Your search keyword '"José L. Neira"' showing total 204 results

101. Binding of the C-terminal domain of the HIV-1 capsid protein to lipid membranes: a biophysical characterization

Author

María C. Lidón-Moya, Estefanía Hurtado-Gómez, Francisco N. Barrera, and José L. Neira

Subjects

Liposome, Calorimetry, Differential Scanning, C-terminus, Cell Biology, Phosphatidic acid, Plasma protein binding, Phosphatidylserine, Lipids, Biochemistry, Fluorescence, Protein Structure, Tertiary, chemistry.chemical_compound, chemistry, Capsid, Phosphatidylcholine, Liposomes, HIV-1, lipids (amino acids, peptides, and proteins), Capsid Proteins, Sphingomyelin, Molecular Biology, Protein Binding, Research Article

Abstract

The capsid protein, CA, of HIV-1 forms a capsid that surrounds the viral genome. However, recent studies have shown that an important proportion of the CA molecule does not form part of this capsid, and its location and function are still unknown. In the present work we show, by using fluorescence, differential scanning calorimetry and Fourier-transform infrared spectroscopy, that the C-terminal region of CA, CA-C, is able to bind lipid vesicles in vitro in a peripheral fashion. CA-C had a greater affinity for negatively charged lipids (phosphatidic acid and phosphatidylserine) than for zwitterionic lipids [PC/Cho/SM (equimolar mixture of phosphatidylcholine, cholesterol and sphingomyelin) and phosphatidylcholine]. The interaction of CA-C with lipid membranes was supported by theoretical studies, which predicted that different regions, occurring close in the three-dimensional CA-C structure, were responsible for the binding. These results show the flexibility of CA-C to undergo conformational rearrangements in the presence of different binding partners. We hypothesize that the CA molecules that do not form part of the mature capsid might be involved in lipid-binding interactions in the inner leaflet of the virion envelope.

Published

2006

102. Unfolding and Refolding in Vitro of a Tetrameric, α-Helical Membrane Protein: The Prokaryotic Potassium Channel KcsA

Author

José Antonio Encinar, M. Lourdes Renart, M. Luisa Molina, José A. Poveda, Asia M. Fernández, José L. Neira, José M. González-Ros, and Francisco N. Barrera

Subjects

Protein Denaturation, Protein Folding, Potassium Channels, Chemistry, Tetrameric protein, Circular Dichroism, Tryptophan, KcsA potassium channel, Membrane Proteins, Sodium Dodecyl Sulfate, Trifluoroethanol, Biochemistry, Potassium channel, Dissociation (chemistry), Electrophysiology, Potassium channel activity, Crystallography, Spectrometry, Fluorescence, Protein structure, Bacterial Proteins, Electrophoresis, Polyacrylamide Gel, Protein secondary structure

Abstract

2,2,2-Trifluoroethanol (TFE) effectively destabilizes the otherwise highly stable tetrameric structure of the potassium channel KcsA, a predominantly alpha-helical membrane protein [Valiyaveetil, F. I., Zhou, Y., and MacKinnon, R. (2002) Biochemistry 41, 10771-10777]. Here, we report that the effects on the protein structure of increasing concentrations of TFE in detergent solution include two successive protein concentration-dependent, cooperative transitions. In the first of such transitions, occurring at lower TFE concentrations, the tetrameric KcsA simultaneously increases the exposure of tryptophan residues to the solvent, partly loses its secondary structure, and dissociates into its constituent subunits. Under these conditions, simple dilution of the TFE permits a highly efficient refolding and tetramerization of the protein in the detergent solution. Moreover, following reconstitution into asolectin giant liposomes, the refolded protein exhibits nativelike potassium channel activity, as assessed by patch-clamp methods. Conversely, the second cooperative transition occurring at higher TFE concentrations results in the irreversible denaturation of the protein. These results are interpreted in terms of a protein and TFE concentration-dependent reversible equilibrium between the folded tetrameric protein and partly unfolded monomeric subunits, in which folding and oligomerization (or unfolding and dissociation in the other direction of the equilibrium process) are seemingly coupled processes. At higher TFE concentrations this is followed by the irreversible conversion of the unfolded monomers into a denatured protein form.

