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Dive into the research topics where Satoshi Akanuma is active.

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Featured researches published by Satoshi Akanuma.


Proceedings of the National Academy of Sciences of the United States of America | 2013

Experimental evidence for the thermophilicity of ancestral life

Satoshi Akanuma; Yoshiki Nakajima; Shin-ichi Yokobori; Mitsuo Kimura; Naoki Nemoto; Tomoko Mase; Ken Ichi Miyazono; Masaru Tanokura; Akihiko Yamagishi

Theoretical studies have focused on the environmental temperature of the universal common ancestor of life with conflicting conclusions. Here we provide experimental support for the existence of a thermophilic universal common ancestor. We present the thermal stabilities and catalytic efficiencies of nucleoside diphosphate kinases (NDK), designed using the information contained in predictive phylogenetic trees, that seem to represent the last common ancestors of Archaea and of Bacteria. These enzymes display extreme thermal stabilities, suggesting thermophilic ancestries for Archaea and Bacteria. The results are robust to the uncertainties associated with the sequence predictions and to the tree topologies used to infer the ancestral sequences. Moreover, mutagenesis experiments suggest that the universal ancestor also possessed a very thermostable NDK. Because, as we show, the stability of an NDK is directly related to the environmental temperature of its host organism, our results indicate that the last common ancestor of extant life was a thermophile that flourished at a very high temperature.


Proceedings of the National Academy of Sciences of the United States of America | 2002

Combinatorial mutagenesis to restrict amino acid usage in an enzyme to a reduced set

Satoshi Akanuma; Takanori Kigawa; Shigeyuki Yokoyama

We developed an effective strategy to restrict the amino acid usage in a relatively large protein to a reduced set with conservation of its in vivo function. The 213-residue Escherichia coli orotate phosphoribosyltransferase was subjected to 22 cycles of segment-wise combinatorial mutagenesis followed by 6 cycles of site-directed random mutagenesis, both coupled with a growth-related phenotype selection. The enzyme eventually tolerated 73 amino acid substitutions: In the final variant, 9 amino acid types (A, D, G, L, P, R, T, V, and Y) occupied 188 positions (88%), and none of 7 amino acid types (C, H, I, M, N, Q, and W) appeared. Therefore, the catalytic function associated with a relatively large protein may be achieved with a subset of the 20 amino acid. The converged sequence also implies simpler constituents for proteins in the early stage of evolution.


Analytical Biochemistry | 2008

Methods for reducing nonspecific interaction in antibody-antigen assay via atomic force microscopy

Jun’ichi Wakayama; Hiroshi Sekiguchi; Satoshi Akanuma; Toshio Ohtani; Shigeru Sugiyama

We developed a method to measure the rupture forces between antibody and antigen by atomic force microscopy (AFM). Previous studies have reported that in the measurement of antibody-antigen interaction using AFM, the specific intermolecular forces are often obscured by nonspecific adhesive binding forces between antibody immobilized cantilever and substrate surfaces on which antigen or nonantigen are fixed. Here, we examined whether detergent and nonreactive protein, which have been widely used to reduce nonspecific background signals in ordinary immunoassay and immunoblotting, could reduce the nonspecific forces in the AFM measurement. The results showed that, in the presence of both nonreactive protein and detergent, the rupture forces between anti-ferritin antibodies immobilized on a tip of cantilever and ferritin (antigen) on the substrate could be successfully measured, distinguishing from nonspecific adhesive forces. In addition, we found that approach/retraction velocity of the AFM cantilever was also important in the reduction of nonspecific adhesion. These insights will contribute to the detection of specific molecules at nanometer scale region and the investigation of intermolecular interaction by the use of AFM.


Journal of Biochemistry | 2010

Mimicking the evolution of a thermally stable monomeric four-helix bundle by fusion of four identical single-helix peptides

Satoshi Akanuma; Taku Matsuba; Emi Ueno; Naoki Umeda; Akihiko Yamagishi

Internal symmetry is a common feature of the tertiary structures of proteins and protein domains. Probably, because the genes of homo-oligomeric proteins duplicated and fused, their evolutionary descendants are proteins with internal symmetry. To identify any advantages that cause monomeric proteins with internal symmetry to be selected evolutionarily, we characterized some of the physical properties of a recombinant protein with a sequence consisting of two tandemly fused copies of the Escherichia coli Lac repressor C-terminal alpha-helix. This polypeptide exists in solution mainly as dimer that likely maintains a four-helix bundle motif. Thermal unfolding experiments demonstrate that the protein is considerably more stable at elevated temperatures than is a homotetramer consisting of four non-covalently associated copies of a 21-residue polypeptide similar in sequence to that of the Lac repressor C-terminal alpha-helix. A tandem duplication of our helix-loop-helix polypeptide yields an even more thermally stable protein. Our results exemplify the concept that fusion of non-covalently assembled polypeptide chains leads to enhanced protein stability. Herein, we discuss how our work relates to the evolutionary selective-advantages realized when symmetrical homo-oligomers evolve into monomers. Moreover, our thermally stable single-chain four-helix bundle protein may provide a robust scaffold for development of new biomaterials.


