39 resultados para Verticillium dahliae
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DAFF scholarship to train in the recognition and identification of defoliating strains of Verticillium dahliae in cotton and vegetable crops.
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1999
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O gênero Verticillium apresenta duas importantes espécies de fitopatógenos (V. dahliae e V. albo-atrum). A capacidade de produção de microescleródios dos isolados de V. dahliae em cultura tem sido empregada como a principal característica para distinção destas duas espécies. Verticillium dahliae é um fungo bastante polífago, amplamente disseminado no território brasileiro, causando murcha vascular em tomate, berinjela, jiló, algodão, morango, cacau, quiabo, dentre outras hospedeiras. Verticillium dahliae apresenta especialização fisiológica em tomateiro tendo sido descritas duas raças. O presente trabalho teve por objetivo investigar a capacidade de isolados de V. dahliae em infectar e causar doença em plantas de diversas famílias botânicas. Para avaliação da gama de hospedeiros, quatro isolados do fungo foram inoculados em 62 acessos de 54 espécies em 40 gêneros e 18 famílias botânicas. A maioria dos acessos mostrou-se susceptível ao patógeno. Foram classificadas como plantas não-hospedeiras todas as gramíneas avaliadas, as solanáceas Datura stramonium, Nicandra physaloides e Physalis ?oridana, couve-flor (linhagem CNPH-003), melancia (cv. Crimson Sweet), melão (cv. Eldorado 300) alface (cvs. Regina e Robinson), cenoura, feijão, soja-verde, beterraba, maracujá azedo (Passi?ora edulis), capuchinha (Trapaeolum majus) e cariru (Talinum triangulare). Foram identificadas 27 novas hospedeiras experimentais de V. dahliae.
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Root-knot nematode [RKN] (Meloidogyne incognita) can increase the severity of Verticillium (V dahliae) and Fusarium (F oxysporum f.sp. vasinfectum) wilt diseases in cotton (Gossypium hirsutum). This study was conducted to determine some of the physiological responses caused by nematode invasion that might decrease resistance to vascular wilt diseases. The effect of RKN was investigated on spore germination and protein, carbohydrate and peroxidase content in the xylem fluids extracted from nematode-infected plants. Two cotton cultivars were used with different levels of resistance to both of the wilt pathogens. Spore germination was greater in the xylem fluids from nematode-infected plants than from nematode-free plants. The effect on spore germination was greater in the Fusarium-resistant cultivar (51%). Analysis of these fluids showed a decrease in total protein and carbohydrate levels for both wilt-resistant cultivars, and an increase in peroxidase concentration. Fluids from nematode-free plants of the Verticillium-resistant cultivar contained 46% more peroxidase than the Fusarium-resistant cultivar. The results provide further evidence that the effect of RKN on vascular wilt resistance is systemic and not only local. Changes in metabolites in the xylem pass from the root to the stem, accelerating disease development.
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2006
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The effect of root-knot nematode (RKN) (Meloidogyne incognita) on Verticillium dahliae and Fusarium oxysporum f.sp. vasinfectum in cotton (Gossypium hirsutum) was investigated. Two different inoculation methods were used, one in which inoculum was added to the soil, so that nematode and fungal inoculum were in close proximity; the other, inoculation into the stem, whereby the two inocula were spatially separated. Invasion of the roots by RKN enhanced disease severity, as measured by the height of vascular browning in the stem, following inoculation with either wilt pathogen. The effect of RKN on Fusarium wilt was more pronounced than that on Verticillium wilt. Nematode-enhanced infection by F. oxysporum is a well known effect but there are few reports of enhanced infection by Verticillium due to RKN. Relative resistance of a number of cotton cultivars to both wilt diseases, as measured by height of vascular browning, was similar to the known field performance of the cultivars. The use of vascular browning as an estimate of disease severity was therefore validated.
