具有细菌群体感应抑制活性海洋来源真菌的筛选鉴定

许多致病菌的致病机制依赖于群体感应系统的调控,经实验证明群体感应系统突变或缺失的菌株致病能力显著下降,筛选高效的群体感应抑制剂有望成为解决细菌感染以及细菌耐药性问题的一个有效途径。从海洋软体动物体内分离海洋真菌69株,发酵液粗提物经QSIS2 (Quorum Sensing Inhibitor Selector 2) 筛选模型和紫色杆菌CV026指示菌株筛选后得到编号QY013的粗提物具有群体感应抑制活性,进一步实验表明该粗提物能够显著降低铜绿假单胞菌群体感应调控的毒力因子绿脓菌素的产量,以及紫色杆菌群体感应调控的紫色菌素的产量,且在有效浓度范围内对细菌生长不产生影响。形态学特征和18S rDNA序列分析表明菌株QY013为Penicillium属。文中筛选到一株具有细菌群体感应抑制活性的海洋来源真菌,其发酵液粗提物中的有效活性成分可用于新型抗菌药物的研究。     

一株海洋真菌Penicillium sp.QF046的细菌群体感应抑制剂的分离和鉴定

目的:从海洋真菌中筛选得到新型群体感应抑制剂,并对其进行活性评价。方法:首先利用紫色杆菌CV026指示菌株对真菌发酵粗提物进行活性筛选。其次通过18S r DNA序列比对进行菌种鉴定,同时采用硅胶柱色谱、凝胶柱色谱和高效液相色谱等技术并结合活性追踪检测分离纯化的活性化合物,再通过核磁质谱分析确定其结构。最后利用定量测定方法检测其在亚抑菌浓度下对紫色杆菌紫色菌素产量影响以及RT-PCR检测与QS调控相关基因的m RNA表达的影响。结果:从海藻共生菌中筛选到一株具有紫色杆菌群体感应抑制活性的海洋真菌Penicillium sp.QF046,其次级代谢产物中纯化到的活性化合物根据结构鉴定为一种星形曲霉毒素(asteltoxin)。该化合物对于紫色杆菌群体感应抑制浓度低于阳性对照化合物呋喃酮C30,同时抑制了群体感应相关基因m RNA水平的表达。结论:从海洋真菌Penicillium sp.QF046代谢产物中发现了一种抑制紫色杆菌群体感应的星形曲霉毒素,为进一步通过结构改造研发新型抗菌药物提供良好的前体化合物。     

具有群体感应抑制活性的海洋细菌的筛选

【目的】从海洋环境中筛选出能有效抑制细菌群体感应的活性菌株,为以致病菌群体感应为靶点的新型疗法提供新的天然产物资源。【方法】以紫色杆菌(Chromobacteriumviolaceum)为报告菌,采用滤纸片法和双层软琼脂法相结合的筛选模型进行群体感应抑制活性菌的筛选。【结果】通过对美国圣璜岛海域海绵中分离出来的272株海洋细菌群体感应抑制活性的筛选,得到了具有抑制紫色杆菌素产生的细菌51株,其中74号菌株抑制效果最好,具有进一步研究的价值。【结论】海洋细菌中有很多具有抑制细菌群体感应效应的菌株,是天然群体感应抑制剂的潜在来源。     

具有群体感应抑制活性海洋放线菌的筛选与鉴定

目的:从海洋放线菌中筛选得到具有群体感应抑制活性菌株,并对其进行鉴定。方法:利用紫色杆菌CV026指示菌株对放线菌发酵粗提物进行活性筛选。其次通过16Sr DNA序列比对进行菌种鉴定。结果:其发酵提取物经紫色杆菌CV026模型筛选后,发现放线菌J501提取物具有群体感应抑制活性,且在有效浓度时对细菌的生长没有影响。16Sr DNA分析表明J501属于Streptomyces属。结论:海洋放线菌中有具有抑制细菌群体感应效应的菌株,是天然群体感应抑制剂的潜在来源。     

