Your search keyword '"Uno Carlsson"' showing total 93 results

1. Metaproteomics-guided selection of targeted enzymes for bioprospecting of mixed microbial communities

Author

Jutta Speda, Bengt-Harald Jonsson, Uno Carlsson, and Martin Karlsson

Subjects

Biofuel, Metaproteome, Bioprospecting, Microbial community, Enzyme discovery, Induction, Fuel, TP315-360, Biotechnology, TP248.13-248.65

Abstract

Abstract Background Hitherto, the main goal of metaproteomic analyses has been to characterize the functional role of particular microorganisms in the microbial ecology of various microbial communities. Recently, it has been suggested that metaproteomics could be used for bioprospecting microbial communities to query for the most active enzymes to improve the selection process of industrially relevant enzymes. In the present study, to reduce the complexity of metaproteomic samples for targeted bioprospecting of novel enzymes, a microbial community capable of producing cellulases was maintained on a chemically defined medium in an enzyme suppressed metabolic steady state. From this state, it was possible to specifically and distinctively induce the desired cellulolytic activity. The extracellular fraction of the protein complement of the induced sample could thereby be purified and compared to a non-induced sample of the same community by differential gel electrophoresis to discriminate between constitutively expressed proteins and proteins upregulated in response to the inducing substance. Results Using the applied approach, downstream analysis by mass spectrometry could be limited to only proteins recognized as upregulated in the cellulase-induced sample. Of 39 selected proteins, the majority were found to be linked to the need to degrade, take up, and metabolize cellulose. In addition, 28 (72%) of the proteins were non-cytosolic and 17 (44%) were annotated as carbohydrate-active enzymes. The results demonstrated both the applicability of the proposed approach for identifying extracellular proteins and guiding the selection of proteins toward those specifically upregulated and targeted by the enzyme inducing substance. Further, because identification of interesting proteins was based on the regulation of enzyme expression in response to a need to hydrolyze and utilize a specific substance, other unexpected enzyme activities were able to be identified. Conclusions The described approach created the conditions necessary to be able to select relevant extracellular enzymes that were extracted from the enzyme-induced microbial community. However, for the purpose of bioprospecting for enzymes to clone, produce, and characterize for practical applications, it was concluded that identification against public databases was not sufficient to identify the correct gene or protein sequence for cloning of the identified novel enzymes.

Published

2017

2. Conformational effects on the circular dichroism of Human Carbonic Anhydrase II: a multilevel computational study.

Author

Tatyana G Karabencheva-Christova, Uno Carlsson, Kia Balali-Mood, Gary W Black, and Christo Z Christov

Subjects

Medicine, Science

Abstract

Circular Dichroism (CD) spectroscopy is a powerful method for investigating conformational changes in proteins and therefore has numerous applications in structural and molecular biology. Here a computational investigation of the CD spectrum of the Human Carbonic Anhydrase II (HCAII), with main focus on the near-UV CD spectra of the wild-type enzyme and it seven tryptophan mutant forms, is presented and compared to experimental studies. Multilevel computational methods (Molecular Dynamics, Semiempirical Quantum Mechanics, Time-Dependent Density Functional Theory) were applied in order to gain insight into the mechanisms of interaction between the aromatic chromophores within the protein environment and understand how the conformational flexibility of the protein influences these mechanisms. The analysis suggests that combining CD semi empirical calculations, crystal structures and molecular dynamics (MD) could help in achieving a better agreement between the computed and experimental protein spectra and provide some unique insight into the dynamic nature of the mechanisms of chromophore interactions.

Published

2013

3. Transient conformational remodeling of folding proteins by GroES—individually and in concert with GroEL

Author

Uno Carlsson, Laila Villebeck, Daniel Sjölander, Per Hammarström, Satish Babu Moparthi, and Bengt-Harald Jonsson

Subjects

Biophysics, Chaperone, macromolecular substances, Biochemistry, MreB, Chaperonin, Opinion Paper, Biologiska vetenskaper, Protein folding, Carbonic anhydrase, FRET, Molten globule, biology, Kemi, Cell Biology, GroES, Biological Sciences, GroEL, enzymes and coenzymes (carbohydrates), Chaperone (protein), Chemical Sciences, biological sciences, Foldase, biology.protein, bacteria

Abstract

The commonly accepted dogma of the bacterial GroE chaperonin system entails protein folding mediated by cycles of several ATP-dependent sequential steps where GroEL interacts with the folding client protein. In contrast, we herein report GroES-mediated dynamic remodeling (expansion and compression) of two different protein substrates during folding: the endogenous substrate MreB and carbonic anhydrase (HCAII), a well-characterized protein folding model. GroES was also found to influence GroEL binding induced unfolding and compression of the client protein underlining the synergistic activity of both chaperonins, even in the absence of ATP. This previously unidentified activity by GroES should have important implications for understanding the chaperonin mechanism and cellular stress response. Our findings necessitate a revision of the GroEL/ES mechanism. Electronic supplementary material The online version of this article (doi:10.1007/s12154-013-0106-5) contains supplementary material, which is available to authorized users.

Published

2013

4. Assessment of sample preparation methods for metaproteomics of extracellular proteins

Author

Uno Carlsson, Jutta Speda, Martin Karlsson, and Mikaela A. Johansson

Subjects

0301 basic medicine, Proteomics, Two-dimensional gel electrophoresis, Chromatography, Bacteria, Microorganism, 030106 microbiology, Extraction (chemistry), Biophysics, Cell Biology, Fractionation, Biology, Biochemistry, Specimen Handling, 03 medical and health sciences, 030104 developmental biology, Bacterial Proteins, Metaproteomics, Extracellular, Sample preparation, Electrophoresis, Gel, Two-Dimensional, Molecular Biology

Abstract

Enzyme discovery in individual strains of microorganisms is compromised by the limitations of pure culturing. In principle, metaproteomics allows for fractionation and study of different parts of the protein complement but has hitherto mainly been used to identify intracellular proteins. However, the extracellular environment is also expected to comprise a wealth of information regarding important proteins. An absolute requirement for metaproteomic studies of protein expression, and irrespective of downstream methods for analysis, is that sample preparation methods provide clean, concentrated and representative samples of the protein complement. A battery of methods for concentration, extraction, precipitation and resolubilization of proteins in the extracellular environment of a constructed microbial community was assessed by means of 2D gel electrophoresis and image analysis to elucidate whether it is possible to make the extracellular protein complement available for metaproteomic analysis. Most methods failed to provide pure samples and therefore negatively influenced protein gel migration and gel background clarity. However, one direct precipitation method (TCA-DOC/acetone) and one extraction/precipitation method (phenol/methanol) provided complementary high quality 2D gels that allowed for high spot detection ability and thereby also spot detection of less abundant extracellular proteins.

Published

2016

5. Differential conformational modulations of MreB folding upon interactions with GroEL/ES and TRiC chaperonin components

Author

Renaud Vincentelli, Jérôme Wenger, Uno Carlsson, Bengt-Harald Jonsson, Satish Babu Moparthi, Per Hammarström, MOSAIC (MOSAIC), Institut FRESNEL (FRESNEL), Aix Marseille Université (AMU)-École Centrale de Marseille (ECM)-Centre National de la Recherche Scientifique (CNRS)-Aix Marseille Université (AMU)-École Centrale de Marseille (ECM)-Centre National de la Recherche Scientifique (CNRS), Department of Physics, Chemistry and Biology [Linköping] (IFM), Linköping University (LIU), Architecture et fonction des macromolécules biologiques (AFMB), Institut National de la Recherche Agronomique (INRA)-Aix Marseille Université (AMU)-Centre National de la Recherche Scientifique (CNRS), European Project: 278242,EC:FP7:ERC,ERC-2011-StG_20101014,EXTENDFRET(2012), Centre National de la Recherche Scientifique (CNRS)-École Centrale de Marseille (ECM)-Aix Marseille Université (AMU)-Centre National de la Recherche Scientifique (CNRS)-École Centrale de Marseille (ECM)-Aix Marseille Université (AMU), and Centre National de la Recherche Scientifique (CNRS)-Aix Marseille Université (AMU)-Institut National de la Recherche Agronomique (INRA)

Subjects

0301 basic medicine, Models, Molecular, Protein Folding, Protein Conformation, Biophysics, macromolecular substances, Biology, MreB, Article, Chaperonin, 03 medical and health sciences, Protein structure, Chaperonin 10, Escherichia coli, Fluorescence Resonance Energy Transfer, [SPI.NANO]Engineering Sciences [physics]/Micro and nanotechnologies/Microelectronics, Actin, MreB protein, [PHYS.PHYS.PHYS-OPTICS]Physics [physics]/Physics [physics]/Optics [physics.optics], Multidisciplinary, 030102 biochemistry & molecular biology, Escherichia coli Proteins, Fluorescence Resonance Energy Transfer FRET, GroES, Chaperonin 60, GroEL, Biofysik, Actins, Single Molecule Imaging, Cell biology, Protein Structure, Tertiary, enzymes and coenzymes (carbohydrates), 030104 developmental biology, Förster resonance energy transfer, Mutation, biological sciences, [SPI.OPTI]Engineering Sciences [physics]/Optics / Photonic, bacteria, Protein folding, sense organs, Chaperonin Containing TCP-1, Protein Binding

Abstract

Here, we study and compare the mechanisms of action of the GroEL/GroES and the TRiC chaperonin systems on MreB client protein variants extracted from E. coli. MreB is a homologue to actin in prokaryotes. Single-molecule fluorescence correlation spectroscopy (FCS) and time-resolved fluorescence polarization anisotropy report the binding interaction of folding MreB with GroEL, GroES and TRiC. Fluorescence resonance energy transfer (FRET) measurements on MreB variants quantified molecular distance changes occurring during conformational rearrangements within folding MreB bound to chaperonins. We observed that the MreB structure is rearranged by a binding-induced expansion mechanism in TRiC, GroEL and GroES. These results are quantitatively comparable to the structural rearrangements found during the interaction of beta-actin with GroEL and TRiC, indicating that the mechanism of chaperonins is conserved during evolution. The chaperonin-bound MreB is also significantly compacted after addition of AMP-PNP for both the GroEL/ES and TRiC systems. Most importantly, our results showed that GroES may act as an unfoldase by inducing a dramatic initial expansion of MreB (even more than for GroEL) implicating a role for MreB folding, allowing us to suggest a delivery mechanism for GroES to GroEL in prokaryotes. Funding Agencies|European Commission [FP7-ICT-2011-7, ERC StG 278242]; Goran Gustafsson Foundation; Swedish Alzheimer Foundation

Published

2016

6. A nonessential role for Arg 55 in cyclophilin18 for catalysis of proline isomerization during protein folding

Author

Satish Babu Moparthi, Uno Carlsson, and Per Hammarström

Subjects

Protein Folding, Stereochemistry, Isomerase, Arginine, Protein Engineering, Carbonic Anhydrase II, Biochemistry, Isomerism, Catalytic Domain, Cyclosporin a, Escherichia coli, Humans, Molecular Biology, Cyclophilin, biology, Chemistry, Active site, Protein engineering, Folding (chemistry), Kinetics, For the Record, Mutation, Cyclosporine, biology.protein, Protein folding, Erratum, Peptides, Cyclophilin A, Isomerization

Abstract

The protein folding process is often in vitro rate-limited by slow cis-trans proline isomerization steps. Importantly, the rate of this process in vivo is accelerated by prolyl isomerases (PPIases). The archetypal PPIase is the human cyclophilin 18 (Cyp18 or CypA), and Arg 55 has been demonstrated to play a crucial role when studying short peptide substrates in the catalytic action of Cyp18 by stabilizing the transition state of isomerization. However, in this study we show that a R55A mutant of Cyp18 is as efficient as the wild type to accelerate the refolding reaction of human carbonic anhydrase II (HCA II). Thus, it is evident that the active-site located Arg 55 is not required for catalysis of the rate-limiting prolyl cis-trans isomerization steps during the folding of a protein substrate as HCA II. Nevertheless, catalysis of cis-trans proline isomerization in HCA II occurs in the active-site of Cyp18, since binding of the inhibitor cyclosporin A abolishes rate acceleration of the refolding reaction. Obviously, the catalytic mechanisms of Cyp18 can differ when acting upon a simple model peptide, four residues long, with easily accessible Pro residues compared with a large protein molecule undergoing folding with partly or completely buried Pro residues. In the latter case, the isomerization kinetics are significantly slower and simpler mechanistic factors such as desolvation and/or strain might operate during folding-assisted catalysis, since binding to the hydrophobic active site is still a prerequisite for catalysis.

