Common Name(s)		Pmel 17; gp100; gp87;
Gene Symbol and Name		Si, silver
Chromosome		10
Gene Common Name(s)		D10H12S53E; D12S53E; D12S53Eh; DNA segment, Chr 10, human D12S53E; ME20; PMEL; PMEL17; SIL; gp100; gp87;
General Note		This mutation arose in an unspecified English fancy stock.
Molecular Note		Sequencing of partial gp87 cDNA from homozygous mutant melanocytes showed this mutation comprises a G to A substitution at base 1808, resulting in a premature stop codon and truncation of the protein in the C-terminal cystolic domain. [MGI Ref ID J:22779] [MGI Ref ID J:58687]
Allele Symbol		Tyrp1b
Allele Name		brown
Strain of Origin		C57BL
Gene Symbol and Name		Tyrp1, tyrosinase-related protein 1
Chromosome		4
Gene Common Name(s)		B; CAS2; CATB; GP75; TRP; TRP-1; TRP1; TYRP; Tyrp; b; b-PROTEIN; brown; iris stromal atrophy; isa; tyrosinase-related protein;
General Note		Tyrp1b, brown, recessive. This type mutant of the brown locus is an old mutation of the mouse fancy. The eumelanin of the hair and eyes is brown rather than black. The pigment granules also appear brown rather than black and are spheroid rather than ovoid in shape (J:12970). The fine structure of the developing pigment granules is fibrillar, like that of wild type mice, but the appearance of the mature granule may be more coarsely granular (J:5346, J:5001, J:5068). The granules incorporate twice as much 14C-tyrosine as normal (J:12173).
Molecular Note		A G-to-A transition point mutation at position 329 was shown by revertant analysis to be responsible for the mutant phenotype seen in the brown mutant. This mutation is predicted to change a cysteine residue to a tyrosine in the encoded protein. Three other point mutations in the brown sequence were identified, but do not contribute to the mutant phenotype. [MGI Ref ID J:44435]
Allele Symbol		a
Allele Name		nonagouti
Strain of Origin		old mutant of the mouse fancy
Molecular Note		Characterization of this allele shows an insertion of DNA comprised of a 5.5kb virus-like element, VL30, into the first intron of the agouti gene. The VL30 element itself contains an additional 5.5 kb sequence, flanked by 526 bp of direct repeats. The host intergration site is the same as for at-2Gso and Aw-38J and includes a duplication of four nucleotides of host DNA and a deletion of 2 bp from the end of each repeat. Northern analysis of mRNA from skin of homozygotes shows a smaller agouti message and levels 8 fold lower than found in wild-type. [MGI Ref ID J:16984] [MGI Ref ID J:24934]

Related Strains

Strains carrying   Tyrp1^b allele

000004	ABP/LeJ
000571	B6.Cg-Whrnwi Tyrp1b/+ +/J
000027	B6.D-Tyrp1b m/J
000670	DBA/1J
000265	MY/HuLeJ
001045	SI/Col Tyrp1b Dnahc11iv/J
002238	STOCK a Tyrp1b shmy/J
001432	STOCK a/a Tyrp1b sks/Tyrp1b +/J
000594	STOCK T(2;8)26H a/T(2;8)26H a Tyrp1+/Tyrp1b/J
001101	STOCK T(3;4)5Rk Tyrp1b/J
000274	TSJ/LeJ

View Strains carrying   Tyrp1^b     (11 strains)

