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Dive into the research topics where Hideya Tanaka is active.

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Featured researches published by Hideya Tanaka.


Food Additives and Contaminants Part A-chemistry Analysis Control Exposure & Risk Assessment | 2006

Determination of genotoxic phenylhydrazine agaritine in mushrooms using liquid chromatography–electrospray ionization tandem mass spectrometry

Kazunari Kondo; Asako Watanabe; Yuko Iwanaga; Ikuro Abe; Hideya Tanaka; Megumi Hamano Nagaoka; Hiroshi Akiyama; Tamio Maitani

A new method with good sensitivity and specificity for detecting and quantifying genotoxic hydrazines, agaritine and 4-(hydroxymethyl)phenylhydrazine (HMPH), was developed using liquid chromatography–electrospray tandem mass spectrometry (MS). Synthetic agaritine and HMPH were structurally assigned by 1H-, 13C- and two-dimensional nuclear magnetic resonance (NMR) analysis (HMBC and HMQC), high-resolution fast-atom bombardment (HR-FAB) MS and time of flight (TOF) MS. The polar molecule agaritine was separated on an ODS column using 0.01% AcOH–MeOH (99:1, v/v) as an eluent with a simple solid-phase extraction cleanup. There were no interference peaks for any of the mushrooms. Agaricus spp. contained 1247 and 2017 µg g−1 agaritine. Other species of mushroom had no agaritine. Recoveries of agaritine from spiked mushroom samples were 60.3–114%. Intra-day precision values were 5.5 and 4.2%, and the inter-day precision values were acceptable (15.0 and 23.0%), as agaritine is unstable. The limit of quantification was 0.003 µg g−1. Even a trace amount of agaritine in mushrooms can, therefore, be determined using this method. We also directly analysed HMPH, an active free hydrazine form of genotoxic agaritine, and obtained direct evidence of its absence from mushrooms. A precursor ion scan confirmed that agaritine derivatives, which could exert similar toxicity, were absent. The results indicate that this specific and sensitive analytical method for detecting and quantifying agaritine and its derivatives could help evaluate the risk of mushroom hydrazines to humans.


Journal of the American Chemical Society | 2002

Enzymatic Formation of an Unnatural Hexacyclic C35 Polyprenoid by Bacterial Squalene Cyclase

Ikuro Abe; Hideya Tanaka; Hiroshi Noguchi


Organic Letters | 2005

Enzymatic formation of indole-containing unnatural cyclic polyprenoids by bacterial squalene:hopene cyclase.

Hideya Tanaka; Hiroshi Noguchi; Ikuro Abe


Organic Letters | 2004

1-methylidenesqualene and 25-methylidenesqualene as active-site probes for bacterial squalene:hopene cyclase.

Hideya Tanaka; Hiroshi Noguchi; Ikuro Abe


Journal of the American Chemical Society | 2004

Mechanism and stereochemistry of enzymatic cyclization of 24, 30-bisnor-2, 3-oxidosqualene by recombinant β-amyrin synthase

Ikuro Abe; Yuichi Sakano; Megumi Sodeyama; Hideya Tanaka; Hiroshi Noguchi; Masaaki Shibuya; Yutaka Ebizuka


Biochemical and Biophysical Research Communications | 2007

Enzymatic formation of unnatural cytokinin analogs by adenylate isopentenyltransferase from mulberry.

Ikuro Abe; Hideya Tanaka; Tsuyoshi Abe; Hiroshi Noguchi


Tetrahedron Letters | 2006

Enzymatic formation of pyrrole-containing novel cyclic polyprenoids by bacterial squalene:hopene cyclase

Hideya Tanaka; Hisashi Noma; Hiroshi Noguchi; Ikuro Abe


Tetrahedron Letters | 2004

Enzymatic cyclization of 26- and 27-methylidenesqualene to novel unnatural C31 polyprenoids by squalene:hopene cyclase☆

Hideya Tanaka; Hiroshi Noguchi; Ikuro Abe


Tetrahedron Letters | 2004

Enzymatic formation of an unnatural novel tetracyclic sesterterpene by β-amyrin synthase

Hisashi Noma; Hideya Tanaka; Hiroshi Noguchi; Masaaki Shibuya; Yutaka Ebizuka; Ikuro Abe


Journal of Chromatography B | 2006

Analysis of agaritine in mushrooms and in agaritine-administered mice using liquid chromatography-tandem mass spectrometry.

Kazunari Kondo; Asako Watanabe; Yuko Iwanaga; Ikuro Abe; Hideya Tanaka; Megumi Hamano Nagaoka; Hiroshi Akiyama; Tamio Maitani

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