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以分离在牛乳中表达的人α-1抗胰蛋白酶为目标,研究聚乙二醇-柠檬酸钠双水相体系中乳清蛋白的分配特性。

Features of the milk whey protein partitioning in polyethyleneglycol-sodium citrate aqueous two-phase systems with the goal of isolating human alpha-1 antitrypsin expressed in bovine milk.

作者信息

Boaglio Andrea, Bassani Georgina, Picó Guillermo, Nerli Bibiana

机构信息

Chemical Physics Department, Bioseparation Lab., CONICET, and FonCyT, Faculty of Biochemical and Pharmaceutical Sciences, National University of Rosario, S2002LRK Rosario, Argentina.

出版信息

J Chromatogr B Analyt Technol Biomed Life Sci. 2006 Jun 6;837(1-2):18-23. doi: 10.1016/j.jchromb.2006.03.049. Epub 2006 Apr 27.

Abstract

Partitioning behaviour of the bovine whey proteins (bovine serum albumin, alpha-lactoalbumin and beta-lactoglobulin) and human alpha-1 antitrypsin in aqueous two-phase systems prepared with polyethyleneglycol (molecular masses: 1000, 1450 and 3350)-sodium citrate was analysed at pH 5.2, 6.2 and 8.2. Alpha lactoalbumin concentrated in the polyethyleneglycol rich-phase, while beta-lactoglobulin, bovine serum albumin and alpha-1 antitrypsin showed affinity for the citrate rich-phase. In aqueous two-phase systems of high medium pH and high polyethyleneglycol molecular mass the protein partitioning equilibrium is displaced to the citrate rich-phase. The polyethyleneglycol 1450-pH 5.2 system with a top/bottom phase-volume ratio of 3 showed to have the best capability of recovering the alpha-1 antitrypsin from a mixture prepared with natural milk whey and human alpha-1 antitrypsin. The recovery of this protein in the bottom phase was of 90% and the purity of the obtained product was of 98%. The method appears to be suitable as a starting point to isolate other human proteins expressed in transgenic bovine milk.

摘要

分析了牛血清白蛋白、α-乳白蛋白和β-乳球蛋白等牛乳清蛋白以及人α-1抗胰蛋白酶在由聚乙二醇(分子量分别为1000、1450和3350)-柠檬酸钠制备的水相双相体系中,在pH值为5.2、6.2和8.2时的分配行为。α-乳白蛋白富集于富含聚乙二醇的相中,而β-乳球蛋白、牛血清白蛋白和α-1抗胰蛋白酶则对富含柠檬酸盐的相表现出亲和力。在高pH值和高分子量聚乙二醇的水相双相体系中,蛋白质分配平衡向富含柠檬酸盐的相移动。具有3的顶/底相体积比的聚乙二醇1450-pH 5.2体系显示出从天然乳清和人α-1抗胰蛋白酶制备的混合物中回收α-1抗胰蛋白酶的最佳能力。该蛋白质在底相中的回收率为90%,所得产物的纯度为98%。该方法似乎适合作为分离转基因牛乳中表达的其他人类蛋白质的起点。

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