牡丹根部内生细菌的分离鉴定及脂肽类物质的拮抗活性研究

【目的】从牡丹(Paeonia suffruticosa Andr.)根部组织中分离鉴定内生细菌,测定拮抗菌株脂肽类活性物质的体外抑菌活性。【方法】采用平板对峙法筛选出对牡丹灰霉病菌(Botrytis paeoniae Oadem)、牡丹炭疽病菌(Gloeosporium sp.)、牡丹黑斑病菌(Altenaria sp.)、牡丹黄斑病菌(Phyllosticta commonsii)有拮抗作用的内生细菌。基于形态特征、生理生化特性和16S rRNA基因序列同源性鉴定拮抗菌株。根据脂肽类抗菌物质合成相关基因序列对拮抗菌株进行基因扩增检测,采用酸沉淀法提取拮抗菌株的脂肽类物质,平板对峙法测定脂肽类物质的体外抑菌活性。【结果】从牡丹根部组织中共分离获得62株内生细菌,其中菌株Md31和Md33对4种病原菌均有较明显的抑制作用。Md31和Md33被鉴定为解淀粉芽孢杆菌(Bacillus amyloliquefaciens)。通过对菌株Md31和Md33进行5个脂肽类合成功能基因bmyB、fenD、ituC、srfAA和srfAB的检测,序列同源性分析,表明两个菌株具有合成脂肽类物质的能力。菌株Md31和Md33的脂肽类粗提物对所测试的牡丹病原真菌均具有不同程度的抑制作用。【结论】获得了2株对牡丹病原菌有良好抑制效果的解淀粉芽孢杆菌Md31和Md33,两个菌株的脂肽类粗提物也具有较强的体外抑菌活性,该研究为牡丹内生细菌的进一步开发应用奠定了基础。     

一株紫罗兰蓝色素产生菌的分离、鉴定及其活性产物的特性分析

[目的]调查秦巴山地区微生物物种的多样性,建立用于活性产物筛选的微生物代谢产物库和菌种资源库,通过数据库平台进行资源共享.[方法]采用不同的分离方法,分离存在于不同生境的微生物类群,通过形态、生理生化及分子生物手段鉴定菌种,发酵并通过甲醇提取代谢产物.[结果]从本地区土壤样本中分离获得一株产水溶性紫罗兰蓝色素的放线菌Str-4331,在高氏培养基上其气生菌丝为白色,产生水溶性紫罗兰色素,镜检观察孢子丝螺旋形,孢子椭圆形至长圆形,通过形态、生理生化特征初步确定为链霉菌.利用ClustalX对其16S rRNA进行序列比对,用Neighbor-Joining (NJ)构建系统发育树,并用Bootstraping法对其评价.实验结果表明,该菌基因序列与砖红链霉菌(Streptomyces lateritius) LMG 19372基因序列有99％的最高相似性.抑菌试验表明,活性产物具有较强的抗革兰氏阳性细菌活性.色素在水溶液中颜色随着pH的变化而变化.质谱分析显示3个主要化合物,分子量分别为557.68、588.43、485.18 kD,其中分子量为557.68 kD化合物与榴菌素B分子量一致.[结论]根据菌株的16S rRNA序列分析结果,结合菌株的培养特性和生理生化特性,将菌株Str-4331归属为砖红链霉菌(S.lateritius).该菌种首次在本地区分离到,具有进一步研究开发的价值.     

利用合成生物学技术深入挖掘放线菌中活性次级代谢产物

放线菌是一类能够产生丰富生物小分子药物的微生物, 对人类的健康事业做出了杰出的贡献。但近几十年来, 来源于微生物并最终上市的药物越来越少, 而病原菌的抗药性问题却越发严重, 人们对新药的期待越来越迫切。本文介绍了近十年里发展迅速的合成生物学对微生物次级代谢产物研发的促进作用。合成生物学以工程化的思想对生命系统进行设计与改造, 使传统方法难以获取的放线菌次级代谢产物通过外源宿主得以产生, 充分利用了自然界的资源; 此外, 对次级代谢基因簇的合理设计和对生物元件的应用不仅使人们获得了自然界中原本不存在的新化合物, 还能使某些具有广泛应用价值药物的产量得以显著提高; 最后, 本文还介绍了合成生物学领域近些年DNA组装的新技术和新方法, 为从事次级代谢产物研发的工作者提供便利。     

Immunological cost of chemical defence and the evolution of herbivore diet breadth

Selective pressures from host plant chemistry and natural enemies may contribute independently to driving insect herbivores towards narrow diet breadths. We used the specialist caterpillar, Junonia coenia (Nymphalidae), which sequesters defensive compounds, iridoid glycosides, from its host plants to assess the effects of plant chemistry and sequestration on the larval immune response. A series of experiments using implanted glass beads to challenge immune function showed that larvae feeding on diets with high concentrations of iridoid glycosides are more likely to have their immune response compromised than those feeding on diets low in these compounds. These results indicate that larvae feeding on plants with high concentrations of toxins might be more poorly defended against parasitoids, while at the same time being better defended against predators, suggesting that predators and parasitoids can exert different selective pressures on the evolution of herbivore diet breadth.     

