| Production of transgenic calves by somatic cellnuclear transfer |
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| 作者姓名: | GONGGuochun DAIYunping FANBaoliang ZHUHuabing WANGLili WANGHaiping TANGBo LIUYing LIRong WANGRong HUANGYinghua LINing |
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| 作者单位: | [1]StateKeyLaboratoryforAgrobiotechnology,ChinaAgriculturalUniversity,Beijing100094,China [2]InstituteofAnimalScience,ChineseAcademyofAgriculturalScience,Beijing100094,China [3]GentitanBiotechnologyLtd.,Beijing100084,China |
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| 摘 要: | Bovine fetal oviduct epithelial cells were transfected with constructed double marker selective vector(pCE-EGFP-IRES-Neo-dNdB) containing the enhanced green fluorescent protein (EGFP) and neomycin-resistant(Neo^r) genes by electroporation, and a transgenic cell line was obtained. Somatic cell nuclear transfer (SCNT) was cartied out using the transgenic cells as nuclei donor. A total of 424 SCNT embryos were reconstructed and 208 (49.1%) of them developed to blastocyst stage. 17 blastocysts on D 7 after reconstruction were transferred to 17 surrogate calves,and 5 (29.4%) recipients were found to be pregnant. Three of them maintained to term and delivered three cloned calves.PCR and Southern blot analysis confirmed the integration of transgene in all of the three cloned calves. In addition, expression of EGFP was detected in biopsy isolated from the transgenic cloned calves and fibroblasts derived from the biopsy. Our results suggest that transgenic calves could be efficiently produced by SCNT using transgenic cells as nuclei donor. Furthermore, all cloned animals could be ensured to be transgenic by efficiently pre-screening transgenic cells and SCNT embryos using the constructed double marker selective vector.
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| 关 键 词: | 核移植 体细胞 增强绿荧光蛋白质 EGFP 转基因技术 |
| 收稿时间: | 2003-09-25 |
| 修稿时间: | 2003-11-24 |
Production of transgenic calves by somatic cell nuclear transfer |
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| GONGGuochun DAIYunping FANBaoliang ZHUHuabing WANGLili WANGHaiping TANGBo LIUYing LIRong WANGRong HUANGYinghua LINing.Production of transgenic calves by somatic cellnuclear transfer[J].Chinese Science Bulletin,2004,49(2):161-166. |
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| Authors: | Guochun Gong Yunping Dai Baoliang Fan Huabing Zhu Lili Wang Haiping Wang Bo Tang Ying Liu Rong Li Rong Wan Yinghua Huang Ning Li |
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| Institution: | (1) State Key Laboratory for Agrobiotechnology, China Agricultural University, 100094 Beijing, China;(2) Institute of Animal Science, Chinese Academy of Agricultural Science, 100094 Beijing, China;(3) Gentitan Biotechnology Ltd., 100084 Beijing, China |
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| Abstract: | Bovine fetal oviduct epithelial cells were trans-fected with constructed double marker selective vector (pCE-EGFP-IRES-Neo-dNdB) containing the enhanced green fluorescent protein (EGFP) and neomycin-resistant (Neor) genes by electroporation, and a transgenic cell line was obtained. Somatic cell nuclear transfer (SCNT) was carried out using the transgenic cells as nuclei donor. A total of 424 SCNT embryos were reconstructed and 208 (49.1%) of them developed to blastocyst stage. 17 blastocysts on D 7 after reconstruction were transferred to 17 surrogate calves, and 5 (29.4%) recipients were found to be pregnant. Three of them maintained to term and delivered three cloned calves. PCR and Southern blot analysis confirmed the integration of transgene in all of the three cloned calves. In addition, expression of EGFP was detected in biopsy isolated from the transgenic cloned calves and fibroblasts derived from the biopsy. Our results suggest that transgenic calves could be efficiently produced by SCNT using transgenic cells as nuclei donor. Furthermore, all cloned animals could be ensured to be transgenic by efficiently pre-screening transgenic cells and SCNT embryos using the constructed double marker selective vector. |
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| Keywords: | transgenic somatic cell nuclear transfer EGFP bovine |
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