Your search keyword '"Dipeptidases isolation & purification"' showing total 169 results

1. Prolidase is a critical enzyme for complete gliadin digestion in Tenebrio molitor larvae.

Author

Tereshchenkova VF, Goptar IA, Zhuzhikov DP, Belozersky MA, Dunaevsky YE, Oppert B, Filippova IY, and Elpidina EN

Subjects

Amino Acid Sequence, Animals, Dipeptidases antagonists & inhibitors, Dipeptidases isolation & purification, Gastrointestinal Tract enzymology, Insect Proteins antagonists & inhibitors, Insect Proteins isolation & purification, Larva enzymology, Membrane Transport Proteins metabolism, Substrate Specificity, Transcriptome, Dipeptidases metabolism, Gliadin metabolism, Insect Proteins metabolism, Tenebrio enzymology

Abstract

Prolidase is a proline-specific metallopeptidase that cleaves imidodipeptides with C-terminal Pro residue. Prolidase was purified and characterized from the Tenebrio molitor larval midgut. The enzyme was localized in the soluble fraction of posterior midgut tissues, corresponding to a predicted cytoplasmic localization of prolidase according to the structure of the mRNA transcript. Expression of genes encoding prolidase and the major digestive proline-specific peptidase (PSP)-dipeptidyl peptidase 4-were similar. The pH optimum of T. molitor prolidase was 7.5, and the enzyme was inhibited by Z-Pro, indicating that it belongs to type I prolidases. In mammals, prolidase is particularly important in the catabolism of a proline-rich protein-collagen. We propose that T. molitor larval prolidase is a critical enzyme for the final stages of digestion of dietary proline-rich gliadins, providing hydrolysis of imidodipeptides in the cytoplasm of midgut epithelial cells. We propose that the products of hydrolysis are absorbed from the luminal contents by peptide transporters, which we have annotated in the T. molitor larval gut transcriptome. The origin of prolidase substrates in the insect midgut is discussed in the context of overall success of grain feeding insects., (© 2017 Wiley Periodicals, Inc.)

Published

2017

2. N-acetylated α-linked acidic dipeptidase is identified as an antigen of Histoplasma capsulatum.

Author

Toyotome T, Watanabe A, Ochiai E, and Kamei K

Subjects

Acetylation, Antigens, Fungal blood, Antigens, Fungal isolation & purification, Dipeptidases blood, Dipeptidases isolation & purification, Enzyme-Linked Immunosorbent Assay, Histoplasmosis blood, Histoplasmosis microbiology, Humans, Antigens, Fungal immunology, Dipeptidases immunology, Histoplasma enzymology, Histoplasma immunology, Histoplasmosis immunology

Abstract

Histoplasmosis, one of the most important mycoses, needs to be diagnosed rapidly and accurately. The main method used to diagnose histoplasmosis is serological detection of antibodies to the Histoplasma capsulatum H and M antigens. Several other protein antigens have been reported in H. capsulatum; however, they have not been used for diagnosis. In this study, we explored novel antigens that were detected during H. capsulatum infection. We obtained a protein mixture from H. capsulatum yeast cells after vigorous mixing in a 0.1% Triton X-100 solution. From the resultant pool, we detected nine spots that reacted with sera from patients with histoplasmosis and identified eight seroactive proteins with mass spectrometry. The seroactive proteins were purified, and their antigenicities were tested with an enzyme-linked immunosorbent assay (ELISA). ELISA revealed that the titer of the patients' sera to N-acetylated α-linked acidic dipeptidase was significantly higher than those of healthy volunteers (P < 0.01). These data indicate that N-acetylated α-linked acidic dipeptidase of H. capsulatum is recognized as a major antigen during histoplasmosis., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2015

3. Hydrolysis of S-aryl-cysteinylglycine conjugates catalyzed by porcine kidney cortex membrane dipeptidase.

Author

Poon JC and Josephy PD

Subjects

Animals, Cysteine metabolism, Dipeptidases chemistry, Dipeptidases isolation & purification, Electrophoresis, Polyacrylamide Gel, Glutathione metabolism, Hydrolysis, Kinetics, Membranes enzymology, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Substrate Specificity, Biocatalysis, Dipeptidases metabolism, Dipeptides metabolism, Kidney Cortex enzymology, Sus scrofa metabolism

Abstract

Following conjugation with glutathione, xenobiotics are converted into cysteinylglycine conjugates, cysteine conjugates, and finally, mercapturic acids. The structural factors determining the activities of dipeptidases for the metabolism of toxicologically-relevant cysteinylglycine conjugates are not well understood. We purified porcine kidney cortex membrane dipeptidase (MDP) to homogeneity, via phosphatidylinositol-specific phospholipase C-mediated cleavage of the protein's membrane anchor and cilastatin affinity chromatography. The homodimeric structure of the MDP protein was confirmed by mass spectrometry. The cysteinylglycine conjugates of 1-(chloromethyl)naphthalene, 4-nitrobenzyl chloride, and 1-chloro-2,4-dinitrobenzene were synthesized and HPLC separation methods for their quantitation were developed. MDP catalyzed the hydrolysis of all three conjugates, but the rate of this activity was strongly dependent on the nature of the substituent on the cysteine sulfur atom.

Published

2012

4. Purification and identification of two carnosine-cleaving enzymes, carnosine dipeptidase I and Xaa-methyl-His dipeptidase, from Japanese eel (Anguilla japonica).

Author

Oku T, Ando S, Tsai HC, Yamashita Y, Ueno H, Shiozaki K, Nishi R, and Yamada S

Subjects

Amino Acid Sequence, Anguilla, Animals, Molecular Sequence Data, Muscle, Skeletal enzymology, Sequence Alignment, Substrate Specificity, Carnosine metabolism, Dipeptidases isolation & purification, Dipeptidases metabolism, Fish Proteins isolation & purification, Fish Proteins metabolism

Abstract

Three enzymes, carnosine dipeptidase I (EC 3.4.13.20, CNDP1), carnosine dipeptidase II (EC 3.4.13.18, CNDP2), and Xaa-methyl-His dipeptidase (or anserinase: EC 3.4.13.5, ANSN), are known to be capable of catalyzing the hydrolysis of carnosine (β-alanyl-l-histidine), in vertebrates. Here we report the purification and identification of two unidentified carnosine-cleaving enzymes from Japanese eel (Anguilla japonica). Two different dipeptidases were successfully purified to homogeneity from the skeletal muscle; one exhibited a broad substrate specificity, while the other a narrow specificity. N-terminal amino-acid sequencing, deglycosylation analysis, and genetic analysis clearly revealed that the former is a homodimer of glycosylated subunits, encoded by ANSN, and the latter is another homodimer of glycosylated subunits, encoded by CNDP1; that is, Xaa-methyl-His dipeptidase, and carnosine dipeptidase I respectively. This is the first report on the identification of carnosine dipeptidase I from a non-mammal. Database search revealed presence of a CNDP1 ortholog only from salmonid fishes, including Atlantic salmon and rainbow trout, but not from other ray-finned fish species, such as zebrafish, fugu, and medaka whose genomes have been completely sequenced. The mRNAs of CNDP1 and ANSN are strongly expressed in the liver of Japanese eel, compared with other tissues, while that of CNDP2 is widely distributed in all tissues tested., (Copyright © 2012 Elsevier Masson SAS. All rights reserved.)

Published

2012

5. Characterization of an Aspergillus oryzae cysteinyl dipeptidase expressed in Escherichia coli.

Author

Hattori R, Matsushita-Morita M, Marui J, Tada S, Suzuki S, Furukawa I, Yamagata Y, Amano H, Ishida H, Takeuchi M, and Kusumoto K

Subjects

Cloning, Molecular, Dipeptidases biosynthesis, Dipeptidases isolation & purification, Gene Expression, Humans, Oligopeptides metabolism, Substrate Specificity, Aspergillus oryzae enzymology, Cysteine metabolism, Dipeptidases genetics, Dipeptidases metabolism, Escherichia coli genetics

Abstract

Cysteinyl dipeptidase from Aspergillus oryzae (CdpA) was produced in Escherichia coli and purified. The enzyme showed activity specific toward cysteine-containing dipeptides, but its substrate specificity was distinct from those of other cysteinyl dipeptidases of the M20 family. It was optimally active at pH 7-8 and stable at pH 6-9 and at up to 40 °C.

Published

2011

6. Hydrophilic residues surrounding the S1 and S2 pockets contribute to dimerisation and catalysis in human dipeptidyl peptidase 8 (DP8).

Author

Pitman MR, Menz RI, and Abbott CA

Subjects

Databases, Protein, Dipeptidases genetics, Dipeptidases isolation & purification, Dipeptidyl Peptidase 4 chemistry, Dipeptidyl-Peptidases and Tripeptidyl-Peptidases chemistry, Endopeptidases, Gelatinases chemistry, Humans, Hydrogen-Ion Concentration, Hydrophobic and Hydrophilic Interactions, Kinetics, Membrane Proteins chemistry, Mutagenesis, Site-Directed, Mutant Proteins chemistry, Mutant Proteins isolation & purification, Mutant Proteins metabolism, Protein Stability, Protein Structure, Quaternary, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Sequence Alignment, Sequence Homology, Amino Acid, Serine Endopeptidases chemistry, Substrate Specificity, Biocatalysis, Catalytic Domain, Dimerization, Dipeptidases chemistry, Dipeptidases metabolism, Protein Interaction Domains and Motifs

Abstract

Dipeptidyl peptidase (DP) 8 belongs to the dipeptidyl peptidase IV gene family. DP8 has been implicated in immune function and asthma, although its biological function is yet unknown. Structures of the homologs, fibroblast activation protein (FAP) and DPIV, are known but the DP8 structure is yet to be resolved. To help characterise the DP8 substrate pocket, mutants of residues lining the pocket were produced at DP8(D772), DP8(Y315), DP8(H434) and DP8(D435) and assessed by substrate kinetics and size-exclusion chromatography. Mutations of DP8(D772A/E/S/V) affected catalysis but did not confer endopeptidase activity. Mutations of DP8(H434F), DP8(D435F) and DP8(Y315F) reduced catalytic activity. Furthermore, mutations to DP8(D772A/E/S/V), DP8(H434F), DP8(D435F) and DP8(Y315F) affected dimer stabilisation. Homology modelling of DP8 using DPIV and FAP crystal structures suggested that DP8(D772), DP8(H434) and DP8(D435) were located at the edge of the S2 catalytic pocket, contributing to the junction between the alpha-beta hydrolase and beta-propeller domains. This study provides insights into how the DP8 substrate pocket and dimer interface differ from DPIV and FAP which could be utilised for designing more selective DP8 inhibitors.

Published

2010

7. Improving the catalytic activity of hyperthermophilic Pyrococcus prolidases for detoxification of organophosphorus nerve agents over a broad range of temperatures.

