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β-葡萄糖苷酶固定化设计与合成稀有人参皂苷的研究
Abstract
Study of β- glucosidase immobilized design and synthesis of rare
ginsenosides
β-glucosidase (Tnap0602) derived from Thermotoga Naphthophila RUK-10 can
efficiently transform ginsenoside Rb1 to form rare ginsenoside Rd. In this paper, a
novel β-glucosidase (Carbamate-binding module) The method of immobilization was
used to study the immobilization method of heteroenzyme, which laid the foundation
for the application of β-glucosidase.
In this paper, two engineered bacteria capable of expressing the fusion proteins
0602-CBM2 and 0602-CBM3 were constructed and the target protein was purified.
The purified protein was adsorbed to microcrystalline cellulose, regenerated
amorphous cellulose and filter paper pulp, respectively. The preliminary
immobilization of β-glucosidase was achieved and the ginsenoside conversion
experiment was carried out. The results showed that the maximum binding capacity of
microcrystalline cellulose of recombinant enzyme 0602-CBM2 was 2mg / ml, while
0602-CBM3 did not bind to microcrystalline cellulose, regenerated amorphous
cellulose and filter paper pulp. The results showed that the immobilized β-glucosidase
could be used in the re-use of immobilized enzyme, and the activity of immobilized
β-glucosidase could be improved after the repeated use of immobilized enzyme
0602-CBM2 for three times , The HPLC assay showed that a single product peak was
evident at 35 minutes compared to the extract without the enzyme.
Keywords:
β-glucosidase, cellulose-binding modules, immobilization, ginsenoside
II
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