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罗汉果SRAP反应体系的建立与优化
引用本文:刘丽华,马小军,孙晶晶,覃嘉明,魏建和. 罗汉果SRAP反应体系的建立与优化[J]. 广西植物, 2009, 29(6): 894-898
作者姓名:刘丽华  马小军  孙晶晶  覃嘉明  魏建和
作者单位:1. 中国医学科学院,北京协和医学院,药用植物研究所,北京,100193
2. 辽宁工程技术大学,理学院,阜新,123000
3. 广西玉米研究所,南宁,530227
基金项目:国家科技支撑计划课题(2006BA109B01-07) 
摘    要:建立适合罗汉果的SRAP-PCR扩增体系,为罗汉果的遗传图谱构建及基因定位奠定基础。实验对罗汉果SRAP-PCR反应体系的影响因素(引物,dNTP,Taq酶,Mg~(2+),模板DNA)在多个水平上进行优化试验,筛选出各反应因素的最佳水平,建立了罗汉果SRAP-PCR反应的最佳体系(10μL):引物0.6μmol/L、dNTP0.25 mmol/L、Taq DNA聚合酶0.5U、Mg~(2+)2.0 mmol/L和模板DNA 30 ng。该体系的建立能很好的满足罗汉果基因组DNA的扩增要求,SRAP标记应用于罗汉果遗传研究是可行的。

关 键 词:罗汉果  SRAP-PCR  反应体系  建立

Establishment and optimization of SRAP reaction system in Siraitia grosvenorii
LIU Li-Hu,MA Xiao-Jun,SUN Jing-Jing,QIN Jia-Ming,WEI Jian-He. Establishment and optimization of SRAP reaction system in Siraitia grosvenorii[J]. Guihaia, 2009, 29(6): 894-898
Authors:LIU Li-Hu  MA Xiao-Jun  SUN Jing-Jing  QIN Jia-Ming  WEI Jian-He
Affiliation:1.Institute of Medicinal Plant Development, China Academy Medicinal Science, Chinese Peking Union Medical Colledge, Beijing 100193, China; 2.College of Science, Liaoning Technical University, Fuxin 123000, China; 3.Guangxi Maize Research Institute, Nanning 530227, China
Abstract:The design was used to establish SRAP-PCR amplification system on Siraitia grosvenorii DNA so as to lay foundation for genetic map construction and gene mapping. The factors influencing SRAP analysis,including primers,dNTP,Taq polymerase,Mg~(2+),and the concentration of DNA template were studied in a number of levels respectively. The results showed that: 0.6 μmol/L primer,0.25 mmol/L dNTP,0.5U Taq DNA polymerase,2.0 mmol/L Mg~(2+) and 30 ng DNA template in 10 μL reaction system were the best suitable SRAP-PCR system for Siraitia grosvenorii. It was feasible to apply SRAP marker in genetic research in Siraitia grosvenorii.
Keywords:SRAP-PCR  Siraitia grosvenorii  SRAP-PCR reaction system  establishment
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