短短芽孢杆菌JK-2菌株对番茄枯萎病的抑菌作用及其小区防效

对分离自土壤的短短芽孢杆菌JK-2菌株对番茄枯萎病菌的防治效果和抑制作用进行了研究。结果表明：JK-2对番茄枯萎病菌的盆栽防效和田间防效分别为83．82％、74．70％。该菌株能抑制枯萎病菌菌丝的生长，当其无菌滤液终浓度为15％时，对菌丝生长的抑制率达到81．69％。JK-2菌株对病菌孢子萌发也有较强的抑制作用。扫描电镜观察结果：JK-2菌株可造成菌丝消解、产生泡状物、破坏生长点、引起细胞内含物外溢。     

T-DNA随机插入法获得甘薯蔓割病菌非致病生防菌株

由尖孢镰刀菌甘薯专化型Fusarium oxysporum f.sp.batatas引起的甘薯蔓割病是甘薯生产上一种重要病害。本研究将带有GFP绿色荧光蛋白基因的T-DNA随机插入到蔓割病菌基因组中,获得711个突变体。经过致病力筛选,获得了3株非致病突变体,编号为50-5、55-7和103-4,其中50-5和103-4产孢能力显著下降。平板对峙试验结果表明这3株非致病突变体均可和蔓割病菌发生营养竞争作用。通过提前对感病品种"新种花"接种非致病突变体,再接种蔓割病菌,结果显示当蔓割病菌和非致病突变体孢子浓度同为5×10~5 CFU/m L时,103-4和55-7分别预处理感病品种8 h后,生防效果趋于稳定,分别为86.95%和83.80%;50-5预处理16 h后生防效果趋于稳定,为75.65%。以上结果表明,通过农杆菌转化筛选非致病突变体的方法,成功获得3株蔓割病生防菌株,为深入开展甘薯蔓割病的生物防治提供基础,也为其他尖孢镰刀菌创造非致病生防菌提供借鉴。     

番茄枯萎病和青枯病拮抗细菌的筛选、评价与鉴定

从宁夏银川、江苏沭阳和福建厦门的番茄、辣椒、西瓜等作物根际土壤中,分离纯化获得367株细菌菌株。以番茄枯萎病菌Fusarium oxysporum f.sp.lycopersici和番茄青枯病菌Ralstonia solanacearum为靶标菌,从367株菌株中筛选出对两种病菌皆具有很强拮抗作用的菌株22株。拮抗细菌抑菌物质的研究结果表明：22株拮抗细菌均能分泌蛋白酶;不能分泌几丁质酶;3株细菌能分泌纤维素酶;3株细菌能分泌嗜铁素。盆栽试验结果表明：拮抗细菌PTS-394对番茄枯萎病和青枯病的防效最高,分别为77.4%和80%;菌株H-70、L-1和SJ-280对番茄枯萎病和青枯病的防效均大于60%。对上述4株拮抗细菌进行16S rRNA种属鉴定,均为枯草芽孢杆菌Bacillus subtilis。     

韭菜对巴西香蕉枯萎病发生的抑制作用

采取田间试验、盆栽试验及实验室研究相结合的方法,研究了韭菜对香蕉枯萎病的防控效果。田间试验表明,韭菜之后轮作香蕉,第1年香蕉枯萎病平均发病率仅为1.73%（对照为52%）。盆栽试验表明,韭菜处理对香蕉枯萎病发病抑制率为85.9%,病情抑制率为82%;而且韭菜叶片的水提取液对香蕉枯萎病菌（Fusarium oxysporum f.sp.cubense,FOC）孢子增殖抑制率为91.2%,对其致死率为86.97%。本研究表明,韭菜轮作香蕉的种植模式是一种防控香蕉枯萎病的有效途径,而且韭菜及其制剂有望发展成为防控香蕉枯萎病的环境友好型的新型生物试剂。     

