Your search keyword '"Enteropeptidase chemistry"' showing total 72 results

1. Preparation of recombinant neuritin protein.

Author

Meng P, Zhu L, Guo J, Li Y, Wei Y, Sun J, and Zhu J

Subjects

Animals, PC12 Cells, Rats, Neuropeptides genetics, Neuropeptides chemistry, Neuropeptides metabolism, Enteropeptidase metabolism, Enteropeptidase genetics, Enteropeptidase chemistry, Chromatography, Affinity, Neuronal Outgrowth drug effects, Chromatography, Gel, Gene Expression, GPI-Linked Proteins genetics, GPI-Linked Proteins chemistry, GPI-Linked Proteins metabolism, Recombinant Proteins genetics, Recombinant Proteins chemistry, Recombinant Proteins metabolism, Recombinant Proteins biosynthesis, Recombinant Proteins isolation & purification, Escherichia coli genetics, Escherichia coli metabolism

Abstract

Neuritin plays an important role in promoting nerve injury repair and maintaining synaptic plasticity, making it a potential therapeutic target for the treatment of nerve injury and neurodegenerative diseases. The present study aimed to obtain an active, unlabeled neuritin protein. Initially, a neuritin protein expression system with an enterokinase site was constructed in Escherichia coli. After optimizing induction conditions and screening for high expression, a neuritin recombinant protein with purity exceeding 85 % was obtained through Ni-affinity chromatography. Subsequently, unlabeled neuritin with a molecular weight of 11 kDa was obtained through the enzymatic cleavage of the His label using an enterokinase. Furthermore, a neuritin recombinant protein with purity exceeding 95 % was obtained using gel chromatography. Functional investigations revealed that neurite outgrowth of PC12 cells was stimulated by the isolated neuritin. This study establishes a method to obtain active and unlabeled neuritin protein, providing a foundation for subsequent research on its biological functions., (Copyright © 2024 Elsevier Inc. All rights reserved.)

Published

2024

2. Cryo-EM structures reveal the activation and substrate recognition mechanism of human enteropeptidase.

Author

Yang X, Ding Z, Peng L, Song Q, Zhang D, Cui F, Xia C, Li K, Yin H, Li S, Li Z, and Huang H

Subjects

Humans, Cryoelectron Microscopy, Trypsin, Enteropeptidase chemistry, Trypsinogen

Abstract

Enteropeptidase (EP) initiates intestinal digestion by proteolytically processing trypsinogen, generating catalytically active trypsin. EP dysfunction causes a series of pancreatic diseases including acute necrotizing pancreatitis. However, the molecular mechanisms of EP activation and substrate recognition remain elusive, due to the lack of structural information on the EP heavy chain. Here, we report cryo-EM structures of human EP in inactive, active, and substrate-bound states at resolutions from 2.7 to 4.9 Å. The EP heavy chain was observed to clamp the light chain with CUB2 domain for substrate recognition. The EP light chain N-terminus induced a rearrangement of surface-loops from inactive to active conformations, resulting in activated EP. The heavy chain then served as a hinge for light-chain conformational changes to recruit and subsequently cleave substrate. Our study provides structural insights into rearrangements of EP surface-loops and heavy chain dynamics in the EP catalytic cycle, advancing our understanding of EP-associated pancreatitis., (© 2022. The Author(s).)

Published

2022

3. Comparison of Periplasmic and Cytoplasmic Expression of Bovine Enterokinase Light Chain in E. coli.

Author

Ayat H, Darvishi O, Moazeni E, and Momeni Bidezard A

Subjects

Animals, Cattle, Cytoplasm genetics, Cytoplasm metabolism, Escherichia coli genetics, Escherichia coli metabolism, Iran, Recombinant Fusion Proteins chemistry, Enteropeptidase chemistry, Enteropeptidase genetics, Enteropeptidase metabolism, Periplasm metabolism

Abstract

Enterokinase enzyme is widely used in production of recombinant proteins. This enzyme is isolated from the intestine and recognizes a specific cleavage site (X↓LYS-ASP 4 ). Several studies have been performed to produce recombinant active enterokinase. In this study, the coding sequence of bovine enteropeptidase light chain (bEK L ) was isolated from Iranian Sarabi cattle and its expression was investigated in the periplasm and cytoplasm of E. coli by two different expression vectors, pET22 and pET32RH. RNA was extracted from the duodenum part of cattle, cDNA was amplified, the enterokinase light chain coding fragment was cloned and the expression was examined by SDS-PAGE analysis. The higher amounts of soluble enterokinase as a fusion with thioredoxin (Trx) were detected in cytoplasmic expression. The functional enterokinase was purified with a yield of 45 mg per litter by two-steps Ni 2+ affinity chromatography. The effective activity of the enzyme implies that it can be produced in large scale for biotechnological applications., (© 2021. The Author(s), under exclusive licence to Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2022

4. Targeting Enteropeptidase with Reversible Covalent Inhibitors To Achieve Metabolic Benefits.

Author

Sun W, Zhang X, Cummings MD, Albarazanji K, Wu J, Wang M, Alexander R, Zhu B, Zhang Y, Leonard J, Lanter J, and Lenhard J

Subjects

Animals, Blood Glucose metabolism, Body Weight drug effects, CHO Cells, Cricetulus, Diabetes Mellitus metabolism, Eating drug effects, Enteropeptidase chemistry, Enzyme Inhibitors chemistry, Half-Life, Humans, Kinetics, Models, Molecular, Obesity metabolism, Protein Conformation, Structure-Activity Relationship, Enteropeptidase antagonists & inhibitors, Enzyme Inhibitors pharmacology, Metabolism drug effects

Abstract

Inhibition of the serine protease enteropeptidase (EP) opens a new avenue to the discovery of chemotherapeutics for the treatment of metabolic diseases. Camostat has been used clinically for treating chronic pancreatitis in Japan; however, the mechanistic basis of the observed clinical efficacy has not been fully elucidated. We demonstrate that camostat is a potent reversible covalent inhibitor of EP, with an inhibition potency ( k inact /K I ) of 1.5 × 10 4 M -1 s -1 High-resolution liquid chromatography-mass spectrometry (LC-MS) showed addition of 161.6 Da to EP after the reaction with camostat, consistent with insertion of the carboxyphenylguanidine moiety of camostat. Covalent inhibition of EP by camostat is reversible, with an enzyme reactivation half-life of 14.3 hours. Formation of a covalent adduct was further supported by a crystal structure resolved to 2.19 Å, showing modification of the catalytic serine of EP by a close analog of camostat, leading to formation of the carboxyphenylguanidine acyl enzyme identical to that expected for the reaction with camostat. Of particular note, minor structural modifications of camostat led to changes in the mechanism of inhibition. We observed from other studies that sustained inhibition of EP is required to effect a reduction in cumulative food intake and body weight, with concomitant improved blood glucose levels in obese and diabetic leptin-deficient mice. Thus, the structure-activity relationship needs to be driven by not only the inhibition potency but also the mechanistic and kinetic characterization. Our findings support EP as a target for the treatment of metabolic diseases and demonstrate that reversible covalent EP inhibitors show clinically relevant efficacy. SIGNIFICANCE STATEMENT: Interest in targeted covalent drugs has expanded in recent years, particularly so for kinase targets, but also more broadly. This study demonstrates that reversible covalent inhibition of the serine protease enteropeptidase is a therapeutically viable approach to the treatment of metabolic diseases and that mechanistic details of inhibition are relevant to clinical efficacy. Our mechanistic and kinetic studies outline a framework for detailed inhibitor characterization that is proving essential in guiding discovery efforts in this area., (Copyright © 2020 The Author(s).)

Published

2020

5. Site-specific, covalent immobilization of an engineered enterokinase onto magnetic nanoparticles through transglutaminase-catalyzed bioconjugation.

Author

Wang JH, Tang MZ, Yu XT, Xu CM, Yang HM, and Tang JB

Subjects

Enteropeptidase metabolism, Enzymes, Immobilized chemistry, Models, Molecular, Particle Size, Substrate Specificity, Surface Properties, Transglutaminases chemistry, Biocatalysis, Enteropeptidase chemistry, Enzymes, Immobilized metabolism, Magnetite Nanoparticles chemistry, Protein Engineering, Transglutaminases metabolism

Abstract

Enterokinase (EK) is one of the most popular enzymes for the in vitro cleavage of fusion proteins due to its high degree of specificity for the amino-acid sequence (Asp) 4 -Lys. Enzyme reusability is desirable for reducing operating costs and facilitating the industrial application of EK. In this work, we report the controlled, site-specific and covalent cross-linking of an engineered EK LC on amine-modified magnetic nanoparticles (NH 2 -MNPs) via microbial transglutaminase-catalyzed bioconjugation for the development of the oriented-immobilized enzyme, namely, EK LC @NH 2 -MNP biocatalyst. Upon the site-specific immobilization, approximately 90% EK LC enzymatic activity was retained, and the biocatalyst exhibited more than 85% of initial enzymatic activity regardless of storage or reusable stability over a month. The EK LC @NH 2 -MNP biocatalyst was further applied to remove the His tag-(Asp) 4 -Lys fusion partner from the His tag-(Asp) 4 -Lys-(GLP-1) 3 substrate fusion protein, result suggested the EK LC @NH 2 -MNP possessed remarkable reusability, without a significant decrease of enzymatic activity over 10 cycles (P >  0.05). Supported by the unique properties of MNPs, the proposed EK LC @NH 2 -MNP biocatalyst is expected to promote the economical utilization of enterokinase in fusion protein cleavage., (Copyright © 2019 Elsevier B.V. All rights reserved.)

Published

2019

6. Effects of N-glycosylation on the biochemical properties of recombinant bEK L expressed in Pichia pastoris.

Author

Wang Z, Guo C, Liu L, and Huang H

Subjects

Animals, Catalysis, Cattle, Enteropeptidase genetics, Enzyme Stability, Gene Expression, Glycosylation, Hot Temperature, Hydrogen-Ion Concentration, Mutagenesis, Site-Directed, Pichia metabolism, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Enteropeptidase chemistry, Enteropeptidase metabolism, Pichia genetics

Abstract

Enterokinase is an ideal tool protease for cleaving fusion proteins in genetic engineering. The bovine enterokinase light chain (bEK L ) produced in Pichia pastoris was shown to be a glycoprotein. To study the effects of N-glycosylation on the biochemical properties of bEK L , the enzyme was deglycosylated via site-directed mutagenesis. The results showed that elimination of the N-glycosylation sites of bEK L (N64, N103 and N165) did not significantly affect the protein secretion level in P. pastoris, but it does greatly influence its enzymatic activity. The N64Q increased the specific activity of the enzyme for GD 4 K-β-naphthylamide and improved its catalytic efficiency. Moreover, the glycosylated bEK L is more thermostable than its deglycosylated counterparts. Structural analysis of glycosylated and deglycosylated bEK L revealed that the removal of N-glycosylation did not have pronounced changes on the secondary structure but there was a significant difference in the tertiary structure. In conclusion, this study demonstrated that the effects of glycosylation at different degrees and sites in bEK L were diverse. Moreover, this work will provide theoretical support for designing enzymes on the basis of N-glycosylation to meet the demands of the biochemical industry., (Copyright © 2018. Published by Elsevier Inc.)

