侵染肥城桃的病毒和类病毒的分子检测与鉴定

为明确山东肥城桃种植区桃树上主要存在的病毒和类病毒及其发生情况,采集具有花叶、斑驳和皱缩典型症状的肥城桃样品,提取叶片总RNA后,分别选用桃树上已报道的啤酒花矮化类病毒Hopstuntviroid(HSVd)、桃潜隐花叶类病毒Peach latent mosaic viroid(PLMVd)、苹果褪绿叶斑病毒Apple chlorotic leaf spot virus(ACLSV)、樱桃锉叶病毒Cherry rasp leaf virus(CRLV)、桃花叶病毒Peach mosaic virus(PMV)、李属坏死环斑病毒Prunus necrotic ringspot virus(PNRSV)、李痘病毒Plum pox virus(PPV)、李矮缩病毒Prunus dwarf virus(PDV)、樱桃绿环斑驳病毒Cherry green ring mottle virus(CGRMV)、杏假褪绿叶斑病毒Apricot pseudo-chlorotic leaf spot virus(APCLSV)、李树皮坏死茎纹孔伴随病毒Plum bark necrosis stem pitting-associated virus(PBNSPaV)和小樱桃病毒1号Little cherry virus 1(LchV1)的特异性引物进行RT-PCR检测。PCR结果显示仅HSVd、PLMVd、ACLSV、PNRSV和PBNSPaV的扩增产物中得到了预期大小的目的片段,将目的片段克隆测序后,经NCBI BLAST比对发现,山东肥城桃分离物HSVd、PLMVd、ACLSV、PNRSV和PBNSPaV与GenBank已报道分离物序列一致性均达90%以上。表明山东肥城桃已感染HSVd、PLMVd 2种类病毒和ACLSV、PNRSV、PBNSPaV 3种病毒。     

我国梅树上病毒及类病毒的检测和鉴定

目前, 我国梅树上的病毒种类及发生情况仍不完全清楚。本研究从北京、武汉、南京和无锡的梅园中采集了64份疑似感染病毒的叶片样品, 通过RT-PCR和斑点杂交, 对7种病毒和2种类病毒进行了检测。共检测到6种病毒和1种类病毒。其中, 李属坏死环斑病毒(prunus necrotic ringspot virus, PNRSV)和桃潜隐花叶类病毒(peach latent mosaic viroid, PLMVd)为我国梅树上的首次检出。PNRSV、亚洲李属病毒2号(Asian prunus virus 2, APV2)、桃叶痘伴随病毒(peach leaf pitting-associated virus, PLPaV)的检出率高于30%。综合考虑病毒的分布及检出率, PLPaV、APV2、PNRSV和李树皮坏死茎痘伴随病毒(plum bark necrosis stem pitting-associated virus, PBNSPaV)是武汉、南京和无锡梅树上的主要病毒。此外, 通过克隆和测序, 获得了PLMVd和梅树病毒A(mume virus A, MuVA)的基因组, PLPaV的RNA1组分和PNRSV外壳蛋白(CP)基因序列。序列比较分析显示, 我国PLMVd梅分离物和PNRSV梅分离物与我国桃分离物亲缘关系最近, 表明PLMVd和PNRSV可能在梅和桃树间交互侵染;我国MuVA梅分离物序列与日本梅分离物序列的相似性高达98.56%;PLPaV梅分离物与我国桃分离物之间序列变异较大。上述结果不仅进一步明确了我国梅树上的病毒及类病毒种类和分布情况, 而且有助于深入了解它们的流行与传播。     

桃潜隐花叶类病毒中国分离株P3的克隆与序列分析

 本研究以提取的类病毒cRNA为模板,采用RT-PCR方法,从5株表现明显花叶症状的"雨花露"桃树上检测到桃潜隐花叶类病毒(PLMVd),并对其中的样品P₃通过2次RT-PCR扩增,然后分别将扩增产物回收、克隆测序,确定了该分离株(命名为PLMVd-P₃分离株)的全长核苷酸序列,其cDNA分子全长为337 nt,这与已经报道的PLMVd典型分离株基因组大小相似。序列比较分析结果表明,该分离株与已经报道的不同地区来源的其它分离株相似性为90%~96%。     

