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作 者:陈琴[1] 彭超 赵峰[1] 李军 高炳淼[3] CHEN Qin;PENG Chao;ZHAO Feng;LI Jun;GAO Bingmiao(Hainan Radio and Television University,Haikou,Hainan 570208;Shenzhen Huada Marine Science and Technology Ltd.,Shenzhen,Guangdong 518083;College of Pharmacy,Hainan Medical University,Haikou,Hainan 571199,China)
机构地区:[1]海南广播电视大学,海南海口570208 [2]深圳华大海洋科技有限公司,广东深圳518083 [3]海南医学院药学院,海南海口571199
出 处:《贵州农业科学》2018年第12期25-28,共4页Guizhou Agricultural Sciences
基 金:海南省自然科学基金项目(317170)
摘 要:为了建立适合南海芋螺的ITS-PCR体系以研究不同种类芋螺的遗传多样性,以多种芋螺的3种不同组织为材料,利用海洋生物基因组试剂盒法提取芋螺基因组DNA为模板,采用正交试验对ITS-PCR过程中的关键影响因素进行优化,以最优ITS-PCR体系扩增获得不同种类芋螺的ITS序列并进行测序鉴定。结果表明:最佳ITS-PCR反应体系(25μL)为Taq酶0.3U,dNTPs 3mmol/L,Mg^(2+)1.0mmol/L,引物2.0μmol/L,模板40ng,10×PCR Buffer(不含Mg^(2+))2.5μL,ddH_2O补足25μL。采用该最佳体系对芋螺基因组DNA进行PCR扩增,产物经单向测序获得芋螺ITS部分序列,经NCBI数据库比对其匹配度为83%。The genomic DNA of different Conus spectrum is extracted from three different tissues by Marine Genomes Extraction Kit method.The key factors influencing ITS-PCR process are optimized by an orthogonal test.ITS sequence of different C.spectrum acquired by the optimum ITS-PCR system is sequenced and identified to establish the suitable ITS-PCR system of C.spectrum in South China Sea for studying genetic diversity of C.spectrums.Result:The optimum ITS-PCR system(25μL)includes 0.3 U Taq DNA polymerase,3 mmol/L dNTPs,1.0 mmol/L Mg^2+,2.0μmol/L primer,40 ng template DNA,2.5μL 10×PCR Buffer and 25μL ddH2O.The genomic DNA of C.spectrum is amplified by the optimal ITS-PCR system.The identity between part ITS sequence of C.spectrum obtained by sequencing the amplified product and NCBI database reaches 83%.
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