Genetic diversity of Ustilago hordei in Tibetan areas as revealed by RAPD and SSR

Covered smut, which is caused by Ustilago hordei（Pers.） Lagerh., is one of the most damaging diseases of highland barley（Hordeum vulgare Linn. var. nudum Hook. f） in Tibetan areas of China. To understand the molecular diversity of U. hordei, a total of 27 isolates, which were collected from highland barley plants from Tibet, Sichuan, Qinghai, and Gansu provinces/autonomous region, were analyzed using random amplified polymorphic DNA（RAPD） and simple sequence repeat（SSR） markers. Among the 100 RAPD primers used, 24 primers exhibited polymorphism. A total of 111 fragments were amplified, of which 103 were polymorphic with a polymorphic rate of 92.79%. The average observed number of alleles（Na）, effective number of alleles（Ne）, Nei＇s genetic diversity（H）, Shannon＇s information index（I） and polymorphism information content（PIC） value in the RAPD markers were 1.9279, 1.5016, 0.2974, 0.4503 and 0.6428, respectively. For the SSR markers, 40 of the 111 primer pairs exhibited polymorphism and provided a total of 119 bands, of which 109 were polymorphic and accounted for 91.60% of the total bands. The Na, Ne, H, I and PIC values of the SSR markers were 1.9160, 1.4639, 0.2757, 0.4211 and 0.4340, respectively. The similarity coefficients ranged from 0.4957 to 0.9261 with an average of 0.7028 among all the 27 isolates used. The dendrogram, which was developed based on the RAPD and SSR combined marker dataset showed that the 27 U. hordei isolates were divided into 3 clusters at similarity coefficient of 0.7314. We determined that RAPD and SSR markers can be successfully used to assess the genetic variation among U. hordei isolates. The RAPD markers revealed higher levels of genetic polymorphism than did the SSR markers in this study. There existed a moderate genetic difference among isolates. The molecular variation and differentiation was somewhat associated with geographical origin but not for all of the isolates.

大麦黑粉菌研究进展

大麦黑粉菌呈世界范围分布,是大麦生产中的主要病害之一,可造成严重经济损失,但在中医上又具有药用和食用价值。本文主要介绍大麦黑粉菌的分类及生理特性,大麦黑粉菌与寄主大麦的互作及其侵染机理,大麦黑粉菌的药用和食用价值,大麦黑粉菌转基因技术体系建立和大麦黑粉菌基因组研究的进展。

青稞黑穗病菌LAMP检测体系的建立

【目的】大麦坚黑粉菌(Ustilago hordei)和裸黑粉菌(Ustilago nuda)是引起青藏高原青稞黑穗病的主要病原菌,建立快速、简便、特异性强的大麦坚黑粉菌和裸黑粉菌环介导等温扩增技术(LAMP)检测体系,检测青稞种子的带菌量,再依据带菌程度进行播前种子处理,是控制青稞黑穗病的重要技术手段。【方法】根据大麦坚黑粉菌(Ustilago hordei)和裸黑粉菌(Ustilago nuda)的ITS基因序列与其他对照菌株同源性低的区段设计并获得有效引物1组,建立LAMP检测体系,并选取影响LAMP反应体系的5个主要因素dNTPs、甜菜碱、镁离子、Bst DNA聚合酶及温度进行单因素试验对其进行优化,最后对优化后的LAMP检测体系进行灵敏度和特异性检测。【结果】建立了青稞黑穗病菌的LAMP检测体系,其优化后dNTPs浓度为1.8 mmol/L、甜菜碱浓度为0.8 mmol/L、镁离子浓度为10 mmol/L、Bst DNA聚合酶浓度为320 U/mL,反应温度为65℃。应用该体系在45 min内能检测出2×10^(-4)ng/μL的裸黑粉菌,在60 min内能检测出2×10^(-4)ng/μL的大麦坚黑粉菌,即在60 min内可检测出2×10^(-4)ng/μL的大麦坚黑粉菌和裸黑粉菌。建立的青稞黑穗病菌LAMP检测体系对大麦坚黑粉菌和祼黑粉菌具有特异性。【结论】建立了青稞黑穗病菌的LAMP检测体系,该体系能在1 h内检测出2×10^(-4)ng/μL的裸黑粉菌和大麦坚黑粉菌。

青稞坚黑穗病LAMP快速检测技术的建立

由大麦坚黑粉菌(Ustilgo hordei)引起的坚黑穗病广泛分布于我国青稞主产区,病原侵染后形成病穗从而造成产量损失。基于前期初步建立的青稞黑穗病快速检测体系,通过对种子洗涤沉淀物的总基因组DNA进行提取,并进行环介导等温扩增技术(loop-mediated isothermal amplification,LAMP)检测人工模拟及实际种子带菌情况,以期建立完善的青稞坚黑穗病快速检测技术。结果表明,裂解液快速提取法可以对样品总DNA进行有效提取,完善后的LAMP快速检测技术可以有效开展青稞种子携带大麦坚黑粉菌的检测。