Your search keyword '"M Takagi"' showing total 45 results

1. The hydrophobic repeated domain of the Clostridium cellulovorans cellulose-binding protein (CbpA) has specific interactions with endoglucanases

Author

M Takagi, Roy H. Doi, Marc A. Goldstein, and Seiichi Hashida

Subjects

Monosaccharide Transport Proteins, Recombinant Fusion Proteins, Two-hybrid screening, Blotting, Western, Molecular Sequence Data, Restriction Mapping, Cellulase, medicine.disease_cause, Microbiology, Maltose-Binding Proteins, Immunoenzyme Techniques, Bacterial Proteins, medicine, Binding site, Molecular Biology, Escherichia coli, Clostridium cellulovorans, Repetitive Sequences, Nucleic Acid, Clostridium, chemistry.chemical_classification, Binding Sites, Base Sequence, biology, Escherichia coli Proteins, Binding protein, Cellulose binding, biology.organism_classification, Enzyme, Biochemistry, chemistry, Periplasmic Binding Proteins, Protein Biosynthesis, biology.protein, ATP-Binding Cassette Transporters, Electrophoresis, Polyacrylamide Gel, Carrier Proteins, Research Article

Abstract

We overexpressed one of the hydrophobic repeated domains (HBDs) (110 amino acid residues) of the cellulose-binding protein (CbpA) from Clostridium cellulovorans by making a hybrid protein with the Escherichia coli maltose-binding protein (MalE). The HBD was purified to homogeneity, and interactions between the HBD and endoglucanases were analyzed by a novel interaction Western blotting (immunoblotting) method. The HBD had specific interactions with endoglucanases (EngB and EngD) from C. cellulovorans. These results indicated that the HBD was an endoglucanase binding site of CbpA.

Published

1993

2. A transformation system for the yeast Candida utilis: use of a modified endogenous ribosomal protein gene as a drug-resistant marker and ribosomal DNA as an integration target for vector DNA

Author

Toshiko Saito, M Takagi, S Kajiwara, N Misawa, and Keiji Kondo

Subjects

Ribosomal Proteins, Base Sequence, Genetic Vectors, Molecular Sequence Data, Molecular Probe Techniques, Drug Resistance, Microbial, Biology, Ribosomal RNA, Microbiology, Marker gene, Molecular biology, DNA, Ribosomal, Transformation (genetics), Plasmid, Transformation, Genetic, Ribosomal protein, Amino Acid Sequence, DNA, Fungal, Molecular Biology, Gene, In vitro recombination, Biomarkers, Transformation efficiency, Candida, Research Article

Abstract

We have developed a transformation system for the yeast Candida utilis. A novel strategy was applied to construct the transformation system, since auxotrophic mutants which could be used as hosts for transformation are not available. A gene encoding the ribosomal protein L41 was cloned from C. utilis, which is sensitive to cycloheximide, and used as a marker gene conferring cycloheximide resistance after modification of its amino acid sequence. The marker gene was constructed by substitution of the proline codon at position 56 with the glutamine codon by in vitro mutagenesis, as it had been reported previously that the 56th amino acid residue of L41 is responsible for the cycloheximide sensitivity of various organisms (S. Kawai, S. Murao, M. Mochizuki, I. Shibuya, K. Yano, and M. Takagi, J. Bacteriol. 174:254-262 1992). The ribosomal DNA (i.e., DNA coding for rRNA) of C. utilis was also cloned and used as a multiple-copy target for the integration of vector DNA into the genome, which resulted in a high transformation efficiency. Transformants were obtained by electroporation with a maximum efficiency of approximately 1,400 transformants per 1 microgram of linearized DNA carrying the gene for cycloheximide resistance and part of the ribosomal DNA. No transformants were obtained with intact plasmids. Multiple copies of the linearized plasmid were integrated into the host chromosome by homologous recombination. Southern analysis of the transformants in which vector DNA was integrated at the L41 gene locus indicated that there are two copies of gene for the L41 protein per cell, suggesting that C. utilis is diploid. Transformants were obtained from a variety of C. utilis strains, indicating that this method is applicable to the transformation of other C. utilis strains, even though there is significant heterogeneity in chromosomal karyotypes among these strains.

Published

1995

3. Characterization of the cellulose-binding domain of the Clostridium cellulovorans cellulose-binding protein A

Author

Marc A. Goldstein, Irwin H. Segel, M Takagi, Oded Shoseyov, Roy H. Doi, and Seiichi Hashida

Subjects

DNA, Bacterial, Molecular Sequence Data, Cellobiose, Cellulase, Polysaccharide, Microbiology, digestive system, Binding, Competitive, chemistry.chemical_compound, Bacterial Proteins, Polysaccharides, medicine, Amino Acid Sequence, Cellulose, Cloning, Molecular, Molecular Biology, Clostridium cellulovorans, chemistry.chemical_classification, Clostridium, biology, Base Sequence, Binding protein, Hydrogen-Ion Concentration, biology.organism_classification, Cellulose binding, digestive system diseases, Carboxymethyl cellulose, Kinetics, surgical procedures, operative, chemistry, Biochemistry, Solubility, biology.protein, Carrier Proteins, medicine.drug, Research Article

Abstract

Cellulose-binding protein A (CbpA), a component of the cellulase complex of Clostridium cellulovorans, contains a unique sequence which has been demonstrated to be a cellulose-binding domain (CBD). The DNA coding for this putative CBD was subcloned into pET-8c, an Escherichia coli expression vector. The protein produced under the direction of the recombinant plasmid, pET-CBD, had a high affinity for crystalline cellulose. Affinity-purified CBD protein was used in equilibrium binding experiments to characterize the interaction of the protein with various polysaccharides. It was found that the binding capacity of highly crystalline cellulose samples (e.g., cotton) was greater than that of samples of low crystallinity (e.g., fibrous cellulose). At saturating CBD concentration, about 6.4 mumol of protein was bound by 1 g of cotton. Under the same conditions, fibrous cellulose bound only 0.2 mumol of CBD per g. The measured dissociation constant was in the 1 microM range for all cellulose samples. The results suggest that the CBD binds specifically to crystalline cellulose. Chitin, which has a crystal structure similar to that of cellulose, also was bound by the CBD. The presence of high levels of cellobiose or carboxymethyl cellulose in the assay mixture had no effect on the binding of CBD protein to crystalline cellulose. This result suggests that the CBD recognition site is larger than a simple cellobiose unit or more complex than a repeating cellobiose moiety. This CBD is of particular interest because it is the first CBD from a completely sequenced nonenzymatic protein shown to be an independently functional domain.

Published

1993

4. Nucleotide sequence and promoter region for the neutral protease gene from Bacillus stearothermophilus

Author

S Aiba, T Imanaka, and M Takagi

Subjects

Transcription, Genetic, medicine.medical_treatment, Bacillus, Bacillus subtilis, Microbiology, Geobacillus stearothermophilus, Species Specificity, Endopeptidases, medicine, Coding region, Amino Acid Sequence, Promoter Regions, Genetic, Molecular Biology, Gene, Peptide sequence, chemistry.chemical_classification, Protease, Base Sequence, biology, Single-Strand Specific DNA and RNA Endonucleases, Nucleic acid sequence, Protein primary structure, DNA Restriction Enzymes, Endonucleases, biology.organism_classification, Molecular biology, Amino acid, Genes, Biochemistry, chemistry, Genes, Bacterial, Neprilysin, Research Article, Plasmids

Abstract

The thermostable neutral protease gene nprT of Bacillus stearothermophilus was sequenced. The DNA sequence revealed only one large open reading frame, composed of 1,644 bases and 548 amino acid residues. A Shine-Dalgarno sequence was found 9 bases upstream from the translation start site (ATG), and the deduced amino acid sequence contained a signal sequence in its amino-terminal region. The sequence of the first 14 amino acids of purified extracellular protease completely matched that deduced from the DNA sequence starting at GTC (Val), 687 bases (229 amino acids) downstream from ATG. This suggests that the protease is translated as a longer polypeptide. The amino acid sequence of the extracellular form of this protease (319 amino acids) was highly homologous to that of the thermostable neutral protease from Bacillus thermoproteolyticus but less homologous to the thermolabile neutral protease from Bacillus subtilis. A promoter region determined by S1 nuclease mapping (TTTTCC for the -35 region and TATTTT for the -10 region) was different from the conserved promoter sequences recognized by the known or factors in bacilli. However, it was very homologous to the promoter sequence of the spo0B gene from B. subtilis. The guanine-plus-cytosine content of the coding region of the nprT gene was 58 mol%, while that of the third letter of the codons was much higher (72 mol%).

Published

1985

5. Nucleotide sequencing and characterization of the genes encoding benzene oxidation enzymes of Pseudomonas putida

Author

S Irie, T Yorifuji, K Yano, S Doi, and M Takagi

Subjects

Molecular Sequence Data, Biology, medicine.disease_cause, Microbiology, Mixed Function Oxygenases, chemistry.chemical_compound, Cistron, Pseudomonas, medicine, Amino Acid Sequence, Cloning, Molecular, Benzene, Molecular Biology, Escherichia coli, Peptide sequence, Base Sequence, Nucleic acid sequence, biology.organism_classification, Pseudomonas putida, Open reading frame, Genes, chemistry, Biochemistry, Genes, Bacterial, Ferredoxins, Oxidoreductases, Oxidation-Reduction, Research Article, Plasmids

Abstract

The nucleotide sequence of the genes from Pseudomonas putida encoding oxidation of benzene to catechol was determined. Five open reading frames were found in the sequence. Four corresponding protein molecules were detected by a DNA-directed in vitro translation system. Escherichia coli cells containing the fragment with the four open reading frames transformed benzene to cis-benzene glycol, which is an intermediate of the oxidation of benzene to catechol. The relation between the product of each cistron and the components of the benzene oxidation enzyme system is discussed.

