无花果内生菌Alternaria sp.QDFB-2菌丝体化学成分的研究

为研究无花果枝条内生真菌Alternaria sp.QDFB-2菌丝体的化学成分,采用硅胶柱层析、Sephadex LH-20凝胶柱层析、反相柱层析和高效液相色谱等方法对Alternaria sp.QDFB-2菌丝体粗浸膏进行分离纯化,利用核磁共振谱(NMR)和质谱(MS)等现代波谱技术、结合文献比对方法确定化合物的结构;采用MTT法进行化合物的体外细胞毒活性评价。结果表明:从Alternaria sp.QDFB-2菌丝体粗浸膏中分离纯化得到7种化合物:alternariol(1)、tentoxin(2)、dihydrotentoxin(3)、cyclo(Gly-Pro)(4)、cyclo(4-hydroxy-Pro-Pro)(5)、cyclo(S-Leu-S-N-methyl-Phe)(6)和uridine(7)。体外细胞毒活性评价显示,化合物1和7对SMMC-7721细胞具有中等增殖抑制活性,其IC50值分别为50.47μg·mL^(-1)(195.62μmol·L^(-1))和42.50μg·mL^(-1)(174.18μmol·L^(-1));化合物1对A549细胞也具有中等的增殖抑制活性,浓度为100μg·mL^(-1)时抑制率为52.12%;阳性对照顺铂的IC50值分别为3.46μg·mL^(-1)(11.53μmol·L^(-1))和5.12μg·mL^(-1)(17.06μmol·L^(-1))。Alternaria sp.QDFB-2菌丝体的化学成分丰富,值得深入研究。

Comparative transcriptome analysis reveals key genes and pathways in response to Alternaria alternata apple pathotype infection

Apple leaf spot,caused by the Alternaria alternata apple pathotype(AAAP),is an important fungal disease of apple.To understand the molecular basis of resistance and pathogenesis in apple leaf spot,the transcriptomes of two apple cultivars‘Hanfu'(HF)(resistant)and‘Golden Delicious'(GD)(susceptible)were analyzed at 0,6,18,24 and 48 h after AAAP inoculation by RNA-Seq.At each time point,a large number of significantly differentially expressed genes(DEGs)were screened between AAAP-inoculated and uninoculated apple leaves.Analysis of the common DEGs at four time points revealed significant differences in the resistance of‘HF'and‘GD'apple to AAAP infection.RLP,RNL,and JA signal-related genes were upregulated in both cultivars to restrict AAAP development.However,genes encoding CNLs,TNLs,WRKYs,and AP2s were only activated in‘HF'as part of the resistance response,of which,some play major roles in the regulation of ET and SA signal transduction.Further analysis showed that many DEGs with opposite expression trends in the two hosts may play important regulatory roles in response to AAAP infection.Transient expression of one such gene MdERF110 in‘GD'apple leaves improved AAAP resistance.Collectively,this study highlights the reasons for differential resistance to AAAP infection between‘HF'and‘GD'apples which can theoretically assist the molecular breeding of disease-resistant apple crops.

响应面法研究链格孢菌Alternaria ochroleuca的产毒条件

比较了不同链格孢菌(Alternaria ochroleuca、Alternaria alternata和Alternaria tenuissima)的产毒能力,并通过单因素实验和响应面试验考察了不同的培养温度、培养时间和培养基初始pH对A.ochroleuca产主要链格孢霉毒素链格孢酚(AOH)、链格孢甲基醚(AME)和细交链格孢菌酮酸(TeA)3种毒素的影响。结果表明:3种毒素的产量均随培养温度、培养时间和培养基初始pH的增加呈先增加后逐渐减少的趋势,培养温度26.8℃、培养时间11.4 d、培养基初始pH 4.7是TeA的最佳产生条件,最大产量为4841.3 mg∕kg;当培养温度为25.9℃、培养时间为7.8 d、培养基初始pH为6.4时,AOH和AME的产量最高,分别达2096.1 mg∕kg和152.8 mg∕kg。培养温度和培养基初始pH对TeA的产生具有显著的交互作用,而培养温度和培养时间对AOH和AME的产生具有显著的交互作用。本研究明确了链格孢菌A.ochroleuca产生链格孢霉毒素的主要影响因素,对控制链格孢霉毒素污染、保障食品安全具有重要意义。

