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人乳中蛋白质的区室化与定量分析

Compartmentalization and quantitation of protein in human milk.

作者信息

Lönnerdal B, Woodhouse L R, Glazier C

出版信息

J Nutr. 1987 Aug;117(8):1385-95. doi: 10.1093/jn/117.8.1385.

DOI:10.1093/jn/117.8.1385
PMID:3498019
Abstract

Human milk protein was determined by three colorimetric methods and by Kjeldahl analysis. The distribution of nitrogen (N) and protein was determined within various milk compartments. Total N, whey, casein, nonprotein nitrogen (NPN), cell N and N in the fat fraction were analyzed by micro-Kjeldahl analysis after a series of centrifugation and ultracentrifugation separations. Fresh milk samples (colostrum, transitional milk and mature milk) were centrifuged at 500 X g to separate milk cells and at 5000 X g to skim the milk. Decelled milk and skimmed milk were ultracentrifuged at 189,000 X g to separate fat and casein micelles from whey. NPN was analyzed after trichloroacetic acid precipitation. Whole milk, decelled milk, skimmed milk and whey were analyzed for protein with the Lowry method, modified for fat-containing samples, the Bradford dye-binding assay (Bio-Rad) and the Pierce bicinchoninic acid (BCA) assay. Cell nitrogen had a tendency to be lower in mature milk than in colostrum. Colostrum contained only 6% casein protein, whereas mature milk contained 13%. Fat from skimming was lower in N than fat from ultracentrifugation. Average NPN levels were similar for milk from all three lactation periods, and constituted 10% of colostrum N and 25% of mature milk N. Protein determined by the Bio-Rad method on whole milk samples had the lowest variability (square root MSE) when correlated to Kjeldahl values. All three assays had lower variability when analyzing whey and skimmed milk than when analyzing whole milk. The Lowry method and the Bio-Rad method had low variability for whey and skimmed milk samples, but the Lowry method yielded analytical values closest to Kjeldahl protein values. The BCA method consistently overestimated Kjeldahl protein by 30%.

摘要

采用三种比色法和凯氏定氮法测定人乳蛋白。测定了不同乳成分中氮(N)和蛋白质的分布。通过一系列离心和超速离心分离后,采用微量凯氏定氮法分析总氮、乳清、酪蛋白、非蛋白氮(NPN)、细胞氮和脂肪部分的氮。新鲜牛奶样本(初乳、过渡乳和成熟乳)先以500×g离心以分离乳细胞,再以5000×g离心以撇去乳脂肪。脱细胞乳和脱脂乳以189,000×g超速离心,以从乳清中分离脂肪和酪蛋白胶粒。三氯乙酸沉淀后分析NPN。采用针对含脂肪样本改良的Lowry法、Bradford染料结合法(Bio-Rad)和Pierce双缩脲法(BCA)分析全脂乳、脱细胞乳、脱脂乳和乳清中的蛋白质。成熟乳中的细胞氮含量往往低于初乳。初乳仅含6%的酪蛋白,而成熟乳含13%。脱脂所得脂肪的氮含量低于超速离心所得脂肪。所有三个泌乳期的牛奶中NPN平均水平相似,初乳氮的10%和成熟乳氮的25%为NPN。与凯氏定氮值相关时,用Bio-Rad法测定全脂乳样本中的蛋白质时变异性最低(均方根误差)。分析乳清和脱脂乳时,所有三种测定方法的变异性均低于分析全脂乳时。Lowry法和Bio-Rad法分析乳清和脱脂乳样本时变异性较低,但Lowry法得出的分析值最接近凯氏定氮蛋白值。BCA法始终高估凯氏定氮蛋白30%。

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