基本情報
- 所属
- 自治医科大学 医学部生理学講座 生物物理学部門 講師
- 学位
- 修士(理学)(神戸大学)博士(理学)(神戸大学)
- J-GLOBAL ID
- 201301098522794474
- researchmap会員ID
- 7000003898
経歴
4-
2022年11月 - 現在
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2018年4月 - 2022年10月
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2014年6月 - 2018年3月
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2010年4月 - 2014年6月
学歴
1-
- 2010年3月
論文
27-
Biochemical and Biophysical Research Communications 778 152343-152343 2025年9月
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Life 13(2) 318-318 2023年1月23日 査読有りIncoherent inelastic and quasi-elastic neutron scattering (INS) and terahertz time-domain spectroscopy (THz-TDS) are spectroscopy methods that directly detect molecular dynamics, with an overlap in the measured energy regions of each method. Due to the different characteristics of their probes (i.e., neutron and light), the information obtained and the sample conditions suitable for each method differ. In this review, we introduce the differences in the quantum beam properties of the two methods and their associated advantages and disadvantages in molecular spectroscopy. Neutrons are scattered via interaction with nuclei; one characteristic of neutron scattering is a large incoherent scattering cross-section of a hydrogen atom. INS records the auto-correlation functions of atomic positions. By using the difference in neutron scattering cross-sections of isotopes in multi-component systems, some molecules can be selectively observed. In contrast, THz-TDS observes the cross-correlation function of dipole moments. In water-containing biomolecular samples, the absorption of water molecules is particularly large. While INS requires large-scale experimental facilities, such as accelerators and nuclear reactors, THz-TDS can be performed at the laboratory level. In the analysis of water molecule dynamics, INS is primarily sensitive to translational diffusion motion, while THz-TDS observes rotational motion in the spectrum. The two techniques are complementary in many respects, and a combination of the two is very useful in analyzing the dynamics of biomolecules and hydration water.
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The Journal of Physical Chemistry B 126(51) 10797-10812 2022年12月29日
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Biophysics and Physicobiology 19 n/a-n/a 2022年9月8日
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Molecules (Basel, Switzerland) 27(13) 2022年6月21日Amyloid fibrils have been an important subject as they are involved in the development of many amyloidoses and neurodegenerative diseases. The formation of amyloid fibrils is typically initiated by nucleation, whereas its exact mechanisms are largely unknown. With this situation, we have previously identified prefibrillar aggregates in the formation of insulin B chain amyloid fibrils, which have provided an insight into the mechanisms of protein assembly involved in nucleation. Here, we have investigated the formation of insulin B chain amyloid fibrils under different pH conditions to better understand amyloid nucleation mediated by prefibrillar aggregates. The B chain showed strong propensity to form amyloid fibrils over a wide pH range, and prefibrillar aggregates were formed under all examined conditions. In particular, different structures of amyloid fibrils were found at pH 5.2 and pH 8.7, making it possible to compare different pathways. Detailed investigations at pH 5.2 in comparison with those at pH 8.7 have suggested that the evolution of protofibril-like aggregates is a common mechanism. In addition, different processes of evolution of the prefibrillar aggregates have also been identified, suggesting that the nucleation processes diversify depending on the polymorphism of amyloid fibrils.
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PLOS ONE 17(5) e0261699-e0261699 2022年5月5日 査読有りWe report expression and purification of a FLT3 protein with ITD mutation (FLT3-ITD) with a steady tyrosine kinase activity using a silkworm-baculovirus system, and its application as a fast screening system of tyrosine kinase inhibitors. The FLT3-ITD protein was expressed in Bombyx mori L. pupae infected by gene-modified nucleopolyhedrovirus, and was purified as an active state. We performed an inhibition assay using 17 kinase inhibitors, and succeeded in screening two inhibitors for FLT3-ITD. The result has paved the way for screening FLT3-ITD inhibitors in a fast and easy manner, and also for structural studies.
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Biophysics and Physicobiology 19 e190017 2022年 査読有り筆頭著者
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Biophysics and Physicobiology 18 284-288 2021年11月 査読有り筆頭著者
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生物物理 61(4) 236-239 2021年7月 査読有り招待有り筆頭著者
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The journal of physical chemistry letters 12(8) 2172-2176 2021年2月25日 査読有りHydration water plays a crucial role for activating the protein dynamics required for functional expression. Yet, the details are not understood about how hydration water couples with protein dynamics. A temperature hysteresis of the ice formation of hydration water is a key phenomenon to understand which type of hydration water, unfreezable or freezable hydration water, is crucial for the activation of protein dynamics. Using neutron scattering, we observed a temperature-hysteresis phenomenon in the diffraction peaks of the ice of freezable hydration water, whereas protein dynamics did not show any temperature hysteresis. These results show that the protein dynamics is not coupled with freezable hydration water dynamics, and unfreezable hydration water is essential for the activation of protein dynamics. Decoupling of the dynamics between unfreezable and freezable hydration water could be the cause of the distinct contributions of hydration water to protein dynamics.
