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ABSTRACT The exo-beta-1,3-glucanase (EC 3.2.1.58) activity of Pichia anomala strain K, an antagonistic yeast of Botrytis cinerea on postharvest apples, was studied in a synthetic medium supplemented with laminarin, a cell wall preparation (CWP) of B. cinerea, or glucose. The highest enzyme activity was detected in culture media containing a CWP of B. cinerea as the sole carbon source, whereas the lowest activity was observed in culture media supplemented with glucose. Exoglc1, an exo-beta-1,3-glucanase, was purified to homogeneity from culture filtrates of strain K containing a CWP. The molecular mass of exoglc1 was estimated to be under 15 kDa. Optimum activity of exoglc1 was recorded at 50 degrees C and pH 5.5. The exoglc1 K(m) value was estimated at 22.4 mg/ml. Exoglc1 showed in vitro a stronger inhibitory effect on germ tube growth of B. cinerea than on conidia germination and caused morphological changes such as leakage of cytoplasm and cell swelling. Exo-beta-1,3-glucanase activity was detected on apples treated with strain K and was similar to exoglc1 on the basis of activity on native gel. Moreover, the addition of a CWP to a suspension of P. anomala stimulated both in situ exo-beta-1,3-glucanase activity and protective activity against the pathogen, strengthening the hypothesis that exo-beta-1,3-glucanase activity is one of the mechanisms of action involved in the suppression of B. cinerea by P. anomala strain K. 相似文献
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ABSTRACT Lysobacter enzymogenes produces extracellular lytic enzymes capable of degrading the cell walls of fungi and oomycetes. Many of these enzymes, including beta-1,3-glucanases, are thought to contribute to the biological control activity expressed by several strains of the species. L. enzymogenes strain C3 produces multiple extracellular beta-1,3-glucanases encoded by the gluA, gluB, and gluC genes. Analysis of the genes indicates they are homologous to previously characterized genes in the related strain N4-7, each sharing >95% amino acid sequence identity to their respective counterparts. The gluA and gluC gene products encode enzymes belonging to family 16 glycosyl hydrolases, whereas gluB encodes an enzyme belonging to family 64. Mutational analysis indicated that the three genes accounted for the total beta-1,3-glucanase activity detected in culture. Strain G123, mutated in all three glucanase genes, was reduced in its ability to grow in a minimal medium containing laminarin as a sole carbon source. Although strain G123 was not affected in antimicrobial activity toward Bipolaris sorokiniana or Pythium ultimum var. ultimum using in vitro assays, it was significantly reduced in biological control activity against Bipolaris leaf spot of tall fescue and Pythium damping-off of sugar beet. These results provide direct supportive evidence for the role of beta-1,3-glucanases in biocontrol activity of L. enzymogenes strain C3. 相似文献
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优化高效拮抗生防菌哈茨木霉T2-16的转化条件,筛选出与野生型菌株具有相似生防特性的阳性转化子,为生防木霉菌T2-16的定殖动态、分布规律等研究打下基础。通过PCR和分子克隆技术构建具有G418抗性基因的绿色荧光(GFP)表达载体pKN-sGFP,利用PEG-CaCl2介导的原生质体转化法,获得强荧光表达的哈茨木霉T2-16转化子,并将其与野生型菌株的生物特性进行比较,筛选出与野生型菌株具有相似生防特性的阳性转化子。试验结果显示,哈茨木霉T2-16在20℃培养条件下对1000 μg/mL G418敏感,在上述优化条件下,转化获得稳定遗传的阳性转化子TG2-10;进一步比较其与野生型菌株的生物特性发现,两者之间无明显差异,可用于下一步哈茨木霉T2-16生防机理的研究。 相似文献
