耐低水活度高毒力虫生真菌菌株选育

以球孢白僵菌Beauveria bassiana和玫烟色拟青霉Paecilomyces fumosoroseus为研究对象,利用紫外线诱变芽生孢子和低水活度条件胁迫筛选,选育出突变株Bb07240、Pf01120和Pf01160,它们在低水活度（或相对湿度）下的生长和萌发均明显优于其相应的初始菌株。生物测定表明,突变株对桃蚜的毒力明显高于其初始菌株。     

光合细菌Rhodobacter sphaeroides glnB—lacZ融合子的构建

亚克隆了Ｒｈｏｄｏｂａｃｔｅｒ ｓｐｈａｅｒｏｉｄｅｓｇｌｎＢ启动子,以ｐＭＰ２２０为载体构建成ｂｌｎＢ－ｌａｃＺ融合子。将ｇｌｎＢ－ｌａｃＺ、ｎｉｆＨ－ｌａｃＺ、ｎｉｆＡ＝ｌａｃＺ分别导入Ｒ．ｓｐｈａｅｒｏｉｄｅｓ谷氨酸合酶突变株ｇｌｔＢ、ｇｌｔＤ和野生型菌株中,分析了突变对固氮基因转录表达的影响,试验证明,在ｇｌｔＢＤ突变株中ｎｉｆＨ的表达受阻遏,ｎｉｆＡ表达水平很低。这证明ｇｌｔ基因的突变引     

紫云黄根瘤菌质粒功能研究

紫云英根瘤菌ＣＨ２０３含有３条质粒,用带蔗糖敏感基因Ｔｎ５－ｓａｃＢ进行菌株质粒消除和质粒缺失突变株筛选,获得一系列突变株。与野生型菌相比。质粒ｐＲＨａ的丢失导致菌株结无效根瘤,质粒ｐＲＨｂ的丢失使菌株失去共生能力。在ＴＹ培养基平板上菌落变得粗糙,失去了脂多糖。质粒ｐＲＨｃ的丢失显然失去其菌株的共生能力,同时使菌株抗酸性明显减弱。     

光合细菌Rhodobacter sphaeroides glnBlacZ 融合子的构建与表达

亚克隆了Ｒｈｏｄｏｂａｃｔｅｒ ｓｐｈａｅｒｏｉｄｅｓ ｇｌｎＢ启动子,以ｐＭＰ２２０ 为载体构建成ｇｌｎＢｌａｃＺ融合子。将ｇｌｎＢｌａｃＺ、ｎｉｆＨｌａｃＺ、ｎｉｆＡｌａｃＺ分别导入Ｒ． ｓｐｈａｅｒｏｉｄｅｓ 谷氨酸合酶突变株ｇｌｔＢ－ 、ｇｌｔＤ－ 和野生型菌株中,分析了突变对固氮基因转录表达的影响。试验证明,在ｇｌｔＢＤ 突变株中ｎｉｆＨ 的表达受阻遏,ｎｉｆＡ 表达水平很低。这证明ｇｌｔ 基因的突变引起固氮酶结构基因和固氮正调节基因的转录被阻遏,而ｇｌｎＢ 基因的表达几乎不受影响。试验还测定了环境中结合态氮和有机酸等信号分子对ｇｌｎＢ 和ｎｉｆＨ 表达的影响,发现加入氨或谷氨酰胺后,ｎｉｆＨ 的表达受到明显的阻遏作用,ｇｌｎＢｌａｃＺ的β半乳糖苷酶活性虽下降３０ ％ 左右但不随结合态氮浓度升高而变化,仍维持在一个较高的水平。α酮戊二酸和丙酮酸对ｎｉｆＨ 的表达有部分去阻遏作用而对ｇｌｎＢ的表达无诱导作用     

一种具有纤溶活性的枯草杆菌蛋白激酶的研究──Ⅰ高产酶菌株的筛选与鉴定

本文主要阐述了一种具有纤溶活性的枯草杆菌（Ｂａｃｉｌｌｕｓｓｕｂｔｉｌｉｓ）蛋白激酶产生菌株的筛选与鉴定的研究结果。作者从初筛的１２株Ｂａｃｉｌｌｕｓｓｕｂｌｉｌｉｓ菌中,通过对固体发酵和液体发酵所产生的枯草杆菌蛋白激酶,用琼脂糖－纤维蛋白平板法测其活性,经比较不同菌株的活性,筛选出两株高产酶菌株：Ｂ．ｓｕｂｔｉｌｉｓＨＷ—１２和Ｂ．ｓｕｂｔｉｌｉｓＨＷ—３。同时对菌体和菌落形态特点、生理生化反应进行了鉴定,认为Ｂ．ＳｕｂｔｉｌｉｓＨＷ－１２菌株可用来做为发酵生产该酶的菌种。     

