基于URP-PCR多态性片段的苦瓜枯萎病菌特异性检测技术的建立

 通过URP(Universal Rice Primers)-PCR分析尖孢镰孢菌苦瓜专化型基因组DNA扩增片段多态性,筛选检测尖孢镰孢菌苦瓜专化型的特异性引物,并建立了基于该引物的PCR检测方法。结果表明,特异性引物为FOMM-SPF/FOMM-SPR, PCR检测体系为25 SymbolmAL,包括2SymboltB Green Taq Master Mix 12.5 SymbolmAL,10 mmol·L^-1 的上下游引物各1 SymbolmAL,模板DNA 1 SymbolmAL,灭菌去离子水补足至25 SymbolmAL;PCR程序为95℃预变性3 min,94℃变性15 s,57℃退火30 s,72℃延伸20 s,共30个循环,循环结束后72℃延伸5 min;特异性扩增片段大小294 bp,检测灵敏度为2 ng·μL^-1 DNA或50个孢子·500 mg^-1土壤。该引物及其检测方法对尖孢镰孢菌苦瓜专化型的检测特异性好、灵敏度高,可以从土壤和植物样品中快速准确地检测出苦瓜枯萎病菌,无需病原菌的分离培养和致病性检测,对苦瓜枯萎病的早期诊断和预警及有效防控具有重要的指导意义。     

大豆根腐病致病镰孢菌的多重PCR检测技术

为建立大豆根腐病镰孢菌的多重PCR检测方法,以四川大豆根腐病致病菌包括尖孢镰孢菌、腐皮镰孢菌、禾谷镰刀菌和木贼镰孢菌为对象,设计镰孢菌翻译延伸因子基因EF-1α的种特异引物,建立多重PCR扩增体系,并进行优化与验证。结果表明:25μL体系为最优镰孢菌多重PCR扩增体系,4种镰孢菌等体积混合DNA 4.0μL,各镰孢菌特异正向引物1.0μL,共用反向引物4.0μL,最佳退火温度为54℃,当循环30次时,能清晰地扩增出各镰孢菌EF-1α条带,对4种镰孢菌混合DNA的检测灵敏度可达0.1 ng/μL。室内环境样本验证结果表明,依据EF-1α扩增片段大小,该体系能够特异地检测出大豆黄化苗与致病镰孢菌混合样本中的镰孢菌,但无法从其它真菌的DNA中扩增获得目的片段。表明基于EF-1α基因特异引物建立的镰孢菌多重PCR检测技术可快速、特异地检测大豆根腐病镰孢菌。     

尖镰孢菌EST-SSR遗传多样性分析及通用性评价

为了解38株尖镰孢菌的遗传多样性并开发可在近缘镰孢菌种中通用的尖镰孢菌EST-SSR标记,利用设计和筛选的18对多态性EST-SSR引物对38株尖镰孢菌和5种近缘镰孢菌进行SSRPCR扩增,经6%非变性聚丙烯酰胺凝胶分离扩增产物,并用NTSYS软件分析供试尖镰孢菌的PCR扩增结果。结果表明,18对EST-SSR标记引物在38株尖镰孢菌中检测到75条多态性条带,多态性比率达92.6%,平均每对引物可扩增4.2条;各菌株间的遗传相似系数介于0.565~0.946之间,平均为0.721;来源于同科寄主植物群体的菌株间的平均遗传相似系数以葫芦科最大,锦葵科最小,依次为葫芦科兰科豆科亚麻科茄科锦葵科。在相似系数为0.756时,供试38株菌有35株按照不同科寄主植物聚为不同的类群,说明尖镰孢菌SSR类群的划分与其寄主来源具有一定的相关性。18对EST-SSR引物在近缘镰孢菌种中均能有效扩增的引物数及通用性比率为10对和55.6%,均显示多态性的引物有2对,占供试引物总数的11.1%。表明尖镰孢菌ESTSSR区域遗传多样性丰富,基于尖镰孢菌EST序列开发镰孢菌通用SSR标记是可行的。     