马铃薯纺锤块茎类病毒的检测和防治

马铃薯纺锤块茎类病毒病(potato spindle tuber viroid,PSTVd)是一种严重为害马铃薯生产的病害,降低产量20%—30%。防治的主要措施是应用无类病毒的种薯。由于目前还没有脱掉类病毒的有效措施,只能从未被饱和侵染的群体中鉴定筛选出未被侵染的个体,再脱掉其它病毒,作为核心繁殖材料。1987年以来,利用自制的电泳设备,以往复聚丙烯酰胺凝胶电泳法(return-polyacrylamide gel electrophoresis,R-PAGE)检测类病毒,筛选出未感病的个体,再用茎尖组织培养法脱掉其它病毒。经用马铃薯卷叶病毒等8种病毒酶标抗体鉴定筛选,获得既无类病毒也无主要马铃薯病毒的克新1、2、3和4号等主栽马铃薯品种的核心种。并已提供给省内外的良种场繁殖推广。1989和1990年抽样检测克山良种场繁殖的原种、一级和二级良种,未检测到类病毒。     

应用酶联免疫吸附试验法鉴定几种主要马铃薯病毒

制备了PVX,PVY_o,PVY~n,PVA,PVS,PVM,PLRV和TRV等8种主要马铃薯病毒抗体的辣根过氧化物酶结合物,在检测黑龙江省马铃薯主栽品种克新一、二、三、四号等品种的植株样品1155份和800余份正在脱毒中的试管苗样品中,发现上述8种马铃薯病毒在几个主栽品种中的侵染率较高,而且大多数感病植株是由3至7种病毒复合侵染,并首次查明本省存在PVY~n和PVM病毒。对不带上述8种病毒的样品又用双向反向聚丙烯酰胺凝胶电泳鉴定带马铃薯纺锤块茎类病毒(Potato spindle Tuber Viroid)状况,现已获得无上述8种病毒和类病毒的种植材料。     

啤酒花矮化类病毒实时荧光定量RT-PCR检测方法的建立与应用

为建立一种快速、灵敏、特异的定量检测啤酒花矮化类病毒(Hop stunt viroid,HSVd)的实时荧光定量RT-PCR (RT-qPCR)方法,设计了2对引物及特异探针,体外转录制备了RNA标准品,绘制标准曲线,并对该方法的特异性、灵敏度和重复性进行评估.建立的定量标准曲线Ct值与模板拷贝数对数之间呈良好的线性关系,相关系数R2为0.9988,扩增效率为95％;该方法的特异性好,与啤酒花潜隐类病毒(HLVd)、葡萄黄斑类病毒1(GYSVd-1)、葡萄黄斑类病毒2(GYSVd-2)和桃潜隐花叶类病毒(PLMVd)均无交叉反应;灵敏度为1.0×102拷贝/μL,比普通RT-PCR高10倍;试验内及试验间重复性试验的变异系数均小于3％.研究表明该方法适用于实际样品中HSVd的快速定量检测.     

山东泰安甜樱桃“花叶病”树体症状观察及病毒检测

为了探明山东泰安患有"花叶病"的甜樱桃树体内感染病毒的种类,本研究以嫁接在3种不同砧木上的甜樱桃品种‘红灯’叶片为试验材料,提取植物样本总RNA,采用随机六聚体引物反转录,选取10种甜樱桃病毒作为检测对象,根据各病毒基因组序列设计特异引物,进行RT-PCR检测。结果显示,10种甜樱桃待检病毒中,5种病毒检测结果呈阳性,分别为PNRSV(Prunus necrotic ringspot virus,PNRSV)、PDV(Prune dwarf virus,PDV)、CVA(Cherry virus A,CVA)、CGRMV(Cherry green ring mottle virus,CGRMV)、LChV-2(Little cherry virus-2,LChV-2),各病毒检出率较高。各"花叶病"甜樱桃样品均至少同时感染2种病毒,多病毒复合感染比例较高。     

河南甜樱桃病毒病害调查及病原检测

在河南省郑州市、巩义市、荥阳市、新郑市选择具有代表性的甜樱桃生产园对病毒病发生情况进行调查,采集表现为疑似病毒病症状的样本65份,利用7种病毒引物进行RT-PCR检测。5种病毒检测结果呈阳性,分别是李属坏死环斑病毒(Prunus necrotic ringspot virus,PNRSV)、李矮缩病毒(Prune dwarf virus,PDV)、樱桃绿环斑驳病毒(Cherry green ring mottle virus,CGRMV)、樱桃坏死锈斑病毒(Cherry necrotic rusty mottle virus,CNRMV)及樱桃病毒A(Cherry virus A,CVA);序列分析结果表明,5种病毒扩增片段与GenBank中注册的相应病毒核苷酸序列均具有较高的一致性;样本病毒检出率为100%,其中13份样本为单独侵染,其余52份样本均为多病毒复合侵染,占比高达80%,复合侵染比例随着侵染病毒种类的增多逐渐降低;病毒侵染组合与叶片表型症状无明显对应关系。     

