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201. Gypsophilin, a New Type 1 Ribosome-inactivating Protein from Gypsophila elegans: Purification, Enzymatic Characterization, and Subcellular Localization

Author

Yoshinari, Shigeo, Koresawa, Shigehiro, Yokota, Sadaki, Sawamoto, Hiroshi, Tamura, Minoru, and Endo, Yaeta

Abstract

Gypsophila eleganscontains a new type 1 ribosome-inactivating protein, which we named gypsophilin. The protein was purified to apparent homogeneity by (NH4)2SO4fractionation, ion-exchange chromatography, and adsorption chromatography. The protein was found to have a molecular mass of 28.0 kDa and a pIof about 10.1. It does not contain glycosidic linkages. The sequence of the N-terminal 22 amino acids of the protein shows a close relationship to other RIPs. The enzyme strongly inhibits protein synthesis in a rabbit reticulocyte lysate and depurinates 28S rRNA in rat liver ribosomes in a manner identical to that of ricin A-chain and other RIPs. Using a direct method for the measurement of the RNA N-glycosidase activity, the substrate spcificity of gypsophilin was identified. EC50of the protein for ribosomes of rat liver, wheat germ, and E. coliwas 39.8 pm, 0.24 nm, and 0.82 μμ, respectively. Gypsophilin may be one of the most active RNA N-glycosidases among the RIPs known to date. Immunoelectron microscopic localization of gypsophilin in the leaves shows that the protein is accumulated densely in the intercellular spaces and is also distributed within vacuoles in the cytoplasm.

Published
1997
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202. Mechanisms of Action of Ribotoxins

Author

Endo, Yaeta, Morishita, Ryo, Imashevich, Kairat Madin, and Yoshinari, Shigeo

Abstract

AbstractThe ribotoxins α-sarcin and ricin and their homologs catalyze covalent modifications in adjacent nucleotides in the large RNA of ribosomes. α-Sarcin is a ribonuclease that cleaves the phosphodiester bond on the 3’ side of G4325 in a universal, 14-nucleotide, purine-rich sequence in 28SrRNA. The A-chain of ricin and of other related toxins such as Shiga toxin and Vero toxin is a RNA N-glycosidase that catalyses the depurination of the 5’ adjacent A4324. There are nearly 7000 nucleotides in mammalian ribosomes. The toxins, however, catalyze only a single covalent modification that inactivates the ribosomes and is entirely responsible for the toxicity.

Published
1998
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203. The mechanism of action of the cytotoxic lectin from Phoradendron californicum: The RNA N-glycosidase activity of the protein

Author

Endo, Yaeta, Oka, Tatsuzo, Tsurugi, Kunio, and Franz, Hartmut

Abstract

A toxic lectin from Phoradendron californicum(PCL) was found to inactivate catalytically 60 S ribosomal subunits of rabbit reticulocytes, resulting in the inhibition of protein synthesis. To study the mechanism of action of PCL, rat liver ribosomes were treated with the toxin and the extracted rRNA was treated with aniline. A fragment containing about 450 nucleotides was released from the 28 S rRNA. Analysis of the nucleotide sequence of the fragment revealed that the aniline-sensitive phosphodiester bond was between A4324 and G4325 of the 28 S rRNA. These results indicate that PCL inactivates the ribosomes by cleaving an N-glycosidic bond at A4324 of 28 S rRNA in the ribosomes as does ricin A-chain.

Published
1989
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215. The site of action of the A-chain of mistletoe lectin I on eukaryotic ribosomes The RNA N-glycosidase activity of the protein

Author

Endo, Yaeta, Tsurugi, Kunio, and Franz, Hartmut

Abstract

The site of action of the A-chain of mistletoe lectin (ML-A) from Viscum albumon eukaryotic ribosomes was studied. Treatment of rat liver ribosomes with ML-A, followed by treatment of the isolated rRNA with aniline, caused the release of a fragment with about 450 nucleotides from 28 S rRNA. Further analysis of nucleotide sequences of this fragment revealed that the aniline-sensitive site of phosphodiester bond was between positions A-4324 and G-4325 in 28 S rRNA. These results indicate that ML-A inactivates the ribosomes by cleaving a N-glycosidic bond at A-4324 of 28 S rRNA in the ribosomes as ricin A-chain does.

Published
1988
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216. Production of monoclonal antibodies against GPCR using cell-free synthesized GPCR antigen and biotinylated liposome-based interaction assay.

Author

Takeda, Hiroyuki, Ogasawara, Tomio, Ozawa, Tatsuhiko, Muraguchi, Atsushi, Jih, Pei-Ju, Morishita, Ryo, Uchigashima, Motokazu, Watanabe, Masahiko, Fujimoto, Toyoshi, Iwasaki, Takahiro, Endo, Yaeta, and Sawasaki, Tatsuya

Subjects
MONOCLONAL antibodies, G protein coupled receptors, MONOCLONAL antibody probes, LIPOSOMES, HEMODIALYSIS
Abstract

G-protein-coupled receptors (GPCRs) are one of the most important drug targets, and anti-GPCR monoclonal antibody (mAb) is an essential tool for functional analysis of GPCRs. However, it is very difficult to develop GPCR-specific mAbs due to difficulties in production of recombinant GPCR antigens, and lack of efficient mAb screening method. Here we describe a novel approach for the production of mAbs against GPCR using two original methods, bilayer-dialysis method and biotinylated liposome-based interaction assay (BiLIA), both of which are developed using wheat cell-free protein synthesis system and liposome technology. Using bilayer-dialysis method, various GPCRs were successfully synthesized with quality and quantity sufficient for immunization. For selection of specific mAb, we designed BiLIA that detects interaction between antibody and membrane protein on liposome. BiLIA prevented denaturation of GPCR, and then preferably selected conformation-sensitive antibodies. Using this approach, we successfully obtained mAbs against DRD1, GHSR, PTGER1 and T1R1. With respect to DRD1 mAb, 36 mouse mAbs and 6 rabbit mAbs were obtained which specifically recognized native DRD1 with high affinity. Among them, half of the mAbs were conformation-sensitive mAb, and two mAbs recognized extracellular loop 2 of DRD1. These results indicated that this approach is useful for GPCR mAb production. [ABSTRACT FROM AUTHOR]

Published
2015
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217. Production of yeast (m2G10) methyltransferase (Trm11 and Trm112 complex) in a wheat germ cell-free translation system

Author

Okada, Kazuki, Muneyoshi, Yuki, Endo, Yaeta, and Hori, Hiroyuki

Abstract

Transfer RNA (guanine-N2-)–methyltransferase [tRNA (m2G10) methyltransferase] catalyzes a methyl-transfer from S-adenosyl-<$O_SCPLOW>L<$C_SCPLOW>-methionine to N2-atom of guanine at position 10 (G10) in tRNA and generates N2-methylguanine at position 10 (m2G10). Yeast enzyme contains two protein subunits (Trm11 and Trm112). Trm11 protein is expected to be a catalytic subunit and Trm112 contains a Zinc-finger. In yeast cells, Trm112 binds not only to Trm11 but also to other proteins such as Lys9, Trm9, and Mtq2. Therefore, the Trm112 protein may regulate population of several protein complexes. To address these issues, we started the study on synthesis of Trm112 related protein complexes. In this meeting, we report synthesis of active Trm11-Trm112 complex in a wheat germ cell-free translation system.