京津冀设施大棚根际土壤中筛选出的防治根腐病的生防镰孢菌

 由致病性尖孢镰孢菌(Fusarium oxysporum)引起的根腐病严重危害果蔬生产,但非致病性镰孢菌可作为潜在的生防菌。为筛选防治根腐病的非致病生防镰孢菌,从京津冀设施大棚采集茄科、葫芦科果蔬78份根际土样中分离2 402株真菌,筛选出对致病性尖孢镰孢菌(F. oxysporum)具有拮抗效果的真菌173株。利用镰孢菌通用引物进行PCR扩增,从中筛选出28株候选镰孢菌;通过镰孢菌发酵液泡根进行安全性测试,筛选出对寄主黄瓜幼苗安全无害的镰孢菌菌株4株(1418、1441、1436和1473)。进一步通过镰孢菌测序通用引物TEF1αF/TEF1αR结合菌落和分生孢子的形态学特征,1418菌株和1441菌株被鉴定为尖孢镰孢菌(F. oxysporum)、1436菌株被鉴定为茄病镰孢菌(F. solani)。盆栽测试发现,除1441菌株外,1418菌株、1436菌株和1473菌株对黄瓜根腐病的防效均在50%以上,其中1418菌株的防效为70%,与杀菌剂咪酰胺的防效相当,具有很好的应用潜力。本研究筛选获得的具有生防潜力的镰孢菌不仅为镰孢菌致病力分化的研究提供了实验材料,也为新型生防产品的研制奠定了基础。     

快速检测马铃薯干腐病病原接骨木镰孢的环介导等温扩增技术

 本研究基于环介导等温扩增技术(loop-mediated isothermal amplification, LAMP),建立了一种快速、准确和灵敏的接骨木镰孢的检测技术。通过比对接骨木镰孢与其近源种之间的候选靶标序列,选取TEF1-α(translation elongation factor 1-α,翻译延伸因子)基因作为靶标,设计并筛选出一套对该病原菌具有种特异性的LAMP引物,建立了检测接骨木镰孢的 LAMP 体系。该体系在反应前加入染料羟基萘酚蓝(hydroxynaphthol blue,HNB),经62℃恒温反应70 min之后,可根据肉眼观察到的反应物的颜色判定结果。特异性分析结果表明,仅接骨木镰孢的DNA经检测后呈天蓝色的阳性反应,而其他供试菌株的DNA均呈紫色的阴性反应。该方法对DNA的最低检测限为100 pg·μL^-1。在采自内蒙古和黑龙江的28份马铃薯干腐病疑似病害样本中,检测到14份阳性样品。该方法的建立为接骨木镰孢的检测及其所致病害的诊断提供了快捷准确的技术。     

建兰胶孢炭疽菌ITS序列分析及其PCR快速检测

由胶孢炭疽菌Colletotrichum gloeosporioides引起的炭疽病是建兰的重要病害.为建立快速检测该病原菌的方法,以ITSl/ITS4为引物,对15个建兰胶孢炭疽菌的ITS进行PCR扩增及测序,将测定的序列与炭疽菌属其它种的ITS序列进行比对分析,设计特异性引物CFl/CR1,并通过常规和巢式PCR对建兰胶孢炭疽菌进行检测.结果显示,15个菌株中有13个菌株ITS序列与该菌的模式种序列相似性高达99％以上,而另外2个菌株相似性则为86％;供试菌株在系统发育树上聚为2个不同的分支;引物CFl/CR1通过常规PCR可从1 ng的建兰胶孢炭疽菌基因组DNA中扩增到目的条带,而利用引物ITSl/ITS4和CF1/CR1通过巢式PCR可从1 pg的基因组DNA中扩增到目的条带,即巢式PCR反应检测灵敏度较常规PCR至少高1 000倍.表明建立的巢式PCR法可从自然感病的建兰叶片组织中检测到胶孢炭疽菌.     

