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Survival of Host-Associated Bacteroidales Cells and Their Relationship with Enterococcus spp. Campylobacter jejuni Salmonella enterica Serovar Typhimurium and Adenovirus in Freshwater Microcosms as Measured by Propidium Monoazide-Quantitative PCR

机译:单叠氮化物-定量PCR检测淡水微生物中宿主相关细菌的存活及其与肠球菌空肠弯曲杆菌肠炎沙门氏菌血清型鼠伤寒杆菌和腺病毒的关系

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摘要

The ideal host-associated genetic fecal marker would be capable of predicting the presence of specific pathogens of concern. Flowthrough freshwater microcosms containing mixed feces and inocula of the pathogens Campylobacter jejuni, Salmonella enterica serovar Typhimurium, and adenovirus were placed at ambient temperature in the presence and absence of diurnal sunlight. The total Enterococcus DNA increased during the early periods (23 h) under sunlight exposure, even though cultivable Enterococcus and DNA in intact cells, as measured by propidium monoazide (PMA), decreased with first-order kinetics during the entire period. We found a significant difference in the decay of host-associated Bacteroidales cells between sunlight exposure and dark conditions (P value < 0.05), whereas the persistence of host-associated Bacteroidales DNA was comparable. The 2-log reduction times of adenovirus were 72 h for sunlight exposure and 99 h for dark conditions with similar decay rate constants (P value = 0.13). The persistences of fecal Bacteroidales cells and Campylobacter cells exposed to sunlight were similar, and host-associated Bacteroidales DNA and waterborne pathogen DNA were degraded at comparable rates (P values > 0.05). Overall, the ratio of quantitative PCR (qPCR) cycle threshold (CT) values with and without PMA treatment was indicative of the time elapsed since inoculation of the microcosm with (i) fecal material from different animal sources based on host-associated Bacteroidales and (ii) pure cultures of bacterial pathogens. The use of both PMA-qPCR and qPCR may yield more realistic information about recent sources of fecal contamination and result in improved prediction of waterborne pathogens and assessment of health risk.
机译:理想的宿主相关遗传粪便标记物将能够预测所关注的特定病原体的存在。将含有混合粪便和空肠弯曲菌空肠弯曲菌,肠炎沙门氏菌血清型鼠伤寒沙门氏菌和腺病毒的混合流过的淡水缩影放置在环境温度下,在有无日照的情况下。在阳光照射下的早期(23小时),总肠球菌DNA有所增加,即使完整细胞中可培养的肠球菌和DNA(按单叠氮化丙锭(PMA)测量)在整个时期中均以一级动力学下降。我们发现,在阳光照射和黑暗条件下,宿主相关细菌的细菌衰变具有显着差异(P值<0.05),而宿主相关细菌DNA的持久性却相当。具有相似衰减率常数(P值= 0.13)的腺病毒的2-log减少时间在阳光照射下为72 h,在黑暗条件下为99 h。粪便细菌杆菌细胞和弯曲杆菌细胞在阳光下的持久性相似,并且与宿主相关的细菌杆菌DNA和水生病原体DNA的降解速率相当(P值> 0.05)。总体而言,有无PMA处理的定量PCR(qPCR)循环阈值(CT)值之比表明,自从微观接种了(i)来自不同动物来源的粪便材料的寄主以来,该粪便是基于宿主相关的细菌和ii)细菌病原体的纯培养物。 PMA-qPCR和qPCR的使用可能会提供有关近期粪便污染来源的更实际的信息,并改善对水传播病原体的预测和对健康风险的评估。

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