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首页> 外文期刊>Archives of Environmental Contamination and Toxicology >Development of an Improved Rapid Enzyme Inhibition Bioassay with Marine and Freshwater Microalgae Using Flow Cytometry
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Development of an Improved Rapid Enzyme Inhibition Bioassay with Marine and Freshwater Microalgae Using Flow Cytometry

机译:流式细胞术开发一种改进的海洋和淡水微藻快速酶抑制生物测定方法

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摘要

A rapid toxicity test based on inhibition of esterase activity in marine and freshwater microalgae (Selenastrum capricornutum, Chlorella sp., Dunaliella tertiolecta, Phaeodactylum tricornutum, Tetraselmis sp., Entomoneis cf. punctulata, Nitzschia cf. paleacea) was developed using flow cytometry. Uptake of fluorescein diacetate (FDA) was optimized for each species by varying the substrate concentration, incubation time, and media pH. Propidium iodide (PI) was utilized to assess membrane integrity. The optimized FDA/PI staining procedure was then used to assess the toxicity of copper in short-term exposures (1–24 h). Esterase activity was a sensitive indicator of copper toxicity in S. capricornutum and E. cf. punctulata. As copper concentrations increased, esterase activity decreased in a concentration-dependent manner. The 3- and 24-h EC50 values (based on mean activity states) were 112 μg Cu L−1 (95% confidence limits 88–143) and 51 μg Cu L−1 (95% confidence limits 38–70) for S. capricornutum and 47 μg Cu L−1 (95% confidence limits 43–51) and 9.1 μg Cu L−1 (95% confidence limits 7.6–11) for E. cf. punctulata, respectively. This enzyme inhibition endpoint showed similar sensitivity to chronic growth rate inhibition in E. cf. punctulata (48-h and 72-h EC50 values of 17 and 18 μg L−1, respectively) but was less sensitive compared to growth for S. capricornutum (48-h and 72-h EC50 values of 4.9 and 7.5 μg L−1, respectively). For the other five species tested, inhibition of FDA fluorescence was relatively insensitive to copper, even at copper concentrations that severely inhibited cell division rate. These short-term bioassays that detect sublethal endpoints may provide a more rapid and cost-effective way of monitoring contaminant impacts in natural waters.
机译:使用流式细胞仪开发了一种基于抑制海洋和淡水微藻类(长绒毛小球藻,小球藻,杜氏杜氏藻,毛状线虫,四角藻,Tetraselmis sp。,Entomoneis cf. punlata,Nitzschia cf。通过改变底物浓度,孵育时间和培养基pH,针对每个物种优化了双乙酸荧光素(FDA)的吸收。碘化丙啶(PI)用于评估膜的完整性。然后将优化的FDA / PI染色程序用于评估铜在短期暴露(1–24小时)中的毒性。酯酶活性是铜对链球菌和大肠杆菌中铜毒性的敏感指标。准时。随着铜浓度的增加,酯酶活性以浓度依赖性方式降低。 3小时和24小时EC50 值(基于平均活性状态)分别为112μgCu L-1 (95%置信度88-143)和51μgCu L-1 山羊乳链球菌和47μgCu L-1 (95%置信度限制43-51)和9.1μgCu L-1 (95%置信度限制)的(95%置信度限制38-70) 7.6 – 11)。分别是该酶抑制终点对大肠杆菌中的慢性生长速率抑制显示相似的敏感性。击穿(48-h和72-h EC50 值分别为17和18μgL-1 ),但与沙门氏菌的生长(48-h和72-h EC50)相比,敏感性较低值分别为4.9和7.5μgL-1 )。对于其他五个受测物种,即使在严重抑制细胞分裂速率的铜浓度下,FDA荧光的抑制对铜也相对不敏感。这些检测亚致死终点的短期生物测定法可能会提供一种更快速,更具成本效益的方法来监测天然水中的污染物影响。

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    Centre for Advanced Analytical Chemistry CSIRO Energy Technology PMB 7 Bangor New South Wales 2234 Australia;

    Centre for Advanced Analytical Chemistry CSIRO Energy Technology PMB 7 Bangor New South Wales 2234 Australia;

    Centre for Advanced Analytical Chemistry CSIRO Energy Technology PMB 7 Bangor New South Wales 2234 Australia;

    Department of Environmental Sciences University of Technology Sydney PO Box 123 Broadway New South Wales 2007 Australia;

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