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ABSTRACT Ulocladium atrum (strain 385) consistently reduced Botrytis cinerea sporulation on necrotic fragments of strawberry leaves. On these tissues, two strains of U. atrum (isolates 18558 and 18559) showed lower antagonistic activities than the reference strain 385. Colonization of strawberry leaflets by the three U. atrum strains appeared similar in the absence of B. cinerea, whether quantified by chitin or immunological assays. The second method (based on anti-U. atrum antibodies) revealed that strawberry leaflet colonization by U. atrum 385 was better than by the other U. atrum strains in the presence of B. cinerea. An immunoassay using anti-B. cinerea antibodies revealed that the colonization of B. cinerea in tissues was lower in the presence of U. atrum 385 than with the two other U. atrum strains. The enzymatic activities produced by U. atrum 385 during the colonization phases of necrotic tissues were compared to B. cinerea and U. atrum strains 18558 and 18559. U. atrum 385 had the highest lipase, pectate lyase, and cellobiase activities while B. cinerea had the highest endo-beta-1,4-glucanase activity. The study of lytic activities hydrolyzing the fungal cell wall revealed higher beta-1,3-glucanase activity with U. atrum 385, which was stimulated by B. cinerea on necrotic strawberry leaflets. These results suggest that plant and fungal cell wall-degrading enzymes produced by U. atrum 385 may play a complementary role in the competitive colonization of dead strawberry leaves against B. cinerea. 相似文献
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Maryline Magnin-Robert Patricia Trotel-Aziz Daniel Quantinet Sylvie Biagianti Aziz Aziz 《European journal of plant pathology / European Foundation for Plant Pathology》2007,118(1):43-57
In this study, the biocontrol ability of seven grapevine-associated bacteria, previously reported as efficient against Botrytis cinerea under in vitro conditions, was evaluated in two vineyard orchards with the susceptible cv. Chardonnay during four consecutive
years (2002–2005). It was shown that the severity of disease on grapevine leaves and berries was reduced to different levels,
depending on the bacterial strain and inoculation method. Drenching the plant soil with these bacteria revealed a systemic
resistance to B. cinerea, even without renewal of treatment. Accordingly, this resistance was associated with a stimulation of some plant defense
responses such as chitinase and β-1,3-glucanase activities in both leaves and berries. In leaves, chitinase activity increased
before veraison (end-July) while β-1,3-glucanase reached its maximum activity at ripening (September). Reverse patterns were
observed in berries, with β-1,3-glucanase peaking at full veraison (end-August) and chitinase at a later development stage.
Highest activities were observed with Acinetobacter lwoffii PTA-113 and Pseudomonas fluorescens PTA-CT2 in leaves, and with A. lwoffii PTA-113 and Pantoea agglomerans PTA-AF1 in berries. These results have demonstrated an induced protection of grapevine against B. cinerea by selected bacteria under field conditions, and suggest that induced resistance could be related to a stimulation of plant
defense reactions in a successive manner. 相似文献
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贝莱斯芽孢杆菌Bacillus velezensis YB15β-葡聚糖酶的抑菌作用与基因克隆 总被引:1,自引:0,他引:1