Published

2018

7. Recombinant production of the insecticidal scorpion toxin BjαIT in Escherichia coli.

Author

Li H and Xia Y

Subjects

Animals, Chromatography, Ion Exchange methods, Cloning, Molecular, Enteropeptidase chemistry, Escherichia coli drug effects, Escherichia coli genetics, Escherichia coli metabolism, Gene Expression, Insecticides isolation & purification, Insecticides metabolism, Insecticides toxicity, Isopropyl Thiogalactoside pharmacology, Larva physiology, Locusta migratoria physiology, Plasmids chemistry, Plasmids metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Recombinant Fusion Proteins toxicity, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Scorpion Venoms genetics, Scorpion Venoms isolation & purification, Scorpion Venoms toxicity, Solubility, Thioredoxins genetics, Thioredoxins metabolism, Larva drug effects, Locusta migratoria drug effects, Recombinant Fusion Proteins biosynthesis, Scorpion Venoms biosynthesis, Scorpions chemistry

Abstract

Scorpion long-chain insect neurotoxins have important potential application value in agricultural pest control. The difficulty of obtaining natural toxins is the major obstacle preventing analyses of their insecticidal activity against more agricultural insect pests. Here we cloned the insect neurotoxin BjαIT gene into the pET32 expression vector and expressed the resulting thioredoxin (Trx)-BjαIT fusion protein in Escherichia coli. Soluble Trx-BjαIT was expressed at a high level when induced at 18 °C with 0.1 mM isopropyl β-d-1-thiogalactopyranoside, and it was purified by Ni 2+ -nitriloacetic acid affinity chromatography. After cleaving the Trx tag with recombinant enterokinase, the digestion products were purified by CM Sepharose FF ion-exchange chromatography, and 1.5 mg of purified recombinant BjαIT (rBjαIT) was obtained from 100 ml of induced bacterial cells. Injecting rBjαIT induced obvious neurotoxic symptoms and led to death in locust (Locusta migratoria) larvae. Dietary toxicity was not observed in locusts. The results demonstrate that active rBjαIT could be obtained efficiently from an E. coli expression system, which is helpful for determining its insecticidal activity against agricultural insect pests., (Copyright © 2017 Elsevier Inc. All rights reserved.)

Published

2018

8. Preparation of umami octopeptide with recombined Escherichia coli: Feasibility and challenges.

Author

Zhao L, Zhang Y, Venkitasamy C, Pan Z, Zhang L, Guo S, Xiong W, Xia H, Wenlong L, and Xinhua G

Subjects

Amino Acid Sequence, Cloning, Molecular, Escherichia coli metabolism, Food Technology methods, Gene Expression, Genetic Vectors chemistry, Genetic Vectors metabolism, Humans, Hydrolysis, Oligopeptides genetics, Oligopeptides isolation & purification, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Taste physiology, Enteropeptidase chemistry, Escherichia coli genetics, Odorants analysis, Oligopeptides biosynthesis, Protein Engineering methods

Abstract

The taste of umami peptide H-Lys-Gly-Asp-Glu-Glu-Ser-Leu-Ala-OH (LGAGGSLA) is controversial. One possible reason for this controversy is the use of chemically synthesized LGAGGSLA to confirm its taste. To explore other ways to further confirm the flavor of LGAGGSLA, we developed a new strategy to prepare a bio-source peptide by adopting a gene engineering method to express LGAGGSLA in recombinant Escherichia coli. In our previous work, we structured the LGAGGSLA recombinant expression system and optimized the culturing conditions for preparing a fusion protein. However, the fusion protein was not cleaved by enterokinase to obtain LGAGGSLA. Because the cleavage conditions of commercial enterokinase were not specific and recombinant engineered bacteria had the potential to be used in industrial processes, in this addendum, we calculated the mass and volume yields of key processing steps in the preparation of LGAGGSLA, and established a model of cleavage conditions with the cleavage ratio of LGAGGSLA. When the LGAGGSLA was confirmed to show umami taste, it is considered as a new umami or umami enhancer. The gene information of LGAGGSLA should have a great potential in the development of new flavor product and food product containing high umami flavor.

Published

2018

9. Fine-tuning sortase-mediated immobilization of protein layers on surfaces using sequential deprotection and coupling.

Author

Raeeszadeh-Sarmazdeh M, Parthasarathy R, and Boder ET

Subjects

Enteropeptidase chemistry, Enteropeptidase metabolism, Enzymes, Immobilized chemistry, Protein Engineering, Aminoacyltransferases chemistry, Aminoacyltransferases metabolism, Bacterial Proteins chemistry, Bacterial Proteins metabolism, Cysteine Endopeptidases chemistry, Cysteine Endopeptidases metabolism, Enzymes, Immobilized metabolism

Abstract

Increasing interest in protein immobilization on surfaces has heightened the need for techniques enabling layer-by-layer protein attachment. Here, we report a technique for controlling enzyme-mediated immobilization of layers of protein on the surface using a genetically encoded protecting group. An enterokinase-cleavable peptide sequence was inserted at the N-terminus of bifunctional fluorescent proteins containing Sortase A substrate recognition tags at both ends to control Sortase A-mediated protein immobilization on the surface layer-by-layer. Efficient, sequential immobilization of a second layer of protein using Sortase A required removal of the N-terminal protecting group, suggesting the method enables multilayer synthesis using cyclic deprotection and coupling steps. © 2017 American Institute of Chemical Engineers Biotechnol. Prog., 33:824-831, 2017., (© 2017 American Institute of Chemical Engineers.)

Published

2017

10. A High Yield and Cost-efficient Expression System of Human Granzymes in Mammalian Cells.

Author

Dotiwala F, Fellay I, Filgueira L, Martinvalet D, Lieberman J, and Walch M

Subjects

Calcium chemistry, Cell Culture Techniques methods, Chromatography, Affinity methods, Enteropeptidase chemistry, Granzymes genetics, Granzymes isolation & purification, HEK293 Cells, Humans, Plasmids genetics, Granzymes biosynthesis, Transfection methods

Abstract

When cytotoxic T lymphocytes (CTL) or natural killer (NK) cells recognize tumor cells or cells infected with intracellular pathogens, they release their cytotoxic granule content to eliminate the target cells and the intracellular pathogen. Death of the host cells and intracellular pathogens is triggered by the granule serine proteases, granzymes (Gzms), delivered into the host cell cytosol by the pore forming protein perforin (PFN) and into bacterial pathogens by the prokaryotic membrane disrupting protein granulysin (GNLY). To investigate the molecular mechanisms of target cell death mediated by the Gzms in experimental in-vitro settings, protein expression and purification systems that produce high amounts of active enzymes are necessary. Mammalian secreted protein expression systems imply the potential to produce correctly folded, fully functional protein that bears posttranslational modification, such as glycosylation. Therefore, we used a cost-efficient calcium precipitation method for transient transfection of HEK293T cells with human Gzms cloned into the expression plasmid pHLsec. Gzm purification from the culture supernatant was achieved by immobilized nickel affinity chromatography using the C-terminal polyhistidine tag provided by the vector. The insertion of an enterokinase site at the N-terminus of the protein allowed the generation of active protease that was finally purified by cation exchange chromatography. The system was tested by producing high levels of cytotoxic human Gzm A, B and M and should be capable to produce virtually every enzyme in the human body in high yields.

Published

2015

11. Expression and purification of short hydrophobic elastin-like polypeptides with maltose-binding protein as a solubility tag.

Author

Bataille L, Dieryck W, Hocquellet A, Cabanne C, Bathany K, Lecommandoux S, Garbay B, and Garanger E

Subjects

Amino Acid Sequence, Base Sequence, Biomimetic Materials, Elastin chemistry, Elastin isolation & purification, Enteropeptidase chemistry, Escherichia coli metabolism, Escherichia coli Proteins metabolism, Gene Expression, Hydrophobic and Hydrophilic Interactions, Maltose-Binding Proteins chemistry, Maltose-Binding Proteins metabolism, Molecular Sequence Data, Peptides chemistry, Peptides isolation & purification, Plasmids metabolism, Proteolysis, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins metabolism, Solubility, Transition Temperature, Elastin biosynthesis, Escherichia coli genetics, Escherichia coli Proteins genetics, Maltose-Binding Proteins genetics, Peptides metabolism, Plasmids chemistry, Recombinant Fusion Proteins genetics

Abstract

Elastin-like polypeptides (ELPs) are biodegradable polymers with interesting physico-chemical properties for biomedical and biotechnological applications. The recombinant expression of hydrophobic elastin-like polypeptides is often difficult because they possess low transition temperatures, and therefore form aggregates at sub-ambient temperatures. To circumvent this difficulty, we expressed in Escherichia coli three hydrophobic ELPs (VPGIG)n with variable lengths (n=20, 40, and 60) in fusion with the maltose-binding protein (MBP). Fusion proteins were soluble and yields of purified MBP-ELP ranged between 66 and 127mg/L culture. After digestion of the fusion proteins by enterokinase, the ELP moiety was purified by using inverse transition cycling. The purified fraction containing ELP40 was slightly contaminated by traces of undigested fusion protein. Purification of ELP60 was impaired because of co-purification of the MBP tag during inverse transition cycling. ELP20 was successfully purified to homogeneity, as assessed by gel electrophoresis and mass spectrometry analyses. The transition temperature of ELP20 was measured at 15.4°C in low salt buffer. In conclusion, this method can be used to produce hydrophobic ELP of low molecular mass., (Copyright © 2015 Elsevier Inc. All rights reserved.)

Published

2015

12. Improvement of an antibody-enzyme coupling yield by enzyme surface supercharging.

Author

Prasse AA, Zauner T, Büttner K, Hoffmann R, and Zuchner T

Subjects

Enteropeptidase genetics, Enteropeptidase metabolism, Enzyme-Linked Immunosorbent Assay, Humans, Mutagenesis, Site-Directed, Antibodies chemistry, Enteropeptidase chemistry

Abstract

Background: Protein cross-coupling reactions demand high yields, especially if the products are intended for bioanalytics, like enzyme-linked immunosorbent assays. Amongst other factors, the coupling yield depends on the concentration of the proteins being used for coupling. Protein supercharging of enzymes can increase the solubility dramatically, which could promote enzyme-antibody coupling reactions. A highly soluble, supercharged variant of the enzyme human enteropeptidase light chain was created by a site-directed mutagenesis of surface amino acids, used for the production of an antibody-enzyme conjugate and compared to the wild type enzyme., Results: Wild type and mutant enzyme could successfully be cross-coupled to an antibody to give antibody-enzyme conjugates suitable for ELISA. Their assay performances and the analysis of the enzyme activities in solution demonstrate that the supercharged version could be coupled to a higher extent, which resulted in better assay sensitivities. The generated conjugate, based on the supercharged enzyme, was feasible as a reporter molecule in a sandwich ELISA and allowed the detection of epidermal growth factor with a detection limit of 15.63 pg (25 pmol/L)., Conclusion: The highly soluble, surface supercharged, human enteropeptidase light chain mutant provided better yields in coupling the enzyme to an antibody than the wild type. This is most likely related to the higher protein concentration during the coupling. The data suggest that supercharging can be applied favourably to other proteins which have to be covalently linked to other polymers or surfaces with high yields without losses in enzyme activity or specificity.