Published

2009

7. A conformationally isoformic thermophilic protein with high kinetic unfolding barriers

Author

Uno Carlsson, Ian A. Nicholls, Martin Karlsson, Rajesh Mishra, Linus Olofsson, and Per Hammarström

Subjects

Models, Molecular, Guanidinium chloride, Protein Folding, Prions, Protein Conformation, Protein Renaturation, Kinetics, Supramolecular chemistry, Thermoanaerobacter, Saccharomyces cerevisiae, Cellular and Molecular Neuroscience, chemistry.chemical_compound, Urea, Molecular Biology, Guanidine, Alcohol dehydrogenase, Pharmacology, biology, Chemistry, Thermophile, Alcohol Dehydrogenase, Cell Biology, Isoenzymes, Folding (chemistry), Crystallography, Cross-Linking Reagents, Models, Chemical, biological sciences, biology.protein, Unfolded protein response, Thermodynamics, Molecular Medicine, Dimerization

Abstract

The basis for the stability of thermophilic proteins is of fundamental interest for extremophile biology. We investigated the folding and unfolding processes of the homotetrameric Thermoanaerobacter brockii alcohol dehydrogenase (TBADH). TBADH subunits were 4.8 kcal/mol less stable towards guanidinium chloride (GdmCl) unfolding compared to urea, indicating ionic modulation of TBADH stability. Strongly denaturing conditions promoted mono-exponential unfolding kinetics with linear dependence on denaturant concentration. Here TBADH unfolded >40-fold slower when extrapolated from urea as compared to GdmCl unfolding. A marked unfolding hysteresis was shown when comparing refolding and unfolding in urea. An unusual biphasic unfolding trajectory with an exceptionally slow phase at intermediate concentrations of GdmCl and urea was also observed. We advocate that TBADH forms two distinctly different tetrameric isoforms, and likely an ensemble of native states. This unusual supramolecular folding behavior has been shown responsible for formation of amyloidotic yeast prion strains and can have functional importance for TBADH.

Published

2008

8. Liquid–Solid Interface: Protein Stability on Conformational Changes

Author

Martin Karlsson and Uno Carlsson

Subjects

Protein stability, Chemical engineering, Interface (Java), Chemistry, Liquid solid

Published

2015

9. Reduction of Irreversible Protein Adsorption on Solid Surfaces by ProteinEngineering for IncreasedStability

Author

Johan Ekeroth, Uno Carlsson, Martin Karlsson, and Hans Elwing

Subjects

Protein Folding, Infrared Rays, Protein Conformation, Kinetics, Protein Engineering, Carbonic Anhydrase II, Biochemistry, Adsorption, Phase (matter), Desorption, Electrochemistry, Humans, Denaturation (biochemistry), Surface plasmon resonance, Molecular Biology, Chromatography, Chemistry, Water, Cell Biology, Protein engineering, Molecular Weight, Chemical engineering, Hydrophobic and Hydrophilic Interactions, Protein adsorption

Abstract

The influence of protein stability on the adsorption and desorption behavior to surfaces with fundamentally different properties (negatively charged, positively charged, hydrophilic, and hydrophobic) was examined by surface plasmon resonance measurements. Three engineered variants of human carbonic anhydrase II were used that have unchanged surface properties but large differences in stability. The orientation and conformational state of the adsorbed protein could be elucidated by taking all of the following properties of the protein variants into account: stability, unfolding, adsorption, and desorption behavior. Regardless of the nature of the surface, there were correlation between (i) the protein stability and kinetics of adsorption, with an increased amplitude of the first kinetic phase of adsorption with increasing stability; (ii) the protein stability and the extent of maximally adsorbed protein to the actual surface, with an increased amount of adsorbed protein with increasing stability; (iii) the protein stability and the amount of protein desorbed upon washing with buffer, with an increased elutability of the adsorbed protein with increased stability. All of the above correlations could be explained by the rate of denaturation and the conformational state of the adsorbed protein. In conclusion, protein engineering for increased stability can be used as a strategy to decrease irreversible adsorption on surfaces at a liquid-solid interface.

Published

2005

10. Activity, Folding, Misfolding, and Aggregation in Vitro of the Naturally Occurring Human Tissue Factor Mutant R200W

Author

Anna Herland, Karin Carlsson, Jimmy Wiréhn, Egon Persson, Uno Carlsson, Magdalena Svensson, and Per Hammarström

Subjects

Amyloid, Protein Denaturation, Protein Folding, Mutant, Population, Factor VIIa, Plasma protein binding, Biology, Arginine, Biochemistry, Anilino Naphthalenesulfonates, Substrate Specificity, Thromboplastin, Tissue factor, Nephelometry and Turbidimetry, Mutant protein, Extracellular, Humans, Denaturation (biochemistry), Benzothiazoles, education, education.field_of_study, Genetic Carrier Screening, Tryptophan, Molecular biology, Kinetics, Thiazoles, Spectrometry, Fluorescence, Mutation, Biophysics, Protein folding, Extracellular Space, Protein Binding

Abstract

Tissue factor (TF), a small transmembrane receptor, binds factor VIIa (FVIIa), and the formed complex initiates blood coagulation by proteolytic activation of substrate factors IX and X. A naturally occurring mutation in the human TF gene was recently reported, where a single-base substitution results in an R200W mutation in the TF extracellular domain [Zawadzki, C., Preudhomme, C., Gaveriaux, V., Amouyel, P., and Jude, B. (2002) Thromb. Haemost. 87, 540-541]. This mutation appears to be associated with low monocyte TF expression and may protect against thrombosis but has not been associated with any pathological condition, and individuals who present the heterozygous trait appear healthy. Here, we report the activity, folding, and aggregation behavior of the R200W mutant of the 219-residue soluble extracellular domain of TF (sTF(R200W)) compared to that of the wild-type protein (sTF(wt)). No differences in stability or FVIIa cofactor activity but an impaired ability to promote FX activation at physiological conditions between the sTF(R200W) mutant and sTF(wt) were evident. Increased binding of 1-anilino-8-naphthalene-sulfonic acid (ANS) to sTF(R200W) indicated a population of partially folded intermediates during denaturation. sTF(R200W) showed a dramatically increased propensity for aggregate formation compared to sTF(wt) at mildly acidic pHs, with an increased rate of aggregation during conditions, promoting the intermediate state. The lowered pH resistance could explain the loss of sTF(R200W) in vivo because of aggregation of the mutant. The intrinsic structure of the sTF aggregates appears reminiscent of amyloid fibrils, as revealed by thioflavin T fluorescence, atomic force microscopy, and transmission electron microscopy. We conclude that the lowered activity for FX activation and the propensity of the mutant protein to misfold and aggregate will both contribute to decreased coagulation activity in TF(R200W) carriers, which could protect from thrombotic disease.

Published

2005

11. Denaturant-Assisted Formation of a Stabilizing Disulfide Bridge from Engineered Cysteines in Nonideal Conformations

Author

Uno Carlsson, Carin Karlsson, Lars-Göran Mårtensson, and Martin Karlsson

Subjects

Models, Molecular, Protein Denaturation, Protein Folding, Protein Conformation, Hydrochloride, Entropy, Carbonic anhydrase II, Protein Engineering, Carbonic Anhydrase II, Biochemistry, Structure-Activity Relationship, chemistry.chemical_compound, Leucine, Carbonic anhydrase, Enzyme Stability, Native state, Humans, Cysteine, Disulfides, Homology modeling, Guanidine, Alanine, biology, Neisseria gonorrhoeae, Crystallography, chemistry, Mutagenesis, Site-Directed, biology.protein, Electrophoresis, Polyacrylamide Gel, Software, Protein adsorption

Abstract

The engineered disulfide bridge A23C/L203C in human carbonic anhydrase II, inserted from homology modeling of Neisseria gonorrhoeae carbonic anhydrase, significantly stabilizes the native state of the protein. The inserted cysteine residues are placed in the interior of the structure, and because of the conformationally restrained localization, the protein is expressed in the reduced state and the cysteines are not readily oxidized. However, upon exposure to low concentrations of denaturant (0.6 M guanidine hydrochloride), corresponding to the lower part of the denaturation curve for the first unfolding transition, the oxidation rate of correctly formed disulfide bridges was markedly increased. By entropy estimations it appears that the increased flexibility, induced by the denaturant, enables the cysteines to find each other and hence to form the disulfide bridge. The outlined strategy of facilitating formation of disulfide bonds by addition of adjusted concentrations of a denaturant should be applicable to other proteins in which engineered cysteine residues are located in nonideal conformations. Moreover, a S99C/V242C variant was constructed, in which the cysteine residues are located on the surface. In this mutant the disulfide bridge was spontaneously formed and the native state was considerably stabilized (midpoint concentration of unfolding was increased from 1.0 to 1.4 M guanidine hydrochloride).

Published

2005

12. Unfolding a Folding Disease: Folding, Misfolding and Aggregation of the Marble Brain Syndrome-associated Mutant H107Y of Human Carbonic Anhydrase II

Author

Martin Karlsson, Per Hammarström, Karin Almstedt, Martin Lundqvist, Uno Carlsson, Jonas Carlsson, Bengt Persson, and Bengt-Harald Jonsson

Subjects

Models, Molecular, Protein Folding, Magnetic Resonance Spectroscopy, Chemistry, Circular Dichroism, Carbonic anhydrase II, Mutant, Brain Diseases, Metabolic, Inborn, Carbonic Anhydrase II, Protein tertiary structure, Molten globule, chemistry.chemical_compound, Amino Acid Substitution, Biochemistry, Structural Biology, Mutation, Native state, Humans, Protein folding, Denaturation (biochemistry), Guanidine, Molecular Biology

Abstract

Most loss-of-function diseases are caused by aberrant folding of important proteins. These proteins often misfold due to mutations. The disease marble brain syndrome (MBS), known also as carbonic anhydrase II deficiency syndrome (CADS), can manifest in carriers of point mutations in the human carbonic anhydrase II (HCA II) gene. One mutation associated with MBS entails the His107Tyr substitution. Here, we demonstrate that this mutation is a remarkably destabilizing folding mutation. The loss-of-function is clearly a folding defect, since the mutant shows 64% of CO(2) hydration activity compared to that of the wild-type at low temperature where the mutant is folded. On the contrary, its stability towards thermal and guanidine hydrochloride (GuHCl) denaturation is highly compromised. Using activity assays, CD, fluorescence, NMR, cross-linking, aggregation measurements and molecular modeling, we have mapped the properties of this remarkable mutant. Loss of enzymatic activity had a midpoint temperature of denaturation (T(m)) of 16 degrees C for the mutant compared to 55 degrees C for the wild-type protein. GuHCl-denaturation (at 4 degrees C) showed that the native state of the mutant was destabilized by 9.2kcal/mol. The mutant unfolds through at least two equilibrium intermediates; one novel intermediate that we have termed the molten globule light state and, after further denaturation, the classical molten globule state is populated. Under physiological conditions (neutral pH; 37 degrees C), the His107Tyr mutant will populate the molten globule light state, likely due to novel interactions between Tyr107 and the surroundings of the critical residue Ser29 that destabilize the native conformation. This intermediate binds the hydrophobic dye 8-anilino-1-naphthalene sulfonic acid (ANS) but not as strong as the molten globule state, and near-UV CD reveals the presence of significant tertiary structure. Notably, this intermediate is not as prone to aggregation as the classical molten globule. As a proof of concept for an intervention strategy with small molecules, we showed that binding of the CA inhibitor acetazolamide increases the stability of the native state of the mutant by 2.9kcal/mol in accordance with its strong affinity. Acetazolamide shifts the T(m) to 34 degrees C that protects from misfolding and will enable a substantial fraction of the enzyme pool to survive physiological conditions.