苏云金芽孢杆菌的电穿孔及其工程菌的构建

本文对苏芸金芽孢杆菌 (Ｂａｃｉｌｌｕｓｔｈｕｒｉｎｇｉｅｎｓｉｓ,Ｂｔ)和蜡状芽孢杆菌 (Ｂａｃｉｌｌｕｓｃｅｒｅｕｓ,Ｂｃ)等部分菌株的电穿孔转化进行了研究 ,主要从电穿孔的供体质粒和受体菌株等方面讨论了各种因素对该方法的影响。同时利用电穿孔方法对部分Ｂｔ的高效野生株进行遗传改良 ,希望获得含有ｃｒｙ1Ａｃ和ｃｒｙ1Ｃ高效基因组合的对鳞翅目棉铃虫、甜菜夜蛾都有效的广谱工程株。利用质粒 ｐＳＢ1 40 2 (ｃｒｙ1Ｃ) ,ｐＡＭＹ(ｃｒｙ1Ａｃ) ,ｐＮＱ1 2 2 (Ｃｍｒ)对所有的供试菌株进行电穿孔转化 ,不同菌株表现出不同的转…     

金属硫蛋白产生菌的诱变育种

采用亚硝基胍和紫外线诱变,自金属硫蛋白（ＭＴ）产生菌酿酒酵母（ｄｅｃｃｈａｒｏｍｙｃｅｓｃｅｒｅｖｉｓｉａｅ）ＢＤ１０１－２５单倍体中获得遗传稳定的高Ｃｕ２＋、Ｃｄ２＋抗性突变株ＢＤ１０１－６９和ＢＤ１０１－３０。并对其重金属解毒、桔抗ｕ．ｖ．和６０Ｃｏ辐射效应、清除羟基自由基能力等生物学功能进行了研究。与出发菌株相比,上述生物学活性与酵母细胞对Ｃｉ２＋抗性、ＭＴ表达量表现出正相关性。两个突变株类ＭＴ表达量与生物学活性皆有所提高,为酿酒酵母ＭＴ的理论和应用研究打下了基础。     

我国仓贮昆虫病原芽孢杆菌的研究

对９５１个样品分离鉴定,有７４７个样品含芽孢杆菌,有菌率为７８．５５％．共分离得到芽孢杆菌１１３８株,其中苏云金杆菌（Ｂａｃｉｌｌｕｓｔｈｕｒｉｎｇｉｅｎｓｉｓ,简称Ｂ．ｔ）１４３株,占１２．５％;球形芽孢杆菌（Ｂａｃｉｌｌｕｓｓｐｈａｅｒｉｃｕｓ,简称Ｂ．ｓ）１１株,占０．９７％;其他芽孢杆菌９８４株,占８６．４０％．从芽孢杆菌中选出产生晶体、苏云金素或磷酸酯酶Ｃ（ＰｈｏｓｐｈａｌｉｐａｓｅＣ,简称ＰＬＣ）的毒素菌株１６８株,其中Ｂ．ｔ占１４３株,Ｂ．ｓ有５株,其他芽孢杆菌１０株．在产毒素菌株中,经测定有１２０株菌对供试昆虫毒性达标．占７７．９２％．不同菌株的杀虫毒素、杀虫范围和毒力各异,认为这种差异取决于毒素和虫种两方面的特异性．     

金属硫蛋白产生菌的诱变育种*

采用亚硝基胍和紫外线诱变,自金属硫蛋白（ＭＴ）产生菌酿酒酵母（ｄｅｃｃｈａｒｏｍｙｃｅｓｃｅｒｅｖｉｓｉａｅ）ＢＤ１０１－２５单倍体中获得遗传稳定的高Ｃｕ^２＋、Ｃｄ^２＋抗性突变株ＢＤ１０１－６９和ＢＤ１０１－３０。并对其重金属解毒、桔抗ｕ．Ｖ．和６０Ｃｏ辐射效应、清除羟基自由基能力等生物学功能进行了研究。与出发菌株相比,上述生物学活性与酵母细胞对Ｃｉ^２＋抗性、ＭＴ表达量表现出正相关性。两个突变株类ＭＴ表达量与生物学活性皆有所提     

