ISSN 1007-7626 CN 11-3870 / Q http / /cjbmb. bjmu. edu. cn Chinese Journal of Biochemistry and Molecular Biology 2016 3 32 3 339 ~ 345 DOI 10. 13865 /j. cnki. cjbmb. 2016. 03. 15 3 1 1 2 1 1 1 3 * 1 030801 2 030801 3 200065 3 endothelin 3 PCR 2 P < 0. 01 5 2 ELISA 1. 8 1. 4 P < 0. 01 3 S852. 2 Localization and Expression of in Mouse Skin with Different Coat Colors WANG Hai-Dong 1 LI Ya-Nan 1 XUE Lin-Li 2 ZHAO Bing-Ling 1 HE Xiao-Yan 1 DONG Chang-Sheng 1 WANG Juan 3 * 1 College of Animal Science and Veterinary Medicine Shanxi Agricultural University Taigu 030801 Shanxi China 2 College of Information Shanxi Agricultural University Taigu 030801 Shanxi China 3 The Affiliated Tongji Hospital of Tongji University Shanghai 200065 China Abstract Endothelin 3 END3 binds to its receptor to promote the migration proliferation and differentiation of early melanocyte also boosts the synthesis of melanin. The diversity of END3 among different coat color mice and the effects of END3 on the formation of coat color need to be investigated. The real - time quantitative PCR result showed that expression in gray mouse skin was significantly higher about 2 folds P < 0. 01 than those from black and brown mice whereas in Western blotting the fold difference was 5 or 2 between brown and black mice P < 0. 01. The ELISA result indicated that protein levels in gray mice was 1. 8 times higher than in black mice or 1. 4 times than in brown mice P < 0. 01. Immunohistochemistry showed that the was predominantly expressed in the matrix outer root sheath but weak in dermal papilla of hair follicular. The results indicated that END3 was an essential factor in melanocytes which played a role in the conversion 2015-11-13 2016-01-14 No. 31302049 20131403120002 * Tel 0354-6288980 E-mail wangjuanshanghai@ 163. com Received November 13 2015 Accepted January 14 2016 Supported by National Natural Science Foundation of China No. 31302049 Doctoral Program of Higher Education 20131403120002 * Corresponding author Tel 0354-6288980 E-mail wangjuanshanghai@ 163. com
340 32 between two types of pigment particles. Key words endothelin-3 mice immunohistochemistry melanin 1 eumelanin pheomelanin 1. 1 RNA TaKaRa 1-3 QuantiFast SYBR Green PCR Kit QIAGEN 3 ELISA DAB 4 Streptavidin-HRP C57BL/6J 14 6 5 3 2 RNA 1 Bouin s 1. 2 RNA cdna Trizol RNA 6 7 TaKaRa cdna 8 oligdt Primer 1 μl dntp Mix 1 μl RNA 2 μg 10 μl PCR 65 5 min 2 min 10 μl 5 Primer Script Buffer 4 μl RNase inhibitor 0. 5 μl Primer script II RNase 1 μl 20 μl PCR 9 45 40 min 70 15 min -20 cdna 1. 3 PCR GenBank EDNRB Premier5. 0 PCR NCBI Table 1 Table 1 Sequence of premier and condition of PCR amplification Gene Primer sequence 5' 3' Product size /bp EDNRB β-actin F TCCTGAACAGACTGTGCCCTA R CGGTGGGCTTTATCTGTCCTT F CAGGAAGAAGAGCGGTATGC R CAGAGCGATTGGATTGATGC F TTGCTGACAGGATGCAGAAG R ACATCTGCTGGAAGGTGGAC 279 256 140
3 3 341 PCR 25 μl 2 Taq MasterMix 12. 5 μl 1 μl cdna 1 μg 25 μl 94 5 min 94 30 s 60 30 s 72 30 s 35 72 5 min 1. 7 1% PCR 200 V 15 min 37 10 min PBS 1. 4 qrt-pcr PCR QIAGEN 37 10 min 10 μl 2 QuantiFast SYBR Green PCR Master Mix 5 μl 1 μl 1 100 ng 10 μl 95 5 min 95 10 s 60 30 s 40 ~ 45 37 10 min PBS 2 - CT EDNRB 5 min 3 HRP = 37 10 min PBS 5 CT CT - CT CT = CT - CT mrna 2 - CT 1. 5 ELISA 4 TBST NC 10 min 3 HRP 1 10 000 37 1 h TBST NC 5 min 6 ECL Image- = = /βactin Means ± SE SPSS 5 min 3 1 100 PBS 4 30 min PBS 5 min 3 min 3 DAB 10 min PBS 3 min 3 2 ELISA 2. 1 EDNRB 1% EDNRB 37 40 min 279 bp 30 s 5 256 bp Fig. 1 50 μl EDNRB 37 20 min 30 s 5 2. 2 EDNRB 100 μl 37 10 min 30 s 5 qrt-pcr 100 μl 37 1 Tm 15 min 100 μl 450 nm S 1. 6 qrt-pcr 50 μg SDS-PAGE NC 2. 0515 ± 5% 1 h 0. 0790 1 1 000 GAPDH 1 1 000 1. 0780 ± 0. 1101 2 P < 0. 01 Fig. 2A EDNRB 26 27 ProPlus 6. 0 P < 0. 01 Fig. 2B
342 32 Fig. 1 Electrophoresis pattern of β-actin and EDNRB PCR product Total RNA was extracted from mouse skin. Then cdna was synthesized and gene was amplified by PCR. We used 1% agarose to detected sequences. The result showed a clear electrophoresis band of 279 bp 140 bp and 256 bp. There was no other band for this experiment. M DL 20000 DNA marker Fig. 2 qrt-pcr analysis of the expression of and EDNRB mrna in different colors of skin tissue collected from mice with black grey brown n = 3 each Data are presented as mean ± SD and three groups comparisons were done with one-way ANOVA. * P < 0. 05 ** P < 0. 01 compared to black 2. 3 ELISA 8. 4417 28. 4032 450 nm ± 4. 5076 CurveExpert 1. 4 Fig. 3 1. 8 1. 4 2. 4 23. 1722 ± 9. 2797 40. 8393 ± 0. 3362 ± 0. 052 Fig. 3 Relative expression of in different hair color mouse skin A The standard curve of B ELISA analysis of in different colors of mouse skin. Data are presented as mean ± SD. The experimental operation accorded to ELISA kits. Three groups comparisons were done with one-way ANOVA. Note ** Mean significant difference P < 0. 01 compared to black
3 3 343 0. 1332 ± 0. 017 5 0. 0665 ± 0. 024 2 Fig. 4 Western blot analysis of protein expression in different color of mouse skin The proteins of different coat color mice were resolved by SDS-PAGE transferred into a nitrocellulose membrane and immunoblotted using an antibody of. The second panel was imaged after longer exposure to confirm the presence of. Three groups comparisons were done with one-way ANOVA. * P < 0. 05 ** P < 0. 01 compared to black 2. 5 Fig. 5 Immunohistochemistry results of in different hair color mouse skin 400 Different coat color mouse skin was stained with immunohistochemistry. Immunohistochemistry were probed with rabbit anti- polyclonal antibody and goat anti-rabbit IgG conjugated HRP as the second antibody then detected colorimetricly using a DAB detection kit. A black mouse skin positive group a black mouse skin negative control group B grey mouse skin positive group b grey mouse skin negative control group C brown mouse skin positive group c brown mouse skin negative control group. 1 hair follicle matrix 2 dermal papilla 3 inside root sheath 4 outside root sheath 3 MC1R Agouti 10 5 5
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