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Staphylococcal Acid Phosphatase: Extensive Purification and Characterization of the Loosely Bound Enzyme

机译:葡萄球菌酸性磷酸酶:广泛束缚酶的纯化和表征。

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摘要

Acid phosphatase of Staphylococcus aureus PS55 was eluted from the surface of these cells with 1.0 m KCl at pH 8.5 by gentle agitation at 25 C and was purified 44-fold (51% recovery) by two cycles of dialysis and gel filtration. The eluted enzyme which had a 280/260 (nm) absorbancy ratio of 0.71 required at least 0.5 m salt solution for solubilization; however, most of the purified product which had a 280/260 (nm) absorbancy ratio of 1.72 was soluble in dilute buffer solution [0.01 m tris(hydroxymethyl)aminomethane chloride, pH 8.5]. Purified acid phosphatase appeared homogeneous according to the criteria of gel filtration, starch-block electrophoresis, and analytical ultracentrifugation. In a starch block, migration was toward the cathode at pH 8.0. Maximal activity occurred at pH 5.2 to 5.3 and salt concentration had little effect on phosphatase activity up to 1.0 m KCl or NaCl. Progressive loss of enzymatic acitivity occurred at higher salt concentrations. Molecular weight of purified acid phosphatase was estimated to be 58,000.
机译:通过在25°C轻轻搅拌,在pH 8.5下用1.0 m KCl从这些细胞的表面洗脱金黄色葡萄球菌PS55的酸性磷酸酶,并通过两次透析和凝胶过滤循环将其纯化44倍(回收率为51%)。 280/260(nm)吸收比为0.71的洗脱酶至少需要0.5 m的盐溶液才能溶解。但是,大多数吸收率为280/260(nm)为1.72的纯化产物可溶于稀缓冲液[0.01 m三(羟甲基)氨基甲烷氯化物,pH 8.5]。根据凝胶过滤,淀粉阻滞电泳和分析超速离心的标准,纯化的酸性磷酸酶显得均质。在淀粉嵌段中,在pH 8.0下向阴极迁移。在pH值为5.2至5.3时,活性最高,盐浓度最高至1.0 m KCl或NaCl时对磷酸酶活性的影响很小。在较高的盐浓度下,酶活性逐渐下降。纯化的酸性磷酸酶的分子量估计为58,000。

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