Author

Theriot CM, Du X, Tove SR, and Grunden AM

Subjects

Amino Acid Substitution genetics, Archaeal Proteins chemistry, Archaeal Proteins genetics, Archaeal Proteins isolation & purification, Culture Media chemistry, Dipeptidases chemistry, Dipeptidases genetics, Dipeptidases isolation & purification, Enzyme Stability, Escherichia coli genetics, Models, Molecular, Mutagenesis, Plasmids, Polymerase Chain Reaction methods, Protein Stability, Protein Structure, Tertiary, Pyrococcus furiosus genetics, Sequence Deletion, Temperature, Archaeal Proteins metabolism, Chemical Warfare Agents metabolism, Dipeptidases metabolism, Organophosphorus Compounds metabolism, Pesticides metabolism, Pyrococcus furiosus enzymology

Abstract

Prolidase isolated from the hyperthermophilic archaeon Pyrococcus furiosus has potential for application for decontamination of organophosphorus compounds in certain pesticides and chemical warfare agents under harsh conditions. However, current applications that use an enzyme-based cocktail are limited by poor long-term enzyme stability and low reactivity over a broad range of temperatures. To obtain a better enzyme for OP nerve agent decontamination and to investigate structural factors that influence protein thermostability and thermoactivity, randomly mutated P. furiosus prolidases were prepared by using XL1-red-based mutagenesis and error-prone PCR. An Escherichia coli strain JD1 (lambdaDE3) (auxotrophic for proline [DeltaproA] and having deletions in pepQ and pepP dipeptidases with specificity for proline-containing dipeptides) was constructed for screening mutant P. furiosus prolidase expression plasmids. JD1 (lambdaDE3) cells were transformed with mutated prolidase expression plasmids and plated on minimal media supplemented with 50 muM Leu-Pro as the only source of proline. By using this positive selection, Pyrococcus prolidase mutants with improved activity over a broader range of temperatures were isolated. The activities of the mutants over a broad temperature range were measured for both Xaa-Pro dipeptides and OP nerve agents, and the thermoactivity and thermostability of the mutants were determined.

Published

2010

8. Screening, purification, and identification of the enzyme producing N-(L-alpha-L-aspartyl)-L-phenylalanine methyl ester from l-isoasparagine and L-phenylalanine methyl ester.

Author

Kira I, Asano Y, and Yokozeki K

Subjects

Biotechnology methods, Catalysis, Citrobacter enzymology, Dipeptidases analysis, Dipeptidases chemistry, Electrophoresis, Polyacrylamide Gel, Enterobacteriaceae enzymology, Escherichia coli enzymology, Hydrogen-Ion Concentration, Models, Chemical, Phenylalanine chemistry, Recombinant Proteins chemistry, Salmonella typhimurium enzymology, Shigella flexneri enzymology, Asparagine chemistry, Dipeptidases isolation & purification, Phenylalanine analogs & derivatives

Abstract

Screening was carried out for microorganisms able to produce N-(l-alpha-l-aspartyl)-l-phenylalanine methyl ester [APM] from l-isoasparagine and l-phenylalanine methyl ester hydrochloride. Of the 422 strains examined, 44 strains belonging to the family Enterobacteriaceae were found to produce APM. The enzyme catalyzing APM production was purified and identified as dipeptidase E.

Published

2009

9. Characterization of prolidase I and II purified from normal human erythrocytes: comparison with prolidase in erythrocytes from a patient with prolidase deficiency.

Author

Uramatsu S, Liu G, Yang Q, Uramatsu M, Chi H, Lu J, Yamashita K, and Kodama H

Subjects

Dipeptidases blood, Dipeptidases isolation & purification, Dipeptides metabolism, Humans, Isoenzymes, Kinetics, Stereoisomerism, Substrate Specificity, Amino Acids, Sulfur metabolism, Dipeptidases deficiency, Dipeptidases metabolism, Erythrocytes enzymology

Abstract

The effect of various sulfur-containing amino acids on the activities of prolidase isoenzymes I and II isolated from erythrocytes of healthy individuals, and erythrocyte lysates from a patient with prolidase deficiency was investigated. The activity of prolidase I against glycylproline was strongly enhanced by D: -methionine. L: -Methionine and D: ,L: -methionine slightly enhanced the activity at low concentration, but N-acetyl-L: -methionine had no effect. D: -Ethionine, L: -ethionine, and D: ,L: -ethionine also enhanced the activity of prolidase I. D: ,L: -Homocysteine enhanced the activity at low concentration, but inhibited the activity at 50 mM: . The activity of prolidase II against methionylproline was enhanced by D: -methionine, D: ,L: -methionine, and L: -methionine, but N-acetyl-L: -methionine had no effect. D: -Ethionine and D: ,L: -ethionine strongly enhanced the activity of prolidase II compared with L: -ethionine; D: ,L: -homocysteine weakly enhanced the activity. D: ,L: -Homocysteine-thiolactone inhibited the activities of prolidase I and II in a concentration-dependent manner. The effect of various sulfur-containing amino acids on prolidase activity against methionylproline in erythrocyte lysates from a patient with prolidase deficiency was almost the same as that on prolidase II. The kinetics of the activities of prolidase I, II, and patient prolidase were also studied. Their K (m) values were changed by adding sulfur-containing amino acids, but V (max) values were unchanged.

Published

2009

10. Functional identification of incorrectly annotated prolidases from the amidohydrolase superfamily of enzymes.

Author

Xiang DF, Patskovsky Y, Xu C, Meyer AJ, Sauder JM, Burley SK, Almo SC, and Raushel FM

Subjects

Amidohydrolases isolation & purification, Amidohydrolases metabolism, Amino Acid Sequence, Arginine chemistry, Bacterial Proteins isolation & purification, Bacterial Proteins metabolism, Carboxylic Acids chemistry, Catalysis, Catalytic Domain physiology, Combinatorial Chemistry Techniques, Computational Biology methods, Crystallography, X-Ray, Dipeptidases isolation & purification, Dipeptidases metabolism, Dipeptides isolation & purification, Dipeptides metabolism, Dipeptides physiology, Hydrolysis, Lysine chemistry, Molecular Sequence Data, Static Electricity, Substrate Specificity physiology, Amidohydrolases physiology, Bacterial Proteins physiology, Caulobacter crescentus enzymology, Dipeptidases physiology, Multigene Family physiology, Peptide Library

Abstract

The substrate profiles for two proteins from Caulobacter crescentus CB15 (Cc2672 and Cc3125) and one protein (Sgx9359b) derived from a DNA sequence ( gi|44368820 ) isolated from the Sargasso Sea were determined using combinatorial libraries of dipeptides and N-acyl derivatives of amino acids. These proteins are members of the amidohydrolase superfamily and are currently misannotated in NCBI as catalyzing the hydrolysis of l-Xaa-l-Pro dipeptides. Cc2672 was shown to catalyze the hydrolysis of l-Xaa-l-Arg/Lys dipeptides and the N-acetyl and N-formyl derivatives of lysine and arginine. This enzyme will also hydrolyze longer peptides that terminate in either lysine or arginine. The N-methyl phosphonate derivative of l-lysine was a potent competitive inhibitor of Cc2672 with a K(i) value of 120 nM. Cc3125 was shown to catalyze the hydrolysis of l-Xaa-l-Arg/Lys dipeptides but will not hydrolyze tripeptides or the N-formyl and N-acetyl derivatives of lysine or arginine. The substrate profile for Sgx9359b is similar to that of Cc2672 except that compounds with a C-terminal lysine are not recognized as substrates. The X-ray structure of Sgx9359b was determined to a resolution of 2.3 A. The protein folds as a (beta/alpha)(8)-barrel and self-associates to form a homooctamer. The active site is composed of a binuclear metal center similar to that found in phosphotriesterase and dihydroorotase. In one crystal form, arginine was bound adventitiously to the eight active sites within the octamer. The orientation of the arginine in the active site identified the structural determinants for recognition of the alpha-carboxylate and the positively charged side chains of arginine-containing substrates. This information was used to identify 18 other bacterial sequences that possess identical or similar substrate profiles.

Published

2009

11. Purification, crystallization and preliminary X-ray analysis of an aminoacylhistidine dipeptidase (PepD) from Vibrio alginolyticus.

Author

Chang CY, Hsieh YC, Wang TY, Chen CJ, and Wu TK

Subjects

Crystallization, Crystallography, X-Ray, Electrophoresis, Polyacrylamide Gel, Dipeptidases chemistry, Dipeptidases isolation & purification, Vibrio alginolyticus enzymology

Abstract

The aminoacylhistidine dipeptidase (PepD) protein encoded by Vibrio alginolyticus pepD was successfully overexpressed and characterized and the putative active-site residues responsible for metal binding and catalysis were identified. The purified enzyme contained two zinc ions per monomer. The recombinant dipeptidase enzyme, which was identified as a homodimer in solution, exhibited broad substrate specificity for Xaa-His dipeptides, with highest activity towards the His-His dipeptide. The purified protein was crystallized using the hanging-drop vapour-diffusion method. Preliminary crystallographic analysis showed that the crystal belonged to space group P6(1) or P6(5), with unit-cell parameters a = b = 80.42, c = 303.11 A. The crystal contained two molecules per asymmetric unit and the predicted solvent content was 53.4%.

Published

2009

12. Stromal cell-derived factors 1alpha and 1beta, inflammatory protein-10 and interferon-inducible T cell chemo-attractant are novel substrates of dipeptidyl peptidase 8.

Author

Ajami K, Pitman MR, Wilson CH, Park J, Menz RI, Starr AE, Cox JH, Abbott CA, Overall CM, and Gorrell MD

Subjects

Chemokine CXCL10 chemistry, Chemokine CXCL11 chemistry, Chemokine CXCL12 chemistry, Dipeptidases isolation & purification, Dipeptidyl Peptidase 4 isolation & purification, Dipeptidyl Peptidase 4 metabolism, Half-Life, Humans, Kinetics, Molecular Weight, Protein Processing, Post-Translational, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Solubility, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Substrate Specificity, Chemokine CXCL10 metabolism, Chemokine CXCL11 metabolism, Chemokine CXCL12 metabolism, Dipeptidases metabolism

Abstract

N-terminal truncation of chemokines by proteases including dipeptidyl peptidase (DP) IV significantly alters their biological activity; generally ablating cognate G-protein coupled receptor engagement and often generating potent receptor antagonists. DP8 is a recently recognised member of the prolyl oligopeptidase gene family that includes DPIV. Since DPIV is known to process chemokines we surveyed 27 chemokines for cleavage by DP8. We report DP8 cleavage of the N-terminal two residues of IP10 (CXCL10), ITAC (CXCL11) and SDF-1 (CXCL12). This has implications for DP8 substrate specificity. Chemokine cleavage and inactivation may occur in vivo upon cell lysis and release of DP8 or in the inactivation of internalized chemokine/receptor complexes.

