摘要
[目的]研究SRAP分子标记用于苦荞分析中的条件优化。[方法]采用交互正交设计L27(313)对苦荞SRAP-PCR反应体系进行了5因素(Mg2+、dNTP、Taq酶、模板DNA和引物)3水平优化筛选,比较了非变性和变性PAGE检测方法,并进行了DYCZ-24F与DYCZ-20C2种电泳操作系统的对比试验。[结果]4个单因素(Mg2+、dNTP、Taq酶和引物)和2个交互作用(Mg2+×dNTP、Mg2+×Taq酶)对苦荞SRAP-PCR有极显著影响;最佳反应体系为:20μl总体积,Mg2+1.5mmol/L,dNTP0.2mmol/L,Taq酶1.5U,模板DNA40ng,引物0.25μmol/L,10×缓冲液2μl。运用该体系对7份苦荞材料进行扩增,扩增条带清晰、多态性高、重复性好。将扩增产物进行非变性与变性PAGE和2种电泳操作系统检测,结果显示非变性PAGE、DYCZ-24F操作系统更适合于SRAP的分析。[结论]为今后构建苦荞SRAP遗传图谱奠定了基础。
[Objective]The aim was to investigate the optimal conditions of SRAP molecular marker used in the analysis on Fagopyrum tataricum(L.) Gaertn.[Method]SRAP-PCR amplification system on Fagopyrum tataricum was optimized by interactive orthogonal design L27(313) in 5 elements(Mg2+,dNTP,Taq DNA polymerase,template DNA and primer) at 3 levels. And the non-denaturing and denaturing PAGE detection methods were compared. The comparative test of DYCZ-24F and DYCZ-20C electrophoresis operating systems was carried out.[Result]The effects of four single-factor(Mg2+,dNTP,Taq DNA polymerase and primer) and two interactions(Mg2+×dNTP,Mg2+×Taq DNA polymerase) on tartary buckwheat SRAP-PCR were significant.An optimal reaction system was established containing 1.5 mmol/L Mg2+,0.2 mmol/L dNTP,1.5 U Taq DNA polymerase,40 ng DNA,0.25 μmol/L primer and 2 μl 10×buffer.Seven samples of tartary buckwheat were amplified using this system,and electrophoresis results showed clear bands,high level of polymorphism and good reproducibility.The PCR products were tested by denaturing and non-denaturing PAGE,and the results showed that the non-denaturing PAGE,DYCZ-24F operating system was more suitable for SRAP analysis.[Conclusion]This study established a foundation for the construction of SRAP genetic map of tartary buckwheat.
出处
《安徽农业科学》
CAS
北大核心
2011年第1期44-48,共5页
Journal of Anhui Agricultural Sciences
基金
国家自然科学基金项目(30771310)
