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506. Short Metal Capillary Columns Packed with Polymer-Coated Fibrous Materials in High-Temperature Gas Chromatography

Author

Saito, Yoshihiro, Ogawa, Mitsuhiro, Imaizumi, Motohiro, Ban, Kazuhiro, Abe, Akira, Takeichi, Tsutomu, Wada, Hiroo, and Jinno, Kiyokatsu

Abstract

The high-temperature gas chromatographic (GC) separation of several semivolatile compounds is studied with a short metal capillary column packed with fibrous material, having a polydimethylsiloxane coating thereon. Taking advantage of the excellent heat-resistance of the fiber and also the combination of the surface-deactivated metal capillary, a temperature-programmed separation up to 450°C is successfully demonstrated for the separation of polymer standard samples. The average molecular weight of the commercially-available polymer standard samples for size exclusion chromatography (SEC) is estimated by high-temperature GC analysis and compared with the nominal value determined by a conventional SEC method. Although a slight deviation for the number-average molecular weight is observed between the GC and SEC analysis, the data for the weight-average molecular weight shows a good agreement in these methods. The results also suggest the future possibility of the fiber-packed metal capillary as a miniaturized GC column with an increased sample loading capacity.

Published
2005
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507. Ceramide-1-Phosphate a Novel Mediator for Phagocytosis.

Author

Hinkovska-Galcheva, Vania Tz, Shayman, Jmes A., Kindzelskii, Andrei L., Hiraoka, Miki, Abe, Akira, Petty, Howard R., and Boxer, Laurence A.

Abstract

We identified the generation of ceramide-1-phosphate (C1P) through activation of a ceramide kinase in neutrophils. Our previous studies indicated that C1P enhanced calcium-dependent fusion of liposomes. We hypothesized that human ceramide kinase (hCERK) activity and C1P synthesis leads to enhanced phagocytosis through a mechanism involving modulating membrane fluidity and Ca2+ generation. hCERK was stably transfected into COS-1 cells bearing FcγRIIA. hCERK activity was 2.3 times higher in cells transfected with hCERK than in the FcγRIIA cells or cells transfected with pc-vector. Stably transfected cells showed a 3-fold increase in phagocytosis. Besides increasing phagocytosis, the percentage of ingesting COS-1 cells increased from 43+ 11 in control cells and 50 + 11 in pc-vector control to 70 + 9 (p<0.0001, n=6) in pc-hCERK transfected cells. Cells labeled with [3H]-D-erythro-sphingosine and challenged with particles increased both phagocytosis by three fold and C1P levels by two times compared to resting controls. FcγRIIA, pc-vector and pc-hCERK transfected cells were subjected to cellular fractionation. Utilizing an antibody to c-Myc we confirmed that c-Myc tagged pc-hCERK was localized in the raft fraction, which was identified by a caveolin-1 marker. To assess plasma membrane fluidity we labeled COS–1 cells with 2-dimethylamino-6-lauroylnaphthalene (Laurdan). Cells transfected with pc-hCERK showed higher liquid crystalline order than control and vector transfected cells, a condition favorable to promote membrane fusion. Such ordered structures are reported to be the site of Ca2+ waves ignition. High speed imaging revealed that cells bearing pc-hCERK showed two Ca2+ waves beginning at the leading edge of the cell that propagated in both directions. When the two waves reached the vicinity of the phagosome, a secondary waves split off from each of them, then propagated about the perimeter of the phagosome. That was inhibitable by employing a store-operated Ca2+ channel (SOC) inhibitor. This behavior is unique to the FcγRIIA/pc-hCERK transfected cells. In conclusion transfected COS-1 cells were able to increase their C1P levels during phagocytosis. This changed the structural order parameter of the lipid rafts where hCERK is localized and likely contributed to phagocytosis by promoting phagosome development. Lipid rafts were enriched in Ca2+ signaling machinery and in turn pc-hCERK transfection resulted in a novel means to markedly enhance phagocytosis by generating Ca2+ movement from SOC.

Published
2004
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508. Genome Analysis Revives a Forgotten Hybrid Crop Edo-dokoro in the Genus Dioscorea.

Author

Natsume, Satoshi, Sugihara, Yu, Kudoh, Aoi, Oikawa, Kaori, Shimizu, Motoki, Ishikawa, Yuko, Nishihara, Masahiro, Abe, Akira, Innan, Hideki, and Terauchi, Ryohei

Subjects
*YAMS, *CROPS, *GENOMES, *PLANT hybridization, *GENOMICS
Abstract

A rhizomatous Dioscorea crop 'Edo-dokoro' was described in old records of Japan, but its botanical identity has not been characterized. We found that Edo-dokoro is still produced by four farmers in Tohoku-machi of the Aomori prefecture, Japan. The rhizomes of Edo-dokoro are a delicacy to the local people and are sold in the markets. Morphological characters of Edo-dokoro suggest its hybrid origin between the two species, Dioscorea tokoro and Dioscorea tenuipes. Genome analysis revealed that Edo-dokoro likely originated by hybridization of a male D. tokoro to a female D. tenuipes , followed by a backcross with a male plant of D. tokoro. Edo-dokoro is a typical minor crop possibly maintained for more than 300 years but now almost forgotten by the public. We hypothesize that there are many such uncharacterized genetic heritages passed over generations by small-scale farmers that await serious scientific investigation for future use and improvement by using modern genomics information. [ABSTRACT FROM AUTHOR]

Published
2022
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509. De Novo Transcriptome Analysis Reveals Flowering-Related Genes That Potentially Contribute to Flowering-Time Control in the Japanese Cultivated Gentian Gentiana triflora.

Author

Takase, Tomoyuki, Shimizu, Motoki, Takahashi, Shigekazu, Nemoto, Keiichirou, Goto, Fumina, Yoshida, Chiharu, Abe, Akira, and Nishihara, Masahiro

Subjects
*RNA sequencing, *GENTIANA, *FLOWERING time, *TRANSCRIPTOMES, *GENES, *AUTUMN
Abstract

Japanese cultivated gentians are perennial plants that flower in early summer to late autumn in Japan, depending on the cultivar. Several flowering-related genes, including GtFT1 and GtTFL1, are known to be involved in regulating flowering time, but many such genes remain unidentified. In this study, we obtained transcriptome profiling data using the Gentiana triflora cultivar 'Maciry', which typically flowers in late July. We conducted deep RNA sequencing analysis using gentian plants grown under natural field conditions for three months before flowering. To investigate diurnal changes, the plants were sampled at 4 h intervals over 24 h. Using these transcriptome data, we determined the expression profiles of leaves based on homology searches against the Flowering-Interactive Database of Arabidopsis. In particular, we focused on transcription factor genes, belonging to the BBX and MADS-box families, and analyzed their developmental and diurnal variation. The expression levels of representative BBX genes were also analyzed under long- and short-day conditions using in-vitro-grown seedlings, and the expression patterns of some BBX genes differed. Clustering analysis revealed that the transcription factor genes were coexpressed with GtFT1. Overall, these expression profiles will facilitate further analysis of the molecular mechanisms underlying the control of flowering time in gentians. [ABSTRACT FROM AUTHOR]

Published
2022
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510. MutMap accelerates breeding of a salt-tolerant rice cultivar.

Author

Takagi, Hiroki, Tamiru, Muluneh, Abe, Akira, Yoshida, Kentaro, Uemura, Aiko, Yaegashi, Hiroki, Obara, Tsutomu, Oikawa, Kaori, Utsushi, Hiroe, Kanzaki, Eiko, Mitsuoka, Chikako, Natsume, Satoshi, Kosugi, Shunichi, Kanzaki, Hiroyuki, Matsumura, Hideo, Urasaki, Naoya, Kamoun, Sophien, and Terauchi, Ryohei

Subjects
*RICE breeding, *SALT-tolerant crops, *GENETIC mutation, *EFFECT of salts on plants, *GENOMICS, *NUCLEOTIDE sequencing
Abstract

The article presents a study related to development of a salt-tolerant rice variety using a method called MutMap, which helps in identifying the loss-of-function mutations in rice that was further used in developing the variety. Topics discussed include physiological effects of excess amount of salts such as nitrates and potassium on rice, the MutMap, which is based on whole genome sequencing and pertinence of advantages of genomics-based crop breeding in improving traits such as yield.

