首页> 外文期刊>Nepal Journal of Science and Technology >Optimization of RAPD-PCR Conditions for the Study of Genetic Diversity in Nepalese Isolates of Bacillus thuringiensis Berliner
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Optimization of RAPD-PCR Conditions for the Study of Genetic Diversity in Nepalese Isolates of Bacillus thuringiensis Berliner

机译:优化苏芸金芽胞杆菌柏林分离株尼泊尔遗传多样性的RAPD-PCR条件的研究

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Random amplified polymorphic DNA (RAPD) is a simple and reliable method to detect DNA polymorphism and has been used extensively for genetic diversity studies. In the present investigation the RAPD reaction and cycling conditions were optimized for generating RAPD fingerprints of ten Nepalese strains of Bacillus thuringiensis Berliner (Bt) isolated from an altitudinal range of 70 meter above sea level (masl) to 5050 masl . To determine the optimum conditions, different concentrations of MgCl 2 , template DNA, Taq DNA polymerase, primer, dNTPs as well as different cycling programs were analyzed. Reproducible amplification patterns were obtained using 0.4 μM of primer, 2.5 mM of MgCl 2 , 125 ng of template DNA, 0.2mM of dNTPs and 1U Taq DNA polymerase in 25 μl of the reaction volume. Cycling programs were also optimized. Out of 100 arbitrary primers screened, amplification performed with 24 primers generated the best RAPD fingerprints. The optimized RAPD-PCR conditions and the selected primers are suitable for further work on genetic diversity analysis of Nepalese isolates of Bt. Key words: DNA fingerprint; primer; Taq DNA polymerase; template DNA DOI: 10.3126jst.v9i0.3171 Nepal Journal of Science and Technology 9 (2008) 91-97
机译:随机扩增多态性DNA(RAPD)是检测DNA多态性的一种简单可靠的方法,已被广泛用于遗传多样性研究。在本研究中,优化了RAPD反应和循环条件,以生成从海拔70米至5050 masl的十个尼泊尔苏云金芽胞杆菌柏林(Bt)菌株的RAPD指纹。为了确定最佳条件,分析了不同浓度的MgCl 2,模板DNA,Taq DNA聚合酶,引物,dNTPs和不同的循环程序。在25μl反应体积中,使用0.4μM引物,2.5 mM MgCl 2,125 ng模板DNA,0.2mM dNTPs和1U Taq DNA聚合酶可获得可再现的扩增模式。自行车程序也得到了优化。在筛选出的100个任意引物中,用24个引物进行的扩增产生了最佳的RAPD指纹。优化的RAPD-PCR条件和选择的引物适合进一步研究尼泊尔Bt分离株的遗传多样性。关键字:DNA指纹图谱;底漆Taq DNA聚合酶;模板DNA DOI:10.3126 / njst.v9i0.3171尼泊尔科学技术杂志9(2008)91-97

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