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A solarização do solo por 30 e 50 dias reduziu a ocorrência da murcha de Verticillium dahliae na cultura de tomate e apresentou efeito residual na cultura subsequente de berinjelas. Porém, não houve aumento de produção das duas culturas. As plantas invasoras foram sensivelmente reduzidas com a solarização, sendo que a importância relativa das dicotiledoneas foi maior na testemunha e com brometo de metila, enquanto que, com a solarização, a importância relativa de gramíneas e dicotiledoneas foi semelhante. De modo que, a solarização e o brometo de metila reduziram acentuadamente as populações de diversos grupos de ácaros e insetos, sendo que 11,5 meses após os tratamentos, as populações voltaram a ser semelhantes a testemunha.
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本论文主要包括以下两部分内容: 一、真菌诱导子对青蒿发根生长和青蒿素生物合成的影响 用3种真菌诱导子[大丽花轮枝孢(Verticillium dahliae Kleb.)、葡枝根霉(Rhizopus stolonifer (Ehrenb. ex Fr.) Vuill)和束状刺盘孢(Colleto trichumdematium (Pers.) Grove)]分别处理青蒿(Ar temisia annuaL.)的发根,这3种真菌诱导子均能促进发根中青蒿素的合成,其中以大丽花轮枝孢的诱导效果最好;对细胞生长均没有明显影响。经大丽花轮枝孢处理的发根中青蒿素含量达1. 12 mg/gDW,比对照(0. 77 mg/g DW)提高45%。诱导子的作用效果与诱导子浓度、诱导子作用时间及发根的生长状态有关。对大丽花轮枝孢来说,诱导子作用的最适浓度为每毫升培养基含糖0.4 mg;发根在指数生长末期对诱导作用最敏感:在加入诱导子4d后收获发根,发根中的青蒿素含量最高。 二、早花基因FPF1、co对青蒿开花时间的影响及开花与青蒿素生物合成的相关性 1.将来源于拟南芥的早花基因Flowering Promoting Factorl (FPFl)插入到植物表达载体pBI121中,构建CaMV 35S启动子控制下含FPFl基因的植物表达载体pBI121FPF/,用含有pBI121FPF/质粒的根癌农杆菌(Agrobacterium tumefaciens)LBA4404感染青蒿(Artemisia annua L.)叶片并诱导丛生芽,经卡那霉素筛选,获得转基因抗性植株。PCR、 PCR-Southem blot及Southern blot检测表明,外源基因FPFI已整合到青蒿基因组中:RT-PCR及RT-PCR Southern blot分析表明,外源基因在转录水平上已有表达。在短日照条件下,FPF1转基因植株的开花时间较对照提前20天左右,但提早开花的转基因植株与未开花的对照其青蒿素含量无明显差异,即提早开花并不能使开花植株的青蒿素含量有所提高,开花与青蒿素合成之间可能没有直接的关系。 2.将拟南芥的早花基因CONSTANS (CO)置于CaMV 35S启动子之下,通过根癌农杆菌(Agrobacterium tumefaciens)LBA4404介导转入青蒿(Artemisia annuaL.),使之在青蒿中表达,并得到了抗性植株。PCR、PCR-Southem blot及Southemblot检测表明,外源基因co已整合到青蒿基因组中;RT-PCR及RT-PCR Southemblot分析表明,外源基因在转录水平上已有表达。在短日照条件下,co转基因植株的开花时间较对照提前2周左右,但提早开花的转基因植株的青蒿素含量与未丌花的对照无明显差异,即植株开花前青蒿素含量的提高并不是由于开花本身引起的,再次证明,开花与青蒿素合成之间可能没有直接的关系。
