袁玉国
  • 学位:博士
  • 职称:副高级
  • 所在单位:兽医学院

博士生导师

硕士生导师

教师英文名称:Yuguo Yuan
教师拼音名称:Yuan Yuguo
电子邮箱:
入职时间:2010-06-01
学历:博士研究生毕业
办公地点:扬州大学文汇路校区45楼102室
性别:
联系方式:0514-87979228
在职信息:在岗
毕业院校:扬州大学

学科:临床兽医学

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Generation of human lactoferrin transgenic cloned goats using donor cells with dual markers and a modified selection procedure
点击次数:
影响因子:
2.8
发表刊物:
Theriogenology
摘要:
The objective was to use dual markers to accurately select genetically modified donor cells and ensure that the resulting somatic cell nuclear transfer kids born were transgenic. Fetal fibroblast cells were transfected with dual marking gene vector (pCNLF-ng) that contained the red-shifted variant of the jellyfish green fluorescent protein (LGFP) and neomycin resistance (Neo) markers. Cell clones that were G418-resistant and polymerase chain reaction-positive were subcultured for several passages; individual cells of the clones were examined with fluorescence microscopy to confirm transgenic integration. Clones in which every cell had bright green fluorescence were used as donor cells for nuclear transfer. In total, 86.7% (26/30) cell clones were confirmed to have transgenic integration of the markers by polymerase chain reaction, 76.7% (23/30) exhibited fluorescence, but only 40% (12/30) of these fluorescent cell clones had fluorescence in all cell populations. Moreover, through several cell passages, only 20% (6/30) of the cell clones exhibited stable LGFP expression. Seven transgenic cloned offspring were produced from these cells by nuclear transfer. Overall, the reconstructed embryo fusion rate was 76.6%, pregnancy rates at 35 and 60 days were 39.1% and 21.7%, respectively, and the offspring birth rate was 1.4%. There were no significant differences between nuclear transfer with dual versus a single (Neo) marker (overall, 73.8% embryo fusion rate, 53.8% and 26.9% pregnancy rates, and 1.9% birth rate with five offspring). In conclusion, the use of LGFP/Neo dual markers and an optimized selection procedure reliably screened genetically modified donor cells, excluded pseudotransgenic cells, and led to production of human lactoferrin transgenic goats. Furthermore, the LGFP/Neo markers had no adverse effects on the efficiency of somatic cell nuclear transfer.
合写作者:
Yu-Guo Yuan,Yang TJ,Yu BL
第一作者:
Li-You An
论文类型:
Research Atricle
通讯作者:
Cheng Y
是否译文:
发表时间:
2012-10-04
个人简介

袁玉国,博士,副教授,硕士、博士生导师。2010年毕业于扬州大学兽医学院,获临床兽医学博士学位,并留校任教。2015.10—2017.7韩国Konkuk University博士后,2017.9—2018.9韩国Gyeongsang National University访问学者。

长期从事动物体细胞克隆和转基因克隆的研究工作,2007在国内外首次报道利用成年乳腺上皮细胞获得克隆山羊,先后获得转人乳铁蛋白,白蛋白等转基因克隆羊。利用TALENCas9技术获得Fel d1基因敲除猫、MSTN基因敲除山羊,人高血脂兔动物模型(兔)等。同时开展了功能纳米材料的制备及其在抗菌、抗肿瘤和化妆品上的应用。先后主持了国家自然科学基金、国家转基因重大专项子课题、江苏省种业“揭榜挂帅”等15余项课题的研究工作,在 EBioMedicineInt J NanomedicineCellsOxid Med Cell Longev,  Int J Mol Sci,Mol Reprod DevTheriogenology等杂志发表SCI论文30余篇,获得省部级等科技奖励2项、发明专利1项。


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