FEBS Letters | 1997

Effect of polar side chains at position 172 on thermal stability of 3- isopropylmalate dehydrogenase from Thermus thermophilus

Satoshi Akanuma; Chunxu Qu; Akihiko Yamagishi; Nobuo Tanaka; Tairo Oshima

To understand the role of the amino acid residue at position 172 in the conformational stability, four mutant enzymes of Thermus thermophilus 3‐isopropylmalate dehydrogenase in which Ala172 was replaced with Asp, Glu, Asn, and Gln were prepared by site‐directed mutagenesis. Three mutants were more stable than the wild‐type enzyme. No significant change in catalytic properties was found in the mutant enzymes. The molecular modeling studies suggested that the enhanced thermostability of the mutant enzymes resulted from the formation of extra electrostatic interactions and/or improvement of hydrophobic packing of the interior core.


Evolution | 2015

Robustness of predictions of extremely thermally stable proteins in ancient organisms

Satoshi Akanuma; Shin-ichi Yokobori; Yoshiki Nakajima; Mizumo Bessho; Akihiko Yamagishi

A number of studies have addressed the environmental temperatures experienced by ancient life. Computational studies using a nonhomogeneous evolution model have estimated ancestral G + C contents of ribosomal RNAs and the amino acid compositions of ancestral proteins, generating hypotheses regarding the mesophilic last universal common ancestor. In contrast, our previous study computationally reconstructed ancestral amino acid sequences of nucleoside diphosphate kinases using a homogeneous model and then empirically resurrected the ancestral proteins. The thermal stabilities of these ancestral proteins were equivalent to or greater than those of extant homologous thermophilic proteins, supporting the thermophilic universal ancestor theory. In this study, we reinferred ancestral sequences using a dataset from which hyperthermophilic sequences were excluded. We also reinferred ancestral sequences using a nonhomogeneous evolution model. The newly reconstructed ancestral proteins are still thermally stable, further supporting the hypothesis that the ancient organisms contained thermally stable proteins and therefore that they were thermophilic.


PLOS ONE | 2014

Preparation of Phi29 DNA Polymerase Free of Amplifiable DNA Using Ethidium Monoazide, an Ultraviolet-Free Light-Emitting Diode Lamp and Trehalose

Hirokazu Takahashi; Hiroyuki Yamazaki; Satoshi Akanuma; Hiroko Kanahara; Toshiyuki Saito; Tomoyuki Chimuro; Takayoshi Kobayashi; Toshio Ohtani; Kimiko Yamamoto; Shigeru Sugiyama; Toshiro Kobori

We previously reported that multiply-primed rolling circle amplification (MRPCA) using modified random RNA primers can amplify tiny amounts of circular DNA without producing any byproducts. However, contaminating DNA in recombinant Phi29 DNA polymerase adversely affects the outcome of MPRCA, especially for negative controls such as non-template controls. The amplified DNA in negative control casts doubt on the result of DNA amplification. Since Phi29 DNA polymerase has high affinity for both single-strand and double-stranded DNA, some amount of host DNA will always remain in the recombinant polymerase. Here we describe a procedure for preparing Phi29 DNA polymerase which is essentially free of amplifiable DNA. This procedure is realized by a combination of host DNA removal using appropriate salt concentrations, inactivation of amplifiable DNA using ethidium monoazide, and irradiation with visible light from a light-emitting diode lamp. Any remaining DNA, which likely exists as oligonucleotides captured by the Phi29 DNA polymerase, is degraded by the 3′-5′ exonuclease activity of the polymerase itself in the presence of trehalose, used as an anti-aggregation reagent. Phi29 DNA polymerase purified by this procedure has little amplifiable DNA, resulting in reproducible amplification of at least ten copies of plasmid DNA without any byproducts and reducing reaction volume. This procedure could aid the amplification of tiny amounts DNA, thereby providing clear evidence of contamination from laboratory environments, tools and reagents.


Proteins | 2004

A detailed unfolding pathway of a (β/α)8‐barrel protein as studied by molecular dynamics simulations

Satoshi Akanuma; Hiroh Miyagawa; Kunihiro Kitamura; Akihiko Yamagishi

The (β/α)8‐barrel is the most common protein fold. Similar structural properties for folding intermediates of (β/α)8‐barrel proteins involved in tryptophan biosynthesis have been reported in a number of experimental studies; these intermediates have the last two β‐strands and three α‐helices partially unfolded, with other regions of the polypeptide chain native‐like in conformation. To investigate the detailed folding/unfolding pathways of these (β/α)8‐barrel proteins, temperature‐induced unfolding simulations of N‐(5′‐phosphoribosyl)anthranilate isomerase from Escherichia coli were carried out using a special‐purpose parallel computer system. Unfolding simulations at five different temperatures showed a sequential unfolding pathway comprised of several events. Early events in unfolding involved disruption of the last two strands and three helices, producing an intermediate ensemble similar to those detected in experimental studies. Then, denaturation of the first two βα units and separation of the sixth strand from the fifth took place independently. The remaining central βαβαβ module persisted the longest during all simulations, suggesting an important role for this module as the incipient folding scaffold. Our simulations also predicted the presence of a nucleation site, onto which several hydrophobic residues condensed forming the foundation for the central βαβαβ module. Proteins 2005.