6种植物次生物质对斜纹夜蛾解毒酶活性的影响

草食性昆虫取食植物时遇到宿主植物中大量次生物质的化学防御,研究昆虫适应植物毒素的反防御策略具有重要的科学意义。分别添加0.01%肉桂酸、0.01%水杨酸、0.01%花椒毒素、0.02%槲皮素、0.05%黄酮和0.1%香豆素等6种植物次生物质的人工饲料饲养斜纹夜蛾(Spodoptera litura)五龄幼虫48 h后,测定斜纹夜蛾幼虫中肠和脂肪体中谷胱甘肽S-转移酶(GSTs)、羧酸酯酶(CarE)、P450的酶含量及头部乙酰胆碱酯酶(AChE)的活性,利用半定量RT-PCR检测中肠和脂肪体中CYP4M14和CYP4S9的基因表达水平。结果表明:取食肉桂酸和香豆素后,斜纹夜蛾中肠中CarE的酶活性分别提高了1.67和1.37倍,取食6种次生物质均能显著提高斜纹夜蛾脂肪体中GSTs酶活性。取食肉桂酸和香豆素48 h后,脂肪体中P450酶含量比对照增加2.93和14.50倍。取食肉桂酸、花椒毒素、槲皮素和香豆素后,斜纹夜蛾头部AchE酶活性与对照相比提高了1.53、1.80、2.36和1.56倍。6种次生物质均可诱导脂肪体中CYP4M14基因表达,槲皮素、肉桂酸和香豆素强烈诱导CYP4S9在脂肪体中表达。表明,斜纹夜蛾具有利用植物次生物质诱导其解毒酶的能力,进而提高其对毒素的抗性。     

Isolation and synthesis of trans- and cis-(−)-clovamides and their deoxy analogues from the bark of Dalbergia melanoxylon

N-(3′,4′-Dihydroxy-trans-cinnamoyl)-3-(3,4-dihydroxyphenyl)-L-alanine [(?)-clovamide], the major phenolic metabolite (0.1%) in the bark of Dalbergia melanoxylon, is associated with minor proportions of its cis-isomer, and similar pairs of geometrical isomers of their deoxy analogues N-(4′-hydroxycinnamoyl)-3-(3,4-dihydroxyphenyl)-L-alanine and N-(4′-hydroxycinnamoyl)-3-(4-hydroxyphenyl)-L-alanine. (?)-Trans-clovamide is synthesized by direct condensation of the acid chloride of caffeic acid with L-DOPA. Diagnostic CD spectra of these compounds and ¹³C spectra of (?)-trans- and (?)-cis-clovamides are recorded.     

Molecular dynamics simulation studies for DNA sequence recognition by reactive metabolites of anticancer compounds

The discovery of novel anticancer molecules 5F‐203 (NSC703786) and 5‐aminoflavone (5‐AMF, NSC686288) has addressed the issues of toxicity and reduced efficacy by targeting over expressed Cytochrome P450 1A1 (CYP1A1) in cancer cells. CYP1A1 metabolizes these compounds into their reactive metabolites, which are proven to mediate their anticancer effect through DNA adduct formation. However, the drug metabolite–DNA binding has not been explored so far. Hence, understanding the binding characteristics and molecular recognition for drug metabolites with DNA is of practical and fundamental interest. The present study is aimed to model binding preference shown by reactive metabolites of 5F‐203 and 5‐AMF with DNA in forming DNA adducts. To perform this, three different DNA crystal structures covering sequence diversity were selected, and 12 DNA‐reactive metabolite complexes were generated. Molecular dynamics simulations for all complexes were performed using AMBER 11 software after development of protocol for DNA‐reactive metabolite system. Furthermore, the MM‐PBSA/GBSA energy calculation, per‐nucleotide energy decomposition, and Molecular Electrostatic Surface Potential analysis were performed. The results obtained from present study clearly indicate that minor groove in DNA is preferable for binding of reactive metabolites of anticancer compounds. The binding preferences shown by reactive metabolites were also governed by specific nucleotide sequence and distribution of electrostatic charges in major and minor groove of DNA structure. Overall, our study provides useful insights into the initial step of mechanism of reactive metabolite binding to the DNA and the guidelines for designing of sequence specific DNA interacting anticancer agents. Copyright © 2014 John Wiley & Sons, Ltd.     

艾纳香内生真菌Diaporthe sp.次生代谢产物

【目的】从艾纳香内生菌J1中获得活性次生代谢产物。【方法】对菌株J1进行ITS序列分子鉴定,综合运用多种色谱技术对其发酵产物进行分离纯化,结合波谱学技术对其进行结构表征。【结果】经构建系统进化树,鉴定菌株J1为Diaporthe sp.,从该菌株大米培养基中分离得到7个单体化合物,经鉴定分别为Dicerandrol A (1)、Dicerandrol B (2)、4,6-dihydroxy-1H-isoindole1,3(2H)-dione (3)、Cytochalasin H (4)、Cytochalasin J (5)、4,6-dihydroxy-2,3-dihydro-1H-isoindol-1-one (6)、Cerebroside C (7)。所有化合物均为首次从该菌中分得,化合物1对枯草芽孢杆菌Bacillus subtilis KCTC 1021具有非常强的抑制活性,MIC值为0.125μg/mL。【结论】Diaporthe sp.富含抑菌活性化合物,具有开发成微生物源农药潜力。