本文在对峙法验证贝莱斯芽孢杆菌B. velezensis YB15具抑菌作用的基础上,用透明圈法、DNS法研究其产β-葡聚糖酶特性,利用对峙法验证该酶抑菌作用,通过PCR法获得目的基因,分析克隆序列并预测其蛋白质结构与功能。结果表明,该菌株对多种病原真菌有拮抗作用,杨树紫纹羽病菌拮抗带达11.0 mm,该菌提取的葡聚糖酶粗酶液对杨树紫纹羽病菌抑菌带为10.6 mm,说明葡聚糖酶在菌株YB15抑菌中有重要作用。不同接种方法影响菌株YB15葡聚糖酶水解透明圈形成,点种法水解圈与菌落直径之比在72 h可达14.1,效果最好。克隆所得菌株YB15葡聚糖酶基因命名为Bglu1,该基因序列长732 bp,编码243个氨基酸,此酶蛋白氨基酸序列与解淀粉芽孢杆菌TB2β-1,3-1,4-葡聚糖酶同源性较高,属糖基水解酶16家族,N端疏水区存在信号肽并具跨膜区域,推测其为分泌蛋白。 相似文献
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ABSTRACT Infection of peanut (Arachis hypogaea) seed by Aspergillus flavus and A. parasiticus is a serious problem that can result in aflatoxin contamination in the seed. Breeding resistant cultivars would be an effective approach to reduce aflatoxin accumulation. The objective of this study was to investigate the expression of the pathogenesis-related (PR) protein beta-1,3-glucanase and the isoform patterns in peanut seed inoculated with A. flavus. Peanut genotypes GT-YY9 and GT-YY20 (both resistant to A. flavus infection) and Georgia Green and A100 (both susceptible to A. flavus infection) were used in this study. The activities of beta-1,3-glucanase were similar in the uninfected seed of all genotypes, but increased significantly in the resistant genotypes after inoculation in comparison with the susceptible genotypes. An in-gel (native polyacrylamide gel electrophoresis [PAGE]) enzymatic activity assay of beta-1,3-glucanase revealed that there were more protein bands corresponding to beta-1,3-glucanase isoforms in the infected seed of resistant genotypes than in the infected seed of susceptible genotypes. Both acidic and basic beta-1,3-glucanase isoforms were detected in the isoelectric focusing gels. Thin-layer chromatography analysis of the hydrolytic products from the reaction mixtures of the substrate with the total protein extract or individual band of native PAGE revealed the presence of enzymatic hydrolytic oligomer products. The individual bands corresponding to the bands of beta-1,3-glucanase isoforms Glu 1 to 5 were separated on the sodium dodecyl sulfate-PAGE, resulting in two bands of 10 and 13 kDa, respectively. The sequences of fragments of the 13-kDa major protein band showed a high degree of homology to conglutin, a storage protein in peanut seed. Conglutin is reported as a peanut allergen, Ara h2. Our data provide the first evidences for peanut having beta-1,3-glucanase activities and the association with the resistance to A. flavus colonization in peanut seed. We have not directly demonstrated that conglutin has beta-1,3-glucanase activity. 相似文献
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生防菌哈茨木霉FJAT-9040的GFP标记及土壤定殖示踪 总被引:1,自引:1,他引:0
哈茨木霉Trichoderma harzianum FJAT-9040对茄科尖孢镰刀菌具有较强拮抗作用。为跟踪分析该菌株在土壤中的存活与定殖特性,利用PEG-CaCl2介导的原生质体转化体系,筛选获得1株荧光性状稳定的菌株FJAT-9295,该菌株在生长速率、产孢量、对酸碱度和温度的适应性及对尖孢镰刀菌的抑菌活性等方面与野生型菌株FJAT-9040无显著差异(P〉0.05)。同时,研究了菌株FJAT-9295在4种类型土壤中的定殖能力以及作物生长对该菌株在土壤中定殖的影响。结果表明:菌株在育苗土中定殖最好,其次为沙土及菜园土,黄泥土中定殖最差;种植茄子比未种植作物的土壤更有利于菌株的存活;菌株FJAT-9295在不同类型土壤中的菌落数随时间的延长均略有下降,16天后趋于稳定,维持在105 CFU/g,较初始接菌量下降了约1个数量级。 相似文献
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内生菌螺旋毛壳抗生素和水解酶的协同抗真菌作用 总被引:2,自引:0,他引:2
生防因子螺旋毛壳(Chaetomium spirale) ND35生长于含立枯丝核菌(Rhizoctonia solani)菌丝细胞壁制备物的SM培养基中,从培养滤液提取的粗酶液强烈抑制Valsa sordida、Valsa mali、Glomerella cingulata和Curvulavia lunata病原真菌的菌丝生长和孢子萌发。经DNS法检测,粗酶液同时具有β-1,3-葡聚糖酶(包括内切和外切酶)和几丁质酶活性,分别为0.19 U.mg-1和0.09 U.mg-1。生长于3%玉米粉浸渍液的螺旋毛壳ND35的培养滤液也能抑制上述病原菌的菌丝生长和孢子萌发。离体条件下检测了ND35产生的一纯化的具有分子量为73 kD的内切β-1,3-葡聚糖酶(GLUC73)和一纯化的抗生素对苹果炭疽病菌的分生孢子萌发和芽管延长的抑制效果。当内切β-1,3-葡聚糖酶使用浓度为180 μg·mL-1时,抑制了测试真菌的孢子萌发,造成细胞壁的改变,导致了菌丝顶端的破裂;抗生素的有效抑菌中浓度ED50为1.75 μg·mL-1。单独应用时,1.0 μg·mL-1的抗生素或40 μg·mL-1的内切β-1,3-葡聚糖酶没有或仅有很低的抑菌效果;两者组合导致孢子萌发约78%受抑制。甚至10 μg·mL-1的内切β-1,3-葡聚糖酶也使1.5 μg·mL-1抗生素的抑菌作用从低于25%增加到超过50%的抑菌效果。此外,80 μg·mL-1的内切β-1,3-葡聚糖酶使1.0 μg·mL-1抗生素的抑菌活性从0%提高到90%。抗生素和β-1,3-葡聚糖酶的协同抗菌活性可能在内生菌螺旋毛壳的植病生防中起重要作用。 相似文献