Published

2014

13. Structure basis for the unique specificity of medaka enteropeptidase light chain.

Author

Xu J, Hu S, Wang X, Zhao Z, Zhang X, Wang H, Zhang D, and Guo Y

Subjects

Animals, Biocatalysis, Cattle, Humans, Models, Molecular, Structure-Activity Relationship, Substrate Specificity, Enteropeptidase chemistry, Enteropeptidase metabolism, Oryzias metabolism

Published

2014

14. Do-it-yourself histidine-tagged bovine enterokinase: a handy member of the protein engineer's toolbox.

Author

Skala W, Goettig P, and Brandstetter H

Subjects

Animals, Cattle, Cloning, Molecular, Enteropeptidase biosynthesis, Escherichia coli genetics, Inclusion Bodies enzymology, Protein Folding, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins genetics, Enteropeptidase chemistry, Enteropeptidase genetics, Histidine chemistry, Protein Engineering

Abstract

Enterokinase, a two-chain duodenal serine protease, activates trypsinogen by removing its N-terminal propeptide. Due to a clean cut after the non-primed site recognition sequence, the enterokinase light chain is frequently employed in biotechnology to separate N-terminal affinity tags from target proteins with authentic N-termini. In order to obtain large quantities of this protease, we adapted an in vitro folding protocol for a pentahistidine-tagged triple mutant of the bovine enterokinase light chain. The purified, highly active enzyme successfully processed recombinant target proteins, while the pentahistidine-tag facilitated post-cleavage removal. Hence, we conclude that producing enterokinase in one's own laboratory is an efficient alternative to the commercial enzyme., (Copyright © 2013 The Authors. Published by Elsevier B.V. All rights reserved.)

Published

2013

15. Heterogeneous catalysis on the phage surface: Display of active human enteropeptidase.

Author

Gasparian ME, Bobik TV, Kim YV, Ponomarenko NA, Dolgikh DA, Gabibov AG, and Kirpichnikov MP

Subjects

Bacteriophages genetics, Catalysis, Catalytic Domain genetics, Cloning, Molecular, Enteropeptidase genetics, Enteropeptidase metabolism, Genetic Vectors, Humans, Kinetics, Mutation, Naphthalenes pharmacology, Recombinant Fusion Proteins genetics, Substrate Specificity, Cell Surface Display Techniques methods, Enteropeptidase chemistry, Recombinant Fusion Proteins chemistry

Abstract

Enteropeptidase (EC 3.4.21.9) plays a key role in mammalian digestion as the enzyme that physiologically activates trypsinogen by highly specific cleavage of the trypsinogen activation peptide following the recognition sequence D4K. The high specificity of enteropeptidase makes it a powerful tool in modern biotechnology. Here we describe the application of phage display technology to express active human enteropeptidase catalytic subunits (L-HEP) on M13 filamentous bacteriophage. The L-HEP/C122S gene was cloned in the g3p-based phagemid vector pHEN2m upstream of the sequence encoding the phage g3p protein and downstream of the signal peptide-encoding sequence. Heterogeneous catalysis of the synthetic peptide substrate (GDDDDK-β-naphthylamide) cleavage by phage-bound L-HEP was shown to have kinetic parameters similar to those of soluble enzyme, with the respective Km values of 19 μM and 20 μM and kcat of 115 and 92 s(-1). Fusion proteins containing a D4K cleavage site were cleaved with phage-bound L-HEP/C122S as well as by soluble L-HEP/C122S, and proteolysis was inhibited by soybean trypsin inhibitor. Rapid large-scale phage production, one-step purification of phage-bound L-HEP, and easy removal of enzyme activity from reaction samples by PEG precipitation make our approach suitable for the efficient removal of various tag sequences fused to the target proteins. The functional phage display technology developed in this study can be instrumental in constructing libraries of mutants to analyze the effect of structural changes on the activity and specificity of the enzyme or generate its desired variants for biotechnological applications., (Copyright © 2013 Elsevier Masson SAS. All rights reserved.)

Published

2013

16. Human enteropeptidase light chain: bioengineering of recombinants and kinetic investigations of structure and function.

Author

Smith ET and Johnson DA

Subjects

Amino Acid Sequence, Cloning, Molecular, Enteropeptidase isolation & purification, Enteropeptidase metabolism, Humans, Kinetics, Models, Molecular, Molecular Sequence Data, Pichia genetics, Protein Conformation, Protein Stability, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Sequence Alignment, Substrate Specificity, Amino Acid Substitution, Enteropeptidase chemistry, Enteropeptidase genetics

Abstract

The serine protease enteropeptidase exhibits a high level of substrate specificity for the cleavage sequence DDDDK∼ X, making this enzyme a useful tool for the separation of recombinant protein fusion domains. In an effort to improve the utility of enteropeptidase for processing fusion proteins and to better understand its structure and function, two substitution variants of human enteropeptidase, designated R96Q and Y174R, were created and produced as active (>92%) enzymes secreted by Pichia pastoris with yields in excess of 1.7 mg/Liter. The Y174R variant showed improved specificities for substrates containing the sequences DDDDK (kcat /KM = 6.83 × 10⁶ M⁻¹ sec⁻¹) and DDDDR (kcat /KM = 1.89 × 10⁷ M⁻¹ sec⁻¹) relative to all other enteropeptidase variants reported to date. BPTI inhibition of Y174R was significantly decreased. Kinetic data demonstrate the important contribution of the positively charged residue 96 to extended substrate specificity in human enteropeptidase. Modeling shows the importance of the charge-charge interactions in the extended substrate binding pocket., (Copyright © 2013 The Protein Society.)

Published

2013

17. Preparation and functional evaluation of RGD-modified streptavidin targeting to integrin-expressing melanoma cells.

Author

Syrkina MS, Shirokov DA, Rubtsov MA, Kadyrova EL, Veiko VP, and Manuvera VA

Subjects

Animals, Cattle, Cell Line, Tumor, Chromatography, Gel, Enteropeptidase chemistry, Escherichia coli, Fluorescein-5-isothiocyanate chemistry, Fluorescent Dyes chemistry, Humans, Male, Melanoma, Mice, Oligopeptides biosynthesis, Oligopeptides genetics, Protein Binding, Protein Engineering, Proteolysis, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Staining and Labeling, Streptavidin biosynthesis, Streptavidin genetics, Integrin alphaVbeta3 metabolism, Oligopeptides chemistry, Streptavidin chemistry

Abstract

The vertical growth stage is the most dangerous stage of melanoma and is often associated with a poor prognosis. The increased invasiveness and metastasis that is typical for vertically growing melanoma are mediated by the molecules of cell adhesion (particularly, integrins). Integrin αvβ3, which is abundantly expressed on melanoma cells with high metastatic potentials and is characterized by low expression levels in normal melanocytes, is potentially an attractive target for melanoma diagnostics and therapy. Integrin αvβ3 is known to recognize the arginine-glycine-aspartic (RGD) sequence, which has been found in a wide variety of its natural ligands. Here expression vectors bearing the genes of fusion proteins have been constructed for producing these proteins in Escherichia coli. Such fusion proteins consist of a peptidic 'address,' targeting the integrins on melanoma cells, linked to an 'adaptor' for the attachment of a diagnostic or toxic agent. The peptidic 'address' contains the RGD motif, which is stabilized by a disulfide bond to achieve the optimal receptor binding conformation. The 'adaptor' is a tetrameric protein, namely, streptavidin, that is able to achieve high-affinity binding of d-biotin (K(d) = 10(-15) M) and confer avidity to the address peptide. This binding ability facilitates the generation of anti-melanoma diagnostic and therapeutic agents using the appropriate biotin derivatives. These recombinant proteins were purified from the periplasm of E.coli using columns with 2-iminobiotin agarose and demonstrated an ability to adhere to the surface of murine and human melanoma cells.

Published

2013

18. Fusion expression and purification of four disulfide-rich peptides reveals enterokinase secondary cleavage sites in animal toxins.

Author

Chen Z, Han S, Cao Z, Wu Y, Zhuo R, and Li W

Subjects

Amino Acid Motifs, Amino Acid Sequence, Base Sequence, Charybdotoxin chemistry, Charybdotoxin isolation & purification, Chromatography, Affinity, Cloning, Molecular, Cystine chemistry, Enteropeptidase chemistry, Escherichia coli, Glutathione Transferase biosynthesis, Glutathione Transferase chemistry, Isoelectric Point, Molecular Sequence Data, Molecular Weight, Proteolysis, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins isolation & purification, Scorpion Venoms chemistry, Scorpion Venoms isolation & purification, Spectrometry, Mass, Matrix-Assisted Laser Desorption-Ionization, Charybdotoxin biosynthesis, Recombinant Fusion Proteins biosynthesis, Scorpion Venoms biosynthesis

Abstract

Animal toxins are powerful tools for testing the pharmacological, physiological, and structural characteristics of ion channels, proteases, and other receptors. However, most animal toxins are disulfide-rich peptides that are difficult to produce functionally. Here, a glutathione S-transferase (GST) fusion expression strategy was used to produce four recombinant animal toxin peptides, ChTX, StKTx23, BmP01, and ImKTx1, with different isoelectric points from 4.7 to 9.2. GST tags were removed by enterokinase, a widely used and effective commercial protease that cleaves after lysine at the cleavage site DDDDK. Using this strategy, two disulfide-rich animal toxins ChTX and StKTx23 were obtained successfully with a yield of approximately 1-2 mg/l culture. Electrophysiological experiments further showed that these two recombinant toxins showed good bioactivities, indicating that our method was effective in producing large amounts of functional disulfide-rich animal toxins. Interestingly, by analyzing the separated fractions of BmP01, StKTx23, and ImKTx1 using matrix-assisted laser desorption ionization time-of-flight mass spectrometry, four new enterokinase secondary cleavage sites were found, consisting of the sequences "WEYR," "EDK," "QNAR," and "DNDK." To our knowledge, this is the first report of the presence of secondary cleavage sites for commercial enterokinase in animal toxins. These findings will help us use commercial enterokinase appropriately as a cleavage tool in the production of animal toxins., (Copyright © 2012 Elsevier Inc. All rights reserved.)

Published

2013

19. Crystal structure of a supercharged variant of the human enteropeptidase light chain.

Author

Simeonov P, Zahn M, Sträter N, and Zuchner T

Subjects

Animals, Cattle, Enteropeptidase genetics, Enzyme Stability, Humans, Kinetics, Models, Molecular, Mutation, Protein Conformation, Protein Subunits chemistry, Static Electricity, X-Ray Diffraction, Enteropeptidase chemistry

Abstract

The highly specific serine protease human enteropeptidase light chain cleaves the Asp4Lys recognition sequence and represents an interesting enzyme for biotechnological applications. The human enzyme shows 10 times faster kinetics compared to other animal sources but low solubility under low salt conditions, which hampers protein production and crystallization. Therefore, a supercharged variant (N6D/G21D/G22D/N142D/K210E/C112S) with increased solubility was used for crystallization. The structure (resolution, 1.9 Å) displays a typical α/β trypsin-like serine protease-fold. The mutations introduced for protein supercharging generate larger clusters of negative potential on both sites of the active cleft but do not affect the structural integrity of the protein., (Copyright © 2012 Wiley Periodicals, Inc.)