蛹虫草（Cordceps militaris）无性型的多型现象

在萨氏琼脂和ＰＤＡ上,蛹虫草Ｃｏｒｄｙｃｅｐｓ ｍｉｌｉｔｅｒｉｓ（Ｖｕｉｌｌ）．Ｆｒ无性型,蛹草拟青霉Ｐａｅｃｉｌｏｍｙｃｅｓ ｍｉｌｉｔａｒｉｓ（Ｋｏｂ）．Ｂｒ＆Ｓｍ．的一些单孢子株可自发产生突变,基于多型现象及其它形态特征可分为三种类型：（１）具野生型菌株特征,产孢结构拟青霉型（Ｐａｅｃｉｌｏｍｙｃｅｓ－ｔｙｐｅ）,稳定,菌落通常不自发产生角变,大多数单孢了株属此类群。（２）属此类群的单孢子     

两种杀虫真菌制剂对茶小绿叶蝉的田间防效评价

于2002年盛夏在浙江遂昌一高山茶园对茶小绿叶蝉(Empoasca spp．)进行了真菌杀虫剂的田间药效试验。所用菌剂为球孢白僵菌(Beauveria bassiana)和玫烟色拟青霉(Paecilomyces fumosoroseus)的纯孢子悬乳剂及其与3％吡虫啉10％可湿剂的混配剂．各菌剂稀释500倍喷雾2次,间隔12d．结果表明。两种真菌的混配剂明显优于纯菌剂,其中球孢白僵菌混配剂的最高防效达83．4％,而玫烟色拟青霉的最高防效为71．3％．根据25d期间历次调查结果计算平均防效,球孢白僵菌混配剂达66．8％,玫烟色拟青霉混配剂为62．1％,含微量吡虫啉的矿物油为50．3％,球孢白僵菌和玫烟色拟青霉的纯菌剂分别为49．5％和19．0％,结合试验期间气候及田间种群结构特征,讨论了各处理问差异的来源及提高真菌杀虫剂控制茶小绿叶蝉效果的可能途径。     

ARTP诱变猴头菌株的发酵菌丝体多糖理化性质及体外免疫活性

为探讨常压室温等离子体诱变的3株高产多糖猴头菌和出发菌株的多糖组分差异,通过液体发酵获得的菌丝体经水提、分级醇沉获得8个胞内多糖组分,对它们的理化性质、结构特征及体外免疫活性进行了研究。结果表明,3株ARTP诱变菌株414、321、236菌丝体多糖含量较出发菌株有较明显提升;ARTP诱变的猴头菌20%醇沉多糖组分较出发菌株分子量大,所占比例增加;诱变菌株60%醇沉多糖组分的分子量略大于出发菌株,所占比例相近。20%醇沉多糖主要由半乳糖、葡萄糖、甘露糖构成,诱变菌株该多糖组分中葡萄糖和甘露糖的比例较出发菌株均有明显提升,60%醇沉多糖组分单糖组成无明显差异;8个多糖组分均具有体外刺激巨噬细胞释放NO的活性,其中20%醇沉多糖的活性优于60%醇沉多糖,诱变菌株的生物活性优于出发菌株。本研究探讨了ARTP诱变对猴头菌胞内多糖结构及活性的影响,为猴头菌相关产品的开发提供了优质资源。     

杀虫遗传工程荧光假单胞菌IPP202部分生物学特性

对遗传工程荧光假单胞菌IPP202进行了质粒稳定性检 测、抑菌活性测定、在棉花根部和叶面定殖能力分析、杀虫蛋白抗紫外能力检测及田间杀虫 活性测定等试验。结果表明,工程菌与出发菌株P303相比,其抑菌、定殖等有益于植物的优 良特性未发生显著变化;经过连续培养和连续稀释培养后工程菌的质粒都非常稳定;广波长 紫外线照射2 h后,苏云金芽胞杆菌(Bacillus thuringiensis,简称Bt)由于裸露的伴 孢晶体杀虫蛋白受紫外线破坏因而杀虫活性大大下降,而荧光假单胞菌工程菌的活性变化不 大;IPP202田间杀虫活性与Bt野生菌株接近。工程菌有望解决Bt本身存在的杀虫蛋白多以裸 露晶体的形式存在而易受紫外线破坏的弱点,同时也发挥了P303菌株在多种植物上定殖能力 的优点,使其具有在植物周围大量繁殖而直到杀虫作用的优势。通过进一步研究,将有望构 建成更有实用价值的工程菌。     