甘肃省陇南市核桃枝枯病菌Alternaria alternate的生物学特性

以核桃枝枯病菌(Alternaria alternate)为对象,研究温度、碳源、氮源、光照、培养基和pH等对菌丝生长、产孢量和孢子萌发的影响。结果表明,pH 7和全黑暗有利于核桃枝枯病菌的菌丝生长、产孢和孢子萌发;25℃有利于菌丝生长,25~30℃有利于产孢,20~30℃有利于孢子萌发;最适生长的碳源为可溶性淀粉,氮源为酵母浸粉、KNO_(3)和蛋白胨,最适产孢的碳源和氮源分别为山梨醇和KNO_(3),最适孢子萌发的碳源和氮源分别为乳糖和NH_(4)NO_(3);PSA、OA和PDA培养基适合菌丝生长,LB培养基适合产孢,OA培养基适合孢子萌发。该研究结果为明确核桃枝枯病的发生规律提供理论依据,也为综合防治措施的制定提供参考。

无花果内生菌Alternaria sp.QDFB-2发酵液的聚酮类化学成分研究

目的研究无花果内生菌Alternaria sp.QDFB-2发酵液的聚酮类化学成分及其体外细胞毒活性。方法综合采用硅胶柱、Sephadex LH-20凝胶柱、ODS反相柱和高效液相色谱法等方法对Alternaria sp.QDFB-2发酵液的化学成分进行分离纯化,再利用核磁共振谱(NMR)、高分辨质谱(HR-MS)等现代波谱技术和文献比对方法鉴定化合物结构,最后采用四甲基偶氮唑蓝(MTT)法测定化合物的体外细胞毒活性。结果从Alternaria sp.QDFB-2发酵液乙酸乙酯粗浸膏中共分离得到7个聚酮类化合物,分别为7-hydroxy-2,5-dimethyl-4H-1-benzopyran-4-one(1)、1-deoxyrubralactone(2)、alternariol-9-O-monomethyl ether(3)、alternariol(4)、altenuisol(5)、stemphyperylenol(6)和altertoxinⅠ(7)。体外细胞毒活性测定结果表明,化合物4对人宫颈癌细胞株HeLa和人肝癌细胞株SMMC-7721具有显著的增殖抑制活性,半抑制浓度(IC50)分别为13.43和50.47μg/mL。结论Alternaria sp.QDFB-2能产生丰富的聚酮类化合物,极具开发微生物药物的研究价值。