Fusarium boothii特异性PCR检测方法的建立与应用

根据报道的Fusariumspp.的reductase-like基因序列,设计合成了1对用于Fusarium boothii的特异性检测引物F-Fg/R-Fg。利用该对引物对包括F.boothii在内的35株镰刀菌的基因组DNA进行了扩增。结果表明:该引物特异性强,仅从F.boothii基因组DNA中扩增出300bp左右的特异性条带,其他参照菌株及阴性对照均无任何条带;灵敏度验证结果表明,该检测法可以检测出50pg F.boothii基因组DNA。     

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

为快速、准确地对番茄煤污假尾孢Pseudocercospora fuligena进行检测与定量分析,基于其Avr4基因设计特异性引物JWB-9F/JWB-7R,建立实时荧光定量PCR检测技术,分析该检测技术的特异性和灵敏度,并利用采集自重庆市、河北省和广西壮族自治区的14份材料对该检测技术的应用效果进行验证。结果表明,引物JWB-9F/JWB-7R仅可从番茄煤污假尾孢基因组DNA中扩增出232 bp的目的片段,特异性良好;实时荧光定量PCR检测技术的灵敏度为67.09 copies/μL,是普通PCR检测技术的1 000倍。且该实时荧光定量PCR检测技术可以实现未显症样本中番茄煤污假尾孢的定量检测,检测限为6.02×10~2copies/μL,实际应用效果较好。表明所建立的实时荧光定量PCR检测技术可用于番茄煤污假尾孢叶斑病的早期诊断和预测预报。     

引起玉米穗腐病的两种镰孢菌双重PCR快速检测体系的建立

禾谷镰孢(Fusarium graminearum)和拟轮枝镰孢(Fusarium verticillioides)是引起玉米穗腐病的两种主要病原菌。为了建立这两种病原菌的快速和定量检测体系,本研究分别设计了针对F.graminearum和F.verticillioides的基因特异性引物,建立了双重PCR反应体系,并从DNA浓度、引物浓度和退火温度3个方面对反应体系进行了优化。结果表明,退火温度为54℃和58℃时扩增效果较好,DNA模版的检测灵敏度可以达到6.25 ng·μL~(-1);F.graminearum和F.verticillioides引物最佳终浓度配比为0.2μmol·L~(-1)/0.4μmol·L~(-1)。本研究建立的双重PCR对同时鉴别引起玉米穗腐病的两种主要镰孢菌提供了准确、快速、灵敏的检验检疫技术。     

玉米圆斑病病原的快速检测

玉米生平脐蠕孢菌(Bipolaris zeicola)是引起玉米圆斑病的病原菌。本研究通过对玉米生平脐蠕孢菌及其近似种的EF-1α基因(elongation factor 1α)部分序列进行比对,设计出玉米生平脐蠕孢菌的特异性引物Y-EF-F和Y-EF-R,利用该引物可以从B.zeicola中扩增出137 bp的特异片段,而其余的17个参试菌株扩增结果为阴性。灵敏度实验表明该对引物可以检测到目标DNA的浓度为1 pg·μL~(-1)。用B.zeicola接种玉米叶片、苞叶以及玉米粒,然后以接种发病的病组织DNA为模板,利用引物Y-EF-F和Y-EF-R进行PCR扩增,可以扩增出137 bp的特异性条带,而健康玉米组织DNA中未能扩增出任何条带。用B.zeicola孢子悬浮液接种大田玉米叶片,接种第3 d可以检测到未发病组织中有B.zeicola病原菌,第5 d可以看到明显的病斑。研究结果表明该方法可用于快速、准确和灵敏地检测玉米组织中的潜伏期玉米生平脐蠕孢菌,为玉米圆斑病的快速检测,进而及早采取防治措施提供积极的指导。     