Published

1987

6. Proton translocation coupled to trimethylamine N-oxide reduction in anaerobically grown Escherichia coli

Author

M Ishimoto, T Tsuchiya, and M Takagi

Subjects

Coenzymes, Trimethylamine, Trimethylamine N-oxide, Trimethylamine N-oxide reductase, Reductase, medicine.disease_cause, Nitrate reductase, Microbiology, Cofactor, Membrane Potentials, Methylamines, chemistry.chemical_compound, Nitrate Reductases, Metalloproteins, Escherichia coli, medicine, NADH, NADPH Oxidoreductases, Anaerobiosis, Molecular Biology, Molybdenum, Oxidoreductases Acting on CH-NH Group Donors, biology, Pteridines, Hydrogen-Ion Concentration, chemistry, Biochemistry, Chlorates, biology.protein, Molybdenum cofactor, Molybdenum Cofactors, Oxidation-Reduction, Hydrogen, Research Article, Nuclear chemistry

Abstract

Proton translocation coupled to trimethylamine N-oxide reduction was studied in Escherichia coli grown anaerobically in the presence of trimethylamine N-oxide. Rapid acidification of the medium was observed when trimethylamine N-oxide was added to anaerobic cell suspensions of E. coli K-10. Acidification was sensitive to the proton conductor 3,5-di-tert-butyl-4-hydroxybenzylidenemalononitrile (SF6847). No pH change was shown in a strain deficient in trimethylamine N-oxide reductase activity. The apparent H+/trimethylamine N-oxide ratio in cells oxidizing endogenous substrates was 3 to 4 g-ions of H+ translocated per mol of trimethylamine N-oxide added. The addition of trimethylamine N-oxide and formate to ethylenediaminetetraacetic acid-treated cell suspension caused fluorescence quenching of 3,3'-dipropylthiacarbocyanine [diS-C3-(5)], indicating the generation of membrane potential. These results indicate that the reduction of trimethylamine N-oxide in E. coli is catalyzed by an anaerobic electron transfer system, resulting in formation of a proton motive force. Trimethylamine N-oxide reductase activity and proton extrusion were also examined in chlorate-resistant mutants. Reduction of trimethylamine N-oxide occurred in chlC, chlG, and chlE mutants, whereas chlA, chlB, and chlD mutants, which are deficient in the molybdenum cofactor, could not reduce it. Protons were extruded in chlC and chlG mutants, but not in chlA, chlB, and chlD mutants. Trimethylamine N-oxide reductase activity in a chlD mutant was restored to the wild-type level by the addition of 100 microM molybdate to the growth medium, indicating that the same molybdenum cofactor as used by nitrate reductase is required for the trimethylamine N-oxide reductase system.

Published

1981

7. Gene responsible for protecting Escherichia coli from sodium dodecyl sulfate and toluidine blue plus light

Author

Y Wakayama, M Takagi, and K Yano

Subjects

Light, Ultraviolet Rays, Tolonium chloride, Mutant, medicine.disease_cause, Microbiology, chemistry.chemical_compound, Species Specificity, medicine, Escherichia coli, Toluidine, Tolonium Chloride, Sodium dodecyl sulfate, Cloning, Molecular, Molecular Biology, Gel electrophoresis, biology, Base Sequence, Genetic transfer, Sodium Dodecyl Sulfate, Dose-Response Relationship, Radiation, DNA Restriction Enzymes, biology.organism_classification, Enterobacteriaceae, Molecular biology, Kinetics, chemistry, Genes, Bacterial, Mutation, Plasmids, Research Article

Abstract

Escherichia coli cells were killed by visible light irradiation in the presence of the photosensitizing dye, toluidine blue. Two uvrB mutant strains of E. coli K-12 (AB1885 and N3-1) were much more sensitive than the isogenic uvrA and uvrC strains to treatment with toluidine blue plus light, suggesting that the uvrB+ gene product was involved in repair of DNA damage induced by the treatment. The uvrB+ gene cloned in a high- or low-copy-number plasmid was transformed into the uvrB strain (AB1885). Although all the transformants showed the same resistance as its wild-type strain (AB1157) to UV irradiation, they were as sensitive as AB1885 was to treatment with toluidine blue plus light. The two uvrB strains were more sensitive to sodium dodecyl sulfate than the other strains, suggesting that these strains had a defect in the cell surface. A sodium dodecyl sulfate-resistant revertant obtained from AB1885 was more resistant than AB1885 was to treatment with toluidine blue plus light. The two uvrB strains (AB1885 and N3-1) appear to have a defective gene (tentatively called dvl) different from uvrB. Its map position was around 7 min on the E. coli map.

Published

1984

8. Pantothenate kinase from the thermoacidophilic archaeon Picrophilus torridus.

Author

Takagi M, Tamaki H, Miyamoto Y, Leonardi R, Hanada S, Jackowski S, and Chohnan S

Subjects

Acetyl Coenzyme A metabolism, Amino Acid Sequence, Coenzyme A metabolism, Electrophoresis, Polyacrylamide Gel, Genome, Archaeal genetics, Kinetics, Malonyl Coenzyme A metabolism, Molecular Sequence Data, Phosphotransferases (Alcohol Group Acceptor) chemistry, Phosphotransferases (Alcohol Group Acceptor) genetics, Phylogeny, Sequence Analysis, DNA, Sequence Homology, Amino Acid, Substrate Specificity, Thermoplasmales classification, Phosphotransferases (Alcohol Group Acceptor) metabolism, Thermoplasmales enzymology

Abstract

Pantothenate kinase (CoaA) catalyzes the first step of the coenzyme A (CoA) biosynthetic pathway and controls the intracellular concentrations of CoA through feedback inhibition in bacteria. An alternative enzyme found in archaea, pantoate kinase, is missing in the order Thermoplasmatales. The PTO0232 gene from Picrophilus torridus, a thermoacidophilic euryarchaeon, is shown to be a distant homologue of the prokaryotic type I CoaA. The cloned gene clearly complements the poor growth of the temperature-sensitive Escherichia coli CoaA mutant strain ts9, and the recombinant protein expressed in E. coli cells transfers phosphate to pantothenate at pH 5 and 55 degrees C. In contrast to E. coli CoaA, the P. torridus enzyme is refractory to feedback regulation by CoA, indicating that in P. torridus cells the CoA levels are not regulated by the CoaA step. These data suggest the existence of two subtypes within the class of prokaryotic type I CoaAs.

Published

2010

9. Extracellular synthesis, specific recognition, and intracellular degradation of cyclomaltodextrins by the hyperthermophilic archaeon Thermococcus sp. strain B1001.

Author

Hashimoto Y, Yamamoto T, Fujiwara S, Takagi M, and Imanaka T

Subjects

Amino Acid Sequence, Base Sequence, Chromatography, Thin Layer, DNA, Bacterial chemistry, Glucosyltransferases genetics, Glucosyltransferases metabolism, Glycoside Hydrolases genetics, Glycoside Hydrolases metabolism, Hydrogen-Ion Concentration, Hydrolysis, Molecular Sequence Data, Molecular Weight, Recombinant Proteins chemistry, Starch metabolism, Temperature, Thermococcus enzymology, Polysaccharides metabolism, Thermococcus metabolism

Abstract

A unique extracellular and thermostable cyclomaltodextrin glucanotransferase (CGTase) from the hyperthermophilic archaeon Thermococcus sp. strain B1001 produces predominantly (>85%) alpha-cyclomaltodextrin (alpha-CD) from starch (Y. Tachibana, et al., Appl. Environ. Microbiol. 65:1991--1997, 1999). Nucleotide sequencing of the CGTase gene (cgtA) and its flanking region was performed, and a cluster of five genes was found, including a gene homolog encoding a cyclomaltodextrinase (CDase) involved in the degradation of CDs (cgtB), the gene encoding CGTase (cgtA), a gene homolog for a CD-binding protein (CBP) (cgtC), and a putative CBP-dependent ABC transporter involved in uptake of CDs (cgtDE). The CDase was expressed in Escherichia coli and purified. The optimum pH and temperature for CD hydrolysis were 5.5 and 95 degrees C, respectively. The molecular weight of the recombinant enzyme was estimated to be 79,000. The CDase hydrolyzed beta-CD most efficiently among other CDs. Maltose and pullulan were not utilized as substrates. Linear maltodextrins with a small glucose unit were very slowly hydrolyzed, and starch was hydrolyzed more slowly. Analysis by thin-layer chromatography revealed that glucose and maltose were produced as end products. The purified recombinant CBP bound to maltose as well as to alpha-CD. However, the CBP exhibited higher thermostability in the presence of alpha-CD. These results suggested that strain B1001 possesses a unique metabolic pathway that includes extracellular synthesis, transmembrane uptake, and intracellular degradation of CDs in starch utilization. Potential advantages of this starch metabolic pathway via CDs are discussed.

Published

2001

10. A gene cluster for the mevalonate pathway from Streptomyces sp. Strain CL190.

Author

Takagi M, Kuzuyama T, Takahashi S, and Seto H

Subjects

Escherichia coli enzymology, Escherichia coli metabolism, Fosfomycin analogs & derivatives, Fosfomycin pharmacology, Hydroxymethylglutaryl CoA Reductases genetics, Hydroxymethylglutaryl CoA Reductases metabolism, Hydroxymethylglutaryl-CoA-Reductases, NADP-dependent, Isopropyl Thiogalactoside pharmacology, Magnetic Resonance Spectroscopy, Models, Chemical, Open Reading Frames, Sequence Analysis, DNA, Streptomyces metabolism, Antigens, Bacterial biosynthesis, Hemiterpenes, Mevalonic Acid, Organophosphorus Compounds metabolism, Streptomyces genetics

Abstract

A biosynthetic 3-hydroxy-3-methylglutaryl coenzyme A reductase (EC 1. 1.1.34), the rate-limiting enzyme of the mevalonate pathway for isopentenyl diphosphate biosynthesis, had previously been purified from Streptomyces sp. strain CL190 and its corresponding gene (hmgr) had been cloned (S. Takahashi, T. Kuzuyama, and H. Seto, J. Bacteriol. 181:1256-1263, 1999). Sequence analysis of the flanking regions of the hmgr gene revealed five new open reading frames, orfA to -E, which showed similarity to those encoding eucaryotic and archaebacterial enzymes for the mevalonate pathway. Feeding experiments with [1-(13)C]acetate demonstrated that Escherichia coli JM109 harboring the hmgr gene and these open reading frames used the mevalonate pathway under induction with isopropyl beta-D-thiogalactopyranoside. This transformant could grow in the presence of fosmidomycin, a potent and specific inhibitor of the nonmevalonate pathway, indicating that the mevalonate pathway, intrinsically absent in E. coli, is operating in the E. coli transformant. The hmgr gene and orfABCDE are thus unambiguously shown to be responsible for the mevalonate pathway and to form a gene cluster in the genome of Streptomyces sp. strain CL190.

Published

2000

11. Cloning and characterization of 1-deoxy-D-xylulose 5-phosphate synthase from Streptomyces sp. Strain CL190, which uses both the mevalonate and nonmevalonate pathways for isopentenyl diphosphate biosynthesis.

