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Determination of lactate dehydrogenase (LDH) activity in milk by a fluorometric assay

机译:荧光测定法测定牛奶中的乳酸脱氢酶(LDH)活性

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Indigenous L-lactate dehydrogenase (LDH) in milk originates mainly from somatic cells, leucocytes and invading microorganisms. Its activity may be used for detection of mastitis. However, existing methods to measure LDH activity in milk both need pretreatment of the samples and still suffer from methodological problems. The present paper describes a fast, reliable method for determination of LDH activity, suitable for milk samples. The method is based on fluorometric determination of enzyme kinetics when L-lactate is converted to pyruvate. The assay uses raw milk without pretreatment and the method is easily adjustable to large-scale analyses on micro assay plates. Detection is based on (straight line) linear response within 4-7 min of initiation of the reaction. A substrate concentration of 35 mm in the reaction mixture was considered to be optimal for the assay. Intra plate assay precision was approx. 6% (CV) and the inter plate precision approx. 10%. Known inhibitors of LDH activity (oxidative direction), i.e., oxalic acid, oxamate, and pyruvate, were tested 'in different concentrations in order to verify the specificity of the response. The detailed kinetics of samples analysed indicated that the isoenzyme composition may have differed between milk samples, and that this composition may have been altered in high activity samples.
机译:牛奶中的本地L-乳酸脱氢酶(LDH)主要来自体细胞,白细胞和侵袭性微生物。其活性可用于乳腺炎的检测。但是,测量牛奶中LDH活性的现有方法既需要对样品进行预处理,又会遇到方法上的问题。本文介绍了一种快速,可靠的测定LDH活性的方法,适用于牛奶样品。该方法基于荧光测定法,当L-乳酸转化为丙酮酸时,酶动力学得以测定。该测定法使用未经预处理的原奶,该方法易于调整,可在微量测定板上进行大规模分析。检测基于反应开始后4-7分钟内的(直线)线性响应。在反应混合物中35mm的底物浓度被认为对于该测定是最佳的。板内分析精度约为6%(CV),板间精度约10%。为了证实反应的特异性,以不同浓度测试了已知的LDH活性(氧化方向)的抑制剂,即草酸,草酸盐和丙酮酸。分析样品的详细动力学过程表明,牛奶样品之间的同工酶组成可能有所不同,并且在高活性样品中该组成可能已经改变。

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