Comparison of genetic diversity and pathogenicity of fusarium head blight pathogens from China and Europe by SSCP and seedling assays on wheat

The genetic diversity and pathogenicity of isolates of Fusarium graminearum and F. asiaticum isolated from wheat heads in China were examined and compared with those of isolates of F. graminearum , F. asiaticum and F. meridionale from Europe, USA and Nepal. Genetic diversity was assessed by SSCP (single strand conformation polymorphism) and AFLP (amplified fragment length polymorphism) analysis and by molecular chemotyping. SSCP analysis of the Fg16F/Fg16R PCR amplicon differentiated F. graminearum , F. asiaticum and F. meridionale and revealed three haplotypes among sequence-characterized amplified region (SCAR) type 1 F. graminearum isolates. AFLP analysis showed a high level of genetic diversity and clustered the majority of Chinese isolates in one group along with other isolates of Asian origin. The second cluster contained F. graminearum isolates from China, Europe and the USA. Of the Chinese isolates, 79% were F. asiaticum and 81% of these were of the 3-AcDON chemotype, with only 9·5% of either chemotype 15-AcDON or NIV. All the Chinese and USA isolates of F. graminearum were 15-AcDON, whereas among the isolates from Europe, 21% were NIV and 8% were 3-AcDON chemotype. No evidence was found for possible differences in aggressiveness between F. graminearum and F. asiaticum . Highly aggressive isolates were present in each region and no evidence was found for any association between aggressiveness and geographical origin or chemotype among the isolates examined. No difference was observed in pathogenicity towards wheat seedlings between Chinese isolates and those from Europe, the USA or Nepal.     

分子检测土壤中南美大豆猝死综合症病菌和北美大豆猝死综合症病菌

对南美大豆猝死综合症病菌（Fusarium tucumaniae）和北美大豆猝死综合症病菌（Fusarium virguliforme）rDNA基因间间隔区（IGS）进行分析,设计并筛选出3对特异性引物FT1/FT6、FT1/FT9和FV1/FV1A。分别利用FT1/FT6、FT1/FT9进行PCR反应,对F.tucumaniae分别扩增出250bp、656bp的特异性片段,而F.virguliforme、F.brasiliense、F.cuneirostrum和F.phaseoli等近似种均无特异性PCR产物出现。利用FV1/FV1A进行PCR反应,F.virguliforme出现228bp特异性PCR产物,而F.tucumaniae、F.brasiliense、F.cuneirostrum和F.phaseoli等近似种无特异性PCR产物。引物FT1/FT6、FV1/FV1A检测F.tucumaniae和F.virguliforme的最低DNA含量为1pg/μL,利用FT1/FT6和FT1/FT9对土壤中的病菌进行巢式PCR,能检测到接种量为每g土壤含100个大分生孢子的F.tucumaniae,FV1/FV1A能检测到接种量为每g土壤含1000个大分生孢子的F.virguliforme。     

马铃薯干腐病优势病原菌Fusarium sambucinum 分子检测技术的建立

马铃薯干腐病是马铃薯最重要的贮藏期病害之一,现已成为马铃薯贮藏期烂窖的重要原因。实现病原菌的快速检测对病害诊断和科学防控具有重要的实践意义。本研究基于镰刀菌翻译延伸因子序列设计了一对检测接骨木镰刀菌Fusarium sambucinum的特异引物Fs-F/Fs-R。该特异引物可从接骨木镰刀菌中获得309bp的特异性扩增片段,而其他种类镰刀菌及马铃薯重要病害病原菌中均无此片段,说明该引物具有专一性。该体系的灵敏度检测结果表明,最低能检测到的接骨木镰刀菌基因组DNA浓度为70pg/μL。该引物也适用于发病马铃薯块茎中接骨木镰刀菌的快速检测。     