群体感应抑制活性海洋细菌的筛选与鉴定

从黄海青岛海域海洋污泥中分离纯化微生物菌株,然后采用紫色色杆菌(Chromobacterium violaceum) 为指示菌株,检测其代谢产物的群体感应(Quorum sensing) 抑制活性,并对具有抑制功能的细菌菌株进行16S rDNA分子鉴定及生理生化特征分析.结果表明,1株蜡样芽孢杆菌和1株水莱茵海默氏菌具有较强的细菌群体感应抑制活性,分别命名为Bacillus cereus QSI01和Rheinheimera aquimaris QSI02.从海洋环境中筛选的具有细菌群体感应抑制活性的菌株,为以致病菌群体感应系统为靶点的新型药物的研发提供了菌种资源.     

一株海洋微小链霉菌群体感应抑制活性及培养条件的研究

以一株分离自连云港海区表层海水中的海洋微小链霉菌(Streptomyces parvulus HY026)为研究对象,采用滤纸片法对其进行群体感应抑制活性测试。结果显示S. parvulus HY026的代谢产物能显著抑制群体感应报告菌紫色杆菌产紫色素,表现出较强的群体感应抑制活性;采用单因子实验,对HY026进行培养基碳源及氮源的优化。发现以玉米粉为碳源时,所得粗提物的质量及群体感应抑制活性最高;以黄豆粉为氮源时,所得粗提物的质量及其活性最高。根据单因子实验结果,选取玉米粉和黄豆粉为最佳碳、氮源,连同盐度、磷酸氢二钾共4个因素进行L16(45)正交实验,以各处理所得的发酵液粗提物质量和群体感应活性为指标进行分析。确定4个因素的重要性顺序为磷酸氢二钾盐度玉米粉黄豆粉,最佳培养基配方为:磷酸氢二钾1.0 g/L,盐度34.0 g/L,玉米粉10.0 g/L,黄豆粉5.0 g/L。以此配方培养时,与原高氏一号培养基培养相比,S. parvulus HY026的发酵液粗提物质量和群体感应抑制活性分别提高了398%和19%。     

具有群体感应抑制活性海洋放线菌的分离和鉴定

群体感应系统在许多致病菌的致病过程中发挥了重要的作用, 可作为开发新型抗菌药物的理想的靶标, 筛选高效的群体感应抑制剂有望成为解决细菌耐药问题的一个有效途径。我们从胶州湾海泥中分离得到放线菌47株, 其发酵提取物经紫色杆菌CV026模型筛选后, 发现放线菌WA-7提取物具有群体感应抑制活性, 且在有效浓度时对细菌的生长没有影响。16S rDNA分析表明WA-7应属于Streptomyces属。进一步研究表明, WA-7提取物能够显著降低紫色杆菌受群体感应调节的紫色菌素产量和相关蛋白酶的表达量, 且呈浓度依赖性。     

海洋弧菌(Vibrio sp.)LA-05发酵液粗提物的群体感应抑制活性及其发酵条件优化

【背景】海洋微生物代谢产物被认为是发掘新型天然活性物质的潜在来源,其中不可避免地包含新型群体感应抑制剂(quorum sensing inhibitors, QSIs)。响应面法是运用多元二次回归模型拟合各因素和响应值之间的函数关系,对各因素及其交互作用进行评价,可有效地从影响代谢产物发酵条件的各因素中预测出最佳条件。【目的】以紫色杆菌(Chromobacterium violaceum)ATCC 12472^T为指示菌株,研究海洋弧菌(Vibrio sp.)LA-05发酵液粗提物的群体感应抑制活性。在单因素试验基础上,应用响应面法对菌株发酵条件进行优化,以提高其发酵代谢产物中活性物质的产量。【方法】使用琼脂平板扩散法进行初筛后,通过分析发酵液粗提物对紫色杆菌生长曲线及紫色素产量的影响研究其群体感应抑制活性。在单因素试验基础上,采用Box-Behnken设计原则,以紫色素抑制率为响应值,通过响应面试验优化菌株发酵条件,从而提高其发酵液中活性物质的产量。【结果】在基本不影响紫色杆菌正常生长的浓度范围内,粗提物可不同程度地抑制紫色素的产生。模型预测结果表明,最优发酵条件...     