Published

2004

13. Probing the interface between factor Xa and tissue factor in the quaternary complex tissue factor-factor VIIa-factor Xa-tissue factor pathway inhibitor

Author

Karin Carlsson, Uno Carlsson, Egon Persson, Magdalena Svensson, and Per-Ola Freskgård

Subjects

Models, Molecular, Lipoproteins, Factor VIIa, Biochemistry, Cofactor, Protein–protein interaction, Tissue factor, Tissue factor pathway inhibitor, Escherichia coli, Cloning, Molecular, Binding site, Protein Structure, Quaternary, Fluorescent Dyes, Binding Sites, biology, Mutagenesis, Genetic Variation, Molecular biology, Recombinant Proteins, Spectrometry, Fluorescence, Amino Acid Substitution, Coagulation, Factor Xa, Mutagenesis, Site-Directed, Phosphatidylcholines, biology.protein

Abstract

Blood coagulation is triggered by the formation of a complex between factor VIIa (FVIIa) and its cofactor, tissue factor (TF). TF-FVIIa is inhibited by tissue factor pathway inhibitor (TFPI) in two steps: first TFPI is bound to the active site of factor Xa (FXa), and subsequently FXa-TFPI exerts feedback inhibition of TF-FVIIa. The FXa-dependent inhibition of TF-FVIIa activity by TFPI leads to formation of the quaternary complex TF-FVIIa-FXa-TFPI. We used site-directed fluorescence probing to map part of the region of soluble TF (sTF) that interacts with FXa in sTF-FVIIa-FXa-TFPI. We found that the C-terminal region of sTF, including positions 163, 166, 200 and 201, is involved in binding to FXa in the complex, and FXa, most likely via its Gla domain, is also in contact with the Gla domain of FVIIa in this part of the binding region. Furthermore, a region that includes the N-terminal part of the TF2 domain and the C-terminal part of the TF1 domain, i.e. the residues 104 and 197, participates in the interaction with FXa in the quaternary complex. Moreover, comparisons of the interaction areas between sTF and FX(a) in the quaternary complex sTF-FVIIa-FXa-TFPI and in the ternary complexes sTF-FVII-FXa or sTF-FVIIa-FX demonstrated large similarities.

Published

2003

14. Dramatic Stabilization of the Native State of Human Carbonic Anhydrase II by an Engineered Disulfide Bond

Author

Martin Karlsson, Uno Carlsson, and Lars-Göran Mårtensson

Subjects

Protein Denaturation, Protein Folding, Stereochemistry, Carbonic anhydrase II, Mutant, Carbonic Anhydrase II, Biochemistry, Leucine, Carbonic anhydrase, Enzyme Stability, Mole, Native state, Humans, Cysteine, Disulfides, Guanidine, chemistry.chemical_classification, Alanine, Transition (genetics), biology, Circular Dichroism, Disulfide bond, Genetic Variation, Neisseria gonorrhoeae, Enzyme Activation, Enzyme, Amino Acid Substitution, chemistry, Mutagenesis, Site-Directed, biology.protein

Abstract

To find a disulfide pair that could stabilize the enzyme human carbonic anhydrase II (HCA II), we grafted the disulfide bridge from the related and unusually stable carbonic anhydrase form from Neisseria gonorrhoeae (NGCA) into the human enzyme. Thus, the two Cys residues at positions 23 and 203 were engineered into a pseudo-wild-type form of HCA II (C206S), giving the mutant C206S/A23C/L203C. The disulfide bond was not formed spontaneously. The native state of the reduced form of the mutant was markedly destabilized (2.9 kcal/mol) compared to that of HCA II. Formation of a disulfide bridge was achieved by treatment by oxidized glutathione. This led to a significant stabilization of the native conformation. Compared to HCA II the unfolding midpoint for the variant was increased from 0.9 to 1.7 M guanidine HCl, corresponding to a stabilization of 3.7 kcal/mol. This makes the human enzyme almost as stable as the model protein NGCA, for which the unfolding of the native state has a midpoint at 2.1 M guanidine HCl. The stabilized protein underwent, contrary to all other investigated variants of HCA II, an apparent two-state unfolding transition, as judged from intrinsic Trp fluorescence measurements. A molten-globule intermediate is nevertheless formed but is suppressed because of the high denaturant pressure it faces upon rupture of the native state.

Published

2002

15. The importance of being knotted: effects of the C-terminal knot structure on enzymatic and mechanical properties of bovine carbonic anhydrase II1

Author

M T Alam, Uno Carlsson, Atsushi Ikai, and Takafumi Yamada

Subjects

chemistry.chemical_classification, Circular dichroism, biology, Stereochemistry, Chemistry, Carbonic anhydrase II, Biophysics, Cell Biology, Biochemistry, Folding (chemistry), Crystallography, Enzyme, Affinity chromatography, Structural Biology, Carbonic anhydrase, Genetics, biology.protein, Molecular Biology, Conformational isomerism, Knot (mathematics)

Abstract

In order to better understand the contribution of the knotted folding pattern to the enzymatic and mechanical properties of carbonic anhydrases, we replaced Gln-253 of bovine carbonic anhydrase II with Cys, which allowed us to measure the mechanical strength of the protein against tensile deformation by avoiding knot tightening. The expressed protein, to our surprise, turned out to contain two conformational isomers, one capable of binding an enzymatic inhibitor and the other not, which led to their separation through affinity chromatography. In near- and far-UV circular dichroism and fluorescence spectra, the separated conformers were very similar to each other and to the wild-type enzyme, indicating that they both had native-like conformations. We describe new evidence which supports the notion that the difference between the two conformers is likely to be related to the completeness of the C-terminal knot formation.

Published

2002

16. Spin and Fluorescent Probing of the Binding Interface between Tissue Factor and Factor VIIa at Multiple Sites

Author

Mikael Lindgren, Uno Carlsson, Egon Persson, Magdalena Svensson, Per-Ola Freskgård, Maria Österlund, and Rikard Owenius

Subjects

chemistry.chemical_classification, Binding Sites, Surface Properties, Chemistry, Globular protein, Electron Spin Resonance Spectroscopy, Biophysics, Factor VIIa, Models, Biological, Fluorescence, Fluorescence spectroscopy, Thromboplastin, law.invention, Tissue factor, Crystallography, Amino Acid Substitution, law, Mutagenesis, Site-Directed, Spin Labels, Binding site, Structural rigidity, Electron paramagnetic resonance, Research Article, Fluorescent Dyes, Cysteine

Abstract

The specific complex between the extracellular part of tissue factor (sTF) and factor VIIa (FVIIa) was chosen as a model for studies of the binding interface between two interacting proteins. Six surface-exposed positions in sTF, residues known to contribute to the sTF-FVIIa interaction, were selected for cysteine mutation and site-directed labeling with spin and fluorescent probes. The binding interface was characterized by spectral data from electron paramagnetic resonance (EPR) and steady-state and time-domain fluorescence spectroscopy. The labels reported on compact local environments at positions 158 and 207 in the interface region between sTF and the γ-carboxyglutamic acid (Gla) domain of FVIIa, and at positions 22 and 140 in the interface region between sTF and the first epidermal growth factor-like (EGF1) domain of FVIIa. The tightness of the local interactions in these parts of the interface is similar to that seen in the interior of globular proteins. This was further emphasized by the reduced local polarity detected by the fluorescent label upon FVIIa binding, especially in the sTF-Gla region. There were indications of structural rigidity also at positions 45 and 94 in the interface region between sTF and the protease domain (PD) of FVIIa, despite the perturbed cofactor function of these sTF variants. The results of the present study indicate that the multi-probing approach enables comparison of the tightness and characteristics of interaction along the binding interface of a protein complex. This approach also increases the probability of acquiring reliable structural data that are descriptive of the wild-type proteins.

Published

2001

17. Probing Inhibitor-Induced Conformational Changes along the Interface between Tissue Factor and Factor VIIa

Author

Egon Persson, Uno Carlsson, Mikael Lindgren, Per-Ola Freskgård, Maria Österlund, Karin Carlsson, Magdalena Svensson, and Rikard Owenius

Subjects

Serine Proteinase Inhibitors, Protein Conformation, Stereochemistry, Allosteric regulation, Factor VIIa, Biochemistry, Amino Acid Chloromethyl Ketones, Thromboplastin, Tissue factor, Naphthalenesulfonates, Activated factor VII, medicine, Fluorescent Dyes, Binding Sites, Blood clotting, Chemistry, Sulfhydryl Reagents, Electron Spin Resonance Spectroscopy, Anticoagulants, Spectrometry, Fluorescence, medicine.anatomical_structure, Solubility, Mutagenesis, Site-Directed, Biophysics, Spin Labels, Protein Binding, Blood vessel

Abstract

Upon injury of a blood vessel, activated factor VII (FVIIa) forms a high-affinity complex with its allosteric regulator, tissue factor (TF), and initiates blood clotting. Active site-inhibited factor VIIa (FVIIai) binds to TF with even higher affinity. We compared the interactions of FVIIai and FVIIa with soluble TF (sTF). Six residues in sTF were individually selected for mutagenesis and site-directed labeling. The residues are distributed along the extensive binding interface, and were chosen because they are known to interact with the different domains of FVIIa. Fluorescent and spin probes were attached to engineered Cys residues to monitor local changes in hydrophobicity, accessibility, and rigidity in the sTF--FVIIa complex upon occupation of the active site of FVIIa. The results show that inhibition of FVIIa caused the structures around the positions in sTF that interact with the protease domain of FVIIa to become more rigid and less accessible to solvent. Thus, the presence of an active site inhibitor renders the interface in this region less flexible and more compact, whereas the interface between sTF and the light chain of FVIIa is unaffected by active site occupancy.

Published

2001

18. Protein Compactness Measured by Fluorescence Resonance Energy Transfer

Author

Malin Persson, Uno Carlsson, and Per Hammarström

Subjects

Carbonic anhydrase II, Cell Biology, Biochemistry, GroEL, Molten globule, chemistry.chemical_compound, Crystallography, Förster resonance energy transfer, chemistry, Native state, Denaturation (biochemistry), Protein folding, Guanidine, Molecular Biology

Abstract

Nine single-cysteine mutants were labeled with 5-(2-iodoacetylaminoethylamino)naphthalene-1-sulfonic acid, an efficient acceptor of Trp fluorescence in fluorescence resonance energy transfer. The ratio between the fluorescence intensity of the 5-(2-acetylaminoethylamino)naphthalene-1-sulfonic acid (AEDANS) moiety excited at 295 nm (Trp absorption) and 350 nn (direct AEDANS absorption) was used to estimate the average distances between the seven Trp residues in human carbonic anhydrase II (HCA II) and the AEDANS label, Guanidine HCl denaturation of the HCA II variants was also performed to obtain a curve that reflected the compactness of the protein at various stages of the unfolding, which could serve as a scale of the expansion of the protein. This approach was developed in this study and was used to estimate the compactness of HCA II during heat denaturation and interaction with GroEL, It was shown that thermally induced unfolding of HCA II proceeded only to the molten globule state. Reaching this state was sufficient to allow HCA II to bind to GroEL, and the volume of the molten globule intermediate increased similar to2.2-fold compared with that of the native state. GroEL-bound HCA II expands to a volume three to four times that of the native state (to similar to 117,000 Angstrom (3)), which correlates well with a stretched and loosened-up HCA II molecule in an enlarged GroEL cavity, Recently, we found that HCA II binding causes such an inflation of the GroEL molecule, and this probably represents the mechanism by which GroEL actively stretches its protein substrates apart (Hammarstrom, P., Persson, M., Owenius, R., Lindgren, M., and Carlsson, U. (2000) J. Biol. Chem. 275, 22832-22838), thereby facilitating rearrangement of misfolded structure.

