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进境油菜籽中黑胫病菌和茎基溃疡病菌的检测 总被引:1,自引:0,他引:1
为准确鉴定从进境澳大利亚油菜籽样品中分离的真菌分离物,利用形态学特征、PCR检测、序列分析以及致病性测试等方法对分离物6382-43和6382-51进行了鉴定试验。结果表明,分离物6382-43的形态特征和油菜茎基溃疡病菌Leptosphaeria maculans相似,菌丝生长较慢,菌落边缘不规则,不产生色素。油菜茎基溃疡病菌特异性引物LmacF/LmacR检测为PCR阳性;ITS区序列和油菜茎基溃疡病菌的序列相似性为99.8%;接种幼嫩油菜子叶产生油菜茎基溃疡病的典型症状。分离物6382-51的形态特征和油菜黑胫病菌L.biglobosa相似,菌丝生长较快,菌落边缘规则,产生色素;油菜黑胫病菌特异性引物LbigF/LmacR检测为PCR阳性;ITS区序列和油菜黑胫病菌的序列相似性为100%;接种幼嫩油菜子叶产生油菜黑胫病的典型症状。根据分离物的形态特征、PCR检测结果、序列分析以及致病性测试结果,将进境澳大利亚油菜籽样品中的真菌分离物6382-43和6382-51分别鉴定为油菜茎基溃疡病菌Leptosphaeria maculans和油菜黑胫病菌L.biglobosa。 相似文献
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油菜茎基溃疡病菌LAMP-LFD检测方法的建立 总被引:1,自引:0,他引:1
本文基于环介导等温扩增技术与横向流动试纸条相结合的方法,建立了一种应用于油菜茎基溃疡病菌(Leptosphaeria maculans)的LAMP-LFD快速检测方法。以油菜茎基溃疡病菌的ITS基因序列为靶序列,设计出一套用于LAMP-LFD检测的引物和探针,优化了反应体系与反应条件(63℃,35 min)。结果表明:只有油菜茎基溃疡病菌出现阳性条带,其他参照菌株和阴性对照均未出现阳性条带,说明LAMP-LFD检测特异性强;灵敏度检测表明,对油菜茎基溃疡病菌的检测极限可低至114 fg/μL,灵敏度比传统PCR高10倍;该方法可从进境船载油菜籽样品中成功检测出油菜茎基溃疡病菌,检测结果与传统的鉴定方法一致。LAMP-LFD检测方法能够快速检测油菜茎基溃疡病菌,具有简便、灵敏、特异性高,不依赖特殊检测设备等优点,极具推广前景。 相似文献
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自进境澳大利亚大麦样品上,采用常规平板分离法获得1株疑似葡萄茎枯病菌菌株74919。通过形态学特征观察、β-tubulin和actin序列比对分析以及致病性测定,对该菌株进行了种类鉴定。结果表明:菌株74919在PDA培养基上生长良好,可产生大量分生孢子器和厚垣孢子;基于β-tubulin和actin序列构建的系统发育树中,菌株74919和其他葡萄茎枯病菌相关序列划分在同一分支;菌株74919接种大麦叶片,在接种部位引起叶斑症状。根据上述实验结果,将菌株74919鉴定为葡萄茎枯病菌(Didymella glomerata),这是我国口岸首次从进境澳大利亚大麦中截获葡萄茎枯病菌。 相似文献
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《植物检疫》2015,(1)
分别对来自比利时和荷兰的水曲柳原木进行了病原菌分离,结果在原木的树皮中各分离到1株疑似苹果壳色单隔孢溃疡病菌的菌株Bs-1268和Bs-8212。对其进行了病原菌形态学观察、致病性测定并结合分子生物学方法检测,实验结果表明,菌株Bs-1268和Bs-8212在PDA和OA培养基上均能产生一定量的分生孢子器和分生孢子,分生孢子器通常为球形;经真菌通用引物(ITS4/ITS5)扩增和测序,菌株Bs-1268和Bs-8212与Gen Bank中登录号KF766158.1的菌株序列同源性达到100%;病菌分别接种苹果和梨6 d后发病。根据上述实验结果,将分离获得的菌株Bs-1268和Bs-8212鉴定为苹果壳色单隔孢溃疡病菌(Botryosphaeria stevensii Shoemaker)。 相似文献
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根据油菜茎基溃疡病菌Leptosphaeria maculans与其近似种ITS序列的差异,设计了检测L. maculans的引物Lmb3/R2和探针Probe-M,建立了L. maculans的实时荧光PCR检测方法。试验结果表明,来自加拿大、澳大利亚和乌克兰等国的22株L. maculans菌株都能得到阳性扩增,而供试的30株L. biglobosa菌株和6株其他菌株以及空白对照没有荧光信号的增加。该检测方法的灵敏度达到4 pg菌丝DNA,整个检测过程控制在4 h内,其快速、特异和灵敏的特点可以满足进境油菜籽样品的快速初检以及病菌分离物的快速鉴定。 相似文献
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对来自美国的苹果进行了病原菌分离,结果在果实中分离到1株疑似苹果牛眼果腐病菌的菌株Nk-2968。对其进行了病原菌形态学观察、致病性测定并结合分子生物学方法检测,实验结果表明,菌株Nk-2968在PDA培养基上生长良好,能产生大量的分生孢子;经真菌通用引物(ITS4/ITS5)及β-tubulin引物(Bt-T2m-Up/Bt-LVL-Lo)分别扩增和测序,菌株Nk-2968与Gen Bank中登录号AF281462.1、HG793110.1和HG793112.1的菌株序列同源性达到100%;病菌接种苹果8 d后开始发病。根据上述实验结果,将分离获得的菌株Nk-2968鉴定为苹果牛眼果腐病菌(Neofabraea kienholzii)。这是我国口岸首次在进境的苹果果实上截获该危险性有害生物。 相似文献
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法国向日葵种子中向日葵黑茎病菌的首次截获与检测 总被引:2,自引:0,他引:2
从法国进境向日葵种子中分离到3株疑似向日葵黑茎病的菌株,对所有菌株进行形态学、致病性测定和分子序列比对分析。分离菌菌落乳白色或象牙色至灰白色,有大量黑褐色分生孢子器产生,分生孢子器球形至扁球形,内含无色单胞、卵圆形分生孢子,有明显或不明显油球;针刺接种4片真叶向日葵幼苗的下胚轴,7~9d后茎部产生典型黑茎病黑色椭圆形病斑,病斑上着生黑色分生孢子器;菌丝DNA用ActF1/R1和ITS1/ITS4扩增,序列与NCBI基因库中P.macdonaldii序列相似性为98%~100%。形态学、分子生物学及致病性检测结果显示,截获的3株菌均为向日葵黑茎病菌。 相似文献
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对来自新西兰的猕猴桃进行了病原菌的分离培养,结果在果实中分离到2株疑似猕猴桃果腐病菌的菌株Na-3419和Na-4756。对其进行了病原菌形态学观察、致病性测定并结合分子生物学方法检测,实验结果表明,菌株Na-3419和Na-4756在PDA培养基上生长良好,能产生大量的分生孢子;经真菌通用引物(ITS4/ITS5)扩增和测序,菌株Na-3419与Gen Bank中登录号EU482221.1和EU482220.1的菌株序列同源性达到100%,菌株Na-4756与Gen Bank中登录号AY359230.1、AY359226.1和KR859079.1的菌株序列同源性达到100%;病菌接种猕猴桃3 d后开始发病。根据上述试验结果,将分离获得的菌株Na-3419和Na-4756鉴定为猕猴桃果腐病菌(Neofabraea actinidiae)。这是上海口岸首次在进境的猕猴桃果实上截获该有害生物。 相似文献
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Vincenot L Balesdent MH Li H Barbetti MJ Sivasithamparam K Gout L Rouxel T 《Phytopathology》2008,98(3):321-329
