根结线虫生防细菌物种多样性及生防潜力研究

从库存的1471株细菌中筛选出对南方根结线虫二龄幼虫(J2)杀线率≥30%的生防菌99株,进一步从这99株生防菌中筛选出能吸引J2的菌株58株,其中11株的CI>0.2。这58株吸引J2的生防细菌分属于放线菌门(Actinobacteria)、变形菌门(Proteobacteria)厚壁菌门(Firmicutes)和拟杆菌门(Bacteroidetes)4个大类;其中,厚壁菌门种类最多,共30株,芽孢杆菌属(Bacillus)为优势属,共6种16株菌。Pseudomonas corrugate YMF3.02205和P.rhodesiae YMF3.02254对J2的致死活性和吸引活性最高。这2株生防菌能趋化烟草根系分泌物尼古丁,对烟草根结线虫病的防效分别为65.5%和67.3%,当与40μmol·L^(-1)尼古丁配合使用时,防效显著提高到75%和76.9%。研究结果表明趋化性生防菌与趋化底物配合使用能显著提高生防菌防效。

拮抗烟草疫霉菌的趋化性内生细菌筛选及其对烟草黑胫病的防效

以烟草疫霉菌为靶标,从3000株烟草叶片内生细菌中筛选出拮抗菌483株,抑菌率在9.55%~55.96%之间.从这483株拮抗菌中筛选出11株趋化性内生生防细菌,鉴定为Brevibacillus brevis、Br.parabrevis、Br.formosus、Br.reuszeri、Pseudomonas aeruginosa、Ps.tremae、Ps.umsongensis和Erwinia rhapontici.温室试验结果显示,Br.brevis Hs8-19,Br.brevis Hs8-13和Ps.tremae Ht3-25单独使用时,对烟草黑胫病的防效分别为62.43%、57.67%和53.43%.当在菌液中添加终浓度为40μmol/L尼古丁时,Br.brevis Hs8-19,Br.brevis Hs8-13和Ps.tremae Ht3-25对烟草黑胫病的防效分别增加了6.11%、4.79%和4.72%.

云南江城雪茄烟根结线虫病的病原鉴定及生物源氨气熏蒸的防治效果研究

雪茄产业是近年来中国烟草行业新的经济增长点,雪茄烟种植中根结线虫病危害严重.然而,目前国内外雪茄烟病原线虫的种类尚未明确,对该病害的绿色防控也鲜有报道.基于雌虫、雄虫和二龄幼虫的形态特征、PCR扩增特异性条带及科赫法则验证结果,将普洱市江城县雪茄烟叶“云雪1号”品种上发生的根结线虫病病原鉴定为爪哇根结线虫(Meloidogyne javanica).评估了4种食用菌(金针菇、杏鲍菇、香菇、姬菇)菌渣脲酶催化尿素释放氨气熏蒸土壤对雪茄烟叶爪哇根结线虫病的防治效果.结果表明:致死100%二龄幼虫(J2)所需的NH3最低质量浓度为136.8 mg/m^(3);将含4%尿素的4种菌渣分别与土壤按质量比为1∶18的比例混合,在水分含量约60%、28℃下放置3 d时,各处理组释放的氨气质量浓度在130.9~218.7 mg/m^(3),对根结线虫病的防效在75.7%~92.3%.研究结果显示“菌渣+尿素”熏蒸土壤对防控雪茄烟根结线虫病具有很好的应用潜力.

钩状木霉(Trichoderma hamatum YMF1.00247)促进烟草生长及其诱导抗性研究

γ-氨基丁酸(GABA)能有效促进作物生长,在农业种植中有重要应用价值.研究报道一株GABA产生菌(钩状木霉YMF1.00247),通过盆栽试验分析其发酵液促进烟草生长的效果和对烟草黑胫病的防效,并从植物防御酶的变化分析其抗病机制.YMF1.00247菌株发酵液中GABA质量浓度可达1.33 g·L^−1,但该菌株不产吲哚乙酸(IAA)、铁载体和ACC脱氨酶.用YMF1.00247发酵液灌根能显著增加烟草的株高、叶片数、茎围和中部叶面积;施用100 mL/株的YMF1.00247发酵液和1.5 g·L^−1 GABA能显著减少烟草黑胫病的发病率和病情指数,防效分别达78.41%和72.36%,且能显著提高烟株的苯丙氨酸解氨酶(PAL)、过氧化物酶(POD)、多酚氧化酶(PPO)酶活.YMF1.00247菌株产生的GABA可能是其具有促进烟株生长和诱导抗病功能的主要活性成分.

Phosphate Solubilizing Ability and Phylogenetic Diversity of Bacteria from P-Rich Soils Around Dianchi Lake Drainage Area of China

The phylogenetic diversity of phosphate solubilizing bacteria (PSB) distributed in P-rich soils in the Dianchi Lake drainage area of China was characterized, and the tricalcium phosphate (TCP) solubilizing activities of isolated PSB were determined. Among 1328 bacteria isolated from 100 P-rich soil samples, 377 isolates (28.39% of the total) that exhibited TCP solubilization activity were taken as PSB. These PSB showed different abilities to solubilize TCP, with the concentrations of solubilized P in bacterial cultures varying from 33.48 to 69.63 mg L-1. A total of 123 PSB isolates, with relatively high TCP solubilization activity (> 54.00 mg L-1), were submitted for restriction fragment length polymorphism (RFLP) analysis, which revealed 32 unique RFLP patterns. Based on these patterns, 62 representative isolates, one to three from each RFLP pattern, were selected for 16S rRNA sequencing. Phylogenetic analysis placed the 123 PSB into three bacterial phyla, namely Proteobacteria, Actinobacteria and Firmicutes. Members of Proteobacteria were the dominant PSB, where 107 isolates represented by 26 RFLP patterns were associated with the genera of Burkholderia, Pseudomonas, Acinetobacter, Enterobacter, Pantoea, Serratia, Klebsiella, Leclercia, Raoultella and Cedecea. Firmicutes were the subdominant group, in which 13 isolates were affliated with the genera of Bacillus and Brevibacterium. The remaining 3 isolates were identified as three species of the genus Arthrobacter. This research extends the knowledge on PSB in P-rich soils and broadens the spectrum of PSB for the development of environmentally friendly biophosphate fertilizers.

Vero细胞生物反应器微载体无血清培养甲型流感病毒

目的采用Vero细胞生物反应器微载体无血清培养甲型流感病毒。方法将Vero细胞分别采用无血清和有血清培养基于生物反应器(pH 7.2,温度37℃,溶氧量50%,转数60 r/min)中培养24 h,均用无血清培养基进行灌流培养至7 d,进行计数,并按MOI=0.1接种H1N1型流感病毒,加入终浓度为1μg/mL的TPCK-胰酶,于生物反应器(pH 7.8,温度33.0℃,溶氧量25%,转数60 r/min)中培养18、22、42、48、66 h,取样,检测血凝效价。结果Vero细胞经无血清和有血清培养基培养7 d的细胞数分别为(133.4±2.0)×104和(193.8±1.3)×104个/mL,接种H1N1流感病毒66 h后血凝效价几何平均数分别为1∶388和1∶675,前者细胞数及病毒血凝效价几何平均数均显著低于后者(t分别为7.068和4.332,P均<0.05)。结论采用Vero细胞通过生物反应器微载体无血清培养H1N1型流感病毒的血凝效价可满足流感病毒裂解疫苗制备的要求。