假单胞菌对香蕉枯萎病菌的抑制作用

从已感染香蕉枯萎病的果园中分离到1株对香蕉枯萎病菌（Fusarium oxysporum f.sp.cubense）抑制作用很好的菌种,命名为G1。采用固体和液体培养法从不同角度证实了G1对香蕉枯萎病菌生长的抑制作用。结果表明,G1的发酵液、无菌滤液、挥发性物质、非挥发性代谢产物的平均抑菌率分别为92.5%、27.4%、73.8%、57.7%,可见抑制作用与活菌体有直接关系,其中产生挥发性物质尤其重要。液体培养的病原菌浓度为1.0×107cfu/mL经G1作用10d后,取样镜检发现G1通过抑制病原菌菌丝正常生长以至不能产孢,从而导致菌丝消融;通过吸附在孢子的周围,融解细胞壁,造成原生质泄露致使孢子死亡。     

龟裂链霉菌M527抗真菌物质的分离鉴定及其在黄瓜枯萎病防治中的应用

为探明龟裂链霉菌Streptomyces rimosus M527发酵液中抗真菌成分及其对黄瓜枯萎病菌的拮抗作用,本试验以黄瓜枯萎病菌F. oxysporum f. sp. cucumerinum为活性跟踪指示菌。首先,通过有机溶剂萃取、硅胶柱层析、DiaionHP-20凝胶柱层析、制备型HPLC对活性化合物进行分离纯化,结合MS、1H-NMR和13 C-NMR波谱数据对活性化合物结构进行解析,从菌株M527的发酵液中分离得到活性化合物与龟裂杀菌素一致。结果表明,当龟裂杀菌素浓度为2.20 mg/L时,能够完全抑制黄瓜枯萎病菌的孢子萌发;当龟裂杀菌素浓度为8.78 mg/L时,黄瓜枯萎病菌的菌丝生长受到明显抑制。17.56 mg/L的龟裂杀菌素溶液与传统农药乙蒜素（80%）1000倍稀释液进行黄瓜盆栽试验,施药后14和21 d龟裂杀菌素的治疗效果分别为78.3%和70.6%,乙蒜素的治疗效果为66.7%和42.7%。     

杨浦链霉菌WLU210的筛选、鉴定及其对苦瓜枯萎病的生防作用研究

本研究从河南黄河湿地采集土壤样品,采用梯度稀释涂布平板法分离和平板对峙培养法筛选获得一株对苦瓜枯萎病菌具有稳定拮抗活性的链霉菌WLU210。在形态学鉴定和生理生化特征测定的基础上,对菌株WLU210的16S rRNA基因序列进行比对分析,将WLU210鉴定为杨浦链霉菌Streptomyces yangpuensis;拮抗谱测定结果表明,杨浦链霉菌WLU210对苦瓜枯萎病菌、苹果轮纹病菌、小麦茎基腐病菌、辣椒疫霉病菌、西瓜炭疽病菌、小麦全蚀病菌和玉米大斑病菌等7种植物病原菌均具有一定的拮抗活性;盆栽试验和田间试验结果表明,杨浦链霉菌WLU210发酵液具有有效防治苦瓜枯萎病和促进苦瓜生长的作用,田间防治效果达68.89%。由此可见,杨浦链霉菌WLU210具有作为防治苦瓜枯萎病生防菌剂研发的潜力。     

甘蓝枯萎病菌REMI转化体系的建立

建立高效、稳定的甘蓝枯萎病菌REMI转化体系,为进一步获得特定表型突变体及基因功能研究建立技术储备.利用REMI(restriction enzyme mediate intergration)转化方法,将线性化的含有潮霉素抗性基因的pUCAT-PH质粒转化甘蓝枯萎病菌A6菌株的原生质体,摸索获得转化子最适的潮霉素筛选浓度以及不同限制性内切酶和酶量对转化效率的影响;利用PCR(polymerase chain reaction)技术对潮霉素抗性转化子进行验证.结果表明转化子的最适潮霉素筛选浓度为50 μg/mL;转化效率较高的限制性内切酶为HindⅢ,并且转化效率最高时的酶量为20 U.利用该转化体系构建了含1 050个转化子的甘蓝枯萎病菌转化子库,对转化子进行Southern验证,证明该转化体系是可行的.     

