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.     

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.     

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.     

苯甲酸盐厌氧驯化体系中三氯乙烯的还原脱氯特性

采用气相色谱法实时监测了厌氧条件下,以苯甲酸盐为唯一碳源的驯化活性污泥体系对三氯乙烯(TCE)的还原脱氯情况;同时,结合454焦磷酸测序和实时荧光定量PCR技术对该体系中的微生物群落结构及脱卤拟球菌(DHC)的数量进行分析.结果表明,该驯化体系在94 d内能将TCE完全去除,最终转化产物为一氯乙烯(VC),同时伴随大量的甲烷产生;体系中微生物的多样性很高,涵盖了16个门、33个纲、52个目、88个科和129个属,而且体系中约有51.2%的微生物的分类地位尚未明确,说明体系中还存在很多未知的功能菌;体系对TCE的降解过程其实就是还原脱氯菌与其它功能菌相互作用的结果,且起主要还原脱氯作用的是携带tce A功能基因的DHC.     

太湖和巢湖夏季蓝藻水华期间产毒微囊藻和非产毒微囊藻种群丰度的空间分布

应用荧光定量PCR技术对蓝藻水华暴发期间太湖和巢湖水体中产毒微囊藻和总微囊藻种群丰度的空间分布进行了研究.分别以微囊藻毒素合成基因基因家族成员mcyD和小核糖体16S rDNA序列构建定量PCR标准曲线,研究产毒微囊藻和总微囊藻种群丰度.结果表明:太湖和巢湖微囊藻种群由产毒微囊藻和非产毒微囊藻组成;蓝藻水华暴发期间,微囊藻种群组成及其丰度分布具有明显的空间差异性:太湖产毒微囊藻种群丰度为9.89×104～4.51×106 copies mL-1,产毒微囊藻占总微囊藻种群的比例为20.5%～38.1%;巢湖产毒微囊藻种群丰度为4.12×104～5.44×106 copies mL-1,其占总微囊藻种群的比例为8.4%～96.6%.总的来说,富营养化严重的湖区总微囊藻和产毒微囊藻种群丰度较高,产毒微囊藻占总微囊藻种群的比例也较高.图7表3参29     

北京地区菜田土壤抗生素抗性基因的分布特征

为研究北京地区菜田土壤抗生素抗性基因(antibiotic resistance genes,ARGs)的污染状况和分布特征,采集了11个长期施用粪肥蔬菜基地的温室土壤和大田土壤,进行了抗生素以及ARGs种类和丰度的检测.结果表明,菜田土壤中四环素类抗生素残留量最高,其次为磺胺类抗生素,温室土壤抗生素残留普遍高于大田土壤.温室和大田土壤磺胺类抗性基因sul1、sul2和四环素类抗性基因tet L的检出率均为100%.温室土壤的Ⅰ类整合子(int I1)检出率比大田土壤高1.5倍.定量PCR的检测结果表明,菜田土壤中sul2和tet L的相对丰度介于10-4~10-2之间,温室土壤sul2和tet L的相对丰度普遍高于大田土壤.sul2的相对丰度与磺胺二甲嘧啶和强力霉素的含量显著正相关(P0.05),tet L相对丰度与抗生素含量无明显相关性(P0.05).本研究结果对于掌握北京地区农田土壤ARGs的污染现状,以及从ARGs角度评估农艺措施具有重要的指导意义.     

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.     

天津沿岸海水中创伤弧菌的PCR检测和定量

采用普通PCR方法和SYBR Green实时定量PCR方法,根据创伤弧菌16S rDNA和23S rDNA基因间隔序列(internal transcribed spacer,ITS)设计引物,对渤海湾天津沿岸海水中的创伤弧菌进行了定性和定量检测.8个样品采集自天津市汉沽区沿岸海水,采集时间分别为2008年7月、10月和2009年3月、5月.PCR检测结果表明,这些样品都能扩增出276 bp的ITS序列,这些序列和GenBank上的同源序列(DQ462478)的相似性为96%～98%.用SYBR Green实时定量PCR方法测定了8个海水样品,样品中创伤弧菌的浓度为7.12×10~3～8.40×10~5 个/L,表明天津沿岸海水存在严重的创伤弧菌污染.     

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。