Published

2005

103. An extensive thermodynamic characterization of the dimerization domain of the HIV-1 capsid protein

Author

María C. Lidón-Moya, Raul Perez-Jimenez, Francisco N. Barrera, Mauricio G. Mateu, Javier Sancho, Marta Bueno, and José L. Neira

Subjects

Protein Denaturation, Protein Folding, Circular dichroism, Magnetic Resonance Spectroscopy, Protein Conformation, Dimer, Biochemistry, Anilino Naphthalenesulfonates, Fluorescence, Article, Dissociation (chemistry), chemistry.chemical_compound, Protein structure, Spectroscopy, Fourier Transform Infrared, Denaturation (biochemistry), Molecular Biology, Chemistry, Circular Dichroism, Tryptophan, Nuclear magnetic resonance spectroscopy, Hydrogen-Ion Concentration, Protein Structure, Tertiary, Crystallography, HIV-1, Anisotropy, Thermodynamics, Tyrosine, Capsid Proteins, Protein folding, Dimerization, Fluorescence anisotropy, Chromatography, Liquid

Abstract

The type 1 human immunodeficiency virus presents a conical capsid formed by several hundred units of the capsid protein, CA. Homodimerization of CA occurs via its C-terminal domain, CA-C. This self-association process, which is thought to be pH-dependent, seems to constitute a key step in virus assembly. CA-C isolated in solution is able to dimerize. An extensive thermodynamic characterization of the dimeric and monomeric species of CA-C at different pHs has been carried out by using fluorescence, circular dichroism (CD), absorbance, nuclear magnetic resonance (NMR), Fourier transform infrared (FTIR), and size-exclusion chromatography (SEC). Thermal and chemical denaturation allowed the determination of the thermodynamic parameters describing the unfolding of both CA-C species. Three reversible thermal transitions were observed, depending on the technique employed. The first one was protein concentration-dependent; it was observed by FTIR and NMR, and consisted of a broad transition occurring between 290 and 315 K; this transition involves dimer dissociation. The second transition (Tm approximately 325 K) was observed by ANS-binding experiments, fluorescence anisotropy, and near-UV CD; it involves partial unfolding of the monomeric species. Finally, absorbance, far-UV CD, and NMR revealed a third transition occurring at Tm approximately 333 K, which involves global unfolding of the monomeric species. Thus, dimer dissociation and monomer unfolding were not coupled. At low pH, CA-C underwent a conformational transition, leading to a species displaying ANS binding, a low CD signal, a red-shifted fluorescence spectrum, and a change in compactness. These features are characteristic of molten globule-like conformations, and they resemble the properties of the second species observed in thermal unfolding.

Published

2005

104. NMR for Chemists and Biologists

Author

Rodrigo J Carbajo, Jose L Neira, Rodrigo J Carbajo, and Jose L Neira

Subjects

Nuclear magnetic resonance

Abstract

This book intends to be an easy and concise introduction to the field of nuclear magnetic resonance or NMR, which has revolutionized life sciences in the last twenty years. A significant part of the progress observed in scientific areas like Chemistry, Biology or Medicine can be ascribed to the development experienced by NMR in recent times. Many of the books currently available on NMR deal with the theoretical basis and some of its main applications, but they generally demand a strong background in Physics and Mathematics for a full understanding. This book is aimed to a wide scientific audience, trying to introduce NMR by making all possible effort to remove, without losing any formality and rigor, most of the theoretical jargon that is present in other NMR books. Furthermore, illustrations are provided that show all the basic concepts using a naive vector formalism, or using a simplified approach to the particular NMR-technique described. The intention has been to show simply the foundations and main concepts of NMR, rather than seeking thorough mathematical expressions.

Published

2013

105. The inactivating factor of glutamine synthetase, IF7, is a 'natively unfolded' protein

Author

M. Isabel Muro-Pastor, José L. Neira, Francisco N. Barrera, José C. Reyes, and Francisco J. Florencio

Subjects

Protein Denaturation, Protein Folding, Circular dichroism, Magnetic Resonance Spectroscopy, Time Factors, Molecular Sequence Data, Biochemistry, Protein Structure, Secondary, Article, Bacterial Proteins, Glutamate-Ammonia Ligase, Glutamine synthetase, Spectroscopy, Fourier Transform Infrared, Amino Acid Sequence, Binding site, Molecular Biology, Protein secondary structure, Binding Sites, Chemistry, Circular Dichroism, Temperature, Glutamic acid, Protein tertiary structure, Protein Structure, Tertiary, Glutamine, Spectrometry, Fluorescence, Spectrophotometry, Chromatography, Gel, Protein folding