Stem canker of crucifers is caused by an ascomycete species complex comprising of two main species, Leptosphaeria maculans and L. biglobosa. These are composed of at least seven distinct subclades based on biochemical data or on sequences of internal transcribed spacer (ITS), the mating type MAT1-2 or fragments of actin or beta-tubulin genes. In the course of a wide-scale characterization of the race structure of L. maculans from Western Australia, a few isolates from two locations failed to amplify specific sequences of L. maculans, i.e., the mating-type or minisatellite alleles. Based on both pathogenicity tests and ITS size, these isolates were classified as belonging to the L. biglobosa species. Parsimony and distance analyses performed on ITS, actin and beta-tubulin sequences revealed that these isolates formed a new L. biglobosa subclade, more related to the Canadian L. biglobosa 'canadensis' subclade than to the L. biglobosa 'australensis' isolates previously described in Australia (Victoria). They are termed here as L. biglobosa 'occiaustralensis'. These isolates were mainly recovered from resistant oilseed rape cultivars that included the Brassica rapa sp. sylvestris-derived resistance source, but not from the susceptible cv. Westar. The pathogenicity of L. biglobosa 'occiaustralensis' to cotyledons of most oilseed rape genotypes was higher than that of L. biglobosa 'canadensis' or L. biglobosa 'australensis' isolates. 相似文献
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A. Dilmaghani M. H. Balesdent J. P. Didier C. Wu J. Davey M. J. Barbetti Hua Li O. Moreno-Rico D. Phillips J. P. Despeghel L. Vincenot L. Gout T. Rouxel 《Plant pathology》2009,58(6):1044-1058
Stem canker of oilseed rape (canola, Brassica napus ) is associated with a species complex of two closely related fungal species, Leptosphaeria maculans and L. biglobosa . Of these, L. maculans is the most damaging and develops gene-for-gene relationships with the host . Here, a wide scale analysis of the L. maculans - L. biglobosa species complex was performed throughout the American continent (23 locations from Chile to Canada) plus several locations in Western Australia for comparison purposes, based on a collection of 1132 isolates from infected tissues of a susceptible cultivar. Fungal species were discriminated on the basis of morphological, phytopathological and molecular criteria and showed that L. biglobosa was closely associated with L. maculans in most of the locations. Multiple gene phylogeny using sequences of ITS, actin and β-tubulin confirmed the prevalence of the L. biglobosa 'canadensis' sub-clade in Canada, whereas up to three different sub-clades of L. biglobosa were found in Georgia (USA). Race structure of L. maculans was investigated using a combination of pathogenicity tests and PCR amplification of avirulence alleles AvrLm1 , AvrLm4 and AvrLm6 . Three contrasting situations were observed: (i) race structure in Ontario, Chile and Georgia was related to that of European and Western Australian populations, with a low race diversity; (ii) only one race was found in Mexico, and not found outside of this country; (iii) a large diversity of races was observed in central Canada (Manitoba, Alberta and Saskatchewan) with very specific features including maintenance of avirulence alleles absent from Europe, absence of the AvrLm7 allele common in Europe (or eastern Canada) and wide location-to-location variability. 相似文献
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进境澳大利亚油菜籽中茎基溃疡病菌的检测 总被引:1,自引:0,他引:1
41 fungal isolates with similar morphological characteristics to Leptosphaeria maculans were obtained by the deep-freezing filter paper method from 2100 seeds of Brassica napus imported from Australia.The isolate 8129-5 showed a slower growth on PDA at 20℃with growth rate of 2.8 mm/day.The colonies on PDA at 20℃ had an irregular or regular margin with white or grayish white compact aerial mycelium.No diffusible pigment was produced on PDA at 31℃ or in liquid Czapek-Dox media at 20℃.PCR detection showed that the isolate 8129-5 could be amplified by L.maculans-specific primers LmacF/LmacR and got expected product of 331 bp.The sequence analysis revealed that the ITS sequence of isolate 8129-5 had 99.8% identity with L.maculans.Pathogenicity of the isolate 8129-5 was confirmed on cotyledons of rape seed by artificial inoculation compared with typical symptom of L.maculans.Based on the morphological characteristics, PCR detection and the result of pathogenicity test, the isolate 8129-5 was identified as L.maculans. 相似文献