Published

2008

13. Purification and characterization of dipeptidase hydrolyzing L-cysteinylglycine from radish cotyledon.

Author

Kumada HO, Koizumi Y, and Sekiya J

Subjects

Dipeptidases isolation & purification, Hydrolysis, Plant Proteins isolation & purification, Stereoisomerism, Cotyledon enzymology, Dipeptidases metabolism, Dipeptides metabolism, Plant Proteins metabolism, Raphanus enzymology

Abstract

Dipeptidase activity was detected in the soluble fraction of radish (Raphanus sativus L.) cotyledon, and the purified enzyme had a specific activity of 7.32 nkat/mg protein for hydrolyzing L-cysteinylglycine. The dipeptidase was found to be a hexameric metalloenzyme, composed of homological 55 kDa-subunits. This is the first glutathione catabolism-related dipeptidase isolated from higher plants.

Published

2007

14. Characterization of a Bifidobacterium longum BORI dipeptidase belonging to the U34 family.

Author

Seo JM, Ji GE, Cho SH, Park MS, and Lee HJ

Subjects

Amino Acid Sequence, Bacterial Proteins classification, Bacterial Proteins genetics, Bacterial Proteins isolation & purification, Bacterial Proteins metabolism, Base Sequence, Cloning, Molecular, Dipeptides metabolism, Escherichia coli enzymology, Escherichia coli genetics, Genetic Vectors, Molecular Sequence Data, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Substrate Specificity, Bifidobacterium enzymology, Dipeptidases classification, Dipeptidases genetics, Dipeptidases isolation & purification, Dipeptidases metabolism

Abstract

A dipeptidase was purified from a cell extract of Bifidobacterium longum BORI by ammonium sulfate precipitation and chromatography on DEAE-cellulose and Q-Sepharose columns. The purified dipeptidase had a molecular mass of about 49 kDa and was optimally active at pH 8.0 and 50 degrees C. The enzyme was a strict dipeptidase, being capable of hydrolyzing a range of dipeptides but not tri- and tetrapeptides, p-nitroanilide derivatives of amino acids, or N- or C-terminus-blocked dipeptides. A search of the amino acid sequence of an internal tryptic fragment against protein sequences deduced from the total genome sequence of B. longum NCC2705 revealed that it was identical to an internal sequence of the dipeptidase gene (pepD), which comprised 1,602 nucleotides encoding 533 amino acids with a molecular mass of 60 kDa, and thereby differed considerably from the 49-kDa mass of the purified dipeptidase. To understand this discrepancy, pepD was cloned into an Escherichia coli expression vector (pBAD-TOPO derivative) to generate the recombinant plasmids pBAD-pepD and pBAD-pepD-His (note that His in the plasmid designation stands for a polyhistidine coding region). Both plasmids were successfully expressed in E. coli, and the recombinant protein PepD-His was purified using nickel-chelating affinity chromatography and reconfirmed by internal amino acid sequencing. The PepD sequence was highly homologous to those of the U34 family of peptidases, suggesting that the B. longum BORI dipeptidase is a type of cysteine-type N-terminal nucleophile hydrolase and has a beta-hairpin motif similar to that of penicillin V acylase, which is activated by autoproteolytic processing.

Published

2007

15. Prolidase isoenzymes in the rat: their organ distribution, developmental change and specific inhibitors.

Author

Liu G, Nakayama K, Awata S, Tang S, Kitaoka N, Manabe M, and Kodama H

Subjects

Animals, Captopril metabolism, Dipeptidases chemistry, Dipeptidases isolation & purification, Humans, Isoenzymes chemistry, Isoenzymes isolation & purification, Kidney enzymology, Male, Nickel metabolism, Proline chemistry, Proline metabolism, Rats, Rats, Wistar, Substrate Specificity, Tissue Distribution, Dipeptidases antagonists & inhibitors, Dipeptidases metabolism, Enzyme Inhibitors metabolism, Isoenzymes antagonists & inhibitors, Isoenzymes metabolism

Abstract

Lack of prolidase I (PD I) leads to prolidase deficiency, a disease characterized by intractable skin lesions, recurrent respiratory infections, and mental retardation. The present study was undertaken to characterize and determine the physiologic roles of different prolidase isoenzymes. Two isoforms of prolidase were isolated from rat kidney. PD I showed higher activity against seryl-proline and alanyl-proline, whereas PD II was active especially against methionyl-proline. PD I was highly concentrated in the small intestine and kidney, whereas PD II was shown not to vary in the organs examined. Expression of PD I and PD II in the small intestine were maximal within 1 wk of birth, and then rapidly declined. The changes of prolidase in the kidney and heart were found to differ slightly. N-benzyloxycarbonyl-l-proline and captopril inhibited PD I dose-dependently, but showed no inhibition of PD II at low concentrations. NiCl2 inhibited PD II much more effectively than PD I. Our findings suggest that PD I functions by way of an intestinal peptide carrier, which may also be regulated by the uptake of various iminodipeptides. Similarly, age-related alterations of prolidase isoenzymes suggest that intestinal PD II also participates in absorption of proline and other amino acids early in life.

Published

2007

16. Purification and characterization of a novel imidazole dipeptide synthase from the muscle of the Japanese eel Anguilla japonica.

Author

Tsubone S, Yoshikawa N, Okada S, and Abe H

Subjects

Amino Acid Sequence, Animals, Anserine metabolism, Carnosine metabolism, Dipeptides metabolism, Edetic Acid pharmacology, Enzyme Activation drug effects, Haptoglobins chemistry, Hydrogen-Ion Concentration, Hydrolysis, Imidazoles metabolism, Molecular Sequence Data, Molecular Weight, Peptide Synthases drug effects, Sequence Homology, Amino Acid, Temperature, Zebrafish Proteins chemistry, Zinc metabolism, Anguilla, Dipeptidases isolation & purification, Dipeptidases metabolism, Muscles enzymology, Peptide Synthases isolation & purification, Peptide Synthases metabolism

Abstract

We have purified a novel enzyme from eel white muscle which catalyzes the syntheses of imidazole dipeptides, such as carnosine (beta-alanyl-L-histidine), anserine (beta-alanyl-pi-methyl-L-histidine), and balenine (ophidine; beta-alanyl-tau-methyl-L-histidine), directly from their precursors. The enzyme was purified 1130-fold from eel muscle by a series of column chromatographies. Although eel muscle contains a large amount of carnosine and only trace amounts of anserine and balenine, the anserine synthesizing activity was by far the highest. From gel permeation chromatography, the molecular mass of the enzyme was calculated to be 275kDa. SDS-PAGE of the purified enzyme represented a band around 43kDa, suggesting that the native enzyme is a hexamer or heptamer. The optimal pH and temperature were around 9.5 and 60 degrees C, respectively. K(m) values for beta-alanine and pi-methyl-L-histidine were 44 and 89mM, respectively. The enzyme was greatly activated by Zn(2+) and inhibited by EDTA. The N-terminal amino acid sequence of 25 residues of the purified enzyme showed 52% amino acid identity to 38-62 residues of zebrafish haptoglobin precursor. The purified enzyme also exhibited hydrolytic activity against these imidazole dipeptides.

Published

2007

17. Investigation of the dimer interface and substrate specificity of prolyl dipeptidase DPP8.

Author

Lee HJ, Chen YS, Chou CY, Chien CH, Lin CH, Chang GG, and Chen X

Subjects

Amino Acid Sequence, Base Sequence, DNA Primers, Dimerization, Dipeptidases chemistry, Dipeptidases genetics, Dipeptidases isolation & purification, Electrophoresis, Polyacrylamide Gel, Humans, Molecular Sequence Data, Mutagenesis, Site-Directed, Sequence Homology, Amino Acid, Substrate Specificity, Dipeptidases metabolism

Abstract

DPP8 belongs to the family of prolyl dipeptidases, which are capable of cleaving the peptide bond after a penultimate proline residue. Unlike DPP-IV, a drug target for type II diabetes, no information is available on the crystal structure of DPP8, the regulation of its enzymatic activity, or its substrate specificity. In this study, using analytical ultracentrifugation and native gel electrophoresis, we show that the DPP8 protein is predominantly dimeric when purified or in the cell extracts. Four conserved residues in the C-terminal loop of DPP8 (Phe(822), Val(833), Tyr(844), and His(859)), corresponding to those located at the dimer interface of DPP-IV, were individually mutated to Ala. Surprisingly, unlike DPP-IV, these single-site mutations abolished the enzymatic activity of DPP8 without disrupting its quaternary structure, indicating that dimerization itself is not sufficient for the optimal enzymatic activity of DPP8. Moreover, these mutations not only decreased k(cat), as did the corresponding DPP-IV mutations, but also dramatically increased K(m). We further show that the K(m) effect is independent of the substrate assayed. Finally, we identified the distinctive and strict substrate selectivity of DPP8 for hydrophobic or basic residues at the P2 site, which is in sharp contrast to the much less discriminative substrate specificity of DPP-IV. Our study has identified the residues absolutely required for the optimal activity of DPP8 and its unique substrate specificity. This study extends the functional importance of the C-terminal loop to the whole family of prolyl dipeptidases.

Published

2006

18. Human recombinant prolidase from eukaryotic and prokaryotic sources. Expression, purification, characterization and long-term stability studies.

Author

Lupi A, Della Torre S, Campari E, Tenni R, Cetta G, Rossi A, and Forlino A

Subjects

Animals, CHO Cells, Cricetinae, Dipeptidases genetics, Enzyme Stability, Escherichia coli genetics, Escherichia coli metabolism, Fibroblasts metabolism, Histidine chemistry, Histidine metabolism, Humans, Hydrogen-Ion Concentration, Recombinant Proteins genetics, Substrate Specificity, Temperature, Transfection, Dipeptidases isolation & purification, Dipeptidases metabolism, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism

Abstract

Prolidase is a Mn(2+)-dependent dipeptidase that cleaves imidodipeptides containing C-terminal proline or hydroxyproline. In humans, a lack of prolidase activity causes prolidase deficiency, a rare autosomal recessive disease, characterized by a wide range of clinical outcomes, including severe skin lesions, mental retardation, and infections of the respiratory tract. In this study, recombinant prolidase was produced as a fusion protein with an N-terminal histidine tag in eukaryotic and prokaryotic hosts and purified in a single step using immobilized metal affinity chromatography. The enzyme was characterized in terms of activity against different substrates, in the presence of various bivalent ions, in the presence of the strong inhibitor Cbz-Pro, and at different temperatures and pHs. The recombinant enzyme with and without a tag showed properties mainly indistinguishable from those of the native prolidase from fibroblast lysate. The protein yield was higher from the prokaryotic source, and a detailed long-term stability study of this enzyme at 37 degrees C was therefore undertaken. For this analysis, an 'on-column' digestion of the N-terminal His tag by Factor Xa was performed. A positive effect of Mn(2+) and GSH in the incubation mixture and high stability of the untagged enzyme are reported. Poly(ethylene glycol) and glycerol had a stabilizing effect, the latter being the more effective. In addition, no significant degradation was detected after up to 6 days of incubation with cellular lysate. Generation of the prolidase in Escherichia coli, because of its high yield, stability, and similarity to native prolidase, appears to be the best approach for future structural studies and enzyme replacement therapy.

Published

2006

19. Identification of carboxypeptidase of glutamate like-B as a candidate suppressor in cell growth and metastasis in human hepatocellular carcinoma.