Author

Kuzuyama T, Takagi M, Takahashi S, and Seto H

Subjects

Amino Acid Sequence, Base Sequence, Cloning, Molecular, Electrophoresis, Polyacrylamide Gel, Escherichia coli enzymology, Escherichia coli genetics, Molecular Sequence Data, Sequence Alignment, Sequence Analysis, DNA, Streptomyces genetics, Hemiterpenes, Mevalonic Acid metabolism, Organophosphorus Compounds metabolism, Streptomyces enzymology, Transferases genetics, Transferases metabolism

Abstract

In addition to the ubiquitous mevalonate pathway, Streptomyces sp. strain CL190 utilizes the nonmevalonate pathway for isopentenyl diphosphate biosynthesis. The initial step of this nonmevalonate pathway is the formation of 1-deoxy-D-xylulose 5-phosphate (DXP) by condensation of pyruvate and glyceraldehyde 3-phosphate catalyzed by DXP synthase. The corresponding gene, dxs, was cloned from CL190 by using PCR with two oligonucleotide primers synthesized on the basis of two highly conserved regions among dxs homologs from six genera. The dxs gene of CL190 encodes 631 amino acid residues with a predicted molecular mass of 68 kDa. The recombinant enzyme overexpressed in Escherichia coli was purified as a soluble protein and characterized. The molecular mass of the enzyme was estimated to be 70 kDa by sodium dodecyl sulfate-polyacrylamide gel electrophoresis and 130 kDa by gel filtration chromatography, suggesting that the enzyme is most likely to be a dimer. The enzyme showed a pH optimum of 9.0, with a V(max) of 370 U per mg of protein and K(m)s of 65 microM for pyruvate and 120 microM for D-glyceraldehyde 3-phosphate. The purified enzyme catalyzed the formation of 1-deoxyxylulose by condensation of pyruvate and glyceraldehyde as well, with a K(m) value of 35 mM for D-glyceraldehyde. To compare the enzymatic properties of CL190 and E. coli DXP synthases, the latter enzyme was also overexpressed and purified. Although these two enzymes had different origins, they showed the same enzymatic properties.

Published

2000

12. Cloning and sequencing of a novel meta-cleavage dioxygenase gene whose product is involved in degradation of gamma-hexachlorocyclohexane in Sphingomonas paucimobilis.

Author

Miyauchi K, Adachi Y, Nagata Y, and Takagi M

Subjects

Amino Acid Sequence, Biodegradation, Environmental, Blotting, Northern, Blotting, Southern, Gas Chromatography-Mass Spectrometry, Hydroquinones metabolism, Molecular Sequence Data, Mutagenesis, Site-Directed, Oxygen Consumption, Oxygenases chemistry, Oxygenases metabolism, Sequence Analysis, DNA, Sphingomonas genetics, Cloning, Molecular, Genes, Bacterial, Hexachlorocyclohexane metabolism, Oxygenases genetics, Sphingomonas enzymology

Abstract

Sphingomonas (formerly Pseudomonas) paucimobilis UT26 utilizes gamma-hexachlorocyclohexane (gamma-HCH), a halogenated organic insecticide, as a sole source of carbon and energy. In a previous study, we showed that gamma-HCH is degraded to chlorohydroquinone (CHQ) and then to hydroquinone (HQ), although the rate of reaction from CHQ to HQ was slow (K. Miyauchi, S. K. Suh, Y. Nagata, and M. Takagi, J. Bacteriol. 180:1354-1359, 1998). In this study, we cloned and characterized a gene, designated linE, which is located upstream of linD and is directly involved in the degradation of CHQ. The LinE protein consists of 321 amino acids, and all of the amino acids which are reported to be essential for the activity of meta-cleavage dioxygenases are conserved in LinE. Escherichia coli overproducing LinE could convert both CHQ and HQ, producing gamma-hydroxymuconic semialdehyde and maleylacetate, respectively, with consumption of O(2) but could not convert catechol, which is one of the major substrates for meta-cleavage dioxygenases. LinE seems to be resistant to the acylchloride, which is the ring cleavage product of CHQ and which seems to react with water to be converted to maleylacetate. These results indicated that LinE is a novel type of meta-cleavage dioxygenase, designated (chloro)hydroquinone 1, 2-dioxygenase, which cleaves aromatic rings with two hydroxyl groups at para positions preferably. This study represents a direct demonstration of a new type of ring cleavage pathway for aromatic compounds, the hydroquinone pathway.

Published

1999

13. Two different types of dehalogenases, LinA and LinB, involved in gamma-hexachlorocyclohexane degradation in Sphingomonas paucimobilis UT26 are localized in the periplasmic space without molecular processing.

Author

Nagata Y, Futamura A, Miyauchi K, and Takagi M

Subjects

Periplasm enzymology, Protein Processing, Post-Translational, Bacterial Proteins analysis, Hexachlorocyclohexane metabolism, Hydrolases analysis, Lyases, Pseudomonas enzymology

Abstract

gamma-Hexachlorocyclohexane (gamma-HCH) is one of several highly chlorinated insecticides that cause serious environmental problems. The cellular proteins of a gamma-HCH-degrading bacterium, Sphingomonas paucimobilis UT26, were fractionated into periplasmic, cytosolic, and membrane fractions after osmotic shock. Most of two different types of dehalogenase, LinA (gamma-hexachlorocyclohexane dehydrochlorinase) and LinB (1,3,4,6-tetrachloro-1,4-cyclohexadiene halidohydrolase), that are involved in the early steps of gamma-HCH degradation in UT26 was detected in the periplasmic fraction and had not undertaken molecular processing. Furthermore, immunoelectron microscopy clearly showed that LinA and LinB are periplasmic proteins. LinA and LinB both lack a typical signal sequence for export, so they may be secreted into the periplasmic space via a hitherto unknown mechanism.

Published

1999

14. Proliferation of intrahyphal hyphae caused by disruption of csmA, which encodes a class V chitin synthase with a myosin motor-like domain in Aspergillus nidulans.

Author

Horiuchi H, Fujiwara M, Yamashita S, Ohta A, and Takagi M

Subjects

Aspergillus niger genetics, Genotype, Microscopy, Electron, Scanning, Myosins genetics, Myosins metabolism, Plasmids, Restriction Mapping, Aspergillus niger enzymology, Aspergillus niger ultrastructure, Chitin Synthase genetics, Chitin Synthase metabolism

Abstract

We have found that the Aspergillus nidulans csmA gene encodes a novel protein which consists of an N-terminal myosin motor-like domain and a C-terminal chitin synthase domain (M. Fujiwara, H. Horiuchi, A. Ohta, and M. Takagi, Biochem. Biophys. Res. Commun. 236:75-78, 1997). To clarify the roles of csmA in fungal morphogenesis, we constructed csmA null mutants. The growth rate of the mutant colonies was almost the same as that of the wild-type strain, but hyphal growth was severely inhibited when a chitin-binding reagent, Calcofluor white or Congo red, was added to the medium. Moreover, morphological abnormalities in tip growth and septum formation were identified microscopically. Proliferation of intracellular new hyphae, called intrahyphal hyphae, which behaved as intrinsic hyphae, was the most striking phenotypic feature among them. These phenotypes were not suppressed when the only chitin synthase domain of csmA was expressed under the control of the alcA promoter, whereas they were suppressed when the intact form of csmA was expressed. Therefore, it was concluded that the product of csmA (CsmA) has important roles in polarized cell wall synthesis and maintenance of cell wall integrity and that the myosin motor-like domain is indispensable for these functions.

Published

1999

15. Isolation and characterization of EPD1, an essential gene for pseudohyphal growth of a dimorphic yeast, Candida maltosa.

Author

Nakazawa T, Horiuchi H, Ohta A, and Takagi M

Subjects

Amino Acid Sequence, Candida cytology, Centromere genetics, DNA, Fungal metabolism, Fungal Proteins biosynthesis, Fungal Proteins chemistry, Molecular Sequence Data, Plasmids, Recombinant Fusion Proteins biosynthesis, Restriction Mapping, Sequence Alignment, Sequence Homology, Amino Acid, Species Specificity, Transcription, Genetic, Candida genetics, Candida growth & development, Fungal Proteins genetics, Genes, Fungal

Abstract

Additional copies of the centromeric DNA (CEN) region induce pseudohyphal growth in a dimorphic yeast, Candida maltosa (T. Nakazawa, T. Motoyama, H. Horiuchi, A. Ohta, and M. Takagi, J. Bacteriol. 179:5030-5036, 1997). To understand the mechanism of this transition, we screened the gene library of C. maltosa for sequences which could suppress this morphological change. As a result, we isolated the 5' end of a new gene, EPD1 (for essential for pseudohyphal development), and then cloned the entire gene. The predicted amino acid sequence of Epdlp was highly homologous to those of Ggp1/Gas1/Cwh52p, a glycosylphosphatidylinositol-anchored protein of Saccharomyces cerevisiae, and Phr1p and Phr2p of Candida albicans. The expression of EPD1 was moderately regulated by environmental pH. A homozygous EPD1 null mutant showed some morphological defects and reduction in growth rate and reduced levels of both alkali-soluble and alkali-insoluble beta-glucans. Moreover, the mutant could not undergo the transition from yeast form to pseudohyphal form induced by additional copies of the CEN sequence at pH 4 or by n-hexadecane at pH 4 or pH 7, suggesting that EPD1 is not essential for yeast form growth but is essential for transition to the pseudohyphal form. Overexpression of the amino-terminal part of Epd1p under the control of the GAL promoter suppressed the pseudohyphal development induced by additional copies of the CEN sequence, whereas overexpression of the full-length EPD1 did not. This result and the initial isolation of the 5' end of EPD1 as a suppressor of the pseudohyphal growth induced by the CEN sequence suggest that the amino-terminal part of Epd1p may have a dominant-negative effect on the functions of Epd1p in the pseudohyphal growth induced by the CEN sequence.

Published

1998

16. Cloning and sequencing of a 2,5-dichlorohydroquinone reductive dehalogenase gene whose product is involved in degradation of gamma-hexachlorocyclohexane by Sphingomonas paucimobilis.