Published

2012

20. Effects of operating parameters on the efficiency of liposomal encapsulation of enzymes.

Author

Hwang SY, Kim HK, Choo J, Seong GH, Hien TB, and Lee EK

Subjects

Animals, Armoracia, Buffers, Chromatography, Gel, Drug Compounding, Enteropeptidase chemistry, Horseradish Peroxidase chemistry, Hyaluronoglucosaminidase chemistry, Hydrogen-Ion Concentration, Isoelectric Point, Molecular Weight, Osmolar Concentration, Particle Size, Trypsin chemistry, 1,2-Dipalmitoylphosphatidylcholine chemistry, Liposomes chemistry, Static Electricity

Abstract

Encapsulation of active proteins in the hydrophilic core of vesicular liposomes is important for developing a therapeutic protein carrier system. The efficiency of liposomal encapsulation of proteins is generally low. A better understanding of the fundamental mechanisms of encapsulation is needed to increase this efficiency. In this study we investigated the effects of operating parameters such as phospholipid concentration, buffer pH and ionic strength, protein size and surface charge, and liposome size on the enzyme encapsulation yield. Four model enzymes of different molecular weights and isoelectric points (trypsin, horseradish peroxidase, enterokinase and hyaluronidase) were encapsulated into three different sized liposomes (125 nm, 194 nm, and 314 nm in mean diameter). Relatively inert and neutral DPPC (1,2-dipalmitoyl-sn-glycero-3-phosphocholine) was used as the main phospholipid in the liposomes. Size exclusion chromatography was used to separate the enzyme-encapsulated liposomes from the free enzyme, and the encapsulation yield was determined from the peak area. The encapsulation yield was generally low ranging from ca. 5% to 20%, and did not depend much on the molecular weight of the enzyme encapsulated. Larger liposomes had higher encapsulation yields. The electrostatic interaction between the phospholipid and enzyme was the most significant parameter in determining the encapsulation yield. Thus adjusting buffer pH and ionic strength and adding charged phospholipids to the liposome preparation to impart electric charge to the lipid bilayer could significantly improve the yield. This approach can be used to optimize the liposomal encapsulation of clinically significant proteins., (Copyright © 2012 Elsevier B.V. All rights reserved.)

Published

2012

21. Enhanced soluble expression of recombinant Flavobacterium heparinum heparinase I in Escherichia coli by fusing it with various soluble partners.

Author

Huang J, Cao L, Guo W, Yuan R, Jia Z, and Huang K

Subjects

Bacterial Proteins genetics, Bacterial Proteins metabolism, Cloning, Molecular, Electrophoresis, Polyacrylamide Gel, Enteropeptidase chemistry, Enteropeptidase genetics, Enteropeptidase metabolism, Escherichia coli genetics, Flavobacterium genetics, Heparin Lyase genetics, Heparin Lyase metabolism, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Solubility, Bacterial Proteins chemistry, Escherichia coli metabolism, Flavobacterium enzymology, Heparin Lyase chemistry, Recombinant Fusion Proteins chemistry

Abstract

Heparinase I (HepA) was originally isolated from Flavobacterium heparinum (F. heparinum) and specifically cleaves heparin/heparan sulfate in a site-dependent manner, showing great promise for producing low molecular weight heparin (LMWH). However, expressing recombinant HepA is extremely difficult in Escherichia coli because it suffers from low yields, insufficient purity and insolubility. In this paper, we systematically cloned and fused the HepA gene to the C-terminus of five soluble partners, including translation initiation factor 2 domain I (IF2), glutathione S-transferase (GST), maltose-binding protein (MBP), small ubiquitin modifying protein (SUMO) and N-utilization substance A (NusA), to screen for their abilities to improve the solubility of recombinant HepA when expressed in E. coli. A convenient two-step immobilized metal affinity chromatography (IMAC) method was utilized to purify these fused HepA hybrids. We show that, except for NusA, the fusion partners dramatically improved the soluble expression of recombinant HepA, with IF2-HepA and SUMO-HepA creating almost completely soluble HepA (98% and 94% of expressed HepA fusions are soluble, respectively), which is the highest yield rate published to the best of our knowledge. Moreover, all of the fusion proteins show comparable biological activity to their unfused counterparts and could be used directly without removing the fusion tags. Together, our results provide a viable option to produce large amounts of soluble and active recombinant HepA for manufacturing., (Copyright © 2012 Elsevier Inc. All rights reserved.)

Published

2012

22. Lipid-bound apolipoproteins in tyrosyl radical-oxidized HDL stabilize ABCA1 like lipid-free apolipoprotein A-I.

Author

Hossain MA, Ngeth S, Chan T, Oda MN, and Francis GA

Subjects

ATP Binding Cassette Transporter 1, ATP-Binding Cassette Transporters genetics, Apolipoprotein A-I chemistry, Calpain metabolism, Cell Membrane metabolism, Cells, Cultured, Cholesterol metabolism, Enteropeptidase chemistry, Esterification, Gene Expression, Humans, Lipoproteins, HDL chemistry, Oxidation-Reduction, Protein Binding, Protein Stability, Protein Transport, Proteolysis, Tyrosine chemistry, ATP-Binding Cassette Transporters metabolism, Apolipoprotein A-I metabolism, Lipoproteins, HDL metabolism, Tyrosine analogs & derivatives, Tyrosine metabolism

Abstract

Background: ATP-binding cassette transporter A1 (ABCA1) mediates the lipidation of exchangeable apolipoproteins, the rate-limiting step in the formation of high density lipoproteins (HDL). We previously demonstrated that HDL oxidized ex vivo by peroxidase-generated tyrosyl radical (tyrosylated HDL, tyrHDL) increases the availability of cellular cholesterol for efflux and reduces the development of atherosclerosis when administered to apolipoprotein E-deficient mice as compared to treatment with control HDL., Results: In the current study we determined that tyrHDL requires functional ABCA1 for this enhanced activity. Like lipid-free apolipoprotein A-I (apoA-I), tyrHDL increases total and cell surface ABCA1, inhibits calpain-dependent and -independent proteolysis of ABCA1, and can be bound by cell surface ABCA1 in human skin fibroblasts. Additionally, tyrHDL apoproteins are susceptible to digestion by enteropeptidase like lipid-free apoA-I, but unlike lipid-bound apoA-I on HDL, which is resistant to proteolysis., Conclusions: These results provide the first evidence that lipid-bound apolipoproteins on the surface of spherical HDL particles can behave like lipid-free apoA-I to increase ABCA1 protein levels and activity.

Published

2012

23. Dissecting structural basis of the unique substrate selectivity of human enteropeptidase catalytic subunit.

Author

Ostapchenko VG, Gasparian ME, Kosinsky YA, Efremov RG, Dolgikh DA, and Kirpichnikov MP

Subjects

Amino Acid Sequence, Animals, Cattle, Humans, Hydrolysis, Molecular Dynamics Simulation, Molecular Sequence Data, Peptides chemistry, Peptides metabolism, Protein Binding, Protein Conformation, Sequence Alignment, Substrate Specificity, Catalytic Domain, Enteropeptidase chemistry, Enteropeptidase metabolism

Abstract

Enteropeptidase is a key enzyme in the digestion system of higher animals. It initiates enzymatic cascade cleaving trypsinogen activation peptide after a unique sequence DDDDK. Recently, we have found specific activity of human enteropeptidase catalytic subunit (L-HEP) being significantly higher than that of its bovine ortholog (L-BEP). Moreover, we have discovered that L-HEP hydrolyzed several nonspecific peptidic substrates. In this work, we aimed to further characterize species-specific enteropeptidase activities and to reveal their structural basis. First, we compared hydrolysis of peptides and proteins lacking DDDDK sequence by L-HEP and L-BEP. In each case human enzyme was more efficient, with the highest hydrolysis rate observed for substrates with a large hydrophobic residue in P2-position. Computer modeling suggested enzyme exosite residues 96 (Arg in L-HEP, Lys in L-BEP) and 219 (Lys in L-HEP, Gln in L-BEP) to be responsible for these differences in enteropeptidase catalytic activity. Indeed, human-to-bovine mutations Arg96Lys, Lys219Gln shifted catalytic properties of L-HEP toward those of L-BEP. This effect was amplified in case of the double mutation Arg96Lys/Lys219Gln, but still did not cover the full difference in catalytic activities of human and bovine enzymes. To find a missing link, we studied monopeptide benzyl-arginine-β-naphthylamide hydrolysis. L-HEP catalyzed it with an order lower K (m) than L-BEP, suggesting the monopeptide-binding S1 site input into catalytic distinction between two enteropeptidase species. Together, our findings suggest structural basis of the unique catalytic properties of human enteropeptidase and instigate further studies of its tentative physiological and pathological roles.

Published

2012

24. High level expression of human enteropeptidase light chain in Pichia pastoris.

Author

Pepeliaev S, Krahulec J, Černý Z, Jílková J, Tlustá M, and Dostálová J

Subjects

Bioreactors, Cloning, Molecular, Electrophoresis, Polyacrylamide Gel, Enteropeptidase chemistry, Enteropeptidase genetics, Enzymes, Immobilized chemistry, Enzymes, Immobilized genetics, Enzymes, Immobilized metabolism, Histidine genetics, Histidine metabolism, Humans, Pichia genetics, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Enteropeptidase biosynthesis, Pichia metabolism, Recombinant Fusion Proteins biosynthesis

Abstract

Human enterokinase (enteropeptidase, rhEP), a serine protease expressed in the proximal part of the small intestine, converts the inactive form of trypsinogen to active trypsin by endoproteolytic cleavage. The high specificity of the target site makes enterokinase an ideal tool for cleaving fusion proteins at defined cleavage sites. The mature active enzyme is comprised of two disulfide-linked polypeptide chains. The heavy chain anchors the enzyme in the intestinal brush border membrane, whereas the light chain represents the catalytic enzyme subunit. The synthetic gene encoding human enteropeptidase light chain with His-tag added at the C-terminus to facilitate protein purification was cloned into Pichia pastoris expression plasmids under the control of an inducible AOX1 or constitutive promoters GAP and AAC. Cultivation media and conditions were optimized as well as isolation and purification of the target protein. Up to 4 mg/L of rhEP was obtained in shake-flask experiments and the expression level of about 60-70 mg/L was achieved when cultivating in lab-scale fermentors. The constitutively expressing strains proved more efficient and less labor-demanding than the inducible ones. The rhEP was immobilized on AV 100 sorbent (Iontosorb) to allow repeated use of enterokinase, showing specific activity of 4U/mL of wet matrix., (Copyright © 2011 Elsevier B.V. All rights reserved.)

Published

2011

25. Design and efficient production of bovine enterokinase light chain with higher specificity in E. coli.

Author

Chun H, Joo K, Lee J, and Shin HC

Subjects

Amino Acid Sequence, Amino Acid Substitution, Animals, Biotechnology, Cattle, Enteropeptidase chemistry, Escherichia coli genetics, Escherichia coli metabolism, In Vitro Techniques, Kinetics, Models, Molecular, Mutagenesis, Site-Directed, Oligopeptides chemistry, Oligopeptides metabolism, Protein Engineering, Protein Structure, Quaternary, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Substrate Specificity, Enteropeptidase genetics, Enteropeptidase metabolism

Abstract

Enterokinase light chain (EKL) is a serine protease that recognizes Asp-Asp-Asp-Asp-Lys (D(4)K) sequence and cleaves the C-terminal peptide bond of the lysine residue. The utility of EKL as a site-specific cleavage enzyme is hampered by sporadic cleavage at other sites than the canonical D(4)K recognition sequence. In order to produce more site-specific EKL, we have generated several EKL mutants in E. coli with substitutions at Tyr174 and Lys99 using PDI (protein disulfide isomerase) fusion system. Substitution of Tyr174 by basic residues confers higher specificity on EKL. The production of EKL with higher specificity could widen the utility of EKL as a site-specific cleavage enzyme to produce various recombinant proteins with therapeutic or industrial values.

Published

2011

26. [Designing of hybrid human interferon alfa-2 strain-producers and the use of enteropeptidase for obtaining N-terminal methionine-free interferons].

