ABSTRACT
Recent advances in using biological scaffolds for nanoparticle synthesis have proven to be useful for preparing various nanostructures with uniform shape and size. Proteins are significant scaffolds for generating various nanostructures partly because of the presence of many functional groups to recognize different chemistries. In this endeavor, cocosin protein, an 11S allergen, is prepared from coconut fruit and employed as a potential scaffold for synthesizing Mn3O4 materials. The interaction between protein and manganese ions is studied in detail through isothermal calorimetric titration. At increased scaffold availability, the Mn3O4 material adopts the exact hexamer structure of the cocosin protein. The electrochemical supercapacitive properties of the cocosin-Mn3O4 material are found to have a high specific capacitance of 751.3 F g-1 at 1 A g-1 with cyclic stability (92% of capacitance retention after 5000 CV cycles) in a three-electrode configuration. The Mn3O4//Mn3O4 symmetric supercapacitor device delivers a specific capacitance of 203.8 F g-1 at 1 A g-1 and an outstanding energy and power density of 91.7 W h kg-1 and 899.5 W kg-1, respectively. These results show that cocosin-Mn3O4 could be considered a suitable electrode for energy storage applications. Moreover, the cocosin protein to be utilized as a novel scaffold in protein-nanomaterial chemistry could be useful for protein-assisted inorganic nanostructure synthesis in the future.
Subject(s)
Manganese Compounds , Oxides , Electric Capacitance , ElectrodesABSTRACT
BACKGROUND: The pesticidal properties of many Kunitz-type inhibitors have been reported previously; however, the mechanism of action is not well established. In this study, the activity of alocasin against Aedes aegypti is demonstrated and the structure-activity relationship of this Kunitz-type inhibitor is explained through X-ray structure analyses. RESULTS: Alocasin was purified from mature rhizomes of Alocasia as a single polypeptide chain of â¼ 20 kDa. The structure at 2.5 Å resolution revealed a Kunitz-type fold, but variation in the loop regions makes this structure unique; one loop with a single disulfide bridge is replaced by a long loop with two bridges. Alignment of homologous sequences revealed that this long loop contains a conserved Arg residue and modeling studies showed interaction with the catalytic Ser residue of trypsin-like enzymes. The anti-Aedes aegypti activity of alocasin is examined and discussed in detail. The in vitro activity of alocasin against midgut proteases of Aedes aegypti showed profound inhibition. Further, morphological changes in larvae upon treatment with alocasin revealed its activity against Ae. aegypti. Docking studies of alocasin with trypsin (5G1), a midgut protease involved in the development cycle and blood meal digestion, illustrated its insecticidal activity. CONCLUSION: The three-dimensional structure of alocasin was determined and its structure-function relationship established for its anti Ae. aegypti activity. © 2018 Society of Chemical Industry.
