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固定化产气荚膜梭菌神经氨酸酶。孵育过程中的底物裂解和酶释放。

Immobilized Clostridium perfringens neuraminidase. Substrate cleavage and enzyme release during incubation.

作者信息

Parker T L, Corfield A P, Veh R W, Schauer R

出版信息

Hoppe Seylers Z Physiol Chem. 1977 Jul;358(7):789-95. doi: 10.1515/bchm2.1977.358.2.789.

Abstract

Pure Clostridium perfringens neuraminidase was immobilized on Sepharose 4 B, azido-Sepharose 4 B and controlled pore glass (CPG)- glycophase using different coupling procedures. The immobilized enzyme showed increased stability under various conditions relative to the soluble enzyme. The low release of active enzyme from the supports under incubation conditions was quantitated using a highly sensitive radioactive assay. The activity of the immobilized enzyme was dependent on the nature of the support and the substrate. Activity decreased with increasing substrate molecular weight, but the enzyme showed improved cleavage with GD1a micelles and human erythrocytes, substrates having ordered surface properties. Uses of immobilized neuraminidase in biochemistry and cell biology are considered and evaluated relative to the measured release of enzyme from the supports reported and to the molecular size and organization of possible substrates.

摘要

采用不同的偶联方法,将纯产气荚膜梭菌神经氨酸酶固定在琼脂糖4B、叠氮琼脂糖4B和可控孔径玻璃(CPG)-糖相上。相对于可溶性酶,固定化酶在各种条件下表现出更高的稳定性。在孵育条件下,使用高灵敏度放射性测定法定量测定了活性酶从载体上的低释放量。固定化酶的活性取决于载体和底物的性质。活性随底物分子量的增加而降低,但该酶对具有有序表面性质的底物GD1a胶束和人红细胞表现出更好的切割效果。相对于所报道的酶从载体上的实测释放量以及可能底物的分子大小和组织情况,对固定化神经氨酸酶在生物化学和细胞生物学中的应用进行了考虑和评估。

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