Influence of chickpea genotype and Bacillus sp. on protection from Fusarium wilt by seed treatment with nonpathogenic Fusarium oxysporum

Seeds of kabuli chickpea cultivars ICCV 4 and PV 61 were treated with conidia of nonpathogenic Fusarium oxysporum isolate Fo 90105 suspended in methylcellulose (3 × 10⁶ conidia.seed^-1), or with methylcellulose alone, and sown in soil artificially infested with 500 or 1,000 chlamydospores.g^-1 of F. oxysporum f. sp. ciceris race 5. At an inoculum concentration of 500 chlamydospores.g^-1, seed treatment with Fo 90105 significantly increased the incubation period of the disease by 11 (ICCV 4) or 25 (PV 61) days, and reduced the final disease incidence, disease intensity and the standardized area under the curve of disease intensity over time. This protection from disease was higher and more consistent in PV 61 than in ICCV 4. However, it was annulled with an inoculum concentration of 1,000 chlamydospores.g^-1, except for the incubation period in PV 61 which was increased by 10 days. When ICCV 4 seeds were treated with Fo 90105 (3 × 10⁶ conidia.seed^-1) and/or Bacillus sp. isolate RGAF 51 (1 × 10⁷ cfu.seed^-1), then sown in infested soil, there was no influence by the Bacillus isolate on protection conferred by Fo 90105. However, the degree of protection by the nonpathogenic F. oxysporum was higher and more consistent when plants from treated seeds were grown in sterile sand for 6 days, then transplanted into infested soil.     

Fusarium confers protection against several mycelial pathogens of pepper plants

Inoculation of nonhost pepper ( Capsicum annuum ) plants with the tomato wilt pathogen, Fusarium oxysporum f.sp. lycopersici (FOL), caused no symptoms and the fungus was not recovered from any part of the plant. FOL, however, partially protected pepper plants from subsequent infection with Phytophthora capsici , Verticillium dahliae or Botrytis cinerea by significantly reducing the percentage of diseased plants and the appearance and intensity of symptoms. FOL did not inhibit the mycelial growth of these pathogens in vitro . The protection induced by FOL against Botrytis was inhibited by 1-methylcyclopropene (MCP), an inhibitor of ethylene perception, suggesting the involvement of this hormone in the signalling of FOL-induced resistance. The activities of β-1,3-glucanase and peroxidase 48 h after FOL induction were similar to those in control plants. Chitinase activity, however, was higher in the stems of plants inoculated with FOL. A study of the levels of phenolic compounds revealed that cell-wall-bound phenolics were more abundant in plants treated with FOL, especially in stems, while soluble phenolic contents did not differ.     

黄瓜枯萎病菌毒力、营养体亲和性及ISSR分析

 本研究对来自哈尔滨、长春、沈阳、北京、西宁5个城市的70个尖孢镰刀菌黄瓜专化型菌株进行了毒力、营养体亲和性及ISSR分析。毒力测定结果显示黄瓜枯萎病菌在东农803品种上存在明显的毒力分化。在营养体亲和群的测定中有8个菌株没有产生nit突变体,2个菌株经测定为异核体自身不亲和性菌株,不能进行营养体亲和群的测定;其余60个菌株可分为5个营养体亲和群。利用筛选的7个引物对70个菌株进行了ISSR分子标记,聚类分析可将70个菌株分为3个类群,其中IGⅠ的41个菌株均来自东北三省,IGⅡ的21个菌株均来自北京,IGⅢ的8个菌株全部来自西宁。VCGs和ISSRs与菌株的地理来源及毒力存在一定的相关性。     