Author

Shirokov DA, Riabichenko VV, Akishina RI, Ospel'nikova TP, Glazunov AV, Chestukhina GG, and Veĭko VP

Subjects

Escherichia coli enzymology, Escherichia coli genetics, Genetic Vectors genetics, Humans, Interferon alpha-2, Interferon-alpha biosynthesis, Methionine chemistry, Plasmids genetics, Protein Renaturation, Recombinant Fusion Proteins biosynthesis, Recombinant Proteins, Enteropeptidase chemistry, Industrial Microbiology methods, Interferon-alpha chemistry, Interferon-alpha isolation & purification, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins isolation & purification

Abstract

A system for production of human interferon-alpha2a (IFN-alpha2a) and IFN-alpha2b lacking N-terminal methionine has been developed. Plasmids containing genes of hybrid IFN-alpha2 under the control of different promoters were constructed; a sequence encoding the enteropeptidase hydrolysis site being introduced in proximal part of the genes. As the result, 4 strains of Escherichia coli producing hybrid IFN-alpha2 have been obtained. The methodology for IFN-alpha2 renaturation, hydrolysis of its N-terminal part, chromatographic purification of N-terminal methionine-free IFN-alpha2 has been developed.

Published

2011

27. Surface supercharged human enteropeptidase light chain shows improved solubility and refolding yield.

Author

Simeonov P, Berger-Hoffmann R, Hoffmann R, Sträter N, and Zuchner T

Subjects

Amino Acid Sequence, Amino Acid Substitution, Animals, Biocatalysis, Cloning, Molecular, Enteropeptidase isolation & purification, Enteropeptidase metabolism, Enzyme Stability, Escherichia coli genetics, Hot Temperature, Humans, Models, Molecular, Molecular Sequence Data, Protein Conformation, Protein Subunits isolation & purification, Protein Subunits metabolism, Solubility, Enteropeptidase chemistry, Enteropeptidase genetics, Protein Engineering methods, Protein Refolding, Protein Subunits chemistry, Protein Subunits genetics, Static Electricity

Abstract

Enteropeptidase is a serine protease used in different biotechnological applications. For many applications the smaller light chain can be used to avoid the expression of the rather large holoenzyme. Recombinant human enteropeptidase light chain (hEPL) shows high activity but low solubility and refolding yields, currently limiting its use in biotechnological applications. Here we describe several protein modifications that lead to improved solubility and refolding yield of human hEPL whilst retaining the enzyme activity. Specifically, protein surface supercharging (N6D, G21D, G22D, N141D, K209E) of the protein increased the solubility more than 100-fold. Replacement of a free cysteine residue with serine (C112S) improved the refolding yield by 50%. The heat stability of this C112S variant was also significantly improved by supercharging. This study shows that even mild protein surface supercharging can have pronounced effects on protein solubility and stability.

Published

2011

28. Self-degrading, MRI-detectable hydrogel sensors with picomolar target sensitivity.

Author

Colomb J, Louie K, Massia SP, and Bennett KM

Subjects

Animals, Biocompatible Materials chemistry, Drug Delivery Systems, Enteropeptidase chemistry, Ferric Compounds chemistry, Linear Models, Macromolecular Substances chemistry, Nanoparticles chemistry, Polymers chemistry, Proteoglycans chemistry, Rats, Rats, Sprague-Dawley, Tissue Engineering, Trypsinogen chemistry, Enzyme Precursors chemistry, Hydrogels chemistry, Magnetic Resonance Imaging instrumentation

Abstract

Nanostructured hydrogels have been developed as synthetic tissues and scaffolds for cell and drug delivery, and as guides for tissue regeneration. A fundamental problem in the development of synthetic hydrogels is that implanted gel structure is difficult to monitor noninvasively. This work demonstrates that the aggregation of magnetic nanoparticles, attached to specific macromolecules in biological and synthetic hydrogels, can be controlled to detect changes in gel macromolecular structure with MRI. It is further shown that the gels can be made to self-degrade when they come into contact with a target molecule in as low as pM concentrations. The sensitivity of the gels to the target is finely controlled using an embedded zymogen cascade amplifier. These "MRI reporter gels" may serve as smart, responsive polymer implants, as tissue scaffolds to deliver drugs, or to detect specific pathogens in vivo., (Copyright © 2010 Wiley-Liss, Inc.)

Published

2010

29. The trail of my studies on glycoproteins from enterokinase to tumor markers.

Author

Yamashina I

Subjects

Amino Acid Sequence, Animals, Antibodies, Monoclonal immunology, Humans, Membrane Glycoproteins chemistry, Membrane Glycoproteins metabolism, Molecular Sequence Data, Neoplasms immunology, Biomarkers, Tumor chemistry, Biomarkers, Tumor metabolism, Enteropeptidase chemistry, Enteropeptidase metabolism, Glycoproteins chemistry, Glycoproteins immunology, Glycoproteins metabolism

Abstract

This review describes the results of the author's studies on glycoproteins which have been carried out for more than 50 years. Starting from the elucidation of basic structures of glycoproteins, i.e. the structure of the linkage between an amino acid and a sugar and the occurrence of the beta-mannosidic linkage as the common structure of glycoproteins, the author became interested in the cell membrane glycoproteins focused on the comparison of cancer cells versus normal cells. These studies were then extended to the establishment of sugar-directed and cancer-associated monoclonal antibodies. Some of the monoclonal antibodies are useful for cancer diagnosis.

Published

2010

30. [Preparation of rhIL-11 from fusion protein by using enterokinase].

Author

Zhao Y and Huang H

Subjects

Enteropeptidase chemistry, Enteropeptidase metabolism, Escherichia coli genetics, Escherichia coli metabolism, Genetic Vectors genetics, Humans, Interleukin-11 genetics, Protein Engineering methods, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Enteropeptidase genetics, Interleukin-11 biosynthesis, Recombinant Fusion Proteins biosynthesis

Abstract

The study was aimed to investigate the technological parameters of rhIL-11 preparation from fusion protein by using enterokinase. Fusion expression vector pET32a/IL-11 was transferred into E.coli BL21 (DE3) pLysS and its expression was induced by IPTG, the lysis supernatant of the engineering strain was purified by Ni-NTA resin and then the target rhIL-11 was digested by auto-cleavaged DsbA-EKL-(His)(8). The results showed that after affinity chromatography, Trx-IL-11 was obtained with the yield of 11.25mg/g, the purity of 89.2% and the recovery of 91.8%. Finally the target rhIL-11 was digested and purified to over 95%. In conclusion, the preparation method of rhIL-11 from fusion protein by using enterokinase is simple and feasible with good separation, which can meet industrial requirements.

Published

2008

31. Enhancing the specificity of the enterokinase cleavage reaction to promote efficient cleavage of a fusion tag.

Author

Shahravan SH, Qu X, Chan IS, and Shin JA

Subjects

Amino Acid Sequence, CCAAT-Enhancer-Binding Proteins chemistry, CCAAT-Enhancer-Binding Proteins genetics, Hydrogen-Ion Concentration, Molecular Sequence Data, Receptors, Aryl Hydrocarbon chemistry, Receptors, Aryl Hydrocarbon genetics, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Temperature, Urea chemistry, CCAAT-Enhancer-Binding Proteins isolation & purification, Enteropeptidase chemistry, Receptors, Aryl Hydrocarbon isolation & purification, Recombinant Fusion Proteins isolation & purification

Abstract

In our work with designed minimalist proteins based on the bZIP motif, we have found our His-tagged proteins to be prone to inclusion body formation and aggregation; we suspect this problem is largely due to the His tag, known to promote aggregation. Using AhR6-C/EBP, a hybrid of the AhR basic region and C/EBP leucine zipper, as representative of our bZIP-like protein family, we attempted removal of the His tag with enterokinase (EK) but obtained the desired cleavage product in very small yield. EK is known for proteolysis at noncanonical sites, and most cleavage occurred at unintended sites. We manipulated experimental conditions to improve specificity of proteolysis and analyzed the cleavage products; no effect was observed after changing pH, temperature, or the amount of EK. We then suspected the accessibility of the EK site was impeded due to protein aggregation. We found that the easily implemented strategy of addition of urea (1-4 M) greatly improved EK cleavage specificity at the canonical site and reduced adventitious cleavage. We believe that this enhancement in specificity is due to a more "open" protein structure, in which the now accessible canonical target can compete effectively with adventitious cleavage sites of related sequence.

Published

2008

32. Immobilisation of bovine enterokinase and application of the immobilised enzyme in fusion protein cleavage.

Author

Kubitzki T, Noll T, and Lütz S

Subjects

Animals, Biochemistry methods, Biotechnology methods, Cattle, Glutaral chemistry, Immunoglobulin G chemistry, Magnetics, Microspheres, Models, Chemical, Mucin-1 chemistry, Temperature, Time Factors, Enteropeptidase chemistry, Enzymes, Immobilized chemistry, Recombinant Fusion Proteins chemistry

Abstract

Two immobilisation methods for enterokinase were developed, which yielded high remaining activities for the cleavage of the fusion protein MUC1-IgG Fc. Different carrier materials were compared regarding remaining enzyme activity and storage stability. Immobilisation procedures involving support material activation using glutardialdehyde were found to result in low remaining activities. Applying less aggressive activation procedures, remaining activities of approximately 60% were received when immobilising enterokinase on either Estapor paramagnetic microspheres or hexamethylamino Sepabeads. In case of hexamethylamino Sepabeads we were able to increase the half-life time 4.3-fold at 23 degrees C and 3.8-fold at 4 degrees C compared to the free enzyme at the same temperatures. By immobilising the biocatalyst the downstream process is simplified allowing the easy removal of the enzyme from the reaction mixture. The immobilised enterokinase cleaves the fusion protein MUC1-IgG Fc in at least two repeated batches, proving the efficiency of the immobilisation method and the reusability of the biocatalyst.

Published

2008

33. [A rate-limiting stage of enteropeptidase hydrolysis].

Author

Mikhaĭlova AG, Likhareva VV, and Rumsh LD

Subjects

Acylation, Hydrolysis, Kinetics, Structure-Activity Relationship, Enteropeptidase chemistry, Oligopeptides chemistry

Abstract

It has been shown for the first time that deacylation is the rate-limiting stage in the enteropeptidase-catalyzed hydrolysis of highly efficient oligopeptide substrates containing four Asp residues in positions P2-P5. On the other hand, the rate-limiting stage in the hydrolysis of low-efficiency peptide substrates containing less than four Asp or Glu residues in positions P2-P5 is acylation, as has previously been suggested for all amide and peptide substrates of serine proteases on the basis of the classic studies by Bender et al. The method of introduction of an additional nucleophile or another effector that selectively affects the deacylation stage was used to determine the rate-limiting stage in the enteropeptidase hydrolysis of Nalpha-benzyloxycarbonyl-L-lysine thiobenzyl ester, the highly efficient amide substrate GlyAsp4-Lys beta-naphthyl amide, and the low-efficiency peptide substrate VLSAADK-GNVKAAWG (where a hyphen denotes the hydrolysis site). The English version of the paper: Russian Journal of Bioorganic Chemistry, 2008, vol. 34, no. 2; see also http://www.maik.ru.