Strains carrying   a allele

003879	B10;TFLe-a/a T tf/+ tf/J
001538	B6 x B6C3Sn a/A-T(1;9)27H/J
000916	B6 x B6C3Sn a/A-T(5;12)31H/J
000602	B6 x B6C3Sn a/A-T(8;16)17H/J
000618	B6 x FSB/GnEi a/a Ctslfs/J
000577	B6 x STOCK a Oca2p Hps5ru2 Ednrbs/J
000601	B6 x STOCK a/a T(7;18)50H/J
000592	B6 x STOCK T(2;4)13H a/J
000001	B6.C3 A/a Mgrn1md/J
000785	B6;D2-a Es1e/J
000604	B6C3 a/A-T(10;13)199H +/+ Lystbg-J/J or Lystbg-2J/J
002807	B6C3Fe a/a-Meox2fla/J
000224	B6C3Fe a/a-Scyl1mdf/J
001037	B6C3Fe a/a-Agtpbp1pcd/J
000221	B6C3Fe a/a-Alx4lst-J/J
002062	B6C3Fe a/a-Atp7aMo-8J/J
001756	B6C3Fe a/a-Cacng2stg/J
001815	B6C3Fe a/a-Col1a2oim/J
000231	B6C3Fe a/a-Csf1op/J
000209	B6C3Fe a/a-Dh/J
000211	B6C3Fe a/a-Dstdt-J/J
000210	B6C3Fe a/a-Edardl-J/J
000207	B6C3Fe a/a-Edaraddcr/J
000182	B6C3Fe a/a-Eef1a2wst/J
001278	B6C3Fe a/a-Glra1spd/J
000241	B6C3Fe a/a-Glrbspa/J
002875	B6C3Fe a/a-Hoxd13spdh/J
000304	B6C3Fe a/a-Krt71Ca Scn8amed-J/J
000226	B6C3Fe a/a-Largemyd/J
000636	B6C3Fe a/a-Lmx1adr-J/J
001280	B6C3Fe a/a-Lse/J
001573	B6C3Fe a/a-MitfMi/J
001035	B6C3Fe a/a-Napahyh/J
000181	B6C3Fe a/a-Otogtwt/J
000278	B6C3Fe a/a-Papss2bm Hps1ep Hps6ru/J
000205	B6C3Fe a/a-Papss2bm/J
002078	B6C3Fe a/a-Pcdh15av-2J/J
000246	B6C3Fe a/a-Pitpnavb/J
001430	B6C3Fe a/a-Ptch1mes/J
000506	B6C3Fe a/a-Qkqk/J
000235	B6C3Fe a/a-Relnrl/J
000237	B6C3Fe a/a-Rorasg/J
000290	B6C3Fe a/a-Sox10Dom/J
000230	B6C3Fe a/a-Tcirg1oc/J
003612	B6C3Fe a/a-Trak1hyrt/J
001512	B6C3Fe a/a-Ttnmdm/J
001607	B6C3Fe a/a-Unc5crcm/J
000005	B6C3Fe a/a-Wc/J
000243	B6C3Fe a/a-Wnt1sw/J
000248	B6C3Fe a/a-Xpl/J
001750	B6C3Fe a/a-XsJ/J
000624	B6C3Fe a/a-anx/J
003020	B6C3Fe a/a-dep/J
002018	B6C3Fe a/a-din/J
002339	B6C3Fe a/a-nma/J
000240	B6C3Fe a/a-soc/J
000063	B6C3Fe a/a-sy/J
001055	B6C3Fe a/a-tip/J
000245	B6C3Fe a/a-tn/J
000296	B6C3Fe-a/a Hoxa13Hd Mcoln3Va-J/J
000019	B6C3Fe-a/a-Itpr1opt/J
001022	B6C3FeF1/J a/a
000971	B6EiC3 a/A-Och/J
000551	B6EiC3 a/A-Tbx15de-H/J
006450	B6EiC3 a/A-Vss/J
000557	B6EiC3-+ a/LnpUl A/J
000503	B6EiC3Sn a/A-Gy/J
001811	B6EiC3Sn a/A-Otcspf-ash/J
002343	B6EiC3Sn a/A-Otcspf/J
000391	B6EiC3Sn a/A-Pax6Sey-Dey/J
001924	B6EiC3Sn a/A-Ts(1716)65Dn
001923	B6EiC3Sn a/A-Ts(417)2Lws Tim/J
000225	C3FeLe.B6 a/a-Ptpn6me/J
000198	C3FeLe.B6-a/J
000291	C3FeLe.Cg-a/a Hm KitlSl Krt71Ca-J/J
001886	C3HeB/FeJLe a/a-gnd/J
000584	C57BL/6J-+ T(1;2)5Ca/a +/J
000284	CWD/LeJ
000670	DBA/1J
000671	DBA/2J
001057	HPT/LeJ
000260	JGBF/LeJ
000265	MY/HuLeJ
000308	SSL/LeJ
000994	STOCK a Myo5ad Mregdsu/J
002238	STOCK a Tyrp1b shmy/J
001433	STOCK a skt/J
000579	STOCK a tp/J
000319	STOCK a us/J
002648	STOCK a/a Cln6nclf/J
000317	STOCK a/a Egfrwa2/J
000302	STOCK a/a MitfMi-wh +/+ Itpr1opt/J
000286	STOCK a/a Myo5ad fd/+ +/J
000206	STOCK a/a Tyrc-h/J
001432	STOCK a/a Tyrp1b sks/Tyrp1b +/J
000281	STOCK a/a ma ft/ma ft/J
000312	STOCK stb + a/+ Fignfi a/J
000596	STOCK T(2;11)30H/+ x AEJ-a Gdf5bp-H/J or A/J-a Gdf5bp-J/J
000970	STOCK T(2;16)28H A/T(2;16)28H a/J
000590	STOCK T(2;4)1Sn a/J
000594	STOCK T(2;8)26H a/T(2;8)26H a Tyrp1+/Tyrp1b/J
000623	TR/DiEiJ

