Enzymatic biodegradable micro‐reactors for therapeutic applications

Rubio-Retama, Jorge; Tamimi, Faleh; López-Cabarcos, Enrique

doi:10.1002/jbm.b.30778

Cited by 2 publications

(1 citation statement)

References 29 publications

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“…In the past decades, enzyme immobilization methods have offered effective ways to overcome the limitations of free enzyme during enzymatic reaction, which provide strategies for obtaining rapid, highly sensitive, and high throughput digestion. A series of novel supports, such as silica , nanoparticles , capillaries , membranes , monoliths , and other surface anchored systems have been utilized in enzyme immobilization. Nowadays, exploration of the novel biocompatible surface for enzyme anchoring is an interesting topic for exerting good application of enzyme reactors in biosensing and biomedical field.…”

Section: Introductionmentioning

confidence: 99%

Microchip CE‐LIF method for the hydrolysis of L‐glutamine by using L‐asparaginase enzyme reactor based on gold nanoparticle

Qiao

Yan

et al. 2013

Electrophoresis

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L-Asparaginase (L-Asnase) can suppress the growth of malignant cells by rapid depletion of two essential amino acids, L-glutamine (L-Gln) and L-asparagine (L-Asn). To study the cytotoxic effect and the secondary complications of L-Asnase in the treatment of acute lymphoblastic leukemia, the development of a novel enzyme reactor of L-Asnase for the hydrolysis of L-Gln, employing the enzyme-gold nanoparticle conjugates in capillary, was reported in this work. First, a microchip CE (MCE)-LIF was established for the separation of L-amino acids (L-Gln and L-glutamic acid) and studying the hydrolysis of L-Gln by using L-Asnase enzyme reactor. Then, using L-Gln as target analyte, the enzyme kinetics of L-Asnase in free solution, enzyme-gold nanoparticle conjugates (E-GNP), and the enzyme-gold nanoparticle conjugates immobilized in capillary (E-GNP-C) were investigated in detail with the proposed MCE-LIF method. Moreover, for optimizing the enzymatic reaction efficiency, three important parameters, including the length of capillary, the enzyme concentration reacted with gold nanoparticle and the amount of L-Asnase immobilized on the gold nanoparticle, have been studied. Owing to the high specific activity, the E-GNP-C enzyme reactor exhibited the best performance for the hydrolysis of L-Gln.

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Section: Introductionmentioning

confidence: 99%

Microchip CE‐LIF method for the hydrolysis of L‐glutamine by using L‐asparaginase enzyme reactor based on gold nanoparticle

Qiao

Yan

et al. 2013

Electrophoresis

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Biocatalytic oxidation by chloroperoxidase from Caldariomyces fumago in polymersome nanoreactors

et al. 2009

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The encapsulation of chloroperoxidase from Caldariomyces fumago (CPO) in block copolymer polymersomes is reported. Fluorescence and electron microscopy show that when the encapsulating conditions favour self-assembly of the block copolymer, the enzyme is incorporated with concentrations that are 50 times higher than the enzyme concentration before encapsulation. The oxidation of two substrates by the encapsulated enzyme was studied: i) pyrogallol, a common substrate used to assay CPO enzymatic activity and ii) thioanisole, of which the product, (R)-methyl phenyl sulfoxide, is an important pharmaceutical intermediate. The CPO-loaded polymersomes showed distinct reactivity towards these substrates. While the oxidation of pyrogallol was limited by diffusion of the substrate into the polymersome, the rate-limiting step for the oxidation of thioansiole was the turnover by the enzyme.

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Enzymatic biodegradable micro‐reactors for therapeutic applications

Cited by 2 publications

References 29 publications

Microchip CE‐LIF method for the hydrolysis of L‐glutamine by using L‐asparaginase enzyme reactor based on gold nanoparticle

Microchip CE‐LIF method for the hydrolysis of L‐glutamine by using L‐asparaginase enzyme reactor based on gold nanoparticle

Biocatalytic oxidation by chloroperoxidase from Caldariomyces fumago in polymersome nanoreactors

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