Published

2008

34. Hydrogen peroxide enhances enterokinase-catalysed proteolytic cleavage of fusion protein.

Author

Cui T, Gao Y, Ang CX, Puah CM, Gutte B, and Lam Y

Subjects

Catalysis, Enteropeptidase genetics, Patents as Topic, Peptide Hydrolases chemistry, Peptide Hydrolases genetics, Biotechnology trends, Enteropeptidase chemistry, Hydrogen Peroxide chemistry, Protein Engineering trends, Recombinant Fusion Proteins chemical synthesis

Abstract

The effects of hydrogen peroxide on enterokinase catalysis were studied using several fusion proteins recombinantly produced from E. coli. It was demonstrated that hydrogen peroxide enhanced the rate of enterokinase cleavage reaction, leading to a faster release of the target peptide as discussed in patent WO07149053. Among the conditions tested, we observed that hydrogen peroxide could exert its effect on the cleavage of fusion proteins over a wide range of pH and temperature. This finding might provide a simple solution for the accelerated enterokinase cleavage of thermolabile fusion proteins at low temperature.

Published

2008

35. A study of conformational restraints on reactivity of human PR3-specific autoantibodies (ANCA) facilitated through protein folding manipulations of a new recombinant proteinase 3 protein.

Author

Farrag L, Pendergraft WF 3rd, Yang JJ, Jennette JC, Falk RJ, and Preston GA

Subjects

Antibodies, Antineutrophil Cytoplasmic immunology, Enteropeptidase chemistry, Enzyme-Linked Immunosorbent Assay, Epitope Mapping, Epitopes genetics, Epitopes immunology, Female, Granulomatosis with Polyangiitis immunology, Histidine chemistry, Histidine genetics, Humans, Male, Mutagenesis, Site-Directed, Myeloblastin genetics, Myeloblastin immunology, Recombinant Proteins genetics, Recombinant Proteins immunology, Antibodies, Antineutrophil Cytoplasmic chemistry, Epitopes chemistry, Myeloblastin chemistry, Protein Folding, Recombinant Proteins chemistry

Abstract

Proteinase 3 (PR3)-specific antineutrophil cytoplasmic autoantibodies (PR3-ANCA) recognize conformational epitopes on PR3. This study evaluates PR3-ANCA target epitopes utilizing a novel recombinant PR3 (rPR3) produced to accommodate manipulations of the N-terminal domain. The rPR3 molecule contains an N-terminus six histidine tag, which can be removed by enterokinase (EK) cleavage of an adjacent EK cleavage site. Once cleaved the remaining amino acids correspond to the mature N-terminus of PR3. This rPR3 can be manipulated to produce three variant forms: tagged rPR3(+his), EK-cleaved (his-tag removed) rPR3(- his), and EK-cleaved, denatured/refolded rPR3(- his/dr) (the proteolytically active form). Patients with clinically positive PR3-ANCA titers (n = 40) were confirmed for reactivity against purchased native PR3 in our system. Controls included 29 healthy volunteers and 34 MPO-ANCA patients. All PR3-ANCA sera samples tested were reactive with one or more forms of the recombinant protein (greater than mean ELISA OD 405 + 2 SDs of controls). Of significance, three sera were reactive with non-active forms only and three others were more reactive with rPR3(- his/dr) than with native PR3. The results of our evaluation of PR3-ANCA sera for reactivity against the three forms of our rPR3 protein uniquely exemplify the diverse array of epitopes within the PR3-ANCA population. This new recombinant form of PR3 should provide a suitable approach to mapping ANCA epitopes using site-directed mutagenesis.

Published

2007

36. Purification and refolding optimization of recombinant bovine enterokinase light chain overexpressed in Escherichia coli.

Author

Tan H, Wang J, and Zhao ZK

Subjects

Animals, Cattle, Enteropeptidase chemistry, Escherichia coli metabolism, Protein Folding, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins isolation & purification, Enteropeptidase isolation & purification

Abstract

The nucleotide sequence encoding bovine enterokinase light chain (EK) from Chinese northern yellow bovine was isolated. Two single-nucleotide mutations, namely, C245G and A528T were identified. The gene encoding the Pro82Arg/Glu176Asp variant of known bovine EK was fused with glutathione S-transferase and overexpressed mainly as an inclusion body in Escherichia coli BL21 (DE3), upon induction with IPTG and glucose. Effective fusion protein purification, refolding, auto-catalytic cleavage and mature EK recovery were described. The specific activity of the purified EK was determined as 110+/- 10 U/mg, which was comparable to a specific activity of > or =20 U/mg of the E. coli expressed EK sample provided by Sigma (Cat. No. E4906). This procedure produced approximately 53 mg of EK per 500 mL of cell culture, which was much higher than previous reports, thus providing a basis for large-scale production of EK and for further applications in biotechnology.

Published

2007

37. Trypsin IV or mesotrypsin and p23 cleave protease-activated receptors 1 and 2 to induce inflammation and hyperalgesia.

Author

Knecht W, Cottrell GS, Amadesi S, Mohlin J, Skåregärde A, Gedda K, Peterson A, Chapman K, Hollenberg MD, Vergnolle N, and Bunnett NW

Subjects

Animals, Aprotinin chemistry, Capsaicin pharmacology, Edema chemically induced, Edema genetics, Edema metabolism, Edema pathology, Enteropeptidase chemistry, Ganglia, Spinal metabolism, Ganglia, Spinal pathology, Granulocytes metabolism, Granulocytes pathology, Humans, Hyperalgesia chemically induced, Hyperalgesia genetics, Hyperalgesia pathology, Inflammation chemically induced, Inflammation genetics, Inflammation metabolism, Inflammation pathology, Male, Mice, Mice, Knockout, Nociceptors metabolism, Nociceptors pathology, Pain Measurement, Rats, Rats, Sprague-Dawley, Receptor, PAR-1 deficiency, Receptor, PAR-2 deficiency, Receptors, Proteinase-Activated metabolism, Receptors, Thrombin metabolism, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins metabolism, Recombinant Proteins pharmacology, Trypsin chemistry, Trypsin genetics, Trypsin pharmacology, Trypsin Inhibitors chemistry, Calcium Signaling drug effects, Hyperalgesia metabolism, Receptor, PAR-1 metabolism, Receptor, PAR-2 physiology, Trypsin metabolism

Abstract

Although principally produced by the pancreas to degrade dietary proteins in the intestine, trypsins are also expressed in the nervous system and in epithelial tissues, where they have diverse actions that could be mediated by protease-activated receptors (PARs). We examined the biological actions of human trypsin IV (or mesotrypsin) and rat p23, inhibitor-resistant forms of trypsin. The zymogens trypsinogen IV and pro-p23 were expressed in Escherichia coli and purified to apparent homogeneity. Enteropeptidase cleaved both zymogens, liberating active trypsin IV and p23, which were resistant to soybean trypsin inhibitor and aprotinin. Trypsin IV cleaved N-terminal fragments of PAR(1), PAR(2), and PAR(4) at sites that would expose the tethered ligand (PAR(1) = PAR(4) > PAR(2)). Trypsin IV increased [Ca(2+)](i) in transfected cells expressing human PAR(1) and PAR(2) with similar potencies (PAR(1), 0.5 microm; PAR(2), 0.6 microm). p23 also cleaved fragments of PAR(1) and PAR(2) and signaled to cells expressing these receptors. Trypsin IV and p23 increased [Ca(2+)](i) in rat dorsal root ganglion neurons that responded to capsaicin and which thus mediate neurogenic inflammation and nociception. Intraplantar injection of trypsin IV and p23 in mice induced edema and granulocyte infiltration, which were not observed in PAR (-/-)(1)(trypsin IV) and PAR (-/-)(2) (trypsin IV and p23) mice. Trypsin IV and p23 caused thermal hyperalgesia and mechanical allodynia and hyperalgesia in mice, and these effects were absent in PAR (-/-)(2) mice but maintained in PAR (-/-)(1) mice. Thus, trypsin IV and p23 are inhibitor-resistant trypsins that can cleave and activate PARs, causing PAR(1)- and PAR(2)-dependent inflammation and PAR(2)-dependent hyperalgesia.

Published

2007

38. The ways of realization of high specificity and efficiency of enteropeptidase.

Author

Mikhailova AG, Likhareva VV, Teich N, and Rumsh LD

Subjects

Amino Acid Sequence, Animals, Cattle, Enteropeptidase chemistry, Humans, Hydrolysis, Models, Biological, Molecular Sequence Data, Mutant Proteins chemistry, Mutant Proteins metabolism, Protein Subunits chemistry, Protein Subunits metabolism, Structure-Activity Relationship, Substrate Specificity, Trypsinogen metabolism, Enteropeptidase metabolism, Protein Engineering

Abstract

Comparative substrate analysis of full-length bovine enteropeptidase and trypsin, bovine and human enteropeptidase light chains was performed using model N-terminal dodecapeptides corresponding to wild-type human trypsinogen and pancreatitis-associated mutant trypsinogens K23R and D22G. The substitution of Lys residue by Arg at P1 leads to 2-fold increase in the efficiency of enteropeptidase hydrolysis; the absence of the negatively charged residue at P2 reduces the efficiency of such hydrolysis by two orders of magnitude. The difference in efficiency of peptide chain hydrolysis after Lys/Arg residues by enteropeptidase compared to trypsin is equal to the difference in hydrolysis by serine proteases of different primary specificity of their specific substrates.

Published

2007

39. An SRLLR motif downstream of the scissile bond enhances enterokinase cleavage efficiency.

Author

Liew OW, Jenny Chong PC, Lim YZ, Ang CX, Amy Lau YC, Yandle TG, and Brennan SO

Subjects

Amino Acid Motifs, Animals, Chromatography, High Pressure Liquid, Cloning, Molecular, Electrophoresis, Polyacrylamide Gel, Enteropeptidase chemistry, Humans, Mice, Molecular Sequence Data, Natriuretic Peptide, C-Type isolation & purification, Recombinant Fusion Proteins isolation & purification, Recombinant Fusion Proteins metabolism, Sequence Homology, Amino Acid, Spectrometry, Mass, Electrospray Ionization, Enteropeptidase genetics, Enteropeptidase metabolism, Natriuretic Peptide, C-Type metabolism, Thioredoxins metabolism

Abstract

In a previous paper, we reported more efficient enterokinase cleavage at a C-terminal non-target LKGDR(201) site compared with an internally sited canonical recognition site, DDDDK(156). When this non-target site was placed internally to replace DDDDK(156) between the thioredoxin moiety and mouse NT-proCNP(1-50), this site was poorly processed leading us to conclude that efficient processing at LKGDR(201) in the first instance was due to its accessibility at the C-terminus of the fusion protein. Subsequently, we reasoned that treatment of thioredoxin-fused NT-proCNP(1-81) would allow us to retrieve full-length NT-proCNP(1-81) without undue processing at the LKGDR(201) site since this non-target site would now be located internally about 36 residues away from the C-terminus and hence not be hydrolyzed efficiently. Surprisingly, ESI-MS data showed that the LKGDR site in thioredoxin-fused human NT-proCNP(1-81) was still very efficiently cleaved and revealed a new but slow hydrolysis site with the sequence RVDTK/SRAAW to yield a peptide consistent with NT-proCNP(58-81). The evidence obtained from these experiments led us to postulate that efficient cleavage at the non-target LKGDR(201) site was not merely influenced by steric constraints but also by the sequence context downstream of the scissile bond. Hence, we constructed variants of thioredoxin-mouse NT-proCNP(1-50) where SRLLR residues (i.e. those immediately downstream from the LKGDR(201) site in NT-proCNP(1-50)) were systematically added one at a time downstream of the internal DDDDK(156) site. To evaluate the relative effects of site accessibility and downstream sequence context on the efficiency of enterokinase cleavage, we have also replaced the native LKGDR(201) sequence with DDDDK(201). Our results showed that incremental addition of SRLLR residues led to a steady increase in the rate of hydrolysis at DDDDK(156). Further variants comprising DDDDK(156)SS, DDDDK(156)SD and DDDDK(156)RR showed that the minimal critical determinants for enhanced enterokinase cleavage are serine in the P1' position followed by a serine or a basic residue, lysine or arginine, in the P2' position. Our data provided conclusive evidence that the influence of downstream sequences on recombinant light chain enterokinase activity was greater than accessibility of the target site at the terminus region of the protein. We further showed that the catalytic efficiency of the native holoenzyme was influenced primarily by residues on the N-terminal side of the scissile bond while being neutral to residues on the C-terminal side. Finally, we found that cleavage of all nine fusion proteins reflects accurate hydrolysis at the DDDDK(156) and DDDDK(201) sites when recombinant light chain enterokinase was used while non-specific processing at secondary sites were observed when these fusion proteins were treated with the native holoenzyme.