Published
2015
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511. Rice apoplastic CBM1-interacting protein counters blast pathogen invasion by binding conserved carbohydrate binding module 1 motif of fungal proteins.

Author

Takeda, Takumi, Takahashi, Machiko, Shimizu, Motoki, Sugihara, Yu, Yamashita, Tetsuro, Saitoh, Hiromasa, Fujisaki, Koki, Ishikawa, Kazuya, Utsushi, Hiroe, Kanzaki, Eiko, Sakamoto, Yuichi, Abe, Akira, and Terauchi, Ryohei

Subjects
*FUNGAL proteins, *FUNGAL enzymes, *XYLANASES, *CARBOHYDRATES, *PLANT proteins, *HEMICELLULOSE, *PLANT cell walls, *RICE
Abstract

When infecting plants, fungal pathogens secrete cell wall-degrading enzymes (CWDEs) that break down cellulose and hemicellulose, the primary components of plant cell walls. Some fungal CWDEs contain a unique domain, named the carbohydrate binding module (CBM), that facilitates their access to polysaccharides. However, little is known about how plants counteract pathogen degradation of their cell walls. Here, we show that the rice cysteine-rich repeat secretion protein OsRMC binds to and inhibits xylanase MoCel10A of the blast fungus pathogen Magnaporthe oryzae, interfering with its access to the rice cell wall and degradation of rice xylan. We found binding of OsRMC to various CBM1-containing enzymes, suggesting that it has a general role in inhibiting the action of CBM1. OsRMC is localized to the apoplast, and its expression is strongly induced in leaves infected with M. oryzae. Remarkably, knockdown and overexpression of OsRMC reduced and enhanced rice defense against M. oryzae, respectively, demonstrating that inhibition of CBM1-containing fungal enzymes by OsRMC is crucial for rice defense. We also identified additional CBM-interacting proteins (CBMIPs) from Arabidopsis thaliana and Setaria italica, indicating that a wide range of plants counteract pathogens through this mechanism. Author summary: Plants have evolved various activity-inhibiting proteins as a defense against fungal cell wall-degrading enzymes (CWDEs), but how plants counteract the function of fungal enzymes containing carbohydrate binding modules (CBMs) remains unknown. Here, we demonstrate that OsRMC, a member of the cysteine-rich repeat secretion protein family, interacts with fungal CBM1. OsRMC binding to CBM1 of a blast fungal xylanase blocks access to cellulose, resulting in the inhibition of xylanase enzymatic activity. Our study provides significant insights into plant countermeasures against CWDEs in the apoplastic space during plant-fungal pathogen interactions. It also reveals a molecular function of the DUF26 domain widely distributed in plant proteins. [ABSTRACT FROM AUTHOR]

Published
2022
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512. Gain Curves of a Microchannel Plate Ion Detector for Measurement of End-Loss Ions in the Tandem Mirror

Author

Tetsuya Goto, Tetsuya Goto, Kameo Ishii, Kameo Ishii, Toshiki Takahashi, Toshiki Takahashi, Akira Abe, Akira Abe, Yuzo Katsuki, Yuzo Katsuki, Nagayoshi Kikuno, Nagayoshi Kikuno, Yasuhiro Goi, Yasuhiro Goi, Yoshihiro Ono, Yoshihiro Ono, Nobutsugu Ishibashi, Nobutsugu Ishibashi, Yousuke Nakashima, Yousuke Nakashima, Kiyoshi Yatsu, Kiyoshi Yatsu, and Teruo Tamano, Teruo Tamano

Abstract

A microchannel plate (MCP) is used as an ion detector in the end-loss energy component analyzer, which has been developed in order to measure velocity distribution functions of end-loss ions in the tandem mirror GAMMA10. The gain of the MCP depends on variable parameters of the incident ion energy, the incident ion current density, and the MCP bias voltage. The gain characteristics was obtained using a hydrogen beam test stand, and the gain curves were described as a function of the parameters for the purpose of the quantitative evaluation of end-loss ions.

Published
1996
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513. New Type of End-Loss Energy Component Analyzer and Velocity Distribution Function of End-Loss Ions in Tandem Mirror

Author

Kameo Ishii, Kameo Ishii, Toshiaki Tanaka, Toshiaki Tanaka, Toshitaka Nakada, Toshitaka Nakada, Takehiro Katori, Takehiro Katori, Akira Abe, Akira Abe, Toshiki Takahashi, Toshiki Takahashi, Isao Katanuma, Isao Katanuma, Akiyosi Itakura, Akiyosi Itakura, Kiyoshi Yatsu, Kiyoshi Yatsu, and Teruo Tamano, Teruo Tamano

Abstract

A new type of end-loss energy component analyzer (ELECA) has been developed in order to investigate ion confinement of the tandem mirror. The essential advantage of the use of the ELECA is the ability to determine distribution functions of end-loss ions every moment during plugging in one shot. The ELECA was carefully designed, taking account of the influence of the fringing electrostatic field and weak leakage magnetic field on ion trajectories in the analyzer. The new diagnostics has been applied to the tandem mirror GAMMA 10. Consequently, it was verified from the viewpoint of ion distribution in velocity space that plug potential was created upon turning on electron cyclotron resonance heating (ECRH) even without sloshing ions caused by neutral beam injection (NBI), and at the same time, the structure with double loss boundaries changed to a simple structure.

Published
1994
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514. Quantitative analysis of active oxygen for soot oxidation over Ag/ZrO2: Characterization with temperature-programmed reduction by NH3

Author

Nanba, Tetsuya, Masukawa, Shoichi, Abe, Akira, Uchisawa, Junko, and Obuchi, Akira

Subjects
*QUANTITATIVE chemical analysis, *REACTIVE oxygen species, *OXIDATION of soot, *SILVER nanoparticles, *ZIRCONIUM oxide, *TEMPERATURE-programmed reduction, *AMMONIA, *CARBON-black
Abstract

Abstract: Active oxygen species for soot oxidation over Ag/ZrO2 were characterized by means of X-ray photoelectron spectroscopy (XPS) and temperature-programmed desorption and reduction methods. The temperature-programmed surface reaction (TPSR) between carbon black (CB), a model soot, and surface oxygen revealed that two kinds of adsorbed oxygen species were involved in CB oxidation over Ag/ZrO2. The results of XPS, temperature-programmed desorption of O2, and temperature-programmed reduction by H2 were insufficient to distinguish the two kinds of active oxygen species. Temperature-programmed reduction by NH3 (NH3-TPR) resulted in N2 and N2O formation as products of reduction of the Ag/ZrO2 surface and bulk oxygen. The N2O formation profile in NH3-TPR exhibited two peaks, corresponding to two kinds of oxygen species having a strong oxidation capacity. The effect of Ag loading on the total amount of N2O formation was in good agreement with that on the amount of active oxygen species observed by TPSR-CB. We concluded that NH3-TPR was an appropriate technique for quantitative characterization of the amount of active oxygen species for soot oxidation on Ag/ZrO2. [Copyright &y& Elsevier]

Published
2012
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515. A multifaceted genomics approach allows the isolation of the rice Pia-blast resistance gene consisting of two adjacent NBS-LRR protein genes.