Published
2009
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218. Hetero subunit interaction and RNA recognition of yeast tRNA (m7G46) methyltransferase synthesized in a wheat germ cell-free translation system

Author

Muneyoshi, Yuki, Matsumoto, Keisuke, Tomikawa, Chie, Toyooka, Takashi, Ochi, Anna, Masaoka, Takashi, Endo, Yaeta, and Hori, Hiroyuki

Abstract

Yeast tRNA (m7G46) methyltransferase contains two protein subunits (Trm8 and Trm82). The enzyme catalyzes a methyl-transfer from S-adenosyl-L-methionine to the N7 atom of guanine at position 46 in tRNA. We deviced synthesis of active Trm8-Trm82 heterodimer in a wheat germ cell-free translation system. When Trm8 or Trm82 mRNA were used for a synthesis, Trm8 or Trm82 protein could be synthesized. Upon mixing the synthesized Trm8 and Trm82 proteins, no active Trm8-Trm82 heterodimer was produced. Active Trm8-Trm82 heterodimer was only synthesized under conditions, in which both Trm8 and Trm82 mRNAs were co-translated. To address the RNA recognition mechanism of the Trm8-Trm82 complex, we investigated methyl acceptance activities of eight truncated yeast tRNAPhe transcripts. In this meeting, we demonstrate that yeast Trm8-Trm82 has stricter recognition requirements for the tRNA molecule as compared to the bacterial enzyme, TrmB.

Published
2007
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220. Purification of eukaryotic translation factors from wheat germ for reconstitution of protein synthesis

Author

Nagano, Hikaru, Sugihara, Shouhei, Takagi, Hisanori, Ogasawara, Tomio, Endo, Yaeta, and Takai, Kazuyuki

Abstract

The wheat germ cell-free protein synthesis is a powerful and versatile method for preparation of proteins based on the accumulated DNA sequence information. As the cell extract used for it contains many factors that are unknown or do not directly involve in protein synthesis, details of the translation reaction is yet to be understood. Therefore, we have decided to try reconstitution ofprotein synthesis, which would be useful for better understanding of the mechanisms supporting eukaryotic protein synthesis and translational regulation and probably applicable to synthetic biology. In the present study, we fractionated an extract from crude wheat germ according to published protocols to obtain the fractions containing the eukaryoticelongation factors (eEFs) 1A, 1B, and 2. The eEF1A and eEF2 fractions supported polyphenylalanine synthesis.

Published
2008
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222. Identification of Aquifex aeolicus tRNA (m22G26) methyltransferase gene

Author

Takeda, Hiroshi, Hori, Hiroyuki, and Endo, Yaeta

Abstract

The modifications of N2,N2-dimethylguanine (m2&lt;inf>2&lt;/inf>G) are found in tRNAs and rRNAs from eukarya and archaea. In tRNAs, modification at position G26 is generated by tRNA (m2&lt;inf>2&lt;/inf>G26) methyltransferase, which is encoded by the corresponding gene, &lt;it>trm1&lt;/it>. This enzyme catalyzes the methyl-transfer from S-adenosyl-L-methionine to the semi-conserved residue, G26, via the intermediate modified base, m2G26. Recent genome sequencing project has been reported that the putative &lt;it>trm1&lt;/it> is encoded in the genome of &lt;it>Aquifex aeolicus&lt;/it>, a hyper-thermophilic eubacterium as only one exception among eubacteria. In order to confirm whether this bacterial &lt;it>trm1&lt;/it> gene product is a real tRNA (m2&lt;inf>2&lt;/inf>G26) methyltransferase or not, we expressed this protein by wheat germ &lt;it>in vitro&lt;/it> cell-free translation system. Our biochemical analysis clearly showed that this gene product possessed tRNA (m2&lt;inf>2&lt;/inf>G26) methyltransferase activity.

Published
2002
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223. Identification of essential amino acid residues of tRNA (Gm18)methyltransferase for methyl-transfer activity

Author

Watanabe, Kazunori, Hori, Hiroyuki, and Endo, Yaeta

Abstract

Recent computation analyses have pointed out an existence of conserved amino add motifs among RNA ribose 2′-O-methyltransferases. However, the functions of these motifs are unclear yet We carried out the site-directed mutagenesis studies systematically on &lt;it>Thermus thermophilus&lt;/it> HB8 tRNA (Gml8) methyltransferase gene. Subsequent biochemical analyses with purified variant enzymes clearly revealed that five conserved amino add residues (Asn35, Arg41, Glul24, Serl50, and Asnl52) are involved in S-adenosyl-L-methionine binding. This is for the first time reporting the function of the conserved motifs among RNA ribose 2′-O-methyltransferases.

Published
2001
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224. Construction of an efficient expression vector for coupled transcription/translation in a wheat germ cell-free system

Author

Sawasaki, Tatsuya, Hasegawa, Yoshinori, Tsuchimochi, Masateru, Kasahara, Yuko, and Endo, Yaeta

Abstract

Using the expression vector, pEU, which we have constructed, highly efficient in vitro protein synthesis can be achieved: The system works for 150 hours and without further template addition once the reaction has started, yielding 5 mg of enzymatically active protein in a 1 ml reaction.

Published
2000
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225. Mechanism of ribosome RNA apurinic site specific lyase

Author

Sawasaki, Tatsuya, Morishita, Ryo, Ozawa, Akihiko, Ogasawara, Tomio, Madin, Kairat, and Endo, Yaeta

Abstract

A new enzyme, which we named ribosome RNA apurinic site specific lyase (RALyase), has been characterized. The enzyme specifically cleaves a phosphodiester bond at the apurinic site in the sarcin/ricin domain of 28S rRNA in ribosomes. The cut ends of wheat 28S rRNA were determined as 5′—GUACG-α-hydroxy-α, β-unsaturated aldehyde and pGAGGA—3′ for the 3′ fragment, demonstrating that the enzyme catalyzes the β-elimination reaction.

Published
1999
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226. The ribosomal RNA identity elements for ricin and for {alpha}-sarcin: mutations in the putative CG pair that closes a GAGA tetraloop

Author

Glück, Anton, Endo, Yaeta, and Wool, Ira G.

Abstract

α-Sarcin is a ribonuclease that cleaves the phosphodiester bond on the 3′ side of G4325 in 28S rRNA; ricin A-chain is a RNA N-glycosidase that depurinates the 5′ adjacent A4324. These single covalent modifications Inactivate the ribosome. An oligoribonucleotide that reproduces the structure of the sarcin/ricin domain in 28S rRNA was synthesized and mutations were constructed in the 5′ C and the 3′ G that surround a GAGA tetrad that has the sites of toxin action. Covalent modification of the RNA by ricin, but not by α-sarcin, requires a Watson-Crick pair to shut off a putative GAGA tetraloop. Either the recognition elements for the two toxins are different despite their catalyzing covalent modification of adjacent nucleotides in 28S rRNA or there are transitions in the conformation of the α-sarcin/ricin domain in 28S rRNA and one conformer is recognized by α-sarcin and the other by ricin A-chain.

