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作 者:张弘韬[1] 潘求真[1] 冯国兴[1] 邓守龙[2] 连正兴[2]
机构地区:[1]黑龙江八一农垦大学生命科学技术学院,大庆163319 [2]中国农业大学动物科技学院
出 处:《黑龙江八一农垦大学学报》2013年第6期26-30,共5页journal of heilongjiang bayi agricultural university
基 金:国家重大转基因专项(2009ZX08010-020-2);黑龙江八一农垦大学校启动基金(校启B2008-5)
摘 要:Toll样受体2(Toll-like receptor 2,TLR2)是识别革兰氏阳性细菌如引起羊乳腺炎、炭疽病、破伤风等病原体的一种重要受体,而TLR2过表达转基因羊为研究TLR2在防卫细菌侵染中的作用提供了一个理想的模型。因此,研究首先通过显微注射TLR-2过表达载体3S-Loxp-TLR2的方法对绵羊进行外源基因TLR2整合,然后采用PCR和Southern blot方法对其进行鉴定、拷贝数验证和表达量分析。结果表明,注射148个受精卵,共产下15只小羊,其中8只小羊检测为阳性,转基因率为53.3%;Southern杂交结果发现转TLR2小羊的基因组中外源TLR2基因均为单拷贝;且转基因羊TLR2 mRNA表达高于对照。说明成功构建了转TLR2基因羊。TLR2 (Toll-like Receptor 2) was the important receptor to recognize the invaded gram-positive microbes which caused serious mastiffs, anthrax,tetanus and so on. Transgenic sheep constitutively over-expressing TLR2 in all tissues would be the ideal model to uncover the role of TLR2 on bacteria clearance. TLR-2 over-expression vector (3S-Loxp-TLR2) was used to generate transgenic sheep by egg microinjection. One hundred and forty eight zygotes was microinjected TLR-2 over-expression vector and fifteen lambs were born. The results showed that totally 8 transgenic sheep were identified by PCR and southern blot analysis,the integration efficiency of foreign gene by nficroinjection reached 53.3%. We also found exogenous TLR2 was one copy in all transgenic sheep. The expression level of TLR2 gene of different transgenic lambs were analyzed by using real time PCR, the results showed that transgenic sheep built higher levels of mRNA expression and protein secretion of TLR2.
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