Author

Okuyama, Yudai, Kanzaki, Hiroyuki, Abe, Akira, Yoshida, Kentaro, Tamiru, Muluneh, Saitoh, Hiromasa, Fujibe, Takahiro, Matsumura, Hideo, Shenton, Matt, Galam, Dominique Clark, Undan, Jerwin, Ito, Akiko, Sone, Teruo, and Terauchi, Ryohei

Subjects
*GENOMICS, *PLANT gene isolation, *PLANT proteins, *PHYTOPATHOGENIC fungi, *PHENOTYPES, *LEUCINE, RICE genetics
Abstract

The Oryza sativa (rice) resistance gene Pia confers resistance to the blast fungus Magnaporthe oryzae carrying the AVR-Pia avirulence gene. To clone Pia, we employed a multifaceted genomics approach. First, we selected 12 R-gene analog (RGA) genes encoding nucleotide binding site-leucine rich repeats (NBS-LRRs) proteins from a region on chromosome 11 that shows linkage to Pia. By using seven rice accessions, we examined the association between Pia phenotypes and DNA polymorphisms in the 10 genes, which revealed three genes ( Os11gRGA3-Os11gRGA5) exhibiting a perfect association with the Pia phenotypes. We also screened ethyl methane sulfonate (EMS)-treated mutant lines of the rice cultivar 'Sasanishiki' harboring Pia, and isolated two mutants that lost the Pia phenotype. DNA sequencing of Os11gRGA3-Os11gRGA5 from the two mutant lines identified independent mutations of major effects in Os11gRGA4. The wild-type 'Sasanishiki' allele of Os11gRGA4 ( SasRGA4) complemented Pia function in both mutants, suggesting that SasRGA4 is necessary for Pia function. However, when the rice cultivar 'Himenomochi' lacking Pia was transfected with SasRGA4, the Pia phenotype was not recovered. An additional complementation study revealed that the two NBS-LRR-type R genes, SasRGA4 and SasRGA5, that are located next to each other and oriented in the opposite direction are necessary for Pia function. A population genetics analysis of SasRGA4 and SasRGA5 suggests that the two genes are under long-term balancing selection. [ABSTRACT FROM AUTHOR]

Published
2011
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516. Isolation of lactic acid bacteria capable of reducing environmental alkyl and fatty acid hydroperoxides, and the effect of their oral administration on oxidative-stressed nematodes and rats.

Author

Watanabe, Akio, Yamaguchi, Takuro, Murota, Kaeko, Ishii, Naoaki, Terao, Junji, Okada, Sanae, Tanaka, Naoto, Kimata, Shinya, Abe, Akira, Suzuki, Tomonori, Uchino, Masataka, and Niimura, Youichi

Subjects
*LACTIC acid bacteria, *LACTOBACILLUS plantarum, *FATTY acids, *HYDROPEROXIDES, *RATS, *HYDROGEN peroxide, *LARGE intestine
Abstract

Reinforcement of the hydroperoxide-eliminating activity in the small and large intestines should prevent associated diseases. We previously isolated a lactic acid bacterium, Pediococcus pentosaceus Be1 that facilitates a 2-electron reduction of hydrogen peroxide to water. In this study, we successfully isolated an alternative lactic acid bacterium, Lactobacillus plantarum P1-2, that can efficiently reduce environmental alkyl hydroperoxides and fatty acid hydroperoxides to their corresponding hydroxyl derivatives through a 2-electron reduction. Each strain exhibited a wide concentration range with regard to the environmental reducing activity for each hydroperoxide. Given this, the two lactic acid bacteria were orally administered to an oxygen-sensitive short-lived nematode mutant, and this resulted in a significant expansion of its lifespan. This observation suggests that P. pentosaceus Be1 and L. plantarum P1-2 inhibit internal oxidative stress. To determine the specific organs involved in this response, we performed a similar experiment in rats, involving induced lipid peroxidation by iron-overloading. We observed that only L. plantarum P1-2 inhibited colonic mucosa lipid peroxidation in rats with induced oxidative stress. [ABSTRACT FROM AUTHOR]

Published
2020
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517. Next-generation sequencing-based bulked segregant analysis for QTL mapping in the heterozygous species Brassica rapa.

Author

Itoh, Noriaki, Segawa, Tenta, Tamiru, Muluneh, Abe, Akira, Sakamoto, Shota, Uemura, Aiko, Oikawa, Kaori, Kutsuzawa, Hiroto, Koga, Hironori, Imamura, Tomohiro, Terauchi, Ryohei, and Takagi, Hiroki

Subjects
*CHINESE cabbage, *SPECIES, *BRASSICA, *PLANT species, *TURNIPS, *PROOF of concept, *EDIBLE greens
Abstract

Key message: An improved protocol of QTL-seq, an NGS-based method for bulked segregant analysis we previously developed in rice, allowed successful mapping of QTLs of interest in the highly heterozygous genome of B. rapa, demonstrating the power of this elegant method for genetic analyses in heterozygous species of economic importance. Recent advances in next-generation sequencing (NGS) and the various NGS-based methods developed for rapidly identifying candidate genes of interest have accelerated genetic analysis mainly in the model plants rice and Arabidopsis. Brassica rapa includes several economically important crops such as Chinese cabbage, turnip and various leafy vegetables. The application of NGS-based approaches for the analysis of B. rapa has been limited mainly due to its highly heterozygous genome and poor quality of the reference genome sequence currently available for this species. In this study, we have improved QTL-seq, a method for NGS-based bulked segregant analysis we previously developed in rice, extending its applicability for accelerating the genetic analysis and molecular breeding of B. rapa. Addition of new filters to the original QTL-seq pipeline allowed removal of spurious single-nucleotide polymorphisms caused by alignment/sequencing errors and variability between parents, significantly improving accuracy of the analysis. As proof of principle, we successfully applied the new approach to identify candidate genomic regions controlling flowering and trichome formation using segregating F2 progeny obtained from crosses made between cultivars of B. rapa showing contrasting phenotypes for these traits. We strongly believe that the improved QTL-seq method reported here will extend the applicability of NGS-based genetic analysis not only to B. rapa but also to other plant species of economic importance with heterozygous genomes. [ABSTRACT FROM AUTHOR]

Published
2019
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518. Next generation long-culm rice with superior lodging resistance and high grain yield, Monster Rice 1.

Author

Nomura, Tomohiro, Arakawa, Naoya, Yamamoto, Toshio, Ueda, Tadamasa, Adachi, Shunsuke, Yonemaru, Jun-ichi, Abe, Akira, Takagi, Hiroki, Yokoyama, Tadashi, and Ookawa, Taiichiro

Subjects
*GRAIN yields, *BROWN rice, *RICE yields, *RICE, *GREEN Revolution, *BENDING moment
Abstract

During late 1960s Green Revolution, researchers utilized semidwarf 1 (sd1) to improve the yield and lodging resistance in rice (Oryza sativa L.). However, sd1 has a negative effect to culm strength and biomass production. To increase yield dramatically in 21th century, development of next generation long-culm rice for non-lodging and high grain yield independent of sd1 has been needed. The present study developed Monster Rice 1, a long-culm and heavy-panicle type of rice line and compared it with Takanari, a high-yielding semidwarf rice variety about yield and lodging resistance associated traits. Brown rice yield and bending moment at breaking of the basal elongated internode were higher in Monster Rice 1 than those in Takanari due to a large number of spikelets per panicle and thicker culm. Furthermore, to identify QTLs with superior alleles for these traits, QTL and haplotype analyses were performed using F2 population and recombinant inbred lines derived from a cross between Monster Rice 1 and Takanari. The results from this study suggest that long-culm and heavy-panicle type of rice with a superior lodging resistance by culm strength can perform its high yield potential by using these identified QTLs contributing yield and lodging resistance. [ABSTRACT FROM AUTHOR]

Published
2019
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519. Genome-wide association mapping for phenotypic plasticity in rice.