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Balesdent MH Barbetti MJ Li H Sivasithamparam K Gout L Rouxel T 《Phytopathology》2005,95(9):1061-1071
ABSTRACT Leptosphaeria maculans, the causal agent of stem canker of oilseed rape, develops gene-for-gene interactions with its hosts. To date, eight L. maculans avirulence (Avr) genes, AvrLm1 to AvrLm8, have been genetically characterized. An additional Avr gene, AvrLm9, that interacts with the resistance gene Rlm9, was genetically characterized here following in vitro crosses of the pathogen. A worldwide collection of 63 isolates, including the International Blackleg of Crucifers Network collection, was genotyped at these nine Avr loci. In a first step, isolates were classified into pathogenicity groups (PGs) using two published differential sets. This analysis revealed geographical disparities as regards the proportion of each PG. Genotyping of isolates at all Avr loci confirmed the disparities between continents, in terms of Avr allele frequencies, particularly for AvrLm2, AvrLm3, AvrLm7, AvrLm8, and AvrLm9, or in terms of race structure, diversity, and complexity. Twenty-six distinct races were identified in the collection. A larger number of races (n = 18) was found in Australia than in Europe (n = 8). Mean number of virulence alleles per isolate was also higher in Australia (5.11 virulence alleles) than in Europe (4.33) and Canada (3.46). Due to the diversity of populations of L. maculans evidenced here at the race level, a new, open terminology is proposed for L. maculans race designation, indicating all Avr loci for which the isolate is avirulent. 相似文献
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Balesdent MH Jedryczka M Jain L Mendes-Pereira E Bertrandy J Rouxel T 《Phytopathology》1998,88(11):1210-1217
ABSTRACT The blackleg disease of oilseed rape is caused by an ascomycete species complex termed Leptosphaeria maculans (anamorph Phoma lingam). L. maculans isolates collected worldwide were gathered in the International Blackleg of Crucifers Network (IBCN) collection. Representative IBCN isolates, along with one P. nigrificans isolate, were further analyzed using polymerase chain reaction (PCR) amplification of the internal transcribed spacer (ITS) region. ITS size polymorphism discriminated three groups: (i) P. nigrificans, (ii) Tox(+) and 'Lepidium' isolates, and (iii) NA1, NA2, NA3, 'Thlaspi', and 'Erysimum' isolates. Digestion of the ITS region with 19 selected endonucleases showed restriction site polymorphism between the different subgroups: digestion with RsaI could discriminate Tox(+) from 'Lepidium' isolates, whereas digestion with four enzymes, i.e., HaeIII, EcoRII, RsaI, and AluI, was needed to discriminate between NA1, NA2, NA3, 'Thlaspi', and 'Erysimum' isolates. No restriction site polymorphism was observed between isolates within the 'Thlaspi', Tox(+), NA1, and NA2 subgroups. Direct amplification of the ITS region could be achieved using intact conidia, collected either in axenic cultures or on leaf lesions, with only a 4-min 95 degrees C denaturation step prior to PCR reaction. A routine identification protocol requiring no DNA extraction and a sequential use of a few restriction enzymes following PCR has been used successfully for large-scale identification of French field isolates. 相似文献