尖镰孢菌(Fusarium oxysporum)的快速分子检测

 由尖镰孢菌(Fusarium oxysporum Schlecht.)引起的大豆枯萎病是危害大豆生产的主要土传病害^［1］。该菌在土壤和病残体上均可长期生存造成危害。快速准确地在发病初期植株和带病土壤中进行鉴定和检测对防治该病害至关重要。     

小麦赤霉病流行区镰刀菌致病种及毒素化学型分析

 为从分子水平上明确小麦赤霉病流行区镰刀菌致病种及其B 型毒素化学型的分布特点,本研究对2008 年度采自四川、重庆、湖北、安徽、江苏、河南6 省33 县市的赤霉病穗上分离获得的433 个镰刀菌单孢菌株,用鉴定种和鉴定B 型毒素化学型的特异性引物进行了鉴定分析。致病种检测结果表明,四川病穗检测到Fusarium asiaticum、F. graminearum、F.avenaceum 和F. meridionale 4 个镰刀菌种,重庆、湖北、安徽和江苏病穗检测到F. asiaticum 和F. graminearum 2 个种,河南病穗仅检测到F. graminearum 1 个种。毒素化学型检测结果表明,Nivalenol(NIV)是四川和重庆镰刀菌主要毒素化学型,Deoxynivalenol(DON)是湖北、河南、安徽和江苏镰刀菌主要毒素化学型;将DON 化学型进一步划分为3-AcDON 和15-AcDON 显示,四川、湖北、江苏镰刀菌毒素以3-AcDON 为主,安徽镰刀菌毒素为3-AcDON 和15-AcDON 两者参半,河南镰刀菌全部产生15-AcDON。结果揭示,F. asiaticum 是四川、重庆、湖北和江苏等赤霉病流行麦区的优势致病种;镰刀菌产生的DON 和NIV 毒素化学型存在明显的地域分布,长江上游的麦区以NIV 为优势化学型,长江中下游麦区以DON 为优势化学型;镰刀菌致病种与DON 毒素的化学型间存在一定关系。     

Trichothecene mycotoxin genotypes of Fusarium graminearum sensu stricto and Fusarium meridionale in wheat from southern Brazil

A total of 82 fungal isolates was obtained from wheat kernel samples affected by fusarium head blight collected from 20 locations in southern Brazil. Polymerase chain reaction (PCR) assays were used to characterize trichothecene mycotoxin genotypes [deoxynivalenol (DON), nivalenol (NIV) and two acetylated derivatives of DON]. To identify isolates that producing DON and NIV, portions of the Tri13 gene were amplified. To identify 3-acetyl-deoxynivalenol (3-ADON) and 15-acetyl-deoxynivalenol (15-ADON) genotypes, portions of Tri3 and Tri12 were amplified. Nearly all of the isolates studied (76/82) were of the DON/15-ADON genotype. Six of the isolates were of the NIV genotype. The DON/3-ADON genotype was not observed. Portions of three genes were sequenced from representative isolates of the NIV and DON/15-ADON genotypes and compared with sequences from curated reference isolates of Fusarium in GenBank. blast queries for individual gene sequences and pairwise comparisons of percentage identity and percentage divergence based on 1676 bp of concatenated DNA sequence suggested that the isolates representing the DON/15-ADON genotype were Fusarium graminearum sensu stricto and the isolates representing the NIV genotype were Fusarium meridionale . This is the first detailed report of trichothecene mycotoxin genotypes of F. graminearum and F. meridionale in Brazil.     