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利用mariner转座子对产酶溶杆菌Lysobacter enzymogenes OH11进行转座诱变,构建菌株OH11的突变体文库.筛选到1株4种胞外酶(蛋白酶、纤维素酶、几丁质酶和β-1,3-葡聚糖酶)产生均减少的突变株D-11.通过亚克隆,鉴定转座子的插入位点,涉及1个羧基末端蛋白酶(carboxy-terminal protease)编码基因ctp.通过同源重组的方法对该基因进行敲除,对缺失突变体Δctp表型分析发现:(1)Δctp与野生型OH11在营养丰富型(2YT)与营养缺陷型(MMX)培养基中生长速率基本一致;(2)Δctp降低了蛋白酶、纤维素酶和β-1,3-葡聚糖酶的产生,但不影响几丁质酶的产生;(3)Δctp生物膜的产生量明显减少.研究还表明,突变体基本不改变其对油菜菌核病菌Sclerotinia sclerotiorum、水稻纹枯病菌Rhizoctonia solani和辣椒疫霉病菌Phytophthora capsici的拮抗能力.互补菌株均恢复了野生型的相关功能. 相似文献
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Ramón Penyalver Begonya Vicedo María M. López 《European journal of plant pathology / European Foundation for Plant Pathology》2000,106(9):801-810
Strain K84 of Agrobacterium (formerly called A. radiobacter) has been a successful biocontrol agent of crown gall disease for almost 30 years all over the world. In spite of its demonstrated efficiency, the most important risk of failure when using strain K84 is the possibility of transfer of plasmid pAgK84 to pathogenic Agrobacterium strains. pAgK84 codifies production of and immunity to agrocin 84, the main factor involved in crown gall biocontrol by strain K84. Then, a second generation of strain K84 was obtained and the genetically engineered strain was called K1026. It contains a deletion in the transfer region of pAgK84. To date, a considerable number of studies have been performed to compare both strains in its ability to control crown gall, plasmid transfer, antibiotic production, root colonization and survival in the rhizosphere. The aim of this review is to discuss all this comparative available information which advises that strain K1026 should be used as a biopesticide to safeguard biocontrol of crown gall wherever strain K84 is employed. 相似文献
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Alternaria solani 《Physiological and Molecular Plant Pathology》1996,48(6):361-377
Accumulation of pathogenesis-related proteins is thought to play a role in pathogen-induced plant defense responses. Although early accumulation of hydrolytic enzymes such as chitinase and β-1,3-glucanase has been associated previously with genetically-inherited and induced systemic resistance, their role in resistance in tomato(Lycopersicon esculentum)to the phytopathogenic fungusAlternaria solaniis not yet understood. Here we describe the accumulation patterns of specific isozymes of pathogenesis-related proteins in the resistant tomato genotypes 71B2, NC EBR-1, NC EBR-2 and the susceptible cultivar Piedmont. Western blot analysis demonstrated that four isozymes of chitinase (26, 27, 30, and 32kDa) were induced in all genotypes upon challenge withA. solani,but only resistant lines had significantly higher constitutive levels of the 30kDa isozyme as well as total chitinase activity. In addition, the 30kDa chitinase isozyme was found to accumulate to significantly higher levels in resistant lines during pathogenesis than the susceptible genotype. Two isozymes of β-1,3-glucanase (33 and 35kDa) were detected in all genotypes, but a slightly higher constitutive level was detectable in