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Preserving catalytic activity and enhancing biochemical stability of the therapeutic enzyme asparaginase by biocompatible multilayered polyelectrolyte microcapsules

(2013) BIOMACROMOLECULES. 14(12). p.4398-4406
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Center for nano- and biophotonics (NB-Photonics)
Abstract
The present study focuses on the formation of microcapsules containing catalytically active L-asparaginase (L-ASNase), a protein drug of high value in antileukemic therapy. We make use of the layer-by-layer (LbL) technique to coat protein-loaded calcium carbonate (CaCO3) particles with two or three poly dextran/poly-L-arginine-based bilayers. To achieve high loading efficiency, the CaCO3 template was generated by coprecipitation with the enzyme. After assembly of the polymer shell, the CaCO3 core material was dissolved under mild conditions by dialysis against 20 mM EDTA. Biochemical stability of the encapsulated L-asparaginase was analyzed by treating the capsules with the proteases trypsin and thrombin, which are known to degrade and inactivate the enzyme during leukemia treatment, allowing us to test for resistance against proteolysis by physiologically relevant proteases through measurement of residual L-asparaginase activities. In addition, the thermal stability, the stability at the physiological temperature, and the long-term storage stability of the encapsulated enzyme were investigated. We show that encapsulation of L-asparaginase remarkably improves both proteolytic resistance and thermal inactivation at 37 degrees C, which could considerably prolong the enzyme's in vivo half-life during application in acute lymphoblastic leukemia (ALL). Importantly, the use of low EDTA concentrations for the dissolution of CaCO3 by dialysis could be a general approach in cases where the activity of sensitive biomacromolecules is inhibited, or even irreversibly damaged, when standard protocols for fabrication of such LbL microcapsules are used. Encapsulated and free enzyme showed similar efficacies in driving leukemic cells to apoptosis.
Keywords
capsules, enzymes, leukemia, capsules, calcium carbonate, polymers, ACUTE LYMPHOBLASTIC-LEUKEMIA, PROTEIN ENCAPSULATION, CHILDREN, MICROPARTICLES, CAPSULES, STABILIZATION, RESISTANCE, PARTICLES, REMISSION, IMPROVE

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Citation

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Chicago
Karamitros, Christos S, Alexey M Yashchenok, Helmuth Möhwald, Andre Skirtach, and Manfred Konrad. 2013. “Preserving Catalytic Activity and Enhancing Biochemical Stability of the Therapeutic Enzyme Asparaginase by Biocompatible Multilayered Polyelectrolyte Microcapsules.” Biomacromolecules 14 (12): 4398–4406.
APA
Karamitros, C. S., Yashchenok, A. M., Möhwald, H., Skirtach, A., & Konrad, M. (2013). Preserving catalytic activity and enhancing biochemical stability of the therapeutic enzyme asparaginase by biocompatible multilayered polyelectrolyte microcapsules. BIOMACROMOLECULES, 14(12), 4398–4406.
Vancouver
1.
Karamitros CS, Yashchenok AM, Möhwald H, Skirtach A, Konrad M. Preserving catalytic activity and enhancing biochemical stability of the therapeutic enzyme asparaginase by biocompatible multilayered polyelectrolyte microcapsules. BIOMACROMOLECULES. 2013;14(12):4398–406.
MLA
Karamitros, Christos S, Alexey M Yashchenok, Helmuth Möhwald, et al. “Preserving Catalytic Activity and Enhancing Biochemical Stability of the Therapeutic Enzyme Asparaginase by Biocompatible Multilayered Polyelectrolyte Microcapsules.” BIOMACROMOLECULES 14.12 (2013): 4398–4406. Print.
@article{4285403,
  abstract     = {The present study focuses on the formation of microcapsules containing catalytically active L-asparaginase (L-ASNase), a protein drug of high value in antileukemic therapy. We make use of the layer-by-layer (LbL) technique to coat protein-loaded calcium carbonate (CaCO3) particles with two or three poly dextran/poly-L-arginine-based bilayers. To achieve high loading efficiency, the CaCO3 template was generated by coprecipitation with the enzyme. After assembly of the polymer shell, the CaCO3 core material was dissolved under mild conditions by dialysis against 20 mM EDTA. Biochemical stability of the encapsulated L-asparaginase was analyzed by treating the capsules with the proteases trypsin and thrombin, which are known to degrade and inactivate the enzyme during leukemia treatment, allowing us to test for resistance against proteolysis by physiologically relevant proteases through measurement of residual L-asparaginase activities. In addition, the thermal stability, the stability at the physiological temperature, and the long-term storage stability of the encapsulated enzyme were investigated. We show that encapsulation of L-asparaginase remarkably improves both proteolytic resistance and thermal inactivation at 37 degrees C, which could considerably prolong the enzyme's in vivo half-life during application in acute lymphoblastic leukemia (ALL). Importantly, the use of low EDTA concentrations for the dissolution of CaCO3 by dialysis could be a general approach in cases where the activity of sensitive biomacromolecules is inhibited, or even irreversibly damaged, when standard protocols for fabrication of such LbL microcapsules are used. Encapsulated and free enzyme showed similar efficacies in driving leukemic cells to apoptosis.},
  author       = {Karamitros, Christos S and Yashchenok, Alexey M and Möhwald, Helmuth and Skirtach, Andre and Konrad, Manfred},
  issn         = {1525-7797},
  journal      = {BIOMACROMOLECULES},
  keywords     = {capsules,enzymes,leukemia,capsules,calcium carbonate,polymers,ACUTE LYMPHOBLASTIC-LEUKEMIA,PROTEIN ENCAPSULATION,CHILDREN,MICROPARTICLES,CAPSULES,STABILIZATION,RESISTANCE,PARTICLES,REMISSION,IMPROVE},
  language     = {eng},
  number       = {12},
  pages        = {4398--4406},
  title        = {Preserving catalytic activity and enhancing biochemical stability of the therapeutic enzyme asparaginase by biocompatible multilayered polyelectrolyte microcapsules},
  url          = {http://dx.doi.org/10.1021/bm401341k},
  volume       = {14},
  year         = {2013},
}

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