生物技术通报 ›› 2016, Vol. 32 ›› Issue (9): 65-71.doi: 10.13560/j.cnki.biotech.bull.1985.2016.09.010

• 技术与方法 • 上一篇    下一篇

云生毛茛ISSR-PCR体系优化与引物筛选

石琳1, 2, 胡延萍1, 王建科1, 2, 王钧1, 2, 许小宁3, 李毅1, 王莉1   

  1. 1. 中国科学院西北高原生物研究所,西宁 810001; 2. 中国科学院大学,北京 100049; 3. 青海省县镇企业技术组厂站,西宁 810008
  • 收稿日期:2016-01-06 出版日期:2016-09-25 发布日期:2016-10-10
  • 作者简介:石琳,女,硕士研究生,研究方向:植物生物技术;E-mail:silvia20@163.com
  • 基金资助:
    国家自然科学基金项目(31300269),青海(应用)基础研究计划项目(2013-Z-756)

Optimization of ISSR-PCR Reaction System on Ranunculus nephelogenes var. nephelogenes and Primer Selection

SHI Lin, HU Yan-ping, WANG Jian-ke, WANG Jun, XU Xiao-ning, LI Yi, WANG Li   

  1. 1. Northwest Institute of Plateau Biology,Chinese Academy of Sciences,Xining 810001; 2. University of Chinese Academy of Sciences,Beijing 100049; 3. Technology Extension Stations of Township Enterprises of Qinghai Province,Xining 810008
  • Received:2016-01-06 Published:2016-09-25 Online:2016-10-10

摘要: 旨在建立稳定可靠的云生毛茛ISSR-PCR反应体系。采用正交试验设计方法,对影响云生毛茛ISSR-PCR扩增结果的Mg2+、dNTP、Taq DNA聚合酶、引物、模板DNA五个因素进行优化筛选,对反应程序进行优化,建立适用于云生毛茛的最佳反应体系和扩增程序,并对反应体系和扩增程序进行验证;在此基础上筛选多态性好的ISSR引物,采用梯度法筛选各个引物的最适退火温度。结果表明,云生毛茛20 µL ISSR-PCR的最佳反应体系为:模板DNA 30 ng,Mg2+ 1.95 mmol/L,Taq DNA聚合酶0.04 U/µL,dNTP 0.150 mmol/L,引物 0.5 µmol/L;最佳反应程序为:94℃预变性5 min;94℃变性20 s,49.6-60.6℃复性1 min,72℃延伸100 s,38个循环;72℃下延伸6 min。在优化的反应体系和反应程序条件下,从100条ISSR引物中筛选获得16条ISSR扩增引物,并确定了引物各自的最适退火温度。经过不同居群云生毛茛的验证,证明优化后体系扩增条带清晰且重复性好,可用于后续云生毛茛遗传多样性的研究。

关键词: 云生毛茛, ISSR-PCR, 正交实验设计, 体系优化, 引物筛选

Abstract: This work is aimed to establish a stable ISSR-PCR system for Ranunculus nephelogenes var. nephelogenes. A L16(45)orthogonal design was used to screen 5 main parameters(Mg2+,dNTP,Taq DNA polymerase,primer,and template DNA);then the process of ISSR-PCR reaction was optimized,and consequently the optimal reaction system and amplifying procedure for R. nephelogenes var. nephelogenes was established;further,the optimized reaction system and amplifying procedure was verified. Results showed that the optimal concentrations in 20 µL reaction mixture were template DNA 30 ng,Mg2+ 1.95 mmol/L,Taq DNA polymerase 0.04 U/µL,dNTP 0.150 mmol/L, and primer 0.5 µmol/L. The optimal reaction procedure was:pre-denaturalization for 5 mins at 94℃,denaturalization for 20 s at 94℃,renaturation for 1 min at 49.6-60.6℃,followed by 38 cycles of extension for 100 s at 72℃,and final extension for 6 min at 72℃. Under the above optimized reaction system and procedure,16 amplified primers were screened from 100 ISSR primers,and the optimal annealing temperature for each primer was determined. Verification in R. nephelogenes var. nephelogenes of different populations with the optimized ISSR system confirmed that bands amplified were clear and steady,thus the established ISSR-PCR could favor further studies on the genetic diversity of R. nephelogenes var. nephelogenes.

Key words: Ranunculus nephelogenes var. nephelogenes, ISSR-PCR, orthogonal design, optimization of system, primer selection