Author

Miyauchi K, Suh SK, Nagata Y, and Takagi M

Subjects

Amino Acid Sequence, Base Composition, Blotting, Northern, Chromatography, Gas, Chromatography, Thin Layer, Cloning, Molecular, DNA Transposable Elements, DNA, Bacterial analysis, DNA, Bacterial genetics, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression, Gene Library, Glutathione metabolism, Glutathione Transferase genetics, Hydroquinones metabolism, Molecular Sequence Data, Plasmids, Restriction Mapping, Sequence Alignment, Sequence Analysis, DNA, Sequence Deletion, Sequence Homology, Amino Acid, Sodium Dodecyl Sulfate pharmacology, Bacterial Proteins, Hexachlorocyclohexane metabolism, Hydrolases genetics, Pseudomonas genetics

Abstract

Sphingomonas (formerly Pseudomonas) paucimobilis UT26 utilizes gamma-hexachlorocyclohexane (gamma-HCH), a halogenated organic insecticide, as a sole carbon and energy source. In a previous study, we showed that gamma-HCH is degraded to 2,5-dichlorohydroquinone (2,5-DCHQ) (Y. Nagata, R. Ohtomo, K. Miyauchi, M. Fukuda, K. Yano, and M. Takagi, J. Bacteriol. 176:3117-3125, 1994). In the present study, we cloned and characterized a gene, designated linD, directly involved in the degradation of 2,5-DCHQ. The linD gene encodes a peptide of 343 amino acids and has a low level of similarity to proteins which belong to the glutathione S-transferase family. When LinD was overproduced in Escherichia coli, a 40-kDa protein was found after sodium dodecyl sulfate-polyacrylamide gel electrophoresis. Northern blot analysis revealed that expression of the linD gene was induced by 2,5-DCHQ in S. paucimobilis UT26. Thin-layer chromatography and gas chromatography-mass spectrometry analyses with the LinD-overexpressing E. coli cells revealed that LinD converts 2,5-DCHQ rapidly to chlorohydroquinone (CHQ) and also converts CHQ slowly to hydroquinone. LinD activity in crude cell extracts was increased 3.7-fold by the addition of glutathione. All three of the Tn5-induced mutants of UT26, which lack 2,5-DCHQ dehalogenase activity, had rearrangements or a deletion in the linD region. These results indicate that LinD is a glutathione-dependent reductive dehalogenase involved in the degradation of gamma-HCH by S. paucimobilis UT26.

Published

1998

17. Evidence that part of a centromeric DNA region induces pseudohyphal growth in a dimorphic yeast, Candida maltosa.

Author

Nakazawa T, Motoyama T, Horiuchi H, Ohta A, and Takagi M

Subjects

Base Sequence, Centromere physiology, Cloning, Molecular, DNA Mutational Analysis, Gene Library, Genome, Fungal, Molecular Sequence Data, Mutagenesis, Site-Directed, Plasmids, Transformation, Genetic, Candida genetics, Candida growth & development, Centromere genetics, DNA, Fungal genetics

Abstract

We observed that a YCp-type vector having the centromeric DNA (CEN) sequence previously isolated from the genome, but not a YRp-type vector lacking the CEN sequence, induced pseudohyphal growth in a dimorphic fungi, Candida maltosa, which had been shown to be closely related to Candida albicans by phylogenetic analysis. Deletion analysis of the CEN sequence revealed that the intact CEN sequence was not required for the induction, but part of it, having partial centromeric activity, was enough for the induction. By screening the gene library of this yeast for the sequences which induced pseudohyphal growth, we isolated three different DNA fragments which also had part of the centromere-like sequence. Partial centromeric activity of these fragments was confirmed by three criteria: low copy number and high stability of the plasmids carrying these fragments and rearrangement at high frequency of the plasmid DNA with one of these fragments plus the CEN sequence. Furthermore, when the GGTAGCG sequence commonly found in one copy in each of these four sequences was mutated in the CEN sequence by site-directed mutagenesis, both partial centromeric activity and pseudohyphal growth-inducing activity of the CEN sequence were lost. These results indicated that part of CEN region with partial centromeric activity induces pseudohyphal growth in C. maltosa. It is suggested that some cellular components which interact with the sequence containing GGTAGCG required for centromeric activity are involved in the regulation of the transition between yeast forms and pseudohyphal forms of the cells.

Published

1997

18. Characterization of a gene cluster for glycogen biosynthesis and a heterotetrameric ADP-glucose pyrophosphorylase from Bacillus stearothermophilus.

Author

Takata H, Takaha T, Okada S, Takagi M, and Imanaka T

Subjects

1,4-alpha-Glucan Branching Enzyme genetics, Amino Acid Sequence, Base Sequence, Chromosomes, Bacterial, DNA, Bacterial, Escherichia coli, Geobacillus stearothermophilus enzymology, Glucans biosynthesis, Glucose-1-Phosphate Adenylyltransferase, Glycogen Synthase chemistry, Glycogen Synthase metabolism, Molecular Sequence Data, Nucleotidyltransferases biosynthesis, Nucleotidyltransferases metabolism, Phosphorylases chemistry, Phosphorylases metabolism, Sequence Homology, Amino Acid, Genes, Bacterial, Geobacillus stearothermophilus genetics, Glycogen biosynthesis, Multigene Family, Nucleotidyltransferases genetics

Abstract

A chromosomal region of Bacillus stearothermophilus TRBE14 which contains genes for glycogen synthesis was cloned and sequenced. This region includes five open reading frames (glgBCDAP). It has already been demonstrated that glgB encodes branching enzyme (EC 2.4.1.18 [H. Takata et al., Appl. Environ. Microbiol. 60:3096-3104, 1994]). The putative GlgC (387 amino acids [aa]) and GlgD (343 aa) proteins are homologous to bacterial ADP-glucose pyrophosphorylase (AGP [EC 2.7.7.27]): the sequences share 42 to 70% and 20 to 30% identities with AGP, respectively. Purification of GlgC and GlgD indicated that AGP is an alpha2beta2-type heterotetrameric enzyme consisting of these two proteins. AGP did not seem to be an allosteric enzyme, although the activities of most bacterial AGPs are known to be allosterically controlled. GlgC protein had AGP activity without GlgD protein, but its activity was lower than that of the heterotetrameric enzyme. The GlgA (485 aa) and GlgP (798 aa) proteins were shown to be glycogen synthase (EC 2.4.1.21) and glycogen phosphorylase (EC 2.4.1.1), respectively. We constructed plasmids harboring these five genes (glgBCDAP) and assayed glycogen production by a strain carrying each of the derivative plasmids on which the genes were mutated one by one. Glycogen metabolism in B. stearothermophilus is discussed on the basis of these results.

Published

1997

19. Cyclization reaction catalyzed by branching enzyme.

Author

Takata H, Takaha T, Okada S, Takagi M, and Imanaka T

Subjects

Glucan 1,4-alpha-Glucosidase metabolism, Glucans chemistry, Glucans metabolism, Mass Spectrometry, Models, Chemical, 1,4-alpha-Glucan Branching Enzyme metabolism, Amylose metabolism, Geobacillus stearothermophilus enzymology

Abstract

The action of branching enzyme (EC 2.4.l.l8) from Bacillus stearothermophilus on amylose was analyzed. The enzyme reduced the molecular size of amylose without increasing the reducing power. This result could not be explained by the normal branching reaction model. When the product was treated with glucoamylase (an exo++-type amylase), a resistant component remained. The glucoamylase-resistant component was easily digested by an endo-type alpha-amylase or by isoamylase plus glucoamylase. These results suggested that the glucoamylase-resistant component was a cyclic glucan composed of alpha-1,4- and alpha-l,6-glucosidic linkages. In other words, it was suggested that branching enzyme catalyzed cyclization of the alpha-l,4-glucan chain of the amylose molecule to form an alpha-l,6-glucosidic linkage, thereby forming two smaller molecules. Mass spectrometry also supported the cyclic nature of the product.

Published

1996

20. A transformation system for the yeast Candida utilis: use of a modified endogenous ribosomal protein gene as a drug-resistant marker and ribosomal DNA as an integration target for vector DNA.

Author

Kondo K, Saito T, Kajiwara S, Takagi M, and Misawa N

Subjects

Amino Acid Sequence, Base Sequence, Biomarkers, Drug Resistance, Microbial, Genetic Vectors, Molecular Probe Techniques, Molecular Sequence Data, Candida genetics, DNA, Fungal genetics, DNA, Ribosomal genetics, Ribosomal Proteins genetics, Transformation, Genetic

Abstract

We have developed a transformation system for the yeast Candida utilis. A novel strategy was applied to construct the transformation system, since auxotrophic mutants which could be used as hosts for transformation are not available. A gene encoding the ribosomal protein L41 was cloned from C. utilis, which is sensitive to cycloheximide, and used as a marker gene conferring cycloheximide resistance after modification of its amino acid sequence. The marker gene was constructed by substitution of the proline codon at position 56 with the glutamine codon by in vitro mutagenesis, as it had been reported previously that the 56th amino acid residue of L41 is responsible for the cycloheximide sensitivity of various organisms (S. Kawai, S. Murao, M. Mochizuki, I. Shibuya, K. Yano, and M. Takagi, J. Bacteriol. 174:254-262 1992). The ribosomal DNA (i.e., DNA coding for rRNA) of C. utilis was also cloned and used as a multiple-copy target for the integration of vector DNA into the genome, which resulted in a high transformation efficiency. Transformants were obtained by electroporation with a maximum efficiency of approximately 1,400 transformants per 1 microgram of linearized DNA carrying the gene for cycloheximide resistance and part of the ribosomal DNA. No transformants were obtained with intact plasmids. Multiple copies of the linearized plasmid were integrated into the host chromosome by homologous recombination. Southern analysis of the transformants in which vector DNA was integrated at the L41 gene locus indicated that there are two copies of gene for the L41 protein per cell, suggesting that C. utilis is diploid. Transformants were obtained from a variety of C. utilis strains, indicating that this method is applicable to the transformation of other C. utilis strains, even though there is significant heterogeneity in chromosomal karyotypes among these strains.

Published

1995

21. Inducible expression of a gene encoding an L41 ribosomal protein responsible for the cycloheximide-resistant phenotype in the yeast Candida maltosa.

Author

Mutoh E, Mochizuki M, Ohta A, and Takagi M

Subjects

Base Sequence, Candida drug effects, Cloning, Molecular, Drug Resistance, Microbial genetics, Genes, Fungal genetics, Molecular Sequence Data, RNA, Fungal genetics, RNA, Messenger genetics, Recombinant Fusion Proteins biosynthesis, Restriction Mapping, Sequence Analysis, DNA, Candida genetics, Cycloheximide pharmacology, Fungal Proteins genetics, Gene Expression Regulation, Fungal drug effects, Ribosomal Proteins genetics

Abstract

In a previous paper (S. Kawai, S. Murao, M. Mochizuki, I. Shibuya, K. Yano, and M. Takagi, J. Bacteriol. 174:254-262, 1992), we showed that in each genome of several yeast species, there is one of two types of L41 gene, one for an L41 (Q-type) protein which confers cycloheximide (CYH) resistance or one for an L41 (P-type) protein which does not. These genes have been suggested to be responsible for the CYH response used in taxonomy. For example, Saccharomyces cerevisiae, which is CYH sensitive, has a P-type L41 gene, while Kluyveromyces fragilis and Candida maltosa, which are CYH resistant, have Q-type L41 genes. However, in contrast to K. fragilis, which is constitutively resistant to CYH, C. maltosa is inducibly resistant to CYH. Here, we show that C. maltosa has both types of the L41 gene in its genome and that expression of the Q-type L41 gene is induced by CYH while the P-type L41 gene is constitutively expressed.

