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青枯菌SRAP—PCR体系的建立与优化
引用本文:智艳平,武喜艳,安瑶瑶,郜刚. 青枯菌SRAP—PCR体系的建立与优化[J]. 山西师范大学学报:自然科学版, 2013, 0(4): 69-72
作者姓名:智艳平  武喜艳  安瑶瑶  郜刚
作者单位:山西师范大学生命科学学院,山西临汾041004
基金项目:国家自然基金项目资助(31271774).
摘    要:本研究以马铃薯青枯菌19046为试验材料,应用单因素试验法优化SRAP—PCR反应体系,得出重复性好、带型清晰、稳定性强的最佳反应体系:总体积为10μL,50.g/μL模板DNA0.6μ、10μmol/L引物0.8μL、TapDNA聚合酶1.0U、10mol/L、dNTPs1.0μL.该反应体系可用于青枯菌遗传多样性、基因定位与克隆等的研究.

关 键 词:青枯菌  SRAP  体系优化

Establishment and Optimization of SRAP Analysis System of Ralstonia solanacearum Genome
ZHI Yan-ping,WU Xi-yan,AN Yao-yao,GAO Gang. Establishment and Optimization of SRAP Analysis System of Ralstonia solanacearum Genome[J]. Journal of Shanxi Teachers University, 2013, 0(4): 69-72
Authors:ZHI Yan-ping  WU Xi-yan  AN Yao-yao  GAO Gang
Affiliation:* (School of Life Science, Shanxi Normal University, Lirifen 041004, Shanxi, China)
Abstract:Some factors affecting PCR amplification of SRAP(Sequence-related amplified polymorphism) were studied using Ralstonia solanacearum P046. A reliable, effective,reproductive and legible repeats optimized technical system was developed. In the 10 μL PCR reaction nfixture,30 ng of genomic DNA, 1.0 U of Taq polymerase,0.8 μL 10 umol/L primers,and 1.0 μL dNTPs were used. This reaction system can be used to study genetic diversify,gene tagging cloning and genetics mapping for SRAP of differ- cnt Ralstonia solanacearum.
Keywords:Ralstonia solanacearum  SRAP  optimization
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