紫苏籽油抗菌活性研究

以革兰氏阴性菌大肠杆菌和革兰氏阳性菌枯草芽孢杆菌作为供试菌株,采用滤纸片法测定评估了紫苏籽油经过皂化提取之后其提取液抑制大肠杆菌和枯草芽孢杆菌的能力,并将所得的结果与大豆油的抑菌作用进行比较。结果表明,紫苏籽油提取液对大肠杆菌和枯草芽孢杆菌两个供试菌株的抑制效果较强,且对于枯草芽孢杆菌的抑制效果要优于大肠杆菌,且紫苏籽油对大肠杆菌和枯草芽孢杆菌的抑制效果要优于大豆油。     

具细菌群体感应抑制活性海洋细菌的筛选鉴定

目的:从海洋环境中筛选对细菌群体感应有抑制作用的活性菌株,为以致病菌群体感应系统为靶点的新型疗法提供新的药用资源。方法:从海水中分离纯化细菌菌株,采用根癌农杆菌平板筛选模型筛选细菌群体感应抑制活性细菌,对筛选出的海洋细菌进行生理生化和16S rDNA序列测定,根据《伯杰氏手册》进行菌种分类鉴定。结果:从217株海洋细菌中筛选出1株能显著抑制细菌群体感应效应的海洋细菌Y2,该海洋细菌具有蜡样芽孢杆菌(Bacillus cereus)的典型特征,其16S rDNA序列与GenBank中蜡样芽孢杆菌16S rDNA的部分序列有100%的同源性。结论:海洋环境中也存在具有抑制细菌群体感应活性的微生物。     

Screening of certain medicinal plants from India for their anti-quorum sensing activity

Discovery of quorum sensing (QS) system to coordinate virulence and biofilm formation in bacterial pathogens has triggered search for safe, stable and non-toxic anti-QS compounds from natural products. Ethanolic extracts of 24 Indian medicinal plants were tested by agar well and disc diffusion assay for anti-QS activity using Chromobacterium violaceum (CV12472 and CVO26) reporter strains. AHL from C. violaceum CV31532 was isolated and partially purified for its use in CVO26 based bioassay. Effect on swarming-motility of Pseudomonas aeruginosa (PAO1) was also recorded at sub-MIC concentrations of extracts. Of the 24 medicinal plants screened Hemidesmus indicus (L.) Schult (root), Holarrhena antidysenterica (Roth) A.DC. (bark), Mangifera indica L. (seed) Punica granatum L. (pericarp) and Psoralea corylifolia L. (seed) demonstrated varying level of inhibition of violacein production in the reporter strains. Moreover, a significant reduction in swarms was recorded over control. The inhibition of violacein production and swarming motility may be due to direct or indirect interference on QS by active constituents or the interactive effect of different phytocompounds present in the extracts. These plant extracts may be selected for activity guided fractionation to identify and characterize the active principle.     

Inhibition of bacterial quorum sensing by vanilla extract

AIMS: The purpose of this study was to search for a novel quorum sensing inhibitor and analyse its inhibitory activity. METHODS AND RESULTS: Quorum sensing inhibition was monitored using the Tn-5 mutant, Chromobacterium violaceum CV026. Vanilla beans (Vanilla planifolia Andrews) were extracted using 75% (v/v) aqueous methanol and added to C. violaceum CV026 cultures. Inhibitory activity was measured by quantifying violacein production using a spectrophotometer. The results have revealed that vanilla extract significantly reduced violacein production in a concentration-dependent manner, indicating inhibition of quorum sensing. CONCLUSIONS: Vanilla, a widely used spice and flavour, can inhibit bacterial quorum sensing. SIGNIFICANCE AND IMPACT OF THE STUDY: The results suggest that the intake of vanilla-containing food materials might promote human health by inhibiting quorum sensing and preventing bacterial pathogenesis. Further studies are required to isolate specific substances from vanilla extract acting as quorum sensing inhibitors.     