Proceedings of the National Academy of Sciences of the United States of America | 2017

Reconstructed ancestral enzymes suggest long-Term cooling of Earth's photic zone since the Archean

Amanda K. Garcia; J. William Schopf; Shin-ichi Yokobori; Satoshi Akanuma; Akihiko Yamagishi

Significance Geological evidence suggesting that Earths oceans cooled from ∼55–85 °C in the Archean (∼3,500 Ma) to the present has met with skepticism due to possible geochemical alteration of the rocks analyzed and uncertainties about their depositional environment. Determination of the thermostability of experimentally reconstructed ancestral enzymes provides independent means to assess paleotemperature. Because some previously analyzed taxa may have inhabited atypically high-temperature environments (e.g., deep-sea hydrothermal vents), we have restricted our analyses to ancestral enzymes reconstructed from photic-zone cyanobacteria and land plants. Our findings indicate a cooling of Earths surface temperature from ∼75 °C in the Archean (∼3,000 Ma) to ∼35 °C in the Devonian (∼420 Ma), consistent with previous geological and enzyme-based results. Paleotemperatures inferred from the isotopic compositions (δ18O and δ30Si) of marine cherts suggest that Earth’s oceans cooled from 70 ± 15 °C in the Archean to the present ∼15 °C. This interpretation, however, has been subject to question due to uncertainties regarding oceanic isotopic compositions, diagenetic or metamorphic resetting of the isotopic record, and depositional environments. Analyses of the thermostability of reconstructed ancestral enzymes provide an independent method by which to assess the temperature history inferred from the isotopic evidence. Although previous studies have demonstrated extreme thermostability in reconstructed archaeal and bacterial proteins compatible with a hot early Earth, taxa investigated may have inhabited local thermal environments that differed significantly from average surface conditions. We here present thermostability measurements of reconstructed ancestral enzymatically active nucleoside diphosphate kinases (NDKs) derived from light-requiring prokaryotic and eukaryotic phototrophs having widely separated fossil-based divergence ages. The ancestral environmental temperatures thereby determined for these photic-zone organisms––shown in modern taxa to correlate strongly with NDK thermostability––are inferred to reflect ancient surface-environment paleotemperatures. Our results suggest that Earths surface temperature decreased over geological time from ∼65–80 °C in the Archean, a finding consistent both with previous isotope-based and protein reconstruction-based interpretations. Interdisciplinary studies such as those reported here integrating genomic, geologic, and paleontologic data hold promise for providing new insight into the coevolution of life and environment over Earth history.


Biochemistry | 2011

Substitutions of coenzyme-binding, nonpolar residues improve the low-temperature activity of thermophilic dehydrogenases

Sayaka Hayashi; Satoshi Akanuma; Wakana Onuki; Chihiro Tokunaga; Akihiko Yamagishi

Although enzymes of thermophilic organisms are often very resistant to thermal denaturation, they are usually less active than their mesophilic or psychrophilic homologues at moderate or low temperatures. To explore the structural features that would improve the activity of a thermophilic enzyme at less than optimal temperatures, we randomly mutated the DNA of single-site mutants of the thermostable Thermus thermophilus 3-isopropylmalate dehydrogenase that already had improved low-temperature activity and selected for additional improved low-temperature activity. A mutant (Ile279 → Val) with improved low-temperature activity contained a residue that directly interacts with the adenine of the coenzyme NAD(+), suggesting that modulation of the coenzyme-binding pockets volume can enhance low-temperature activity. This idea was further supported by a saturation mutagenesis study of the two codons of two other residues that interact with the adenine. Furthermore, a similar type of amino acid substitution also improved the catalytic efficiency of another thermophilic dehydrogenase, T. thermophilus lactate dehydrogenase. Steady-state kinetic experiments showed that the mutations all favorably affected the catalytic turnover numbers. Thermal stability measurements demonstrated that the mutants remain very resistant to heat. Calculation of the energetic contributions to catalysis indicated that the increased turnover numbers are the result of destabilized enzyme-substrate-coenzyme complexes. Therefore, small changes in the side chain volumes of coenzyme-binding residues improved the catalytic efficiencies of two thermophilic dehydrogenases while preserving their high thermal stabilities and may be a way to improve low-temperature activities of dehydrogenases in general.

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Akihiko Yamagishi

Tokyo University of Pharmacy and Life Sciences

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Shin-ichi Yokobori

Tokyo University of Pharmacy and Life Sciences

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Masako Takasu

Tokyo University of Pharmacy and Life Sciences

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Yoshiki Nakajima

Tokyo University of Pharmacy and Life Sciences

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Masaki Fukuda

Tokyo University of Pharmacy and Life Sciences

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Sota Yagi

Tokyo University of Pharmacy and Life Sciences

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Hironao Yamada

Tokyo University of Pharmacy and Life Sciences

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