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Optimization of hydrolytic and oxidative enzyme methods for ecosystem studies

机译:用于生态系统研究的水解和氧化酶方法的优化

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Microbial digestive enzymes in soil and litter have been studied for over a half century, yet the understanding of microbial enzymes as drivers of ecosystem processes remains hindered by methodological differences among researchers and laboratories. Modern techniques enable the comparison of enzyme activities from different sites and experiments, but most researchers do not optimize enzyme assay methods for their study sites, and thus may not properly assay potential enzyme activity. In this review, we characterize important procedural details of enzyme assays, and define the steps necessary to properly assay potential enzyme activities in environmental samples. We make the following recommendations to investigators measuring soil enzyme activities: 1) run enzyme assays at the environmental pH and temperature; 2) run proper standards, and if using fluorescent substrates with NaOH addition, use a standard time of 1 min between the addition of NaOH and reading in a fluorometer; 3) run enzyme assays under saturating substrate concentrations to ensure V-max is being measured; 4) confirm that product is produced linearly over the duration of the assay; 5) examine whether mixing during the reaction is necessary to properly measure enzyme activity; 6) find the balance between dilution of soil homogenate and assay variation; and 7) ensure that enzyme activity values are properly calculated. These steps should help develop a unified understanding of enzyme activities in ecosystem ecology
机译:已经研究了土壤和垃圾中的微生物消化酶已有半个多世纪,但是研究人员和实验室之间的方法差异仍然阻碍了对微生物酶作为生态系统过程驱动力的理解。现代技术可以比较不同位点和实验的酶活性,但是大多数研究人员并未针对其研究位点优化酶分析方法,因此可能无法正确分析潜在的酶活性。在这篇综述中,我们描述了酶分析的重要程序细节,并定义了适当分析环境样品中潜在酶活性的必要步骤。我们向测量土壤酶活性的研究人员提出以下建议:1)在环境pH和温度下进行酶分析; 2)运行适当的标准液,如果使用添加了NaOH的荧光底物,则在添加NaOH和荧光计之间的标准时间为1分钟; 3)在饱和底物浓度下进行酶分析,以确保测量V-max; 4)确认在检测过程中线性产生产物; 5)检查反应期间是否需要混合以适当地测量酶活性; 6)找到土壤匀浆稀释度与测定变异之间的平衡; 7)确保正确计算酶活性值。这些步骤应有助于建立对生态系统生态系统中酶活性的统一理解

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