Author

Kikuchi, Shinji, Bheemanahalli, Raju, Jagadish, Krishna S.V., Kumagai, Etsushi, Masuya, Yusuke, Kuroda, Eiki, Raghavan, Chitra, Dingkuhn, Michael, Abe, Akira, and Shimono, Hiroyuki

Subjects
*PLANT genomes, *VEGETATION mapping, *PHENOTYPIC plasticity in plants, *RICE, *EFFECT of environment on plants
Abstract

Phenotypic plasticity of plants in response to environmental changes is important for adapting to changing climate. Less attention has been paid to exploring the advantages of phenotypic plasticity in resource-rich environments to enhance the productivity of agricultural crops. Here, we examined genetic variation for phenotypic plasticity in indica rice ( Oryza sativa L.) across two diverse panels: (1) a Phenomics of Rice Adaptation and Yield (PRAY) population comprising 301 accessions; and (2) a Multi-parent Advanced Generation Inter-Cross (MAGIC) indica population comprising 151 accessions. Altered planting density was used as a proxy for elevated atmospheric CO2 response. Low planting density significantly increased panicle weight per plant compared with normal density, and the magnitude of the increase ranged from 1.10 to 2.78 times among accessions for the PRAY population and from 1.05 to 2.45 times for the MAGIC population. Genome-wide-association studies validate three Environmental Responsiveness (ER) candidate alleles (qER1-3) that were associated with relative response of panicle weight to low density. Two of these alleles were tested in 13 genotypes to clarify their biomass responses during vegetative growth under elevated CO2 in Japan. Our study provides evidence for polymorphisms that control rice phenotypic plasticity in environments that are rich in resources such as light and CO2. [ABSTRACT FROM AUTHOR]

Published
2017
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525. Whole genome sequencing approaches to understand Magnaporthe-rice interactions.

Author

Terauchi, Ryohei, Kanzaki, Hiroyuki, Fujisaki, Koki, Takagi, Hiroki, Abe, Akira, Yoshida, Kentaro, Okuyama, Yudai, Tamiru, Muluneh, and Saitoh, Hiromasa

Subjects
*NUCLEOTIDE sequencing, *PYRICULARIA oryzae, *HOST-parasite relationships, *MICROBIAL virulence, *RICE diseases & pests
Abstract

Due to the recent advances in DNA sequencing technologies, whole genome sequencing (WGS)-based approaches are now accelerating the pace of our research toward a better understanding of host-pathogen interactions. Using WGS-based methods, we have isolated three avirulence ( AVR ) genes: AVR-Pia , AVR-Pii and AVR-Pik from Magnaporthe oryzae and two cognate rice resistance ( R -) genes: Pia and Pii . We briefly review our current understanding of the interactions between AVR-Pia and Pia , AVR-Pik and Pik , and AVR-Pii and Pii . [ABSTRACT FROM AUTHOR]

Published
2016
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526. The rice ( Oryza sativa L.) LESION MIMIC RESEMBLING, which encodes an AAA-type ATPase, is implicated in defense response.

Author

Fekih, Rym, Tamiru, Muluneh, Kanzaki, Hiroyuki, Abe, Akira, Yoshida, Kentaro, Kanzaki, Eiko, Saitoh, Hiromasa, Takagi, Hiroki, Natsume, Satoshi, Undan, Jerwin, Undan, Jesusa, and Terauchi, Ryohei

Subjects
*RNA interference, *GENE expression in plants, *ADENOSINE triphosphatase, *PLANT mutation, *DNA insertion elements, RICE genetics
Abstract

Lesion mimic mutants (LMMs) provide a useful tool to study defense-related programmed cell death (PCD) in plants. Although a number of LMMs have been identified in multiple species, most of the candidate genes are yet to be isolated. Here, we report the identification and characterization of a novel rice ( Oryza sativa L.) lesion mimic resembling ( lmr) mutant, and cloning of the corresponding LMR gene. The LMR locus was initially delineated to 1.2 Mb region on chromosome 6, which was further narrowed down to 155-kb using insertions/deletions (INDELs) and cleavage amplified polymorphic sequence markers developed in this study. We sequenced the open reading frames predicted within the candidate genomic region, and identified a G-A base substitution causing a premature translation termination in a gene that encodes an ATPase associated with various cellular activities type (AAA-type) protein. RNA interference transgenic lines with reduced LMR transcripts exhibited the lesion mimic phenotype similar to that of lmr plants. Furthermore, expression of the wild-type LMR in the mutant background complemented the lesion phenotype, confirming that the mutation identified in LMR is responsible for the mutant phenotype. The pathogenesis-related (PR) genes PBZ1 and PR1 were induced in lmr, which also showed enhanced resistance to rice blast ( Magnaporthe oryzae) and bacterial blight ( Xanthomonas oryzae pv. oryzae), suggesting LMR is a negative regulator of cell death in rice. The identification of lmr and cloning of the corresponding LMR gene provide an additional resource for the study of PCD in plants. [ABSTRACT FROM AUTHOR]

Published
2015
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527. QTL Map Meets Population Genomics: An Application to Rice.

Author

Fawcett, Jeffrey A., Kado, Tomoyuki, Sasaki, Eriko, Takuno, Shohei, Yoshida, Kentaro, Sugino, Ryuichi P., Kosugi, Shunichi, Natsume, Satoshi, Mitsuoka, Chikako, Uemura, Aiko, Takagi, Hiroki, Abe, Akira, Ishii, Takashige, Terauchi, Ryohei, and Innan, Hideki

Subjects
*GENOMICS, *RICE yields, *AGRONOMY, *METAGENOMICS, *PLANT gene mapping, RICE genetics
Abstract

Genes involved in the transition from wild to cultivated crop species should be of great agronomic importance. Population genomic approaches utilizing genome resequencing data have been recently applied for this purpose, although it only reports a large list of candidate genes with no biological information. Here, by resequencing more than 30 genomes altogether of wild rice Oryza rufipogon and cultivated rice O. sativa, we identified a number of regions with clear footprints of selection during the domestication process. We then focused on identifying candidate domestication genes in these regions by utilizing the wealth of QTL information in rice. We were able to identify a number of interesting candidates such as transcription factors that should control key domestication traits such as shattering, awn length, and seed dormancy. Other candidates include those that might have been related to the improvement of grain quality and those that might have been involved in the local adaptation to dry conditions and colder environments. Our study shows that population genomic approaches and QTL mapping information can be used together to identify genes that might be of agronomic importance. [ABSTRACT FROM AUTHOR]

Published
2013
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528. Mut Map- Gap: whole-genome resequencing of mutant F2 progeny bulk combined with de novo assembly of gap regions identifies the rice blast resistance gene Pii.

Author

Takagi, Hiroki, Uemura, Aiko, Yaegashi, Hiroki, Tamiru, Muluneh, Abe, Akira, Mitsuoka, Chikako, Utsushi, Hiroe, Natsume, Satoshi, Kanzaki, Hiroyuki, Matsumura, Hideo, Saitoh, Hiromasa, Yoshida, Kentaro, Cano, Liliana M., Kamoun, Sophien, and Terauchi, Ryohei

Subjects
*GENOMICS, *PROGENY tests (Botany), *RICE blast disease, *GENETICS of disease resistance of plants, RICE genetics
Abstract

Next-generation sequencing allows the identification of mutations responsible for mutant phenotypes by whole-genome resequencing and alignment to a reference genome. However, when the resequenced cultivar/line displays significant structural variation from the reference genome, mutations in the genome regions missing from the reference (gaps) cannot be identified by simple alignment., Here we report on a method called ' Mut Map- Gap', which involves delineating a candidate region harboring a mutation of interest using the recently reported Mut Map method, followed by de novo assembly, alignment, and identification of the mutation within genome gaps., We applied Mut Map- Gap to isolate the blast resistant gene Pii from the rice cv Hitomebore using mutant lines that have lost Pii function., Mut Map- Gap should prove useful for cloning genes that exhibit significant structural variations such as disease resistance genes of the nucleotide-binding site-leucine rich repeat ( NBS- LRR) class. [ABSTRACT FROM AUTHOR]

Published
2013
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529. Prefoldin Protects Neuronal Cells from Polyglutamine Toxicity by Preventing Aggregation Formation.

