Keisuke Iwahori scite author profile

Zinc selenide nanoparticles (ZnSe NPs) were synthesized in the cavity of the cage-shaped protein apoferritin by designing a slow chemical reaction system, which employs tetraaminezinc ion and selenourea. The chemical synthesis of ZnSe NPs was realized in a spatially selective manner from an aqueous solution, and ZnSe cores were formed in almost all apoferritin cavities with little bulk precipitation. Three factors are found to be important for ZnSe NP synthesis in the apoferritin cavity: (1) the threefold channel, which selectively introduces zinc ion into the apoferritin cavity, (2) the apoferritin internal potential, which favors zinc ion accumulation in the cavity, and (3) the nucleation site, which nucleates ZnSe inside the cavity. The characterization of the synthesized ZnSe NPs by X-ray powder diffraction and energy-dispersive spectrometry revealed that the synthesized NPs are a collection of cubic ZnSe polycrystals. It was shown that the 500 degrees C heat treatment for 1 h under nitrogen gas transformed the polycrystalline ZnSe core into a single crystal, and single-crystal ZnSe NPs free of protein were obtained.

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Fabrication of nickel and chromium nanoparticles using the protein cage of apoferritin

Okuda

Iwahori

Yamashita

et al. 2003

Biotech & Bioengineering

195

154

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The iron storage protein, apoferritin, has a cavity in which iron is oxidized and stored as a hydrated oxide core. The size of the core is about 7 nm in diameter and is regulated by the cavity size. The cavity can be utilized as a nanoreactor to grow inorganic crystals. We incubated apoferritin in nickel or chromium salt solutions to fabricate hydroxide nanoparticles in the cavity. By using a solution containing dissolved carbon dioxide and by precisely controlling the pH, we succeeded in fabricating nickel and chromium cores. During the hydroxylation process of nickel ions a large portion of the apoferritin precipitated through bulk precipitation of nickel hydroxide. Bulk precipitation was suppressed by adding ammonium ions. However, even in the presence of ammonium ions the core did not form using a degassed solution. We concluded that carbonate ions were indispensable for core formation and that the ammonium ions prevented precipitation in the bulk solution. The optimized condition for nickel core formation was 0.3 mg/mL horse spleen apoferritin and 5 mM ammonium nickel sulfate in water containing dissolved carbon dioxide. The pH was maintained at 8.65 using two buffer solutions: 150 mM HEPES (pH 7.5) and 195 mM CAPSO (pH 9.5) with 20 mM ammonium at 23 degrees C. The pH had not changed after 48 h. After 24 h of incubation, all apoferritins remained in the supernatant and all of them had cores. Recombinant L-ferritin showed less precipitation even above a pH of 8.65. A chromium core was formed under the following conditions: 0.1 mg/mL apoferritin, 1 mM ammonium chromium sulfate, 100 mM HEPES (pH 7.5) with a solution containing dissolved carbon dioxide. About 80% of the supernatant apoferritin (0.07 mg/mL) formed a core. In nickel and chromium core formation, carbonate ions would play an important role in accelerating the hydroxylation in the apoferritin cavity compared to the bulk solution outside.

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Ferritin in the field of nanodevices

Yamashita

Iwahori

Kumagai

2010

Biochimica et Biophysica Acta (BBA) - General Subjects

162

146

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Mechanism Underlying Specificity of Proteins Targeting Inorganic Materials

et al. 2006

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Adhesion force analysis using atomic force microscopy clearly revealed for the first time the mechanism underlying the specific binding between a titanium surface and ferritin possessing the sequence of Ti-binding peptide in its N-terminal domain. Our results proved that the specific binding is due to double electrostatic bonds between charged residue and surface groups of the substrate. Furthermore, it is also demonstrated that the accretion of surfactant reduces nonspecific interactions, dramatically enhancing the selectivity and specificity of Ti-binding peptide.

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Circularly Polarized Luminescent CdS Quantum Dots Prepared in a Protein Nanocage

et al. 2010

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Endowing a Ferritin‐Like Cage Protein with High Affinity and Selectivity for Certain Inorganic Materials

Sano

Ajima

Iwahori

et al. 2005

Small

118

114

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Enzymatic formation of manganese oxides by an Acremonium-like hyphomycete fungus, strain KR21-2

et al. 2004

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A Mn-depositing fungus, Acremonium-like hyphomycete strain KR21-2, was isolated from a Mn deposit occurring on the wall of a storage bottle containing Mn(III, IV) oxide-coated streambed pebbles and stream water. 18S rRNA gene sequence analysis revealed that strain KR21-2 was phylogenetically related to members of the order Hypocreales within the class Ascomycetes. The spent culture medium at the stationary phase of fungal growth contained a 54-kDa protein capable of depositing Mn oxides. The enzymatic activity was inhibited by azide and o-phenanthroline. The Mn(II)-oxidizing protein possessed a laccase activity, as indicated by direct oxidation of p-phenylenediamine and 2,2'-azinobis(3-ethylbenzothiazoline-6-sulfonic acid). These results are consistent with the role assumed for laccase-like multicopper oxidase, which is proposed to be involved in the Mn(II)-oxidizing factors from some bacteria. Unlike laccases of basidiomycete fungi, however, the protein of strain KR21-2 did not produce soluble Mn(III) species in the presence of either of the Mn chelators pyrophosphate and malonate. This is the first report on the possible involvement of laccase and/or multicopper oxidase in Mn oxide deposition by ascomycetes (including their anamorphs) ubiquitous in natural environments.

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Microbial manganese oxide formation and interaction with toxic metal ions

Miyata

Tani

Sakata

et al. 2007

Journal of Bioscience and Bioengineering

162

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Keisuke Iwahori

Fabrication of ZnSe Nanoparticles in the Apoferritin Cavity by Designing a Slow Chemical Reaction System

Fabrication of nickel and chromium nanoparticles using the protein cage of apoferritin

Ferritin in the field of nanodevices

Mechanism Underlying Specificity of Proteins Targeting Inorganic Materials

Circularly Polarized Luminescent CdS Quantum Dots Prepared in a Protein Nanocage

Endowing a Ferritin‐Like Cage Protein with High Affinity and Selectivity for Certain Inorganic Materials

Enzymatic formation of manganese oxides by an Acremonium-like hyphomycete fungus, strain KR21-2

Microbial manganese oxide formation and interaction with toxic metal ions

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