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Biophysical Journal 120(2) 284-295 2020年12月 査読有りAmyloid fibrils are aberrant protein aggregates associated with various amyloidoses and neurodegenerative diseases. It is recently indicated that structural diversity of amyloid fibrils often results in different pathological phenotypes, including cytotoxicity and infectivity. The diverse structures are predicted to propagate by seed-dependent growth, which is one of the characteristic properties of amyloid fibrils. However, much remains unknown regarding how exactly the amyloid structures are inherited to subsequent generations by seeding reaction. Here, we investigated the behaviors of self- and cross-seeding of amyloid fibrils of human and bovine insulin in terms of thioflavin T fluorescence, morphology, secondary structure, and iodine staining. Insulin amyloid fibrils exhibited different structures, depending on species, each of which replicated in self-seeding. In contrast, gradual structural changes were observed in cross-seeding, and a new type of amyloid structure with distinct morphology and cytotoxicity was formed when human insulin was seeded with bovine insulin seeds. Remarkably, iodine staining tracked changes in amyloid structure sensitively, and singular value decomposition analysis of the ultraviolet-visible absorption spectra of the fibril-bound iodine has revealed the presence of one or more intermediate metastable states during the structural changes. From these findings, we propose a propagation scheme with multistep structural changes in cross-seeding between two heterologous proteins, which is accounted for as a consequence of the rugged energy landscape of amyloid formation.
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Scientific Reports 10(1) 16741-16741 2020年12月 査読有り<title>Abstract</title> It is recently suggested that amyloid polymorphism, i.e., structural diversity of amyloid fibrils, has a deep relationship with pathology. However, its prompt recognition is almost halted due to insufficiency of analytical methods for detecting polymorphism of amyloid fibrils sensitively and quickly. Here, we propose that iodine staining, a historically known reaction that was firstly found by Virchow, can be used as a method for distinguishing amyloid polymorphs. When insulin fibrils were prepared and iodine-stained, they exhibited different colors depending on polymorphs. Each of the colors was inherited to daughter fibrils by seeding reactions. The colors were fundamentally represented as a sum of three absorption bands in visible region between 400 and 750 nm, and the bands showed different titration curves against iodine, suggesting that there are three specific iodine binding sites. The analysis of resonance Raman spectra and polarization microscope suggested that several polyiodide ions composed of I3− and/or I5− were formed on the grooves or the edges of β-sheets. It was concluded that the polyiodide species and conformations formed are sensitive to surface structure of amyloid fibrils, and the resultant differences in color will be useful for detecting polymorphism in a wide range of diagnostic samples.
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The European Physical Journal E 42(10) 2019年10月
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Biochemistry 58(24) 2769-2781 2019年3月 査読有り
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Scientific Reports 8(1) 62 2018年12月1日 査読有り
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Biophysical Reviews 10(2) 527-534 2018年4月1日 査読有り
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Journal of Physical Chemistry B 122(4) 1367-1377 2018年2月1日 査読有り
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LANGMUIR 33(33) 8311-8318 2017年8月 査読有り
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JOURNAL OF PHYSICAL CHEMISTRY B 120(21) 4743-4755 2016年6月 査読有り
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JOURNAL OF PHYSICAL CHEMISTRY B 119(29) 9359-9368 2015年7月 査読有り招待有り
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BIOMACROMOLECULES 15(2) 512-523 2014年2月 査読有り
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JOURNAL OF INFRARED MILLIMETER AND TERAHERTZ WAVES 35(1) 147-157 2014年1月 査読有り
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JOURNAL OF BIOLOGICAL CHEMISTRY 285(29) 22696-22705 2010年7月 査読有り
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PEPTIDES 31(5) 794-805 2010年5月 査読有り
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BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS 369(2) 609-615 2008年5月 査読有り
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BIOCHEMICAL AND BIOPHYSICAL RESEARCH COMMUNICATIONS 369(2) 327-332 2008年5月 査読有り
MISC
5-
日本生物工学会大会講演要旨集 20 167-167 2008年
書籍等出版物
5-
Proceedings of 3rd International THz-Bio Workshop 2012年
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Proceedings of the conference IRMMW-THz 2011 2011年
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Proceedings of the conference IRMMW-THz 2011 2011年
講演・口頭発表等
40担当経験のある科目(授業)
2-
2019年9月 - 現在疾病関連タンパク質概論 (自治医科大学)
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2014年4月 - 2018年3月有機化学II (神戸大学)
共同研究・競争的資金等の研究課題
4-
日本学術振興会 科学研究費助成事業 2022年4月 - 2025年3月
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日本学術振興会 科学研究費助成事業 2018年4月 - 2021年3月
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日本学術振興会 科学研究費助成事業 2016年4月 - 2020年3月
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日本学術振興会 科学研究費助成事業 2016年4月 - 2018年3月