4.8 Article

Decorating Self-Assembled Peptide Cages with Proteins

期刊

ACS NANO
卷 11, 期 8, 页码 7901-7914

出版社

AMER CHEMICAL SOC
DOI: 10.1021/acsnano.7b02368

关键词

coiled coil; nanoreactor; protein cage; protein design; self-assembly; supramolecular assembly; synthetic biology

资金

  1. GSK
  2. BBSRC [BB/L010518/1, BBM002969/1]
  3. ERC [340764]
  4. BBSRC South West Doctoral Training Partnership
  5. BrisSynBio, a BBSRC/EPSRC [BB/L01386X/1]
  6. Royal Society [WM140008]
  7. EPSRC [EP/K03927X/1]
  8. MRC
  9. Wolfson Foundation
  10. Biotechnology and Biological Sciences Research Council [BB/L010518/1, 1364038, BB/L014181/1, BB/L01386X/1] Funding Source: researchfish
  11. Engineering and Physical Sciences Research Council [EP/K03927X/1, EP/L000253/1, EP/M022609/1] Funding Source: researchfish
  12. Royal Society [WM140008] Funding Source: Royal Society
  13. BBSRC [BB/L01386X/1, BB/L010518/1, BB/L014181/1] Funding Source: UKRI
  14. EPSRC [EP/L000253/1, EP/M022609/1, EP/K03927X/1] Funding Source: UKRI

向作者/读者索取更多资源

An ability to organize and encapsulate multiple active proteins into defined objects and spaces at the nanoscale has potential applications in biotechnology, nanotechnology, and synthetic biology. Previously, we have described the design, assembly, and characterization of peptide-based self-assembled cages (SAGES). These approximate to 100 nm particles comprise thousands of copies of de novo designed peptide-based hubs that array into a hexagonal network and close to give caged structures. Here, we show that, when fused to the designed peptides, various natural proteins can be co-assembled into SAGE particles. We call these constructs pSAGE for protein-SAGE. These particles tolerate the incorporation of multiple copies of folded proteins fused to either the N or the C termini of the hubs, which modeling indicates form the external and internal surfaces of the particles, respectively. Up to 15% of the hubs can be functionalized without compromising the integrity of the pSAGEs. This corresponds to hundreds of copies giving mM local concentrations of protein in the particles. Moreover, and illustrating the modularity of the SAGE system, we show that multiple different proteins can be assembled simultaneously into the same particle. As the peptide protein fusions are made via recombinant expression of synthetic genes, we envisage that pSAGE systems could be developed modularly to actively encapsulate or to present a wide variety of functional proteins, allowing them to be developed as nanoreactors through the immobilization of enzyme cascades or as vehicles for presenting whole antigenic proteins as synthetic vaccine platforms.

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