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Purification of lipoteichoic acid by chromatography in water-organic solvent systems.

机译:在水-有机溶剂体系中通过色谱法纯化脂磷壁酸。

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摘要

Lipoteichoic acid (LTA), extracted from Streptococcus mutans 10449 by hot aqueous phenol, was partially purified by Sepharose 6B column chromatography in 0.01 M sodium acetate, pH 6.0, containing 0.25 M sodium chloride and 0.001 M EDTA. Nucleic acid and polysaccharide were precipitated from the LTA-containing column peak by the addition of 2 volumes of chloroform-methanol (1:5). The resulting single-phase chloroform-methanol-water (1:5:3) supernatant contained LTA and small amounts of several contaminating substances as indicated by reverse-phase high-pressure liquid chromatography and chemical analyses. LTA was purified further by DEAE-cellulose chromatography, using a concentration gradient of sodium chloride in chloroform-methanol-water (1:5:3). Two column peaks of LTA were found to contain phosphate, glycerol, glucose, and fatty acids at molar ratios of 1:1:0.11:0.10 and 1:1:0.09:0.04, respectively. The LTA polymers contained 18 and 22 repeating units of unsubstituted glycerophosphate and two glucose residues. The LTA in one column peak had two fatty acids per molecule, whereas that in the second peak contained only one. The yield of LTA was 1.68 mg per g of cell dry weight or 65 mg per g of phenol-water-extracted material. The specific activity of the LTA preparation was increased 128-fold by the purification scheme as determined by a erythrocyte-binding assay. Reverse-phase high-pressure liquid chromatography may be used for rapid separation of LTA molecules containing different numbers of acyl groups.
机译:通过热苯酚水溶液从变形链球菌10449中提取的脂蛋白酸(LTA)通过Sepharose 6B柱色谱法在0.01 M乙酸钠,pH 6.0,含有0.25 M氯化钠和0.001 M EDTA的条件下进行部分纯化。通过添加2体积的氯仿-甲醇(1:5),从含有LTA的柱峰中沉淀出核酸和多糖。反相高压液相色谱法和化学分析表明,所得的单相氯仿-甲醇-水(1:5:3)上清液含有LTA和少量几种污染物质。通过在氯仿-甲醇-水(1:5:3)中氯化钠的浓度梯度,通过DEAE-纤维素色谱法进一步纯化LTA。发现LTA的两个柱峰分别含有摩尔比为1:1:0.11:0.10和1:1:0.09:0.04的磷酸盐,甘油,葡萄糖和脂肪酸。 LTA聚合物包含18和22个未取代的甘油磷酸酯重复单元和两个葡萄糖残基。一个色谱柱峰中的LTA每个分子具有两种脂肪酸,而第二个色谱峰中的LTA仅包含一种脂肪酸。 LTA的产量为每克细胞干重1.68毫克或每克苯酚-水提取物65毫克。通过红细胞结合测定法确定的纯化方案,LTA制剂的比活性提高了128倍。反相高压液相色谱法可用于快速分离含有不同数量酰基的LTA分子。

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