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为探明西瓜枯萎病菌侵染西瓜根系及茎的过程,本研究选取一株致病力较强的西瓜枯萎病菌FO1022,利用绿色荧光蛋白基因(GFP)标记该菌株,观察病原菌侵染西瓜根茎部的组织学过程。结果表明,用GFP标记的病菌接种感病西瓜品种‘苏蜜1号’,接种后2 d,显微观察显示病原菌的分生孢子附着于西瓜根系表皮细胞并萌发,沿细胞间层定殖生长;接种后5 d,在西瓜根部维管束导管中观察到大量菌丝和大型分生孢子,在根部表皮细胞上观察到大量厚垣孢子,在茎部部分维管束导管中也观察到少量的菌丝,此时48.6%的幼苗表现萎蔫症状;接种后9 d,茎部所有维管束导管都充斥着密集的菌丝体,此时91.7%的幼苗表现枯萎和死亡。与侵染感病品种相比,该菌株在侵染中抗品种和高抗品种时,在侵染时间上要明显滞后。本研究从组织病理学的角度观察并分析了GFP标记的西瓜枯萎病菌侵染西瓜根茎部的过程,为研究西瓜枯萎病菌的致病机理提供参考。 相似文献
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采用洗涤检验法和马铃薯葡萄糖琼脂培养基法,从甜瓜种子上分离得到23个镰刀菌分离物。采用形态观察和分子生物学方法对其进行鉴定,并研究其致病性以及对甜瓜种子发芽的影响。通过观察菌落形态和色素颜色,以及大型分生孢子、小型分生孢子和厚垣孢子形态,同时分析ITS-rDNA序列和翻译延伸因子-1α(TEF-1α)基因序列,以确定真菌分离物的分类属性。结果表明,4个分离物为尖孢镰刀菌(Fusarium oxysporum),5个分离物为层生镰刀菌(F. proliferatum),5个分离物为木贼镰刀菌(F. equiseti),9个分离物为轮枝样镰刀菌(F. verticillioides)。这4种镰刀菌均对甜瓜幼苗有致病性,其分生孢子悬浮液对甜瓜种子发芽有抑制作用。这是我国首例开展甜瓜种子携带致病性镰刀菌的研究报道。 相似文献
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采用洗涤检验法和马铃薯葡萄糖琼脂培养基法,从甜瓜种子上分离得到23个镰刀菌分离物。采用形态观察和分子生物学方法对其进行鉴定,并研究其致病性以及对甜瓜种子发芽的影响。通过观察菌落形态和色素颜色,以及大型分生孢子、小型分生孢子和厚垣孢子形态,同时分析ITS-rDNA序列和翻译延伸因子-1α(TEF-1α)基因序列,以确定真菌分离物的分类属性。结果表明,4个分离物为尖孢镰刀菌(Fusarium oxysporum),5个分离物为层生镰刀菌(F. proliferatum),5个分离物为木贼镰刀菌(F. equiseti),9个分离物为轮枝样镰刀菌(F. verticillioides)。这4种镰刀菌均对甜瓜幼苗有致病性,其分生孢子悬浮液对甜瓜种子发芽有抑制作用。这是我国首例开展甜瓜种子携带致病性镰刀菌的研究报道。 相似文献
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作物根际和叶围中产几丁质酶微生物的分布及其抑制真菌作用 总被引:7,自引:0,他引:7
从几十种作物的根际和叶围分离获得350株微生物,其中细菌和放线菌分别为200株和150株,对所有这些分离物进行了抑制真菌试验和几丁质酶活性测定。在抑菌试验中,以棉花枯萎病菌、棉花黄萎病菌、黄瓜枯萎病菌,及西瓜枯萎病菌作为供试病原菌,有96个分离物对其中的一种或一种以上的病原菌有抑制作用,其中18个分离物对这4种病原菌都具有强烈的抑制作用,在几丁质酶活性方面10%的细菌和40%的放线菌都能不同程度地 相似文献
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近年来,甘肃省白银市靖远县的一些砂田西瓜中出现了严重的叶疫病,严重田块病株率超过70%。2018年7月,从靖远县高湾乡罹病西瓜叶片上分离得到拟多隔孢属Stagonosporopsis真菌,病叶检出率达100%。采用离体叶片和植株接种法评价单孢分离菌株XG-3对西瓜和甜瓜的致病性,所有接种处理在24 h内均发病显症而对照未发病,其中发病叶片原接种菌的检出率为100%。菌株XG-3在PDA和OA平板培养基上20和25 ℃培养20 d,未见产孢。在自然感病的西瓜叶片上观察到少量分生孢子器,在人工接种发病的西瓜和甜瓜茎、叶上产生大量分生孢子器和分生孢子:分生孢子器球形至亚球形,大小为(82.4~243.3) μm×(82.4~188.4)μm,分生孢子器具1~2个孔口,孔口直径15.7~27.5 μm;分生孢子无色,0~3个隔膜,杆状、柱状、长椭圆形、花生形及不规则形,直或稍弯曲,分隔处不缢缩或缢缩,大小为(5.2~28.3)μm×(2.2~6.0)μm,分生孢子形态和大小依基质和环境条件的不同而有较大差异。BLASTn分析结果显示,菌株XG-3(GenBank登录号:MW282128)的rDNA-ITS序列与瓜拟多隔孢Sta. cucurbitacearum分离物287ITS(GenBank登录号:AY293804.1)的序列相似性达99.80%。在基于rDNA-ITS构建的系统发育树中,菌株XG-3与Sta. cucurbitacearum聚为一组,与西瓜拟多隔孢Sta. citrulli和木瓜拟多隔孢Sta. caricae区分开来。依据病菌形态学和分子生物学特征,将菌株XG-3鉴定为瓜拟多隔孢Sta. cucurbitacearum [Basionym: Sphaeria cucurbitacearum]。 相似文献
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大豆枯萎病菌尖孢镰孢遗传多样性及大豆品种抗性 总被引:2,自引:0,他引:2