Author

Zhang P, Chan DW, Zhu Y, Li JJ, Ng IO, Wan D, and Gu J

Subjects

Amino Acid Sequence, Animals, Carcinoma, Hepatocellular pathology, Carcinoma, Hepatocellular therapy, Cell Survival, Cells, Cultured, Cytoplasm metabolism, Dipeptidases genetics, Dipeptidases isolation & purification, Female, Gene Expression Profiling, Gene Expression Regulation, Neoplastic, Humans, Liver metabolism, Liver Neoplasms pathology, Liver Neoplasms therapy, Mice, Mice, Inbred BALB C, Mice, Nude, Molecular Sequence Data, Neoplasm Invasiveness, Sequence Homology, Amino Acid, Tissue Distribution, Transfection methods, Xenograft Model Antitumor Assays, Carcinoma, Hepatocellular metabolism, Dipeptidases physiology, Growth Inhibitors isolation & purification, Liver Neoplasms metabolism, Neoplasm Metastasis prevention & control

Abstract

Purpose: We have previously done large-scale cDNA transfection screening on human hepatocellular carcinoma (HCC) cells and have identified 3,806 cDNA genes that possess the ability of either stimulating or inhibiting cell growth. In this study, we characterized one of these growth suppressor genes, carboxypeptidase of glutamate like-B (CPGL-B), in HCC., Experimental Design: Semiquantitative reverse-transcription PCR was used to examine the expression levels of CPGL-B. The cellular localization and functions of CPGL-B were investigated by enforced expression of CPGL-B in HCC cells., Results: From our previous cDNA transfection screening, we identified a gene named CPGL and its isoform, CPGL-B. With computational analysis, CPGL was located at chromosome 18q22.3 and was a homologue of peptidase family M20. CPGL was expressed in all adult and fetal tissues, whereas its isoform, CPGL-B, lacking exons 3 and 4, was expressed in all fetal tissues but only in liver and placenta of adult tissues. In HCC, CPGL-B was frequently underexpressed (35 of 90, 38.9%) in tumorous tissues compared with the corresponding nontumorous livers. Intriguingly, the underexpression was significantly associated with the presence of venous invasion (P=0.018) and tumor microsatellite formation (P=0.004). Stable transfection of CPGL-B in SMMC7721 HCC cells showed significant inhibition in cell viability, colony formation, cell invasion, and tumor formation in nude mice. CPGL-B also down-regulated CXCR3, matrix metalloproteinase 11, and CD44s, which are involved in cell growth and cell migration., Conclusions: These findings suggest that the frequent underexpression of CPGL-B may be associated with cell growth and metastasis of HCC.

Published

2006

20. Characterization and kinetic analysis of enzyme-substrate recognition by three recombinant lactococcal PepVs.

Author

Mori S, Miyamoto M, Kaneko S, Nirasawa S, Komba S, and Kasumi T

Subjects

Amino Acid Sequence, Bacterial Proteins chemistry, Bacterial Proteins isolation & purification, Binding Sites, Dipeptidases chemistry, Dipeptidases isolation & purification, Electrophoresis, Capillary, Kinetics, Models, Molecular, Molecular Sequence Data, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Substrate Specificity, Bacterial Proteins metabolism, Dipeptidases metabolism, Dipeptides metabolism, Lactococcus lactis enzymology

Abstract

The dipeptidases (PepVs) from three typical lactococcal strains, Lactococcus lactis subsp. lactis (L9), L. lactis subsp. cremoris (L6) and L. lactis subsp. hordniae (hT) were cloned and characterized. The metal-binding, catalytic, and substrate-binding sites are highly conserved among of them. A computer-generated three-dimensional model suggested that the amino acid differences between these PepVs were mostly located away from the active center. L9 PepV does not hydrolyze dipeptides bearing Pro or D-amino acid at the C-terminal amino acid. Unlike PepV from Lactobacillus delbrueckii, L9 PepV does not cleave beta-Asp-His, and has little ability to cleave dipeptides containing a beta-alanine. In addition, L9 PepV has a much higher kcat for dipeptides with an N-terminal Ala but a significantly higher Km when the N-terminal amino acid is Gly. The substrate recognition profile of PepV is further discussed on the basis of the kinetic analysis and the structural model.

Published

2006

21. Crystallization and preliminary crystallographic study of carnosinase CN2 from mice.

Author

Yamashita T, Unno H, Ujita S, Otani H, Okumura N, Hashida-Okumura A, Nagai K, and Kusunoki M

Subjects

Animals, Crystallization, Crystallography, X-Ray, Dipeptidases genetics, Dipeptidases isolation & purification, Mice, Dipeptidases chemistry

Abstract

Mammalian tissues contain several histidine-containing dipeptides, of which L-carnosine is the best characterized and is found in various tissues including the brain and skeletal muscles. However, the mechanism for its biosynthesis and degradation have not yet been fully elucidated. Crystallographic study of carnosinase CN2 from mouse has been undertaken in order to understand its enzymatic mechanism from a structural viewpoint. CN2 was crystallized by the hanging-drop vapour-diffusion technique using PEG 3350 as a precipitant. Crystals were obtained in complex with either Mn(2+) or Zn(2+). Both crystals of CN2 belong to the monoclinic space group P2(1) and have almost identical unit-cell parameters (a = 54.41, b = 199.77, c = 55.49 A, beta = 118.52 degrees for the Zn(2+) complex crystals). Diffraction data were collected to 1.7 and 2.3 A for Zn(2+) and Mn(2+) complex crystals, respectively, using synchrotron radiation. Structure determination is ongoing using the multiple-wavelength anomalous diffraction (MAD) method.

Published

2006

22. Dipeptidyl peptidases 8 and 9: specificity and molecular characterization compared with dipeptidyl peptidase IV.

Author

Bjelke JR, Christensen J, Nielsen PF, Branner S, Kanstrup AB, Wagtmann N, and Rasmussen HB

Subjects

Amino Acid Sequence, Baculoviridae genetics, Baculoviridae metabolism, Chromatography, Gel, Dipeptidases genetics, Dipeptidases isolation & purification, Dipeptidases metabolism, Dipeptidyl Peptidase 4 metabolism, Dipeptidyl-Peptidases and Tripeptidyl-Peptidases genetics, Dipeptidyl-Peptidases and Tripeptidyl-Peptidases isolation & purification, Dipeptidyl-Peptidases and Tripeptidyl-Peptidases metabolism, Enzyme Activation, Enzyme Inhibitors metabolism, Enzyme Inhibitors pharmacology, Humans, Kinetics, Molecular Sequence Data, Peptide Fragments chemistry, Peptide Fragments metabolism, Protein Structure, Quaternary, Pyrroles metabolism, Pyrroles pharmacology, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Sequence Alignment, Substrate Specificity, Valine metabolism, Valine pharmacology, Dipeptidases chemistry, Dipeptidyl Peptidase 4 chemistry, Dipeptidyl-Peptidases and Tripeptidyl-Peptidases chemistry

Abstract

Dipeptidyl peptidases 8 and 9 have been identified as gene members of the S9b family of dipeptidyl peptidases. In the present paper, we report the characterization of recombinant dipeptidyl peptidases 8 and 9 using the baculovirus expression system. We have found that only the full-length variants of the two proteins can be expressed as active peptidases, which are 882 and 892 amino acids in length for dipeptidyl peptidase 8 and 9 respectively. We show further that the purified proteins are active dimers and that they show similar Michaelis-Menten kinetics and substrate specificity. Both cleave the peptide hormones glucagon-like peptide-1, glucagon-like peptide-2, neuropeptide Y and peptide YY with marked kinetic differences compared with dipeptidyl peptidase IV. Inhibition of dipeptidyl peptidases IV, 8 and 9 using the well-known dipeptidyl peptidase IV inhibitor valine pyrrolidide resulted in similar K(i) values, indicating that this inhibitor is non-selective for any of the three dipeptidyl peptidases.

Published

2006

23. Dual activities of human prolidase.

Author

Wang SH, Zhi QW, and Sun MJ

Subjects

Adult, Aryldialkylphosphatase metabolism, Cloning, Molecular, DNA, Complementary analysis, DNA, Complementary genetics, Dipeptidases genetics, Dipeptidases isolation & purification, Gene Expression, Genetic Vectors, Humans, Liver enzymology, Pichia genetics, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Soman metabolism, Dipeptidases metabolism, Pichia metabolism

Abstract

The cDNA encoding human liver prolidase derived from a healthy adult's liver was cloned into the expression vector pPIC9K of Pichia pastoris to construct the recombination expression vector pPIC9K-P. The pPIC9K-P was digested by restriction enzyme Pme I, and then transformed into P. pastoris GS115 by electroporation. Transformants (the insertion recombinant) were induced by methanol to express the recombination protein. The optimal induction conditions (medium pH, methanol concentration and induction time) of the insertion transformant with the highest enzymatic activity were estimated by orthogonal experimental design L9(3(4)). The SDS-PAGE of the recombinant human prolidase (rh-prolidase) in induction medium showed a molecular weight of 73 kDa. The activities of the rh-prolidase and organophosphoric acid anhydrolases (OPAA) were assayed by colorimetric methods. The recombinant enzyme catalyzed the hydrolysis of organophosphorous compound soman as well as the hydrolysis of dipeptide Gly-Pro. Under the optimal induction conditions, the maximal activities of prolidase and OPAA came to 44.1 and 54.8 nmol/min/mg protein respectively in the medium supernatant. The rh-prolidase purified from the supernatant by ion exchange gradient chromatography (DEAE-Sepharose Fast Flow) and gel filtration chromatography (Sephacryl S-200 High Resolution) showed a single band by SDS-PAGE analysis. The purified rh-prolidase could decompose soman via hydrolytic reaction in vitro.

Published

2006

24. Purification and sequence identification of anserinase.

Author

Yamada S, Tanaka Y, and Ando S

Subjects

Amino Acid Sequence, Animals, Base Sequence, Brain enzymology, Cloning, Molecular, Databases, Protein, Dipeptidases classification, Dipeptidases metabolism, Molecular Sequence Data, Open Reading Frames, Phylogeny, Protein Sorting Signals, Sequence Alignment, Sequence Homology, Tilapia, Tissue Distribution, Dipeptidases genetics, Dipeptidases isolation & purification

Abstract

Anserinase (Xaa-methyl-His dipeptidase, EC 3.4.13.5) is a dipeptidase that mainly catalyzes the hydrolysis of Nalpha-acetylhistidine in the brain, retina and vitreous body of all poikilothermic vertebrates. The gene encoding anserinase has not been previously identified. We report the molecular identification of anserinase, purified from brain of Nile tilapia Oreochromis niloticus. The determination of the N-terminal sequence of the purified anserinase allowed the design of primers permitting the corresponding cDNA to be cloned by PCR. The anserinase cDNA has an ORF of 1485 nucleotides and encodes a signal peptide of 18 amino acids and a mature protein of 476 amino acids with a predicted molecular mass of 53.3 kDa. Sequence analysis showed that anserinase is a member of the M20A metallopeptidase subfamily in MEROPS peptidase database, to which 'serum' carnosinase (EC 3.4.13.20) and cytosolic nonspecific dipeptidase (EC 3.4.13.18, CNDP) belong. A cDNA encoding CNDP-like protein was also isolated from tilapia brain. Whereas anserinase mRNA was detected only in brain, retina, kidney and skeletal muscle, CNDP-like protein mRNA was detected in all tissues examined.