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系统获得性抗性(Systematic acquired resistance, SAR)是植物抵御病原菌侵染的最有效手段,利用基因工程技术导入SAR信号发生过程中的关键基因后,植物的SAR基因表达量提高并且对病原菌侵染的反应速度加快,因此植物的抗病性得以增强,与传统的抗病基因工程技术相比它对病原菌没有专一性,许多学者称之为广谱抗病基因工程,该领域已成为目前抗病基因工程研究的热点和前沿。 NDR1和NPR1基因在植物的SAR发生中起着重要的作用,前者功能定位在ROS(reactive oxygen species)的激活和随后的水杨酸(SA)诱导合成之间,突变株病原菌诱导后SA合成能力降低,SAR发生减弱,目前还没有对该基因进行过量表达分析的报道;后者功能定位在SAR信号转导级联反应之中的SA积累和随后的SAR基因表达之间。该突变株在病原菌侵染时不产生病程相关蛋白(PRs),表现为感病,而对照抗病;过量表达该基因的转基因拟南芥对多种病原菌的侵染产生抗性,PR1等PRs蛋白的表达量也提高,异源表达该基因的水稻对白叶枯病的抗性也提高。本研究利用RT-PCR方法从拟南芥中克隆了这两种基因,序列分析表明拟南芥Wassilewskija生态型的NDR1基因与Columbia生态型相比,共有7处碱基不同,引起编码氨基酸变化4处,而NPR1基因与报道的Wassilewskija生态型来源的NPR1基因完全相同。 我们构建了35S启动子驱动的NDR1和NPR1基因的植物组成型高效表达载体,利用农杆菌介导法转化烟草,PCR和Southern鉴定外源基因已经整合到植物基因组中。抗病性分析显示过量表达NDR1和NPR1基因的烟草对晚疫病和赤星病的抗性都有明显提高,说明这两个基因的在其它植物中异源表达后,都能提高植物对多种病原菌的抗性。 本论文提出了利用这两个基因来培育抗黄萎病棉花的设想,一方面为解决这个“世纪性”难题积累新的资料,另一方面也为其它作物的抗病基因工程提供新的经验。利用35S启动子驱动的NDR1和NPR1基因的植物组成型表达载体分别对陆地棉品种石远321进行花粉管通道法转化。同时,还探讨了这两个基因在棉花中的共转化实验,希望它们的“协同增效”能进一步提高棉花的抗病性。对其中2001年夏天在南京注射所获得的5,000粒种子在三亚进行100 g/ml卡那霉素筛选,初步鉴定分别获得转NDR1和NPR1基因株系26和24棵,PCR进一步鉴定其中分别有12和7棵为转基因阳性,转基因频率分别为0.50%和0.27%,目前利用营养钵蘸根法对其二代进行抗枯、黄萎病鉴定,结果显示有转基因植株对枯、黄萎病的抗性都明显增强,进一步的鉴定正在进行中。2002年初海南注射分别获得转NDR1和NPR1基因以及共转化种子22,000、10,500和12,500粒种子,2002年夏在中国农科院植保所黄萎菌病圃筛选抗黄萎病单株,并利用100 g/ml卡那霉素初步筛选出了一批抗性植株,每种转基因株系随机挑选5株进行PCR鉴定,结果显示为阳性。进一步的抗黄萎病鉴定和筛选以及分子分析正在进行中。 同时,本文还探讨了病原菌诱导型启动子在广谱抗病基因工程应用的可能性。根据烟草的Pr1-a启动子已知序列设计引物,PCR扩增启动子序列后,构建病原菌诱导型NPR1基因植物表达载体,并对棉花进行转化,获得种子11,500粒,利用同上的筛选方法,获得了一致的结果,目前抗黄萎病鉴定、分子检测以及生物学分析正在进行中。 最后,鉴于抗生素标记在转基因植物的应用引起了许多“安全性”争论的事实,还构建了无筛选标记的表达载体对抗虫棉进行转化,这样在生产上可以直接获得抗虫棉抗黄萎病棉花新材料,也为其它作物抗病基因工程积累经验。 本研究还提出了一种较为有效的提取高质量棉花总RNA的方法,与原来一些棉花RNA纯化方法相比,该方法所用都为常规试剂,易于重复,质量高。并且利用获得的总RNA构建了黄萎菌激发子诱导的cDNA文库,滴度测定为1╳107pfμ/μg,插入片段大小在5 00~2 000 bp范围内。 鉴于NPR1基因研究的重要性,本研究还利用简并引物PCR技术从海岛棉和陆地棉的基因组中都分离到了NPR1基因的同源片段,大小都为208 bp,与拟南芥NPR1基因的相应部分的同源性分别为66%和65%,它们之间的同源性为87%,目前该基因的全长正在分离鉴定中。 多聚半乳糖醛酸酶抑制蛋白(PGIPs)在植物的防御反应中起着重要的作用,通过分析已知20余种pgip基因序列的保守区,设计简并引物,PCR扩增海岛棉(Gossypium barbadense)7124 cDNA文库,得到一条长561 bp的片段,序列测定后分析确认为pgip基因的一部分。根据此序列和棉花病原菌诱导的cDNA文库载体中已知部分设计RACE引物,扩增后,5’和3’RACE分别得到666bp和906 bp的片段。序列分析表明它具有完整的编码框,产物为330 aa的蛋白质。序列分析该蛋白具有10个串联的LRR(leucine-rich repeat)区,与柑桔(Citrus)和枳(Poncirus)的pgip基因的同源性分别为69.2%和68.7%。进一步PCR扩增得到该基因的全长阅读框,并且获得了相应的基因组片段,序列分析发现该基因没有内含子。这是从棉属植物中克隆的第一个pgip基因。