Published

2001

19. Contribution of tryptophan residues to the CD spectrum of the extracellular domain of human tissue factor

Author

Uno Carlsson, Per-Ola Freskgård, and Dick Andersson

Subjects

chemistry.chemical_classification, Protein Folding, Circular dichroism, biology, Stereochemistry, Circular Dichroism, Tryptophan, Membrane Proteins, Peptide, Factor VIIa, Biochemistry, Protein Structure, Secondary, Protein tertiary structure, Cofactor, Protein Structure, Tertiary, Thromboplastin, Kinetics, Protein structure, chemistry, Mutagenesis, Site-Directed, biology.protein, Humans, Protein folding, Protein secondary structure

Abstract

The contribution to the circular dichroism (CD) spectrum made by each of the four Trp residues in the extracellular domain of human tissue factor, sTF (s designates soluble), was determined from difference CD spectra. The individual Trp CD spectra showed that all four residues contributed to the CD spectrum in almost the entire wavelength region investigated (180-305 nm). The sum of the individual spectra of each Trp residue in the near-UV region was qualitatively identical to the wild-type spectrum, clearly demonstrating that the Trp residues are the major contributors to the spectrum in this wavelength region. Trp CD bands interfere with the peptide bands in the far-UV region, leading to uncertainty in the predictions of the amounts of various types of secondary structure. Accordingly, the best prediction of secondary sTF structure content was achieved using a hypothetical Trp-free CD spectrum obtained after subtraction of all individual Trp spectra from the wild-type spectrum. The mutated Trp residues were also exploited as intrinsic probes to monitor the formation of local native-like tertiary structure by kinetic near-UV CD measurements. The global folding reaction was followed in parallel with a novel functional assay that registered the recovery of cofactor activity, i.e. stimulation of the amidolytic activity of Factor VIIa. From these measurements, it was found that sTF appears to regain FVIIa cofactor activity before the final side-chain packing of the Trp residues. The combined kinetic refolding results suggest that the compact asymmetric environments of the individual Trp residues in sTF are formed simultaneously, leading to the conclusion that the native tertiary structure of the whole protein is formed in a cooperative manner.

Published

2001

20. Localization of the Cl-/HCO3- Anion Exchanger Binding Site to the Amino-Terminal Region of Carbonic Anhydrase II

Author

Uno Carlsson, John W. Vince, and Reinhart A. F. Reithmeier

Subjects

Carbonic anhydrase II, Molecular Sequence Data, Lysine, Peptide Mapping, Biochemistry, Antiporters, Substrate Specificity, Mice, Chlorides, Animals, Humans, Amino Acid Sequence, Chloride-Bicarbonate Antiporters, Binding site, Peptide sequence, Histidine, Carbonic Anhydrases, Alanine, Binding Sites, Sheep, Chemistry, Ligand binding assay, Bicarbonate transport, Peptide Fragments, Rats, Bicarbonates, Mutagenesis, Site-Directed, Cattle, Rabbits, Chickens

Abstract

Human carbonic anhydrase II (CAII) possesses a binding site for an acidic motif (D887ADD) within the carboxyl-terminal region (Ct) of the human erythrocyte chloride/bicarbonate anion exchanger, AE1. In this study, the amino acid sequence comprising this AE1 binding site was localized to the first 17 residues of CAII, which form a basic patch on the surface of the protein. Truncation of the amino terminal of CAII by five residues resulted in a 3-fold reduction in the apparent affinity of the interaction with a GST fusion protein of the Ct of AE1 (GST-Ct) measured by a sensitive microtiter plate binding assay. Further amino-terminal truncation of CAII by 17 or 24 residues caused a loss of binding. The homologous isoform CAI does not bind AE1, despite having 60% sequence identity to CAII. One major difference between the two CA isoforms, within the amino-terminal region, is a high content of histidine residues in CAII (His3, -4, -10, -15, -17) not found in CAI. Mutation of pairs of these histidines (and one lysine) in CAII to the analogous residues in CAI (H3P/H4D or K9D/H10K or H15Q/H17S), or combinations of these various double mutants, did not greatly affect binding between GST-Ct and the mutant CAII. However, when all six of the targeted CAII residues were mutated to the corresponding sequence in CAI, binding of GST-Ct was lost. These results indicate that the AE1 binding site is located within the first 17 residues of CAII, and that the interaction is mediated by electrostatic interactions involving histidine and/or lysine residues. Further specificity for the interaction of AE1 and CAII is provided by a conserved leucine residue (L886) in AE1 that, when mutated to alanine, resulted in loss of GST-Ct binding to immobilized CAII. The binding of the basic amino-terminal region of CAII to an acidic Ct in AE1 provides a structural basis for linking bicarbonate transport across the cell membrane to intracellular bicarbonate metabolism.

Published

2000

21. Spectroscopic probing of the influence of calcium and the Gla domain on the interaction between the first EGF domain in factor VIIa and tissue factor

Author

Rikard Owenius, Magdalena Svensson, Uno Carlsson, Egon Persson, Maria Österlund, Mikael Lindgren, and Per-Ola Freskgård

Subjects

Gla domain, Residue (chemistry), Tissue factor, Coagulation, Biochemistry, chemistry, Binding energy, Biophysics, chemistry.chemical_element, Calcium, Fluorescence, Protein–protein interaction

Abstract

The binding of factor VIIa (FVIIa) to tissue factor (TF) initiates blood coagulation. The binary complex is dependent on Ca2+ binding to several sites in FVIIa and is maintained by multiple contacts distributed throughout the various domains. Although the contributions from various residues and domains, including the Ca2+ coordination, to the global binding energy have been characterized, their importance for specific local interactions is virtually unknown. To address this aspect, we have attached four spectroscopic probes to an engineered Cys residue replacing Phe140 in soluble TF (sTF). This allows the monitoring of local changes in hydrophobicity and rigidity upon complex formation at the interface between the first epidermal growth factor-like (EGF1) domain of FVIIa and sTF. The fluorescent labels used sense a more hydrophobic environment and the spin labels are dramatically immobilized when FVIIa binds sTF. The results obtained with a 4-carboxyglutamic acid (Gla)-domainless derivative of FVIIa indicate that the Gla domain has no or minimal influence on the interaction between EGF1 and sTF. However, there is a difference in local Ca2+ dependence between Gla-domainless and full-length FVIIa.

Published

2000

22. Adsorption of Human Carbonic Anhydrase II Variants to Silica Nanoparticles Occur Stepwise: Binding Is Followed by Successive Conformational Changes to a Molten-Globule-like State

Author

Uno Carlsson, Bengt-Harald Jonsson, Lars-Göran Mårtensson, and Martin Karlsson

Subjects

chemistry.chemical_classification, Conformational change, biology, Chemistry, Carbonic anhydrase II, Active site, Surfaces and Interfaces, Condensed Matter Physics, Protein tertiary structure, Molten globule, Crystallography, Adsorption, Enzyme, Electrochemistry, biology.protein, General Materials Science, Spectroscopy, Protein adsorption

Abstract

The surface adsorption behavior of protein variants of the enzyme human carbonic anhydrase II (HCA II) to silica nanoparticles has been investigated. Various destabilized mutants were produced by site-directed mutagenesis of amino acids located in the interior of the protein. The silica particles induced a molten-globule-like state in all of the variants. All protein variants initially adsorbed to the particles, and then underwent conformational rearrangements in a stepwise manner, as indicated by the loss of activity and the subsequent loss of tertiary structure. Activity, CD, and ANS fluorescence measurements showed that a decrease in the global stability of the protein is strongly correlated to increased rates of conformational change following particle adsorption. In contrast to unfolding processes induced by chemical denaturants or heat, in the transition to the molten-globule-like state induced by the silica particles, the active site region unfolds before the majority of the tertiary interactions a...

Published

2000

23. Conformation of Human Carbonic Anhydrase II Variants Adsorbed to Silica Nanoparticles

Author

Peter Billsten, Uno Carlsson, Bengt-Harald Jonsson, Hans Elwing, Gerd Olofsson, and Fredrik Höök

Subjects

Circular dichroism, Chemistry, Carbonic anhydrase II, Mutant, Nanoparticle, Surfaces and Interfaces, Condensed Matter Physics, Molten globule, Crystallography, Differential scanning calorimetry, Adsorption, Electrochemistry, General Materials Science, Denaturation (biochemistry), Spectroscopy

Abstract

Conformational changes of human carbonic anhydrase II (HCAIIpwt) adsorbed on silica nanoparticles (with an average diameter of 9 nm) have been investigated using differential scanning calorimetry (DSC), and in some specific cases also using circular dichroism (CD) and intrinsic tryptophan fluorescence. To relate the observed conformational changes to the denaturation stability and/or chemical properties in solution, two N-terminally truncated variants and two mutants of HCAIIpwt containing specific single site mutations were also investigated. From the thermal transitions of HCAIIpwt adsorbed to the nanoparticles we found that this variant forms a state that was distinctly different from both the native and molten globule states in solution. No thermal transition at all was observed for any of the other variants adsorbed on nanoparticles. CD and intrinsic tryptophan fluorescence indicate that these variants attain a molten globule-like state at the surface.

Published

1999

24. GroEL provides a folding pathway with lower apparent activation energy compared to spontaneous refolding of human carbonic anhydrase II

Author

Uno Carlsson, Malin Persson, and Nils Bergenhem

Subjects

Protein Folding, Carbonic anhydrase II, Kinetics, Biophysics, Chaperone, Activation energy, Biochemistry, GroEL, Chaperonin, Maltose-binding protein, Enzyme Reactivators, Structural Biology, Human carbonic anhydrase II, Genetics, Humans, Refolding, Molecular Biology, Carbonic Anhydrases, chemistry.chemical_classification, biology, Temperature, Chaperonin 60, Cell Biology, Enzyme, chemistry, Chaperone (protein), biology.protein, Thermodynamics

Abstract

The kinetics of the refolding of the enzyme, human carbonic anhydrase II (HCA II), at different temperatures, together with the Escherichia coli chaperonin GroEL, has been studied. The Arrhenius plots for the spontaneous, GroEL-assisted, and GroEL/ES-assisted refolding of HCA II show that the apparent activation energy (Ea) is lower in the presence of the chaperonin GroEL alone than for the spontaneous reaction, whereas the apparent activation energy for the GroEL/ES-assisted reaction is almost the same as for the spontaneous reaction (85, 46, and 72 kJ/mol, for the spontaneous, GroEL, and GroEL/ES-assisted reactions, respectively).