酚酸介导下连作茶树根际病原菌Alternaria sp.及其拮抗菌Pseudomonas sp.变化

茶树是我国重要的经济作物,然而长期宿根连作铁观音茶园存在土壤微生物群落结构失衡、病害加重等连作障碍问题,探究铁观音茶树连作障碍形成的分子机制对寻求有效的防控技术具有重要意义。采用微生物分离纯化、平板对峙等方法对铁观音茶树根际病原菌及其拮抗菌进行分离、鉴定,并对不同宿根连作年限(0、1、10、20 a)铁观音茶树根际土壤中的病原菌和拮抗菌数量进行定量分析;同时运用高效液相色谱(HPLC)技术分析不同连作年限根际土壤中酚酸含量变化,并模拟土壤中各酚酸配比,研究酚酸类物质对茶树根际病原菌及其拮抗菌的影响。结果显示,从连作20 a患病铁观音茶树根系分离鉴定到1株病原真菌链格孢菌(Alternaria sp.),并从根际土壤中筛选到1株拮抗菌假单胞菌(Pseudomonas sp.)。荧光定量PCR分析发现,与1 a茶园相比,20 a茶园土壤中的链格孢菌绝对含量显著偏高,而假单胞菌含量却显著偏低。连作茶园根际土壤中共检测到对羟基苯甲酸、香草酸、丁香酸、香兰素、阿魏酸5种酚酸类物质,其平均配比为38∶229∶11∶11∶3。连作条件下酚酸类物质并未在土壤中累积,而是随种植年限的延长呈现出先增加后降低的趋势。模拟试验发现,中低浓度(30~120μmol·L^(-1))的混合酚酸能够显著促进链格孢菌菌丝的生长,单一酚酸对羟基苯甲酸、香草酸和丁香酸在低浓度(30μmol·L^(-1)和60μmol·L^(-1))时也能够显著促进链格孢菌菌丝的生长。对羟基苯甲酸对假单胞菌的生长有抑制作用,并且随着浓度的增加抑制作用增强,混合酚酸以及其他单一酚酸对假单胞菌的生长无明显作用。由此可见,铁观音根系分泌物酚酸类物质对根际土壤关键微生物菌群具有不同的生态效应,是引起微生物群落结构失衡、病害增加等连作障碍问题的重要因素。研究结果为进一步揭示铁观音茶树连作障碍机理提供一些理论依据。

链格孢(Alternaria alternata)在枣、梨和苹果果实上的致病性分化研究

链格孢(Alternaria alternata)可侵染多种果树引起产前及产后果实黑斑病,造成严重的经济损失。不同果树来源的链格孢是否能交互传染还不清楚。本文探讨了引起北方枣、梨和苹果果实黑斑病的链格孢在这3种果实上的致病性分化和交互致病性,明确其交互传染特性。从北方不同地区果园采集枣、梨和苹果的黑斑病病果样品,通过组织分离法进行病原菌的分离,然后进行纯化及鉴定。利用离体果实接种法对分离到的各个病菌分别在枣、梨、苹果的果实上进行致病性测定,分析了其致病性的差异。结果显示:从3种病果实上共分离出45株链格孢,其中对枣、梨和苹果表现出强致病性的分别为5、11、7株,表现为弱致病的分别为17、8、20株;对3种果实的致病性均在次强等级以上的有6株,致病性均为弱等级的有3株,而在3种果实上致病性等级表现为次强等级以上的菌株有30株,占到总菌株的66.6%。总之,枣、梨和苹果病果上的链格孢存在致病性分化现象,并在这3种果实上是可以交叉侵染致病,互为侵染源。因此,在病害防治方面,临近的不同果园对黑斑病需联防联治。

广西山口红树内生真菌Alternaria sp.SK6YW3L中的蒽醌类化合物

研究了广西山口红树林自然保护区的红树植物无瓣海桑Sonneratia apetala来源内生真菌Alternaria sp.SK6YW3L的次级代谢产物。利用w=3%盐度的大米培养基对该菌株进行发酵培养,并综合运用正、反相硅胶柱层析,半制备HPLC,Sephadex LH-20凝胶层析和重结晶等分离手段,从中分离获得了13个蒽醌类化合物(1~13)。再利用1D/2D NMR和MS等现代波谱技术,并与文献波谱数据对比分析,鉴定化合物为:7-acetyl-1,3,6-trihydroxyanthracene-9,10-dione(1)、(11S)-1,3,6-trihydroxy-7-(1-hydroxyethyl)anthracene-9,10-dione(2)、7-O-demethyl-6-deoxybostrycoidin(3)、altersolanol A(4)、dactylariol(5)、altersolanol B(6)、emodin(7)、emodin-3-methyl ether(8)、6-hydroxy-aloeemodin(9)、anthraquinone A(10)、1,5-dihydroxy-7-methoxy-2-methylanthracene-9,10-dione(11)、alterporriol N(12)和alterporriol A(13)。采用铜靶单晶X-Ray衍射技术分析了化合物1和4的单晶结构,其中1为新单晶,并确定了化合物4的绝对构型为5R,6S,7R,8S。其他化合物的绝对构型通过比对文献和旋光试验和CD数据确定。活性结果显示,化合物1~3对α-葡萄糖苷酶表现出中等的抑制活性,IC50值分别为(210.1±1.2),(125.8±1.5)和(68.7±1.3)μmol/L。