了解大豆枯萎病菌的群体遗传特征及明确大豆种质对大豆枯萎病的抗性,对抗病育种、抗性品种的合理布局以及制定更有效的病害防治策略具有重要的参考价值。本研究利用随机扩增多态性DNA(random amplified polymorphic DNA,RAPD),对采自我国不同地区的大豆枯萎病菌—尖孢镰孢菌(Fusarium oxysporum)进行遗传多样性分析,筛选到10个多态性随机引物,共扩增出75条RAPD条带,其中55条为多态性条带,占73.3%。利用UPGMA法对DNA扩增图谱进行聚类分析,以相似系数0.68为阈值,55个分离物可分为9个遗传聚类组,表明我国大豆枯萎病菌具有丰富的种内遗传多样性,所划分的群体与分离物来源地不相关。同时,对上述分离物进行致病性分析,发现我国的大豆枯萎病菌具有明显的致病力分化现象。进一步利用3个代表性分离物对来自我国不同大豆产区的180个大豆品种(资源)进行抗大豆枯萎病鉴定,发现皖豆28、中黄13、中黄51、中作X08076和5D034等5个品种对大豆枯萎病具有良好抗性,占供试材料的2.8%,表明不同大豆品种对枯萎病的抗性存在一定的差异。 相似文献
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为获得带GFP标记的西瓜枯萎病菌转化株,用于后期观察病原菌侵染过程,采用农杆菌介导的方法,对西瓜枯萎病菌1号生理小种进行了遗传转化。结果表明:共培养时间为36h,枯萎病菌孢子和农杆菌AGL1比例为1∶1时该菌株的遗传转化效率最高,可以达到117.33个转化子/107个孢子。转化株的孢子、菌丝体及萌发的孢子均能发出稳定而强的绿色荧光。转化株的致病力检测显示其致病力与转化前的野生菌株致病力无明显差异。结果表明本研究获得的带GFP标记的西瓜枯萎病菌转化株可用于观察病菌在西瓜根系的侵染过程。 相似文献
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甜瓜细菌性果斑病菌致病性突变体筛选与hrcR基因的克隆 总被引:2,自引:0,他引:2
细菌性果斑病(Bacterial Fruit Blotch,BFB)是西瓜和甜瓜的重要病害。本实验从发病甜瓜果实上分离得到致病菌株MH21,经鉴定为燕麦食酸菌西瓜亚种(Acidovorax avenae subsp. citrulli)。利用转座子Mini-Tn5构建MH21菌株的突变体库,Southern印迹杂交结果显示Mini-Tn5在菌株MH21染色体上可随机、单拷贝插入。通过浸种处理甜瓜种子进行突变体的致病性检查,筛选得到1株致病性完全丧失的突变体M543。对M543中转座子插入基因的克隆和测序表明其突变基因为燕麦食酸菌Ⅲ型分泌系统(TTSS)中的保守基因hrcR。推测菌株MH21中hrcR基因编码的蛋白定位于细菌内膜,是分泌通道主要成分之一。hrcR基因互补菌株的致病性检查结果显示其致病力恢复到野生型的84%。研究同时发现hrcR基因突变后MH21菌株丧失了在烟草上诱导过敏性坏死反应的能力。本研究从遗传学角度说明TTSS是西甜瓜果斑病菌致病性的重要因子。 相似文献
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自宁波口岸进境日本杜鹃花种苗上,采用常规平板分离法获得1株疑似杜鹃花枯萎病菌的菌株OV5。该菌株可在马铃薯葡萄糖琼脂和玉米粉琼脂培养基上生长,但在麦芽汁培养基上不生长。经培养可产生少量气生菌丝和大量小型分生孢子,小型分生孢子球状,直径 3.0 ~ 3.5 μm,在纺锤体状菌丝的尖端产生,易脱落,有时呈短链状。菌核卵圆形或饼形,明显杯状,凹面光滑,(1.5 ~ 6) mm × (2 ~ 8)mm × (0.5 ~ 1.5) mm,成熟时黑色。经rDNA ITS基因序列比对分析,发现该菌株与来源于CBS的2株杜鹃花枯萎病菌标准菌株的ITS基因序列同源性达99%以上,位于同一个发育分支。致病性测定结果表明,该菌株可侵染杜鹃花,引起典型杜鹃花枯萎病菌症状。上述研究结果表明,所截获病菌为杜鹃花枯萎病菌,这是我国首次截获该种检疫性真菌。 相似文献
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ABSTRACT A total of 106 isolates of Fusarium oxysporum obtained from diseased cucumber plants showing typical root and stem rot or Fusarium wilt symptoms were characterized by pathogenicity, vegetative compatibility, and random amplified polymorphic DNA (RAPD). Twelve isolates of other formae speciales and races of F. oxysporum from cucurbit hosts, three avirulent isolates of F. oxysporum, and four isolates of Fusarium spp. obtained from cucumber were included for comparison. Of the 106 isolates of F. oxysporum from cucumber, 68 were identified by pathogenicity as F. oxysporum f. sp. radicis-cucumerinum, 32 as F. oxysporum f. sp. cucumerinum, and 6 were avirulent on cucumber. Isolates of F. oxysporum f. sp. radicis-cucumerinum were vegetatively incompatible with F. oxysporum f. sp. cucumerinum and the other Fusarium isolates tested. A total of 60 isolates of F. oxysporum f. sp. radicis-cucumerinum was assigned to vegetative compatibility group (VCG) 0260 and 5 to VCG 0261, while 3 were vegetatively compatible with isolates in both VCGs 0260 and 