Published

1997

25. Formation of Local Native-like Tertiary Structures in the Slow Refolding Reaction of Human Carbonic Anhydrase II as Monitored by Circular Dichroism on Tryptophan Mutants

Author

Per-Ola Freskgård, Dick Andersson, Uno Carlsson, and Bengt-Harald Jonsson

Subjects

Protein Folding, Circular dichroism, Stereochemistry, Carbonic anhydrase II, Biochemistry, Substrate Specificity, Residue (chemistry), Humans, Carbonic Anhydrases, Fluorescent Dyes, Dansyl Compounds, Binding Sites, biology, Chemistry, Circular Dichroism, Tryptophan, Active site, Protein tertiary structure, Protein Structure, Tertiary, Folding (chemistry), N-terminus, Kinetics, Crystallography, Mutagenesis, Site-Directed, biology.protein

Abstract

In the present study, near-UV CD kinetic measurements on mutants, in which one Trp residue had been replaced, were performed to probe the development of asymmetric environments around specific Trp residues during the refolding of human carbonic anhydrase II (HCAII). In addition, the formation of the active site was probed by the binding of a fluorescent sulfonamide inhibitor. The development of the individual Trp CD spectra during refolding was obtained by subtracting the CD spectrum of the mutant lacking one Trp from that of HCAII at different time points. The same method was used for the particular Trp residues to obtain the kinetic CD traces monitored at a specific wavelength (270 nm). Trp residues 16, 97, and 245 were analyzed. Trp16 probes the N-terminal domain (amino acid residues 1-25), and this part is forming its tertiary structure slower than the major domain (amino acid residues 26-260) of the protein molecule, which contains the active site and a dominating beta-sheet. An essentially native structure of the major domain seems to act as a template for the correct folding of the N terminus. Trp97 is located in a hydrophobic cluster comprising beta-strands 3-5 in the protein core. Previously, we have shown that this region is remarkably stable and compact, and stopped-flow fluorescence data indicate that Trp97 is buried in an apolar compact cluster within a few milliseconds [Svensson, M., Jonasson, P., Freskgård, P.-O., Jonsson, B.-H., Lindgren, M., Martensson, L.-G., Gentile, M., Bóren, K.,Carlsson, U. (1995) Biochemistry 34, 8606-8620; Jonasson, P., Aronsson, G., Carlsson, U.,Jonsson, B.-H. (1997) Biochemistry 36 (in press)]. Here it is shown that the development of the native tertiary structure at Trp97 occurs in the minute time domain. Trp245 is located in a long loop between the N-terminal domain and the core structure. Although this Trp has attained native-like fluorescence properties within the dead time of the CD experiment, it assumes a native-like asymmetric environment even slower than Trp97. Thus, the investigated Trp residues develop their native CD bands at different rates, showing that formation of native-like tertiary structure is occurring with varying rates in different regions of the protein.

Published

1997

26. Electron spin echo decay as a probe of aminoxyl environment in spin-labeled mutants of human carbonic anhydrase II †

Author

Magdalena Svensson, Bengt-Harald Jonsson, Mikael Lindgren, Uno Carlsson, Sandra S. Eaton, Per Hammarström, and Gareth R. Eaton

Subjects

Solvent, Steric effects, Nitroxide mediated radical polymerization, Proton, Chemistry, Carbonic anhydrase II, Spin echo, Analytical chemistry, Site-directed spin labeling, Spin label

Abstract

Genetically-engineered human carbonic anhydrase II mutants have been prepared with cysteine introduced at selected locations and spin-labeled with an aminoxyl (formerly known as nitroxide) radical. Two-pulse electron spin echo data have been obtained for samples in 1∶1 water–glycerol employing a Bruker ESP380E spectrometer. Data obtained at 11 and 40 K are fitted to the function Y(τ) = Y(0)· exp[–(2τ/Tm)x]. Tm = 4.4 to 4.1 µs with x > 2 for labels near the surface, but the decay shape changes to Tm = 2 µs, x = 1 for a label buried in a hydrophobic region of the protein. To identify characteristics of the spin label environment that impact Tm and x, 0.1 to 0.5 mM solutions of aminoxyls are examined in a series of glassy solvents. At these spin label concentrations spin echo dephasing is dominated by interaction with solvent protons. For solvents that do not contain methyl groups 1/Tm increases as solvent proton concentration increases. The smallest values of x and of Tm are observed for solvents with the least sterically hindered methyl groups. In samples of spin-labeled engineered proteins the aminoxyl-probe is generally used to explore local motions near room temperature. The data presented here indicate that the shape of the echo decay obtained at low temperature is a sensitive indicator of the proton environment of the spin-label. The combination of lineshape studies at room temperature and spin echo studies at low temperature provide complementary information in spin labeling studies of protein folding and protein–protein interaction.

Published

1997

27. Conformational Effects on the Circular Dichroism of Human Carbonic Anhydrase II: A Multilevel Computational Study

Author

Gary W. Black, Uno Carlsson, Tatyana G. Karabencheva-Christova, Kia Balali-Mood, Christo Z. Christov, and Uversky, Vladimir

Subjects

Models, Molecular, Circular dichroism, Protein Structure, Protein Conformation, Carbonic anhydrase II, Science, Biophysics, Molecular Dynamics Simulation, Molecular Dynamics, Biochemistry, Protein Chemistry, Carbonic Anhydrase II, Protein–protein interaction, Molecular dynamics, Protein structure, Computational Chemistry, Teknik och teknologier, Macromolecular Structure Analysis, Humans, Biomacromolecule-Ligand Interactions, Biology, Multidisciplinary, Chemistry, Physics, Circular Dichroism, Proteins, Computational Biology, A100, Chromophore, C700, Enzyme structure, Enzymes, Isoenzymes, Enzyme Structure, Computer Science, Engineering and Technology, Medicine, Density functional theory, Crystallization, Research Article, Computer Modeling

Abstract

Circular Dichroism (CD) spectroscopy is a powerful method for investigating conformational changes in proteins and therefore has numerous applications in structural and molecular biology. Here a computational investigation of the CD spectrum of the Human Carbonic Anhydrase II (HCAII), with main focus on the near-UV CD spectra of the wild-type enzyme and it seven tryptophan mutant forms, is presented and compared to experimental studies. Multilevel computational methods (Molecular Dynamics, Semiempirical Quantum Mechanics, Time-Dependent Density Functional Theory) were applied in order to gain insight into the mechanisms of interaction between the aromatic chromophores within the protein environment and understand how the conformational flexibility of the protein influences these mechanisms. The analysis suggests that combining CD semi empirical calculations, crystal structures and molecular dynamics (MD) could help in achieving a better agreement between the computed and experimental protein spectra and provide some unique insight into the dynamic nature of the mechanisms of chromophore interactions. Funding Agencies|UK National Service for Computational Chemistry Software||UK National Supercomputer Service Hector||Marie Curie Fellowships (FP7 of EU)

Published

2013

28. GroEL reversibly binds to, and causes rapid inactivation of, human carbonic anhydrase II at high temperatures

Author

Uno Carlsson, Nils Bergenhem, and Malin Persson

Subjects

Protein Denaturation, Protein Folding, Hot Temperature, Carbonic anhydrase II, Biophysics, macromolecular substances, Guanidines, Biochemistry, Chaperonin, Structural Biology, Escherichia coli, Prolyl isomerase, Humans, Proline, Molecular Biology, Guanidine, Amino Acid Isomerases, Carbonic Anhydrases, chemistry.chemical_classification, biology, Chemistry, Temperature, Chaperonin 60, Peptidylprolyl Isomerase, GroEL, Recombinant Proteins, Enzyme Activation, enzymes and coenzymes (carbohydrates), Enzyme, Chaperone (protein), biological sciences, health occupations, biology.protein, bacteria, Carrier Proteins, Isomerization, Protein Binding

Abstract

The initial yield of reactivation of GuHCl denatured human carbonic anhydrase II does not change with temperature between 3 and 35 degrees C. At temperatures above 35 degrees C, the enzymatic activity is not stable, but decreases over time. If the bacterial chaperonin GroEL is present during reactivation, the initial yield is lower compared to the spontaneous reaction at temperatures of 35-50 degrees C. However, unlike the spontaneous reactivation, the enzymatic activity with time in the presence of GroEL. In the presence of GroEL, native HCA II incubated at elevated temperatures will rapidly loose enzymatic activity to the same value as during reactivation at that particular temperature; most of the activity will recover if the temperature is lowered when GroEL is present. It is evident that there is an equilibrium between an inactive intermediate of HCA II, probably bound to GroEL, and active enzyme. Furthermore, proline isomerization is part of the rate-limiting step of refolding even in the presence of GroEL, and it is very noteworthy that prolyl isomerase will influence the refolding of HCA II in the presence of GroEL.

Published

1996

29. A comparative CD study of carbonic anhydrase isoenzymes with different number of tryptophans: Impact on calculation of secondary structure content

Author

Per-Ola Freskgård, Kristina Borén, and Uno Carlsson

Subjects

biology, Stereochemistry, Chemistry, Tryptophan, CARBONIC ANHYDRASE III, Crystallography, X-Ray, Biochemistry, Isozyme, Protein Structure, Secondary, Isoenzymes, chemistry.chemical_compound, Carbonic anhydrase, β structure, Aromatic amino acids, biology.protein, Animals, Humans, Cattle, Carbonic Anhydrase I, Molecular Biology, Protein secondary structure, Carbonic Anhydrases, Research Article

Abstract

The CD spectra of human carbonic anhydrase I and II and bovine carbonic anhydrase III were recorded and analyzed. The 3D structures of these isoenzymes are known, showing very similar secondary structure and polypeptide-chain fold. The tryptophan content, however, differs between the isoenzymes, i.e., isoenzymes I, II, and III possess 6, 7, and 8 tryptophans, respectively. All of the tryptophans except the additional tryptophans in isoenzymes II and III, i.e., W245 and W47, are conserved. Despite the fact that X-ray structure determinations showed that the isoenzymes had highly similar secondary structure, the contents of alpha-helix and beta-sheet structure differed considerably when using different CD algorithms for estimation of the fractions of various secondary structural elements. This shows that aromatic amino acids also interfere in the wavelength region (far-UV) used to calculate the amount of secondary structure. Such interference is especially problematic when analyzing proteins like carbonic anhydrase, which consist mainly of beta-structure that gives rise to weak ellipticity bands, compared to the bands arising from alpha-helical structure.

Published

1996

30. Folding of β-sheet proteins

Author

Uno Carlsson and Bengt-Harald Jonsson

Subjects

Protein Denaturation, Protein Folding, Protein Conformation, Chemistry, Beta sheet, Mutagenesis (molecular biology technique), Phi value analysis, Protein Engineering, Protein Structure, Secondary, Folding (chemistry), Kinetics, Biochemistry, Structural Biology, Molecular Probes, Biophysics, Amino Acids, Molecular Biology

Abstract

In the past year, interesting new information concerning various aspects of the folding process of β-sheet proteins has been gleaned. Kinetic and equilibrium folding intermediates have been characterized. Studies of extensively denatured states and of model peptide fragments have enabled important steps to be taken towards an understanding of the initiation of the folding process of β-sheet proteins. Site-directed mutagenesis has been used in combination with various probes to monitor folding events.