抗香蕉枯萎病菌拮抗菌的鉴定及其定殖

通过逐步提高药物浓度方法,获得了抗利福平400μg/ml、对香蕉枯萎病菌拮抗活性稳定的T2WF和W10标记菌株。初步确定两菌株为芽孢杆菌属细菌。采用灌根接种法,在香蕉苗根际土和香蕉苗体内定殖结果表明,拮抗菌液接种浓度为5×104cfu/ml,两菌株均可从香蕉根际土和香蕉体内分离到,并在香蕉体内定殖和传导。在香蕉根际土、根部、球茎和假茎中,T2WF标记菌的菌量高峰分别出现在接种后5、5、11和3d,分别为707、437、273、117cfu/mg;而W10标记菌的菌量高峰分别出现在接种后5、3、5和5d,分别为784、260、253、110cfu/mg。两菌株在香蕉根际土和香蕉体内1~15d的消长动态均有一个共同的“由升到降”趋势。从数量和数量变动幅度上看,香蕉根部的菌量明显高于茎部的菌量。     

西瓜枯萎病菌遗传多样性的相关序列扩增多态性分析

对30个西瓜枯萎病菌Fusarium oxysporum f.sp.niveum菌株基因组DNA进行相关序列扩增多态性(SRAP)分子标记分析,以探究其遗传多样性与地理来源的关系。采用尖孢镰刀菌西瓜专化型Fusarium oxysporumf.sp.niveum0、1、2号生理小种的基因组DNA为模板,对225对SRAP引物进行筛选,筛选出20对多态性、重复性较好且条带清晰的引物,对30个菌株进行PCR扩增,共扩增出386条带,其中多态性条带有371条,多态性比率为96.11%,平均每对引物扩增出19.3个位点和18.55个多态性位点。UPGMA法聚类分析结果显示,供试菌株两两之间的遗传相似系数范围为0.69~0.90,平均为0.79,说明尖孢镰刀菌西瓜专化型的遗传多样性较为丰富。基于SRAP标记聚类分析表明,30个菌株在遗传相似系数为0.70处被划分为3个类群,I类群包含24个菌株,其中18个来自湖南省,Ⅱ类群只包含1个来自黑龙江省哈尔滨市的菌株,它和另一个来自黑龙江地区的菌株被划分到不同的类群,且遗传距离相对较远;Ⅲ类群包含了5个菌株,其中3个来自海南三亚,其余两个来自湖南省。根据菌株的分布情况来看,菌株的聚集与地理来源没有明显的相关性。     

一种快速、有效的香蕉枯萎病病原菌FOC4的分子检测方法

以ITS测序与SCAR分子标记相结合的香蕉病原菌FOC4分子检测方法,利用通用引物ITS1和ITS4对病原菌SF001的rDNA中ITS序列进行PCR扩增,获得560bp左右的特异条带。经Blast分析比对,确定该菌为FOC。再利用FOC4的特异引物PCL/PDL对基因组上的特征序列扩增区域(SCAR)进行PCR扩增,获得677bp的特有序列,鉴定菌株SF001是尖孢镰刀菌古巴专化型4号生理小种。经过致病性测试,菌株SF001表现出典型4号生理小种的病理特征。     

Occurrence of Fusarium oxysporum f. sp. melonis Race 1 in Japan

In 1994, Fusarium wilt of melon cultivars which are resistant to races 0 and 2 of Fusarium oxysporum f. sp. melonis was observed in southern area of the Lake Biwa region, Shiga prefecture. In commercial fields, mature plants of cv. Amus which were grafted onto cv. Enken Daigi 2, and of cv. FR Amus showed yellowing, wilting and finally death before harvesting of fruits. Diseased plants had vascular and root discolorations, and their stem sections yielded typical colonies of F. oxysporum. When the Shiga strains were tested for their pathogenicity to 12 species of cucurbits, they caused wilts only on melon. Using race differential cultivars of melon, the Shiga strains were classified as race 1 of F. oxysporum f. sp. melonis, which has not been reported in Japan. To further characterize their pathogenicity, the strains were used to inoculate 46 additional cultivars of melon, oriental melon and oriental pickling melon. All the race 1 strains were pathogenic to the cultivars tested, and their host range was apparently different from those of strains belonging to other races (races 0, 2 and 1,2y). DNA fingerprinting with a repetitive DNA sequence, FOLR3, differentiated race 1 strains from strains of races 0 and 2, but not from race 1,2y strains. Received 2 July 1999/ Accepted in revised form 30 September 1999     