Pseudomonas fluorescens enhances resistance and natural enemy population in rice plants against leaffolder pest

Plant growth promoting fluorescent pseudomonad strains Pf1, TDK1 and PY15 were evaluated for their efficacy against leaffolder ( Cnaphalocrocis medinalis ) pest in rice plants under field conditions individually and in combinations. Application of mixtures of Pseudomonas fluorescens strains Pf1, TDK1 and PY15 significantly reduced the leaffolder damage in rice plants compared with untreated control. Interestingly, natural enemy population in plots treated with P. fluorescens was greater than the chemical and untreated controls. Further, support for these results was gathered by assaying activities of polyphenol oxidase (PPO) and lipoxygenase (LOX) under glasshouse conditions. The results showed the higher activity of PPO and LOX in plants treated with P. fluorescens mixtures (Pf1 + TDK1 + PY15) than the plants treated with individual strains, chemical and untreated controls. Further, fluorescent pseudomonad mixtures increased the rice yield compared with individual strain and non-bacterized treatments. The present study reveals that in addition to plant growth promotion, plant growth-promoting rhizobacterial (PGPR) strains-mediated induction of PPO and LOX in rice plants could be involved in enhanced natural enemy populations and resistance mechanisms against leaffolder attack.     

Tn5 Insertion Mutants of Pseudomonas fluorescens Defective in Adhesion to Soil and Seeds

Tn5 insertion mutants of a soil isolate, Pseudomonas fluorescens Pf0-1, were selected for decreased ability to adhere to quartz sand in a column assay. Three adhesion-deficient mutants that differed in the location of the Tn5 insertion in the chromosome were isolated and compared with the wild-type strain. One mutant, Pf0-5, was described previously as an adhesion-defective, nonmobile, flagellumless mutant (M. F. DeFlaun, A. S. Tanzer, A. L. McAteer, B. Marshall, and S. B. Levy, Appl. Environ. Microbiol. 56:112-119, 1990). Another insertion mutant, Pf0-10, was also missing flagella and the 34-kDa outer membrane protein that was absent in Pf0-5 but present in the wild-type strain. The third mutant (Pf0-15) had increased amounts of this 34-kDa outer membrane protein and more flagella than the wild-type strain. These mutants also displayed decreased ability to adhere to sterile and natural (live) soil and to a variety of plant seeds. In kinetics studies, the wild-type strain showed an initial rapid binding to seeds followed by a later slow phase of binding. The mutant strains were defective in the initial stages of attachment but did show the later slow binding. The findings indicate that the same mutations that affect binding to sand and soil also affect adhesion to plant seeds.     

Molecular studies of co-formulated strains of the entomopathogenic fungus,Beauveria bassiana

A 28S rDNA intron was used as a molecular marker to distinguish between two single spore strains of Beauveria bassiana, Bb123 and Bb151. When co-formulated and assayed against larvae of Galleria mellonella these strains exhibited no synergistic increase in virulence, rather Bb123 usually dominated. This study shows that the success of any strain to infect Galleria is dependent on the dose and method of inoculation (injection versus immersion). The result of co-formulated strains grown on solid culture also showed that usually one strain dominated, i.e., strain displacement could happen both in vivo and in vitro. The speed by which one strain was displaced following successive sub-culturing on PDA partly depended on the ratio of Bb151 and Bb123. The co-formulated inoculum could widen the window over which parent strains would be active on different water activity media. Co-infection did result in heterokaryosis within the Galleria host. Molecular studies also showed that the heterokaryon was not stable and could revert back to the parent strain.     