Published

2007

40. [Refolding of the fusion protein of recombinant enterokinase light chain rEKL].

Author

Yi JH and Zhang YX

Subjects

Escherichia coli genetics, Recombinant Fusion Proteins isolation & purification, Enteropeptidase chemistry, Protein Folding, Recombinant Fusion Proteins chemistry

Abstract

The fusion protein of enterokinase light chain, DsbA-rEKL, was expressed mainly in inclusion body in E. coli. The recombinant bacteria was fermented to high density, with high expression of the fusion protein. After being washed with 0.5% Triton X-100 and 4mol/L urea, the inclusion body was dissolved in 6mol/L guanidine and 100mmol/L DTP, derivatized by cystine and refolded by pulse refolding. The strategy of pulse refolding involved the addition of 0.03mg/mL of fusion protein until its final concentration reached 0.3mg/mL. The refolded protein was autocleaved and the active EKL molecule was released after adding 2mmol/L CaCl2. Using the two-step purification processes of IDA-Sepharose chromatography and Q-Sepharose chromatography, the purity of rEKL was found to be above 95%, with a high activity to cleave the recombinant reteplase fusion protein Trx-rPA. The yield of purified rEKL was more than 60mg/L of cultures. As a result, the therapeutic proteins like rPA could be produced on a large-scale in a way such as expressed in the form of fusion proteins.

Published

2006

41. Compatible solutes as protectants for zymogens against proteolysis.

Author

Kolp S, Pietsch M, Galinski EA, and Gütschow M

Subjects

Amino Acids, Diamino chemistry, Amino Acids, Diamino pharmacology, Animals, Betaine chemistry, Betaine pharmacology, Catalysis drug effects, Cattle, Chymotrypsinogen metabolism, Endopeptidases metabolism, Enteropeptidase chemistry, Enteropeptidase metabolism, Enzyme Activation drug effects, Enzyme Precursors metabolism, Enzyme Stability, Molecular Structure, Swine, Trypsin chemistry, Trypsin metabolism, Trypsinogen metabolism, Chymotrypsinogen chemistry, Endopeptidases chemistry, Enzyme Precursors chemistry, Trypsinogen chemistry

Abstract

Compatible solutes are small organic osmoprotectants that have the capability to stabilize proteins. In coupled assays, the effect of the solutes ectoine, hydroxyectoine and betaine on the activation of the zymogens trypsinogen and chymotrypsinogen, catalyzed by enteropeptidase and trypsin, respectively, was studied. To different extents, all solutes protected the zymogens against activation. Ectoine (800 mM) was the most potent solute in reducing the formation of trypsin to 4% of the control value and of chymotrypsin to 23%. In separate experiments, the ability of the solutes to preserve proteolytic activity during incubation was investigated. After 4 h, trypsin and chymotrypsin completely lost their activity, but in the presence of ectoine, approximately 50% residual activity was maintained. It is proposed that a conformational shift of the protein towards folded, native-like states induced by preferential exclusion of the solute is responsible for the stabilizing and chaperone-like effects.

Published

2006

42. Tyrosine-based "activatable pro-tag": enzyme-catalyzed protein capture and release.

Author

Lewandowski AT, Small DA, Chen T, Payne GF, and Bentley WE

Subjects

Chemical Precipitation, Chitosan chemistry, Chitosan metabolism, Chromatography, Affinity, Enteropeptidase chemistry, Enteropeptidase metabolism, Enzymes chemistry, Escherichia coli genetics, Glycoside Hydrolases chemistry, Green Fluorescent Proteins genetics, Green Fluorescent Proteins metabolism, Histidine genetics, Monophenol Monooxygenase chemistry, Monophenol Monooxygenase metabolism, Nickel chemistry, Oligopeptides genetics, Peptides genetics, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins metabolism, Biotechnology methods, Enzymes metabolism, Glycoside Hydrolases metabolism, Peptides metabolism, Recombinant Fusion Proteins isolation & purification

Abstract

Protein recovery is often achieved by a series of capture and release steps that often involve chromatographic binding and elution. We report an alternative, non-chromatographic, capture and release approach that employs enzymes and the stimuli-responsive polysaccharide chitosan. We capture our protein using the enzyme tyrosinase that oxidizes accessible tyrosine residues of the protein and "activates" these residues for covalent capture (i.e., conjugation) onto chitosan. Using fusions of green fluorescent protein (GFP) we observed that: (i) enzymatic activation is required for protein capture to chitosan; and (ii) capture is enhanced (approximately five-fold) by engineering the protein to have a penta-tyrosine fusion tag that provides additional accessible tyrosine residues for enzymatic activation. Because the fusion tag appears to be the primary site for capture, and capture requires activation, we designate penta-tyrosine as a "pro-tag." The captured GFP-chitosan conjugate possesses the pH-responsive solubility that is characteristic of chitosan. We exploit this pH-responsive solubility to facilitate purification of the captured protein. Two enzymatic methods were explored to release the captured GFP from the chitosan conjugate. The first method employs enterokinase (EK) to cleave the protein at an engineered EK-cleavage site. The second method employs chitosanase to hydrolyze the chitosan backbone. Using GFP as a model protein, we demonstrated that enzymatic capture and release provides a simple, non-chromatographic means to recover proteins directly from cell lysates.

Published

2006

43. Biochemical characterization of human enteropeptidase light chain.

Author

Gasparian ME, Ostapchenko VG, Dolgikh DA, and Kirpichnikov MP

Subjects

Animals, Calcium metabolism, Catalytic Domain, Cattle, Enteropeptidase antagonists & inhibitors, Enteropeptidase genetics, Enteropeptidase isolation & purification, Enzyme Activation, Enzyme Stability, Humans, Hydrogen-Ion Concentration, Kinetics, Protein Denaturation, Recombinant Proteins antagonists & inhibitors, Recombinant Proteins biosynthesis, Recombinant Proteins chemistry, Recombinant Proteins isolation & purification, Serine Proteinase Inhibitors chemistry, Sodium metabolism, Substrate Specificity, Enteropeptidase chemistry

Abstract

The synthetic gene encoding human enteropeptidase light chain (L-HEP) was cloned into plasmid pET-32a downstream from the gene of fusion partner thioredoxin immediately after the DNA sequence encoding the enteropeptidase recognition site. The fusion protein thioredoxin (Trx)/L-HEP was expressed in Escherichia coli BL21(DE3). Autocatalytic cleavage of the fusion protein and activation of recombinant L-HEP were achieved by solubilization of inclusion bodies and refolding of Trx/L-HEP fusion protein. The kinetic parameters of human and bovine enteropeptidases in the presence of different concentrations of Ca2+ and Na+ for cleavage of the specific substrate GD4K-na and nonspecific substrates such as small ester Z-Lys-SBzl and chromogenic substrates Z-Ala-X-Arg-pNA have been comparatively analyzed. It is demonstrated that positively charged ions increased the Michaelis constant (Km) for cleavage of specific substrate GD4K-na, while the catalytic constant (k(cat)) remained practically unchanged. L-HEP demonstrated secondary specificity to the chromogenic substrate Z-Ala-Phe-Arg-pNA with k(cat)/Km 260 mM(-1) x sec(-1). Enzymatic activity of L-HEP was suppressed by inhibitors of trypsin-like and cysteine (E-64), but not metallo-, amino-, or chymotrypsin-like proteinases. L-HEP was active over a broad range of pH (6-9) with optimum activity at pH 7.5, and it demonstrated high stability to different denaturing agents.

Published

2006

44. Effect of calcium ions on enteropeptidase catalysis.

Author

Mikhailova AG, Likhareva VV, Prudchenko IA, and Rumsh LD

Subjects

Animals, Binding Sites, Catalysis drug effects, Cations, Cattle, Enteropeptidase chemistry, Enteropeptidase genetics, Hydrogen-Ion Concentration, Hydrolysis, Kinetics, Recombinant Fusion Proteins metabolism, Trypsin metabolism, Trypsinogen metabolism, Calcium pharmacology, Enteropeptidase metabolism, Enzyme Activation drug effects

Abstract

The effects of calcium ions on hydrolysis of low molecular weight substrates catalyzed by different forms of enteropeptidase were studied. A method for determining activity of truncated enteropeptidase preparations lacking a secondary trypsinogen binding site and displaying low activity towards trypsinogen was developed using N-alpha-benzyloxycarbonyl-L-lysine thiobenzyl ester (Z-Lys-S-Bzl). The kinetic constants for hydrolysis of this substrate at pH 8.0 and 25 degrees C were determined for natural enteropeptidase (K(m) 59.6 microM, k(cat) 6660 min(-1), k(cat)/K(m) 111 microM(-1) x min(-1)), as well as for enteropeptidase preparation with deleted 118-783 fragment of the heavy chain (K(m) 176.9 microM, k(cat) 6694 min(-1), k(cat)/K(m) 37.84 microM(-1) x min(-1)) and trypsin (K(m) 56.0 microM, k(cat) 8280 min(-1), k(cat)/K(m) 147.86 microM(-1) x min(-1)). It was shown that the enzymes with trypsin-like primary active site display similar hydrolysis efficiency towards Z-Lys-S-Bzl. Calcium ions cause 3-fold activation of hydrolysis of the substrates of general type GD(4)K-X by the natural full-length enteropeptidase. In contrast, the hydrolysis of substrates with one or two Asp/Glu residues at P2-P3 positions is slightly inhibited by Ca2+. In the case of enteropeptidase light chain as well as the enzyme containing the truncated heavy chain (466-800 fragment), the activating effect of calcium ions was not detected for all the studied substrates. The results of hydrolysis experiments with synthetic enteropeptidase substrates GD(4)K-F(NO(2))G, G(5)DK-F(NO(2))G (where F(NO(2)) is p-nitrophenyl-L-phenylalanine residue), and GD(4)K-Nfa (where Nfa is beta-naphthylamide) demonstrate the possibility of regulation of undesired side hydrolysis using natural full-length enteropeptidase for processing chimeric proteins by means of calcium ions.

