ABSTRACT
Cellobiose 2-epimerase (CE) is a promising industrial enzyme that can catalyze bioconversion of lactose to its high-value derivatives, namely epilactose and lactulose. A need exists in the dairy industry to catalyze lactose bioconversions at low temperatures to avoid microbial growth. We focused on the discovery of cold-active CE in this study. A genome mining method based on computational prediction was used to screen the potential genes encoding cold-active enzymes. The CE-encoding gene from Roseburia intestinalis, with a predicted high structural flexibility, was expressed heterologously in Escherichia coli. The catalytic property of the recombinant enzyme was extensively studied. The optimum temperature and pH of the enzyme were 45°C and 7.0, respectively. The specific activity of this enzyme to catalyze conversion of lactose to epilactose was measured to be 77.3 ± 1.6 U/mg. The kinetic parameters, including turnover number (kcat), Michaelis constant (Km), and catalytic efficiency (kcat/Km) using lactose as a substrate were 117.0 ± 7.7 s-1, 429.9 ± 57.3 mM, and 0.27 mM-1s-1, respectively. In situ production of epilactose was carried out at 8°C: 20.9% of 68.4 g/L lactose was converted into epilactose in 4 h using 0.02 mg/mL (1.5 U/mL, measured at 45°C) of recombinant enzyme. The enzyme discovered by this in silico method is suitable for low-temperature applications.
Subject(s)
Carbohydrate Epimerases/analysis , Clostridiales/enzymology , Computing Methodologies , Cellobiose/metabolism , Clostridiales/genetics , Cold Temperature , Data Mining , Disaccharides/metabolism , Escherichia coli/genetics , Hydrogen-Ion Concentration , Kinetics , Lactulose/metabolism , Recombinant Proteins/genetics , Recombinant Proteins/metabolism , TemperatureABSTRACT
Aldose 1-epimerases or mutarotases (EC 5.1.3.3) are catalyzing the interconversion of α- and ß-anomers of hemiacetals of aldose sugars such as D-glucose and D-galactose, and are presumed to play an auxiliary role in carbohydrate metabolism as mutarotation occurs spontaneously in watery solutions. The first step in the Leloir pathway of D-galactose breakdown is preceded by accelerated conversion of ß-D-galactopyranose into the α-anomer, the substrate of the anomer-specific D-galactose 1-kinase. Here, we identified two putative aldose-1-epimerase genes (galmA and galmB) in the model organism Aspergillus nidulans, and characterized them upon generation of single- and double deletion mutant strains, as well as overexpressing mutants carrying multiple copies of either. Assaying cell-free extracts from the galmB single- and galm double mutants, we observed that the mutarotation hardly exceeded spontaneous anomer conversion, while galmB multicopy strains displayed higher activities than the wild type, increasing with the copy number. When grown on D-galactose in submerged cultures, biomass formation and D-galactose uptake rates in mutants lacking galmB were considerably reduced. None such effects were observed studying galmA deletion mutants, which consistently behave like the wild type. We conclude that GalmB is the physiologically relevant mutarotase for the utilization of D-galactose in A. nidulans.
Subject(s)
Aspergillus nidulans/enzymology , Carbohydrate Epimerases/metabolism , Fungal Proteins/metabolism , Galactose/metabolism , Aspergillus nidulans/genetics , Carbohydrate Epimerases/analysis , Carbohydrate Epimerases/genetics , Fungal Proteins/analysis , Fungal Proteins/genetics , Gene Deletion , Glucose/metabolismABSTRACT
Alginates are natural polymers composed of mannuronic and guluronic acid residues. They are currently extracted from brown algae; however, alginate can also be synthesized by some species of Azotobacter and Pseudomonas. Alginates with different proportion of mannuronic and guluronic acids are known to have different characteristics and form gels at different extents in the presence of calcium ions. The aim of this work was to investigate the usefulness of alginate as a non-toxic coagulant used in purification of drinking water. This study utilized alginates from Azotobacter vinelandii having different guluronic acid levels. These were obtained partly by changing the cultivation parameters, partly by epimerizing a purified alginate sample in vitro using the A. vinelandii mannuronan C-5 epimerase AlgE1. The different alginates were then used for coagulation together with calcium. The results showed that turbidity removal capability was dependent on the content of guluronic acid residues. For the best performing samples, the turbidity decreased from 10 NTU to 1 NTU by the use of only 2 mg/L of alginate and 1.5 mM of calcium chloride.
