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通过分子方法监测蓝藻水华毒性的变化

Monitoring changing toxigenicity of a cyanobacterial bloom by molecular methods.

作者信息

Baker Judith A, Entsch Barrie, Neilan Brett A, McKay David B

机构信息

University of New England, Armidale 2351, Australia.

出版信息

Appl Environ Microbiol. 2002 Dec;68(12):6070-6. doi: 10.1128/AEM.68.12.6070-6076.2002.

Abstract

Cyanobacterial blooms are potential health hazards in water supply reservoirs. This paper reports analyses of a cyanobacterial bloom by use of PCR-based methods for direct detection and identification of strains present and determination of their toxigenicity. Serial samples from Malpas Dam, in the New England region of Australia, were analyzed during a prolonged, mixed cyanobacterial bloom in the summer of 2000 to 2001. Malpas Dam has been shown in the past to have toxic blooms of Microcystis aeruginosa that have caused liver damage in the human population drinking from this water supply reservoir. Cyanobacterial genera were detected at low cell numbers by PCR amplification of the phycocyanin intergenic spacer region between the genes for the beta and alpha subunits. The potential for microcystin production was determined by PCR amplification of a gene in the microcystin biosynthesis pathway. The potential for saxitoxin production was determined by PCR amplification of a region of the 16S rRNA gene of Anabaena circinalis strains. Toxicity of samples was established by mouse bioassay and high-pressure liquid chromatography. We show that bloom components can be identified and monitored for toxigenicity by PCR more effectively than by other methods such as microscopy and mouse bioassay. We also show that toxigenic strains of Anabaena and Microcystis spp. occur at this site and that, over the course of the bloom, the cell types and toxicity changed. This work demonstrates that PCR detection of potential toxicity can enhance the management of a significant public health hazard.

摘要

蓝藻水华是供水水库中的潜在健康危害。本文报道了利用基于聚合酶链反应(PCR)的方法对蓝藻水华进行分析,以直接检测和鉴定存在的菌株并确定其产毒性。在2000年至2001年夏季澳大利亚新英格兰地区马尔帕斯大坝持续出现混合蓝藻水华期间,对其连续样本进行了分析。过去已表明,马尔帕斯大坝曾出现过铜绿微囊藻有毒水华,导致饮用该供水水库水的人群出现肝脏损伤。通过对β和α亚基基因之间的藻蓝蛋白基因间隔区进行PCR扩增,在低细胞数量时检测到了蓝藻属。通过对微囊藻毒素生物合成途径中的一个基因进行PCR扩增,确定了微囊藻毒素的产生潜力。通过对环状鱼腥藻菌株16S rRNA基因的一个区域进行PCR扩增,确定了石房蛤毒素的产生潜力。通过小鼠生物测定法和高压液相色谱法确定了样本的毒性。我们表明,与显微镜检查和小鼠生物测定法等其他方法相比,利用PCR能更有效地鉴定水华成分并监测其产毒性。我们还表明,鱼腥藻属和微囊藻属的产毒菌株在该地点出现,并且在水华过程中,细胞类型和毒性发生了变化。这项工作表明,PCR检测潜在毒性可加强对重大公共卫生危害的管理。

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