Published
1994
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227. Stress-Inducible Caspase Substrate TRB3 Promotes Nuclear Translocation of Procaspase-3.

Author

Shimizu, Kouhei, Takahama, Shoukichi, Endo, Yaeta, Sawasaki, Tatsuya, and Chandra, Dhyan

Subjects
*NUCLEAR proteins, *APOPTOSIS, *CASPASES, *CELL death, *CELLS, *CYTOPLASM
Abstract

Pseudokinase TRB3 is a stress-inducible nuclear protein, which has recently been shown to be involved in ER stress-induced apoptosis. However, it remains unclear how TRB3 contributes to the process. We recently demonstrated that TRB3 was cleaved by caspase-3 (CASP3) in vitro and also in apoptosis- induced cells. Thus, we investigate the role of TRB3 cleavage in the apoptotic process to address the above question. Overexpression studies revealed that the cleavage of TRB3 promoted CASP3/7 activation and apoptosis. In contrast, the anti-apoptotic effects were found under TRB3 non-cleavable conditions, such as ER stress, and also when the CASP3/7 activation was enhanced by knockdown of endogenous TRB3 expression. Interestingly, nuclear translocation of procaspase-3 (proCASP3) was observed in cells either overexpressing TRB3 or under tunicamycin-induced ER stress. Although forced cytoplasmic expression of proCASP3 enhanced apoptosis significantly, its nuclear expression did not produce any pro-apoptotic effect, suggesting that nuclear distribution of proCASP3 is not critical for the execution of apoptosis. Thus, TRB3 might prevent cytoplasmic activation of CASP3 by promoting proCASP3 entry into the nucleus, and thereby inhibit apoptosis. Taken together, our results suggest that TRB3, through its own cleavage, functions as a molecular switch between the cell survival and apoptotic pathways under stressful conditions. [ABSTRACT FROM AUTHOR]

Published
2012
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228. Use of domain enzymes from wheat RNA ligase for in vitro preparation of RNA molecules

Author

Makino, Shin-ichi, Sawasaki, Tatsuya, Endo, Yaeta, and Takai, Kazuyuki

Subjects
*LIGASES, *WHEAT, *PHOSPHATES, *PHOSPHODIESTERASES, *MASS spectrometry, *CATALYTIC RNA, *RNA, *ENZYME analysis
Abstract

Abstract: Wheat RNA ligase can be dissected into three isolated domain enzymes that are responsible for its core ligase, 5′-kinase, and 2′,3′-cyclic phosphate 3′-phosphodiesterase activities, respectively. In the present study, we pursued a practical strategy using the domain enzymes for in vitro step-by-step ligation of RNA molecules. As a part of it, we demonstrated that a novel side reaction on 5′-tri/diphosphate RNAs is dependent on ATP, a 2′-phosphate-3′-hydroxyl end, and the ligase domain. Mass spectroscopy and RNA cleavage analyses strongly suggested that it is an adenylylation on the 5′ terminus. The ligase domain enzyme showed a high productivity for any of the possible 16 combinations of terminal bases and a high selectivity for the 5′-phosphate and 2′-phosphate-3′-hydroxyl ends. Two RNA molecules having 5′-hydroxyl and 2′,3′-cyclic monophosphate groups were ligated almost stoichiometrically after separate conversion of respective terminal phosphate states into reactive ones. As the product has the same terminal state as the starting material, the next rounds of ligation are also possible in principle. Thus, we propose a flexible method for in vitro RNA ligation. [Copyright &y& Elsevier]

Published
2011
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229. In vitro dissection revealed that the kinase domain of wheat RNA ligase is physically isolatable from the flanking domains as a non-overlapping domain enzyme

Author

Makino, Shin-ichi, Sawasaki, Tatsuya, Endo, Yaeta, and Takai, Kazuyuki

Subjects
*LIGASES, *CATALYTIC RNA, *PROTEIN structure, *WHEAT, *PROTEIN synthesis, *NUCLEOTIDE sequence, *GENE expression
Abstract

Abstract: Wheat RNA ligase contains 5′-hydroxyl kinase, 2′,3′-cyclic phosphate 3′-phosphodiesterase, and 5′-phosphate 2′-phosphate-3′-hydroxyl RNA ligase activities in a 110-kDa polypeptide. Taking advantage of a wheat cell-free protein production system, we prepared various fragments containing a part of the enzyme. The method allowed us to check the activities of the fragments rapidly, eliminating the time-consuming cloning and sequencing steps for the expression of the fragment proteins. The results showed that each of the three activities can be assigned to a non-overlapping domain that does not require the presence of the other part(s) of the enzyme for its activity. This contrasts to the case of yeast tRNA ligase, in which the central kinase domain has been suggested to require to be tethered to one of the flanking domains for its activity. [Copyright &y& Elsevier]

Published
2010
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230. RIP and RALyase cleave the sarcin/ricin domain, a critical domain for ribosome function, during senescence of wheat coleoptiles

Author

Sawasaki, Tatsuya, Nishihara, Masahiro, and Endo, Yaeta

Subjects
*ADENINE, *CYTOPLASM, *RIBOSOMES, *PHENOTYPES
Abstract

Abstract: Type-I ribosome-inactivating protein (RIP), which is found in many plants, catalyzes depurination of a specific adenine in the sarcin/ricin domain (SRD) of the large rRNA causing loss of ribosomal activity. Previously, we found a RNA apurinic site-specific lyase (RALyase) that catalytically cleaved the phosphodiester bond at the RIP-dependent depurination site by β-elimination reaction. Here we show that both the RIP activity and RIP–RALyase-mediated cleavage of SRD in the cytoplasmic ribosome were induced at the late stage of senescence of wheat coleoptiles. Following this process, tissue death was observed. Furthermore, transgenic tobacco plants expressing glucocorticoid-induced RIP developed senescence-like phenotype. Our results suggest that ribosome inactivation due to the cleavage of SRD by the inducible RIP and constitutively expressed RALyase may be a unique plant system that mediates programmed cell death at the late senescent stage. [Copyright &y& Elsevier]

Published
2008
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231. CIPK23 regulates blue light‐dependent stomatal opening in Arabidopsis thaliana.