Published

1995

22. Nucleotide sequence and functional analysis of the meta-cleavage pathway involved in biphenyl and polychlorinated biphenyl degradation in Pseudomonas sp. strain KKS102.

Author

Kikuchi Y, Yasukochi Y, Nagata Y, Fukuda M, and Takagi M

Subjects

Aldehyde Oxidoreductases metabolism, Amino Acid Sequence, Base Sequence, Biodegradation, Environmental, Electrophoresis, Polyacrylamide Gel, Genes, Bacterial, Hydro-Lyases metabolism, Molecular Sequence Data, Multigene Family, Open Reading Frames, Oxo-Acid-Lyases metabolism, Pseudomonas enzymology, Pseudomonas genetics, Aldehyde Oxidoreductases genetics, Biphenyl Compounds metabolism, Hydro-Lyases genetics, Oxo-Acid-Lyases genetics, Polychlorinated Biphenyls metabolism, Pseudomonas metabolism

Abstract

Pseudomonas sp. strain KKS102 is able to degrade biphenyl and polychlorinated biphenyls via the meta-cleavage pathway. We sequenced the upstream region of the bphA1A2A3BCD (open reading frame 1 [ORF1]) A4 and found four ORFs in this region. As the deduced amino acid sequences of the first, second, and third ORFs are homologous to the meta-cleavage enzymes from Pseudomonas sp. strain CF600 (V. Shingler, J. Powlowski, and U. Marklund, J. Bacteriol. 174:711-724, 1992), these ORFs have been named bphE, bphG, and bphF, respectively. The fourth ORF (ORF4) showed homology with ORF3 from Pseudomonas pseudoalcaligenes KF707 (K. Taira, J. Hirose, S. Hayashida, and K. Furukawa, J. Biol. Chem. 267:4844-4853, 1992), whose function is unknown. The functions of meta-cleavage enzymes (BphE, BphG, and BphF) were analyzed by using crude extracts of Escherichia coli which expressed the encoding genes. The results showed that bphE, bphG, and bphF encode 2-hydroxypenta-2,4-dienoate hydratase, acetaldehyde dehydrogenase (acylating), and 4-hydroxy-2-oxovalerate aldolase, respectively. The biphenyl and polychlorinated biphenyl degradation pathway of KKS102 is encoded by 12 genes in the order bphEGF (ORF4)A1A2A3BCD (ORF1)A4. The functions of ORF1 and ORF4 are unknown. The features of this bph gene cluster are discussed.

Published

1994

23. Cloning and sequencing of a 2,5-dichloro-2,5-cyclohexadiene-1,4-diol dehydrogenase gene involved in the degradation of gamma-hexachlorocyclohexane in Pseudomonas paucimobilis.

Author

Nagata Y, Ohtomo R, Miyauchi K, Fukuda M, Yano K, and Takagi M

Subjects

Alcohol Oxidoreductases biosynthesis, Amino Acid Sequence, Base Sequence, Blotting, Southern, Cloning, Molecular, Cyclohexenes, DNA Mutational Analysis, Databases, Factual, Escherichia coli genetics, Genomic Library, Hydroquinones metabolism, Molecular Sequence Data, Pseudomonas enzymology, Pseudomonas metabolism, Recombinant Proteins biosynthesis, Restriction Mapping, Sequence Analysis, DNA, Sequence Deletion, Sequence Homology, Amino Acid, Alcohol Oxidoreductases genetics, Cyclohexanols metabolism, Genes, Bacterial genetics, Hexachlorocyclohexane metabolism, Pseudomonas genetics

Abstract

In Pseudomonas paucimobilis UT26, gamma-hexachlorocyclohexane (gamma-HCH) is converted to 2,5-dichloro-2,5-cyclohexadiene-1,4-diol (2,5-DDOL), which is then metabolized to 2,5-dichlorohydroquinone. Here, we isolated from the genomic library of UT26 two genes which expressed 2,5-DDOL dehydrogenase activity when they were transformed into P. putida and Escherichia coli. Both gene products had an apparent molecular size of 28 kDa by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. The first gene, named linC, located separately from the two genes (linA and linB) which we had already cloned as genes involved in the gamma-HCH degradation. The other, named linX, located about 1 kb upstream of the linA gene encoding gamma-HCH dehydrochlorinase. A gamma-HCH degradation-negative mutant, named UT72, which lacked the whole linC gene but had the intact linX gene was isolated. The linC gene given in a plasmid could complement UT72. These results strongly suggest that the linC gene but not the linX gene is essential for the assimilation of gamma-HCH in UT26. Deduced amino acid sequences of LinC and LinX show homology to those of members of the short-chain alcohol dehydrogenase family.

Published

1994

24. Identification of the bphA4 gene encoding ferredoxin reductase involved in biphenyl and polychlorinated biphenyl degradation in Pseudomonas sp. strain KKS102.

Author

Kikuchi Y, Nagata Y, Hinata M, Kimbara K, Fukuda M, Yano K, and Takagi M

Subjects

Amino Acid Sequence, Base Sequence, Electrophoresis, Polyacrylamide Gel, Ferredoxin-NADP Reductase metabolism, Genes, Bacterial physiology, Molecular Sequence Data, Oxygenases metabolism, Pseudomonas genetics, Biphenyl Compounds metabolism, Ferredoxin-NADP Reductase genetics, Genes, Bacterial genetics, Iron-Sulfur Proteins, Polychlorinated Biphenyls metabolism, Pseudomonas enzymology

Abstract

The nucleotide sequence of the downstream region of the bph operon from Pseudomonas sp. strain KKS102 was determined. Two open reading frames (ORF1 and ORF2) were found in this region, and the deduced amino acid sequence of ORF2 showed homology with the sequences of four ferredoxin reductases of dioxygenase systems. When this region was inserted just upstream of the bph operon, which does not contain a gene encoding ferredoxin reductase, biphenyl dioxygenase activity was detected. The 24- and 44-kDa polypeptides predicted from the two open reading frames were identified by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. Crude extract which contained the products of ORF2 and bphA1A2A3 showed cytochrome c reduction activity. These data clearly suggest that ORF2 encodes ferredoxin reductase. The deduced amino acid sequence of ORF1 does not show significant homology with the sequences of any other proteins in the SWISS-PROT data bank, and the function of ORF1 is unknown.

Published

1994

25. The hydrophobic repeated domain of the Clostridium cellulovorans cellulose-binding protein (CbpA) has specific interactions with endoglucanases.

Author

Takagi M, Hashida S, Goldstein MA, and Doi RH

Subjects

Bacterial Proteins biosynthesis, Bacterial Proteins isolation & purification, Base Sequence, Binding Sites, Blotting, Western, Carrier Proteins isolation & purification, Carrier Proteins metabolism, Cellulase isolation & purification, Clostridium genetics, Electrophoresis, Polyacrylamide Gel, Immunoenzyme Techniques, Maltose-Binding Proteins, Molecular Sequence Data, Protein Biosynthesis, Recombinant Fusion Proteins isolation & purification, Recombinant Fusion Proteins metabolism, Repetitive Sequences, Nucleic Acid, Restriction Mapping, ATP-Binding Cassette Transporters, Bacterial Proteins metabolism, Cellulase metabolism, Clostridium metabolism, Escherichia coli Proteins, Monosaccharide Transport Proteins, Periplasmic Binding Proteins

Abstract

We overexpressed one of the hydrophobic repeated domains (HBDs) (110 amino acid residues) of the cellulose-binding protein (CbpA) from Clostridium cellulovorans by making a hybrid protein with the Escherichia coli maltose-binding protein (MalE). The HBD was purified to homogeneity, and interactions between the HBD and endoglucanases were analyzed by a novel interaction Western blotting (immunoblotting) method. The HBD had specific interactions with endoglucanases (EngB and EngD) from C. cellulovorans. These results indicated that the HBD was an endoglucanase binding site of CbpA.

Published

1993

26. Cloning and sequencing of a dehalogenase gene encoding an enzyme with hydrolase activity involved in the degradation of gamma-hexachlorocyclohexane in Pseudomonas paucimobilis.

Author

Nagata Y, Nariya T, Ohtomo R, Fukuda M, Yano K, and Takagi M

Subjects

Amino Acid Sequence, Bacterial Proteins genetics, Base Sequence, Cloning, Molecular, DNA, Bacterial genetics, Molecular Sequence Data, Pseudomonas enzymology, Sequence Alignment, Sequence Deletion, Sequence Homology, Amino Acid, Genes, Bacterial, Hexachlorocyclohexane metabolism, Hydrolases genetics, Pseudomonas genetics

Abstract

In Pseudomonas paucimobilis UT26, gamma-hexachlorocyclohexane (gamma-HCH) is converted by two steps of dehydrochlorination to a chemically unstable intermediate, 1,3,4,6-tetrachloro-1,4-cyclohexadiene (1,4-TCDN), which is then metabolized to 2,5-dichloro-2,5-cyclohexadiene-1,4-diol (2,5-DDOL) by two steps of hydrolytic dehalogenation via the chemically unstable intermediate 2,4,5-trichloro-2,5-cyclohexadiene-1-ol (2,4,5-DNOL). To clone a gene encoding the enzyme responsible for the conversion of the chemically unstable intermediates 1,4-TCDN and 2,4,5-DNOL, a genomic library of P. paucimobilis UT26 was constructed in Pseudomonas putida PpY101LA into which the linA gene had been introduced by Tn5. An 8-kb BglII fragment from one of the cosmid clones, which could convert gamma-HCH to 2,5-DDOL, was subcloned, and subsequent deletion analyses revealed that a ca. 1.1-kb region was responsible for the activity. Nucleotide sequence analysis revealed an open reading frame (designated the linB gene) of 885 bp within the region. The deduced amino acid sequence of LinB showed significant similarity to hydrolytic dehalogenase, DhlA (D. B. Janssen, F. Pries, J. van der Ploeg, B. Kazemier, P. Terpstra, and B. Witholt, J. Bacteriol. 171:6791-6799, 1989). The protein product of the linB gene was 32 kDa by sodium dodecyl sulfate-polyacrylamide gel electrophoresis. Not only 1-chlorobutane but also 1-chlorodecane (C10) and 2-chlorobutane, which are poor substrates for other dehalogenases, were good substrates for LinB, suggesting that LinB may be a member of haloalkane dehalogenases with broad-range specificity for substrates.