0261 (bridging isolates). All 68 isolates of F. oxysporum f. sp. radicis-cucumerinum belonged to a single RAPD group. A total of 32 isolates of F. oxysporum f. sp. cucumerinum was assigned to eight different VCGs and two different RAPD groups, while 2 isolates were vegetatively self-incompatible. Pathogenicity, vegetative compatibility, and RAPD were effective in distinguishing isolates of F. oxysporum f. sp. radicis-cucumerinum from those of F. oxysporum f. sp. cucumerinum. Parsimony and bootstrap analysis of the RAPD data placed each of the two formae speciales into a different phylogenetic branch. 相似文献
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ABSTRACT Specific primers and polymerase chain reaction (PCR) assays that identify Fusarium oxysporum f. sp. ciceris and each of the F. oxysporum f. sp. ciceris pathogenic races 0, 1A, 5, and 6 were developed. F. oxysporum f. sp. ciceris- and race-specific random amplified polymorphic DNA (RAPD) markers identified in a previous study were cloned and sequenced, and sequence characterized amplified region (SCAR) primers for specific PCR were developed. Each cloned RAPD marker was characterized by Southern hybridization analysis of Eco RI-digested genomic DNA of a subset of F. oxysporum f. sp. ciceris and nonpathogenic F. oxysporum isolates. All except two cloned RAPD markers consisted of DNA sequences that were found highly repetitive in the genome of all F. oxysporum f. sp. ciceris races. F. oxysporum f. sp. ciceris isolates representing eight reported races from a wide geographic range, nonpathogenic F. oxysporum isolates, isolates of F. oxysporum f. spp. lycopersici, melonis, niveum, phaseoli, and pisi, and isolates of 47 different Fusarium spp. were tested using the SCAR markers developed. The specific primer pairs amplified a single 1,503-bp product from all F. oxysporum f. sp. ciceris isolates; and single 900- and 1,000-bp products were selectively amplified from race 0 and race 6 isolates, respectively. The specificity of these amplifications was confirmed by hybridization analysis of the PCR products. A race 5-specific identification assay was developed using a touchdown-PCR procedure. A joint use of race 0- and race 6-specific SCAR primers in a single-PCR reaction together with a PCR assay using the race 6-specific primer pair correctly identified race 1A isolates for which no RAPD marker had been found previously. All the PCR assays described herein detected up to 0.1 ng of fungal genomic DNA. The specific SCAR primers and PCR assays developed in this study clearly identify and differentiate isolates of F. oxysporum f. sp. ciceris and of each of its pathogenic races 0, 1A, 5, and 6. 相似文献