Published

2005

25. Characterization of prolidase activity in erythrocytes from a patient with prolidase deficiency: comparison with prolidase I and II purified from normal human erythrocytes.

Author

Liu G, Nakayama K, Sagara Y, Awata S, Yamashita K, Manabe M, and Kodama H

Subjects

Amino Acids pharmacology, Chlorides pharmacology, Dipeptidases isolation & purification, Dipeptides metabolism, Electrophoresis, Polyacrylamide Gel, Humans, Kinetics, Manganese Compounds pharmacology, Stereoisomerism, Valine pharmacology, Dipeptidases blood, Dipeptidases deficiency, Erythrocytes enzymology

Abstract

Objectives: The purpose of this study was to investigate the effect of various amino acids and their metabolites on the activities of prolidase I and II from human erythrocytes compared to those in a patient with prolidase deficiency., Design and Methods: Prolidase I and II from human erythrocytes were purified by using column chromatography. Prolidase activity against various iminodipeptides was determined by spectrophotometry using Chinard's method., Results: The activities of prolidase I and II against glycylproline and methionylproline were enhanced by glycine, L- and D-isoforms of alanine and serine and D-isoforms of valine, leucine and isoleucine. L-isoforms of branched amino acids inhibited the activity of prolidase I. On the other hand, the activity of prolidase II was enhanced by all of these L-branched amino acids. The patient's prolidase activity was also enhanced by all the L- and D-branched amino acids., Conclusion: The activities of prolidase I and II against various iminodipeptides were prominently enhanced by glycine, but the effect of L-valine differed between the two enzymes. Enzymatic properties of the patient's prolidase were essentially the same as those of prolidase II.

Published

2005

26. Purification and characterization of recombinant human liver prolidase expressed in Saccharomyces cerevisiae.

Author

Wang SH, Zhi QW, and Sun MJ

Subjects

Cloning, Molecular, Dipeptidases chemistry, Dipeptidases isolation & purification, Humans, Recombinant Proteins, Saccharomyces cerevisiae Proteins, Dipeptidases biosynthesis, Liver enzymology, Saccharomyces cerevisiae enzymology

Abstract

The recombinant human liver prolidase (rh-prolidase, EC 3.4.13.9) from the lysate supernatant of engineering yeast Saccharomyces cerevisiae was purified in two steps employing anion-exchange gradient chromatography (DEAE-Sepharose fast flow) and gel filtration chromatography (Sephacryl S-200 high resolution). The purified recombinant protein furnished a single band with a molecular weight of 56 kD. Intensity scanning of the SDS-PAGE gel revealed that the prolidase accounted for more than 90% of total protein. The optimum pH of the catalytic reaction was 8.0. The enzyme was stimulated by Mn2+, but strongly inhibited by Cu2+ and Zn2+. The rh-prolidase expressed in S. cerevisiae had both dipeptidase and organophosphorus acid anhydrolase activity. It catalyzed the hydrolysis of soman and the dipeptide Gly -Pro. In a detoxification test in vitro, purified rh-prolidase was remarkably efficient at eliminating the toxicity of a lethal dose of soman, with the result that mice survived injection of such a dose.

Published

2005

27. Characterization of an extracellular dipeptidase from Streptococcus gordonii FSS2.

Author

Goldstein JM, Kordula T, Moon JL, Mayo JA, and Travis J

Subjects

Amino Acid Sequence, Dipeptidases genetics, Dipeptidases isolation & purification, Electrophoresis, Polyacrylamide Gel, Molecular Sequence Data, Streptococcus genetics, Streptococcus metabolism, Substrate Specificity, Dipeptidases metabolism, Streptococcus enzymology

Abstract

PepV, a dipeptidase found in culture fluids of Streptococcus gordonii FSS2, was purified and characterized, and its gene was cloned. PepV is a monomeric metalloenzyme of approximately 55 kDa that preferentially degrades hydrophobic dipeptides. The gene encodes a polypeptide of 467 amino acids, with a theoretical molecular mass of 51,114 Da and a calculated pI of 4.8. The S. gordonii PepV gene is homologous to the PepV gene family from Lactobacillus and Lactococcus spp.

Published

2005

28. Production of human liver prolidase by Saccharomyces cerevisiae as host cells.

Author

Wang SH, Liu M, Chi MG, Wang QD, and Sun MJ

Subjects

Adult, Amino Acid Sequence, Aryldialkylphosphatase chemistry, Aryldialkylphosphatase metabolism, Base Sequence, Cloning, Molecular, DNA genetics, Dipeptidases genetics, Dipeptidases isolation & purification, Female, Gene Expression, Humans, Liver enzymology, Recombinant Proteins biosynthesis, Recombinant Proteins genetics, Saccharomyces cerevisiae genetics, Transformation, Genetic, Dipeptidases biosynthesis, Saccharomyces cerevisiae metabolism

Abstract

Aim: To clone and express the recombinant human liver prolidase in yeast and explore the activities of both dipeptidase and organophosphoric acid anhydrolase (OPAA)., Methods: The cDNA encoding human liver prolidase derived from healthy adult liver was cloned into the pYES2, an expression vector of S cerevisiae, and then transformed into S cerevisiae INVSc1 by electroporation. The transformant with the highest enzymatic activity was induced by galactose for expression. The optimal induction conditions (temperature, induction time, and the initial amount of inoculation cells) were estimated by orthogonal experimental design. The recombinant prolidase and OPAA activities were assayed by spectrocolorimetric methods., Results: The recombinant enzyme catalyzed the hydrolysis of organophosphorous compound soman as well as the hydrolysis of dipeptide Gly-Pro. Under the optimal induction conditions (20 h, 25 degree, initial OD(600)=0.4), the maximum activities of prolidase and OPAA came to 226.5 and 578 micromol.min(-1).g(-1) protein in cell lysate supernatants, respectively. SDS-PAGE of the recombinant enzyme in disrupted cell supernatants showed a molecular weight of 56 kDa. Intensity scanning of the SDS-PAGE gel revealed that the enzyme accounted for 3.16 % of the total protein in the supernatant. One liter incubation medium produced 7 g of wet yeast cell containing 4.56 mg of the recombination protein., Conclusion: The recombinant human liver prolidase produced by yeast cell (S cerevisiae) exhibited both dipeptidase and OPAA activities.

Published

2004

29. Purification and characterization of human prolyl dipeptidase DPP8 in Sf9 insect cells.

Author

Chen YS, Chien CH, Goparaju CM, Hsu JT, Liang PH, and Chen X

Subjects

Animals, Baculoviridae genetics, Baculoviridae metabolism, Cell Line, Dipeptidases genetics, Humans, Insecta, Peptides metabolism, Dipeptidases isolation & purification, Dipeptidases metabolism

Abstract

DPP8 is a new member of the prolyl dipeptidases, many of which have important biological functions in vivo. DPP8 catalyzes the cleavage at the carboxyl side of the proline residue at the penultimate position. To study its structure and biochemical properties, we have overexpressed the human DPP8 protein in baculovirus infected Sf9 cells. The protein is soluble and can be purified to homogeneity. Using the chromogenic H-Gly-Pro-pNA as the substrate, a kinetic study shows that purified DPP8 is active and has a similar kcat value as that of DPP-IV, a prolyl dipeptidase that is a drug target for type II diabetes. The kinetic constants of DPP8 are also determined for other chromogenic substrates, and the results indicate that DPP8 has substrate preference at both the P1 and P2 sites. The expression system provides means of better understanding the structure, catalytic mechanism, and biological function of DPP8 protein.

Published

2004

30. New role for leucyl aminopeptidase in glutathione turnover.

Author

Cappiello M, Lazzarotti A, Buono F, Scaloni A, D'Ambrosio C, Amodeo P, Méndez BL, Pelosi P, Del Corso A, and Mura U

Subjects

Animals, Cattle, Dipeptidases chemistry, Dipeptidases isolation & purification, Dipeptides metabolism, Hydrogen-Ion Concentration, Lens, Crystalline enzymology, Leucyl Aminopeptidase chemistry, Leucyl Aminopeptidase isolation & purification, Models, Molecular, Dipeptidases metabolism, Glutathione metabolism, Leucyl Aminopeptidase physiology

Abstract

A manganese-dependent cysteinyl-glycine hydrolysing activity has been purified to electrophoretic homogeneity from bovine lens. The characterization of the purified enzyme (molecular mass of the native protein, molecular mass of the subunit and extensive primary structure analysis) allowed the unequivocal attribution of the cysteinyl-glycine hydrolysing activity, which is usually associated with alanyl aminopeptidase (EC 3.4.11.2) or membrane-bound dipeptidase (EC 3.4.13.19), to LAP (leucyl aminopeptidase; EC 3.4.11.1). Analysis of the pH dependence of Cys-Gly hydrolysis catalysed by LAP, supported by a molecular modelling approach to the enzyme-substrate conformation, gave insights into the ability of the enzyme to recognize Cys-Gly as a substrate. Due to the effectiveness of LAP in hydrolysing Cys-Gly (K(m)=0.57 mM, kcat=6.0x10(3) min(-1) at pH 7.4 and 25 degrees C) with respect to other dipeptide substrates, a new role for this enzyme in glutathione turnover is proposed.

Published

2004

31. Functional and molecular characterization of rat intestinal prolidase.

Author

Hu M, Cheng Z, and Zheng L

Subjects

Aging metabolism, Amino Acid Sequence, Animals, Base Sequence, Blotting, Northern, Chromatography, Gel, Chromatography, Ion Exchange, Cloning, Molecular, DNA, Complementary, Dipeptidases antagonists & inhibitors, Dipeptidases genetics, Dipeptidases isolation & purification, Enzyme Inhibitors pharmacology, Hydrogen-Ion Concentration, Hydrolysis, Kinetics, Molecular Sequence Data, Rats, Rats, Sprague-Dawley, Dipeptidases metabolism, Intestines enzymology

Abstract

Genetic deficiency of prolidase can lead to severe problems in child development, including mental retardation. However, the exact pathogenesis of the disease is unclear. To understand the enzyme's physiologic functions, we studied the regulation of rat intestinal prolidase. The results indicated that 1) the activities of intestinal prolidase and its kinetic parameters (Km and Vmax) are site-dependent; 2) the jejunal prolidase activity was the most sensitive to the dietary restriction, and the duodenal and jejunal but not colonic kinetic parameters changed with dietary restriction; 3) the pH activity profile of jejunal prolidase at 24 h postfeeding was different from that at 48 h postfeeding, whereas the inhibition profiles of prolidase were qualitatively independent of dietary restriction; and 4) old-aged rats have lower prolidase activities in the small intestine. We also purified rat intestinal prolidase I to homogeneity. The characterization study indicated that the purified rat intestinal prolidase I is fairly similar to prolidase I from other species with a molecular weight of 116,000, which consisted of two monomers, 58,000 D each. The purified prolidase I has a Km value of 178 microM and a Vmax value of 601 micromol x min-1. mg protein-1. Screening of a rat intestinal cDNA library produced a 1.8-kb fragment that encodes the rat intestinal prolidase. This enzyme has 494 deduced amino acid sequence, which is 96% or 86% identical to mouse or human erythrocyte prolidase I. This represents the first report of a successful attempt to purify and clone an intestinal prolidase and of investigation to study prolidase regulation by diet.