Author

Inoue, Shin‐Ichiro, Kaiserli, Eirini, Zhao, Xiang, Waksman, Thomas, Takemiya, Atsushi, Okumura, Masaki, Takahashi, Hirotaka, Seki, Motoaki, Shinozaki, Kazuo, Endo, Yaeta, Sawasaki, Tatsuya, Kinoshita, Toshinori, Zhang, Xiao, Christie, John M., and Shimazaki, Ken‐Ichiro

Subjects
*ARABIDOPSIS proteins, *BLUE light, *PROTEIN kinases, *ARABIDOPSIS thaliana, *CELL membranes, *ADENOSINE triphosphatase, *PHOTOTROPISM
Abstract

SUMMARY: Phototropins (phot1 and phot2) are plant blue light receptor kinases that function to mediate phototropism, chloroplast movement, leaf flattening, and stomatal opening in Arabidopsis. Considerable progress has been made in understanding the mechanisms associated with phototropin receptor activation by light. However, the identities of phototropin signaling components are less well understood by comparison. In this study, we specifically searched for protein kinases that interact with phototropins by using an in vitro screening method (AlphaScreen) to profile interactions against an Arabidopsis protein kinase library. We found that CBL‐interacting protein kinase 23 (CIPK23) interacts with both phot1 and phot2. Although these interactions were verified by in vitro pull‐down and in vivo bimolecular fluorescence complementation assays, CIPK23 was not phosphorylated by phot1, as least in vitro. Mutants lacking CIPK23 were found to exhibit impaired stomatal opening in response to blue light but no deficits in other phototropin‐mediated responses. We further found that blue light activation of inward‐rectifying K+ (K+in) channels was impaired in the guard cells of cipk23 mutants, whereas activation of the plasma membrane H+‐ATPase was not. The blue light activation of K+in channels was also impaired in the mutant of BLUS1, which is one of the phototropin substrates in guard cells. We therefore conclude that CIPK23 promotes stomatal opening through activation of K+in channels most likely in concert with BLUS1, but through a mechanism other than activation of the H+‐ATPase. The role of CIPK23 as a newly identified component of phototropin signaling in stomatal guard cells is discussed. [ABSTRACT FROM AUTHOR]

Published
2020
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233. The Solanum chacoense ovary receptor kinase 11 (ScORK11) undergoes tissue-dependent transcriptional, translational and post-translational regulation.

Author

Germain, Hugo, Gray-Mitsumune, Madoka, Houde, Josée, Benhamman, Rachid, Sawasaki, Tatsuya, Endo, Yaeta, and Matton, Daniel P.

Subjects
*SOLANUM, *OVARIES, *GENETIC transcription, *GENETIC translation, *POST-translational modification, *FERTILIZATION (Biology)
Abstract

Abstract: Using a subtraction screen to isolate weakly expressed transcripts from ovule and ovary libraries, we uncovered 30 receptor-like kinases that were predominantly expressed in ovary and fruit tissues following fertilization [1]. Here we describe the analysis of Solanum chacoense ovule receptor kinase 11 (ScORK11), a member of the large LRR III receptor kinase subfamily that localizes to the plasma membrane. In situ analyses demonstrated that ScORK11 gene expression was mainly restricted to the ovule integument, the embryo sac and the pericarp of the fruit. Tight regulation of ScORK11 expression at the mRNA level was also accompanied by both translational and post-translational regulation of protein levels. [Copyright &y& Elsevier]

Published
2013
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234. Novel approach to identifying autoantibodies in rheumatoid synovitis with a biotinylated human autoantigen library and the enzyme-labeled antigen method

Author

Mizutani, Yasuyoshi, Matsuoka, Kazuhiro, Takeda, Hiroyuki, Shiogama, Kazuya, Inada, Ken-ichi, Hayakawa, Kazue, Yamada, Harumoto, Miyazaki, Tatsuhiko, Sawasaki, Tatsuya, Endo, Yaeta, and Tsutsumi, Yutaka

Subjects
*AUTOANTIBODIES, *SYNOVITIS, *RHEUMATISM treatment, *BIOTIN derivatives, *AUTOANTIGENS, *SYNOVIAL membranes, *PLASMA cells, *THERAPEUTICS
Abstract

Abstract: Synovial tissue in rheumatoid arthritis (RA) shows dense infiltration of plasmacytes. The purpose of the present study is to identify and localize autoantibodies produced in these immunocytes in RA synovitis. We developed a novel screening system for detecting specific autoantigens. Protein antigens recognized by antibodies in the serum and synovial tissue extract from five RA patients were screened with the AlphaScreen method. For screening, a biotinylated human autoantigen library was constructed by the wheat germ cell-free protein synthesis system. The AlphaScreen analysis of 2183 proteins detected a limited number of antigens reactive with the serum and synovial tissue extract. Eighteen biotinylated proteins, containing top five showing high signals in each synovitis tissue extract, were utilized as probes for the enzyme-labeled antigen method, in order to visualize the site of specific antibody production in synovial lesions. Specific antibodies against two proteins, tripartite motif-containing 21 (TRIM21, also known as SSA/Ro52) and F-box only protein 2 (FBXO2), were visualized in the cytoplasm of plasmacytes in two RA synovitis lesions, respectively. Absorption experiments using unlabeled proteins confirmed the specificity of staining. No positive signals against these two proteins were identified in the additionally evaluated RA and osteoarthritis synovial lesions. The present study indicated 1) the usefulness of screening the human autoantigen library with the AlphaScreen assay for detecting autoantibodies in RA synovitis, and 2) the applicability of biotinylated proteins to the enzyme-labeled antigen method for visualizing the site of autoantibody production within the lesion. [Copyright &y& Elsevier]

Published
2013
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235. The Quiescin Sulfhydryl Oxidase (hQSOX1b) Tunes the Expression of Resistin-Like Molecule Alpha (RELM-α or mFIZZ1) in a Wheat Germ Cell-Free Extract.

Author

Gad, Wael, Nair, Meera G., Van Belle, Karolien, Wahni, Khadija, De Greve, Henri, Van Ginderachter, Jo A., Vandenbussche, Guy, Endo, Yaeta, Artis, David, and Messens, Joris

Subjects
*PROTEIN research, *DISULFIDES, *RECOMBINANT proteins, *ESCHERICHIA coli, *WHEAT germ, *ENZYMES
Abstract

Background: Although disulfide bond formation in proteins is one of the most common types of post-translational modifications, the production of recombinant disulfide-rich proteins remains a challenge. The most popular host for recombinant protein production is Escherichia coli, but disulfide-rich proteins are here often misfolded, degraded, or found in inclusion bodies. Methodology/Principal findings: We optimize an in vitro wheat germ translation system for the expression of an immunological important eukaryotic protein that has to form five disulfide bonds, resistin-like alpha (mFIZZ1). Expression in combination with human quiescin sulfhydryl oxidase (hQSOX1b), the disulfide bond--forming enzyme of the endoplasmic reticulum, results in soluble, intramolecular disulfide bonded, monomeric, and biological active protein. The mFIZZ1 protein clearly suppresses the production of the cytokines IL-5 and IL-13 in mouse splenocytes cultured under Th2 permissive conditions. Conclusion/Significance: The quiescin sulfhydryl oxidase hQSOX1b seems to function as a chaperone and oxidase during the oxidative folding. This example for mFIZZ1 should encourage the design of an appropriate thiol/disulfide oxidoreductase-tuned cell free expression system for other challenging disulfide rich proteins. [ABSTRACT FROM AUTHOR]

