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机构地区:[1]中国农业科学院北京畜牧兽医研究所,北京100094
出 处:《草地学报》2008年第1期17-22,共6页Acta Agrestia Sinica
基 金:国家自然科学基金(30471230)资助;国家科技支撑项目(2006BAD16B04-1)资助
摘 要:以北京苜蓿假盘菌(Pseudopeziza medicaginis (Lib.) Sacc.)菌株为试材,用ISSR-23引物[序列为(AC)8T]研究PCR反应体系的主要成分及退火温度对假盘菌ISSR扩增的影响,以期为苜蓿假盘菌的深入研究奠定基础。结果表明:Primer、Mg2+、Taq酶和dNTP浓度对扩增均有影响,以Primer影响最为明显;优化的反应体系为:20μL反应体系中含0.1 ng模板DNA,2.0 mmol/L MgCl2、0.5μmol/L Primer、1U Taq DNA聚合酶、0.2 mmol/LdNTP,2μL 10×PCR Buffer和2.5%去离子甲酰胺;在此基础上,建立6个不同地理来源苜蓿假盘菌菌株的指纹图谱并分析其亲缘关系;对44条ISSR引物进行筛选,22条可产生清晰稳定的多态性条带,其中16条可将6个供试菌株完全分开,建立了苜蓿假盘菌指纹图谱;经聚类分析,在0.55遗传相似水平下,6个供试菌株分为两个遗传谱系,菌株的遗传谱系与其地理来源之间不表现相关性。The effects of PCR reaction components and annealing temperature on ISSR (inter-simple sequence repeat) amplification of Pseudopeziza medicaginis (Lib.) Sacc. cv. Beijing were studied using primer ISSR-23 (sequence: (AC)8T). The results show that all of components, i.e. concentrations of primer, Mg^2+, Taq DNA polymerases, and dNTP, affected the amplification results, but the effect of primer concentration was distinct. The optimal concentration of ISSR-PCR reaction system was 0. 1 ng template DNA, 2.0 mmol/L MgC12, 0.5 μmol/L primer, 1U Taq DNA polymerase, 0. 2 mmol/L dNTP, 2 μL 10)〈PCR buffer, and 2.5G deionized formamide per 20 μL reaction volume. The ISSR fingerprinting profiles of 6 P. m edicaginis strains with different geographical originals were established with 22 primers screened out from 44 ISSR primers. The isolated P. medicaginis strains were clustered into 2 genetic lineages at 0.55 genetic similarity and the genetic lineages of 6 strains showed no obvious relation with their geographical originals.
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