Published

2003

32. Purification and primary structure determination of human lysosomal dipeptidase.

Author

Dolenc I and Mihelic M

Subjects

Amino Acid Sequence, Animals, Binding Sites, Dimerization, Dipeptidases genetics, Dipeptidases isolation & purification, Humans, Kidney enzymology, Mice, Molecular Sequence Data, Molecular Weight, Rats, Sequence Homology, Amino Acid, Dipeptidases chemistry, Lysosomes enzymology

Abstract

The lysosomal metallopeptidase is an enzyme that acts preferentially on dipeptides with unsubstituted N- and C-termini. Its activity is highest in slightly acidic pH. Here we describe the isolation and characterization of lysosomal dipeptidase from human kidney. The isolated enzyme has the amino-terminal sequence DVAKAIINLAVY and is a homodimer with a molecular mass of 100 kDa. So far no amino acid sequence has been determined for this metallopeptidase. The complete primary structure as deduced from the nucleotide sequence revealed that the isolated dipeptidase is similar to blood plasma glutamate carboxypeptidase.

Published

2003

33. Localization and activity of membrane dipeptidase in bovine ciliary epithelium.

Author

Ikeda H, Ueda M, Kobayashi H, and Honda Y

Subjects

Amino Acid Sequence, Animals, Antibodies, Monoclonal, Cattle, Chromatography, Affinity, Dipeptidases immunology, Dipeptidases isolation & purification, Enzyme-Linked Immunosorbent Assay, Fluorescent Antibody Technique, Indirect, Glycosylphosphatidylinositols metabolism, Leukotriene D4 metabolism, Leukotriene E4 metabolism, Mice, Mice, Inbred BALB C, Molecular Sequence Data, Sequence Homology, Amino Acid, beta-Lactamases metabolism, Ciliary Body enzymology, Dipeptidases metabolism, Pigment Epithelium of Eye enzymology

Abstract

Purpose: To investigate the localization and the activity of membrane dipeptidase (MDP) in the bovine eye., Methods: A monoclonal antibody (mAb), 49C mAb, raised against bovine ciliary process was used to examine the localization of MDP. Conversion of leukotriene (LT)D4 to LTE4 was evaluated by enzyme-linked immunosorbent assay for LTE4. Hydrolytic activity (beta-lactamase activity) was evaluated with a fluorometric assay. To clarify the contribution of MDP to conversion of LTD4 and beta-lactamase activity, we separated MDP from other enzymes by 49C mAb-conjugated gel., Results: The antigenic molecule of 49C mAb was shown to be MDP by amino acid sequencing. MDP was immunohistochemically detected in the ciliary pigmented and nonpigmented epithelial cells. Conversion of LTD4 to LTE4 in the ciliary process was much greater than that of the neural retina (NR). beta-Lactamase activity in the ciliary process was apparent, but that in the NR or the retinal pigment epithelium was negligible. Approximately 100% of beta-lactamase activity in the ciliary process was catalyzed by the 49C mAb-bound fraction. Conversion of LTD4 was catalyzed by the 49C mAb-bound fraction (55% of total activity) and by the unbound fraction (45% of total activity)., Conclusions: This study produced the first evidence of the presence of MDP in ciliary epithelial cells. The ciliary epithelium converts LTD4 to LTE4 and shows beta-lactamase activity. Conversion of LTD4 is catalyzed by at least two enzymes, and a major part of the conversion is induced by MDP.

Published

2003

34. Purification and characterization of VanXY(C), a D,D-dipeptidase/D,D-carboxypeptidase in vancomycin-resistant Enterococcus gallinarum BM4174.

Author

Podmore AH and Reynolds PE

Subjects

Bacterial Proteins genetics, Dipeptidases isolation & purification, Enterococcus physiology, Kinetics, Muramoylpentapeptide Carboxypeptidase isolation & purification, Recombinant Fusion Proteins metabolism, Substrate Specificity, Bacterial Proteins metabolism, Carboxypeptidases, Dipeptidases metabolism, Membrane Proteins, Muramoylpentapeptide Carboxypeptidase metabolism, Serine-Type D-Ala-D-Ala Carboxypeptidase, Vancomycin Resistance physiology

Abstract

VanXY(C), a bifunctional enzyme from VanC-phenotype Enterococcus gallinarum BM4174 that catalyses D,D-peptidase and D,D-carboxypeptidase activities, was purified as the native protein, as a maltose-binding protein fusion and with an N-terminal tag containing six histidine residues. The kinetic parameters of His(6)-VanXY(C) were measured for a variety of precursors of peptidoglycan synthesis involved in resistance: for D-Ala-D-Ala, the K(m) was 3.6 mm and k(cat), 2.5 s(-1); for UDP-MurNAc-L-Ala-D-Glu-L-Lys-DAla-D-Ala (UDP-MurNAc-pentapeptide[Ala]), K(m) was 18.8 mm and k(cat) 6.2 s(-1); for D-Ala-D-Ser, K(m) was 15.5 mm and k(cat) 0.35 s(-1). His(6)-VanXYC was inactive against the peptidoglycan precursor UDP-MurNAc-L-Ala-D-Glu-L-Lys-D-Ala-D-Ser (UDP-MurNAc-pentapeptide[Ser]). The rate of hydrolysis of the terminal D-Ala of UDP-MurNAc-pentapeptide[Ala] was inhibited 30% by 2 mm D-Ala-D-Ser or UDP-MurNAc-pentapeptide[Ser]. Therefore preferential hydrolysis of substrates terminating in D-Ala would occur during peptidoglycan synthesis in E. gallinarum BM4174, leaving precursors ending in D-Ser with a lower affinity for glycopeptides to be incorporated into peptidoglycan. Mutation of an aspartate residue (Asp59) of His-tagged VanXY(C) corresponding to Asp68 in VanX to Ser or Ala, resulted in a 50% increase and 73% decrease, respectively, of the specificity constant (k(cat)/K(m)) for D-Ala-D-Ala. This situation is in contrast to VanX in which mutation of Asp68-->Ala produced a greater than 200,000-fold decrease in the substrate specificity constant. This suggests that Asp59, unlike Asp68 in VanX, does not have a pivotal role in catalysis.

Published

2002

35. Proline dipeptidase from Pyrococcus furiosus.

Author

Grunden AM, Ghosh M, and Adams MW

Subjects

Amino Acid Sequence, Base Sequence, DNA Primers, Dipeptidases chemistry, Dipeptidases metabolism, Enzyme Stability, Molecular Sequence Data, Protein Conformation, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Sequence Homology, Amino Acid, Dipeptidases isolation & purification, Pyrococcus furiosus enzymology

Published

2001

36. Hydrolysis of carnosine and related compounds by mammalian carnosinases.

Author

Pegova A, Abe H, and Boldyrev A

Subjects

Animals, Carnosine analogs & derivatives, Dipeptidases isolation & purification, Humans, Hydrolysis, Rats, Structure-Activity Relationship, Substrate Specificity, Anserine metabolism, Carnosine metabolism, Dipeptidases metabolism, Kidney enzymology

Abstract

Comparative study of hydrolysis of carnosine and a number of its natural derivatives by human serum and rat kidney carnosinase was carried out. The rate of carnosine hydrolysis was 3-4-fold higher then for anserine and ophidine. The rate of homocarnosine, N-acetylcarnosine and carcinine hydrolysis was negligible by either of the enzymes used. Our data show that methylation, decarboxylation or acetylation of carnosine increases resistance of the molecule toward enzymatic hydrolysis. Thus, metabolic modification of carnosine may increase its half-life in the tissues.

Published

2000

37. Analysis of three overexpression systems for VanX, the Zinc(II) dipeptidase required for high-level vancomycin resistance in bacteria.

Author

Brandt JJ, Chatwood LL, and Crowder MW

Subjects

Bacterial Proteins chemistry, Bacterial Proteins metabolism, Chitin metabolism, Chromatography, Affinity, Circular Dichroism, Cloning, Molecular, Dipeptidases chemistry, Dipeptidases metabolism, Electrophoresis, Polyacrylamide Gel, Enterococcus genetics, Escherichia coli, Gene Expression Regulation, Bacterial, Gene Expression Regulation, Enzymologic, Genetic Vectors genetics, Kinetics, Protein Structure, Secondary, Protein Structure, Tertiary, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins isolation & purification, Recombinant Fusion Proteins metabolism, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Bacterial Proteins genetics, Bacterial Proteins isolation & purification, Dipeptidases genetics, Dipeptidases isolation & purification, Drug Resistance, Microbial genetics, Enterococcus enzymology, Serine-Type D-Ala-D-Ala Carboxypeptidase

Abstract

The gene from Enterococcus faecilis encoding the dipeptidase VanX was subcloned into overexpression vectors pET-5b, pET-27b, and IMPACT-T7, and VanX was overexpressed in BL21(DE3) pLysS Escherichia coli. The pET-5b-vanx overexpression plasmid produces VanX at approximately 12 mg/L under optimum conditions. VanX produced from this overexpression system exists primarily as a dimer in solution, binds ca. 1 Zn(II) ion per monomer, and exhibits K(m) and k(cat) values of 500 +/- 40 microM and 0.074 +/- 0.001 s(-1), respectively, when l-alanine-p-nitroanilide is used as substrate. The IMPACT-T7-vanx overexpression plasmid produces a VanX-fusion protein with a chitin-binding domain that allows for purification of the fusion construct with a chitin column. Cleavage of the fusion protein is completed by an on-column chemical cleavage, resulting in approximately 10 mg/L of purified VanX. VanX produced from this system is identical to that produced from the pET-5b system, except the CD spectrum of the IMPACT-T7-produced VanX suggests a small change in secondary structure. This change in secondary structure does not affect any of the kinetic or metal-binding properties of the enzyme. The pET-27b-vanx overexpression plasmid produces and secretes VanX into the growth medium; this system allows for 20 mg of VanX to be isolated per liter of growth medium. The pET-27b-produced VanX is identical to that produced from pET-5b., (Copyright 2000 Academic Press.)