Published
2013
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236. Genome-wide biochemical analysis of Arabidopsis protein phosphatase using a wheat cell-free system

Author

Takahashi, Hirotaka, Ozawa, Akihiko, Nemoto, Keiichirou, Nozawa, Akira, Seki, Motoaki, Shinozaki, Kazuo, Takeda, Hiroyuki, Endo, Yaeta, and Sawasaki, Tatsuya

Subjects
*WHEAT, *PLANT cells & tissues, *BIOCHEMISTRY, *GENOMES, *ARABIDOPSIS, *PHOSPHOPROTEIN phosphatases, *MYELIN basic protein, *THREONINE
Abstract

Abstract: Plant genome possesses over 100 protein phosphatase (PPase) genes that are key regulators of signal transduction via phosphorylation/dephosphorylation event. Here we report a comprehensive functional analysis of protein serine/threonine, dual-specificity and tyrosine phosphatases using recombinant PPases produced by wheat cell-free protein synthesis system. Eighty-two recombinant PPases were successfully produced using Arabidopsis full-length cDNA as templates. In vitro PPase assay was performed using phosphorylated myelin basic protein as substrate. Among the AtPPases examined, 26 serine/threonine, three dual-specificity and one tyrosine PPases exhibited catalytic activity, including 20 serine/threonine and one dual-specificity PPases that showed in vitro activities for the first time. Our study demonstrates genome-wide biochemical analysis of AtPPases using wheat cell-free system, and provides new information and insights on enzyme activities. Structured summary of protein interactions: PTP1 dephosphorylates MBP by phosphatase assay (View interaction). AtPP2C dephosphorylates MBP by phosphatase assay (View interaction). POLTE dephosphorylates MBP by phosphatase assay (View interaction). TOPP8 dephosphorylates MBP by phosphatase assay (View interaction). HAB1 dephosphorylates MBP by phosphatase assay (View interaction). ABI2 dephosphorylates MBP by phosphatase assay (View interaction). At1g34750 dephosphorylates MBP by phosphatase assay (View interaction). At1g43900 dephosphorylates MBP by phosphatase assay (View interaction). At3g15260 dephosphorylates MBP by phosphatase assay (View interaction). At5g53140 dephosphorylates MBP by phosphatase assay (View interaction). At1g18030 dephosphorylates MBP by phosphatase assay (View interaction). At3g06270 dephosphorylates MBP by phosphatase assay (View interaction). At2g25070 dephosphorylates MBP by phosphatase assay (View interaction). At3g02750 dephosphorylates MBP by phosphatase assay (View interaction). At5g10740 dephosphorylates MBP by phosphatase assay (View interaction). at4g26080 dephosphorylates MBP by phosphatase assay (View interaction). At4g28400 dephosphorylates MBP by phosphatase assay (View interaction). At5g06750 dephosphorylates MBP by phosphatase assay (View interaction). At4g31860 dephosphorylates MBP by phosphatase assay (View interaction). At3g17250 dephosphorylates MBP by phosphatase assay (View interaction). At4g38520 dephosphorylates MBP by phosphatase assay (View interaction). At3g05640 dephosphorylates MBP by phosphatase assay (View interaction). At5g66080 dephosphorylates MBP by phosphatase assay (View interaction). At1g79630 dephosphorylates MBP by phosphatase assay (View interaction). At2g30170 dephosphorylates MBP by phosphatase assay (View interaction). At5g24940 dephosphorylates MBP by phosphatase assay (View interaction). [Copyright &y& Elsevier]

Published
2012
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237. A novel Sec14 phospholipid transfer protein from Nicotiana benthamiana is up-regulated in response to Ralstonia solanacearum infection, pathogen associated molecular patterns and effector molecules and involved in plant immunity

Author

Kiba, Akinori, Nakano, Masahito, Vincent-Pope, Patrick, Takahashi, Hirotaka, Sawasaki, Tatsuya, Endo, Yaeta, Ohnishi, Kouhei, Yoshioka, Hirofumi, and Hikichi, Yasufumi

Subjects
*PHOSPHOLIPIDS, *NICOTIANA benthamiana, *RALSTONIA solanacearum, *PATHOGENIC microorganisms, *PLANT immunology, *GENE expression in plants
Abstract

Summary: To elucidate the molecular mechanisms of plant immune responses, we isolated genes whose expression was regulated by inoculation with Ralstonia solanacearum. Here, we report the characterization of Nicotiana benthamiana belonging to the SEC14-gene superfamily designated as Nicotiana benthamiana SEC14 (NbSEC14). NbSEC14 rescued growth defects and impaired invertase secretion associated with the yeast sec14p temperature-sensitive mutant, while recombinant NbSec14 protein had phospholipids transfer activity. NbSEC14 expression was up-regulated in N. benthamiana leaves after inoculation with virulent or avirulent R. solanacearum. Expression of NbSEC14 was induced by treatment with chitin, flg22, and by Agrobacterium-mediated transient expression of INF1 elicitin, AvrA from R. solanacearum, and co-expression of the capsid protein from Tobacco mild green mosaic virus with its cognate resistance L1 protein. NbSEC14-silenced plants showed accelerated growth of both the virulent and avirulent R. solanacearum as well as acceleration of disease development. This study may provide useful information for the further analysis of the function of plant Sec14 protein homologs in the regulation of plant immune responses. [ABSTRACT FROM AUTHOR]

Published
2012
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238. Structural Basis for Specific Recognition of Rpt1p, an ATPase Subunit of 26 S Proteasome, by Proteasome-dedicated Chaperone Hsm3p.

Author

Takagi, Kenji, Sangwoo Kim, Yukii, Haruka, Ueno, Mika, Morishita, Ryo, Endo, Yaeta, Kato, Koichi, Tanaka, Keiji, Saeki, Yasushi, and Mizushima, Tsunehiro

Subjects
*PROTEASOMES, *ADENOSINE triphosphatase regulation, *MOLECULAR chaperones, *GENETIC mutation, *EUKARYOTIC cells
Abstract

The 26 S proteasome is a 2.5-MDa molecular machine that degrades ubiquitinated proteins in eukaryotic cells. It consists of a proteolytic core particle and two 19 S regulatory particles (RPs) composed of 6 ATPase (Rpt) and 13 non-ATPase (Rpn) subunits. Multiple proteasome-dedicated chaperones facilitate the assembly of the proteasome, but little is known about the detailed mechanisms. Hsm3, a 19 S RP dedicated chaperone, transiently binds to the C-terminal domain of the Rpt1 subunit and forms a tetrameric complex, Hsm3-Rpt1-Rpt2-Rpn1, during maturation of the ATPase ring of 19 S RP. To elucidate the structural basis of Hsm3 function, we determined the crystal structures of Hsm3 and its complex with the C-terminal domain of the Rpt1 subunit (Rpt1C). Hsm3 has a C-shaped structure that consists of 11 HEAT repeats. The structure of the Hsm3-Rpt1C complex revealed that the interacting surface between Hsm3 and Rpt1 is a hydrophobic core and a complementary charged surface. Mutations in the Hsm3-Rpt1 surface resulted in the assembly defect of the 26 S proteasome. Furthermore, a structural model of the Hsm3-Rpt ring complex and an in vitro binding assay suggest that Hsm3 can bind Rpt2 in addition to Rpt1. Collectively, our results provide the structural basis of the molecular functions of Hsm3 for the RP assembly. [ABSTRACT FROM AUTHOR]

Published
2012
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239. BAZF, a novel component of cullin3-based E3 ligase complex, mediates VEGFR and Notch cross-signaling in angiogenesis.

