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利用常规PCR和实时荧光定量PCR检测杨梅凋萎病菌
Use of conventional and real-time quantitative PCR to detect Pestalotiopsis,the cause of bayberry twig blight

查看参考文献31篇

文摘 凋萎病是近年来危害杨梅的主要病害。为了快速灵敏的检测杨梅凋萎病菌(Pestalotiopsis versicolor和P. microspora),本研究开发了常规PCR和SYBR Green实时荧光定量PCR技术各一套。利用P. versicolor(JN861773)和P. microspora(JN861776)的ITS1-5.8S rDNA-ITS2序列的相同部分设计引物对(Pvm1L/Pvm1R)。该引物对利用常规PCR技术能特异性扩增出杨梅凋萎病菌188 bp的目标产物,而对照菌株则呈阴性。该常规PCR体系能够检测人工接种后21 d和田间自然发病的有病症杨梅组织中的凋萎病菌,检测下限是0.6×10~5拷贝数。利用Pvm1L/Pvm1R进行SYBR Green实时荧光定量PCR,检测灵敏度是常规PCR的100倍,检测下限是0.6×10~3拷贝数,能够检测出人工接种及田间已经感染但尚未表现症状的杨梅组织中的凋萎病菌。这两项技术,简单、快速、灵敏,特异性强,可以应用于杨梅凋萎病的诊断和苗木检疫。
其他语种文摘 Twig blight disease is one of the main diseases on bayberry(Myrica rubra Sieb.& Zucc). We developed an effective method to detect and quantify the pathogens Pestalotiopsis versicolor and P. microspora by using conventional PCR and SYBR Green real-time PCR. A primer set,Pvm1L/Pvm1R,was designed based on a conserved sequence of the internal transcribed spacer(ITS1-5.8S rDNA-ITS2) region of the ribosomal DNA gene of P. versicolor(JN861773) and P. microspora(JN861776). The 188 bp DNA fragments were amplified from 30 isolates of P. versicolor and 30 isolates of P. microspora,and no product was amplified from isolates of 11 other fungal genera. Conventional PCR was able to detect the pathogens on symptomatic and artificially infected bayberry plants at 21 days after inoculation,and the detection limit was 0.6×10~5 copies of the Pestalotiopsis DNA. In addition,the Pvm1L/Pvm1R primer set were successfully adapted to SYBR Green real-time PCR, which had a limit 100 times lower(0.6×10~3) than that by conventional PCR and was able to detect the pathogens in symptomless,artificially inoculated,and naturally infected plants. The conventional and SYBR Green real- time PCR developed in this study were simple,fast,sensitive,and specific,and can be used to detect Pestalotiopsis spp. from infected bayberry in the field.
来源 植物病理学报 ,2016,46(1):1-10 【核心库】
DOI 10.13926/j.cnki.apps.2016.01.001
关键词 杨梅 ; 凋萎病菌 ; 常规PCR ; SYBR Green实时荧光定量PCR ; 分子检测
地址

浙江省农业科学院园艺研究所, 杭州, 310021

语种 中文
文献类型 研究性论文
ISSN 0412-0914
学科 植物保护
基金 浙江省重大科技专项重点农业项目 ;  国家公益性行业(农业)科研专项
文献收藏号 CSCD:5653978

参考文献 共 31 共2页

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引证文献 9

1 康华军 番茄煤污假尾孢叶斑病菌实时荧光定量PCR检测技术的建立及应用 植物保护学报,2019,46(6):1214-1221
CSCD被引 3

2 任海英 杨梅凋萎病菌侵染、传播及树体内分布规律 浙江农业学报,2016,28(4):630-639
CSCD被引 4

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