Published

2000

38. Sequence, purification, and cloning of an intracellular serine protease, quiescent cell proline dipeptidase.

Author

Underwood R, Chiravuri M, Lee H, Schmitz T, Kabcenell AK, Yardley K, and Huber BT

Subjects

Amino Acid Sequence, Apoptosis, Cell Line, Cloning, Molecular, DNA, Complementary chemistry, DNA, Complementary genetics, Dipeptidases isolation & purification, Dipeptidases metabolism, Dipeptidyl Peptidase 4 metabolism, Humans, Jurkat Cells, Kinetics, Leukocytes, Mononuclear enzymology, Lymphocytes enzymology, Molecular Sequence Data, Proline metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Sequence Alignment, Sequence Analysis, DNA, Sequence Homology, Amino Acid, Serine Endopeptidases isolation & purification, Serine Endopeptidases metabolism, Substrate Specificity, Dipeptidases genetics, Serine Endopeptidases genetics

Abstract

We recently observed that specific inhibitors of post-proline cleaving aminodipeptidases cause apoptosis in quiescent lymphocytes in a process independent of CD26/dipeptidyl peptidase IV. These results led to the isolation and cloning of a new protease that we have termed quiescent cell proline dipeptidase (QPP). QPP activity was purified from CD26(-) Jurkat T cells. The protein was identified by labeling with [(3)H]diisopropylfluorophosphate and subjected to tryptic digestion and partial amino acid sequencing. The peptide sequences were used to identify expressed sequence tag clones. The cDNA of QPP contains an open reading frame of 1476 base pairs, coding for a protein of 492 amino acids. The amino acid sequence of QPP reveals similarity with prolylcarboxypeptidase. The putative active site residues serine, aspartic acid, and histidine of QPP show an ordering of the catalytic triad similar to that seen in the post-proline cleaving exopeptidases prolylcarboxypeptidase and CD26/dipeptidyl peptidase IV. The post-proline cleaving activity of QPP has an unusually broad pH range in that it is able to cleave substrate molecules at acidic pH as well as at neutral pH. QPP has also been detected in nonlymphocytic cell lines, indicating that this enzyme activity may play an important role in other tissues as well.

Published

1999

39. Alteromonas prolidase for organophosphorus G-agent decontamination.

Author

Cheng TC, DeFrank JJ, and Rastogi VK

Subjects

Aryldialkylphosphatase, Chemical Warfare Agents toxicity, Dipeptidases biosynthesis, Dipeptidases isolation & purification, Esterases metabolism, Organophosphates pharmacokinetics, Organophosphates toxicity, Organophosphorus Compounds toxicity, Sarin pharmacokinetics, Sarin toxicity, Soman pharmacokinetics, Soman toxicity, Chemical Warfare Agents pharmacokinetics, Decontamination, Dipeptidases metabolism, Gram-Negative Aerobic Bacteria enzymology, Organophosphorus Compounds pharmacokinetics

Abstract

Enzymes catalyzing the hydrolysis of highly toxic organophosphorus compounds (OPs) are classified as organophosphorus acid anhydrolases (OPAA; EC 3.1.8.2). Recently, the genes encoding OPAA from two species of Alteromonas were cloned and sequenced. Sequence and biochemical analyses of the cloned genes and enzymes have established Alteromonas OPAAs to be prolidases (E.C. 3.4.13.9), a type of dipeptidase hydrolyzing dipeptides with a prolyl residue in the carboxyl-terminal position (X-Pro). Alteromonas prolidases hydrolyze a broad range of G-type chemical warfare (CW) nerve agents. Efforts to over-produce a prolidase from A. sp.JD6.5 with the goal of developing strategies for long-term storage and decontamination have been successfully achieved. Large-scale production of this G-agent degrading enzyme is now feasible with the availability of an over-producing recombinant cell line. Use of this enzyme for development of a safe and non-corrosive decontamination system is discussed.

Published

1999

40. A continuous fluorometric assay for leukotriene D4 hydrolase.

Author

White IJ, Lawson J, Williams CH, and Hooper NM

Subjects

Animals, Coumarins, Dipeptidases isolation & purification, Evaluation Studies as Topic, Fluorescent Dyes, In Vitro Techniques, Kidney enzymology, Kinetics, Lysine analogs & derivatives, Microvilli enzymology, Substrate Specificity, Swine, Dipeptidases analysis, Dipeptidases metabolism, Leukotriene D4 metabolism, Spectrometry, Fluorescence methods

Abstract

A fluorogenic substrate for assay of leukotriene D4 hydrolase (LTDase; EC 3.4.13.19) has been prepared and evaluated, using enzyme purified from porcine kidney. The compound is based on internal quenching of the synthetic, fluorescent amino acid d, l-2-amino-3-(7-methoxy-4-coumaryl)propanoic acid (d,l-Amp) by a 2, 4-dinitrophenyl (DNP) group. The compound is epsilon-DNP-l-Lys-d-Amp which incorporates the D-isomer of Amp to exploit the unique ability among mammalian peptidases for LTDase to hydrolyze peptides containing a d-amino acid in the C-terminal position. epsilon-DNP-l-Lys-d-Amp was found to be an excellent substrate for LTDase, with Km value of 370 microoffUnder the conditions of assay, the substrate was without noticeable quenching effect on the fluorescence of the product (d-Amp) liberated by the action of LTDase. Using porcine kidney microvillar membranes, which contain a battery of peptidases, the specific inhibitor of LTDase, cilastatin, completely inhibited the breakdown of epsilon-DNP-l-Lys-d-Amp, indicating that the substrate is selective for LTDase., (Copyright 1999 Academic Press.)

Published

1999

41. Studies on the amino acid residues of the active site of alpha-aspartyl dipeptidase.

Author

Lu J, Zhang J, Zhang H, and Hao S

Subjects

Arginine, Binding Sites, Catalytic Domain, Diethyl Pyrocarbonate pharmacology, Dipeptidases isolation & purification, Escherichia coli enzymology, Kinetics, Lysine, Phenylglyoxal pharmacology, Pyridoxal Phosphate pharmacology, Salmonella typhimurium enzymology, Dipeptidases chemistry, Dipeptidases metabolism

Published

1998

42. Membrane dipeptidase and glutathione are major components of pig pancreatic zymogen granules.

Author

Höfken T, Linder D, Kleene R, Göke B, and Wagner AC

Subjects

Amino Acid Sequence, Animals, Dipeptidases genetics, Dipeptidases isolation & purification, Electrophoresis, Gel, Two-Dimensional, Gene Expression Regulation, Glutathione metabolism, Hydrogen-Ion Concentration, Intracellular Membranes enzymology, Male, Molecular Sequence Data, Pancreas chemistry, Pancreas drug effects, Rats, Rats, Wistar, Swine, Tumor Cells, Cultured, Cytoplasmic Granules enzymology, Dipeptidases chemistry, Enzyme Precursors chemistry, Glutathione chemistry, Pancreas enzymology

Abstract

Membrane proteins of highly purified porcine zymogen granules were separated by two-dimensional gel electrophoresis in order to isolate proteins which are involved in intracellular trafficking of digestive enzymes in the exocrine pancreas. A 48-kDa glycoprotein was a major component in membrane preparations washed with 0.1 M Na2CO3 and 0.5 M NaCl. By N-terminal amino acid sequencing this protein was identified as membrane dipeptidase (MDP; EC 3.4.13.19). MDP mRNA levels in rat pancreas were increased threefold by feeding rats with FOY-305, which is a known stimulus of endogenous cholecystokinin release from the gut. Cholecystokinin then stimulates secretion in pancreatic acinar cells. In another set of experiments treatment of the rat pancreatic acinar tumor cell line AR42J with dexamethasone led to an eightfold increase in the expression of MDP. Thus, the expression pattern of the MDP gene in response to hormonal stimulation in vivo and in vitro resembles those found for most of the enzymes and proteins which are involved in secretion. Since MDP has been thought to have a role in glutathione (GSH) metabolism, we also measured GSH concentration in zymogen granules and found high levels of GSH. Based on our data we propose a working model for the function of MDP. According to this model, MDP might play a pivotal role in maintaining the oxidizing conditions in the ER, which are required for the correct folding of secretory proteins., (Copyright 1998 Academic Press.)

Published

1998

43. Characterization of native and recombinant forms of an unusual cobalt-dependent proline dipeptidase (prolidase) from the hyperthermophilic archaeon Pyrococcus furiosus.

Author

Ghosh M, Grunden AM, Dunn DM, Weiss R, and Adams MW

Subjects

Amino Acid Sequence, Base Sequence, Molecular Sequence Data, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Dipeptidases isolation & purification, Pyrococcus enzymology

Abstract

Proline dipeptidase (prolidase) was purified from cell extracts of the proteolytic, hyperthermophilic archaeon Pyrococcus furiosus by multistep chromatography. The enzyme is a homodimer (39.4 kDa per subunit) and as purified contains one cobalt atom per subunit. Its catalytic activity also required the addition of Co2+ ions (Kd, 0.24 mM), indicating that the enzyme has a second metal ion binding site. Co2+ could be replaced by Mn2+ (resulting in a 25% decrease in activity) but not by Mg2+, Ca2+, Fe2+, Zn2+, Cu2+, or Ni2+. The prolidase exhibited a narrow substrate specificity and hydrolyzed only dipeptides with proline at the C terminus and a nonpolar amino acid (Met, Leu, Val, Phe, or Ala) at the N terminus. Optimal prolidase activity with Met-Pro as the substrate occurred at a pH of 7.0 and a temperature of 100 degrees C. The N-terminal amino acid sequence of the purified prolidase was used to identify in the P. furiosus genome database a putative prolidase-encoding gene with a product corresponding to 349 amino acids. This gene was expressed in Escherichia coli and the recombinant protein was purified. Its properties, including molecular mass, metal ion dependence, pH and temperature optima, substrate specificity, and thermostability, were indistinguishable from those of the native prolidase from P. furiosus. Furthermore, the Km values for the substrate Met-Pro were comparable for the native and recombinant forms, although the recombinant enzyme exhibited a twofold greater Vmax value than the native protein. The amino acid sequence of P. furiosus prolidase has significant similarity with those of prolidases from mesophilic organisms, but the enzyme differs from them in its substrate specificity, thermostability, metal dependency, and response to inhibitors. The P. furiosus enzyme appears to be the second Co-containing member (after methionine aminopeptidase) of the binuclear N-terminal exopeptidase family.

Published

1998

44. A non-specific soluble dipeptide hydrolase from guinea-pig brain.

Author

Keane FM and O'Cuinn G

Subjects

Animals, Chromatography, Gel, Chromatography, Ion Exchange, Dipeptidases chemistry, Dipeptidases isolation & purification, Guinea Pigs, Solubility, Brain enzymology, Dipeptidases metabolism

Published

1998

45. Identification by site-directed mutagenesis of three essential histidine residues in membrane dipeptidase, a novel mammalian zinc peptidase.