Author

Tashiro, Erika, Zako, Tamotsu, Muto, Hideki, Itoo, Yoshinori, Sörgjerd, Karin, Terada, Naofumi, Abe, Akira, Miyazawa, Makoto, Kitamura, Akira, Kitaura, Hirotake, Kubota, Hiroshi, Maeda, Mizuo, Momoi, Takashi, Iguchi-Ariga, Sanae M. M., Kinjo, Masataka, and Ariga, Hiroyoshi

Subjects
*HUNTINGTON disease, *PREFOLDIN, *NEURAL stem cells, *POLYGLUTAMINE, *BIOLOGICAL aggregation, *POLYPEPTIDES, *HUNTINGTIN protein
Abstract

Huntington disease is caused by cell death after the expansion of polyglutamine (polyQ) tracts longer than ~40 repeats encoded by exon 1 of the huntingtin (HTT) gene. Prefoldin is a molecular chaperone composed of six subunits, PFD1-6, and prevents misfolding of newly synthesized nascent polypeptides. In this study, we found that knockdown of PFD2 and PFD5 disrupted prefoldin formation in HTT-expressing cells, resulting in accumulation of aggregates of a pathogenic form of HTT and in induction of cell death. Dead cells, however, did not contain inclusions of HTT, and analysis by a fluorescence correlation spectroscopy indicated that knockdown of PFD2 and PFD5 also increased the size of soluble oligomers of pathogenic HTT in cells. In vitro single molecule observation demonstrated that prefoldin suppressed HTT aggregation at the small oligomer (dimer to tetramer) stage. These results indicate that prefoldin inhibits elongation of large oligomers of pathogenic Htt, thereby inhibiting subsequent inclusion formation, and suggest that soluble oligomers of polyQ-expanded HTT are more toxic than are inclusion to cells. [ABSTRACT FROM AUTHOR]

Published
2013
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530. MutMap+: Genetic Mapping and Mutant Identification without Crossing in Rice.

Author

Fekih, Rym, Takagi, Hiroki, Tamiru, Muluneh, Abe, Akira, Natsume, Satoshi, Yaegashi, Hiroki, Sharma, Shailendra, Sharma, Shiveta, Kanzaki, Hiroyuki, Matsumura, Hideo, Saitoh, Hiromasa, Mitsuoka, Chikako, Utsushi, Hiroe, Uemura, Aiko, Kanzaki, Eiko, Kosugi, Shunichi, Yoshida, Kentaro, Cano, Liliana, Kamoun, Sophien, and Terauchi, Ryohei

Subjects
*RICE breeding, *PHENOTYPES, *PLANT gene mapping, *PLANT variation, *PLANT genomes, *PLANT mutation, *NUCLEOTIDE sequence
Abstract

Advances in genome sequencing technologies have enabled researchers and breeders to rapidly associate phenotypic variation to genome sequence differences. We recently took advantage of next-generation sequencing technology to develop MutMap, a method that allows rapid identification of causal nucleotide changes of rice mutants by whole genome resequencing of pooled DNA of mutant F2 progeny derived from crosses made between candidate mutants and the parental line. Here we describe MutMap+, a versatile extension of MutMap, that identifies causal mutations by comparing SNP frequencies of bulked DNA of mutant and wild-type progeny of M3 generation derived from selfing of an M2 heterozygous individual. Notably, MutMap+ does not necessitate artificial crossing between mutants and the wild-type parental line. This method is therefore suitable for identifying mutations that cause early development lethality, sterility, or generally hamper crossing. Furthermore, MutMap+ is potentially useful for gene isolation in crops that are recalcitrant to artificial crosses. [ABSTRACT FROM AUTHOR]

Published
2013
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531. Group XV phospholipase A2, a lysosomal phospholipase A2

Author

Shayman, James A., Kelly, Robert, Kollmeyer, Jessica, He, Yongqun, and Abe, Akira

Subjects
*PHOSPHOLIPASES, *LYSOSOMES, *LECITHIN, *PHOSPHATIDYLETHANOLAMINES, *PHOSPHATIDYLSERINES, *CERAMIDES, *ACYLATION, *AMIODARONE
Abstract

Abstract: A phospholipase A2 was identified from MDCK cell homogenates with broad specificity toward glycerophospholipids including phosphatidylcholine, phosphatidylethanolamine, phosphatidylserine, and phosphatidylglycerol. The phospholipase has the unique ability to transacylate short chain ceramides. This phospholipase is calcium-independent, localized to lysosomes, and has an acidic pH optimum. The enzyme was purified from bovine brain and found to be a water-soluble glycoprotein consisting of a single peptide chain with a molecular weight of 45kDa. The primary structure deduced from the DNA sequences is highly conserved between chordates. The enzyme was named lysosomal phospholipase A2 (LPLA2) and subsequently designated group XV phospholipase A2. LPLA2 has 49% of amino acid sequence identity to lecithin–cholesterol acyltransferase and is a member of the αβ-hydrolase superfamily. LPLA2 is highly expressed in alveolar macrophages. A marked accumulation of glycerophospholipids and extensive lamellar inclusion bodies, a hallmark of cellular phospholipidosis, is observed in alveolar macrophages in LPLA 2 −/− mice. This defect can also be reproduced in macrophages that are exposed to cationic amphiphilic drugs such as amiodarone. In addition, older LPLA 2 −/− mice develop a phenotype similar to human autoimmune disease. These observations indicate that LPLA2 may play a primary role in phospholipid homeostasis, drug toxicity, and host defense. [ABSTRACT FROM AUTHOR]

Published
2011
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532. Chlorella vulgaris Aldehyde Reductase Is Capable of Functioning as Ferric Reductase and of Driving the Fenton Reaction in the Presence of Free Flavin.

Author

Sato, Junichi, Takeda, Kouji, Nisheyama, Rika, Fusayama, Kouichi, Arai, Toshiaki, Sato, Takumi, Watanabe, Toshihiro, Abe, Akira, Nakagawa, Junichi, Kawasaki, Shinji, and Niimura, Youichi

Subjects
*ENZYMATIC analysis, *CHLORELLA, *FLAVINS, *EXTRACTS, *NUCLEOTIDE sequence, *ALCOHOL dehydrogenase
Abstract

The article discusses a study which examines the enzymatic components of Chlorella vulgaris. Findings of the study reveal that a free flavin-dependent Fenton reaction was identified on its cell-free extracts. It also indicates that its N-terminal sequence was similar to aldo-keto reductase family enzymes since it displayed aldehyde reductase activity as well.

Published
2010
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534. Rapid determination of ethylene oxide with fiber-packed sample preparation needle

Author

Ueta, Ikuo, Saito, Yoshihiro, Ghani, Nadia Binti Abdul, Ogawa, Mitsuhiro, Yogo, Kentaro, Abe, Akira, Shirai, Shingoro, and Jinno, Kiyokatsu

Subjects
*ETHYLENE oxide, *FIBERS, *DERIVATIZATION, *HYDROGEN bromide, *GAS chromatography, *EXTRACTION (Chemistry), *STANDARD deviations, *CHEMICAL sample preparation
Abstract

Abstract: Fiber-packed sample preparation device was applied to the simultaneous derivatization/preconcentration of ethylene oxide (EO) in air samples. The polymer-coated filaments were packed longitudinally into the needle, and hydrogen bromide (HBr) was loaded onto the filaments in the preconditioning process. Simultaneous derivatization with HBr in the needle was made during the sampling process of the gaseous EO, and the corresponding derivatized analyte, 2-bromoethanol, was desorbed by passing a small amount of methanol through the extraction needle in the heated gas chromatograph (GC) injector. The basic extraction/desorption parameters for EO have been evaluated. The limit of detection (LOD), limit of quantification (LOQ) and the relative standard deviation (RSD) of run-to-run repeatability were 1.8ng/L, 5.4ng/L and less than 4%, respectively, with an extraction time of about 10min. Satisfactory storage performance for three days at room temperature was also confirmed. [Copyright &y& Elsevier]

Published
2009
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535. Ceramide 1-Phosphate, a Mediator of Phagocytosis.