Molecular and functional study of AQY1 from Saccharomyces cerevisiae: role of the C-terminal domain

The yeast YPR192w gene, which encodes a protein (Aqy1p) with strong homology to aquaporins (AQPs), was cloned from nine S. cerevisiae strains. The osmotic water permeability coefficient (Pf) of X. laevis oocytes expressing the gene cloned from the Sigma1278b strain (AQY1-1) was 5.7 times higher than the Pf of oocytes expressing the gene cloned from other strains (AQY1-2). Aqy1-1p, initially cloned without its C-terminus (Aqy1-1DeltaCp), mediated an approximately 3 times higher water permeability than the full-length protein. This corresponds to a 3-fold higher protein density in the oocyte plasma membrane, as shown by freeze-fracture electron microscopy. Pf measurements in yeast spheroplasts confirmed the presence of functional water channels in Sigma1278b and a pharmacological study indicated that this strain contains at least a second functional aquaporin.     

Mutants of Escherichia coli with altered level of beta-N-acetylglucosaminidase activities.

Five strains of Escherichia coli with reduced level of beta-N-acetylglucosaminidase activity were isolated. The mutations responsible for reduced activity of the enzyme have been localized in one of the strains between 25 and 27 minutes on the genetic map of E. coli. The mutants do not differ morphologically from the original strain. This suggest that beta-N-acetylglucosaminidase is of the secondary importance in the biosynthesis of murein.     

双价杀虫蛋白基因在荧光假单胞菌中的表达及增效

利用广宿主质粒载体pJMS6αlac将苏云金芽胞杆菌(Bacillus thuringiensis)杀虫晶体蛋白基因cry1Ac和cry2Aa基因分别及一起进行克隆,将重组质粒导入能在多种作物上定殖、对植物病菌有良好抑菌和防治作用的荧光假单胞菌(Pseudomonas fluorescens)P303菌株,分别得到工程菌株IPP101、IPP201和IPP202。PCRRFLP和Southern blot检测均证明目的基因已经导入了工程菌。SDSPAGE电泳显示工程菌中存在明显的Cry1Ac蛋白带;透射电镜观察发现含cry1Ac基因的两个菌株IPP101和IPP202中杀虫蛋白形成了典型的菱形晶体和蛋白包含体,而在野生P303菌株中均无这些结构。这些结果说明,工程菌中cry1Ac基因得到了很好表达。室内杀虫试验表明：工程菌对棉铃虫初孵幼虫的致死中浓度(LC50),只含cry1Ac的IPP101为000812mL/g饲料,只含cry2Aa的IPP201为002604mL/g饲料,含双基因的IPP202为000186mL/g饲料;HD73为000170mL/g饲料。cry1Ac和cry2Aa双基因表达产物具有显著增效作用,共毒系数达3328。     

红火蚁活性真菌菌株的室内筛选研究

在实验室条件下采用浸渍法测定了15株白僵菌Beauveria spp.,15株绿僵菌Metarhizium spp.和4株淡紫紫孢菌Purpureocillium lilacinum (Thom)对红火蚁Solenopsis invicta Buren工蚁的活性,并测定分析了高活性菌株对红火蚁工蚁的毒力。结果表明,以1.0×10^8孢子mL的浓度处理红火蚁工蚁后第10天,白僵菌HHY-B、LCM1、ZYSYE-Y2、Bb034、ZG5、Bb720、Bb040、CP728和淡紫紫孢菌LYC1菌株的活性较强,红火蚁工蚁的校正死亡率为84.70%~98.79%,僵虫率为70.61%~90.38%。红火蚁工蚁在接种不同浓度的高活性菌株后,随着孢子浓度的升高,红火蚁的累积校正死亡率和僵虫率增大,致死中时(LT50)缩短,第10天白僵菌ZYSYE-Y2、CP728、HHY-B、LCM1、ZG5、Bb040、Bb720、Bb034和淡紫紫孢菌LCM1菌株对红火蚁工蚁的LC50分别为1.16×10^5、1.49×10^5、2.27×10^5、2.28×10^5、2.32×10^5、3.79×10^5、4.94×10^5、8.47×10^5和3.90×10^6孢子/mL。当孢子浓度为1.0×10^7孢子/mL时,白僵菌HHY-B、CP728、ZG5和Bb040菌株处理的最终校正死亡率分别为91.54%、94.60%、91.23%和94.65%,僵虫率为82.51%、91.74%、85.43%和80.60%,致死中时(LT50)为4.22 d、4.07 d、3.72 d和3.68 d。综合分析表明,白僵菌HHY-B、CP728、ZG5和Bb040菌株对红火蚁工蚁具有较强的活性,可作为红火蚁生物防治的候选菌株