all resistant lines when compared to the susceptible. Similar accumulation patterns of these isozymes were observed in all genotypes during the course of pathogenesis. Purified preparations of acidic and basic tomato chitinase and β-1,3-glucanase isozymes were tested for their antifungal activity againstA. solani in vitro.Results presented in this study indicate that only basic isozymes of chitinase and β-1,3-glucanase were inhibitory toA. solaniwhereas, no inhibitory activity was observed with the acidic isozymes. The results of this study suggest that a higher constitutive level of chitinase and β-1,3-glucanase and the induction pattern of a 30kDa chitinase isozyme in early blight resistant breeding lines is related to genetically-inherited resistance of tomato toA. solani. 相似文献
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Nobutaka Someya Shinichi Numata Masami Nakajima Akira Hasebe Katsumi Akutsu 《Journal of General Plant Pathology》2004,70(6):371-375
Chitinolytic activity of the biocontrol bacterium Serratia marcescens strain B2 was inhibited by bacteria isolated from rice, even though its growth was not affected. Antifungal activity of the strain against Pyricularia oryzae was also reduced under the influence of these bacteria. In contrast, the rice-epiphytic bacterium Erwinia ananas NR1, transformed with chitinase gene chiA derived from strain B2, had high chitinolytic activity regardless of the presence of the bacteria isolated from rice. Therefore, the introduction of an antagonistic factor gene with a promoter from the recipient into the epiphytic bacteria may prove useful in the development of effective biocontrol agents. 相似文献
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螺旋毛壳ND35 β-1,3-葡聚糖酶的诱导、性质及其抑菌作用 总被引:8,自引:0,他引:8
以病原菌Rhizoctonia solani的细胞壁为诱导物,模拟毛壳菌自然的重寄生过程,研究了内生真菌螺旋毛壳(Chaetomium spirale) ND35 β-1,3-葡聚糖酶的产酶条件、性质,尤其是不同碳源的调控作用。结果表明,不同种类的真菌细胞壁及几丁质和昆布多糖,均可诱导产生β-1,3-葡聚糖酶,而作为分解代谢产物的葡萄糖则抑制产酶。经硫酸铵沉淀、DEAE-Sepharose阴离子交换层析及Phenyl-Sepharose疏水层析,并通过SDS-PAGE鉴定,纯化了一种分子量约为73 kDa的内切β-1,3-葡聚糖酶GLUC73。其最适反应温度为55℃,在40℃以下较稳定;最适pH值为5.5,在pH 5-9范围内均很稳定;酶活性受Hg2+、Fe3+、Zn2+、Mg2+等金属离子不同程度的抑制,Mn2+和Co2+对酶有激活作用;以昆布多糖为底物时,该酶的米氏常数Km为0.412 mg·mL-1,最大反直速度Vmax为3.876 U·mL-1。粗酶液同时具有β-1,3-葡聚糖酶和几丁质酶活性,离体抑菌试验表明,对苹果炭疽病菌(Glomerella cingulata)、杨树腐烂病菌(Valsa sordida)、苹果树腐烂病菌(Valsa mali)的菌丝生长和孢子萌发有明显的抑制作用。通过对β-1,3-葡聚糖进行免疫细胞化学标记和超微结构观察,间接证明了β-1,3-葡聚糖酶在螺旋毛壳重寄生过程中的作用。 相似文献
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喷雾压力和药液流量对井冈·枯芽菌在水稻叶片定殖的影响 总被引:1,自引:0,他引:1
研究了施药机具不同工作压力和药液流量对生物农药井冈.枯芽菌在水稻叶片上定殖数量及活性的影响。盆栽试验结果表明:担架式机动喷雾机、机动弥雾喷粉机和背负式机动喷雾器对生防菌的活性无不利影响。其中担架式机动喷雾机工作压力超过2.5 MPa以上有利于生防菌的定殖;机动弥雾喷粉机同一风速挡、不同流量挡的处理中,流量挡达到2.0 L/m有利于生防菌的定殖。同时生防菌在水稻叶片上定殖数量与水稻纹枯病的防效呈正相关的关系。 相似文献
18.
根癌病生防菌——葡萄土壤杆菌E26菌株在葡萄植株的定殖研究 总被引:2,自引:0,他引:2
利用绿色荧光蛋白基因(gfp)标记示踪,研究了葡萄根癌病生防菌葡萄土壤杆菌E26菌株应用到田间后在玫瑰香葡萄(Vitis vinifera cv. Muscat Humbug)根表面和根际土壤中的群体数量变化,比较了E26菌株与葡萄根癌病原菌K308菌株室内人工接种后在玫瑰香葡萄苗茎和根外植体伤口部位的附着情况.在田间自然状况下,E26菌株可以在葡萄根表面和根际土壤中存活定殖.接种5个月后,E26在根表面的平均数量为104cfu/g根(鲜重),在根际土壤中的平均数量为104cfu/g土壤(干重).在室内,E26菌株和K308菌株分别单独接种时均能以相似水平附着在葡萄茎和根的伤口;E26和K308以相同数量同时接种时,附着在葡萄伤口细胞的K308的数量显著低于K308单独接种时所附着在葡萄伤口细胞的数量.扫描电镜显微观察证实E26菌株能够和病菌K308菌株一样附着于葡萄根部伤口处. 相似文献
19.
本试验考察了土壤温度、有机质含量和pH对海洋生防细菌多粘类芽胞杆菌L_1-9在黄瓜根表土壤中定殖的影响。采用实时荧光定量PCR方法检测了不同时期黄瓜根表土壤中菌株L_1-9的16S r DNA拷贝数。结果表明,土壤有机质含量、土壤温度和pH对菌株L_1-9在黄瓜根表的定殖有显著影响(P0.01)。25℃定殖数量最高,为5.79×108拷贝/g土,是15℃时的3.4倍;添加有机肥20~40 g/kg土壤,可以促进菌株L_1-9在黄瓜根际定殖;pH 7时,菌株L_1-9在黄瓜根表土壤中的定殖数量最高。本研究为海洋生防菌L_1-9防治黄瓜土传病害提供了理论依据。 相似文献