Published

1995

31. Mapping the Folding Intermediate of Human Carbonic Anhydrase II. Probing Substructure by Chemical Reactivity and Spin and Fluorescence Labeling of Engineered Cysteine Residues

Author

Uno Carlsson, Mikael Lindgren, Bengt-Harald Jonsson, Massimiliano Gentile, Magdalena Svensson, Kristina Borén, Lars-Goeran Maartensson, Per Jonasson, and Per-Ola Freskgaard

Subjects

Protein Folding, Fluorophore, Protein Conformation, Carbonic anhydrase II, Inorganic chemistry, Antiparallel (biochemistry), Biochemistry, Protein Structure, Secondary, chemistry.chemical_compound, Protein structure, Enzyme Stability, Humans, Cysteine, Protein secondary structure, Carbonic Anhydrases, Fluorescent Dyes, Molecular Structure, Chemistry, Electron Spin Resonance Spectroscopy, Molten globule, A-site, IAEDANS, Molecular Probes, Mutation, Biophysics, Spin Labels

Abstract

Several conformation-sensitive parameters have shown that human carbonic anhydrase II exists as a stable and compact equilibrium folding intermediate of molten globule type. In this study we have continued a previously initiated mapping of the intermediate structure. Cys residues were engineered, one at a time, into various regions of the protein structure, so as to obtain chemically reactive probes and handles for spectroscopic probes. These probes were used to specifically report on conformational changes accompanying the folding process. Thus, the accessibility of the introduced Cys residues to specific chemical labeling by radioactive iodoacetate was used to monitor the stability and compactness of the substructure surrounding each Cys residue. In addition, a spin-label (nitroxide radical) and a fluorescent probe (IAEDANS) were attached to the inserted SH-groups to give complementary information. The mobility of the spin-label was used to indicate local changes in structure, and the fluorophore was used to probe local changes in polarity at various stages of unfolding. Much of the predominant beta-structure, consisting of 10 beta-strands extending throughout the entire molecule, appears to be compact and largely intact in the intermediate. Thus, beta-strands 3-7, probed at positions 68, 97, 118, 123, 206, and 245, seem to have a native-like structure in the folding intermediate. In contrast, a more flexible structure is found around positions 56, 176, and 256 in the peripheral beta-strands 1, 2, and 9, showing that the stability of the secondary structure in the intermediate state is less in the outer parts of the protein. A hydrophobic region, containing beta-strands 3-5, seems to be remarkably stable and is not ruptured until strong denaturing conditions (5 M GuHCl) are applied. The stability of this hydrophobic beta-core appears to increase toward the center. This stable region is contained in the middle of a sequentially continuous antiparallel structure that spans beta-strands 2-6, suggesting that this part might represent a site where folding is initiated.

Published

1995

32. Characterization of a folding intermediate of human carbonic anhydrase II: probing local mobility by electron paramagnetic resonance

Author

Uno Carlsson, P. Jonasson, Lars-Göran Mårtensson, Per-Ola Freskgård, Bengt-Harald Jonsson, Magdalena Svensson, and Mikael Lindgren

Subjects

Protein Denaturation, Protein Folding, Protein Conformation, Carbonic anhydrase II, Population, Biophysics, Guanidines, Spectral line, law.invention, Nuclear magnetic resonance, law, Humans, Intermediate state, education, Electron paramagnetic resonance, Guanidine, Carbonic Anhydrases, education.field_of_study, Chemistry, Electron Spin Resonance Spectroscopy, Rotational diffusion, Models, Theoretical, Recombinant Proteins, Isoenzymes, Folding (chemistry), Crystallography, Absorption (chemistry), Research Article

Abstract

The spin-labeling method was used to investigate human carbonic anhydrase, HCA II, undergoing unfolding induced by guanidine-HCI (Gu-HCI). The spin-probe, N-(2,2,5,5-tetramethyl-1-yloxypyrrolidinyl-3-yl)iodoacetamide, was attached covalently to the single cysteine (position 206) in the enzyme. The electron paramagnetic resonance spectrum of the folded structure showed the characteristic slow motional spectra. When the concentration of the denaturing agent, Gu-HCI, was gradually increased, new spectral components with narrower lines evolved to give complex electron paramagnetic resonance spectra, apparently containing superimposed contributions from several components of different mobility. By a differentiation technique, it was possible to follow the relative increase of the narrow components as a function of Gu-HCI concentration. The amplitude of difference spectra versus Gu-HCI concentration showed two distinct maxima, indicating the existence of a folding intermediate state/structure. The results were found to agree with optical absorption data, which showed similar transitions at the same Gu-HCI concentrations. From line-shape simulations assuming a Brownian diffusion model, the rotational diffusion constants for the spin-label in the folded, folding intermediate, and unfolded structures were determined. The relative abundances of the three conformations in the region 0–4 M Gu-HCI were obtained by least squares fitting of the simulated spectra to the experimental ones. The folding intermediate was found to have a maximum population of 39 +/- 4% at approximately 0.7 M Gu-HCI.

Published

1995

33. GroEL/ES-mediated refolding of human carbonic anhydrase II: role of N-terminal helices as recognition motifs for GroEL

Author

Michael Spangfort, Nils Bergenhem, Per-Ola Freskgård, Göran Aronsson, Bengt-Harald Jonsson, Brian P. Surin, Malin Persson, and Uno Carlsson

Subjects

chemistry.chemical_classification, Protein Folding, Binding Sites, biology, Carbonic anhydrase II, Biophysics, Chaperonin 60, GroES, Protein engineering, Biochemistry, GroEL, Enzyme Reactivators, Enzyme, chemistry, Structural Biology, Chaperone (protein), Carbonic anhydrase, Chaperonin 10, biology.protein, Humans, bacteria, Molecular Biology, Active enzyme, Carbonic Anhydrases

Abstract

The presence of GroEL/13S during the refolding of human carbonic anhydrase II (pseudo-wild type) was found to increase the yield of active enzyme from 65 to 100%. This chaperone action on the enzyme could be obtained by adding GroEL alone, and the time-course in that case was only moderately slower than the spontaneous process. Truncated forms of carbonic anhydrase, in which N-terminal helices were removed, also served as protein substrates for GroEL/ES. This demonstrates that N-terminally located helices are not obligatory as recognition motifs.

Published

1995

34. Effects on the conformation of FVIIa by sTF and Ca²⁺ binding: studies of fluorescence resonance energy transfer and quenching

Author

Karin, Carlsson, Egon, Persson, Mikael, Lindgren, Uno, Carlsson, and Magdalena, Svensson

Subjects

Enzyme Activation, Amino Acid Substitution, Protein Conformation, Catalytic Domain, Fluorescence Resonance Energy Transfer, Calcium, Factor VIIa, Protein Binding, Protein Structure, Tertiary, Thromboplastin

Abstract

The apparent length of FVIIa in solution was estimated by a FRET analysis. Two fluorescent probes, fluorescein (Fl-FPR) and a rhodamine derivative (TMR), were covalently attached to FVIIa. The binding site of Fl-FPR was in the protease domain whereas TMR was positioned in the Gla domain, thus allowing a length measure over virtually the whole extension of the protein. From the FRET measurements, the distances between the two probes were determined to be 61.4 for free FVIIa and 65.5Å for FVIIa bound to soluble tissue factor (sTF). These seemingly short distances, compared to those anticipated based on the complex crystal structure, require that the probes stretch towards each other. Thus, the apparent distance from the FRET analysis was shown to increase with 4Å upon formation of a complex with sTF in solution. However, considering how protein dynamics, based on recent molecular dynamics simulations of FVIIa and sTF:FVIIa (Y.Z. Ohkubo, J.H. Morrissey, E. Tajkhorshid, J. Thromb. Haemost. 8 (2010) 1044-1053), can influence the apparent fluorescence signal our calculations indicated that the global average conformation of active-site inhibited FVIIa is nearly unaltered upon ligation to sTF. It is known from amidolytic activity measurements that Ca(2+) binding leads to activation of FVIIa, but we have for the first time directly demonstrated conformational changes in the environment of the active site upon Ca(2+) binding. Interestingly, this Ca(2+)-induced conformational change can be noted even in the presence of an inhibitor. Forming a complex with sTF further stabilized this conformational change, leading to a more inaccessible active-site located probe.

Published

2011

35. Characterization of folding intermediates of human carbonic anhydrase II: probing substructure by chemical labeling of sulfhydryl groups introduced by site-directed mutagenesis

Author

Per-Ola Freskgård, Lars-Göran Mårtensson, Magdalena Svensson, Kihlgren A, Bengt-Harald Jonsson, and Uno Carlsson

Subjects

Protein Folding, Alkylation, Stereochemistry, Carbonic anhydrase II, Guanidines, Biochemistry, Protein Structure, Secondary, chemistry.chemical_compound, Carbonic anhydrase, Enzyme Stability, Humans, Cysteine, Sulfhydryl Compounds, Site-directed mutagenesis, Guanidine, Protein secondary structure, Carbonic Anhydrases, biology, Chemistry, Circular Dichroism, Mutagenesis, Folding (chemistry), Mutagenesis, Site-Directed, biology.protein, Thermodynamics, Spectrophotometry, Ultraviolet

Abstract

By measurement of UV absorbance, CD spectra, and enzyme activity, we have shown that human carbonic anhydrase II forms a stable and compact folding intermediate at a moderate concentration of guanidine hydrochloride. The major aim of this study was to map the intermediate structure. For that reason, site-directed mutagenesis was used to introduce cysteine residues in various parts of the central beta-structure to give in each case a single cysteine residue. Thereafter, the accessibility of the introduced SH group to specific chemical labeling was used to probe the stability and compactness of the area surrounding each cysteine residue. Our results indicate that the folding intermediate has an ordered native-like secondary structure in the central part of the beta-sheet, whereas the peripheral part of the beta-sheet seems to be less ordered. A large hydrophobic cluster situated between the central beta-sheet core and secondary structure elements on the surface appears to be intact in the intermediate and is remarkably stable even at high GuHCl concentrations (> 5 M). This unusually stable substructure might function as a "seed" during the initiation of the folding process.

Published

1993

36. Probing local mobility in carbonic anhydrase: EPR of spin-labelled SH groups introduced by site-directed mutagenesis

Author

Magdalena Svensson, Uno Carlsson, Mikael Lindgren, Bengt-Harald Jonsson, Per Jonasson, Per-Ola Freskgård, and Lars-Göran Mårtensson

Subjects

chemistry.chemical_classification, biology, Stereochemistry, Reaction intermediate, law.invention, chemistry.chemical_compound, Enzyme, Protein structure, chemistry, law, Carbonic anhydrase, Iodoacetamide, biology.protein, Denaturation (biochemistry), Site-directed mutagenesis, Electron paramagnetic resonance

Abstract

Cloned human carbonic anhydrase, HCAII, and mutants thereof have been investigated by spin-probing methods during its unfolding caused by guanidine·HCl. The spin-probe, N-(2,2,5,5-tetramethyl-1-ylooxypyrrolidin-3-yl)iodoacetamide, has been regiospecifically introduced into cyst-eines by site-directed mutagenesis in various positions of the protein structure. Here we focus on EPR spectra of three different spin-labelled enzymes at various guanidine-HCl concentrations (at equilibrium). The following spin-labelled mutants are discussed: W16C/C206S, W97C/C206S and F176C/C206S. The EPR spectra of the three mutants differ markedly at low guanidine·HCl concentration (0–1 mol dm–3) particularly within the series W97C/C206S and F176C/C206S, showing the characteristic anisotropic slow motional features. The W16C/C206S label position is much more mobile in the folded structures. The rotational correlation times reflect the local environment of the spin-probe in the folded enzyme: in W97C it is located in the core, near the active centre, in W16C and F176C at more peripheral positions. All samples gave EPR spectra characteristic of a ‘free’ unfolded protein chain at guanidine-HCl concentrations of ca. 3 mol dm–3 and above, and could be characterised by using one component in lineshape simulations. The spectra of the W97C/C206S and F176C/C206S samples in low concentrations of guanidine·HCl (between ca. 0.1 and 2.0 mol dm–3) could only be reproduced in simulations by introducing several components associated with rather different rotational correlation times. This seems to imply the co-existence of at least two dynamic structures in equilibrium during the intermediate stages of the unfolding process. It is compatible with earlier suggestions of a folding intermediate based on optical characterisation.