纳米磁珠结合实时荧光RT-PCR技术检测大丽花潜隐类病毒

正大丽花潜隐类病毒(Dahlia latent viroid,DLVd)是Verhoeven et al.(2013)用Return-PAGE和s-PAGE技术从大丽花中鉴定出的一种新类病毒。根据2015年国际病毒分类委员会分类报告,DLVd为马铃薯纺锤形块茎类病毒科啤酒花矮化类病毒属成员。该病毒单独侵染时,大丽花没有明显的症状,其与马铃薯纺锤块茎类病毒(Potato spindle tuber viroid,PSTVd)复合侵染时可使大丽花叶片卷曲(Tsu-     

我国部分地区樱桃病毒病害初步调查和病原检测

对山东泰安、辽宁大连和北京的樱桃病毒病发生情况进行调查,发现8个果园/栽培区均有病毒病发生,主要症状为叶片皱缩、畸形、卷叶、花叶、植株矮缩等。采集20份样品,利用12种病毒的引物进行RT-PCR检测。结果表明,在样品中扩增出与樱桃病毒A(Cherry virus A,CVA)、李属坏死环斑病毒(Prunus necrotic ringspot virus,PNRSV),李矮缩病毒(Prune dwarf virus,PDV)、李树皮坏死与茎痘伴随病毒(Plum bark necrosis stem pitting-associated virus,PBNSPaV)、樱桃绿环斑驳病毒(Cherry green ring mottle virus,CGRMV)、樱桃小果病毒-1(Little cherry virus-1,LChV-1)预期大小一致的目的片段;序列分析表明,与GenBank中注册所测的病毒核苷酸序列均具有较高的一致性。其中,大连、泰安和北京样品均检测到CVA;大连和北京样品中检测到PNRSV和PDV;北京样品中检测到PBNSPaV;大连苗木样品枝条中检测到CGRMV和LChV-1。这是在我国樱桃上首次检测到LChV-1。     

玫烟色虫草和球孢白僵菌对朱砂叶螨和二斑叶螨的致病力评价

为探寻具有杀螨潜力的生防真菌,采用喷雾法测定分析玫烟色虫草Cordyceps fumosorosea IF-1106菌株和球孢白僵菌Beauveria bassiana BB-1339菌株对朱砂叶螨Tetranychus cinnabarinus和二斑叶螨Tetranychus urticae卵、幼螨及雌成螨的致病力。结果表明,感染玫烟色虫草IF-1106菌株和球孢白僵菌BB-1339菌株后螨类的形态特征不一致,感染IF-1106菌株后形成棉絮状菌丝,而感染BB-1339菌株后则形成羊毛状菌丝。IF-1106菌株和BB-1339菌株对朱砂叶螨和二斑叶螨卵的LC₅₀分别为2.38×10⁷、8.26×10⁷CFU/mL和4.48×10⁷、1.21×10⁸CFU/mL,对朱砂叶螨和二斑叶螨幼螨的LC₅₀分别1.97×10⁷、8.26×10⁷CFU/mL和7.65×10⁶、8.99×10^5...     

欧亚种葡萄自交F1代对白粉病和霜霉病的抗性遗传

采用田间自然鉴定、田间接种鉴定及室内离体叶圆片接种鉴定三种方法,研究了10个欧亚种葡萄品种(系)、一个欧山杂种及其493株自交后代幼苗对葡萄霜霉病及白粉病的抗性及遗传关系,同时对其自交后代抗白粉病和霜霉病的遗传趋势进行了分析.结果表明,供试品种(系)及其自交后代对霜霉病与白粉病的抗性存在极显著相关,自交后代对两病表现伴随遗传现象,初步推断这可能是由葡萄抗病基因的多效性引起.在欧亚种葡萄品种自交后代群体中,虽然90%以上都是感病性中等或高的类型,但仍能够得到一定比例(10%以下)抗病性强的类型,这为利用欧亚种葡萄品种进行自交或品种间杂交选育优质抗病新品种提供了依据.     