Subject(s)
Alginates , Hexuronic Acids/analysis , Water Purification , Alginates/chemistry , Amino Acid Sequence , Azotobacter vinelandii/chemistry , Carbohydrate Epimerases/analysis , Glucuronic Acid/chemistryABSTRACT
Several real-time polymerase chain reaction (PCR) assays have been developed to detect and quantify Shiga toxin-producing Escherichia coli (STEC) O157:H7, but none have targeted the O-antigen specific gene (rfbEO157) in combination with the three major virulence genes, stx1, stx2, and eae. Our objectives were to develop and validate a four-plex, quantitative PCR (mqPCR) assay targeting rfbE(O157), stx1, stx2, and eae for the detection and quantification of STEC O157 in cattle feces, and compare the applicability of the assay to detect STEC O157 to a culture method and conventional PCR (cPCR) targeting the same four genes. Specificity of the mqPCR assay to differentially detect the four genes was confirmed with strains of O157 and non-O157 STEC with different profiles of target genes. In cattle feces spiked with pure cultures, detection limits were 2.8×10(4) and 2.8×10(0) colony-forming units/g before and after enrichment, respectively. Detection of STEC O157 in feedlot cattle fecal samples (n=278) was compared between mqPCR, cPCR, and a culture method. The mqPCR detected 48.9% (136/278) of samples as positive for E. coli O157. Of the 100 samples that were randomly picked from 136 mqPCR-positive samples, 35 and 48 tested positive by cPCR and culture method, respectively. Of the 100 samples randomly chosen from 142 mqPCR-negative samples, all were negative by cPCR, but 21 samples tested positive by the culture method. McNemar's chi-square tests indicated significant disagreement between the proportions of positive samples detected by the three methods. In conclusion, the mqPCR assay that targets four genes is a novel and more sensitive method than the cPCR or culture method to detect STEC O157 in cattle feces. However, the use of real-time PCR as a screening method to identify positive samples and then subjecting only positive samples to a culture method may underestimate the presence of STEC O157 in fecal samples.
Subject(s)
Adhesins, Bacterial/analysis , Escherichia coli O157/genetics , Escherichia coli Proteins/analysis , Feces/microbiology , Real-Time Polymerase Chain Reaction/methods , Adhesins, Bacterial/genetics , Animals , Carbohydrate Epimerases/analysis , Carbohydrate Epimerases/genetics , Cattle , Escherichia coli O157/isolation & purification , Escherichia coli Proteins/genetics , Shiga Toxin 1/analysis , Shiga Toxin 1/genetics , Shiga Toxin 2/analysis , Shiga Toxin 2/genetics , Transaminases/analysis , Transaminases/geneticsABSTRACT
Enterohemorrhagic Escherichia coli O157, a verocytotoxin (VT1/2)-producing pathogen, can be deadly because it can induce acute or chronic renal failure. To speed up the clinical diagnosis of related syndromes caused by E. coli O157, there is an urgent need for rapid, simple, and reliable analytical tools for its quantitation. In this study, we developed a novel electrochemical competitive genosensor, featuring gold-electrodeposited screen-printed electrodes (nanoAu/SPE) modified with a self-assembled monolayer of thiol-capped single-stranded DNA (capture probe), for the detection of the rfbE gene, which is specific to E. coli O157. This assay functions based on competition between the target gene (complementary to the capture probe DNA) and reporter DNA-tagged, hexaammineruthenium(III) chloride-encapsulated liposomes. The current signal of the released liposomal Ru(NH(3))(6)(3+) was measured using square wave voltammetry, yielding a sigmoidally shaped dose-response curve whose linear portion was over the range from 1 to 10(6) fmol. This liposomal competitive assay provides an amplification route for the detection of the rfbE gene at ultratrace levels; indeed, we could detect as little as 0.75 amol of the target rfbE DNA (equivalent to the amount present in 5 microL of a 0.15 pM solution).