Published

1993

27. Characterization of the cellulose-binding domain of the Clostridium cellulovorans cellulose-binding protein A.

Author

Goldstein MA, Takagi M, Hashida S, Shoseyov O, Doi RH, and Segel IH

Subjects

Amino Acid Sequence, Bacterial Proteins genetics, Base Sequence, Binding, Competitive, Cloning, Molecular, DNA, Bacterial, Hydrogen-Ion Concentration, Kinetics, Molecular Sequence Data, Polysaccharides metabolism, Solubility, Bacterial Proteins metabolism, Carrier Proteins, Cellulose metabolism, Clostridium metabolism

Abstract

Cellulose-binding protein A (CbpA), a component of the cellulase complex of Clostridium cellulovorans, contains a unique sequence which has been demonstrated to be a cellulose-binding domain (CBD). The DNA coding for this putative CBD was subcloned into pET-8c, an Escherichia coli expression vector. The protein produced under the direction of the recombinant plasmid, pET-CBD, had a high affinity for crystalline cellulose. Affinity-purified CBD protein was used in equilibrium binding experiments to characterize the interaction of the protein with various polysaccharides. It was found that the binding capacity of highly crystalline cellulose samples (e.g., cotton) was greater than that of samples of low crystallinity (e.g., fibrous cellulose). At saturating CBD concentration, about 6.4 mumol of protein was bound by 1 g of cotton. Under the same conditions, fibrous cellulose bound only 0.2 mumol of CBD per g. The measured dissociation constant was in the 1 microM range for all cellulose samples. The results suggest that the CBD binds specifically to crystalline cellulose. Chitin, which has a crystal structure similar to that of cellulose, also was bound by the CBD. The presence of high levels of cellobiose or carboxymethyl cellulose in the assay mixture had no effect on the binding of CBD protein to crystalline cellulose. This result suggests that the CBD recognition site is larger than a simple cellobiose unit or more complex than a repeating cellobiose moiety. This CBD is of particular interest because it is the first CBD from a completely sequenced nonenzymatic protein shown to be an independently functional domain.

Published

1993

28. Purification of two chitinases from Rhizopus oligosporus and isolation and sequencing of the encoding genes.

Author

Yanai K, Takaya N, Kojima N, Horiuchi H, Ohta A, and Takagi M

Subjects

Amino Acid Sequence, Base Sequence, Chitinases metabolism, Chromatography, Gel, Chromatography, Ion Exchange, Cloning, Molecular, DNA, Bacterial isolation & purification, Electrophoresis, Polyacrylamide Gel, Genomic Library, Isoenzymes metabolism, Kinetics, Molecular Sequence Data, Oligonucleotide Probes, Restriction Mapping, Chitinases genetics, Chitinases isolation & purification, DNA, Bacterial genetics, Genes, Bacterial, Isoenzymes genetics, Isoenzymes isolation & purification, Rhizopus enzymology, Rhizopus genetics

Abstract

Two chitinases were purified from Rhizopus oligosporus, a filamentous fungus belonging to the class Zygomycetes, and designated chitinase I and chitinase II. Their N-terminal amino acid sequences were determined, and two synthetic oligonucleotide probes corresponding to these amino acid sequences were synthesized. Southern blot analyses of the total genomic DNA from R. oligosporus with these oligonucleotides as probes indicated that one of the two genes encoding these two chitinases was contained in a 2.9-kb EcoRI fragment and in a 3.6-kb HindIII fragment and that the other one was contained in a 2.9-kb EcoRI fragment and in a 11.5-kb HindIII fragment. Two DNA fragments were isolated from the phage bank of R. oligosporus genomic DNA with the synthetic oligonucleotides as probes. The restriction enzyme analyses of these fragments coincided with the Southern blot analyses described above and the amino acid sequences deduced from their nucleotide sequences contained those identical to the determined N-terminal amino acid sequences of the purified chitinases, indicating that each of these fragments contained a gene encoding chitinase (designated chi 1 and chi 2, encoding chitinase I and II, respectively). The deduced amino acid sequences of these two genes had domain structures similar to that of the published sequence of chitinase of Saccharomyces cerevisiae, except that they had an additional C-terminal domain. Furthermore, there were significant differences between the molecular weights experimentally determined with the two purified enzymes and those deduced from the nucleotide sequences for both genes. Analysis of the N- and C-terminal amino acid sequences of both chitinases and comparison of them with the amino acid sequences deduced from the nucleotide sequences revealed posttranslational processing not only at the N-terminal signal sequences but also at the C-terminal domains. It is concluded that these chitinases are synthesized with pre- and prosequences in addition to the mature enzyme sequences and that the prosequences are located at the C terminal.

Published

1992

29. Design of temperature-sensitive penicillinase repressors by replacement of Pro in predicted beta-turn structures.

Author

Imanaka T, Nakae M, Ohta T, and Takagi M

Subjects

Amino Acid Sequence, Bacillus genetics, Bacillus metabolism, Base Sequence, Blotting, Northern, Molecular Sequence Data, Mutagenesis, Site-Directed, Proline genetics, Proline metabolism, Protein Conformation, Repressor Proteins metabolism, Temperature, Bacillus enzymology, Gene Expression Regulation, Enzymologic genetics, Penicillinase genetics, Repressor Proteins genetics

Abstract

Pro residues in predicted beta-turn structures were substituted with other amino acids to obtain temperature-sensitive penicillinase repressors (PenI). A mutant repressor (P70L; Pro-70 is substituted with Leu) was inactive at 48 degrees C and penP gene expression was derepressed (1,200 U/OD660 [optical density at 660 nm] ), although the mutant was still active at 30 degrees C (27 U). The heat induction ratio (penicillinase activity at 48 degrees C compared with that at 30 degrees C) of the mutant was 98 times higher than that of the wild type (i.e., 44 versus 0.45). This result indicated that the side chain of the Leu residue in P70L destroyed the proper folding of the repressor protein at the elevated temperature, whereas the Pro residue of the wild-type repressor stabilized this predicted beta-turn structure even at 48 degrees C. When the Pro residue was replaced by amino acid residues with smaller side chains (i.e., Gly and Ala), these mutant repressors were less temperature sensitive than P70L. These data suggest that the presence of the Pro residue in the beta-turn structure could be one of the key factors in stabilizing protein structure at elevated temperatures.

Published

1992

30. Drastic alteration of cycloheximide sensitivity by substitution of one amino acid in the L41 ribosomal protein of yeasts.

Author

Kawai S, Murao S, Mochizuki M, Shibuya I, Yano K, and Takagi M

Subjects

Amino Acid Sequence, Base Sequence, Candida genetics, Genetic Engineering, Glutamine genetics, Introns genetics, Molecular Sequence Data, Mutagenesis, Proline genetics, Saccharomyces cerevisiae genetics, Sequence Homology, Nucleic Acid, Codon genetics, Cycloheximide metabolism, Drug Resistance, Microbial genetics, Ribosomal Proteins genetics, Yeasts genetics

Abstract

Cycloheximide is one of the antibiotics that inhibit protein synthesis in most eukaryotic cells. We have found that a yeast, Candida maltosa, is resistant to the drug because it possesses a cycloheximide-resistant ribosome, and we have isolated the gene responsible for this. In this study, we sequenced this gene and found that the gene encodes a protein homologous to the L41 ribosomal protein of Saccharomyces cerevisiae, whose amino acid sequence has already been reported. Two genes for L41 protein, named L41a and L41b, independently present in the genome of S. cerevisiae, were isolated. L41-related genes were also isolated from a few other yeast species. Each of these genes has an intron at the same site of the open reading frame. Comparison of their deduced amino acid sequences and their ability to confer cycloheximide resistance to S. cerevisiae, when introduced in a high-copy-number plasmid, suggested that the 56th amino acid residue of the L41 protein determines the sensitivity of the ribosome to cycloheximide; the amino acid is glutamine in the resistant ribosome, whereas that in the sensitive ribosome is proline. This was confirmed by constructing a cycloheximide-resistant strain of S. cerevisiae having a disrupted L41a gene and an L41b gene with a substitution of the glutamine codon for the proline codon.

Published

1992

31. Molecular cloning of a Pseudomonas paucimobilis gene encoding a 17-kilodalton polypeptide that eliminates HCl molecules from gamma-hexachlorocyclohexane.

Author

Imai R, Nagata Y, Fukuda M, Takagi M, and Yano K

Subjects

Amino Acid Sequence, Bacterial Proteins metabolism, Base Sequence, Blotting, Southern, Cloning, Molecular, Codon, DNA, Bacterial, Genes, Bacterial, Hexachlorocyclohexane analogs & derivatives, Lyases metabolism, Mass Spectrometry, Molecular Sequence Data, Pseudomonas enzymology, Pseudomonas growth & development, Restriction Mapping, Bacterial Proteins genetics, Hexachlorocyclohexane metabolism, Hydrochloric Acid metabolism, Lyases genetics, Pseudomonas genetics

Abstract

Pseudomonas paucimobilis UT26 is capable of growing on gamma-hexachlorocyclohexane (gamma-HCH). A genomic library of P. paucimobilis UT26 was constructed in Pseudomonas putida by using the broad-host-range cosmid vector pKS13. After 2,300 clones were screened by gas chromatography, 3 clones showing gamma-HCH degradation were detected. A 5-kb fragment from one of the cosmid clones was subcloned into pUC118, and subsequent deletion and gas chromatography-mass spectrometry analyses revealed that a fragment of ca. 500 bp was responsible for the conversion of gamma-HCH to 1,2,4-trichlorobenzene via gamma-pentachlorocyclohexene. Nucleotide sequence analysis revealed an open reading frame (linA) of 465 bp within the fragment. The nucleotide sequence of the linA gene and the deduced amino acid sequence showed no similarity to any known sequences. The product of the linA gene was 16.5 kDa according to sodium dodecyl sulfate-polyacrylamide gel electrophoresis.

Published

1991

32. Molecular cloning, nucleotide sequencing, and expression of the Bacillus subtilis (natto) IAM1212 alpha-amylase gene, which encodes an alpha-amylase structurally similar to but enzymatically distinct from that of B. subtilis 2633.