View Strains carrying   a     (102 strains)

Strains carrying other alleles of Tyrp1

000068	C57BL/6J-Tyrp1b-J/J
000093	C57BL/6J-Tyrp1b-cJ/J
000671	DBA/2J
003588	LT/SvEi
006252	LT/SvEiJ
002142	STOCK 11R30m/J
000594	STOCK T(2;8)26H a/T(2;8)26H a Tyrp1+/Tyrp1b/J

View Strains carrying other alleles of Tyrp1     (7 strains)

Strains carrying other alleles of a

003301	(C57BL/6J x C3H-Eya1bor)F1/J
000251	AEJ.Cg-ae +/a Gdf5bp-H/J
000202	AEJ/Gn-bd/J
000199	AEJ/GnLeJ
000427	B10.CE-H13b Aw/(30NX)SnJ
000420	B10.LP-H13b Aw/Sn
000477	B10.PA-Pldnpa H3e at/SnJ
000419	B10.UW-H3b we Pax1un at/SnJ
000593	B6 x B6CBCa Aw-J/A-Grid2Lc T(2;6)7Ca MitfMi-wh/J
000502	B6 x B6CBCa Aw-J/A-Myo5aflr Gnb5flr/J
000599	B6 x B6CBCa Aw-J/A-T(5;13)264Ca KitW-v/J
002083	B6 x B6EiC3 a/A-T(7;16)235Dn/J
000507	B6 x B6EiC3 a/A-Otcspf/J
002016	B6(Cg)-Aw-J EdaTa-6J Chr YB6-Sxr/EiJ
000552	B6-Aw-J-EdaTa-6J.Cg-Sxr
001730	B6-Aw-J-EdaTa-6J.Cg-Sxrb Hya-/J
000841	B6-Aw-J.CBy-EdaTa-By/J
001809	B6-Aw-J.Cg-EdaTa-6J +/+ ArTfm/J
000600	B6-Gpi1b x B6CBCa Aw-J/A-T(7;15)9H Gpi1a/J
000769	B6.C/(HZ18)By-at-44J/J
000203	B6.C3-Aiy/a/J
000017	B6.C3Fe-Avy/J
000628	B6.CE-A Amy1b Amy2b/J
005505	B6.Cg-Ay Slc7a11sut/LmLlp
000021	B6.Cg-Ay/J
001572	B6.Cg-am-J/J
100409	B6129PF1/J-Aw-J/Aw
004200	B6;CBACa Aw-J/A-Npr2cn-2J/J
000505	B6C3 Aw-J/A-Mutedmu/J
000604	B6C3 a/A-T(10;13)199H +/+ Lystbg-J/J or Lystbg-2J/J
000065	B6C3Fe a/a-we Pax1un at/J
000314	B6CBACa Aw-J/A-EdaTa/J-XO
000501	B6CBACa Aw-J/A-Aifm1Hq/J
001046	B6CBACa Aw-J/A-Grid2Lc/J
000500	B6CBACa Aw-J/A-Gs/J
002703	B6CBACa Aw-J/A-Hydinhy3/J
000247	B6CBACa Aw-J/A-Kcnj6wv/J
000287	B6CBACa Aw-J/A-Plp1jp EdaTa/J
000515	B6CBACa Aw-J/A-SfnEr/J
000242	B6CBACa Aw-J/A-spc/J
000288	B6CBACa Aw-J/A-we a Mafbkr/J
001201	B6CBACaF1/J-Aw-J/A
001752	B6CBCa Aw-J/A-T(7;15)9H/J
006450	B6EiC3 a/A-Vss/J
000557	B6EiC3-+ a/LnpUl A/J
000504	B6EiC3Sn a/A-Cacnb4lh/J
000553	B6EiC3Sn a/A-Egfrwa2 Wnt3avt/J
001811	B6EiC3Sn a/A-Otcspf-ash/J
002343	B6EiC3Sn a/A-Otcspf/J
001923	B6EiC3Sn a/A-Ts(417)2Lws Tim/J
000200	C3FeB6 A/Aw-J-Ankank/J
000638	C3FeB6 A/Aw-J-Spnb4qv-J/J
001203	C3FeB6F1/J A/Aw-J
001272	C3H/HeSnJ-Ahvy/J
000099	C3HeB/FeJ-Avy/J
000338	C57BL/6J Aw-J-EdaTa-6J/J
000258	C57BL/6J-Ai/a/J
000774	C57BL/6J-Asy/a/J
000569	C57BL/6J-Aw-J-EdaTa +/+ ArTfm/J
000051	C57BL/6J-Aw-J/J
000055	C57BL/6J-at-33J/J
000070	C57BL/6J-atd/J
002468	KK.Cg-Ay/J
000262	LS/LeJ
000283	LT.CAST-A/J
001759	STOCK A Tyrc Sha/J
001427	STOCK Aw us/J