Author

Ohnuki, Hidetaka, Inoue, Hirofumi, Takemori, Nobuaki, Nakayama, Hironao, Sakaue, Tomohisa, Fukuda, Shinji, Miwa, Daisuke, Nishiwaki, Eiji, Hatano, Masahiko, Tokuhisa, Takeshi, Endo, Yaeta, Nose, Masato, and Higashiyama, Shigeki

Subjects
*VASCULAR endothelial growth factors, *NEOVASCULARIZATION, *CELLULAR signal transduction, *HOMEOSTASIS, *ZINC-finger proteins, *LYMPHOCYTIC leukemia
Abstract

Angiogenic homeostasis is maintained by a balance between vascular endothelial growth factor (VEGF) and Notch signaling in endothelial cells (ECs). We screened for molecules that might mediate the coupling of VEGF signal transduction with down-regulation of Notch signaling, and identified B-cell chronic lymphocytic leukemia/lymphoma6-associated zinc finger protein (BAZFBAZF was induced by VEGF-A in ECs to bind to the Notch signaling factor C-promoter binding factor 1 (CBF1), and to promote the degradation of CBF1 through polyubiquitination in a CBF1-cullin3 (CUL3) E3 ligase complex. BAZF disruption in vivo decreased endothelial tip cell number and filopodia protrusion, and markedly abrogated vascular plexus formation in the mouse retina, overlapping the retinal phenotype seen in response to Notch activation. Further, impaired angiogenesis and capillary remodeling were observed in skin-wounded BAZF'1' mice. We therefore propose that BAZF supports angiogenic sprouting via BAZF-CUL3-based polyubiquitination-dependent degradation of CBF1 to down-regulate Notch signaling [ABSTRACT FROM AUTHOR]

Published
2012
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240. Secreted Opisthorchis viverrini glutathione S-transferase regulates cell proliferation through AKT and ERK pathways in cholangiocarcinoma

Author

Daorueang, Daoyot, Thuwajit, Peti, Roitrakul, Sittiruk, Laha, Thewarach, Kaewkes, Sasithorn, Endo, Yaeta, and Thuwajit, Chanitra

Subjects
*GLUTATHIONE, *CANCER cell proliferation, *CHOLANGIOCARCINOMA, *TRANSFERASES, *MITOGENS, *GEL permeation chromatography, *CARCINOGENESIS
Abstract

Abstract: Opisthorchis viverrini can develop mitogenic substances into the excretory/secretory product (ESP) that may play an important role in promoting the genesis of cholangiocarcinoma (CCA). In the present study, glutathione S-transferase (GST) is identified as being secreted into Ov-ESP and acting as one of the parasitic mitogens. Its proliferative effect and possible mechanism were explored and its association with the tumor development is proposed. Ov-ESP was concentrated and purified by gel filtration chromatography. SDS-PAGE, 2-DE, and LC-MS/MS identified GST predominantly expressed in the proliferative ESP fraction. The recombinant OvGST (rOvGST) was produced by wheat germ cell-free expression and confirmed by an MTS assay to have a proliferative function on NIH-3T3 murine fibroblasts and MMNK1 non-tumorigenic human bile duct epithelial cells in a dose dependent manner with different optimal doses. The cell surface binding of rOvGST was confirmed in vitro and the activation of both pAKT and pERK was revealed as the mechanism of OvGST-mediated cell proliferation. With support from the observation of secreted OvGST on the biliary cells surrounding the parasites, it is suggested that OvGST can promote cell proliferation that consequently may accelerate the genesis of CCA. [Copyright &y& Elsevier]

Published
2012
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241. Autophosphorylation profiling of Arabidopsis protein kinases using the cell-free system

Author

Nemoto, Keiichirou, Seto, Takuya, Takahashi, Hirotaka, Nozawa, Akira, Seki, Motoaki, Shinozaki, Kazuo, Endo, Yaeta, and Sawasaki, Tatsuya

Subjects
*PLANT phosphorylation, *ARABIDOPSIS, *PROTEIN kinases, *PLANT cells & tissues, *PLANT cellular signal transduction, *PLANT genetics, *PLANT proteins, *GERM cells
Abstract

Abstract: Protein phosphorylation is one of the main process in the signal transduction pathway. In recent years, there has been increasing attention to plant phosphorylation signaling and many laboratories are trying to elucidate pathways using various approaches. Although more than 1000 protein kinase (PK) genes have been annotated in the Arabidopsis genome, biochemical characterization of those PKs is limited. In this work, we demonstrate high-throughput profiling of serine/threonine autophosphorylation activity by a combination of the 759N-terminal biotinylated proteins library, produced using a wheat germ cell-free protein production system, and a commercially available luminescence system. Luminescent analysis revealed that 179 of the 759 PKs had autophosphorylation activity. From these 179 PKs, 67 of the most active PKs were analyzed to determine their function using the PlantP database. This analysis revealed that 35 (53%) of the proteins were classified as non-transmembrane protein kinases, and 15 (23%) were receptor-like protein kinases. Additionally, PKs from Group 4.4-MAP3K, Group 1.6, Group 4.5-MAPK/CDC/CK2/GSK kinases and Group 1.10-receptor like cytoplasmic kinases contained the highest percentage of autophosphorylated activity. Next, to get a better overview of the annotated 67 PKs, we used the gene ontology annotation search on the TAIR website to classify the 67 PKs into functional category. As a result, some of these PKs may be involved in phospho-signaling pathways such as signal transduction, stress response, and the regulation of cell division. Information from this study may shed light on many unknown plant PKs. This study will be a basis for understanding the function of PKs in phosphorylation network for future research. [Copyright &y& Elsevier]

Published
2011
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242. Caspase-8 cleavage of the interleukin-21 (IL-21) receptor is a negative feedback regulator of IL-21 signaling

Author

Akagi, Tatsuya, Shimizu, Kouhei, Takahama, Shoukichi, Iwasaki, Takahiro, Sakamaki, Kazuhiro, Endo, Yaeta, and Sawasaki, Tatsuya

Subjects
*INTERLEUKINS, *APOPTOSIS, *CARBONIC anhydrase, *PHOSPHORYLATION, *CYSTEINE proteinases, *GENES, *CYTOKINES, *PROTEINS
Abstract