Author

Hinkovska-Galcheva, Vania, Boxer, Laurence A., Kindzelskii, Andrei, Hiraoka, Miki, Abe, Akira, Goparju, Sravan, Spiegel, Sarah, Petty, Howard R., and Shayman, James A.

Subjects
*CERAMIDES, *GLYCOSPHINGOLIPIDS, *PHOSPHATES, *PHAGOCYTOSIS, *ANTIGEN-antibody reactions, *ENDOCYTOSIS, *IMMUNE response, *IMMUNOLOGY, *MEMBRANE lipids
Abstract

The agonist-stimulated metabolism of membrane lipids produces potent second messengers that regulate phagocytosis. We studied whether human ceramide kinase (hCERK) activity and ceramide 1-phosphate formation could lead to enhanced phagocytosis through a mechanism involving modulation of the membrane-structural order parameter. hCERK was stably transfected into COS-1 cells that were stably transfected with the FcγRIIA receptor. hCERK-transfected cells displayed a significant increase in phgocytic index in association with increased ceramide kinase activation and translocation to lipid rafts after activation with opsonized erythrocytes. When challenged with opsonized erythrocytes, hCERK-transfected cells increased phagocytosis by 1,5-fold compared with vector control and simultaneously increased ceramide 1-phosphate levels 2-fold compared with vector and unstimulated control cells. Control and hCERK-transfected cells were subjected to cellular fractionation. Utilizing an antibody against hCERK, we observed that CERK translocates during activation from the cytosol to a lipid raft fraction. The plasma membrane-structural order parameter of the transfectants was measured by labeling cells with Laurdan. Cells transfected with hCERK showed a higher liquid crystalline order than control cells with stimulation, conditions that are favorable for the promotion of membrane fusion at the sites of phagocytosis. The change in the structural order parameter of the lipid rafts probably contributes to phagocytosis by promoting phagosome formation. [ABSTRACT FROM AUTHOR]

Published
2005
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536. High-temperature separation with polymer-coated fiber in packed capillary gas chromatography.

Author

Saito, Yoshihiro, Ogawa, Mitsuhiro, Imaizumi, Motohiro, Ban, Kazuhiro, Abe, Akira, Takeichi, Tsutomu, Wada, Hiroo, and Jinno, Kiyokatsu

Subjects
*GAS chromatography, *SEPARATION (Technology), *THERMAL analysis, *METALS, *SURFACE coatings
Abstract

High-temperature gas chromatographic separation of several synthetic polymer mixtures with Dexsil-coated fiber-packed columns was studied. A bundle of heat-resistant filaments, Zylon, was longitudinally packed into a short metal capillary, followed by the conventional coating process with Dexsil 300 material. Prior to the packing process the metal capillary was deactivated by the formation of a silica layer. The typical size of the resulting column was 0.3-mm i.d., 0.5-mm o.d., 1-m length, and packed with about 170 filaments of the Dexsil-coated Zylon. The column temperature could be elevated up to 450°C owing to the good thermal stability of the fiber, Dexsil coating, and metal capillary; furthermore, this allowed the separation of low-volatile compounds to be studied. [ABSTRACT FROM AUTHOR]

Published
2005
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538. Genotypic variation in cold tolerance of 18 Ethiopian rice cultivars in relation to their reproductive morphology.

Author

Alemayehu, Habtamu Assega, Dumbuya, Gibrilla, Hasan, Mehedi, Tadesse, Tilahun, Nakajyo, Shinsuke, Fujioka, Tomoaki, Abe, Akira, Matsunami, Maya, and Shimono, Hiroyuki

Subjects
*PLANT fertility, *MALE sterility in plants, *RICE, *MORPHOLOGY, *POLLEN, *CULTIVARS
Abstract

• We evaluated cold tolerance for inducing male sterility of 18 Ethiopian rice cultivars. • Spikelet fertility under cold stress ranged from 0 % to 90 % at phenotyping facilities. • This variation was explained by anther length and pollen number per anther. • Anther length and pollen number without cold stress can be used for prescreening. Male sterility induced by low temperatures during reproductive development is the major constraint on rice production in Ethiopia, which generally lies at high elevations. Because of a lack of phenotyping facilities, limited information is available on the cold tolerance of Ethiopian germplasm. We evaluated the genotypic variation in cold tolerance of 18 Ethiopian rice cultivars in two phenotyping facilities and characterized their cold tolerance in relation to their reproductive morphology in a 2-year trial in Japan. Genotypic variation in spikelet fertility was high after exposure to cold during reproductive development at both facilities, with fertility ranging from 0% to 90 %. 'Andassa' and 'Tana' had the highest fertility and 'Fogera 2' and 'Getachew' had the lowest. The two cold-tolerant germplasms had tolerance similar to that of the Japanese 'Hitomebore' (strong), whereas the susceptible germplasms had tolerance similar to that of the Japanese 'Sasanishiki' (weak). The variation in spikelet fertility was explained by both anther length and number of fertile pollen grains per anther under cold stress, and by anther length under unstressed control conditions in both years of the study; longer anther length and higher fertile pollen number leads to stronger cold tolerance. Our results suggest that anther length under unstressed conditions offers a pre-screening criterion for cold tolerance without requiring phenotyping facilities for screening. [ABSTRACT FROM AUTHOR]

Published
2021
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540. Latitudinal adaptation and dispersal pathway of foxtail millet suggested by geographical distribution of transposable elements inserted in the SiPRR37 gene.

Author

Fukunaga K, Abe A, Ito K, Oikawa K, Tsuji M, and Kawase M

Subjects
Plant Proteins genetics, Alleles, Adaptation, Physiological genetics, Genes, Plant, Setaria Plant genetics, DNA Transposable Elements genetics
Abstract

We investigated the variation and geographical distribution of the Pseudo-regulator response 37 (Setaria italica PRR37; SiPRR37) gene, which is involved in heading time (photoperiodism) in foxtail millet. An allele of the SiPRR37 gene, in which an approximately 4.9-kb transposable element (designated TE1) is inserted (a loss-of-function or reduction-of-function type), is distributed sporadically in East Asia and broadly in Southeast Asia and South Asia, implying that this gene is important in latitudinal adaptation. In addition, we found a new allele of SiPRR37 with an insertion of a 360-bp TE (TE2) at this locus and investigated the geographical distribution of this new type. This SiPRR37 allele with TE2 is distributed in Japan, Korea, Nepal, Iran and Turkey. Both TE1 and TE2 are useful markers for tracing foxtail millet dispersal pathways in Asia.

Published
2024
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541. The role of lysosomal phospholipase A2 in the catabolism of bis(monoacylglycerol)phosphate and association with phospholipidosis.

Author

Abe A, Hinkovska-Galcheva V, Bouchev P, Bouley R, and Shayman JA

Subjects
Humans, Animals, Mice, Phospholipases A2 metabolism, Phospholipids metabolism, Liposomes metabolism, Lipidoses metabolism, Lipidoses chemically induced, Lipidoses enzymology, Lysosomes metabolism, Lysosomes enzymology, Monoglycerides metabolism, Lysophospholipids metabolism
Abstract