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This article documents the addition of 512 microsatellite marker loci and nine pairs of Single Nucleotide Polymorphism (SNP) sequencing primers to the Molecular Ecology Resources Database. Loci were developed for the following species: Alcippe morrisonia morrisonia, Bashania fangiana, Bashania fargesii, Chaetodon vagabundus, Colletes floralis, Coluber constrictor flaviventris, Coptotermes gestroi, Crotophaga major, Cyprinella lutrensis, Danaus plexippus, Fagus grandifolia, Falco tinnunculus, Fletcherimyia fletcheri, Hydrilla verticillata, Laterallus jamaicensis coturniculus, Leavenworthia alabamica, Marmosops incanus, Miichthys miiuy, Nasua nasua, Noturus exilis, Odontesthes bonariensis, Quadrula fragosa, Pinctada maxima, Pseudaletia separata, Pseudoperonospora cubensis, Podocarpus elatus, Portunus trituberculatus, Rhagoletis cerasi, Rhinella schneideri, Sarracenia alata, Skeletonema marinoi, Sminthurus viridis, Syngnathus abaster, Uroteuthis (Photololigo) chinensis, Verticillium dahliae, Wasmannia auropunctata, and Zygochlamys patagonica. These loci were cross-tested on the following species: Chaetodon baronessa, Falco columbarius, Falco eleonorae, Falco naumanni, Falco peregrinus, Falco subbuteo, Didelphis aurita, Gracilinanus microtarsus, Marmosops paulensis, Monodelphis Americana, Odontesthes hatcheri, Podocarpus grayi, Podocarpus lawrencei, Podocarpus smithii, Portunus pelagicus, Syngnathus acus, Syngnathus typhle,Uroteuthis (Photololigo) edulis, Uroteuthis (Photololigo) duvauceli and Verticillium albo-atrum. This article also documents the addition of nine sequencing primer pairs and sixteen allele specific primers or probes for Oncorhynchus mykiss and Oncorhynchus tshawytscha; these primers and assays were cross-tested in both species.