Author

Emori M, Takagi M, Maruo B, and Yano K

Subjects

Amino Acid Sequence, Bacillus subtilis enzymology, Base Sequence, Chimera, Cloning, Molecular methods, DNA, Bacterial genetics, DNA, Bacterial isolation & purification, Gene Library, Molecular Sequence Data, Plasmids, Sequence Homology, Nucleic Acid, Species Specificity, alpha-Amylases metabolism, Bacillus subtilis genetics, Genes, Bacterial, alpha-Amylases genetics

Abstract

An alpha-amylase gene of Bacillus subtilis (natto) IAM1212 was cloned in a lambda EMBL3 bacteriophage vector, and the nucleotide sequence was determined. An open reading frame encoding the alpha-amylase (AMY1212) consists of 1,431 base pairs and contains 477 amino acid residues, which is the same in size as the alpha-amylase (AMY2633) of B. subtilis 2633, an alpha-amylase-hyperproducing strain, and smaller than that of B. subtilis 168, Marburg strain. The amino acid sequence of AMY1212 is different from that of AMY2633 at five residues. Enzymatic properties of these two alpha-amylases were examined by introducing the cloned genes into an alpha-amylase-deficient strain, B. subtilis M15. It was revealed that products of soluble starch hydrolyzed by AMY1212 are maltose and maltotriose, while those of AMY2633 are glucose and maltose. From the detailed analyses with oligosaccharides as substrates, it was concluded that the difference in hydrolysis products of the two similar alpha-amylases should be ascribed to the different activity hydrolyzing low-molecular-weight substrates, especially maltotriose; AMY1212 slowly hydrolyzes maltotetraose and cannot hydrolyze maltotriose, while AMY2633 efficiently hydrolyzes maltotetraose and maltotriose. Further analyses with chimeric alpha-amylase molecules constructed from the cloned genes revealed that only one amino acid substitution is responsible for the differences in hydrolysis products.

Published

1990

33. Nucleotide sequence and cloning in Bacillus subtilis of the Bacillus stearothermophilus pleiotropic regulatory gene degT.

Author

Takagi M, Takada H, and Imanaka T

Subjects

Bacillus subtilis enzymology, Base Sequence, Chromosome Mapping, Flagella physiology, Molecular Sequence Data, Peptide Hydrolases biosynthesis, Protein Conformation, Spores, Bacterial physiology, Transcription, Genetic, Bacillus subtilis genetics, Cloning, Molecular, DNA, Bacterial analysis, Genes, Bacterial, Genes, Regulator, Geobacillus stearothermophilus genetics

Abstract

The regulatory gene (degT) from Bacillus stearothermophilus NCA1503 which enhanced production of extracellular alkaline protease (Apr) was cloned in Bacillus subtilis with pTB53 as a vector. When B. subtilis MT-2 (Npr- [deficiency of neutral protease] Apr+) was transformed with the recombinant plasmid, pDT145, the plasmid carrier produced about three times more alkaline protease than did the wild-type strain. In contrast, when B. subtilis DB104 (Npr- Apr-) was used as a host, the transformant with pDT145 could not exhibit any protease activity. After construction of the deletion plasmids, DNA sequencing was done. A large open reading frame was found, and nucleotide sequence analysis showed that the degT gene was composed of 1,116 bases (372 amino acid residues, molecular weight of 41,244). A Shine-Dalgarno sequence was found nine bases upstream from the open reading frame. A B. subtilis strain carrying degT showed the following pleiotropic phenomena: (i) enhancement of production of extracellular enzymes such as alkaline protease and levansucrase, (ii) repression of autolysin activity, (iii) decrease of transformation efficiency for B. subtilis (competent cell procedure), (iv) altered control of sporulation, (v) loss of flagella, and (vi) abnormal cell division. When B. stearothermophilus SIC1 was transformed with the recombinant plasmid carrying degT, the transformants exhibited abnormal cell division. These phenomena are similar to those of the phenotypes of degSU(Hy) (hyperproduction), degQ(Hy), and degR mutants of B. subtilis. However, the amino acid sequence of the degT product (DegT) is different from those of the reported gene products. Furthermore, DegT includes a hydrophobic core region in the N-terminal portion (amino acid numbers 50 to 160), a consensus sequence for a DNA binding region (amino acid numbers 160 to 179), and a region homologous to transcription activator proteins (amino acid numbers 351 to 366). We discuss the possibility that the membrane protein DegT functions as a sensor protein and transfers the signal of environmental stimuli to the regulatory region of target genes to activate or repress transcription of the genes.

Published

1990

34. Molecular cloning of a thermostable neutral protease gene from Bacillus stearothermophilus in a vector plasmid and its expression in Bacillus stearothermophilus and Bacillus subtilis.

Author

Fujii M, Takagi M, Imanaka T, and Aiba S

Subjects

Bacillus subtilis genetics, DNA Restriction Enzymes, Deoxyribonuclease EcoRI, Geobacillus stearothermophilus enzymology, Hot Temperature, Peptide Hydrolases biosynthesis, Plasmids, Cloning, Molecular, Deoxyribonucleases, Type II Site-Specific, Genes, Geobacillus stearothermophilus genetics, Peptide Hydrolases genetics

Abstract

The structural gene for a thermostable protease from Bacillus stearothermophilus was cloned in plasmid pTB90. It is expressed in both B. stearothermophilus and Bacillus subtilis. B. stearothermophilus carrying the recombinant plasmid produced about 15-fold more protease (310 U/mg of cell dry weight) than did the wild-type strain of B. stearothermophilus. Some properties of the proteases that have been purified from the transformants of B. stearothermophilus and B. subtilis were examined. No significant difference was observed among the enzyme properties studied here despite the difference in host cells. We found that the protease, neutral in pH characteristics and with a molecular weight of 36,000, retained about 80% of its activity even after treatment of 65 degrees C for 30 min.

Published

1983

35. Gene responsible for protecting Escherichia coli from sodium dodecyl sulfate and toluidine blue plus light.

Author

Wakayama Y, Takagi M, and Yano K

Subjects

Base Sequence, Cloning, Molecular, DNA Restriction Enzymes, Dose-Response Relationship, Radiation, Escherichia coli drug effects, Escherichia coli radiation effects, Kinetics, Light, Plasmids, Species Specificity, Ultraviolet Rays, Escherichia coli genetics, Genes, Bacterial, Mutation, Sodium Dodecyl Sulfate toxicity, Tolonium Chloride toxicity

Abstract

Escherichia coli cells were killed by visible light irradiation in the presence of the photosensitizing dye, toluidine blue. Two uvrB mutant strains of E. coli K-12 (AB1885 and N3-1) were much more sensitive than the isogenic uvrA and uvrC strains to treatment with toluidine blue plus light, suggesting that the uvrB+ gene product was involved in repair of DNA damage induced by the treatment. The uvrB+ gene cloned in a high- or low-copy-number plasmid was transformed into the uvrB strain (AB1885). Although all the transformants showed the same resistance as its wild-type strain (AB1157) to UV irradiation, they were as sensitive as AB1885 was to treatment with toluidine blue plus light. The two uvrB strains were more sensitive to sodium dodecyl sulfate than the other strains, suggesting that these strains had a defect in the cell surface. A sodium dodecyl sulfate-resistant revertant obtained from AB1885 was more resistant than AB1885 was to treatment with toluidine blue plus light. The two uvrB strains (AB1885 and N3-1) appear to have a defective gene (tentatively called dvl) different from uvrB. Its map position was around 7 min on the E. coli map.

Published

1984

36. Cloning and sequencing of two tandem genes involved in degradation of 2,3-dihydroxybiphenyl to benzoic acid in the polychlorinated biphenyl-degrading soil bacterium Pseudomonas sp. strain KKS102.

Author

Kimbara K, Hashimoto T, Fukuda M, Koana T, Takagi M, Oishi M, and Yano K

Subjects

Amino Acid Sequence, Base Sequence, Benzoates metabolism, Benzoic Acid, Blotting, Southern, Cloning, Molecular, DNA Mutational Analysis, DNA Transposable Elements, Genes, Molecular Sequence Data, Polychlorinated Biphenyls metabolism, Pseudomonas metabolism, Restriction Mapping, Biphenyl Compounds metabolism, Genes, Bacterial, Pseudomonas genetics

Abstract

Two genes involved in the degradation of biphenyl were isolated from a gene library of a polychlorinated biphenyl-degrading soil bacterium, Pseudomonas sp. strain KKS102, by using a broad-host-range cosmid vector, pKS13. When a 3.2-kilobase (kb) PstI fragment of a 29-kb cosmid DNA insert was subcloned into pUC18 at the PstI site downstream of the lacZ promoter, Escherichia coli cells carrying this recombinant plasmid expressed 2,3-dihydroxybiphenyl dioxygenase activity. Nucleotide sequencing of the 3.2-kb PstI fragment revealed that there were two open reading frames (ORFI [882 base pairs] and ORFII [834 base pairs], in this gene order). Results of analysis of Tn5 insertion mutants and unidirectional deletion mutants suggested that the ORFI coded for 2,3-dihydroxybiphenyl dioxygenase. When the sequence of ORFI was compared with that of bphC of Pseudomonas pseudoalcaligenes KF707 (K. Furukawa, N. Arima, and T. Miyazaki, J. Bacteriol. 169:427-429, 1987), the homology was 68%, with both strains having the same Shine-Dalgarno sequence. The result of gas chromatography-mass spectrometry analysis of the metabolic product suggested that the ORFII had meta cleavage compound hydrolase activity to produce benzoic acid. DNA sequencing suggested that these two genes were contained in one operon.

Published

1989

37. Relaxation of supercoiled plasmid DNA by oxidative stresses in Escherichia coli.

Author

Horiuchi H, Takagi M, and Yano K

Subjects

DNA, Superhelical metabolism, Escherichia coli genetics, Escherichia coli radiation effects, Oxidation-Reduction, Peroxides pharmacology, Photochemistry, Ultraviolet Rays, DNA, Superhelical radiation effects, Escherichia coli metabolism, Plasmids radiation effects

Abstract

The relaxation of plasmid DNA was observed after the visible light irradiation of Escherichia coli AB1157 harboring plasmid pBR322 or some other plasmids in the presence of a photosensitizing dye, such as toluidine blue or acridine orange, and molecular oxygen. Treatment of the cells with hydroperoxides, such as tert-butyl hydroperoxide, cumene hydroperoxide, and hydrogen peroxide, also caused the plasmid DNA relaxation in vivo. Relaxation was not observed in these treatments of purified pBR322 DNA in vitro. Plasmid DNA relaxation was also detected after near-UV irradiation. Far-UV irradiation did not induce such relaxation.

Published

1984

38. Increase of translatable mRNA for major microsomal proteins in n-alkane-grown Candida maltosa.

Author

Sunairi M, Watabe K, Takagi M, and Yano K

Subjects

Candida growth & development, Candida metabolism, Electrophoresis, Polyacrylamide Gel, Fungal Proteins isolation & purification, Kinetics, Alkanes metabolism, Candida genetics, Fungal Proteins genetics, Microsomes metabolism, Protein Biosynthesis, RNA, Messenger genetics

Abstract

In an n-alkane-assimilating Candida sp., transfer from glucose- to n-alkane-containing medium induced changes in the microsomal proteins, and several distinctive polypeptides were demonstrated in the solubilized microsomal fraction derived from n-alkane-grown cells. Long-term-labeling and pulse-labeling experiments in vivo demonstrated the synthesis of the specific microsomal polypeptides. The polypeptides were synthesized as in vitro translation products directed by polyadenylated RNA extracted from n-alkane-grown cells. Two major polypeptides were partially purified from the microsomal fraction from n-alkane-grown cells, and antiserum was prepared in a rabbit. Immunoprecipitation of these two polypeptides was accompanied by an increase in the amount of translatable mRNA. The molecular weights of the polypeptides derived from long-term-labeling, pulse-labeling and in vitro translation experiments appeared to be identical.

