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1.
Identification of interaction site of pseudoazurin with its redox partner, copper-containing nitrite reductase from Alcaligenes faecalis S-6 总被引:1,自引:0,他引:1
Kukimoto Mutsuko; Nishiyama Makoto; Ohnuki Tatsuya; Turley Stewart; Adman Elinor T.; Horinouchi Sueharu; Beppu Teruhiko 《Protein engineering, design & selection : PEDS》1995,8(2):153-158
Pseudoazurin, a low molecular weight protein containing a singletype I copper, functions as an electron donor to a copper-containingnitrite reductase (NIR) in a denitrifying bacterium Alcaligenesfaecalis S-6. To elucidate the proteinprotein interaction betweenthese two copper-containing proteins, each of nine out of 13lysine residues on the surface of pseudoazurin were independentlyreplaced by alanine or aspartate, and the effects of the mutationson the interaction with NIR, as well as the physicochemicalproperties of pseudoazurin, were analyzed. All of the mutatedpseudoazurins showed optical spectra and oxidation-reductionpotentials almost identical to those of wildtype pseudoazurin,suggesting that none of the replacements of these lysine residuesaffected the environment around the type I copper site. Kineticanalysis of electron transfer between mutated pseudoazurinsand NIR reveals that the lysine mutations have very little effecton the rate of electron transfer to NIR, but substitution atresidues 10, 38, 57 and 77, all close to the copper site, substantiallydecreases the affinity of pseudoazurin for NIR. This suggeststhat pseudoazurin interacts with NIR through the region closeto the type I copper site. The refined X-ray structures of Lys38Aspand Lys10Asp/Lys38Asp show that the molecular structure hasindeed changed little. A new space group is observed for theLys109Ala mutant crystal. Crystal packing interactions changefor the Lys10Asp/Lys38Asp mutant but remain the same for Lys38Aspand Lys59Ala mutants. 相似文献
2.
Yoshiki Nakagawa Hiroyuki Satoh Toshifumi Nakamura Kenji Okajima Sueharu Maenosono Osamu Tokuhiro 《Journal of the Society for Information Display》2004,12(4):435-440
Abstract— A novel liquid‐crystal alignment method, diamond‐like carbon and ion beam alignment (DLC/IB) technology, was announced at the 2001 SID Symposium. And since December 2001, a new‐generation ion‐beam machine has been placed into the manufacturing line of IDTech. DLC/IB technology is mainly used for medical displays, which require a monochrome high‐density and super‐uniform display. We report on the latest developments of these advanced monochrome displays. 相似文献
3.
Site-directed mutagenesis reveals functional contribution of Thr218, Lys220 and Asp304 in chymosin 总被引:1,自引:0,他引:1
Suzuki Junko; Hamu Akio; Nishiyama Makoto; Horinouchi Sueharu; Beppu Teruhiko 《Protein engineering, design & selection : PEDS》1990,4(1):69-71
The functional contributions of amino acid residues Thr218 andAsp304 of chymosin, both of which are highly conserved in theaspartic proteinases, are analysed by means of site-directedmutagenesis. The optimum pH values, milk-clotting (C) and proteolytic(P) activities and kinetic parameters for synthetic oligopeptidesas substrates were examined for the mutant enzymes. The mutationThr2l8Ser caused a marked increase in the C/P ratio, which seemedto be due to a change in substrate recognition. Although thenegative charge of Asp304 had been expected to play a role inlowering the optimum pH values in the aspartic proteinases,this turned out not to be the case in chymosin because boththe mutations Asp304Ala and Asp304Glu caused a similar shiftof the optimum pH towards the acidic side. In addition, themutation Lys220Leu, which we generated previously, was foundto cause a decrease in the C/P ratio, mainly due to the increasein the proteolytic activity. 相似文献
4.
Yohei Katsuyama Yasuo Ohnishi Sueharu Horinouchi 《Chembiochem : a European journal of chemical biology》2010,11(14):2034-2041
Gingerol derivatives are bioactive compounds isolated from the rhizome of ginger. They possess various beneficial activities, such as anticancer and hepatoprotective activities, and are therefore attractive targets of bioengineering. However, the microbial production of gingerol derivatives has not yet been established, primarily because the biosynthetic pathway of gingerol is unknown. Here, we report the production of several dehydrogingerdione (a gingerol derivative) analogues from a recombinant Escherichia coli strain that has an “artificial” biosynthesis pathway for dehydrogingerdione that was not based on the original biosynthesis pathway of gingerol derivatives in plants. The system consists of a 4‐coumarate:CoA ligase from Lithospermum erythrorhizon, a fatty acid CoA ligase from Oryza sativa, a β‐oxidation system from Saccharomyces cerevisiae, and a curcuminoid synthase from O. sativa. To our knowledge, this is the first report of the microbial production of a plant metabolite the biosynthetic pathway of which has not yet been identified. 相似文献
5.