香蕉枯萎病菌生理分化研究摘要本研究

本研究对香蕉枯萎病菌菌株FOCAAA9(来自香蕉)和FOCABB1(来自粉蕉)进行培养试验和接种试验;在含粉蕉和香蕉组织浸提液的培养基上2个菌株的培养性状、菌丝生长速度、孢子形态、大小型孢子比率和产孢量显示出差异;接种结果FOCAAA9能侵染香蕉(MusaAAA)品种巴西蕉、红香蕉和台蕉引起枯萎病,而FOCABB1对3个香蕉品种无致病性。研究结果表明侵染香蕉和粉蕉的古巴尖镰孢[Fusariumoxysporumf.sp.cubense(E.F.Smith)Snyder]存在生理分化现象。     

福建省香蕉枯萎病菌硝酸盐营养突变体的营养体亲和性测定

 Fourteen strains of Fusarium oxysporum f. sp. cubense were induced to produce 146 nitrate-nonutilizing(nit) mutants on a chlorate-containing medium. Among them, there were 117 nit1 mutants(80.14%), 17 nit3 mutants(11.64%) and 12 nitM mutants(8.22%). These strains were divided into two vegetative compatibility groups(VCGs) by the vegetative compatibility tests. Twelve strains of F. oxysporum f. sp. cubense from Musa AAA belonged to VCG1, two trains from Musa ABB belonged to VCG2.     

西瓜枯萎菌拮抗细菌的筛选、鉴定及防效测定

从内蒙古、新疆、安徽、河南、江苏、江西6省的西瓜、黄瓜和茄子3种作物根际土壤和病健组织中,共获得样本64份,分离得到细菌1050株。室内抑菌活性测定结果表明：9株细菌分离物对西瓜枯萎病菌Fusariumoxysporumf.sp.niveum、甘蓝黑斑病菌Alternaria brassicicola、辣椒疫霉病菌Phytophthora capsici和番茄灰霉病菌Botrytis cinerea均具有很强的拮抗作用,其中菌株NBT-15和PL-82对西瓜枯萎病菌菌丝生长的抑制作用比较明显,抑制率分别为60.5%和55.3%。盆栽防病试验结果表明：NBT-15和PL-82对西瓜枯萎病的防治效果分别为80.4%和75.6%。形态特征、生理生化特性及16S rDNA序列分析结果确定菌株NBT-15为枯草芽孢杆菌Bacillus subtilis,PL-82为铜绿假单胞菌Pseudomonas aeruginosa。     

Isolation of Pathogenicity Mutants of Fusarium oxysporum f. sp. melonis by Insertional Mutagenesis

Restriction enzyme-mediated integration (REMI) mutagenesis was used to isolate mutants of Fusarium oxysporum f. sp. melonis impaired in pathogenicity. The race 2 strain Mel02010 was transformed with linearized pSH75, conferring resistance to hygromycin B, with or without the enzyme used to linearize the plasmid. Addition of restriction enzymes did not affect the transformation frequency. A total of 2929 REMI transformants were tested for pathogenicity to three melon cultivars, Amus, Ogon 9 and Ohi. The race 2 strains are pathogenic to Amus and Ogon 9, but not to Ohi. Of 43 transformants with reduced pathogenicity on susceptible melon cultivars, 12 mutants were examined in detail for pathogenicity, vegetative growth and integrative mode of pSH75. The levels of pathogenicity varied among these mutants. Two mutants (B48 and B137) almost completely lost pathogenicity to both susceptible cultivars, and the others had reduced pathogenicity. Mutants B48, B241, B886 and X36 were also impaired in vegetative growth. Mutant B809 was a biotin auxotroph. By DNA gel blot analysis, nine mutants were found to contain a single copy of the transformation vector. These mutants may thus be useful in isolating genes involved in pathogenicity. Received 22 December 2000/ Accepted in revised form 16 April 2001