Published

2005

45. Expression and characterization of the carboxyl esterase Rv3487c from Mycobacterium tuberculosis.

Author

Zhang M, Wang JD, Li ZF, Xie J, Yang YP, Zhong Y, and Wang HH

Subjects

Amino Acid Sequence, Carboxylesterase chemistry, Carboxylesterase metabolism, Catalytic Domain genetics, Chromatography, Affinity, Cloning, Molecular, Detergents pharmacology, Enteropeptidase chemistry, Enzyme Stability drug effects, Escherichia coli genetics, Gene Expression genetics, Glutamic Acid genetics, Histidine genetics, Hydrogen-Ion Concentration, Kinetics, Molecular Sequence Data, Mutagenesis, Site-Directed, Mycobacterium tuberculosis genetics, Protein Structure, Tertiary, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Reverse Transcriptase Polymerase Chain Reaction, Sequence Homology, Amino Acid, Serine genetics, Temperature, Thioredoxins genetics, Carboxylesterase genetics, Mycobacterium tuberculosis enzymology, Recombinant Fusion Proteins biosynthesis

Abstract

Rv3487c (lipF), a member of the lipase family of Mycobacterium tuberculosis, is related to virulence of this pathogen. Real-time RT-PCR analysis indicated that Rv3487c was induced at low pH in M. tuberculosis cultured in vitro. The gene of Rv3487c was cloned and expressed as fusion protein in Escherichia coli. After removal of the N-terminal domain of the fusion partner by enterokinase treatment, the effect of pH, temperature, and detergents on the purified enzyme activity and stability was characterized. Rv3487c could efficiently hydrolyze short chain esters. The catalytic triad of Rv3487c consists of residues Ser90, Glu189, and His219 as demonstrated by amino acid sequence alignment, three-dimensional modeling, and site-directed mutagenesis.

Published

2005

46. Expression and preparation of recombinant hepcidin in Escherichia coli.

Author

Zhang H, Yuan Q, Zhu Y, and Ma R

Subjects

Amino Acid Sequence, Antimicrobial Cationic Peptides genetics, Bacillus subtilis drug effects, Cloning, Molecular, Enteropeptidase chemistry, Escherichia coli chemistry, Escherichia coli metabolism, Genetic Vectors genetics, Hepcidins, Imidazoles chemistry, Inclusion Bodies chemistry, Inclusion Bodies metabolism, Microbial Sensitivity Tests, Molecular Sequence Data, Oxidation-Reduction, Recombinant Fusion Proteins biosynthesis, Recombinant Fusion Proteins genetics, Recombinant Fusion Proteins isolation & purification, Antimicrobial Cationic Peptides biosynthesis, Antimicrobial Cationic Peptides isolation & purification, Escherichia coli genetics

Abstract

Hepcidin is a low-molecular-weight, highly disulfide bonded peptide relevant to small intestine iron absorption and body iron homeostasis. In this work, hepcidin was expressed in Escherichia coli as a 10.5 kDa fusion protein (His-hepcidin) with a N-terminal hexahistidine tag. The expressed His-hepcidin existed in the form of inclusion bodies and was purified by IMAC under denaturation condition. Since the fusion partner for hepcidin did not contain other cysteine residues, the formation of disulfide bonds was performed before the His-tag was removed. Then, the oxidized His-hepcidin monomer was separated from protein multimers through gel filtration. Following monomer refolding, hepcidin was cleaved from fusion protein by enterokinase and purified with reverse-phase chromatography. The recombinant hepcidin exhibited obvious antibacterial activity against Bacillus subtilis.

Published

2005

47. Preparation of recombinant thioredoxin fused N-terminal proCNP: Analysis of enterokinase cleavage products reveals new enterokinase cleavage sites.

Author

Liew OW, Ching Chong JP, Yandle TG, and Brennan SO

Subjects

Amino Acid Sequence, Animals, Binding Sites, Cloning, Molecular, Enteropeptidase chemistry, Escherichia coli genetics, Gene Expression Regulation, Humans, Mice, Molecular Sequence Data, Natriuretic Peptide, C-Type chemistry, Recombinant Fusion Proteins analysis, Recombinant Fusion Proteins chemistry, Recombinant Fusion Proteins genetics, Sequence Homology, Amino Acid, Spectrometry, Mass, Electrospray Ionization methods, Enteropeptidase metabolism, Natriuretic Peptide, C-Type analysis, Natriuretic Peptide, C-Type genetics, Thioredoxins chemistry

Abstract

C-type natriuretic peptide (CNP) acts as a paracrine hormone to dilate blood vessels and is also required for the growth of long bones. In vivo, CNP is produced by cleavage from the C-terminal end of a larger proCNP peptide. The remaining N-terminal proCNP fragment (NT-proCNP) escapes into the circulation where its concentration is much higher than that of CNP due presumably to a lower clearance rate. Our strategy to obtain large quantities of pure NT-proCNP for further physiological investigations was to express it as a fusion protein with His(6)-tagged thioredoxin followed by cleavage using enterokinase to yield NT-proCNP alone. We have successfully designed and artificially synthesized the coding sequence specifying both mouse and human NT-proCNP with built-in codon bias towards Escherichia coli codon preference. An enterokinase recognition sequence was incorporated immediately upstream of the NT-proCNP coding sequence to allow the fusion protein to be cleaved without leaving any extra residues on the NT-proCNP peptide. High levels of fusion proteins were obtained, constituting 50-58% of total bacterial proteins. Greater than 90% of recombinant thioredoxin/NT-proCNP was expressed in the soluble form and purified to near homogeneity in a single chromatographic step using nickel as the metal ion in IMAC. A time course analysis of the products released from enterokinase cleavage of the recombinant proteins by ESI-MS revealed three sensitive secondary cleavage sites: two were located on vector-associated sequences linking the thioredoxin moiety and NT-proCNP, and one at the C-terminal end of NT-proCNP. Clearly, substrate specificity of both the native and recombinant forms of enterokinase for the recognition sequence DDDDK was by no means exclusive. Hydrolysis at the unexpected LKGDR site located towards the carboxyl end on NT-proCNP was significantly more efficient than at the internally sited DDDDK target sequence. However, when this same sequence was sited internally replacing the DDDDK in another construct of thioredoxin/mouse NT-proCNP, it was found to be poorly processed by enterokinase. Our results showed that non-target sequences can be preferentially recognized over the canonical DDDDK sequence when located accessibly at the ends of proteins.

Published

2005

48. Expression of recombinant chinese bovine enterokinase catalytic subunit in P. pastoris and its purification and characterization.

Author

Fang L, Sun QM, and Hua ZC

Subjects

Animals, Catalytic Domain, Cattle, Electrophoresis, Polyacrylamide Gel, Enteropeptidase chemistry, Enteropeptidase isolation & purification, Enteropeptidase metabolism, Plasmids, Recombinant Proteins chemistry, Recombinant Proteins genetics, Recombinant Proteins isolation & purification, Recombinant Proteins metabolism, Chromatography, Affinity methods, Enteropeptidase genetics, Pichia genetics

Abstract

Enterokinase is a tool protease widely utilized in the cleavage of recombinant fusion proteins. cDNA encoding the catalytic subunit of Chinese bovine enterokinase (EKL) was amplified by PCR and then fused to the 3' end of prepro secretion signal peptide gene of alpha-mating factor from Saccharomyces cerevisiae to get the alpha-MF signal-EKL-His6 encoding gene by PCR. Then the whole coding sequence was cloned into the integrative plasmid pAO815 under the control of a methanol-inducible promoter and transformed GS115 methylotrophic strain of Pichia pastoris. Secreted expression of recombinant EKL-His6 was attained by methanol induction and its molecular weight is 43 kD. Because of the existence of His6-tag, EKL-His6 was easily purified from P. pastoris fermentation supernatant by using Ni2+ affinity chromatography and the yield is 5.4 mg per liter of fermentation culture. This purified EKL-His6 demonstrates excellent cleavage activity towards fusion protein containing EK cleavage site.

Published

2004

49. High-level secretory production of recombinant bovine enterokinase light chain by Pichia pastoris.

Author

Peng L, Zhong X, Ou J, Zheng S, Liao J, Wang L, and Xu A

Subjects

Animals, Carbon metabolism, Cattle, Enteropeptidase chemistry, Enzyme Activation, Hydrogen-Ion Concentration, Methanol, Mutagenesis, Site-Directed genetics, Pichia growth & development, Recombinant Proteins biosynthesis, Enteropeptidase biosynthesis, Enteropeptidase genetics, Pichia enzymology, Pichia genetics, Protein Engineering methods

Abstract

Enterokinase (EC 3.4.21.9) is a serine proteinase with a specific digest sequence (Asp)4-Lys in the duodenum. Its high specificity for the recognition site makes enterokinase (EK) a useful tool for an in vitro cleavage of fusion proteins. In this work, an active bovine enterokinase light chain (EK(L)) was produced in secretory form by a recombinant strain of the methylotrophic yeast Pichia pastoris. The influences of methanol utilization phenotype of the host strain, induction pH, and carbon source on the recombinant production were studied. The production of recombinant EK(L) by Mut(s) strain was much higher than that by Mut+ strain. When inducted at pH 6.0, on a glycerol/methanol medium, the concentration of recombinant EK(L) (rEK(L)) reached 350 mg l(-1), which was 20-fold higher than that reported previously. The recombinant EK(L) was purified in a simple procedure on the anion exchange chromatography and 15 mg pure active EK(L) were obtained from 100 ml culture broth supernatant. The specific activity of purified rEK(L) was approximately 9000 u mg(-1). To facilitate purification and removal of rEKL after cleavage of fusion protein, the C-terminal His-tagged EK(L) (EK(L)/His) was also expressed in P. pastoris, and this His-tagged EK(L) exhibited a similar enzymatic activity to the untagged EK(L).

Published

2004

50. Evolution of trypsinogen activation peptides.

Author

Chen JM, Kukor Z, Le Maréchal C, Tóth M, Tsakiris L, Raguénès O, Férec C, and Sahin-Tóth M

Subjects

Amino Acid Sequence, Animals, Arginine chemistry, Cations chemistry, Enteropeptidase chemistry, Enzyme Activation, Evolution, Molecular, Fishes, Hydrolysis, Lysine chemistry, Molecular Sequence Data, Mutagenesis, Site-Directed, Mutation, Peptides chemistry, Plasmids metabolism, Recombinant Proteins chemistry, Time Factors, Trypsinogen chemistry, Oligopeptides chemistry, Oligopeptides genetics

Abstract

The activation peptide of mammalian trypsinogens contains a highly conserved tetra-aspartate sequence (D19-D20-D21-D22) preceding the K23-I24 scissile peptide bond, which is hydrolyzed as the first step in the activation process. Here, we examined the evolution and function of trypsinogen activation peptides through integrating functional characterization of disease-associated mutations with comparative genomic analysis. Activation properties of three chronic pancreatitis-associated activation peptide mutants (the novel D19A and the previously reported D22G and K23R) were simultaneously analyzed, for the first time, in the context of recombinant human cationic trypsinogen. A dramatic increase in autoactivation of cationic trypsinogen was observed in all three mutants, with D22G and K23R exhibiting the most marked increases. The physiological activator enteropeptidase activated the D19A mutant normally, activated the D22G mutant very poorly, and stimulated activation of the K23R mutant. The biochemical and structural data, taken together with a comprehensive sequence comparison, indicates that the tetra-aspartate sequence in mammalian trypsinogen activation peptides has evolved not only for optimal enteropeptidase recognition in the duodenum but also for efficient inhibition of trypsinogen autoactivation within the pancreas. Moreover, the use of lysine instead of arginine at the P1 position of activation peptides also has an advantageous effect against trypsinogen autoactivation. Finally, fixed substitutions in the key residues of the trypsinogen activation peptide may suggest the evolution of new functions unrelated to digestion, as found in the group III trypsinogens of cold-adapted fishes.

Published

2003