Evaluation of quorum sensing modulation by plant extracts originating from Turkey

Quorum sensing (QS) is a widespread mechanism utilized by both Gram (+) and Gram (?) bacteria for communication and regulation of specific virulence traits and phenotypes due to population density. Plants are known to produce a number of compounds that can inhibit this communication and most of them have been discovered through well-known Chromobacterium violaceum biomonitor strains assays. In this study, we have analyzed 36 extracts, from 26 Turkish plant species, for their effects on bacterial growth and inhibition or induction of QS in the said biomonitoring assay. Four of the crude plant extracts from Tanacetum balsamita L. subsp. balsamitoides (Compositaceae), Epilobium angustifolium L. (Onograceae), Quercus frainetto Ten. (Fagaceae) and Quercus robur L. (Fagaceae) showed QS inhibitory activity and significantly reduced violacein production in C. violaceum. Particularly, ethyl acetate soluble compounds extracted from leaves of Quercus spp. were efficient in QS inhibition without any apparent increase in bacterial growth. On the other hand, extracts from Mentha longifolia subsp. longifolia and Hypericum orientale showed enhanced violacein production, thus increasing QS-dependent behaviour. Our results clearly demonstrate the QS-inhibitory effects of Q. frainetto Ten., E. angustifolium and T. balsamita L. extracts, while two other species showed QS-inducing effects, for the first time.     

Inhibition of Quorum Sensing–Regulated Behaviors by <Emphasis Type="Italic">Scorzonera sandrasica</Emphasis>

Many Gram-negative bacteria use N-acyl homoserine lactone signal molecules to monitor their own population density and coordinate gene regulation in a process called quorum sensing (QS). Increasing evidence implies that certain eukaryotes produce QS-inhibitory compounds. In this work, we tested 46 terrestrial plants materials for their ability to inhibit QS-regulated behaviors in different bacterial species. Plant materials were dried and extracted using different solvents. The chloroform-soluble compounds extracted from Scorzonera sandrasica were found to inhibit violacein production, a QS-regulated behavior in Chromobacterium violaceum. In addition, the chloroform extract was also able to inhibit QS-regulated carbapenem antibiotic production in Erwinia carotovora. Because the regulation of many bacterial processes is controlled by QS systems, the finding of natural compounds acting as QS inhibitors suggests an attractive tool to control and handle detrimental infections caused by human, animal, and plant pathogens.     

The effect of quorum-sensing blockers on the formation of marine microbial communities and larval attachment

We studied the effect of the quorum-sensing (QS) blockers 5-hydroxy-3[(1R)-1-hydroxypropyl]-4-methylfuran-2(5H)-one (FUR1), (5R)-3,4-dihydroxy-5-[(1S)-1,2-dihydroxyethyl]furan-2(5H)-one (FUR2) and triclosan (TRI) on the formation of bacterial biofilms, and the effect of these biofilms on the larval attachment of the polychaete Hydroides elegans and the bryozoan Bugula neritina. 14-day-old subtidal biofilms were harvested from artificial substrata and were allowed to develop in the laboratory with and without QS blockers. QS blockers inhibited the production of violacein by the QS reporter strain Chromobacterium violaceum CV026 and did not affect the metabolic activity of bacteria in multispecies biofilms. At a concentration of 10(-3) M all three tested compounds inhibited the establishment of microbial communities, but at one of 10(-4) M only FUR2 inhibited establishment. The tested QS blockers caused changes in bacterial density and bacterial community structure, as revealed by terminal restriction fragment length polymorphism and FISH. The groups most affected by QS blockers were Alphaproteobacteria, Gammaproteobacteria and the Cytophagales. Larvae of H. elegans and B. neritina avoided settling on biofilms that had developed in the presence of QS blockers. Our results suggest that QS blockers directly control the formation of multi-species biofilms, and indirectly - by means of biofilm properties - affect larval attachment on these modified biofilms.