Published

1984

39. Nucleotide sequencing and characterization of the genes encoding benzene oxidation enzymes of Pseudomonas putida.

Author

Irie S, Doi S, Yorifuji T, Takagi M, and Yano K

Subjects

Amino Acid Sequence, Base Sequence, Cloning, Molecular, Ferredoxins genetics, Mixed Function Oxygenases genetics, Molecular Sequence Data, Oxidation-Reduction, Oxidoreductases genetics, Plasmids, Pseudomonas enzymology, Benzene metabolism, Genes, Genes, Bacterial, Pseudomonas genetics

Abstract

The nucleotide sequence of the genes from Pseudomonas putida encoding oxidation of benzene to catechol was determined. Five open reading frames were found in the sequence. Four corresponding protein molecules were detected by a DNA-directed in vitro translation system. Escherichia coli cells containing the fragment with the four open reading frames transformed benzene to cis-benzene glycol, which is an intermediate of the oxidation of benzene to catechol. The relation between the product of each cistron and the components of the benzene oxidation enzyme system is discussed.

Published

1987

40. Isolation and sequencing of a genomic clone encoding aspartic proteinase of Rhizopus niveus.

Author

Horiuchi H, Yanai K, Okazaki T, Takagi M, and Yano K

Subjects

Amino Acid Sequence, Aspartic Acid Endopeptidases, Base Sequence, Cloning, Molecular, DNA, Fungal genetics, Molecular Sequence Data, Rhizopus enzymology, Endopeptidases genetics, Genes, Fungal, Rhizopus genetics

Abstract

A gene encoding Rhizopus niveus aspartic proteinase was isolated from an R. niveus genomic library by using oligonucleotides probes corresponding to its partial amino acid sequence, and its nucleotide sequence was determined. By comparing its deduced amino acid sequence with the amino acid sequence of rhizopuspepsin (5, 26), we concluded that the R. niveus aspartic proteinase gene has an intron within its coding region and that it has a preproenzyme sequence of 66 amino acids upstream of the mature enzyme of 323 amino acids.

Published

1988

41. Cloning in Saccharomyces cerevisiae of a cycloheximide resistance gene from the Candida maltosa genome which modifies ribosomes.

Author

Takagi M, Kawai S, Shibuya I, Miyazaki M, and Yano K

Subjects

Candida drug effects, Candida metabolism, Drug Resistance, Microbial, Fungal Proteins biosynthesis, Genes, Fungal, Saccharomyces cerevisiae drug effects, Saccharomyces cerevisiae metabolism, Candida genetics, Cloning, Molecular, Cycloheximide pharmacology, Ribosomes drug effects, Saccharomyces cerevisiae genetics

Abstract

We have previously shown that cycloheximide resistance can be induced in a strain of Candida maltosa by modifying ribosomes (M. Takagi, S. Kawai, Y. Takata, N. Tanaka, M. Sunairi, M. Miyazaki, and K. Yano, J. Gen. Appl. Microbiol. 31:267-275, 1985). The present paper describes the cloning of the gene involved in this resistance (designated RIM-C for ribosome modification by cycloheximide) by using a host-vector system of Saccharomyces cerevisiae.

Published

1986

42. Nucleotide sequence and promoter region for the neutral protease gene from Bacillus stearothermophilus.

Author

Takagi M, Imanaka T, and Aiba S

Subjects

Amino Acid Sequence, Bacillus enzymology, Bacillus genetics, Base Sequence, DNA Restriction Enzymes, Endonucleases, Geobacillus stearothermophilus enzymology, Neprilysin, Plasmids, Single-Strand Specific DNA and RNA Endonucleases, Species Specificity, Transcription, Genetic, Endopeptidases genetics, Genes, Genes, Bacterial, Geobacillus stearothermophilus genetics, Promoter Regions, Genetic

Abstract

The thermostable neutral protease gene nprT of Bacillus stearothermophilus was sequenced. The DNA sequence revealed only one large open reading frame, composed of 1,644 bases and 548 amino acid residues. A Shine-Dalgarno sequence was found 9 bases upstream from the translation start site (ATG), and the deduced amino acid sequence contained a signal sequence in its amino-terminal region. The sequence of the first 14 amino acids of purified extracellular protease completely matched that deduced from the DNA sequence starting at GTC (Val), 687 bases (229 amino acids) downstream from ATG. This suggests that the protease is translated as a longer polypeptide. The amino acid sequence of the extracellular form of this protease (319 amino acids) was highly homologous to that of the thermostable neutral protease from Bacillus thermoproteolyticus but less homologous to the thermolabile neutral protease from Bacillus subtilis. A promoter region determined by S1 nuclease mapping (TTTTCC for the -35 region and TATTTT for the -10 region) was different from the conserved promoter sequences recognized by the known or factors in bacilli. However, it was very homologous to the promoter sequence of the spo0B gene from B. subtilis. The guanine-plus-cytosine content of the coding region of the nprT gene was 58 mol%, while that of the third letter of the codons was much higher (72 mol%).

Published

1985

43. Proton translocation coupled to trimethylamine N-oxide reduction in anaerobically grown Escherichia coli.

Author

Takagi M, Tsuchiya T, and Ishimoto M

Subjects

Anaerobiosis, Chlorates pharmacology, Hydrogen-Ion Concentration, Membrane Potentials, Molybdenum pharmacology, Molybdenum physiology, Molybdenum Cofactors, NADH, NADPH Oxidoreductases metabolism, Nitrate Reductases metabolism, Oxidation-Reduction, Oxidoreductases Acting on CH-NH Group Donors, Pteridines physiology, Coenzymes, Escherichia coli metabolism, Hydrogen metabolism, Metalloproteins, Methylamines metabolism

Abstract

Proton translocation coupled to trimethylamine N-oxide reduction was studied in Escherichia coli grown anaerobically in the presence of trimethylamine N-oxide. Rapid acidification of the medium was observed when trimethylamine N-oxide was added to anaerobic cell suspensions of E. coli K-10. Acidification was sensitive to the proton conductor 3,5-di-tert-butyl-4-hydroxybenzylidenemalononitrile (SF6847). No pH change was shown in a strain deficient in trimethylamine N-oxide reductase activity. The apparent H+/trimethylamine N-oxide ratio in cells oxidizing endogenous substrates was 3 to 4 g-ions of H+ translocated per mol of trimethylamine N-oxide added. The addition of trimethylamine N-oxide and formate to ethylenediaminetetraacetic acid-treated cell suspension caused fluorescence quenching of 3,3'-dipropylthiacarbocyanine [diS-C3-(5)], indicating the generation of membrane potential. These results indicate that the reduction of trimethylamine N-oxide in E. coli is catalyzed by an anaerobic electron transfer system, resulting in formation of a proton motive force. Trimethylamine N-oxide reductase activity and proton extrusion were also examined in chlorate-resistant mutants. Reduction of trimethylamine N-oxide occurred in chlC, chlG, and chlE mutants, whereas chlA, chlB, and chlD mutants, which are deficient in the molybdenum cofactor, could not reduce it. Protons were extruded in chlC and chlG mutants, but not in chlA, chlB, and chlD mutants. Trimethylamine N-oxide reductase activity in a chlD mutant was restored to the wild-type level by the addition of 100 microM molybdate to the growth medium, indicating that the same molybdenum cofactor as used by nitrate reductase is required for the trimethylamine N-oxide reductase system.

Published

1981

44. Construction of a host-vector system in Candida maltosa by using an ARS site isolated from its genome.

Author

Takagi M, Kawai S, Chang MC, Shibuya I, and Yano K

Subjects

Chromosome Mapping, Cloning, Molecular methods, DNA Restriction Enzymes, Escherichia coli genetics, Genes, Fungal, Leucine genetics, Plasmids, Saccharomyces cerevisiae genetics, Transformation, Genetic, Candida genetics, DNA Replication, DNA, Fungal genetics, Genetic Vectors

Abstract

To construct a host-vector system in an n-alkane-assimilating yeast, Candida maltosa, the isolation of an ARS site from its genome which replicates autonomously in C. maltosa was attempted. Leu- mutants of C. maltosa were transformed with a gene library prepared by using YEp13 (LEU2+) as a vector, and Leu+ transformants were obtained at a high frequency. A plasmid named pCS1 was isolated from the recipient cells. pCS1 contained a 6.3-kilobase (kb) fragment of the C. maltosa genome, and a 3.8-kb fragment with ARS activity was subcloned and designated the TRA (transformation ability) region. Vectors (pTRA1 and pTRA11) for C. maltosa J288 were constructed that contained this 3.8-kb fragment, pBR322, and the LEU2 gene of Saccharomyces cerevisiae. Transformation of C. maltosa J288 with these plasmids was successful by both spheroplast and lithium acetate methods. Southern blot analysis suggested that the copy number of pTRA1 in C. maltosa was between 10 and 20, and it was stably maintained during growth without selective pressure in the medium. It was also found that these vectors could transform S. cerevisiae leu2- to LEU2+, suggesting that the TRA region contained an ARS site(s) that was specific not only for C. maltosa but also for S. cerevisiae.

Published

1986

45. Cloning and sequencing of the gene encoding the 72-kilodalton dehydrogenase subunit of alcohol dehydrogenase from Acetobacter aceti.

Author

Inoue T, Sunagawa M, Mori A, Imai C, Fukuda M, Takagi M, and Yano K

Subjects

Amino Acid Sequence, Base Sequence, Cloning, Molecular, DNA, Bacterial genetics, Genes, Genes, Bacterial, Genetic Complementation Test, Molecular Sequence Data, Oligonucleotide Probes, Restriction Mapping, Acetobacter genetics, Alcohol Dehydrogenase genetics

Abstract

A genomic library of Acetobacter aceti DNA was constructed by using a broad-host-range cosmid vector. Complementation of a spontaneous alcohol dehydrogenase-deficient mutant resulted in the isolation of a plasmid designated pAA701. Subcloning and deletion analysis of pAA701 limited the region that complemented the deficiency in alcohol dehydrogenase activity of the mutant. The nucleotide sequence of this region was determined and showed that this region contained the full structural gene for the 72-kilodalton dehydrogenase subunit of the alcohol dehydrogenase enzyme complex. The predicted amino acid sequence of the gene showed homology with sequences of methanol dehydrogenase structural genes of Paracoccus denitrificans and Methylobacterium organophilum.

Published

1989