Published

1993

37. Chaperone activity of Cyp18 through hydrophobic condensation that enables rescue of transient misfolded molten globule intermediates

Author

Per Hammarström, Rikard Fristedt, Uno Carlsson, Karin Almstedt, Rajesh Mishra, Satish Babu Moparthi, and Martin Karlsson

Subjects

Protein Denaturation, Protein Folding, Isomerase, Biochemistry, Carbonic Anhydrase II, Anilino Naphthalenesulfonates, Substrate Specificity, Cyclophilins, Protein structure, Enzyme Stability, Native state, Humans, Cyclophilin, Fluorescent Dyes, biology, Chemistry, GroEL, Molten globule, Recombinant Proteins, Protein Structure, Tertiary, Up-Regulation, Molecular Weight, Chaperone (protein), biology.protein, Biophysics, Mutagenesis, Site-Directed, Protein folding, Hydrophobic and Hydrophilic Interactions, Molecular Chaperones

Abstract

The single-domain cyclophilin 18 (Cyp18) has long been known to function as a peptidyl-prolyl cis/trans isomerase (PPI) and was proposed by us to also function as a chaperone [Freskgard, P.-O., Bergenhem, N., Jonsson, B.-H., Svensson, M., and Carlsson, U. (1992) Science 258, 466-468]. Later several multidomain PPIs were demonstrated to work as both a peptidyl-prolyl cis/trans isomerase and a chaperone. However, the chaperone ability of Cyp18 has been debated. In this work, we add additional results that show that Cyp18 can both accelerate the rate of refolding and increase the yield of native protein during the folding reaction, i.e., function as both a folding catalyst and a chaperone. Refolding experiments were performed using severely destabilized mutants of human carbonic anhydrase II under conditions where the unfolding reaction is significant and a larger fraction of a more destabilized variant populates molten globule-like intermediates during refolding. A correlation of native state protein stability of the substrate protein versus Cyp18 chaperone activity was demonstrated. The induced correction of misfolded conformations by Cyp18 likely functions through rescue from misfolding of transient molten globule intermediates. ANS binding data suggest that the interaction by Cyp18 leads to an early stage condensation of accessible hydrophobic portions of the misfolding-prone protein substrate during folding. The opposite effect was observed for GroEL known as an unfoldase at early stages of refolding. The chaperone effect of Cyp18 was also demonstrated for citrate synthase, suggesting a general chaperone effect of this PPI.

Published

2010

38. GroEL-induced topological dislocation of a substrate protein β-sheet core: a solution EPR spin-spin distance study

Author

Anngelica Jarl, Uno Carlsson, Rikard Owenius, Per Hammarström, and Bengt-Harald Jonsson

Subjects

Conformational change, Chemistry, Biophysics, Beta sheet, Cell Biology, Protein aggregation, Topology, Biochemistry, GroEL, Molten globule, law.invention, Chaperonin, Crystallography, law, biological sciences, Native state, Original Article, Electron paramagnetic resonance

Abstract

The Hsp60-type chaperonin GroEL assists in the folding of the enzyme human carbonic anhydrase II (HCA II) and protects it from aggregation. This study was aimed to monitor conformational rearrangement of the substrate protein during the initial GroEL capture (in the absence of ATP) of the thermally unfolded HCA II molten-globule. Single- and double-cysteine mutants were specifically spin-labeled at a topological breakpoint in the β-sheet rich core of HCA II, where the dominating antiparallel β-sheet is broken and β-strands 6 and 7 are parallel. Electron paramagnetic resonance (EPR) was used to monitor the GroEL-induced structural changes in this region of HCA II during thermal denaturation. Both qualitative analysis of the EPR spectra and refined inter-residue distance calculations based on magnetic dipolar interaction show that the spin-labeled positions F147C and K213C are in proximity in the native state of HCA II at 20 °C (as close as ∼8 A), and that this local structure is virtually intact in the thermally induced molten-globule state that binds to GroEL. In the absence of GroEL, the molten globule of HCA II irreversibly aggregates. In contrast, a substantial increase in spin–spin distance (up to >20 A) was observed within minutes, upon interaction with GroEL (at 50 and 60 °C), which demonstrates a GroEL-induced conformational change in HCA II. The GroEL binding-induced disentanglement of the substrate protein core at the topological break-point is likely a key event for rearrangement of this potent aggregation initiation site, and hence, this conformational change averts HCA II misfolding.

Published

2010

39. Versatile stopped-flow apparatus with adjustable pistons

Author

Per-Ola Freskgård, Uno Carlsson, and Nils Bergenhem

Subjects

Chemistry, Instrumentation, Analytical chemistry, Environmental Chemistry, Mechanical engineering, Stopped flow, Biochemistry, Spectroscopy, Analytical Chemistry, Dilution

Abstract

A stopped-flow apparatus with many potential applications is described, in which the vertical design makes operaton easier. In addition, the system has adjustable driving pistons that facilitate refilling of syringes and changing of reaction solutions without allowing air to enter the system. This means that the use of reservoir syringes is redundant. The driving pistons can easily be adjusted to withstand different pressures and temperatures and the O-rings are simple to change when worn out. The vertical stopped-flow system is also flexible, as syringes of different size can be used and are easily changed when, for instance, different dilution ratios are needed.

Published

1992

40. Thermodynamic interrogation of a folding disease. Mutant mapping of position 107 in human carbonic anhydrase II linked to marble brain disease

Author

Per Hammarström, Uno Carlsson, Lars-Göran Mårtensson, and Karin Almstedt

Subjects

Models, Molecular, Protein Denaturation, Protein Folding, Hot Temperature, Protein family, Carbonic anhydrase II, Mutant, medicine.disease_cause, Biochemistry, Carbonic Anhydrase II, Carbonic anhydrase, Enzyme Stability, medicine, Humans, Carbonic Anhydrase Inhibitors, Protein Structure, Quaternary, Guanidine, chemistry.chemical_classification, Mutation, biology, Brain Diseases, Metabolic, Inborn, Molecular biology, Molten globule, Amino acid, Acetazolamide, Enzyme, Spectrometry, Fluorescence, chemistry, Amino Acid Substitution, biology.protein, Thermodynamics

Abstract

Marble brain disease (MBD) also known as Guibaud-Vainsel syndrome is caused by autosomal recessive mutations in the human carbonic anhydrase II (HCA II) gene. HCA II is a 259 amino acid single domain enzyme and is dominated by a 10-stranded beta-sheet. One mutation associated with MBD entails the H107Y substitution where H107 is a highly conserved residue in the carbonic anhydrase protein family. We have previously demonstrated that the H107Y mutation is a remarkably destabilizing folding mutation [Almstedt et al. (2004) J. Mol. Biol. 342, 619-633]. Here, the exceptional destabilization by the H107Y mutation has been further investigated. A mutational survey of position H107 and a neighboring conserved position E117 has been performed entailing the mutants H107A, H107F, H107N, E117A and the double mutants H107A/E117A and H107N/E117A. All mutants were severely destabilized versus GuHCl and heat denaturation. Thermal denaturation and GuHCl phase diagram and ANS analyses showed that the mutants shifted HCA II toward populating ensembles of intermediates of molten globule type under physiological conditions. The native state stability of the mutants was in the following order: wtH107NE117AH107AH107FH107YH107N/E117AH107A/E117A.(i) H107N is least destabilizing likely due to compensatory H-bonding ability of the introduced Asn residue. (ii) Double mutant cycles surprisingly reveal additive destabilization of H107N and E117A showing that H107 and E117 are independently stabilizing the folded protein. (iii) H107Y and H107F are exceptionally destabilizing due to bulkiness of the side chains whereas H107A is more accommodating, indicating long-range destabilizing effects of the natural pathogenic H107Y mutation.

Published

2008

41. Inhibitors of factor VIIa affect the interface between the protease domain and tissue factor

Author

Egon Persson, Karin Carlsson, Magdalena Svensson, and Uno Carlsson

Subjects

Models, Molecular, Protease, Binding Sites, biology, Chemistry, medicine.medical_treatment, Allosteric regulation, Biophysics, Cell Biology, Factor VIIa, Biochemistry, Cofactor, Protein–protein interaction, Cell biology, Protein Structure, Tertiary, Thromboplastin, Tissue factor, Protein structure, Spectrometry, Fluorescence, Coagulation, medicine, biology.protein, Binding site, Molecular Biology

Abstract

Blood coagulation is triggered by the formation of a complex between factor VIIa (FVIIa) and its cofactor, tissue factor (TF). The gamma-carboxyglutamic acid-rich domain of FVIIa docks with the C-terminal domain of TF, the EGF1 domain of FVIIa contacts both domains of TF, and the EGF2 domain and protease domain (PD) form a continuous surface that sits on the N-terminal domain of TF. Our aim was to investigate the conformational changes that occur in the sTF.PD binding region when different types of inhibitors, i.e., one active-site inhibitor (FFR-chloromethyl ketone (FFR)), two different peptide exosite inhibitors (E-76 and A-183), and the natural inhibitor tissue factor pathway inhibitor (TFPI), were allowed to bind to FVIIa. For this purpose, we constructed two sTF mutants (Q37C and E91C). By the aid of site-directed labeling technique, a fluorescent label was attached to the free cysteine. The sTF.PD interface was affected in position 37 by the binding of FFR, TFPI, and E-76, i.e., a more compact structure was sensed by the probe, while for position 91 located in the same region no change in the surrounding structure was observed. Thus, the active site inhibitors FFR and TFPI, and the exosite inhibitor E-76 have similar effects on the probe in position 37 of sTF, despite their differences in size and inhibition mechanism. The allosteric changes at the active site caused by binding of the exosite inhibitor E-76 in turn induce similar conformational changes in the sTF.PD interface as does the binding of the active site inhibitors. A-183, on the other hand, did not affect position 37 in sTF, indicating that the A-183 inhibition mechanism is different from that of E-76.

Published

2006

42. Soil peroxidase-mediated chlorination of fulvic acid

Author

Anders Grimvall, Uno Carlsson, Hans Borén, and Gunilla Asplund

Subjects

biology, Chemistry, Soil organic matter, Potassium, Enzyme unit, Halogenation, chemistry.chemical_element, complex mixtures, Chloride, chemistry.chemical_compound, Environmental chemistry, medicine, Chlorine, biology.protein, Hydrogen peroxide, medicine.drug, Peroxidase

Abstract

Humic matter has recently been shown to contain considerable quantities of naturally produced organohalogens. The present study investigated the possibility of a non-specific, enzymatically mediated halogenation of organic matter in soil. The results showed that, in the presence of chloride and hydrogen peroxide, the enzyme chloroperoxidase (CPO) from the fungus Caldariomyces fumago catalyzes chlorination of fulvic acid. At pH 2.5 – 6.0, the chlorine to fulvic acid ratio in the tested sample was elevated from 12 mg/g to approximately 40–50 mg/g. It was also shown that this reaction can take place at chloride and hydrogen peroxide concentrations found in the environment. An extract from spruce forest soil was shown to have a measurable chlorinating capacity. The activity of an extract of 0.5 kg soil corresponded to approximately 0.3 enzyme units, measured as CPO activity. Enzymatically mediated halogenation of humic substances may be one of the mechanisms explaining the widespread occurrence of adsorbable organic halogens (AOX) in soil and water.

Published

2005

43. The cyclooxygenase-2 inhibitor celecoxib is a potent inhibitor of human carbonic anhydrase II

Author

Louis R. Cantilena, Uno Carlsson, G. Sokol, J. F. Knudsen, and Per Hammarström

Subjects

Carbonic anhydrase II, Immunology, Pharmacology, Carbonic Anhydrase II, Inhibitory Concentration 50, Structure-Activity Relationship, Carbonic anhydrase, medicine, Immunology and Allergy, Humans, Cyclooxygenase Inhibitors, Carbonic Anhydrase Inhibitors, Rofecoxib, Sulfonamides, biology, Dose-Response Relationship, Drug, Chemistry, Sulfonamide (medicine), Anti-Inflammatory Agents, Non-Steroidal, Isoxazoles, Valdecoxib, Acetazolamide, Celecoxib, biology.protein, Pyrazoles, Cyclooxygenase, medicine.drug

Abstract

Cyclooxygenase-2 (COX-2) is up-regulated in stromal and inflammatory cells. The inducible COX-2 isoform is expressed during inflammation, in some cancers, and in brain tissue after global and focal ischemia. Tissue acidosis is a dominant factor in inflammation, and contributes to pain and hyperalgesia. Recently, compelling epidemiological and clinical evidence has documented the COX-independent effects of some COX-2 inhibitors (i.e., celecoxib, valdecoxib, and rofecoxib); among these effects are carbonic anhydrase (CA) inhibition. Carbonic anhydrases are zinc metalloenzymes expressed in various cell types, including those of the kidney, where they act as general acid–base catalysts. The kidneys are also known to express the highest concentration of COX-2 messenger ribonucleic acid. Celecoxib, like the prototypic CA inhibitor acetazolamide, is structurally characterized by an unsubstituted sulfonamide moiety. In the present study, we report that celecoxib exhibits the characteristics of a potent CA inhibitor, showing inhibitory human carbonic anhydrase II (hCAII) activity in the nanomolar range. Valdecoxib was relatively less potent. Rofecoxib, which lacks the unsubstituted sulfonamide moiety characteristic of CA inhibitors, showed no significant hCAII inhibitory activity. The current study corroborates our earlier report of structure-activity relationships as predictors of such metabolic events as hyperchloremia, acidosis, and changes in calcium and phosphate disposition; and clinical manifestations associated with CA inhibition reported with celecoxib. These data showing inhibition of hCAII by the unsubstituted sulfonamides celecoxib and valdecoxib, but not by rofecoxib, may have important implications for the elucidation of the mechanisms of action as well as the side effects associated with COX-2 inhibitors.

