棉花AFLP技术体系的摸索与建立

对影响棉花AFLP技术体系的多种因素作了探讨 ,得到了一种适于棉花AFLP银染技术的优化体系。该体系中各优化因素为 :①模板DNA浓度为 15 0ng·μL-1;②酶切体系中 ,MseI和EcoRI各加入 3units ,使用NEBbuffer2 ,反应时间为 2h ;③连接最适反应时间为 10h ;④连接产物最适稀释倍数为 10倍 ;⑤预扩增产物最适稀释倍数为10倍。

扁桃基因组DNA的制备和AFLP技术体系的建立

AFLP技术对DNA模板的质量要求较高。桃属果树扁桃的叶片含有较高的糖分、多酚类等物质,基因组DNA的纯化比较繁琐。笔者采用3×CTAB缓冲液提取基因组DNA,并加以纯化,使DNA质量达到AFLP技术的要求。在AFLP分析中,筛选出合适的引物组合:采用E+3/M+3选择性引物组合时,扩增条带少;改用E+2/M+3引物组合后,扩增产物主要分布在600～100bp内,且扩增条带数目适中,多态性适宜,电泳图谱清晰。

小麦基因组AFLP技术体系建立的研究

扩增片断长度多态性(AFLP)可靠性强,多态检出率高,因而被认为是最有效的DNA指纹分析技术.利用这一技术,在不需要预先知道DNA序列信息的情况下就可以同时进行多数DNA酶切片段的PCR扩增.以小麦为材料,对AFLP指纹银染技术及实验操作中的关键技巧作了比较详尽的叙述,并建立起了AFLP技术体系.

影响梨AFLP技术体系关键因素研究

探讨了影响梨扩增片段长度多态性(AFLP)技术体系的关键因素,建立了梨的AFLP标准技术体系,指出DNA的提取、酶的用量和酶切时间、聚丙烯酰胺凝胶电泳、银染程序等都对标准技术体系产生不同程度的影响。

高良姜AFLP技术体系的建立与优化

为了建立适合高良姜的扩增片段长度多态性(AFLP)技术体系,对AFLP技术中主要环节的反应条件进行了优化。研究结果表明,用改良CTAB法可提取高质量的高良姜基因组DNA,基因组DNA用限制性内切酶EcoRⅠ和MseⅠ各4U于37℃水浴2h可以被完全酶切,酶切片段与EcoRⅠ和MseⅠ接头在16℃连接过夜后,用优化的反应体系进行预扩增和选择性扩增,扩增产物经过6%变性聚丙烯酰胺凝胶电泳和银染后获得清晰的多态性指纹图谱,因此说明所建立的AFLP技术体系符合要求。

小麦锈菌AFLP分子标记技术体系的建立

以小麦条锈菌、杆锈菌、叶锈菌的夏孢子为材料,通过DNA提取、酶切、PCR扩增、凝胶电泳等系列程序摸索和优化,建立了锈菌的AFLP分子标记体系如下:40μl酶切体系中采用了EcoRI、TrulI各5U,37℃3h,65℃3h双酶切4μl100ng/μl的DNA;然后加入10μl连接混合液22℃连接3h,16℃10h;连接产物5μl,10μMEcoRI、10μMTru1I预扩引物各1.5μl,PCR反应液25μl,ddH2O17μl进行预扩;预扩产物稀释20倍后取5μl,50ng/μlEcoRI、Tru1I选扩引物各1μl,PCR反应液10μl,ddH2O3μl体系进行选择性扩增,为小麦锈病和其他真菌性病害的分子标记克隆及抗病育种的辅助选择提供了有力工具。

Study on AFLP Technical Protocol for Antagonistic Strains of Streptomyces

[Objective] The aim of this study was to investigate the preparation method and amplification system of antagonistic streptomyces DNA templates based on AFLP assays, and also provide a basis for the application of AFLP technology in the analysis of streptomyces or even actinomyces. [Method] The DNAs were extracted by the modified CTAB method and amplified by the Pst Ⅰ/Mse Ⅰ AFLP kit and its reaction system. The amplified products were analyzed by the denatured polyacrylamide gel electrophoresis. [Result] The genomic DNAs of ten antagonistic strains of Streptomyces were extracted and tested. The result of 0.8% agarose gel electrophoresis showed that the major DNA bands were clear without degradation and RNA residue, with the fragment sizes ranging from 37.64 to 40.86 Kb. By ultraviolet spectrophotometry, the OD260/OD280 values varying from 1.625 to 1.833 were obtained. Furthermore, the agarose gel electrophoresis of DNA products digested by Pst Ⅰ/Mse Ⅰ presented the dispersed fluorescent long band, which indicated that the enzymatic hydrolysis was fully carried out. The amplified bands of DNA templates by the screened three pairs of primers were clear with rich polymorphism. [Conclusion] The preparation method and amplification system of DNA template established in this study can be used in the AFLP analysis of Streptomyces.

黄瓜枯萎病菌遗传多样性的AFLP分析

黄瓜枯萎病是由半知菌亚门尖孢镰刀菌黄瓜专化型（Fusarium oxysporumf.sp.cucumainumOwen）侵染引起的一种土传病害,是影响黄瓜生产的最主要病害之一。近年来随着分子生物学技术的迅速发展,国内外学者对于病原真菌的遗传多样性做了大量的研究,Wang等[2]对影响黄瓜枯萎病菌AFLP技术体系的多种因素作了探讨,得到了1种适合于黄瓜枯萎病菌AFLP分析的优化体系;Duan等[3]应用RAPD、