Antifungal activity of Datura stramonium, Calotropis gigantea and Azadirachta indica against Fusarium mangiferae and floral malformation in mango

Floral malformation caused by Fusarium mangiferae is a serious threat to mango cultivation in various countries. Different long-term measures suggested to control it were found to be unsuccessful. Present studies clearly showed strong antifungal activity of a concoction brewed from Datura stramonium, Calotropis gigantea, Azadirachta indica (neem) and cow manure (T₁) followed by methanol-water (70/30 v/v) extracts of Datura stramonium, Calotropis gigantea and Azadirachta indica (T₂) against Fusarium mangiferae. Optimal control of floral malformation was found in trees sprayed with T₁ followed by T₂ at bud break stage and again at fruit set stage when compared with the control. All the malformed buds or panicles completely dried two days after foliar spray with T₁ or T₂. In the trees treated with T₁ at fruit set stage, flower abscission was observed from the fourth day after spraying and all flowers dropped by the ninth day without requiring any manual de-blossoming, whereas in the control, the malformed panicles remained green and competed with the growing fruits for plant nutrients. In vitro culture of fresh malformed tissues in MS media along with T₁ or T₂ showed no growth of any fungus in the media. However, in vitro culture of the completely dry malformed tissues in MS media after foliar treatment with T₁ or T₂ revealed growth of F. mangiferae on the twenty fifth day indicating that the concoction-brewed compost (T₁) or methanol-water (70/30 v/v) extracts (T₂) could not completely eliminate the pathogen but helped in controlling malformation by suppressing the activity of F. mangiferae. Mango trees sprayed with T₁ and T₂ revealed significant differences in percent fruit set and retention when compared with the control. This could be due to observed higher levels of nitrogen, phosphorus, potassium, calcium, magnesium, copper, zinc, iron and manganese in T_1, followed by T₂ when compared with T₃ (control). Among the different fruit quality parameters analysed, the total flavonoids were found to be significantly higher in T₁ and T₂ when compared with T_3. The study proved that the concoction-brewed compost (T₁) is effective, inexpensive, easy to prepare and constitutes a sustainable and eco-friendly approach to control floral malformation in mango when it is sprayed at bud break stage and again at fruit set stage. In this present study, exogenous treatment of emerging buds with (T_c) further proved that with increase in the number of malformed panicles/tree the number of buds developing into healthy panicles/tree decrease.     

Application of RFLP analysis of recA, gyrA and rpoS gene fragments for rapid differentiation of Erwinia amylovora from Erwinia strains isolated in Korea and Japan

Restriction fragment length polymorphism (RFLP) analysis of the PCR amplified fragments of recA, gyrA and rpoS genes was applied for the characterization of Erwinia amylovora and Erwinia strains, which cause fire blight and Asian pear blight in orchards. Primers, constructed on the basis of the published recA, gyrA and rpoS gene sequences of Erwinia carotovora, allowed us to amplify DNA fragments for RFLP differentiation of E. amylovora and E. pyrifoliae and finally to distinguish strains within these species and relate them to pear pathogens from Japan. Three to seven restriction endonucleases were applied for RFLP analysis of each gene fragment. The electrophoretic patterns generated after PCR–RFLP for each of the tested genes, were characteristic and specific for each species and allowed their differentiation. The data show that PCR–RFLP analysis of the recA, gyrA and rpoS gene fragments may be considered as a useful tool for the identification and differentiation of E. amylovora and E. pyrifoliae. Almost identical restriction patterns of the analyzed gene fragments indicated a high relationship of E. pyrifoliae strains from Korea and pear pathogens from Japan and a divergence to E. amylovora. For quick and effective differentiation of E. amylovora strains from Erwinia strains from Asia without nucleotide sequencing we recommend the amplification of recA and rpoS gene fragments and digestion of each of them with restriction endonuclease Hin6I.     

黄脉爵床棒孢霉叶斑病病原菌及其生物学特性鉴定

 明确黄脉爵床棒孢霉叶斑病病原菌及其生物学特性,为防控提供理论依据。通过病原菌分离、形态特征观察、致病性测定、rDNA-ITS序列分析、生物学特性及寄主范围测定等研究,证明该病病原菌为山扁豆生棒孢Corynespora cassiicola;菌丝生长及产孢适宜温度20℃~28℃,孢子萌发适宜温度24℃~32℃,菌丝致死温度49℃处理10 min;菌丝生长适宜pH 6~10,产孢适宜pH 4~8,孢子萌发最适pH 8;光暗交替适合菌丝生长与产孢,连续光照可抑制菌丝生长;菌丝生长量由少到多培养基顺序为CA、PCA、PDA、CMA、OA,而PDA上产孢最多;刺伤接种,病菌可侵染喜树(Camptotheca acuminata)等植物。黄脉爵床棒孢霉叶斑病病原为山扁豆生棒孢C. cassiicola,病菌易产孢,寄主广,潜育期短。该病菌侵染黄脉爵床为首次报道。     

Antagonismusin vitro vonBacillus spp. gegenüberRhizoctonia solani undPythium spp.