Abstract

Glutamine synthetase (GS) is the key enzyme responsible for the primary assimilation of ammonium in all living organisms, and it catalyses the synthesis of glutamine from glutamic acid, ATP, and ammonium. One of the recently discovered mechanisms of GS regulation involves protein-protein interactions with a small 65-residue-long protein named IF7. Here, we study the structure and stability of IF7 and its binding properties to GS, by using several biophysical techniques (fluorescence, circular dichroism, Fourier transform infrared and nuclear magnetic resonance spectroscopies, and gel filtration chromatography) which provide complementary structural information. The findings show that IF7 has a small amount of residual secondary structure, but lacks a well defined tertiary structure, and is not compact. Thus, all of the studies indicate that IF7 is a "natively unfolded" protein. The binding of IF7 to GS, its natural binding partner, occurs with an apparent dissociation constant of K(D) = 0.3 +/- 0.1 microM, as measured by fluorescence. We discuss the implications for the GS regulation mechanisms of IF7 being unfolded.

Published

2003

106. The histidine-phosphocarrier protein ofStreptomyces coelicolorfolds by a partially folded species at low pH

Author

Javier Maya, Javier Gómez, Alejandro Martín, Stephan Parche, Gregorio Fernández-Ballester, José L. Neira, and Fritz Titgemeyer

Subjects

Circular dichroism, biology, Chemistry, Size-exclusion chromatography, Streptomyces coelicolor, Phosphocarrier protein, biology.organism_classification, Biochemistry, Molten globule, Protein tertiary structure, Crystallography, biology.protein, Titration, Histidine

Abstract

The folding of a 93-residue protein, the histidine-phosphocarrier protein of Streptomyces coelicolor, HPr, has been studied using several biophysical techniques, namely fluorescence, 8-anilinonaphthalene-1-sulfate binding, circular dichroism, Fourier transform infrared spectroscopy, gel filtration chromatography and differential scanning calorimetry. The chemical-denaturation behaviour of HPr, followed by fluorescence, CD and gel filtration, at pH 7.5 and 25 °C, is described as a two-state process, which does not involve the accumulation of thermodynamically stable intermediates. Its conformational stability under those conditions is ΔG = 4.0 ± 0.2 kcal·mol−1 (1 kcal = 4.18 kJ), which makes the HPr from S. coelicolor the most unstable member of the HPr family described so far. The stability of the protein does not change significantly from pH 7–9, as concluded from the differential scanning calorimetry and thermal CD experiments. Conformational studies at low pH (pH 2.5–4) suggest that, in the absence of cosmotropic agents, HPr does not unfold completely; rather, it accumulates partially folded species. The transition from those species to other states with native-like secondary and tertiary structure, occurs with a pKa = 3.3 ± 0.3, as measured by the averaged measurements obtained by CD and fluorescence. However, this transition does not agree either with: (a) that measured by burial of hydrophobic patches (8-anilinonaphthalene-1-sulfate binding experiments); or (b) that measured by acquisition of native-like compactness (gel-filtration studies). It seems that acquisition of native-like features occurs in a wide pH range and it cannot be ascribed to a unique side-chain titration. These series of intermediates have not been reported previously in any member of the HPr family.

Published

2003

107. Structure and dynamics of the potato carboxypeptidase inhibitor by 1H and 15N NMR

Author

Salvador Ventura, Sílvia Bronsoms, F. X. Avilés, Carlos González, José L. Neira, and Manuel Rico

Subjects

Models, Molecular, Stereochemistry, Sequence (biology), Biochemistry, Protein Structure, Secondary, chemistry.chemical_compound, Structural Biology, Amide, Protease Inhibitors, Nuclear Magnetic Resonance, Biomolecular, Molecular Biology, Plant Proteins, Solanum tuberosum, Nitrogen Radioisotopes, biology, Nuclear magnetic resonance spectroscopy, Protein superfamily, Amides, Carboxypeptidase, Potato carboxypeptidase inhibitor, Folding (chemistry), Crystallography, chemistry, Helix, biology.protein, Protons, Hydrogen