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This article documents the addition of 512 microsatellite marker loci and nine pairs of Single Nucleotide Polymorphism (SNP) sequencing primers to the Molecular Ecology Resources Database. Loci were developed for the following species: Alcippe morrisonia morrisonia, Bashania fangiana, Bashania fargesii, Chaetodon vagabundus, Colletes floralis, Coluber constrictor flaviventris, Coptotermes gestroi, Crotophaga major, Cyprinella lutrensis, Danaus plexippus, Fagus grandifolia, Falco tinnunculus, Fletcherimyia fletcheri, Hydrilla verticillata, Laterallus jamaicensis coturniculus, Leavenworthia alabamica, Marmosops incanus, Miichthys miiuy, Nasua nasua, Noturus exilis, Odontesthes bonariensis, Quadrula fragosa, Pinctada maxima, Pseudaletia separata, Pseudoperonospora cubensis, Podocarpus elatus, Portunus trituberculatus, Rhagoletis cerasi, Rhinella schneideri, Sarracenia alata, Skeletonema marinoi, Sminthurus viridis, Syngnathus abaster, Uroteuthis (Photololigo) chinensis, Verticillium dahliae, Wasmannia auropunctata, and Zygochlamys patagonica. These loci were cross-tested on the following species: Chaetodon baronessa, Falco columbarius, Falco eleonorae, Falco naumanni, Falco peregrinus, Falco subbuteo, Didelphis aurita, Gracilinanus microtarsus, Marmosops paulensis, Monodelphis Americana, Odontesthes hatcheri, Podocarpus grayi, Podocarpus lawrencei, Podocarpus smithii, Portunus pelagicus, Syngnathus acus, Syngnathus typhle,Uroteuthis (Photololigo) edulis, Uroteuthis (Photololigo) duvauceli and Verticillium albo-atrum. This article also documents the addition of nine sequencing primer pairs and sixteen allele specific primers or probes for Oncorhynchus mykiss and Oncorhynchus tshawytscha; these primers and assays were cross-tested in both species.
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This article documents the addition of 512 microsatellite marker loci and nine pairs of Single Nucleotide Polymorphism (SNP) sequencing primers to the Molecular Ecology Resources Database. Loci were developed for the following species: Alcippe morrisonia morrisonia, Bashania fangiana, Bashania fargesii, Chaetodon vagabundus, Colletes floralis, Coluber constrictor flaviventris, Coptotermes gestroi, Crotophaga major, Cyprinella lutrensis, Danaus plexippus, Fagus grandifolia, Falco tinnunculus, Fletcherimyia fletcheri, Hydrilla verticillata, Laterallus jamaicensis coturniculus, Leavenworthia alabamica, Marmosops incanus, Miichthys miiuy, Nasua nasua, Noturus exilis, Odontesthes bonariensis, Quadrula fragosa, Pinctada maxima, Pseudaletia separata, Pseudoperonospora cubensis, Podocarpus elatus, Portunus trituberculatus, Rhagoletis cerasi, Rhinella schneideri, Sarracenia alata, Skeletonema marinoi, Sminthurus viridis, Syngnathus abaster, Uroteuthis (Photololigo) chinensis, Verticillium dahliae, Wasmannia auropunctata, and Zygochlamys patagonica. These loci were cross-tested on the following species: Chaetodon baronessa, Falco columbarius, Falco eleonorae, Falco naumanni, Falco peregrinus, Falco subbuteo, Didelphis aurita, Gracilinanus microtarsus, Marmosops paulensis, Monodelphis Americana, Odontesthes hatcheri, Podocarpus grayi, Podocarpus lawrencei, Podocarpus smithii, Portunus pelagicus, Syngnathus acus, Syngnathus typhle,Uroteuthis (Photololigo) edulis, Uroteuthis (Photololigo) duvauceli and Verticillium albo-atrum. This article also documents the addition of nine sequencing primer pairs and sixteen allele specific primers or probes for Oncorhynchus mykiss and Oncorhynchus tshawytscha; these primers and assays were cross-tested in both species.