Identification of Race 1 of Fusarium oxysporum f. sp. lactucae on Lettuce by Inter-Retrotransposon Sequence-Characterized Amplified Region Technique

ABSTRACT Fusarium wilt of lettuce, caused worldwide by Fusarium oxysporum f. sp. lactucae, is an emerging seed-transmitted disease on Lactuca sativa. In order to develop a molecular diagnostic tool for identifying race 1 (VCG0300) of the pathogen on vegetable samples, an effective technique is presented. Inter-retrotransposon amplified polymorphism polymerase chain reaction (PCR), a technique based on the amplification of genomic regions between long terminal repeats, was applied. It was shown to be useful for grouping F. oxysporum f. sp. lactucae race 1 isolates. Inter-retrotransposon sequence-characterized amplified regions (IR-SCAR) was used to develop a specific set of PCR primers to be utilized for differentiating F. oxysporum f. sp. lactucae isolates from other F. oxysporum isolates. The specific primers were able to uniquely amplify fungal genomic DNA from race 1 isolates obtained in Italy, Portugal, the United States, Japan, and Taiwan. The primers also were specific to pathogen DNA obtained from artificially infected lettuce seed and naturally and artificially infected plants.     

禾谷镰孢菌产玉米赤霉烯酮毒素zearalenone的PCR检测

玉米赤霉烯酮（zearalenone,ZEN）是由镰孢菌产生的真菌毒素,该毒素具有雌性激素生物活性。PKS4基因是禾谷镰孢菌中玉米赤霉烯酮生物合成途径中的必需基因。根据PKS4基因序列,设计一对PKS4基因特异性引物,通过检测PKS4基因的存在间接检测ZEN毒素的产生。特异引物在禾谷镰孢菌菌株以及被禾谷镰孢菌侵染的小麦籽粒中都能稳定地扩增出大小为1 076 bp的特异片段,扩增片段与PKS4基因（DQ019316）相同区段序列相似性达99.63%。同时,酶联免疫吸附法（ELISA）验证了PCR的检测结果,证明了该技术的可靠性。     

利用伏马毒素合成基因对玉米种子寄藏镰刀菌的分子检测

我国玉米种子普遍受到拟轮生镰刀菌(Fusarium verticillioides)的侵染,该菌产生的伏马毒素对国家种质库中玉米种质的安全保存有着潜在的影响。fum1基因是F.verticillioides等镰刀菌中伏马毒素生物合成的必需基因。选用3对已知引物Fum5F/Fum5R、P1/P2和P3/P4分别对从玉米种子中分离出的9株镰刀菌和1株阴性对照菌链格孢菌进行PCR扩增检测,在F001和F003菌株中扩增出相应的特异性表达片段。测序表明,这些片段的长度分别为846bp、888bp和703bp,与已知fum1基因(AF155773)的同源性达99%以上。3对引物的检测灵敏度达到88pg/mL。结果表明,这3对引物都能够有效地检测产生伏马毒素的镰刀菌菌株,但引物Fum5F/Fum5R所扩增片段完全来自fum1基因内部,具有更强的特异性。在此定性检测基础上,需要进一步研究定量检测方法并进一步研究伏马毒素对农作物种质保存的影响。     

Rapid preparation of Fusarium DNA from cereals for diagnostic PCR u sing sonification and an extraction kit

Several PCR methods have recently been developed for Fusarium analysis in pure cultures. To use these new techniques in mycological studies and in industrial quality control, a protocol was set up for the rapid preparation of fungal DNA from cereals. An ultrasonification probe (sonotrode) and a lysis buffer were used for mechanical lysis of mycelia from infected grains. Following ultrasonification, DNA was isolated using a commercially available kit. DNA preparation was completed within 5 min per sample. The method resulted in DNA of sufficient quality and quantity for diagnostic PCR. Group- and species-specific primers were used to detect DNA of Fusarium graminearum and F. culmorum in species-specific assays as well as trichothecene-producing Fusarium spp. in a group-specific system. A minimum of one F. graminearum -infected grain added to an uninfected 40 g wheat sample was detectable with a species-specific PCR. The PCR signals produced with primers specific for the tri5 gene of trichothecene-producing Fusarium spp. and with primers for the detection of F. graminearum (gaoA) were in accordance with corresponding concentrations of deoxynivalenol (DON) found in samples by HPLC analysis. The speed of the protocol developed may promote the use of PCR in routine applications in an agro-industrial context.