Exploring the nano-fungicidal efficacy of green synthesized magnesium oxide nanoparticles(MgO NPs)on the development,physiology,and infection of carrot(Daucus carota L.)with Alternaria leaf blight(ALB):Molecular docking

In this research,green synthesized magnesium oxide nanoparticles(MgO NPs)from lemon fruit extracts and their fungicidal potential was evaluated against Alternaria dauci infection on carrot(Daucus carota L.)under greenhouse conditions.The scanning and transmission electron microscopy(SEM and TEM)and ultra-violet(UV)visible spectroscopy were used to validate and characterize MgO NPs.The crystalline nature of MgONPs was determined using selected area electron diffraction(SAED).MgO NPs triggered substantial antifungal activity against A.dauci when exposed to 50 and 100 mg L^(–1)concentrations but the higher antifungal potential was noticed in 100 mg L^(–1)under invitro conditions.In fungal inoculated plants,a marked decrease in growth,photosynthetic pigments,and an increase in phenol,proline contents,and defense-related enzymes of carrot were seen over control(distilled water).However,foliar application of MgO NPs at 50 and 100 mg L^(–1)resulted in significant improvement of plant growth,photosynthetic pigments,phenol and proline contents,and defense enzymes activity of carrots with and without A.dauci infection.Spraying of MgO NPs at 100 mg L^(–1)had more plant length(17.11%),shoot dry weight(34.38%),plant fresh weight(20.46%),and root dry weight(49.09%)in carrots when challenged with A.dauci over inoculated control.The leaf blight indices and percent disease severity were also reduced in A.dauci inoculated plants when sprayed with MgO NPs.The non-bonding interactions of Alternaria genus protein with nanoparticles were studied using molecular docking.

凤丹皮内生真菌Alternaria arborescens发酵产物中甾醇类化合物

目的研究从铜陵凤凰山牡丹根皮中分离得到的一株内生菌Alternaria arborescens的次生代谢产物。方法应用硅胶柱色谱结合半制备高效液相色谱分离技术对发酵液的乙酸乙酯提取部位进行分离纯化,并经核磁共振、质谱分析,与文献对比鉴定结构。结果分离得到6个甾醇类化合物,分别鉴定为(22E,24R)-麦角甾-7,22-二烯-3β,5α,6β-三醇(1)、麦角甾醇(2)、5α,8α-环氧-(22E,24R)麦角甾-6,22-二烯-3β-醇(3),5α,8α-环氧-(22E,24R)麦角甾-6,9,22-三烯-3β-醇(4),麦角甾-7,22-二烯-3β-醇(5)和β-谷甾醇(6)。结论化合物1~6为首次从该内生菌的发酵液中分离得到。

Three new amide derivatives from the fungus Alternaria brassicicola

Three new amide derivatives(alteralkaloids A-C,1-3)and three known alkaloids(4-6)were afforded after phytochemical investigation of fungus Alternaria brassicicola.The structures of these compounds were confirmed by NMR spectroscopic and HRESIMS data.Furthermore,the absolute configuration of 1 was determined using the single-crystal X-ray diffraction analysis.Compounds 1-3 belong to a class of amide derivatives that have not been found in nature before,sharing the same characteristic signals of the butyl moiety and amide group.These isolated compounds mentioned above were tested for the cytotoxic activity.

