基于引物的湖泊沉积物氨氧化细菌PCR扩增策略比较

PCR扩增是检测环境中β-变形杆菌纲氨氧化细菌(β-AOB)群落的主要方法,但是引物的敏感性和特异性对结果具有关键影响.本研究首先比较了2组常用的β-AOB 16S rRNA基因引物,结果显示,在扩增一组不同性质湖泊沉积物样品时,βAMO引物均获得明亮的单一条带,但CTO引物则未能全部扩增.克隆及序列分析证实,βAMO引物扩增获得的序列均不属于β-AOB所在的Nitrosomonadales目,而CTO引物扩增获得的序列来自β-AOB中的Nitrosomonas europaea/"Nitrosococcus mobilis"分支.采用变性梯度凝胶电泳方法,对4种不同引物组合PCR策略扩增所得产物进行分析,发现以βAMO或16S rRNA通用引物结合CTO引物的巢式方案可以提高扩增的效率,且β-AOB的群落轮廓与CTO引物直接扩增方案高度相似.这些结果表明βAMO引物具有较高的敏感性但特异性较低,而CTO引物则相反.因此,特定巢式扩增方案既可提高扩增的效率,也能真实反映湖泊沉积物中β-AOB的群落轮廓,是较为理想的β-AOB研究方法.     

Effect of a high strength chemical industry wastewater on microbial community dynamics and mesophilic methane generation

A high strength chemical industry wastewater was assessed for its impact on anaerobic microbial com- munity dynamics and consequently mesophilic methane generation. Cumulative methane production was 251 mL/g total chemical oxygen demand removed at standard temperature and pressure at the end of 30 days experimental period with a highest recorded methane percentage of 80.6% of total biogas volume. Volatile fatty acids （VFAs） analysis revealed that acetic acid was the major intermediate VFAs produced with propionic acid accumulating over the experimental period. Quantitative analysis of microbial communities in the test and control groups with quantitative real time polymerase chain reaction highlighted that in the test group, Eubacteria （96.3%） was dominant in comparison with methanogens （3.7%）. The latter were dominated by Methanomicrobiales and Methanobacteriales while in test groups increased over the experimental period, reaching a maximum on day 30. Denaturing gradient gel electrophoresis profile was performed, targeting the 16S rRNA gene of Eubacteria and Archaea, with the DNA samples extracted at 3 different time points from the test groups. A phylogenetic tree was constructed for the sequences using the neighborhood joining method. The analysis revealed that the presence of organisms resembling Syntrophomonadaceae could have contributed to increased production of acetic and propionic acid intermediates while decrease of organisms resembling Pelotomaculum sp. could have most likely contributed to accumulation of propionic acid. This study suggested that the degradation of organic components within the high strength industrial wastewater is closely linked with the activity of certain niche microbial communities within eubacteria and methanogens.     

基于EMD-HHT可定位长输天然气管道第三方破坏事件监测技术

为适应目前管道安全监测需要,满足对扰动信号分类监测的实际需求,提出1种基于希尔伯变换和经验模态分解(EMD-HHT)的信号特征提取技术,利用基于φ-OTDR分布式光纤传感系统采集振动信号,通过EMD+HHT区分算法对管道沿线振动事件进行分解并提取6个典型特征向量,各特征事件数据经过EMD后选取IMF3为最终提取特征向量的原始数据,BP神经元网络可有效识别机械破坏、敲击破坏、车辆经过、人工挖掘、动力干扰5种事件。研究结果表明：在长输管道信号识别中,BP神经网络对5类事件平均识别率高达98.6%,该技术分类识别5类事件扰动信号,能够达到较高准确性,并且误报率平均在1.3%,能较好满足现场安全实时监测需求。研究结果对长输油气管道附近第三方破坏扰动信号分类监测具有一定参考意义。     

中温和高温厌氧生物产氢反应器连续运行的研究

采用2个厌氧生物产氢反应器分别在中温(37℃)和高温(55℃)下连续运行.以河底沉积物接种,葡萄糖为基质,在CSTR中成功实现了连续中温厌氧产氢,最高产氢量达8.6L/(L·d),基质产氢摩尔比(H₂/葡萄糖)为1.98.以厌氧产甲烷颗粒污泥接种,蔗糖为基质,在UASB反应器中成功实现了连续高温厌氧产氢过程,最高产氢量达6.8L/(L·d),基质产氢摩尔比(H₂/蔗糖)为3.6.在高温UASB反应器中培养获得了灰白色的产氢颗粒污泥,平均粒径为0.8～1.2mm,沉速为30～40m/h,电镜观察发现其表层生长大量杆状细菌.对2种产氢污泥的总DNA进行提取和纯化,通过PCR扩增和DGGE分析,发现高温和中温厌氧产氢污泥中的大部分真细菌种类相同,但各自的优势菌种明显不同.     

PCR-DGGE研究处理垃圾渗滤液序批式生物膜反应器(SBBR)中的细菌多样性

为了研究序批式生物膜反应器中的细菌多样性及其脱氮的微生物学机理,为工艺改进提供依据,从同步高效去除垃圾渗滤液中高氨氮和高COD的SBBR生物膜和渗滤液原水中采集微生物样品并提取微生物总DNA,使用细菌通用引物对（GC341F/907R）从总DNA中成功扩增出目标16S rDNA片段,然后对扩增的16S rDNA进行DGGE,对凝胶染色并进行条带统计分析和切胶测序,使用序列数据进行同源性分析并建立了系统发育树.结果表明,该驯化后的SBBR生物膜和渗滤液原水中都有比较丰富的细菌多样性,驯化的生物膜细菌主要来自渗滤液原水,而且生物膜细菌在反应器正常运行时不会出现明显的群落结构变化;在该SBBR中有多种硝化细菌与反硝化细菌、好氧反硝化细菌和厌氧氨氧化细菌共存,说明该反应器中可能同时存在全程硝化反硝化、同步硝化反硝化和厌氧氨氧化3种脱氮方式.研究结果为SBBR脱氮微生物机理研究提供了一些有价值的参考依据.     