Subject(s)
Biosensing Techniques/methods , DNA Probes/metabolism , Escherichia coli O157/isolation & purification , Base Sequence , Carbohydrate Epimerases/analysis , Carbohydrate Epimerases/genetics , DNA Probes/genetics , DNA, Bacterial/analysis , DNA, Bacterial/genetics , Electrochemistry , Electrodes , Escherichia coli O157/genetics , Genes, Reporter , Kinetics , Liposomes/chemistry , Liposomes/metabolism , Nucleic Acid Amplification Techniques , Organometallic Compounds/chemistry , Organometallic Compounds/metabolism , Oxidation-Reduction , Ruthenium/chemistry , Staining and Labeling , Surface Plasmon Resonance , Transaminases/analysis , Transaminases/geneticsABSTRACT
A real-time reverse transcription multiplex polymerase chain reaction (rRT-MPCR) was developed for detection of mRNA encoded by rfbE and eae genes of enterohemorrhagic Escherichia coli (EHEC) O157:H7. A 129-bp and a 106-bp sequence specific to rfbE and eae, respectively, were targeted for reverse transcription, amplification, and real-time detection. A single-step RT-PCR kit containing a mixture of reverse transcriptases converted mRNA into cDNA, which was subsequently amplified by Taq polymerase included in the same kit. The real-time detection of amplification products was achieved by incorporating rfbE(O157)- and eae(O157:H7)-specific TaqMan probes in rRT-MPCR. The ability of two sets of primers and probes for specific detection of rfbE(O157) and eae(O157:H7) was initially verified by screening RNA of eight E. coli serotypes possessing different O antigens and eae alleles. These two sets of primers and probes were also tested in a standard real-time PCR (rPCR) using DNA prepared from several E. coli and non-E. coli strains to verify that only rfbE(O157)- and eae(O157:H7)-specific sequences were amplified and detected. The rRT-MPCR was then evaluated for detecting low-level contamination of EHEC O157:H7 in feces. When RNA prepared from bovine feces, which were artificially seeded with EHEC O157:H7 cells and cultured for five hours, was tested in rRT-MPCR as low as 1cfu/g of feces could be detected. The detection range for the two genes in fecal cultures was 5.1 x 10(-1)-5.1 x 10(4) cfu/g of feces. Thus, the described procedure could be applied to rapid detection of very low levels of EHEC O157:H7 using total RNA as a template. Since the presence of rfbE(O157)- and eae(O157:H7)-specific mRNA is dependent on replicating cells, rRT-MPCR could provide important information about the viability of EHEC O157:H7 in feces.
Subject(s)
Adhesins, Bacterial/analysis , Carbohydrate Epimerases/analysis , Cattle/microbiology , Escherichia coli O157/metabolism , Escherichia coli Proteins/analysis , Feces/microbiology , Transaminases/analysis , Animals , DNA Primers/chemistry , Feces/chemistry , Polymerase Chain Reaction/veterinary , RNA, Messenger/analysisSubject(s)
Azotobacter vinelandii/enzymology , Carbohydrate Epimerases/analysis , Carbohydrate Epimerases/chemistry , Nuclear Magnetic Resonance, Biomolecular , Alginates/analysis , Alginates/chemistry , Amino Acid Sequence , Carbon Isotopes , Protein Sorting Signals , Protein Structure, Secondary , Recombinant Proteins/analysis , Recombinant Proteins/chemistryABSTRACT
Alginate biosynthesis involves C-5-mannuronan epimerases catalyzing the conversion of beta-D-mannuronic acid to alpha-L-guluronic acid at the polymer level. Mannuronan epimerases are modular enzymes where the various modules yield specific sequential patterns of the converted residues in their polymer products. Here, the interaction between the AlgE4 epimerase and mannuronan is determined by dynamic force spectroscopy. The specific unbinding between molecular pairs of mannuronan and AlgE4 as well as its two modules, A and R, respectively, was studied as a function of force loading rate. The mean protein-mannuronan unbinding forces were determined to be in the range 73-144 pN, depending on the protein, at a loading rate of 0.6 nN/s, and increased with increasing loading rate. The position of the activation barrier was determined to be 0.23 +/- 0.04 nm for the AlgE4 and 0.10 +/- 0.02 nm for its A-module. The lack of interaction observed between the R-module and mannuronan suggest that the A-module contains the binding site for the polymer substrate. The ratio between the epimerase-mannuronan dissociation rate and the catalytic rate for epimerization of single hexose residues suggests a processive mode of action of the AlgE4 epimerase yielding the observed sequence pattern in the uronan associated with the A-module of this enzyme.
