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作 者:宋凯杰[1,2] 陈宗艳[1] 黄云秀[1,3] 李传峰[1] 孟春春[1] 李丹丹[1,2] 张淼涛[2] 刘光清[1]
机构地区:[1]中国农业科学院上海兽医研究所,上海200241 [2]西北农林科技大学动物医学院,杨凌712100 [3]广西大学动物科学技术学院,南宁530005
出 处:《中国动物传染病学报》2015年第3期42-49,共8页Chinese Journal of Animal Infectious Diseases
基 金:农业部公益性行业科研专项(201303046);国家自然科学基金项目(31270194;31101848);上海市科委创新项目(13391901602)
摘 要:根据鸭Toll样受体3(Toll-like receptor 3,TLR3)的基因序列保守区设计特异性引物,以鸭β肌动蛋白(β-actin)mRNA为内参,建立了一种检测鸭TLR3 mRNA表达水平的实时荧光定量PCR方法。该方法的标准曲线在1×102~1×108copies/μL范围内,具有良好的线性关系,相关系数和扩增效率均在0.9以上。熔解曲线显示,PCR产物为单峰,具有高度扩增特异性。重复性结果表明,该方法组内、组间变异系数均小于3%,最低检测浓度达100 copies/μL。利用该方法检测了TLR3在鸭组织器官中的表达和分布情况,结果表明,TLR3在鸭子的各种组织或器官中均有分布,其中以气管的表达水平最高,而在脾脏的表达水平最低。该检测方法的成功建立为研究TLR3在鸭天然免疫过程中的生物学功能提供了良好的技术手段。The objective of the present study was to develop a real-time fluorescence quantitative PCR(q RT-PCR) assay for detection of duck Toll-like receptor 3(TLR3) mRNA. A pair of specific primers were designed according to the gene sequences of duck TLR3 available in Gen Bank. The β-actin mRNA was used as internal control. The standard curves of this method showed good linear relationships(R20.99) and efficiency about 0.9 in the range of 1×102 to 1×108 copies/μL. The q RT-PCR assay was specific for detecting TLR3 mRNA as analyzed for melting curves. In addition, the minimum detectable concentrations of positive plasmids of TLR3 and β-actin were 100 copies/μL. Both intra-assay and inter-assay coefficients of variation were less than 3%. To verify whether this method was valid, the tissue distribution of TLR3 was examined using the q RT-PCR assay. The results showed that TLR3 was widely expressed in various tissues of duck with the highest expression level in trachea and lowest expression level in spleen.
分 类 号:S852.42[农业科学—基础兽医学]
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