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评估美国公共卫生协会(APHA)和美国官方分析化学师协会(AOAC)第二法测定黄油中磷酸酶的方法,并通过琼脂糖凝胶电泳区分牛奶磷酸酶和微生物磷酸酶。

Evaluation of APHA and AOAC II methods for phosphatase in butter and differentiation of milk and microbial phosphatases by agarose-gel electrophoresis.

作者信息

Murthy G K, Kaylor L O

机构信息

Food and Drug Administration, Division of Microbiology, Cincinnati, OH 45226.

出版信息

J Assoc Off Anal Chem. 1990 Sep-Oct;73(5):681-7.

PMID:2177055
Abstract

Salted and unsalted butters with 3 levels of phosphatase were prepared with both raw and pasteurized cream containing 36% fat. Test samples were analyzed for phosphatase by the modified method of the American Public Health Association (APHA) and the official AOAC method, 16.256 (1984, 14th Ed., 1990 15th Ed., 946.02). In the APHA method, weighing of solid frozen butter for testing yielded repeatable results. Addition of 0.0-1.0 mg magnesium to the butter had little effect on phosphatase activity in the APHA modified rapid colorimetric method (MRCM), but caused the phosphatase activity to decrease in the AOAC method. Phosphatase in salted and unsalted butters was quite stable at -17 +/- 1 degrees C and at 3.0 +/- 0.5 degrees C; however, within 2 to 4 days, freshly prepared butters stored at 22 +/- 1 degrees C developed reactivated and/or microbial phosphatases that were both heat-labile and heat-stable. At 22 +/- 1 degrees C, frozen butters showed decreased milk phosphatase activity before producing microbial phosphatase. Heat-labile phosphatases in salted and unsalted butters were inactivated at 62.8 degrees C for 10 min, and the phosphatase lability was partially due to the heat-denaturing effect of NaCl in salted butter. Some heat-stable phosphatases in unsalted butter survived at 66 degrees C for 30 min. Differentiation of milk phosphatase from microbial phosphatases was difficult by both methods; however, they were successfully differentiated by the agarose-gel electrophoretic technique.

摘要

用含36%脂肪的生乳脂和巴氏杀菌乳脂制备了含有3种磷酸酶水平的加盐黄油和不加盐黄油。采用美国公共卫生协会(APHA)的改良方法和美国官方分析化学家协会(AOAC)的官方方法16.256(1984年第14版,1990年第15版,946.02)对测试样品进行磷酸酶分析。在APHA方法中,称取用于测试的固态冷冻黄油可得到可重复的结果。在APHA改良快速比色法(MRCM)中,向黄油中添加0.0 - 1.0毫克镁对磷酸酶活性影响不大,但在AOAC方法中会导致磷酸酶活性降低。加盐黄油和不加盐黄油中的磷酸酶在-17±1℃和3.0±0.5℃下相当稳定;然而,在2至4天内,新鲜制备的黄油在22±1℃下储存会产生热不稳定和热稳定的再活化和/或微生物磷酸酶。在22±1℃下,冷冻黄油在产生微生物磷酸酶之前,乳磷酸酶活性会降低。加盐黄油和不加盐黄油中的热不稳定磷酸酶在62.8℃下10分钟会失活,这种磷酸酶的不稳定性部分归因于加盐黄油中NaCl的热变性作用。不加盐黄油中的一些热稳定磷酸酶在66℃下30分钟仍能存活。两种方法都很难区分乳磷酸酶和微生物磷酸酶;然而,通过琼脂糖凝胶电泳技术成功地将它们区分开来。

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引用本文的文献

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The use of alkaline phosphatase and possible alternative testing to verify pasteurisation of raw milk, colostrum, dairy and colostrum-based products.使用碱性磷酸酶及可能的替代检测方法来验证生乳、初乳、乳制品和初乳制品的巴氏杀菌效果。
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