Subject(s)
Carbohydrate Epimerases/analysis , Carbohydrate Epimerases/chemistry , Polymers/analysis , Polymers/chemistry , Catalysis , Enzymes, Immobilized/chemistry , Escherichia coli/enzymology , Escherichia coli/genetics , Macromolecular Substances/analysis , Macromolecular Substances/chemistry , Mannans/analysis , Mannans/chemistry , Microscopy, Atomic Force/methods , Polysaccharides/chemistry , Pseudomonas/enzymology , Recombinant Proteins/analysis , Recombinant Proteins/chemistry , Substrate SpecificityABSTRACT
A new procedure for quantitating the amount of N-acetyl-D-mannosamine (ManNAc) or ManNAc-6-phosphate produced by 2'-epimerase activities involved in sialic acid metabolism has been developed. The ManNAc generated by the action of N-acetyl-D-glucosamine (GlcNAc) and UDP-GlcNAc 2'-epimerases is condensed with pyruvate through the action of N-acetylneuraminate lyase and the sialic acid released is measured by the thiobarbituric acid assay. For the analysis of prokaryotic GlcNAc-6-phosphate 2'-epimerase, ManNAc-6-phosphate can also be evaluated by this coupled assay after dephosphorylation of the sugar phosphate. This system provides a sensitive, rapid, reproducible, specific and simple procedure (feasible with commercial reagents) for measuring amino sugar 2'-epimerases from eukaryotic and prokaryotic sources. The technique reported here permitted us to detect UDP-GlcNAc 2'-epimerase and GlcNAc 2'-epimerase in mammalian cell extracts and GlcNAc-6-phosphate 2'-epimerase in bacterial extracts.
Subject(s)
Amino Sugars/metabolism , Carbohydrate Epimerases/analysis , Carrier Proteins , Escherichia coli Proteins , Animals , Bacteria , Carbohydrate Epimerases/chemistry , Kidney/enzymology , Liver/enzymology , Oxo-Acid-Lyases/chemistry , Rats , Scintillation Counting , Spectrophotometry/methods , Swine , ThiobarbituratesABSTRACT
A relatively simple assay procedure for measuring the reactions catalyzed by polyuronic acid C-5 epimerases has been developed. Action of C-5 epimerases inverts the C-6 carboxyl group of polyuronic acids converting beta-linked residues into alpha-linked residues or vice versa. The assay takes advantage of the greater susceptibility of the acid hydrolysis of alpha-glycosidic linkages than beta-glycosidic linkages. The method involves the partial acid hydrolysis of the polyuronic acid before and after reaction with the C-5 epimerase. The greater or lesser amounts of uronic acid released (solubilized) before and after reaction of the C-5 epimerase are a measure of the amount of alpha- or beta-glycosidic linkages that are formed and a measure of the amount of catalysis by the enzyme.
Subject(s)
Carbohydrate Epimerases/analysis , Alginates/chemistry , Azotobacter vinelandii/enzymology , Carbohydrate Conformation , Carbohydrate Epimerases/metabolism , Glucuronates/analysis , Glucuronates/metabolism , Glucuronic Acid , Hexuronic Acids/analysis , Hexuronic Acids/metabolism , Hydrogen-Ion Concentration , Hydrolysis , Kinetics , Spectrophotometry , Uronic Acids/chemistryABSTRACT
A method to prepare UDP-galactofuranose (UDP-Galf) free of UDP-galactopyranose (UDP-Galp) is described. The UDP-Galf is synthesized enzymatically from UDP-Galp using the enzyme UDP-galactopyranose mutase. Treatment of UDP-Galp with the enzyme yields an equilibrium mixture of UDP-Galp and UDP-Galf in which UDP-Galf is approximately 7%. In spite of its low yield, the UDP-Galf is readily purified from starting UDP-Galp using a Dionex PA-100 ion exchange HPLC column. The purified UDP-Galf was characterized by chemical degradations, by electrospray mass spectrometry, and by several nuclear magnetic resonance techniques. In addition, an HPLC assay for the enzyme UDP-galactopyranose mutase is presented that requires 0.5 microgram of UDP-Galf per assay and can be used for both qualitative and quantitative measurements of the enzyme activity. These procedures should thus aid in the characterization of the enzymes involved in galactofuranosyl biosynthesis for the cell walls of Mycobacteria, for the lipophosphoglycan of Leishmania, and for other microorganisms where galactofuranosyl residues are found.