Bis(monoacylglycerol)phosphate (BMP) is an acidic glycerophospholipid localized to late endosomes and lysosomes. However, the metabolism of BMP is poorly understood. Because many drugs that cause phospholipidosis inhibit lysosomal phospholipase A2 (LPLA2, PLA2G15, LYPLA3) activity, we investigated whether this enzyme has a role in BMPcatabolism. The incubation of recombinant human LPLA2 (hLPLA2) and liposomes containing the naturally occurring BMP (sn-(2-oleoyl-3-hydroxy)-glycerol-1-phospho-sn-1'-(2'-oleoyl-3'-hydroxy)-glycerol (S,S-(2,2',C 18:1 )-BMP) resulted in the deacylation of this BMP isomer. The deacylation rate was 70 times lower than that of dioleoyl phosphatidylglycerol (DOPG), an isomer and precursor of BMP. The release rates of oleic acid from DOPG and four BMP stereoisomers by LPLA2 differed. The rank order of the rates of hydrolysis were DOPG>S,S-(3,3',C 18:1 )-BMP>R,S-(3,1',C 18:1 )-BMP>R,R-(1,1',C 18:1 )>S,S-(2,2')-BMP. The cationic amphiphilic drug amiodarone (AMD) inhibited the deacylation of DOPG and BMP isomers by hLPLA2 in a concentration-dependent manner. Under these experimental conditions, the IC 50 s of amiodarone-induced inhibition of the four BMP isomers and DOPG were less than 20 μM and approximately 30 μM, respectively. BMP accumulation was observed in AMD-treated RAW 264.7 cells. The accumulated BMP was significantly reduced by exogenous treatment of cells with active recombinant hLPLA2 but not with diisopropylfluorophosphate-inactivated recombinant hLPLA2. Finally, a series of cationic amphiphilic drugs known to cause phospholipidosis were screened for inhibition of LPLA2 activity as measured by either the transacylation or fatty acid hydrolysis of BMP or phosphatidylcholine as substrates. Fifteen compounds demonstrated significant inhibition with IC 50 s ranging from 6.8 to 63.3 μM. These results indicate that LPLA2 degrades BMP isomers with different substrate specificities under acidic conditions and may be the key enzyme associated with BMP accumulation in drug-induced phospholipidosis., Competing Interests: Conflict of interests The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper. The author is an Editorial Board Member/Editor-in-Chief/Associate Editor/Guest Editor for The Journal of Lipid Research and was not involved in the editorial review or the decision to publish this article., (Copyright © 2024 The Authors. Published by Elsevier Inc. All rights reserved.)

Published
2024
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542. Modulation of hepatic transcription factor EB activity during cold exposure uncovers direct regulation of bis(monoacylglycero)phosphate lipids by Pla2g15 .

Author

Jain R, Geoghegan G, Davidson J, Nesbitt DJ, Abe A, Chao X, James I, Cavanagh A, Michorowska S, Verma R, Scheuler K, Hinkovska-Galcheva V, Shishkova E, Ding WX, Coon JJ, Shayman JA, and Simcox JA

Abstract

Cold exposure is an environmental stress that elicits a rapid metabolic shift in endotherms and is required for survival. The liver provides metabolic flexibility through its ability to rewire lipid metabolism to respond to an increased demand in energy for thermogenesis. We leveraged cold exposure to identify novel lipids contributing to energy homeostasis and found that lysosomal bis(monoacylglycero)phosphate (BMP) lipids were significantly increased in the liver during acute cold exposure. BMP lipid changes occurred independently of lysosomal abundance but were dependent on the lysosomal transcriptional regulator transcription factor EB (TFEB). Knockdown of TFEB in hepatocytes decreased BMP lipid levels. Through molecular biology and biochemical assays, we found that TFEB regulates lipid catabolism during cold exposure and that TFEB knockdown mice were cold intolerant. To identify how TFEB regulates BMP lipid levels, we used a combinatorial approach to identify TFEB target Pla2g15 , a lysosomal phospholipase, as capable of degrading BMP lipids in in vitro liposome assays. Knockdown of Pla2g15 in hepatocytes led to a decrease in BMP lipid species. Together, our studies uncover a required role of TFEB in mediating lipid liver remodeling during cold exposure and identified Pla2g15 as an enzyme that regulates BMP lipid catabolism.

Published
2023
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543. V-primer: software for the efficient design of genome-wide InDel and SNP markers from multi-sample variant call format (VCF) genotyping data.

Author

Natsume S, Oikawa K, Nomura C, Ito K, Utsushi H, Shimizu M, Terauchi R, and Abe A

Abstract

DNA markers are indispensable tools in genetics and genomics research as well as in crop breeding, particularly for marker-assisted selection. Recent advances in next-generation sequencing technology have made it easier to obtain genome sequences for various crop species, enabling the large-scale identification of DNA polymorphisms among varieties, which in turn has made DNA marker design more accessible. However, existing primer design software is not suitable for designing many types of genome-wide DNA markers from next-generation sequencing data. Here, we describe the development of V-primer, high-throughput software for designing insertion/deletion, cleaved amplified polymorphic sequence, and single-nucleotide polymorphism (SNP) markers. We validated the applicability of these markers in different crops. In addition, we performed multiplex PCR targeted amplicon sequencing using SNP markers designed with V-primer. Our results demonstrate that V-primer facilitates the efficient and accurate design of primers and is thus a useful tool for genetics, genomics, and crop breeding. V-primer is freely available at https://github.com/ncod3/vprimer., (Copyright © 2023 by JAPANESE SOCIETY OF BREEDING.)

Published
2023
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544. Upcycling rice yield trial data using a weather-driven crop growth model.

Author

Shimono H, Abe A, Kim CH, Sato C, and Iwata H

Subjects
Plant Breeding, Climate Change, Genome-Wide Association Study, Weather, Oryza genetics
Abstract

Efficient plant breeding plays a significant role in increasing crop yields and attaining food security under climate change. Screening new cultivars through yield trials in multi-environments has improved crop yields, but the accumulated data from these trials has not been effectively upcycled. We propose a simple method that quantifies cultivar-specific productivity characteristics using two regression coefficients: yield-ability (β) and yield-plasticity (α). The recorded yields of each cultivar are expressed as a unique linear regression in response to the theoretical potential yield (Y p ) calculated by a weather-driven crop growth model, called as the "YpCGM method". We apply this to 72510 independent datasets from yield trials of rice that used 237 cultivars measured at 110 locations in Japan over 38 years. The YpCGM method can upcycle accumulated yield data for use in genetic-gain analysis and genome-wide-association studies to guide future breeding programs for developing new cultivars suitable for the world's changing climate., (© 2023. The Author(s).)

Published
2023
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545. Whole-genome analysis of recombinant inbred rice lines reveals a quantitative trait locus on chromosome 3 with genotype-by-environment interaction effects.

Author

Sakai T, Fujioka T, Uemura T, Saito S, Terauchi R, and Abe A

Subjects
Humans, Chromosome Mapping methods, Gene-Environment Interaction, Chromosomes, Human, Pair 3, Genotype, Phenotype, Crops, Agricultural genetics, Quantitative Trait Loci, Oryza genetics
Abstract

Elucidating genotype-by-environment interactions is fundamental for understanding the interplay between genetic and environmental factors that shape complex traits in crops. Genotype-by-environment interactions are of practical importance, as they determine the performance of cultivars grown in different environments, prompting the need for an efficient approach for evaluating genotype-by-environment interactions. Here, we describe a method for genotype-by-environment detection that involves comparing linear mixed models. This method successfully detected genotype-by-environment interactions in rice (Oryza sativa) recombinant inbred lines grown at 3 locations. We identified a quantitative trait locus (QTL) on chromosome 3 that was associated with heading date, grain number, and leaf length. The effect of this QTL on plant growth-related traits varied with environmental conditions, indicating the presence of genotype-by-environment interactions. Therefore, our method enables a powerful genotype-by-environment detection pipeline that should facilitate the production of high-yielding crops in a given environment., Competing Interests: Conflicts of interest The author(s) declare no conflict of interest., (© The Author(s) 2023. Published by Oxford University Press on behalf of The Genetics Society of America.)

Published
2023
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546. Isolation of Pikps, an allele of Pik, from the aus rice cultivar Shoni.