Park Young-Nam; Aikawa Jun-ichi; Nishiyama Makoto; Horinouchi Sueharu; Beppu Teruhiko 《Protein engineering, design & selection : PEDS》1996,9(10):869-875
Residue 75 on the flap, a beta hairpin loop that partially coversthe active site cleft, is tyrosine in most members of the asparticproteinase family. Site-directed mutagenesis was carried outto investigate the functional role of this residue in Rhizomucorpusilus pepsin, an aspartic proteinase with high milk-clottingactivity produced by the fungus Rhizomucor pusillus. A set ofmutated enzymes with replacement of the amino acid at position75 by 17 other amino acid residues except for His and Gly wasconstructed and their enzymatic properties were examined. Strongactivity, higher than that of the wild-type enzyme, was foundin the mutant with asparagine (Tyr75Asn), while weak but distinctactivity was observed in Tyr75Phe. All the other mutants showedmarkedly decreased or negligible activity, less than 1/1000of that of the wild-type enzyme. Kinetic analysis of Tyr75Asnusing a chromogenic synthetic oligopeptide as a substrate revealeda marked increase in kcat with slight change in Km, resultingin a 5.6-fold increase in kcat/km. When differential absorptionspectra upon addition of pepstatin, a specific inhibitor foraspartic proteinase, were compared between the wild-type andmutant enzymes, the wild-type enzyme and Tyr75Asn, showing strongactivity, had spectra with absorption maxima at 280, 287 and293 nm, whereas the others, showing decreased or negligibleactivity, had spectra with only two maxima at 282 and 288 nm.This suggests a different mode of the inhibitor binding in thelatter mutants. These observations suggest a crucial role ofthe residue at position 75 in enhancing the catalytic efficiencythrough affecting the mode of substrate-binding in the asparticproteinases. 相似文献
6.
Hayashi T Kitamura Y Funa N Ohnishi Y Horinouchi S 《Chembiochem : a European journal of chemical biology》2011,12(14):2166-2176
Fatty acyl-AMP ligases (FAALs) activate fatty acids as acyladenylates, and subsequently catalyze their transfer onto the acyl carrier proteins (ACPs) of polyketide synthases (PKSs) or nonribosomal peptide synthetases to produce lipidic metabolites. Myxococcus xanthus contains a polyketide biosynthesis gene cluster in which putative FAAL (FtpD) and ACP (FtpC) genes are located close to a type III PKS (FtpA) gene. Here we describe the characterization of these three proteins in vitro. FtpD adenylated stearic acid and produced stearoyl-FtpC. The stearoyl moiety was then transferred to FtpA. When extender substrates (malonyl-CoA and methylmalonyl-CoA) were added to the reaction, the alkylresorcinol 5-heptadecyl-4-methyl-benzene-1,3-diol was synthesized. Further in vitro analysis indicated that FtpA produces an alkylresorcylic acid as the direct product, and that this decarboxylates to alkylresorcinol nonenzymatically. This is the first report of a FAAL supplying a long-chain fatty acyl-ACP starter substrate to a type III PKS. 相似文献
7.
Awakawa T Fujita N Hayakawa M Ohnishi Y Horinouchi S 《Chembiochem : a European journal of chemical biology》2011,12(3):439-448
A polyketide biosynthesis gene cluster (agq) was found on the genome of a rare actinomycete, Actinoplanes missouriensis. Streptomyces lividans expressing agqA encoding a type III polyketide synthase produced alkylresorcinols mainly from C(16-17) fatty acids. Heterologous expression of the agq genes in S. lividans indicated the function of cognate polyketide modification enzymes; a monooxygenase AgqB hydroxylates the alkylresorcinols to yield 6-alkyl-2-hydroxyhydroquinones, a methyltransferase AgqC catalyzes O-methylation of the alkyl-hydroxyhydroquinones to yield 6-alkyl-2-methoxyhydroquinones, and a UbiA-like prenyltransferase AgqD attaches a prenyl group to the C-4 hydroxy group of the alkyl-methoxyhydroquinones to yield 6-alkyl-4-O-geranyl-2-methoxyhydroquinones and 6-alkyl-4-O-dihydrofarnesyl-2-methoxyhydroquinones derived from C(16-17) fatty acids. In contrast, A. missouriensis was found to produce 6-alkyl-4-O-dihydrogeranyl-2-methoxyhydroquinones derived from C(16-18) fatty acids by the function of the agq gene cluster. All of these prenylated phenolic lipids were novel compounds. 相似文献
8.