Subject(s)
Bacterial Proteins/analysis , Carbohydrate Epimerases/analysis , Chromatography, High Pressure Liquid/methods , Escherichia coli Proteins , Galactose/analogs & derivatives , Intramolecular Transferases , Uridine Diphosphate/analogs & derivatives , Bacterial Proteins/metabolism , Carbohydrate Epimerases/metabolism , Enzyme-Linked Immunosorbent Assay , Escherichia coli/enzymology , Galactose/biosynthesis , Galactose/chemistry , Galactose/isolation & purification , Magnetic Resonance Spectroscopy , Mass Spectrometry , Spectrophotometry, Ultraviolet , Uridine Diphosphate/biosynthesis , Uridine Diphosphate/chemistry , Uridine Diphosphate/isolation & purificationABSTRACT
In order to study the tryptophan biosynthetic enzymes of the plant Arabidopsis thaliana, polyclonal antibodies were raised against five of the tryptophan biosynthetic pathway proteins: anthranilate synthase alpha subunit, phosphoribosylanthranilate transferase, phosphoribosylanthranilate isomerase, and the tryptophan synthase alpha and beta subunits. Immunoblot analysis of Arabidopsis leaf protein extracts revealed that the antibodies identify the corresponding proteins that are enriched in Arabidopsis chloroplast fractions. Precursors of phosphoribosylanthranilate isomerase and tryptophan synthase alpha subunit were synthesized by in vitro translation. The precursors were efficiently imported and processed by isolated spinach chloroplasts, and the cleavage sites within the precursors were determined. These results provide the first direct evidence that the tryptophan biosynthetic enzymes from Arabidopsis are synthesized as higher molecular weight precursors and then imported into chloroplasts and processed into their mature forms.
Subject(s)
Aldose-Ketose Isomerases , Anthranilate Phosphoribosyltransferase/metabolism , Anthranilate Synthase/metabolism , Arabidopsis/enzymology , Carbohydrate Epimerases/metabolism , Chloroplasts/enzymology , Tryptophan Synthase/metabolism , Tryptophan/biosynthesis , Amino Acid Sequence , Anthranilate Phosphoribosyltransferase/analysis , Anthranilate Phosphoribosyltransferase/biosynthesis , Anthranilate Synthase/analysis , Anthranilate Synthase/biosynthesis , Carbohydrate Epimerases/analysis , Carbohydrate Epimerases/biosynthesis , Cloning, Molecular , Enzyme Precursors/metabolism , Escherichia coli , Glutathione Transferase/analysis , Glutathione Transferase/biosynthesis , Immunoblotting , Macromolecular Substances , Molecular Sequence Data , Molecular Weight , Protein Processing, Post-Translational , Recombinant Fusion Proteins/analysis , Recombinant Fusion Proteins/biosynthesis , Tryptophan Synthase/analysis , Tryptophan Synthase/biosynthesisABSTRACT
Glucose isomerase from Streptomyces phaeochromogenes was purified from a commercial preparation, Swetase, by DEAE-cellulose, Bio-Gel A-0.5 m, and hydroxyapatite column chromatographies. It was found to be 2 fractions; F-A, not adsorbed on hydroxyapatite and F-B, adsorbed on hydroxyapatite. They were homogeneous in ordinary and SDS-PAGE and had similarities in some enzymatic and physico-chemical properties. The differences, however, were found in the N-terminal amino acid, which was only serine for F-A while it was serine and alanine for F-B, and also in their peptide mapping patterns of digests with trypsin, Achromobacter protease I, and cyanogen bromide. The results suggest that glucose isomerase from S. phaeochromogenes was composed of the two kinds of isozymes and that each of isozymes was a tetramer constituted of non-identical subunits.