Morphological and Molecular Identification of Alternaria alternata Causing Leaf Spot Disease on Huangdi Banana in China

[Objectives]The paper was to identify Alternaria alternata causing leaf spot disease on Huangdi banana in China.[Methods]Fungal isolates were isolated and identified by morphological features,molecular identification and pathogenicity test.[Results]There were light to dark brown,tiny oval spots on leaves.The causal agent isolated from affected leaves was identified as A.alternata based on the morphological properties,coupled with sequence analyses of the internal transcribed spacer(ITS)region,large subunit ribosomal DNA(LSU rDNA)and the translation elongation factor 1-alpha(TEF-1α)gene.Koch s postulates were fulfilled by successful re-isolation of pathogen from the artificial inoculated leaves.[Conclusions]To our knowledge,this is the first report of leaf spot caused by A.alternata on Huangdi banana in China.The identification of A.alternata as the causal agent of the observed leaf spot disease on Huangdi banana is critical to the prevention and control of this disease in the future.

Molecular Identification of Alternaria alternate (Fr.) Keissl. from the Leaf Blight Disease of Centella asiatica L.

Centella asiatica (L.), frequently known as Thankuni, is an important ethnobotanical plant in Bangladesh. This study was conducted to evaluate the morphological characteristics, cultural factors and molecular identification of the causal agent of Alternaria leaf blight disease of C. asiatica. The potato dextrose agar (PDA) medium recorded the maximum mycelial growth (69 mm), followed by the yeast extract agar (YEA) medium, while the honey peptone agar (HPA) medium recorded the lowest growth (27 mm). The optimal pH and temperature for mycelial growth of Alternaria alternata were 6 and 30°C, respectively. Internal transcribed spacer (ITS) region of Alternaria alternata PCR products measured 558 bp and blast search showed 99% sequence similarity with Alternaria alternata species complex. To the best of our knowledge, Alternaria leaf blight disease caused by Alternaria alternata is the first record in Bangladesh.

茄链格孢Alternaria solani DT-15除草活性及生物学特性初步研究

为了筛选获得高效除草生防菌株,本研究以青海省大通县野薄荷病样中分离到的DT-15菌株作为研究对象,对其进行离体致病性测定、活体除草效果评价、安全性评价、菌株分类鉴定及菌株最适碳氮源筛选研究。离体条件下DT-15菌株对3种杂草的致病性由强到弱依次为密花香薷>冬葵>藜。盆栽条件下藜、冬葵发病率高达91%以上,鲜重防效达94%以上,且对主栽作物蚕豆、小麦、豌豆、油菜表现为相对安全。菌株DT-15鉴定为茄链格孢Alternaria solani。对菌落直径、孢子悬浮液的OD值进行了测定,结果表明:小麦麸皮是最适的碳源,硝酸钠是最适的氮源。DT-15菌株具有蚕豆、小麦、豌豆、油菜田防除部分阔叶杂草的微生物除草剂开发潜力。

烟草叶围细菌的分离及其对Alternaria alternata的拮抗作用

分离到烟草叶围细菌136株,通过对峙培养实验筛选出对烟草赤星病菌A.alternata有较强拮抗活性的9个菌株。离体叶片生防测定实验表明,9株细菌均能不同程度地减轻烟草赤星病的发生。其中菌株Tpb88具有较强和稳定的拮抗作用,无菌滤液实验表明,叶围细菌Tpb88在一定浓度范围内能有效抑制A.alternata菌丝生长、孢子萌发和芽管伸长,且浓度越高,抑制能力越强,结果表明Tpb88对烟草赤星病菌的拮抗机制可能为抗菌物质的产生。

Establishment of Protoplast Transformation System in Alternaria tenuissima Using G418 Selection Marker

[Objective] The study aimed to establish a protoplast transformation system in Alternaria tenuissima. [Method] The protoplast of A.tenuissima was firstly prepared by enzymolysis method; then the yielded protoplast was transformed by G418 resistant DNA plasmid using PEG/CaCl2 method. [Result] The growth phenotype and PCR detection showed that resistance gene had integrated into A.tenuissima genome. The transformation efficiency of this method reached per μg DNA 3-4 transformants. After subculture thrice under nonselective condition, G418 resistance could still inherit stably. [Conclusion] The transformation system of A.tenuissima was successfully established, which laid basis for studying of the gene function of Alternaria tenuissima.