View Strains carrying other alleles of a     (67 strains)

Research Applications

This mouse can be used to support research in many areas including:

Si^si related

Dermatology Research
Color and White Spotting Defects

Tyrp1^b related

Color and White Spotting Defects

Mouse/Human Gene Homologs
oculocutaneous albinism type III

References

Additional References

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Price and Supply Information

Strain Name:	STOCK a Tyrp1b Sisi/J
Stock Number:	000064

Price Details

IMPORTANT NOTE: Prices are based on shipping destination. The shipping destinations are:

• USA, Canada and Mexico
• International

*Pricing for Shipping Destination selected:

        International

Price(s) in US dollars ($)
Cryorecovery Fee	$2470.00

Supply Details

Standard Supply	Repository-Cryopreserved. Must Be Recovered. Please refer to pricing and supply notes for further information.
Supply Notes	Cryorecovery of Strains Needing Progeny Testing. The recovery process begins when a signed agreement form is returned to the Customer Service Department after order placement. Although results vary by strain, at least two untested males and two untested females (two pairs) will be recovered, typically within 15 weeks of our receipt of the signed agreement form. If the first recovery attempt is unsuccessful or only one pair is recovered, a second recovery will be done, extending the overall recovery time to approximately 25 weeks. However, all pups recovered will be sent. Progeny testing is required to identify the genotype of mice of this strain, as a genotyping assay is not available. This type of testing involves breeding the recovered animals and assessing the phenotype of the offspring in order to identify animals carrying the mutation of interest. We can perform the progeny testing for you as a service or we can ship all recovered animals (at least two untested pairs) to you for progeny testing at your facility. If you perform the progeny testing, there is NO guarantee that a carrier will be identified. If we perform progeny testing as a service, additional breeding time will be required. In this case, when a male and female (one pair) are identified that carry the mutation, they and their offspring will be shipped. Delivery time for strains requiring progeny testing often exceeds 25 weeks and may take 12 months or more due to the difficulties in breeding some strains. The progeny testing cost is in addition to the recovery cost and is based on the number of boxes used and the time taken to produce the mice identified as carrying the mutation. Please note that identified pairs may not reflect the mating scheme utilized by The Jackson Laboratory prior to cryopreservation of the strain. Mating schemes are sometimes modified for successful cryopreservation. Please contact Customer Service for more information on the cost of progeny testing for a strain: Tel: 1-800-422-6423 or 1-207-288-5845. Cryorecovery to establish a Dedicated Supply for greater quantities of mice One to two pairs will be recovered to establish a Dedicated Supply of mice. Price by quotation. For more information on Dedicated Supply, please contact JAX® Services, Tel: 1-800-422-6423 or 1-207-288-5845. Genomic DNA is available for this strain from the Mouse DNA Resource.
Licensing	See General Terms and Conditions below

General Terms and Conditions

View JAX^® Mice & Services Conditions of Use.

The Jackson Laboratory's Genotype Promise

The Jackson Laboratory has rigorous genetic quality control and mutant gene genotyping programs to ensure the genetic background of JAX^® Mice strains as well as the genotypes of strains with identified molecular mutations. JAX^® Mice strains are only made available to researchers after meeting our standards. However, the phenotype of each strain may not be fully characterized and/or captured in the strain data sheets. Therefore, we cannot guarantee a strain's phenotype will meet all expectations. To ensure that JAX^® Mice will meet the needs of individual research projects or when requesting a strain that is new to your research, we suggest ordering and performing tests on a small number of mice to determine suitability for your particular project.

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