Subject(s)
Aldose-Ketose Isomerases , Carbohydrate Epimerases/analysis , Isoenzymes/analysis , Streptomyces/enzymology , Amino Acid Sequence , Bacterial Proteins/isolation & purification , Chemical Phenomena , Chemistry, Physical , Chromatography, Ion Exchange , Drug Stability , Electrophoresis, Polyacrylamide Gel , Hydrogen-Ion Concentration , Hydroxyapatites , Isoelectric Focusing , Kinetics , Metals , Molecular Sequence Data , Peptide Mapping , Substrate Specificity , Temperature , TrypsinABSTRACT
Glucose isomerase was immobilized onto granular chicken bone (BIOBONE) by adsorption. The amount of activity bound relative to an equal amount of free enzyme was 32 +/- 1%, with the estimated specific activity decreasing from 11.1 +/- 0.7 to 3.9 +/- 0.5 U/mg protein with immobilization. Compared with the free enzyme, immobilized glucose isomerase showed a threefold increase in the Km for fructose and a fivefold decrease in Vmax. High operating temperatures were possible (greater than 55 degrees C), but continuous use and long-term storage studies showed gradual losses of activity. Both the binding and the activity of the bone-immobilized enzyme were highly resistant to treatments with detergent, ethanol, and KCl. Studies to determine mass transfer limitation effects on immobilized glucose isomerase showed that these were insignificant for this system.
Subject(s)
Aldose-Ketose Isomerases , Carbohydrate Epimerases/chemistry , Enzymes, Immobilized , Adhesiveness , Animals , Carbohydrate Epimerases/analysis , Chickens , Enzyme Stability , Hydrogen-Ion Concentration , Kinetics , Proteins/analysis , TemperatureABSTRACT
Wild-type strains of Escherichia coli were unable to utilize L-ribose for growth. However, L-ribose-positive mutants could be isolated from strains of E. coli K-12 which contained a ribitol operon. L-ribose-positive strains of E. coli, isolated after 15 to 20 days, had a growth rate of 0.22 generation per h on L-ribose. Growth on L-ribose was found to induce the enzymes of the L-arabinose and ribitol pathways, but only ribitol-negative mutants derived from strains originally L-ribose positive lost the ability to grow on L-ribose, showing that a functional ribitol pathway was required. One of the mutations permitting growth on L-ribose enabled the mutants to produce constitutively an NADPH-linked reductase which converted L-ribose to ribitol. L-ribose is not metabolized by an isomerization to L-ribulose, as would be predicted on the basis of other pentose pathways in enteric bacteria. Instead, L-ribose was metabolized by the reduction of L-ribose to ribitol, followed by the conversion to D-ribulose by enzymes of the ribitol pathway.
Subject(s)
Aldose-Ketose Isomerases , Escherichia coli/metabolism , Phosphotransferases (Alcohol Group Acceptor) , Ribose/metabolism , Arabinose/metabolism , Carbohydrate Epimerases/analysis , Chromatography, Thin Layer , Chromosome Mapping , Electrophoresis , Escherichia coli/enzymology , Escherichia coli/genetics , Mutation , Phosphotransferases/analysis , Sugar Alcohol Dehydrogenases/analysis , Transduction, GeneticABSTRACT
The procedure of isolation, purification, and characterization of glucosamine-6-phosphate acetylase from the pig liver is described. The steps of purification were as follows: adsorption on hydroxylapatite, fractionation with ammonium sulfate, chromatography on cellulose phosphate, electrofocusing, and preparative gel electrophoresis. A highly purified (about 3000-fold) preparation of GlcN-6-P acetylase, with a yield of 23%, was obtained. It was found that GlcN-6-P acetylase from pig liver is heterogeneous and exists in two active forms. The characteristic features of the preparation were established: Mr, about 24 kDa; temperature optimum at 37 degrees; pH optimum at 7.45; and Km (GlcN-6-P) 3.7 x 10(-3) M and Km (AcCoA) 1.4 x 10(-3) M. The ions K+, Na+, NH4+, Mg2+, Mn2+, and CH3COO- do not stimulate the acetylase activity. The product of acetylase reaction (GlcNAc-6-P) inhibits this reaction according to the feedback process. The highly purified preparation of GlcN-6-P acetylase is unstable during storage and it is protected by ampholine or glycine from enzyme inactivation, but it is not protected by 2-mercaptoethanol.