Abstract

The solution structure and backbone dynamics of the recombinant potato carboxypeptidase inhibitor (PCI) have been characterized by NMR spectroscopy. The structure, determined on the basis of 497 NOE-derived distance constraints, is much better defined than the one reported in a previous NMR study, with an average pairwise backbone root-mean-square deviation of 0.5 A for the well-defined region of the protein, residues 7–37. Many of the side-chains show now well-defined conformations, both in the hydrophobic core and on the surface of the protein. Overall, the solution structure of free PCI is similar to the one that it shows in the crystal of the complex with carboxypeptidase A. However, some local differences are observed in regions 15–21 and 27–29. In solution, the six N-terminal and the two C-terminal residues are rather flexible, as shown by 15N backbone relaxation measurements. The flexibility of the latter segment may have implications in the binding of the inhibitor by the enzyme. All the remaining residues in the protein are essentially rigid (S2 > 0.8) with the exception of two of them at the end of a short 3/10 helix. Despite the small size of the protein, a number of amide protons are protected from exchange with solvent deuterons. The slowest exchanging protons are those in a small two-strand β-sheet. The unfolding free energies, as calculated from the exchange rates of these protons, are around 5 kcal/mol. Other protected amide protons are located in the segment 7–12, adjacent to the β-sheet. Although these residues are not in an extended conformation in PCI, the equivalent residues in structurally homologous proteins form a third strand of the central β-sheet. The amide protons in the 3/10 helix are only marginally protected, indicating that they exchange by a local unfolding mechanism, which is consistent with the increase in flexibility shown by some of its residues. Backbone alignment-based programs for folding recognition, as opposite to disulfide-bond alignments, reveal new proteins of unrelated sequence and function with a similar structure. Proteins 2003;50:410–422. © 2003 Wiley-Liss, Inc.

Published

2003

108. The carboxy-terminal domain of Erb1 is a seven-bladed ß-propeller that binds RNA

Author

Wegrecki Marcin, José L. Neira, and Jerónimo Bravo

Subjects

Multidisciplinary, lcsh:R, Protein domain, 5.8S ribosomal RNA, lcsh:Medicine, Ribosomal RNA, Biology, Molecular biology, 3. Good health, Cell biology, A-site, WD40 repeat, Ribosomal protein, lcsh:Q, lcsh:Science, Eukaryotic Ribosome, RRNA processing, Research Article

Abstract

22 páginas, 9 figuras, 1 tabla, Erb1 (Eukaryotic Ribosome Biogenesis 1) protein is essential for the maturation of the ribosomal 60S subunit. Functional studies in yeast and mammalian cells showed that altogether with Nop7 and Ytm1 it forms a stable subcomplex called PeBoW that is crucial for a correct rRNA processing. The exact function of the protein within the process remains unknown. The N-terminal region of the protein includes a well conserved region shown to be involved in PeBoW complex formation whereas the carboxy-terminal half was predicted to contain seven WD40 repeats. This first structural report on Erb1 from yeast describes the architecture of a seven-bladed β-propeller domain that revealed a characteristic extra motif formed by two α-helices and a β-strand that insert within the second WD repeat. We performed analysis of molecular surface and crystal packing, together with multiple sequence alignment and comparison of the structure with other β-propellers, in order to identify areas that are more likely to mediate protein-protein interactions. The abundance of many positively charged residues on the surface of the domain led us to investigate whether the propeller of Erb1 might be involved in RNA binding. Three independent assays confirmed that the protein interacted in vitro with polyuridilic acid (polyU), thus suggesting a possible role of the domain in rRNA rearrangement during ribosome biogenesis., This work was supported by the European Community, Seventh Framework Programme (FP7/2007-2013) under BioStruct-X (grant agreement N°283570) to JB; Ministerio de Economía y Competitividad, SAF2012-31405 to JB and CSD2008-00005 and CTQ2013-4493 to JLN; and Generalitat Valenciana PROMETEO/2012/061 (JB) and 2013/018 (JLN). MW received a JAE-PREDOC fellowship from Consejo Superior de Investigaciones Científicas, Spain. The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.

Published

2015

109. Biophysical analysis of the MHR motif in folding and domain swapping of the HIV capsid protein C-terminal domain

Author

Alicia Rodríguez-Huete, Miguel Fuertes, Mauricio G. Mateu, José L. Neira, Rebeca Bocanegra, Ministerio de Economía y Competitividad (España), Comunidad de Madrid, and Fundación Ramón Areces

Subjects

Protein Folding, Dimer, viruses, Amino Acid Motifs, Molecular Sequence Data, Biophysics, environment and public health, chemistry.chemical_compound, Retrovirus, Amino Acid Sequence, Peptide sequence, chemistry.chemical_classification, biology, Protein Stability, C-terminus, fungi, HIV, biology.organism_classification, Amino acid, Protein Structure, Tertiary, Biochemistry, chemistry, Capsid, health occupations, Protein folding, Capsid Proteins, CTD, Protein Multimerization, Proteins and Nucleic Acids