Abstract: We screened a library of human single-transmembrane proteins (sTMPs), produced by a cell-free system, using a luminescent assay to identify those that can be cleaved by caspase-8 (CASP8). Of the 407 sTMPs screened, only the interleukin-21 receptor (IL21R), vezatin (VEZT), and carbonic anhydrase XIV were cleaved at Asp344, Asp655 and Asp53, respectively. We confirmed that IL21R and VEZT were also cleaved in apoptotic HeLa cells with the cleavage sites. Interestingly, IL21R was cleaved within 30min after apoptosis induction. Furthermore the CASP8-cleaved form of IL21R did not induce phosphorylation at Tyr705 of STAT3. Our results suggest that the interleukin-21 signaling cascade is negatively regulated by CASP8. [Copyright &y& Elsevier]

Published
2011
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243. Wheat germ cell-free protein production system for post-genomic research

Author

Madono, Masaki, Sawasaki, Tatsuya, Morishita, Ryo, and Endo, Yaeta

Subjects
*PROTEIN synthesis, *PLANT embryology, *HAZARDOUS substances, *FUNCTIONAL analysis, *WHEAT germ, *GENOMICS
Abstract

Genomic information becomes useful knowledge only when the structures and functions of gene products are understood. In spite of a vast array of analytical tools developed for biological studies in recent years, producing proteins at will is still a bottleneck in post-genomic studies. The cell-free protein production system we developed using wheat embryos has enabled us to produce high quality proteins for genome-wide functional and structural analyses and at the same time circumvent almost all the limitations, such as biohazards and costs, that have hampered conventional cell-free protein synthesis systems. In the present article, we introduce examples of our new wheat germ cell-free protein production system and its application to functional and structural analyses, with the focus on the former. [Copyright &y& Elsevier]

Published
2011
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244. Wheat-germ cell-free production of prion proteins for solid-state NMR structural studies

Author

Noirot, Claire, Habenstein, Birgit, Bousset, Luc, Melki, Ronald, Meier, Beat H., Endo, Yaeta, Penin, François, and Böckmann, Anja

Subjects
*NUCLEAR magnetic resonance, *WHEAT germ, *PRIONS, *GENE expression, *RENILLA luciferase, *YEAST
Abstract

The expression of soluble, functional protein on a preparative scale poses a central challenge for structural studies. Cell-free protein expression has become a valuable alternative to cell-based methods, and allows today the expression of milligram quantities of protein. Its use is particularly attractive for NMR studies as it allows a multitude of isotopic labeling schemes. We have implemented and further developed protocols to prepare cell-free extracts from wheat germ to produce recombinant protein for solid-state NMR studies. Furthermore, we established the Renilla luciferase model to optimise and evaluate extract quality, and report first productions of the prions Ure2p and HET-s devoted to structural studies currently ongoing in our laboratories. [Copyright &y& Elsevier]

Published
2011
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245. Production and partial purification of membrane proteins using a liposome-supplemented wheat cell-free translation system.

Author

Nozawa, Akira, Ogasawara, Tomio, Matsunaga, Satoko, Iwasaki, Takahiro, Sawasaki, Tatsuya, and Endo, Yaeta

Subjects
*MEMBRANE proteins, *LIPOSOMES, *BILAYER lipid membranes, *CYTOPLASM, *PHOSPHOLIPIDS
Abstract

Background: Recently, some groups have reported on cell-free synthesis of functional membrane proteins (MPs) in the presence of exogenous liposomes (liposomes). Previously, we reported synthesis of a functional AtPPT1 plant phosphate transporter that was associated with liposomes during translation. However, it is unclear whether or not lipid/MP complex formation is common to all types of MPs in the wheat cell-free system. Results: AtPPT1 was synthesized using a wheat cell-free system with or without liposomes. AtPPT1 synthesized with liposomes showed high transport activity, but the activity of AtPPT1 synthesized without liposomes was less than 10% activity of that with liposomes. To test whether co-translational association with liposomes is observed in the synthesis of other MPs, we used 40 mammalian MPs having one to 14 transmembrane domains (TMDs) and five soluble proteins as a control. The association rate of all 40 MPs into liposomes was more than 40% (mean value: 59%), while that of the five soluble proteins was less than 20% (mean value: 12%). There were no significant differences in association rate among MPs regardless of the number of TMDs and synthesis yield. These results indicate that the wheat cell-free system is a highly productive method for lipid/MP complex formation and is suitable for large-scale preparation. The liposome association of green fluorescent protein (GFP)-fusion MPs were also tested and recovered as lipid/MP complex after floatation by Accudenz density gradient ultracentrifugation (DGU). Employment of GFP-MPs revealed optimal condition for Accudenz floatation. Using the optimized Accudenz DGU condition, P2RX4/lipid complexes were partially purified and detected as a major band by Coomassie Brilliant Blue (CBB)-staining after SDS-PAGE. Conclusion: Formation of lipid/AtPPT1 complex during the cell-free synthesis reaction is critical for synthesis of a functional MP. The lipid/MP complex during the translation was observed in all 40 MPs tested. At least 29 MPs, as judged by their higher productivity compared to GFP, might be suitable for a large-scale preparation. MPs synthesized by this method form lipid/MP complexes, which could be readily partially purified by Accudenz DGU. Wheat cell-free protein synthesis in the presence of liposomes will be a useful method for preparation of variety type of MPs. [ABSTRACT FROM AUTHOR]

Published
2011
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246. The consensus motif for N-myristoylation of plant proteins in a wheat germ cell-free translation system.

Author

Yamauchi, Seiji, Fusada, Naoki, Hayashi, Hidenori, Utsumi, Toshihiko, Uozumi, Nobuyuki, Endo, Yaeta, and Tozawa, Yuzuru

Subjects
*PLANT proteins, *WHEAT germ, *EUKARYOTIC cells, *GENETIC translation, *AMINO acid sequence, *ARABIDOPSIS thaliana, *AMINOPEPTIDASES
Abstract

Protein N-myristoylation plays key roles in various cellular functions in eukaryotic organisms. To clarify the relationship between the efficiency of protein N-myristoylation and the amino acid sequence of the substrate in plants, we have applied a wheat germ cell-free translation system with high protein productivity to examine the N-myristoylation of various wild-type and mutant forms of Arabidopsis thaliana proteins. Evaluation of the relationship between removal of the initiating Met and subsequent N -myristoylation revealed that constructs containing Pro at position 3 do not undergo N-myristoylation, primarily because of an inhibitory effect of this amino acid on elimination of the initiating Met by methionyl aminopeptidase. Our analysis of the consensus sequence for N -myristoylation in plants focused on the variability of amino acids at positions 3, 6 and 7 of the motif. We found that not only Ser at position 6 but also Lys at position 7 affects the selectivity for the amino acid at position 3. The results of our analyses allowed us to identify several A. thaliana proteins as substrates for N-myristoylation that had previously been predicted not to be candidates for such modification with a prediction program. We have thus shown that a wheat germ cell-free system is a useful tool for plant N-myristoylome analysis. This in vitro approach will facilitate comprehensive determination of N-myristoylated proteins in plants. [ABSTRACT FROM AUTHOR]

Published
2010
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247. Paraquat Toxicity Induced by Voltage-dependent Anion Channel 1 Acts as an NADH-dependent Oxidoreductase.

