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[将腐生葡萄球菌L-1的脲酶固定在活化硅胶上]

[Immobilization of urease from Staphylococcal saprophyticus L-1 on activated silica].

作者信息

Liubinskiĭ G V, Ianishpol'skiĭ V V, Tertykh V A, Iuodval'kite D Iu, Glemzha A A

出版信息

Ukr Biokhim Zh (1978). 1987 Jul-Aug;59(4):35-41.

PMID:2820097
Abstract

The paper deals with immobilization of urease obtained from Staphylococcus saprophyticus L-1 on the organic silica surfaces. The process completion time (4-5 h) and the optimal pH of binding (7-8) are practically independent of the chemical nature of the carrier surface. The value of the specific activity of urease grafted to silica depends not only on the type of the enzyme-carrier bond, but also on the macromolecule protein-to-silica distance. The extent of the retained enzyme activity is shown to be 26% after sorption on the initial silica. It grows to 100% with an increase of the organic radical length which separates the biocatalyst and the carrier.

摘要

该论文研究了从腐生葡萄球菌L-1获得的脲酶在有机硅表面的固定化。过程完成时间(4-5小时)和结合的最佳pH值(7-8)实际上与载体表面的化学性质无关。接枝到二氧化硅上的脲酶的比活性值不仅取决于酶-载体键的类型,还取决于大分子蛋白质与二氧化硅的距离。吸附在初始二氧化硅上后,保留的酶活性程度显示为26%。随着分离生物催化剂和载体的有机基团长度增加,该活性增长至100%。

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