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A preservação de fungos fitopatogênicos por longos períodos de tempo é importante para que pesquisas possam ser realizadas a qualquer momento. Os fungos habitantes do solo são organismos que podem produzir estruturas de resistência em face de situações adversas, tais como ausência de hospedeiros e ou condições climáticas desfavoráveis para a sua sobrevivência. O objetivo deste trabalho foi desenvolver metodologias de preservação de estruturas de resistência para os fungos Fusarium oxysporum f.sp. lycopersici raça 2, Macrophomina phaseolina, Rhizoctonia solani AG4 HGI, Sclerotium rolfsii, Sclerotinia sclerotiorum e Verticillium dahliae. O delineamento foi inteiramente casualizado, com um método de produção de estruturas para cada fungo, submetido a três tratamentos [temperatura ambiente de laboratório (28±2ºC), de geladeira (5ºC) e de freezer (-20ºC)] e com dois frascos por temperatura. Mensalmente, e por um período de um ano, a sobrevivência e o vigor das colônias de cada patógeno foram avaliadas em meios de cultura específicos. Testes de patogenicidade foram realizados após um ano de preservação, com as estruturas que sobreviveram aos melhores tratamentos (temperatura) para todos os fungos. As melhores temperaturas (tratamentos) para preservar os fungos foram: a) F. oxysporum f.sp. lycopersici em temperatura de refrigeração e de freezer (5,2 e 2,9 x 10³ufc.g-1 de talco, respectivamente); b) M. phaseolina em temperatura de refrigeração [100% de sobrevivência (S) e índice 3 de vigor (V)] e S. rolfsii em temperatura ambiente (74,4% S e 1 V) e c) S. sclerotiorum e V. dahliae, ambos em temperatura de freezer (100% S e 3 V). Após um ano de preservação, somente V. dahliae perdeu a patogenicidade na metodologia desenvolvida.
Resumo:
This article documents the addition of 512 microsatellite marker loci and nine pairs of Single Nucleotide Polymorphism (SNP) sequencing primers to the Molecular Ecology Resources Database. Loci were developed for the following species: Alcippe morrisonia morrisonia, Bashania fangiana, Bashania fargesii, Chaetodon vagabundus, Colletes floralis, Coluber constrictor flaviventris, Coptotermes gestroi, Crotophaga major, Cyprinella lutrensis, Danaus plexippus, Fagus grandifolia, Falco tinnunculus, Fletcherimyia fletcheri, Hydrilla verticillata, Laterallus jamaicensis coturniculus, Leavenworthia alabamica, Marmosops incanus, Miichthys miiuy, Nasua nasua, Noturus exilis, Odontesthes bonariensis, Quadrula fragosa, Pinctada maxima, Pseudaletia separata, Pseudoperonospora cubensis, Podocarpus elatus, Portunus trituberculatus, Rhagoletis cerasi, Rhinella schneideri, Sarracenia alata, Skeletonema marinoi, Sminthurus viridis, Syngnathus abaster, Uroteuthis (Photololigo) chinensis, Verticillium dahliae, Wasmannia auropunctata, and Zygochlamys patagonica. These loci were cross-tested on the following species: Chaetodon baronessa, Falco columbarius, Falco eleonorae, Falco naumanni, Falco peregrinus, Falco subbuteo, Didelphis aurita, Gracilinanus microtarsus, Marmosops paulensis, Monodelphis Americana, Odontesthes hatcheri, Podocarpus grayi, Podocarpus lawrencei, Podocarpus smithii, Portunus pelagicus, Syngnathus acus, Syngnathus typhle,Uroteuthis (Photololigo) edulis, Uroteuthis (Photololigo) duvauceli and Verticillium albo-atrum. This article also documents the addition of nine sequencing primer pairs and sixteen allele specific primers or probes for Oncorhynchus mykiss and Oncorhynchus tshawytscha; these primers and assays were cross-tested in both species.
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Fundação de Amparo à Pesquisa do Estado de São Paulo (FAPESP)
