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Development of a sensitive and rapid method for the measurement of total microbial activity using fluorescein diacetate (FDA) in a range of soils

机译:利用荧光素二乙酸酯(FDa)在一系列土壤中开发灵敏,快速的总微生物活性测量方法

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摘要

Fluorescein diacetate (FDA) hydrolysis is widely accepted as an accurate and simple method for measuring total microbial activity in a range of environmental samples, including soils. Colourless fluorescein diacetate is hydrolysed by both free and membrane bound enzymes, releasing a coloured end product fluorescein which can be measured by spectrophotometry. The current method for measuring FDA hydrolysis in soils is limited in its application. FDA activity was very low in sandy and clayey soils. The low activity observed for these soil types was made difficult to measure by the original authors choice of solvent for terminating the hydrolysis reaction. Acetone (50% v/v) was found to be most efficient at stopping the hydrolysis reaction. During this study acetone (50% v/v) was found to cause a decrease of approximately 37% in the absorbance of fluorescein produced by the soil samples measured. Although this colour loss is independent of initial fluorescein concentration, it makes the measurement of FDA hydrolytic activity extremely difficult in soils with low microbial activity i.e. sandy and/or clayey soils. Chloroform/methanol (2:1 v/v) was found to successfully stop the hydrolysis reaction for up to 50 min in a range of soil samples without causing the loss of colour observed with acetone. By changing the solvent used for terminating the hydrolysis reaction, low activity soils could be measured successfully. Other parameters of the hydrolysis reaction were optimised for the measurement of soil samples including effect of pH. optimum temperature of incubation, amount of soil, time of incubation, amount of substrate and preparation of suitable standards. A new, more sensitive method is proposed adapted from the original method, which provides a more accurate determination of FDA hydrolysis in a wide range of soils.
机译:荧光素双乙酸酯(FDA)水解是一种准确而简单的方法,可用于测量包括土壤在内的各种环境样品中的总微生物活性。无色荧光素二乙酸酯被游离酶和膜结合酶水解,释放出有色的终产物荧光素,可以通过分光光度法进行测量。目前测量土壤中FDA水解的方法的应用受到限制。在沙质和粘土质土壤中,FDA的活性非常低。最初作者选择用于终止水解反应的溶剂使这些土壤类型的低活性难以测量。发现丙酮(50%v / v)最有效地终止水解反应。在这项研究中,发现丙酮(50%v / v)使所测土壤样品产生的荧光素的吸光度降低约37%。尽管这种颜色损失不依赖于最初的荧光素浓度,但是在微生物活性低的土壤(即沙质和/或黏性土壤)中,FDA水解活性的测量极为困难。发现氯仿/甲醇(2:1 v / v)在一系列土壤样品中成功地终止了长达50分钟的水解反应,而没有引起丙酮所观察到的颜色损失。通过改变用于终止水解反应的溶剂,可以成功地测定低活性污垢。优化了水解反应的其他参数以测量土壤样品,包括pH值的影响。最佳孵育温度,土壤量,孵育时间,底物量和合适标准液的制备。提出了一种与原始方法相适应的新的,更灵敏的方法,该方法可以更准确地确定FDA在多种土壤中的水解度。

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