Es konnten 132Bacillus-Stämme isoliert und gegenüber7 Rhizoctonia-solani- und 6Pythium-Stämmen auf Antagonismusin vitro untersucht werden. Die gefundenen Antagonisten hemmten die Pilzisolate unterschiedlich stark, so daß Gemische von Antagonisten für die Praxis zu empfehlen sind.There were 132Bacillus-strains isolated and tested for antagonism against 7 strains ofRhizoctonia solani and 6 strains ofPythium spp. The isolated antagonists didn't show a uniform effect against the tested strains ofRhizoctonia solani andPythium spp. For an application in practice it will be better to use a mixture of antagonists.

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Mit 4 Abbildungen und einer Tabelle     

Antagonismusin vivo vonBacillus spp. gegenüberRhizoctonia solani undPythium spp.

Es konntenBacillus-Isolate gefunden werden, die sich in Keimungsversuchen an Samen als antagonistisch gegenüberPythium aphanidermatum undRhizoctonia solani erwiesen. Die Versuche wurden mit Bohnen- und Gurkensamen durchgeführt. Die wirksamsten Antagonisten konnten in infizierter Erde Auflaufraten bei Gurken von 40–60% erzielen.Die Wirksamkeit der Antagonisten an Bohnen war niedriger, hier lagen die Keimraten kaum höher als 30%. Offenbar hängt die Wirksamkeit derBacillus-Antagonisten von der Fähigkeit ab Antibiotika zu produzieren und in Konkurrenz zu anderen Mikroorganismen zu treten.     

Development of PCR assays to Tri7 and Tri13 trichothecene biosynthetic genes, and characterisation of chemotypes of Fusarium graminearum, Fusarium culmorum and Fusarium cerealis

Fusarium graminearum, Fusarium culmorum and Fusarium cerealis are major causal agents of Fusarium Head Blight (scab) which is a disease of global significance in all cereal growing areas. These fungi produce trichothecene mycotoxins, principally nivalenol (NIV) and deoxynivalenol (DON). Genes Tri13 and Tri7 from the trichothecene biosynthetic gene cluster convert DON to NIV (Tri13) and NIV to 4-acetyl-NIV (Tri7). We have developed positive–negative PCR assays based on these two genes, which accurately indicate a DON or NIV chemotype in F. graminearum, F. culmorum and F. cerealis. These assays are useful in assessing the risk of trichothecene contamination, and can be informative in epidemiological studies. All NIV chemotype isolates studied have functional copies of both Tri13 and Tri7, and all DON-producing isolates have both genes disrupted or deleted. We have identified several mutations in these genes, which are conserved across F. graminearum lineage, RAPD and SCAR groupings and between the three species. There appears to be evidence of inter-species hybridisation within the trichothecene biosynthetic gene cluster.     

利用环介导等温扩增方法快速检测瓜类细菌性果斑病菌和番茄细菌性溃疡病菌

为建立简单、快速和灵敏地检测瓜类细菌性果斑病菌Acidovorax avenae subsp. citrulli(Aac)和番茄细菌性溃疡病菌Clavibacter michiganensis subsp. michiganensis(Cmm)的环介导等温扩增(loop-mediated isothermal amplification,LAMP)方法,以Aac的ugpB基因和Cmm的micA基因为靶标,分别设计、合成和筛选特异性引物,摸索和优化各项反应条件和反应体系,成功建立了以钙黄绿素颜色为指示且只需要金属浴恒温反应30～60 min的LAMP扩增体系。特异性分析表明该LAMP方法可以快速检出5株不同的Aac菌株和2株不同的Cmm菌株,其它对照菌株如燕麦嗜酸菌燕麦亚种A. avenae subsp. avenae、丁香假单胞菌Pseudomonas syringae、水稻黄单胞菌水稻致病变种Xanthomonas oryzae pv. oryzae和茄科雷尔氏菌Ralstonia solanacearum则呈现阴性反应;引物比目前报道的LAMP引物有更高的DNA样品检测灵敏度,Aac和Cmm的灵敏度分别为1.72×10~2fg/μL和1.26×10~2fg/μL。研究结果表明,所设计的Aac和Cmm引物特异性好、灵敏度高,更有利于从源头上控制这2种检疫性细菌病害的流行和传播。