基于ITS与factor,1alpha序列桉树焦枯病菌的双重PCR快速检测
摘要
桉树焦枯病是威胁桉树生长的首要病害,建立准确、有效的桉树焦枯病的PCR快速检测技术是桉树焦枯病前期诊断的必要手段。试验以桉树焦枯病原菌(Calonectria morganii) DNA为模板,分别以ITS和factor 1alpha序列为靶区域,针对Calonectria属和C.morganii设计了CYS1/CYS2和EFS1/EFA1两对特异性引物,建立了基于属和种的双重PCR快速检测技术。利用引物CYS1/CYS2可以从全部Calonectria属的供试菌株中扩增出一条351 bp大小的条带,单独用特异性引物EFS1/EFA1进行PCR扩增,仅病原菌扩增出197 bp的条带,同时使用2对引物时,病原菌可扩增出两条明亮条带。当体系退火温度为53 ℃时,DNA灵敏度检测限度达到450 fg/μL。野外田间时效检测结果显示,该体系能准确检测出不同发病程度桉树组织上的病原菌,完全符合田间检测的要求。这是关于桉树焦枯病快速检测的首次报道。
关键词
桉树焦枯病;桉树焦枯病原菌;快速检测;PCR扩增
中图分类号:
S 432.44
文献标识码:A
DOI:10.3969/j.issn.05291542.2015.05.019
Abstract
Eucalyptus dieback is the primary threat to the growth of eucalyptus. It is necessary to establish an accurate and effective PCR rapid detection technique for the early diagnosis of this disease. The duplex PCR technique, for rapid detection of genera and species of eucalyptus dieback disease pathogen was established with the total DNA as templates, and two pairs of specific primers (CYS1/CYS2 and EFS1/EFA1) for Calonectria de Not and C.morganii based on their ITS sequence and factor 1alpha gene were designed, respectively. The results showed that all tested strains belonging to Calonectria genera were amplified a product of 351 bp using primers CYS1/CYS2, while only C.morganii strains were amplified a product of 197 bp using primers EFS1/EFA1, and the duplex PCR with these two pairs of primers could amplify the two products. Furthermore, at the annealing temperature of 53 ℃, the minimum amount of detected DNA ...
|
== 试读已结束,如需继续阅读敬请充值会员 ==
|
|
本站文章均为原创投稿,仅供下载参考,付费用户可查看完整且有格式内容!
(费用标准:38元/2月,98元/2年,微信支付秒开通!) |
| 升级为会员即可查阅全文 。如需要查阅全文,请 免费注册 或 登录会员 |
|