Subject(s)
Acetyltransferases/isolation & purification , Aldose-Ketose Isomerases , Liver/enzymology , Acetyltransferases/analysis , Acetyltransferases/metabolism , Adsorption , Animals , Carbohydrate Epimerases/analysis , Carbohydrate Epimerases/isolation & purification , Carbohydrate Epimerases/metabolism , Chromatography, Gel , Chromatography, Ion Exchange , Electrophoresis, Polyacrylamide Gel , Glucosamine 6-Phosphate N-Acetyltransferase , Hydroxyapatites , In Vitro Techniques , Isoelectric Focusing , Kinetics , Molecular Weight , Proteins/analysis , SwineABSTRACT
The structure of the complex between sodium dodecyl sulfate (SDS) and a deuterated bifunctional enzyme, N-5'-phosphoribosylanthranilate isomerase/indole-3-glycerol-phosphate synthase (Mr 49,484), has been studied in dilute solution by small-angle neutron scattering. The complex nearly acquired its final size, as shown by molecular-sieve chromatography, at the chosen SDS concentration of 1.6 mM, which is slightly below the critical micelle concentration of 1.8 mM (at the ionic strength of 0.1 M). The 452 amino-acid residues of the bifunctional enzyme were combined with 216 detergent molecules. The complex was found to be composed of three protein-decorated SDS micelles of unequal size, connected by short flexible polypeptide segments. The largest of the three micelles was the middle one. The SDS-protein complex contained the dodecyl hydrocarbon moieties in three globular cores. Each core was surrounded by a hydrophilic shell, formed by the hydrophilic and amphiphilic stretches of the polypeptide chain, and by the sulfate head groups of the detergent. The average thickness of these shells was 0.7-0.8 nm. The three-micelle complex was cleaved with trypsin at a single site, possibly in a micelle-connecting segment, into a single-micelle fragment at the carboxyl-terminal which comprised 73 SDS molecules and 163 amino-acid residues, and a dual-micelle fragment. One of the micelles within this larger fragment contained 42 SDS molecules and about 90 amino-acid residues; the other micelle contained 101 SDS molecules and about 190 amino-acid residues. The individual micelle sizes seemed to be determined by the amino-acid sequence.
Subject(s)
Aldose-Ketose Isomerases , Carbohydrate Epimerases/analysis , Carboxy-Lyases/analysis , Colloids , Indole-3-Glycerol-Phosphate Synthase/analysis , Micelles , Multienzyme Complexes/analysis , Sodium Dodecyl Sulfate , Colloids/analysis , Escherichia coli/enzymology , Neutrons , Particle Size , Peptide Fragments/analysis , Peptides/analysis , Protein Conformation , Scattering, Radiation , Solubility , TrypsinABSTRACT
Group-specific chemical modifications of D-xylose isomerase from Streptomyces violaceruber indicated that complete loss of activity is fully correlated with the acylation of a single histidine. Active-site protection, by the ligand combination of xylitol plus Mg2+, completely blocked diethyl pyrocarbonate derivatization of this particular residue [Vangrysperre, Callens, Kersters-Hilderson & De Bruyne (1988) Biochem. J. 250, 153-160]. Differential peptide mapping between D-xylose isomerase, which has previously been treated with diethyl pyrocarbonate in the presence or absence of xylitol plus Mg2+, allowed specific isolation and sequencing of a peptide containing this active-site histidine. For this purpose we used two essentially new techniques: first, a highly reproducible peptide cleavage protocol for protease-resistant, carbethoxylated proteins with guanidinium hydrochloride as denaturing agent and subtilisin for proteolysis; and second, reverse-phase liquid chromatography with dual-wavelength detection at 214 and 238 nm, and calculation of absorbance ratios. It allowed us to locate the single active-site histidine at position 54 in the primary structure of Streptomyces violaceoruber D-xylose isomerase. The sequence around this residue is conserved in D-xylose isomerases from a diversity of micro-organisms, suggesting that this is a structurally and/or functionally essential part of the molecule.
Subject(s)
Aldose-Ketose Isomerases , Carbohydrate Epimerases/analysis , Histidine/isolation & purification , Streptomyces/enzymology , Amino Acid Sequence , Binding Sites , Chromatography, High Pressure Liquid , Histidine/metabolism , Hydrogen-Ion Concentration , Hydrolysis , Molecular Sequence Data , Peptide Mapping , Sequence Homology, Nucleic Acid , Spectrophotometry, UltravioletABSTRACT
A procedure for the determination of inositol by reversed-phase HPLC is described which is based on a precolumn benzoylation and detection at 230 nm. This procedure was used to assay the activity of L-myo-inositol 1-phosphate synthetase (EC 5.5.1.4) after treatment of the enzymatic product by a phosphatase.