危险品运输实时监控及应急救援服务平台构建

针对我国危险品运输监管及应急救援现状,提出构建"危险品运输实时监控及应急救援服务平台"的技术方案。设计了平台系统的技术框架,介绍装载于危险品运输车辆之上的"监控终端"以及应急救援车辆之上的"智能终端"的基本功能,并以环保部门为例阐述了服务平台与危险废物监管政务平台之间的数据交换及功能耦合,以及利用服务平台开展危险品运输事故应急救援联动流程。该平台可望解决"危险品运输多部门监管数据不一致以及多部门联动应急救援调度困难"这一实际问题。     

实时荧光定量PCR法快速测定水中微囊藻

以铜绿微囊藻（Microcystis aeruginosa）16S rRNA基因片段为靶序列设计一对特异性引物,采用Real-time PCR法,对铜绿微囊藻进行定性、定量检测。试验表明,仅含铜绿微囊藻DNA模板的样品有特异性扩增,扩增产物熔解曲线平稳,峰尖且窄,熔解温度为（87±1）℃。以重组质粒pMD-18T-16S为标准品,检测区间为1．1×102 copies/mL～1．1×108 copies/mL,所得标准曲线符合制备实时定量PCR标准曲线的要求,对标准品进行测定,方法检出限为11 copies/mL。用该标准曲线对实验室培养获得的铜绿微囊藻DNA样品进行定量检测,与显微镜计数结果基本一致。     

Diversity of antibiotic resistance genes and encoding ribosomal protection proteins gene in livestock waste polluted environment

The rapid development and increase of antibiotic resistance are global phenomena resulting from the extensive use of antibiotics in human clinics and animal feeding operations. Antibiotics can promote the occurrence of antibiotic resistance genes (ARGs), which can be transferred horizontally to humans and animals through water and the food chain. In this study, the presence and abundance of ARGs in livestock waste was monitored by quantitative PCR. A diverse set of bacteria and tetracycline resistance genes encoding ribosomal protection proteins (RPPs) from three livestock farms and a river were analyzed through denaturing gradient gel electrophoresis (DGGE). The abundance of sul(I) was 10³ to 10⁵ orders of magnitude higher than that of sul(II). Among 11 tet-ARGs, the most abundant was tet(O). The results regarding bacterial diversity indicated that the presence of antibiotics might have an evident impact on bacterial diversity at every site, particularly at the investigated swine producer. The effect of livestock waste on the bacterial diversity of soil was stronger than that of water. Furthermore, a sequencing analysis showed that tet(M) exhibited two genotypes, while the other RPPs-encoding genes exhibited at least three genotypes. This study showed that various ARGs and RPPs-encoding genes are particularly widespread among livestock.     

Detection of Class I and II integrons for the assessment of antibiotic and multidrug resistance among Escherichia coli isolates from agricultural irrigation waters in Bulacan,Philippines

Contaminated irrigation water may greatly affect not only the quality of produce but also the people exposed to it. In this study, agricultural irrigation waters in Bulacan, Philippines were assessed and found to be contaminated with Escherichia coli (E. coli) ranging from 0.58 to 4.51 log₁₀ CFU/mL. A total of 79 isolates of E. coli were confirmed through polymerase chain reaction (PCR) amplifying the uidA gene and were tested for phenotypic resistance using 10 antimicrobials through the Kirby–Bauer disc diffusion method. Forty-six isolates (58.22%) were noted to be multidrug resistant (MDR) with high resistance rate to cephalothin, tetracycline, streptomycin, ampicillin, trimethoprim, nalidixic acid, and chloramphenicol. Moreover, this study also examined the prevalence of Class I and II integrons accounting to 67.39% and 17.39%, respectively, of the MDR E. coli strains using multiplex PCR. The results imply that the agricultural water used in Bulacan is contaminated with the fecal material of man or other animals present in the area, and the presence of MDR bacteria, which pose a potential threat to individuals in these areas, is alarming. In addition, detection of integrons could be a good marker for the identification of MDR isolates. Lastly, this study could develop strategies for the proper management of farming sites leading to the detection of food-borne pathogens and prevention of infectious diseases.     

Investigation into the effect of high concentrations of volatile fatty acids in anaerobic digestion on methanogenic communities

A study was conducted to determine whether differences in the levels of volatile fatty acids (VFAs) in anaerobic digester plants could result in variations in the indigenous methanogenic communities. Two digesters (one operated under mesophilic conditions, the other under thermophilic conditions) were monitored, and sampled at points where VFA levels were high, as well as when VFA levels were low. Physical and chemical parameters were measured, and the methanogenic diversity was screened using the phylogenetic microarray ANAEROCHIP. In addition, real-time PCR was used to quantify the presence of the different methanogenic genera in the sludge samples. Array results indicated that the archaeal communities in the different reactors were stable, and that changes in the VFA levels of the anaerobic digesters did not greatly alter the dominating methanogenic organisms. In contrast, the two digesters were found to harbour different dominating methanogenic communities, which appeared to remain stable over time. Real-time PCR results were inline with those of microarray analysis indicating only minimal changes in methanogen numbers during periods of high VFAs, however, revealed a greater diversity in methanogens than found with the array.