真菌Alternaria sp.XZSBG-1的四氢蒽醌类次级代谢产物

采用硅胶、C-18反相硅胶、Sephadex LH-20等柱色谱及高效液相色谱技术对真菌Alternaria sp.XZSBG-1的次级代谢产物进行系统研究;采用波谱分析及与文献比对等方法鉴定化合物结构;采用MTT法和比色法进行抗肿瘤和酶抑制活性筛选。结果从真菌Alternaria sp.XZSBG-1的发酵物中分离得到8个四氢蒽醌类化合物,分别鉴定为Alterporriol F'(1)、Alterporriol G'(2)、Alterporriol F(3)、Alterporriol G(4)、Altersolanol A(5)、Altersolanol F(6)、Tetrahydroaltersolanol B(7)和Tetrahydroaltersolanol D(8);活性测试结果表明仅化合物6对结肠癌细胞株(HCT-116)和子宫癌细胞株(Hela)具有明显抑制活性,IC50值分别为3.026和8.094μmol/L。

海参共生微生物HS-3 Alternaria sp.次级代谢产物的研究

目的:对自山东半岛芝罘岛海域的刺参中分离出的HS-3 Alternaria sp.真菌的次级代谢产物进行研究。方法:利用土豆培养基对该菌进行培养,通过薄层层析、柱层析、高效液相等分离手段,从HS-3的培养液中分离出4个化合物。结果:经过现代波谱手段,分别鉴定为:1-羟基-3-甲基-9,10-二酮蒽醌(1)、大黄酚(2)、sterigmatocystin(3)、脑苷酯类化合物(4)。结论:该研究为深入研究开发刺参提供了科学数据,这4个化合物首次从海参的共生微生物中得到。

直缘乌头内生真菌Alternaria solani化学成分研究

目的:对直缘乌头内生真菌Alternaria solani的化学成分进行研究。方法:采用各种柱色谱对直缘乌头内生真菌Alternaria solani的甲醇提取物进行分离纯化,经波谱数据(1H-NMR,13C-NMR,MS)进行结构鉴定。结果:分离得到15个化合物,分别鉴定为:20-羟基麦角甾-4,6,8(14),22-四烯-3-酮(1)、(22E,24R)-麦角甾-4,6,8(14),22-四烯-3-酮(2)、(22E,24R)-麦角甾-7,22-二烯-3β-醇(3)、24-亚甲基-麦角甾-7-烯-3β-醇(4)、过氧麦角甾醇(5)、cyclo(D)-Pro-(D)-Leu(6)、cyclo-(L-Val-LPro)(7)、cyclo-(S-Pro-S-Ile)(8)、tentoxin(9)、porrotoxin(10)、7-dehydroxyl-zinniol(11)、zinniol(12)、8-zinniol methyl ether(13)、3-甲氧基-4-甲基-5-(3’,3'-二甲基烯丙氧基)-2-甲氧基甲基苯甲酸(14)、拟盘多毛孢H2-倍半萜内酯(15)。结论:从直缘乌头内生真菌Alternaria solani中分离得到15个化合物,其中化合物2~10,12~15是首次从该植物内生真菌中分离得到。

除草活性菌株极细链格孢菌(Alternaria tenuissima)发酵工艺研究

【目的】探索一株防治藜、冬葵等阔叶杂草的生防菌株极细链格孢(Alternaria tenuissima)HZ-1的发酵工艺.【方法】采用液固双相发酵方式,通过单因素和正交设计试验,对该菌株固态发酵基质、最适碳氮源和固-液发酵条件进行研究.【结果】HZ-1最佳产孢的固态基质为麦麸,最适碳源为麦麸(40 mg/g),最适氮源为蛋白胨(50 mg/g).正交优化试验得出该菌最适固-液发酵条件为:培养基初始含水量为300 mg/g,适宜的接种量为0.3 mL/g,初始pH值7.4,最适温度为24.3℃,发酵最适时间为216 h.【结论】研究结果可为该极细链格孢菌菌株除草活性物质的分离及工业化生产提供依据.