Author

Shimada, Hiroki, Hirai, Kei-Ichi, Simamura, Eriko, Hatta, Toshihisa, Iwakiri, Hiroki, Mizuki, Keiji, Hatta, Taizo, Sawasaki, Tatsuya, Matsunaga, Satoko, Endo, Yaeta, and Shimizu, Shigeomi

Subjects
*PARAQUAT, *HERBICIDE toxicology, *OXIDOREDUCTASES, *MITOCHONDRIA, *SUPEROXIDES, *ANIONS
Abstract

Paraquat (PQ), a herbicide used worldwide, causes fatal injury to organs upon high dose ingestion. Treatments for PQ poisoning are unreliable, and numerous deaths have been attributed inappropriate usage of the agent. It is generally speculated that a microsomal drug-metabolizing enzyme system is responsible for PQ toxicity. However, recent studies have demonstrated cytotoxicity via mitochondria, and therefore, the cytotoxic mechanism remains controversial. Here, we demonstrated that mitochondrial NADHdependent PQ reductase containing a voltage-dependent anion channel 1 (VDAC1) is responsible for PQ cytotoxicity. When mitochondria were incubated with NADH and PQ, superoxide anion (Of) was produced, and the mitochondria ruptured. Outer membrane extract oxidized NADH in a PQ dose-dependent manner, and oxidation was suppressed by VDAC inhibitors. Zymographic analysis revealed the presence of VDAC1 protein in the oxidoreductase, and the direct binding of PQ to VDAC1 was demonstrated using biotinylated PQ. VDAC1-overexpressing cells showed increased O-2 production and cytotoxicity, both of which were suppressed in VDAC1 knockdown cells. These results indicated that a VDAC1-containing mitochondrial system is involved in PQ poisoning. These insights into the mechanism of PQ poisoning not only demonstrated novel physiological functions of VDAC protein, but they may facilitate the development of new therapeutic approaches. [ABSTRACT FROM AUTHOR]

Published
2009
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248. Isolation and identification of ubiquitin-related proteins from Arabidopsis seedlings.

Author

Igawa, Tomoko, Fujiwara, Masayuki, Takahashi, Hirotaka, Sawasaki, Tatsuya, Endo, Yaeta, Seki, Motoaki, Shinozaki, Kazuo, Fukao, Yoichiro, and Yanagawa, Yuki

Subjects
*ARABIDOPSIS, *SEEDLINGS, *UBIQUITIN, *PROTEINS, *BIOMOLECULES
Abstract

The majority of proteins in eukaryotic cells are modified according to highly regulated mechanisms to fulfill specific functions and to achieve localization, stability, and transport. Protein ubiquitination is one of the major post-translational modifications occurring in eukaryotic cells. To obtain the proteomic dataset related to the ubiquitin (Ub)-dependent regulatory system in Arabidopsis, affinity purification with an anti-Ub antibody under native condition was performed. Using MS/MS analysis, 196 distinct proteins represented by 251 distinct genes were identified. The identified proteins were involved in metabolism (23.0%), stress response (21.4%), translation (16.8%), transport (6.7%), cell morphology (3.6%), and signal transduction (1.5%), in addition to proteolysis (16.8%) to which proteasome subunits (14.3%) is included. On the basis of potential ubiquitination-targeting signal motifs, in-gel mobilities, and previous reports, 78 of the identified proteins were classified as ubiquitinated proteins and the rest were speculated to be associated proteins of ubiquitinated proteins. The degradation of three proteins predicted to be ubiquitinated proteins was inhibited by a proteasome inhibitor, suggesting that the proteins were regulated by Ub/proteasome-dependent proteolysis. [ABSTRACT FROM PUBLISHER]

Published
2009
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249. Construction of a Protein Library of Arabidopsis Transcription Factors Using a Wheat Cell-Free Protein Production System and Its Application for DNA Binding Analysis.

Author

Nozawa, Akira, Matsubara, Yuko, Tanaka, Yoshinori, Takahashi, Hirotaka, Akagi, Tatsuya, Seki, Motoaki, Shinozaki, Kazuo, Endo, Yaeta, and Sawasaki, Tatsuya

Subjects
*CHEMICAL libraries, *ARABIDOPSIS, *PROTEIN analysis, *TRANSCRIPTION factors, *PROTEIN binding, *FIRE assay, *EQUIPMENT & supplies
Abstract

The article discusses the creation of a protein library consisting of 647 Arabidosis transcription factors (TF)s using a wheat cell-free protein production system. Binding assay of bZIP family proteins checked the quality of proteins in said library, which was then used in the screening of TFs binding to 5'-regulatory factors of both FLC and GBF1. In conclusion, GBF1 and MYB67 were indentified as binding factors, indicating the library sufficient for large-scale biochemical characterization.

Published
2009
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250. A simple and high-sensitivity method for analysis of ubiquitination and polyubiquitination based on wheat cell-free protein synthesis.

Author

Takahashi, Hirotaka, Nozawa, Akira, Seki, Motoaki, Shinozaki, Kazuo, Endo, Yaeta, and Sawasaki, Tatsuya

Subjects
*PLANT enzymes, *UBIQUITIN, *PLANT proteins, *ARABIDOPSIS, *PLANT genomes, *PLANT genetics
Abstract

Background: Ubiquitination is mediated by the sequential action of at least three enzymes: the E1 (ubiquitin-activating enzyme), E2 (ubiquitin-conjugating enzyme) and E3 (ubiquitin ligase) proteins. Polyubiquitination of target proteins is also implicated in several critical cellular processes. Although Arabidopsis genome research has estimated more than 1,300 proteins involved in ubiquitination, little is known about the biochemical functions of these proteins. Here we demonstrate a novel, simple and high-sensitive method for in vitro analysis of ubiquitination and polyubiquitination based on wheat cell-free protein synthesis and luminescent detection. Results: Using wheat cell-free synthesis, 11 E3 proteins from Arabidopsis full-length cDNA templates were produced. These proteins were analyzed either in the translation mixture or purified recombinant protein from the translation mixture. In our luminescent method using FLAG-or His-tagged and biotinylated ubiquitins, the polyubiquitin chain on AtUBC22, UPL5 and UPL7 (HECT) and CIP8 (RING) was detected. Also, binding of ubiquitin to these proteins was detected using biotinylated ubiquitin and FLAG-tagged recombinant protein. Furthermore, screening of the RING 6 subgroup demonstrated that At1g55530 was capable of polyubiquitin chain formation like CIP8. Interestingly, these ubiquitinations were carried out without the addition of exogenous E1 and/or E2 proteins, indicating that these enzymes were endogenous to the wheat cell-free system. The amount of polyubiquitinated proteins in the crude translation reaction mixture was unaffected by treatment with MG132, suggesting that our system does not contain 26S proteasome-dependent protein degradation activity. Conclusion: In this study, we developed a simple wheat cell-free based luminescence method that could be a powerful tool for comprehensive ubiquitination analysis. [ABSTRACT FROM AUTHOR]

Published
2009
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