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Dive into the research topics where Haruyuki Iefuji is active.

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Featured researches published by Haruyuki Iefuji.


Enzyme and Microbial Technology | 2013

Fusion of cellulose binding domain from Trichoderma reesei CBHI to Cryptococcus sp. S-2 cellulase enhances its binding affinity and its cellulolytic activity to insoluble cellulosic substrates

Jantaporn Thongekkaew; Hiroko Ikeda; Kazuo Masaki; Haruyuki Iefuji

Cryptococcus sp. S-2 carboxymethyl cellulase (CSCMCase) is active in the acidic pH and lacks a binding domain. The absence of the binding domain makes the enzyme inefficient against insoluble cellulosic substrates. To enhance its binding affinity and its cellulolytic activity to insoluble cellulosic substrates, cellulose binding domain (CBD) of cellobiohydrolase I (CBHI) from Trichoderma reesei belonging to carbohydrate binding module (CBM) family 1 was fused at the C-terminus of CSCMCase. The constructed fusion enzymes (CSCMCase-CBD and CSCMCase-2CBD) were expressed in a newly recombinant expression system of Cryptococcus sp. S-2, purified to homogeneity, and then subject to detailed characterization. The recombinant fusion enzymes displayed optimal pH similar to those of the native enzyme. Compared with rCSCMCase, the recombinant fusion enzymes had acquired an increased binding affinity to insoluble cellulose and the cellulolytic activity toward insoluble cellulosic substrates (SIGMACELL(®) and Avicel) was higher than that of native enzyme, confirming the presence of CBDs improve the binding and the cellulolytic activity of CSCMCase on insoluble substrates. This attribute should make CSCMCase an attractive applicant for various application.


Applied Microbiology and Biotechnology | 2014

Heterologous production of horseradish peroxidase C1a by the basidiomycete yeast Cryptococcus sp. S-2 using codon and signal optimizations.

Yuu Utashima; Hirotaka Matsumoto; Kazuo Masaki; Haruyuki Iefuji

In the present study, we attempted to improve the production of recombinant horseradish peroxidase C1a (HRP-C1a; a heme-binding protein) by Cryptococcus sp. S-2. Both native and codon-optimized HRP-C1a genes were expressed under the control of a high-level expression promoter. When the HRP-C1a gene with native codons was expressed, poly(A) tails tended to be added within the coding region, producing truncated messenger RNAs (mRNAs) that lacked the 3′ ends. Codon optimization prevented polyadenylation within the coding region and increased both the mRNA and protein levels of active HRP-C1a. To improve secretion of the recombinant protein, we tested five types of N-terminal signal peptide (NTP). These included the native HRP-C1a NTP (C1a-NTP), short and long xylanase secretion signals (X1-NTP and X2-NTP), cutinase signal (C-NTP), and amylase signal (A-NTP), with and without a C-terminal propeptide (CTP). X2-NTP without CTP resulted in the highest HRP-C1a secretion into the culture medium. HRP-C1a secretion was further increased by using xylose fed-batch fermentation. The production of HRP-C1a in this study was 2.7 and 15 times higher than the production reported in previous studies that used insect cell and Pichia expression systems, respectively.


Applied Microbiology and Biotechnology | 2017

A genetic method to enhance the accumulation of S-adenosylmethionine in yeast

Muneyoshi Kanai; Masaki Mizunuma; Tsutomu Fujii; Haruyuki Iefuji

S-Adenosylmethionine (SAM) is a key component of sulphur amino acid metabolism in living organisms and is synthesised from methionine and adenosine triphosphate by methionine adenosyltransferase. This molecule serves as the main biological methyl donor due to its active methylthio ether group. Notably, SAM has shown beneficial effects in clinical trials for the treatment of alcoholic liver disease, depression and joint pain. Due to the high potential value of SAM, current research efforts are attempting to develop a more rapid, cost-effective and higher yielding SAM production method than the conventional production system. In this mini-review, we describe the previously reported yeast gene that contributes to SAM accumulation by overexpression, mutation or deletion and summarise the genetic approach for the production of SAM in large industrial quantities.


Archive | 2001

Medicinal composition for therapy of tumor and health food

Shigeru Hirose; Haruyuki Iefuji; Ryuichi Kamioka; 龍一 上岡; 治幸 家藤; 茂 廣瀬


Archive | 2000

New lipase cs2 derived from yeast

Tsutomu Fujii; Haruyuki Iefuji; Numbi Ramudu Kamini; Takeyuki Kurosu; エヌ アール カミニ; 治幸 家藤; 力 藤井; 猛行 黒須


SpringerPlus | 2013

Treatment of, and Candida utilis biomass production from shochu wastewater; the effects of maintaining a low pH on DOC removal and feeding cultivation on biomass production

Takashi Watanabe; Haruyuki Iefuji; Hiroko Kitamoto


Archive | 2013

Modified peroxidase enzyme gene which exhibits improved expression properties, and method for producing peroxidase using same

Yuu Utashima; 悠 歌島; Shusaku Yanagidani; 柳谷 周作; Haruyuki Iefuji; 家藤 治幸; Kazuo Masaki; 正木 和夫


日本生物工学会大会講演要旨集 | 2010

2P-1152 Phylogenetic analysis of industrial strains by PCR primer sets based on CGH data

Satoko Yoshida; Tsutomu Fujii; Ken Kobayashi; Kenji Okushima; Haruyuki Iefuji


Archive | 2010

New acid protease and use thereof

Haruyuki Iefuji; Kazuo Masaki; Osamu Mizutani; Shengbin Rao; 治幸 家藤; 和夫 正木; 治 水谷; 聖分 饒


Archive | 2009

Mutant lipase and use thereof

Kunio Nakata; 國夫 中田; Yoshihiro Usuda; 臼田 佳弘; Nobuhisa Shimba; 信久 榛葉; Wataru Hoshino; 亘 星野; Eiichiro Suzuki; 鈴木 榮一郎; Haruyuki Iefuji; 家藤 治幸; Kazuo Masaki; 正木 和夫

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Numbi Ramudu Kamini

Central Leather Research Institute

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Hiroko Kitamoto

National Agriculture and Food Research Organization

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