Published

2005

44. Transition state analysis of the complex between coagulation factor VIIa and tissue factor: suggesting a sequential domain-binding pathway

Author

Egon Persson, Per-Ola Freskgård, Maria Österlund, Uno Carlsson, and Magdalena Svensson

Subjects

Models, Molecular, Time Factors, Stereochemistry, medicine.medical_treatment, Biophysics, Factor VIIa, Biochemistry, Protein–protein interaction, Thromboplastin, Tissue factor, medicine, Humans, Surface plasmon resonance, Molecular Biology, Blood Coagulation, Protease, Transition (genetics), Chemistry, Cell Biology, Protein Structure, Tertiary, Energy Transfer, Domain (ring theory), Thermodynamics, Macromolecule, Cysteine

Abstract

Injury of a blood vessel exposes membrane-bound tissue factor (TF) to blood, which allows binding of coagulation factor VIIa (FVIIa). This initiation of the coagulation cascade is dictated by a specific multi-domain interaction between FVIIa and TF. To examine the energies involved in the transition state of the FVIIa:TF complex, various residues in the extracellular part of TF (sTF) that are known to interact with FVIIa were replaced with a smaller cysteine residue. Determination of Φ values in each of the positions using surface plasmon resonance measurements enabled us to characterize the transition state complex between the resulting sTF variants and FVIIa. We found that the interactions in the transition state seemed to be most pronounced between the protease domain of FVIIa and sTF while detailed specific interactions between the Gla-domain and sTF were missing. Thus, the transition state energy data indicate a sequential binding event between these two macromolecules.

Published

2004

45. Circumnavigating misfolding traps in the energy landscape through protein engineering: suppression of molten globule and aggregation in carbonic anhydrase

Author

Uno Carlsson, Lars-Göran Mårtensson, Martin Karlsson, and Patrik Olofsson

Subjects

chemistry.chemical_classification, Models, Molecular, Protein Denaturation, Protein Folding, biology, Chemistry, Mutant, Stable equilibrium, Energy landscape, Protein engineering, Protein Engineering, Biochemistry, Molten globule, Crystallography, Kinetics, Enzyme, Carbonic anhydrase, Enzyme Stability, biology.protein, Native state, Biophysics, Humans, Disulfides, Carbonic Anhydrases

Abstract

The native state of the enzyme human carbonic anhydrase (HCA II) has been stabilized by the introduction of a disulfide bond, the oxidized A23C/L203C mutant. This stabilized protein variant undergoes an apparent two-state unfolding process with suppression of the otherwise stable equilibrium, molten-globule intermediate, which is normally very prone to aggregation. Stopped-flow measurements also showed that lower amounts of the transiently occurring molten globule were formed during refolding. This led to a markedly lowered tendency for aggregation during equilibrium denaturing conditions and, more importantly, to significantly higher reactivation yields upon refolding of the fully denatured protein. Thus, a general strategy to circumvent aggregation during the refolding of proteins could be to stabilize the native state of a protein at the expense of partially folded intermediates, thereby shifting the unfolding behavior from a three-state process to a two-state one.

Published

2004

46. Reshaping the folding energy landscape by chloride salt: impact on molten-globule formation and aggregation behavior of carbonic anhydrase

Author

Hannah Grankvist, Per Hammarström, Kristina Borén, and Uno Carlsson

Subjects

Denaturant, Protein Denaturation, Protein Folding, Hofmeister series, Protein Conformation, Carbonic anhydrase II, Inorganic chemistry, Biophysics, Sodium Chloride, Biochemistry, Carbonic Anhydrase II, Anilino Naphthalenesulfonates, chemistry.chemical_compound, Structural Biology, Genetics, Native state, Humans, Urea, Denaturation (biochemistry), Molecular Biology, Misfolding, Escherichia coli Proteins, Tryptophan, Cell Biology, Molten globule, Chaotropic agent, Cross-Linking Reagents, Spectrometry, Fluorescence, chemistry, Thermodynamics, Protein folding, Lithium Chloride, Intermediate

Abstract

During chemical denaturation different intermediate states are populated or suppressed due to the nature of the denaturant used. Chemical denaturation by guanidine–HCl (GuHCl) of human carbonic anhydrase II (HCA II) leads to a three-state unfolding process (Cm,NI=1.0 and Cm,IU=1.9 M GuHCl) with formation of an equilibrium molten-globule intermediate that is stable at moderate concentrations of the denaturant (1–2 M) with a maximum at 1.5 M GuHCl. On the contrary, urea denaturation gives rise to an apparent two-state unfolding transition (Cm=4.4 M urea). However, 8-anilino-1-naphthalene sulfonate (ANS) binding and decreased refolding capacity revealed the presence of the molten globule in the middle of the unfolding transition zone, although to a lesser extent than in GuHCl. Cross-linking studies showed the formation of moderate oligomer sized (300 kDa) and large soluble aggregates (>1000 kDa). Inclusion of 1.5 M NaCl to the urea denaturant to mimic the ionic character of GuHCl leads to a three-state unfolding behavior (Cm,NI=3.0 and Cm,IU=6.4 M urea) with a significantly stabilized molten-globule intermediate by the chloride salt. Comparisons between NaCl and LiCl of the impact on the stability of the various states of HCA II in urea showed that the effects followed what could be expected from the Hofmeister series, where Li+ is a chaotropic ion leading to decreased stability of the native state. Salt addition to the completely urea unfolded HCA II also led to an aggregation prone unfolded state, that has not been observed before for carbonic anhydrase. Refolding from this state only provided low recoveries of native enzyme.

Published

2004

47. Site-directed fluorescence probing to dissect the calcium-dependent association between soluble tissue factor and factor VIIa domains

Author

Magdalena Svensson, Egon Persson, Uno Carlsson, Karin Carlsson, Maria Österlund, and Per-Ola Freskgård

Subjects

HEPES, Epidermal Growth Factor, Protein Conformation, Biophysics, Factor VIIa, Biochemistry, Fluorescence, Analytical Chemistry, Protein–protein interaction, Protein Structure, Tertiary, Thromboplastin, chemistry.chemical_compound, Tissue factor, chemistry, IAEDANS, Docking (molecular), Molecular Probes, Calcium, Binding site, Molecular Biology, Fluorescent Dyes, Protein Binding

Abstract

We have used the site-directed labeling approach to study the Ca(2+)-dependent docking of factor VIIa (FVIIa) to soluble tissue factor (sTF). Nine Ca(2+) binding sites are located in FVIIa and even though their contribution to the overall binding between TF and FVIIa has been thoroughly studied, their importance for local protein-protein interactions within the complex has not been determined. Specifically we have monitored the association of the gamma-carboxyglutamic acid (Gla), the first EGF-like (EGF1), and the protease domains (PD) of FVIIa to sTF. Our results revealed that complex formation between sTF and FVIIa during Ca(2+) titration is initiated upon Ca(2+) binding to EGF1, the domain containing the site of highest Ca(2+) affinity. Besides we showed that a Ca(2+)-loaded Gla domain is required for an optimal association of all domains of FVIIa to sTF. Ca(2+) binding to the PD seems to be of some importance for the docking of this domain to sTF.

Published

2003

48. Studies on the Conformation of Adsorbed Proteins with the Use of Nanoparticle Technology

Author

Peter Billsten, Hans Elwing, and Uno Carlsson

Published

2003

49. The importance of being knotted: effects of the C-terminal knot structure on enzymatic and mechanical properties of bovine carbonic anhydrase II

Author

Mohammad Taufiq, Alam, Takafumi, Yamada, Uno, Carlsson, and Atsushi, Ikai

Subjects

Models, Molecular, Protein Folding, Chaperonins, Protein Conformation, Circular Dichroism, Protein Renaturation, Microscopy, Atomic Force, Protein Engineering, Carbonic Anhydrase II, Chromatography, Affinity, Enzyme Activation, Spectrometry, Fluorescence, Amino Acid Substitution, Mutagenesis, Site-Directed, Animals, Cattle, Stress, Mechanical

Abstract

In order to better understand the contribution of the knotted folding pattern to the enzymatic and mechanical properties of carbonic anhydrases, we replaced Gln-253 of bovine carbonic anhydrase II with Cys, which allowed us to measure the mechanical strength of the protein against tensile deformation by avoiding knot tightening. The expressed protein, to our surprise, turned out to contain two conformational isomers, one capable of binding an enzymatic inhibitor and the other not, which led to their separation through affinity chromatography. In near- and far-UV circular dichroism and fluorescence spectra, the separated conformers were very similar to each other and to the wild-type enzyme, indicating that they both had native-like conformations. We describe new evidence which supports the notion that the difference between the two conformers is likely to be related to the completeness of the C-terminal knot formation.

Published

2002

50. Phase memory relaxation times of spin labels in human carbonic anhydrase II: pulsed EPR to determine spin label location

Author

Uno Carlsson, Mikael Lindgren, Sandra S. Eaton, Gareth R. Eaton, Per Hammarström, M Huber, and Lars-Göran Mårtensson

Subjects

Chemistry, Pulsed EPR, Carbonic anhydrase II, Organic Chemistry, Relaxation (NMR), Biophysics, Electron Spin Resonance Spectroscopy, Site-directed spin labeling, Biochemistry, Carbonic Anhydrase II, law.invention, Nuclear magnetic resonance, Deuterium, Energy Transfer, law, Mutagenesis, Site-Directed, Humans, Spin Labels, Spin (physics), Spin label, Electron paramagnetic resonance, Half-Life

Abstract

Phase memory relaxation times (T(M) or T(2)) of spin labels in human carbonic anhydrase II (HCA II) are reported. Spin labels (N-(1-oxyl-2,2,5,5-tetramethyl-3-pyrrolidinyl)iodoacetamide, IPSL) were introduced at cysteines, by site-directed mutagenesis at seven different positions in the protein. By two pulse electron paramagnetic resonance (EPR), electron spin echo decays at 45 K are measured and fitted by stretched exponentials, resulting in relaxation parameters T(M) and x. T(M) values of seven positions are between 1.6 micros for the most buried residue (L79C) and 4.7 micros for a residue at the protein surface (W245C). In deuteriated buffer, longer T(M) are found for all but the most buried residues (L79C and W97C), and electron spin echo envelop modulation (ESEEM) of deuterium nuclei is observed. Different deuterium ESEEM patterns for W95C and W16C (surface residue) indicate differences in the local water concentration, or accessibility, of the spin label by deuterium. We propose T(M) as a parameter to determine the spin label location in proteins. Furthermore, these systems are interesting for studying the pertaining relaxation mechanism.

Published

2002