A rapid, quantitative assay for measuring alkaline phosphatase activity in osteoblastic cells in vitro

A. Sabokbar, P.J. Millett, B. Myer, N. Rushton
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引用次数: 213

Abstract

Alkaline phosphatase (ALP) is the most widely recognized biochemical marker for osteoblast activity. Although its precise function is poorly understood, it is believed to play a role in skeletal mineralization. The aim of this study was to develop an assay suitable for measuring the activity of this enzyme in microtiter plate format. Using the well-characterized osteoblast-like cell line Saos-2, this paper describes an optimized biochemical assay suitable for measuring ALP activity in tissue culture samples. We have determined that a p-nitrophenyl phosphate substrate concentration of 9 mM provides highest enzyme activities. We have found that cell concentration, and hence enzyme concentration, affects both the kinetics and precision of the assay. We also tested several methods of enzyme solubilization and found that freeze-thawing the membrane fractions twice at −70°C/37°C or freeze-thawing once with sonication yielded highest enzyme activities. The activity of the enzyme decreased by 10% after 7 days storage. This assay provides a sensitive and reproducible method that is ideally suited for measuring ALP activity in isolated osteoblastic cells, although sample preparation and storage can influence results.

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体外成骨细胞碱性磷酸酶活性的快速定量测定方法
碱性磷酸酶(ALP)是最广泛认可的成骨细胞活性生化标志物。虽然它的确切功能尚不清楚,但它被认为在骨骼矿化中起作用。本研究的目的是开发一种适合于用微滴板形式测量该酶活性的测定方法。利用具有良好特征的成骨样细胞系Saos-2,本文描述了一种适合于测量组织培养样品中ALP活性的优化生化检测方法。我们已经确定,对硝基苯基磷酸盐底物浓度为9毫米提供最高的酶活性。我们发现细胞浓度,因此酶浓度,影响动力学和测定的精度。我们还测试了几种酶增溶方法,发现在- 70°C/37°C冷冻解冻两次或用超声波冷冻解冻一次产生最高的酶活性。贮藏7 d后,酶活性下降10%。该试验提供了一种敏感和可重复性的方法,非常适合于测量分离成骨细胞中的ALP活性,尽管样品制备和储存会影响结果。
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