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AM真菌和镰刀菌对西瓜根系膜脂过氧化作用和膜透性的影响 总被引:5,自引:0,他引:5
在温室盆栽条件下研究了丛枝菌根(arbuscular mycorrhiza,AM)真菌Glomus versiforme (Karsten) Berch和西瓜枯萎镰刀菌(Fusarium oxysporum f. sp. niveum)对西瓜根系中膜脂过氧化产物丙二醛(MDA)含量和细胞膜透性的影响。结果表明,接种AM真菌的西瓜根系中MDA含量、组织自动氧化速率和膜透性均低于对照,先接种G. versiforme,后接种F. oxysporum f. sp. niveum处理的MDA含量、组织自动氧化速率和细胞膜透性均低于只接种F. oxysporum f. sp. niveum的处理。接种G. versiforme感枯萎病西瓜品种"郑杂5号"MDA含量、组织自动氧化速率和膜透性降低幅度大于抗病品种"京欣1号"的接种处理,说明G. versiforme可降低感病西瓜品种的膜透性和MDA的产生,从而有效地保护细胞膜系统,减轻F. oxysporum f. sp. niveum对西瓜的为害程度。 相似文献
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ABSTRACT In order to elucidate the origin of Fusarium oxysporum f. sp. dianthi in Argentina, the genetic diversity among pathogenic isolates together with co-occurring nonpathogenic isolates on carnation was investigated. In all, 151 isolates of F. oxysporum were obtained from soils and carnation plants from several horticultural farms in Argentina. The isolates were characterized using vegetative compatibility group (VCG), intergenic spacer (IGS) typing, and pathogenicity tests on carnation. Seven reference strains of F. oxysporum f. sp. dianthi also were analyzed and assigned to six different IGS types and six VCGs. Twenty-two Argentinean isolates were pathogenic on carnation, had the same IGS type (50), and belonged to a single VCG (0021). The 129 remaining isolates were nonpathogenic on carnation and sorted into 23 IGS types and 97 VCGs. The same VCG never occurred in different IGS types. Our results suggest that the pathogen did not originate in the local populations of F. oxysporum but, rather, that it was introduced into Argentina. Given the genetic homogeneity within Argentinean isolates of F. oxysporum f. sp. dianthi, either IGS type or VCG can be used for the identification of the forma specialis dianthi currently in Argentina. 相似文献
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Isolates of Fusarium oxysporum obtained from cucumber worldwide were classified into 3 groups by random amplified polymorphic DNA-polymerase chain reaction (RAPD-PCR). All isolates of f. sp. radicis-cucumerinum fall into one group. Isolates of races 1 and 2 of f. sp. cucumerinum fall into a second group related to isolates of f. sp. melonis and niveum. Isolates of race 3 fall into a third group, related to f. sp. momordicae. Because f. sp. radicis-cucumerinum has relatively recently been introduced into Greece, where it is actively spreading and very damaging, RAPD-PCR may be valuable in monitoring populations of F. oxysporum. 相似文献