Author

Keynan S, Hooper NM, and Turner AJ

Subjects

Amino Acid Sequence, Animals, COS Cells, Cell Membrane enzymology, Chlorocebus aethiops, Chromatography, Affinity, Cilastatin chemistry, Dipeptidases biosynthesis, Dipeptidases isolation & purification, Humans, Kidney Cortex, Molecular Sequence Data, Protein Binding, Sepharose, Swine, Dipeptidases chemistry, Dipeptidases genetics, Histidine genetics, Mutagenesis, Site-Directed

Abstract

Membrane dipeptidase (EC 3.4.13.19) is a plasma membrane zinc peptidase that is involved in the renal metabolism of glutathione and its conjugates, such as leukotriene D4. The enzyme lacks the classical signatures of other zinc-dependent hydrolases and shows no homology with any other mammalian protein. We have used site-directed mutagenesis to explore the roles of five histidine residues in pig membrane dipeptidase that are conserved among mammalian species. When expressed in COS-1 cells, the mutants H49K and H128L exhibited a specific activity and Km for the substrate Gly-D-Phe comparable with those of the wild-type enzyme. However, the mutants H20L, H152L and H198K were inactive, but were expressed at the cell surface at equivalent levels to the wild-type, as assessed by immunoblotting and immunofluorescence. These three mutants were compared with regard to their ability to bind to the competitive inhibitor cilastatin, which binds with equal efficacy to native and EDTA-treated pig kidney membrane dipeptidase. Expressed wild-type enzyme and mutants H20L and H198K were efficiently bound by cilastatin-Sepharose, but H152L failed to bind. Thus His-152 appears to be involved in the binding of substrate or inhibitor, whereas His-20 and His-198 appear to be involved in catalysis. Membrane dipeptidase shares some similarity with a dipeptidase recently cloned from Acinetobacter calcoaceticus. In particular, His-20 and His-198 of membrane dipeptidase are conserved in the bacterial enzyme, as are Glu-125 and His-219, previously shown to be required for catalytic activity.

Published

1997

46. Purification and characterization of a dipeptidase from Lactobacillus casei ssp. casei IFPL 731 isolated from goat cheese made from raw milk.

Author

Fernandez-Espla MD and Martin-Hernandez MC

Subjects

Animals, Chromatography, Chromatography, Gel, Chromatography, Ion Exchange, Dipeptidases chemistry, Dipeptidases metabolism, Enzyme Stability, Goats, Hot Temperature, Hydrogen-Ion Concentration, Isoelectric Point, Kinetics, Molecular Weight, Substrate Specificity, Cheese microbiology, Dipeptidases isolation & purification, Lacticaseibacillus casei enzymology

Abstract

A dipeptidase was purified to homogeneity from the cell-free extract of Lactobacillus casei ssp. casei IFPL 731 by a combination of heat treatment, hydrophobic interaction chromatography, anion-exchange chromatography, and gel filtration. A purification factor of 395-fold was obtained, and yield was 20%. The dipeptidase was shown to be a metal-dependent enzyme; optimal activity was at pH 7.5 and 60 to 75 degrees C, and the enzyme had a high degree of thermal stability. Molecular mass was estimated by SDS-PAGE and gel filtration to be 46 kDa, which suggested that the enzyme existed as a monomer. Enzyme activity was most effectively inhibited by metal-chelating agents, reducing agents, or sulfhydryl group reagents. After inhibition with phenanthroline, activity was partially restored by Co2+ and Mn2+. The kinetics of Phe-Ala and Leu-Leu did not follow Michaelis-Menten saturation kinetics but exhibited a mixture of positive and negative cooperativity for the successive binding of molecules of the same substrate.

Published

1997

47. Identification of membrane dipeptidase as a major glycosyl-phosphatidylinositol-anchored protein of the pancreatic zymogen granule membrane, and evidence for its release by phospholipase A.

Author

Hooper NM, Cook S, Lainé J, and Lebel D

Subjects

Animals, Antibodies, Antibody Specificity, Cross Reactions, Dimerization, Dipeptidases chemistry, Dipeptidases isolation & purification, Electrophoresis, Polyacrylamide Gel, Epitopes analysis, Humans, Kidney enzymology, Kinetics, Macromolecular Substances, Microvilli enzymology, Molecular Weight, Phosphatidylinositol Diacylglycerol-Lyase, Phosphoinositide Phospholipase C, Phosphoric Diester Hydrolases, Rats, Swine, Cytoplasmic Granules enzymology, Dipeptidases metabolism, Enzyme Precursors metabolism, Glycosylphosphatidylinositols analysis, Intracellular Membranes enzymology, Pancreas enzymology

Abstract

Membrane dipeptidase (EC 3.4.13.19) enzyme activity that is inhibited by cilastatin has been detected in pancreatic zymogen granule membranes of human, porcine and rat origin. Immunoelectrophoretic blot analysis of human and porcine pancreatic zymogen granule membranes with polyclonal antisera raised against the corresponding kidney membrane dipeptidase revealed that the enzyme is a disulphide-linked homodimer of subunit mass 61 kDa in the human and 45 kDa in the pig. Although membrane dipeptidase was, along with glycoprotein-2, one of the only two major components of carbonate high pH-washed membranes, no enzyme activity or immunoreactivity was detected in the zymogen granule contents. Digestion with bacterial phosphatidylinositol-specific phospholipase C (PI-PLC), and subsequent recognition by antibodies specific for the cross-reacting determinant, revealed that membrane dipeptidase in human and porcine pancreatic zymogen granule membranes is glycosyl-phosphatidylinositol-anchored. Membrane dipeptidase was released from the pancreatic zymogen granule membranes by an endogenous hydrolase, and the released form migrated as a disulphide-linked dimer on SDS/PAGE under non-reducing conditions. Under reducing conditions it migrated with the same apparent molecular mass as the membrane-bound form, and was still a substrate for bacterial PI-PLC. Treatment of kidney microvillar membranes with phospholipase A2 resulted in the release of membrane dipeptidase in a form that demonstrated electrophoretic and cilastatin-Sepharose binding properties identical to those of the endogenously released form of the enzyme from zymogen granule membranes. These results indicate that the glycosyl-phosphatidylinositol anchor on the pancreatic membrane dipeptidase is cleaved by an endogenous hydrolase, probably a phospholipase A, and that this cleavage may promote the release of the protein from the membrane.

Published

1997

48. Purification and characterization of a prolidase from Lactobacillus casei subsp. casei IFPL 731.

Author

Fernández-Esplá MD, Martín-Hernández MC, and Fox PF

Subjects

Amino Acid Sequence, Chelating Agents pharmacology, Dipeptidases chemistry, Dipeptidases metabolism, Enzyme Inhibitors pharmacology, Hydrogen-Ion Concentration, Kinetics, Metals pharmacology, Molecular Weight, Oligopeptides chemistry, Substrate Specificity, Temperature, Dipeptidases isolation & purification, Lacticaseibacillus casei enzymology

Abstract

A peptidase showing a high level of specificity towards dipeptides of the X-Pro type was purified to homogeneity from the cell extract of Lactobacillus casei subsp. casei IFPL 731. The enzyme was a monomer having a molecular mass of 41 kDa. The pH and temperature optima were 6.5 to 7.5 and 55 degrees C, respectively. Metal chelating agents completely inhibited enzyme activity, indicating that the prolidase was a metalloenzyme. The Michaelis constant (K(m)) and Vmax for several proline-containing dipeptides were determined.

Published

1997

49. Purification and kinetic properties of a D-amino-acid peptide hydrolyzing enzyme from pig kidney cortex and its tentative identification with renal membrane dipeptidase.

Author

Watanabe T, Kera Y, Matsumoto T, and Yamada RH

Subjects

Animals, Chelating Agents pharmacology, Dipeptides chemistry, Dipeptides metabolism, Electrophoresis, Polyacrylamide Gel, Enzyme Inhibitors chemistry, Enzyme Inhibitors pharmacology, Kinetics, Metalloproteins metabolism, Peptides chemistry, Peptides metabolism, Substrate Specificity, Swine, Dipeptidases isolation & purification, Dipeptidases metabolism, Kidney Cortex enzymology, Peptide Hydrolases isolation & purification, Peptide Hydrolases metabolism

Abstract

We previously reported the presence of an enzyme activity which hydrolyzes Gly-D-Asp in pig kidney cortex. In the present study, an enzyme which hydrolyzes this peptide and other peptides having a low number of D- and L-amino acids has been purified from the brush border membranes of the same tissue. The native enzyme, having a molecular weight of 99,000, was apparently a homodimer of a subunit with a molecular weight of 48,000 and its optimum pH was 7.8 with Gly-D-Ala as substrate. The enzyme hydrolyzed many dipeptides, but not most of the tripeptides tested with a few exceptions, from which the carboxyl-terminal amino acid was liberated by the enzyme. Of the dipeptides examined, those having a D-amino acid at the amino-terminal were poor substrates, whereas those bearing a D-amino acid at the carboxyl-terminal were good substrates, comparable with their diastereomers with a L-amino acid at the same position. The enzyme was potently inhibited by cilastatin but not by amastatin and bestatin. Metal ion chelators and dithiothreitol were also inhibitory. Comparison of the properties of present enzyme with those of other known enzymes suggests that this should be tentatively identified with renal membrane dipeptidase. The demonstrated high activity toward dipeptides containing various D-amino acids at the carboxyl-terminal suggests a possibility that the enzyme in fact plays a role in degradation in vivo of D-amino-acid-containing peptides.

Published

1996

50. The proteolytic system of Lactobacillus sanfrancisco CB1: purification and characterization of a proteinase, a dipeptidase, and an aminopeptidase.

Author

Gobbetti M, Smacchi E, and Corsetti A

Subjects

Amino Acid Sequence, Aminopeptidases metabolism, Dipeptidases metabolism, Endopeptidases metabolism, Hydrogen-Ion Concentration, Molecular Sequence Data, Molecular Weight, Substrate Specificity, Temperature, Aminopeptidases isolation & purification, Dipeptidases isolation & purification, Endopeptidases isolation & purification, Lactobacillus enzymology

Abstract

A cell envelope 57-kDa proteinase, a cytoplasmic 65-kDa dipeptidase, and a 75-kDa aminopeptidase were purified from Lactobacillus sanfrancisco CB1 sourdough lactic acid bacterium by sequential fast protein liquid chromatography steps. All of the enzymes are monomers. The proteinase was most active at pH 7.0 and 40 degrees C, while aminopeptidase and dipeptidase had optima at pH 7.5 and 30 to 35 degrees C. Relatively high activities were observed at the pH and temperature of the sourdough fermentation. The proteinase is a serine enzyme. Urea-polyacrylamide gel electrophoresis of digest of alpha s1- and beta-caseins showed differences in the pattern of peptides released by the purified proteinase and those produced by crude preparations of the cell envelope proteinases of Lactobacillus delbrueckii subsp. bulgaricus B397 and Lactococcus lactis subsp. lactis SK11. Reversed-phase fast protein liquid chromatography of gliadin digests showed a more-complex peptide pattern produced by the proteinase of Lactobacillus sanfrancisco CB1. The dipeptidase is a metalloenzyme with high affinity for dipeptides containing hydrophobic amino acids but had no activity on tripeptides or larger peptides. The aminopeptidase was also inhibited by metal-chelating agents, and showed a broad N-terminal hydrolytic activity including di- and tripeptides. Km values of 0.70 and 0.44 mM were determined for the dipeptidase on Leu-Leu and the aminopeptidase on Leu-p-nitroanilide, respectively.

Published

1996