Author

Kovi B, Sakai T, Abe A, Kanzaki E, Terauchi R, and Shimizu M

Subjects
Alleles, Oryza genetics, Magnaporthe genetics, Ascomycota genetics
Abstract

Blast disease caused by the filamentous fungus Pyricularia oryzae (syn. Magnaporthe oryzae) is one of the most destructive diseases of rice (Oryza sativa L.) around the globe. An aus cultivar, Shoni, showed resistance against at least four Japanese P. oryzae isolates. To understand Shoni's resistance against the P. oryzae isolate Naga69-150, genetic analysis was carried out using recombinant inbred lines developed by a cross between Shoni and the japonica cultivar Hitomebore, which is susceptible to Naga69-150. The result indicated that the resistance was controlled by a single locus, which was named Pi-Shoni. A QTL analysis identified Pi-Shoni as being located in the telomeric region of chromosome 11. A candidate gene approach in the region indicated that Pi-Shoni corresponds to the previously cloned Pik locus, and we named this allele Pikps. Loss of gene function mediated by RNA interference demonstrated that a head-to-head-orientated pair of NBS-LRR receptor genes (Pikps-1 and Pikps-2) are required for the Pikps-mediated resistance. Amino acid sequence comparison showed that Pikps-1 is 99% identical to Pikp-1, while Pikps-2 is identical to Pikp-2. Pikps-1 had one amino acid substitution (Pro351Ser) in the NBS domain as compared to Pikp-1. The recognition specificity of Pikps against known AVR-Pik alleles is identical to that of Pikp.

Published
2023
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547. A genetically linked pair of NLR immune receptors shows contrasting patterns of evolution.

Author

Shimizu M, Hirabuchi A, Sugihara Y, Abe A, Takeda T, Kobayashi M, Hiraka Y, Kanzaki E, Oikawa K, Saitoh H, Langner T, Banfield MJ, Kamoun S, and Terauchi R

Subjects
Genetic Linkage, Host-Pathogen Interactions immunology, Protein Inhibitors of Activated STAT genetics, Protein Inhibitors of Activated STAT immunology, Evolution, Molecular, Magnaporthe genetics, Magnaporthe pathogenicity, NLR Proteins genetics, NLR Proteins immunology, Oryza immunology, Oryza microbiology, Plant Diseases immunology, Plant Diseases microbiology, Plant Proteins genetics, Plant Proteins immunology, Receptors, Immunologic genetics, Receptors, Immunologic immunology
Abstract

Throughout their evolution, plant nucleotide-binding leucine-rich-repeat receptors (NLRs) have acquired widely divergent unconventional integrated domains that enhance their ability to detect pathogen effectors. However, the functional dynamics that drive the evolution of NLRs with integrated domains (NLR-IDs) remain poorly understood. Here, we reconstructed the evolutionary history of an NLR locus prone to unconventional domain integration and experimentally tested hypotheses about the evolution of NLR-IDs. We show that the rice ( Oryza sativa ) NLR Pias recognizes the effector AVR-Pias of the blast fungal pathogen Magnaporthe oryzae . Pias consists of a functionally specialized NLR pair, the helper Pias-1 and the sensor Pias-2, that is allelic to the previously characterized Pia pair of NLRs: the helper RGA4 and the sensor RGA5. Remarkably, Pias-2 carries a C-terminal DUF761 domain at a similar position to the heavy metal-associated (HMA) domain of RGA5. Phylogenomic analysis showed that Pias-2/RGA5 sensor NLRs have undergone recurrent genomic recombination within the genus Oryza , resulting in up to six sequence-divergent domain integrations. Allelic NLRs with divergent functions have been maintained transspecies in different Oryza lineages to detect sequence-divergent pathogen effectors. By contrast, Pias-1 has retained its NLR helper activity throughout evolution and is capable of functioning together with the divergent sensor-NLR RGA5 to respond to AVR-Pia. These results suggest that opposite selective forces have driven the evolution of paired NLRs: highly dynamic domain integration events maintained by balancing selection for sensor NLRs, in sharp contrast to purifying selection and functional conservation of immune signaling for helper NLRs.

Published
2022
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548. High-performance pipeline for MutMap and QTL-seq.

Author

Sugihara Y, Young L, Yaegashi H, Natsume S, Shea DJ, Takagi H, Booker H, Innan H, Terauchi R, and Abe A

Subjects
Chromosome Mapping methods, Phenotype, Quantitative Trait Loci genetics, Software
Abstract

Summary: Bulked segregant analysis implemented in MutMap and QTL-seq is a powerful and efficient method to identify loci contributing to important phenotypic traits. However, the previous pipelines were not user-friendly to install and run. Here, we describe new pipelines for MutMap and QTL-seq. These updated pipelines are approximately 5-8 times faster than the previous pipeline, are easier for novice users to use, and can be easily installed through bioconda with all dependencies., Availability: The new pipelines of MutMap and QTL-seq are written in Python and can be installed via bioconda. The source code and manuals are available online (MutMap: https://github.com/YuSugihara/MutMap, QTL-seq: https://github.com/YuSugihara/QTL-seq)., Competing Interests: The authors declare there are no competing interests., (©2022 Sugihara et al.)

Published
2022
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549. Recombinant inbred lines and next-generation sequencing enable rapid identification of candidate genes involved in morphological and agronomic traits in foxtail millet.

Author

Fukunaga K, Abe A, Mukainari Y, Komori K, Tanaka K, Fujihara A, Yaegashi H, Kobayashi M, Ito K, Ohsako T, and Kawase M

Subjects
Genome, Plant, High-Throughput Nucleotide Sequencing, Homeodomain Proteins genetics, Hordeum genetics, Inbreeding, Japan, Phenotype, Plant Breeding, Plant Proteins genetics, Quantitative Trait Loci, Setaria Plant growth & development, Taiwan, Chromosomes, Plant genetics, Setaria Plant genetics
Abstract

We constructed recombinant inbred lines (RILs) between a Japanese and a Taiwanese landrace of foxtail millet and employed next-generation sequencing, such as flexible ddRAD-seq and Nanopore sequencing to identify the candidate genes involved in the crop evolution of foxtail millet. We successfully constructed a linkage map using flexible ddRAD-seq with parents and RILs and detected major QTLs for each of three traits: leaf sheath colors, spikelet-tipped bristles (stb), and days to heading (DTH). (1) For leaf sheath colors, we identified the C gene on chromosome IV. (2) We identified a homeobox (HOX14) gene for stb on chromosome II, which shows homology with HvVrs1 in barley. (3) Finally, we identified a QTL with a large effect on DTH on chromosome II. A parent of the RILs from Taiwan and Yugu1 had a Harbinger-like TE in intron 3 of this gene. We also investigated the geographical distribution of the TE insertion type of this gene and found that the insertion type is distributed in the northern part of East Asia and intensively in South and Southeast Asia, suggesting that loss/reduction of function of this gene plays an important role in spreading into the northern part of East Asia and subtropical and tropical zones., (© 2022. The Author(s).)

Published
2022
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550. RIL-StEp: epistasis analysis of rice recombinant inbred lines reveals candidate interacting genes that control seed hull color and leaf chlorophyll content.

Author

Sakai T, Abe A, Shimizu M, and Terauchi R

Subjects
Chlorophyll genetics, Epistasis, Genetic, Quantitative Trait Loci, Seeds genetics, Plant Leaves genetics, Phenotype, Oryza genetics
Abstract

Characterizing epistatic gene interactions is fundamental for understanding the genetic architecture of complex traits. However, due to the large number of potential gene combinations, detecting epistatic gene interactions is computationally demanding. A simple, easy-to-perform method for sensitive detection of epistasis is required. Due to their homozygous nature, use of recombinant inbred lines excludes the dominance effect of alleles and interactions involving heterozygous genotypes, thereby allowing detection of epistasis in a simple and interpretable model. Here, we present an approach called RIL-StEp (recombinant inbred lines stepwise epistasis detection) to detect epistasis using single-nucleotide polymorphisms in the genome. We applied the method to reveal epistasis affecting rice (Oryza sativa) seed hull color and leaf chlorophyll content and successfully identified pairs of genomic regions that presumably control these phenotypes. This method has the potential to improve our understanding of the genetic architecture of various traits of crops and other organisms., (© The Author(s) 2021. Published by Oxford University Press on behalf of Genetics Society of America.)

Published
2021
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