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Auxotrophic mutants were used to determine vegetative relatedness among isolates of Fusarium oxysporum f.sp. dianthi (F.o.d.) , the vascular wilt pathogen of carnation. At the first stage, different nitrate-non-utilizing (nit) mutants were produced from 11 isolates of F.o.d. collected in Israel. Complementation (heterokaryon) tests showed that all the isolates belonged to a single vegetative compatibility group (VCG), and two mutants were chosen as its testers. Additional isolates of Fusarium from carnation, collected during 1986-88, were analysed for pathogenicity and vegetative compatibility with the testers. A total of 170 Fusarium isolates, obtained from 42 cultivars at 40 sites, were tested. All the nit mutants of all the 132 pathogenic isolates formed heterokaryons with the testers, indicating that they belonged to the same VCG. None of the 38 non-pathogenic isolates was vegetatively compatible with the testers. The nit mutants retained pathogenicity to carnation. The F.o.d. testers were not compatible with testers of five other formae speciales of F. oxysporum. Thus, F.o.d. appears to constitute a distinct genetic population within the F. oxysporum complex. 相似文献
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ABSTRACT Eighty-eight isolates of Fusarium oxysporum f. sp. niveum, collected from wilted watermelon plants and infested soil in Maryland and Dela-ware, were characterized by cross pathogenicity to muskmelon, race, and vegetative compatibility. Four isolates (4.5%) were moderately pathogenic to >/=2 of 18 muskmelon cultivars in a greenhouse test, and one representative isolate also was slightly pathogenic in field microplots. The four isolates all were designated as race 2, and were in vegetative compatibility group (VCG) 0082. Of the 74 isolates to which a VCG could be assigned, 41 were in VCG 0080, the VCG distributed most widely; 27 were in VCG 0082, and were distributed in half of the 20 watermelon fields surveyed; and 6 were in the newly described VCG 0083, and were restricted to three fields. Among the isolates in VCG 0080, 8 were designated as race 0, 21 as race 1, and 12 as race 2. Of the isolates in VCG 0082, 6 were designated as race 0, 11 as race 1, and 10 as race 2. All isolates in VCG 0083 were designated as race 2. Isolates from more than one race within the same VCG or isolates from more than one VCG were recovered from single plants and fields. No differences in aggressiveness on differential watermelon cultivars were observed among isolates from different VCGs of the same race. A diverse association between virulence and VCG throughout the Mid-Atlantic region suggests that the pathotypes of F. oxysporum f. sp. niveum may be of local origin or at least long existent in the region. 相似文献