Temperature-Responsive Mixed-Shell Polymeric Micelles for the Refolding of Thermally Denatured Proteins

We have fabricated a mixed‐shell polymeric micelle (MSPM) that closely mimics the natural molecular chaperone GroELGroES complex in terms of structure and functionality. This MSPM, which possesses a shared PLA core and a homogeneously mixed PEG and PNIAPM shell, is constructed through the co‐assemb...

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Bibliographic Details
Published in:Chemistry : a European journal 2013-06, Vol.19 (23), p.7437-7442
Main Authors: Liu, Xue, Liu, Yang, Zhang, Zhenkun, Huang, Fan, Tao, Qian, Ma, Rujiang, An, Yingli, Shi, Linqi
Format: Article
Language:English
Subjects:
Acrylic Resins - chemistry
Agglomeration
Chemistry
Cooling
core-shell structures
Dichroism
Diseases
Hydrophobic and Hydrophilic Interactions
Lactates - chemistry
Light scattering
Micelles
Molecular Chaperones - chemistry
Molecular structure
Polyethylene Glycols - chemistry
polymers
Polymers - chemistry
protein folding
Proteins
Proteins - chemistry
self-assembly
Solutions
Temperature
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Summary:We have fabricated a mixed‐shell polymeric micelle (MSPM) that closely mimics the natural molecular chaperone GroELGroES complex in terms of structure and functionality. This MSPM, which possesses a shared PLA core and a homogeneously mixed PEG and PNIAPM shell, is constructed through the co‐assembly of block copolymers poly(lactide‐b‐poly(ethylene oxide) (PLA‐b‐PEG) and poly(lactide)‐b‐poly(N‐isopropylacryamide) (PLA‐b‐PNIPAM). Above the lower critical solution temperature (LCST) of PNIPAM, the MSPM evolves into a core–shell–corona micelle (CSCM), as a functional state with hydrophobic PNIPAM domains on its surface. Light scattering (LS), TEM, and fluorescence and circular dichroism (CD) spectroscopy were performed to investigate the working mechanism of the chaperone‐like behavior of this system. Unfolded protein intermediates are captured by the hydrophobic PNIPAM domains of the CSCM, which prevent harmful protein aggregation. During cooling, PNIPAM reverts into its hydrophilic state, thereby inducing the release of the bound unfolded proteins. The refolding process of the released proteins is spontaneously accomplished by the presence of PEG in the mixed shell. Carbonic anhydrase B (CAB) was chosen as a model to investigate the refolding efficiency of the released proteins. In the presence of MSPM, almost 93 % CAB activity was recovered during cooling after complete denaturation at 70 °C. Further results reveal that this MSPM also works with a wide spectrum of proteins with more‐complicated structures, including some multimeric proteins. Given the convenience and generality in preventing the thermal aggregation of proteins, this MSPM‐based chaperone might be useful for preventing the toxic aggregation of misfolded proteins in some diseases. Heroes in a mixed shell: Core–shell–corona polymeric micelles with a temperature‐induced hydrophobic shell can act as an artificial chaperone in a process that involves the capture of thermally denatured proteins, thus preventing their aggregation, followed by assisted refolding during cooling (see figure).
ISSN:0947-6539
1521-3765
DOI:10.1002/chem.201300634