Matsuyama A Shirai A Yashiroda Y Kamata A Horinouchi S Yoshida M 《Yeast (Chichester, England)》2004,21(15):1289-1305
A novel series of plasmid vectors named pDUAL have been developed. These vectors enable one to introduce not only multicopies of genes with episomal maintenance but also a single copy with chromosomal integration into the fission yeast, Schizosaccharomyces pombe. The multicopy plasmids can be easily converted to fragments for chromosomal integration by digestion of the plasmids with a certain restriction endonuclease before transformation of the yeast cells. The resultant fragments, lacking the autonomously replicating sequence, are designed for targeting into the chromosomal leu1 locus by homologous recombination. Whether the transformants are the results of episomal maintenance of the plasmid or homologous gene targeting can be readily checked by their requirement for uracil or leucine, or by the PCR diagnostic analysis. Furthermore, we propose the use of pDUAL derivatives for PCR-based chromosomal tagging of a gene to introduce several tags into 5'-terminus of a gene, employing a set of primers. Using these all-in-one vectors, a suitable mode of expression of a cloned gene can be selected for individual analysis without any complicated subcloning processes. 相似文献
9.
Nishiyama Makoto; Suzuki Junko; Ohnuki Tatsuya; Chang Hae Choon; Horinouchi Sueharu; Turley Stewart; Adman Elinor T.; Beppu Teruhiko 《Protein engineering, design & selection : PEDS》1992,5(2):177-184
Pseudoazurin (a blue copper protein or cupredoxin) of a denitrifyingbacterium Alcaligenes faecalis S-6 is a direct electron carrierfor a Cu-containing nitrite reductase (NIR) of the same organism.Site-directed mutagenesis of the pseudoazurin was carried outusing an Escherichia coli expression system. Replacement ofTyr74 by Phe to remove an internal hydrogen bond in the ß-barrelcaused a slight decrease in heat stability as well as a requirementfor a higher concentration of Cu2+ for production in the E.colihost. Exchange of Ala for Pro80 adjacent to His81, one of thefour ligands binding a type I Cu atom, caused a marked increasein reduction potential by 139 mV without change in the opticalabsorption spectrum. The ability of the pseudoazurin to transferelectrons to NIR was markedly diminished but the apparent Kmof NIR for pseudoazurin was not affected by the mutation. X-raydiffraction data collected on the oxidized and reduced formsof the Pro80Ala mutant show that a water molecule occupies thepocket created by the absent side chain. This observation suggeststhat the increase in reduction potential may be caused due tothe increased solvent accessibility to the Cu atom. The electrondensity difference maps on these structures (at 2.0 Å)show that this water moves during the change in oxidation state,and that there are small, but localized, conformational changes>6.5 Å from the copper site, as well as movement ofboth the Cu2+ and the cysteinate sulfur. 相似文献
10.
Suzuki Junko; Sasaki Katsutoshi; Sasao Yuko; Hamu Akio; Kawasaki Hisashi; Nishiyama Makoto; Horinouchi Sueharu; Beppu Teruhiko 《Protein engineering, design & selection : PEDS》1989,2(7):563-569
Artificial mutations of chymosin by recombinant DNA techniqueswere generated to analyze the structurefunction relationshipin this characteristic aspartk proteinase. In order to preparethe mutant enzymes in their active form, we established proceduresfor purification of correctly refolded prochymosin from inclusionbodies produced in Escherichia coli transformants and for itssubsequent activation. Mutagenesis by linker insertion intocDNA produced several mutants with an altered ratio of milkclotting activity to proteolytic activity and a different extentof stability. In addition to these mutants, several mutantswith a single amino acid exchange were also constructed by site-directedmutagenesis and kinetic parameters of these mutant enzymes weredetermined by using synthetic hexa- and octa-peptides as substrates.Exchange of Tyr75 on the flap of the enzyme to Phe caused amarked change of substrate specificity due to the change ofkcat or Km, depending on the substrate used. Exchange of Val110and Phe111 also caused a change of kinetic parameters, whichindicates functional involvement of these hydrophobic residuesin both the catalytic function and substrate binding. The mutantLys220Leu showed a marked shift of the optimum pH tothe acidic side for hydrolysis of acid-denatured haemoglobinalong with a distinct increase in kcat for the octa-peptidein a wide pH range. 相似文献