Abstract

© 2015 Biophysical Society. Infection by human immunodeficiency virus (HIV) depends on the function, in virion morphogenesis and other stages of the viral cycle, of a highly conserved structural element, the major homology region (MHR), within the carboxyterminal domain (CTD) of the capsid protein. In a modified CTD dimer, MHR is swapped between monomers. While no evidence for MHR swapping has been provided by structural models of retroviral capsids, it is unknown whether it may occur transiently along the virus assembly pathway. Whatever the case, the MHR-swapped dimer does provide a novel target for the development of anti-HIV drugs based on the concept of trapping a nonnative capsid protein conformation. We have carried out a thermodynamic and kinetic characterization of the domain-swapped CTD dimer in solution. The analysis includes a dissection of the role of conserved MHR residues and other amino acids at the dimerization interface in CTD folding, stability, and dimerization by domain swapping. The results revealed some energetic hotspots at the domain-swapped interface. In addition, many MHR residues that are not in the protein hydrophobic core were nevertheless found to be critical for folding and stability of the CTD monomer, which may dramatically slow down the swapping reaction. Conservation of MHR residues in retroviruses did not correlate with their contribution to domain swapping, but it did correlate with their importance for stable CTD folding. Because folding is required for capsid protein function, this remarkable MHR-mediated conformational stabilization of CTD may help to explain the functional roles of MHR not only during immature capsid assembly but in other processes associated with retrovirus infection. This energetic dissection of the dimerization interface in MHR-swapped CTD may also facilitate the design of anti-HIV compounds that inhibit capsid assembly by conformational trapping of swapped CTD dimers., Spanish Government (BIO2012-37649) and Comunidad de Madrid (S-2009/MAT/1467) and by an institutional grant from Fundación Ramón Areces.

Published

2015

110. Equilibrium Unfolding of the C-Terminal SAM Domain of p73

Author

José L. Neira, Francisco N. Barrera, Javier Gómez, and María T. Garzón

Subjects

Models, Molecular, Protein Denaturation, Protein Folding, Circular dichroism, Amino Acid Motifs, Equilibrium unfolding, Biochemistry, Deprotonation, Spectroscopy, Fourier Transform Infrared, Genes, Tumor Suppressor, Denaturation (biochemistry), Tyrosine, chemistry.chemical_classification, Calorimetry, Differential Scanning, Chemistry, Circular Dichroism, Tumor Suppressor Proteins, Temperature, Nuclear Proteins, Tumor Protein p73, Hydrogen-Ion Concentration, Fluorescence, Protein Structure, Tertiary, Amino acid, DNA-Binding Proteins, Kinetics, Crystallography, Spectrometry, Fluorescence, Thermodynamics, Sterile alpha motif

Abstract

The sterile alpha motif (SAM) domain is a protein module of approximately 65 to 70 amino acids found in many diverse proteins whose functions range from signal transduction to transcriptional repression. The alpha splice variant of p73 (p73 alpha), a homologue of the tumor suppressor p53, has close to its C-terminus a SAM motif. Here, we report the folding equilibrium properties of the p73 alpha SAM domain (SAMp73) by using different biophysical techniques (circular dichroism, fluorescence, and Fourier transform infrared spectroscopies, and differential scanning calorimetry). Those probes indicate that SAMp73 folds via a two-state mechanism. Fluorescence experiments performed at different pHs showed two titrations: the first one due to an acid residue (with a pK(a) = 4.5 +/- 0.3) and the second due to deprotonation of tyrosine residues. The conformational stability of the protein upon chemical denaturation was determined over the pH range 3 to 10. The maximum conformational stability is DeltaG = 5.7 +/- 0.4 kcal x mol(-1) (at 25 degrees C) and occurs in a broad maximum, with little variation, between pH 6 and 10. The high melting temperature of SAMp73 (T(m) = 93.5 degrees C), despite its moderate conformational stability at 25 degrees C, can be ascribed to its low heat capacity change upon unfolding, DeltaC(p), which is estimated to be around 915 cal x K(-1) x mol(-1) at 25 degrees C and only around 543 cal x K(-1) x mol(-1) at the T(m). The implications of the temperature-dependent nature of DeltaC(p) are discussed in relation to the thermal stability of proteins as opposed to their conformational stability at room temperature.

Published

2002

111. NUPR1 deficiency induces metabolic cell death

Author

Juan L. Iovanna, José L. Neira, Raul Urrutia, Jennifer Bintz, Gwen Lomberk, and Patricia Santofimia Castańo

Subjects

Programmed cell death, Hepatology, business.industry, Endocrinology, Diabetes and Metabolism, Gastroenterology, Cancer research, Medicine, business

Published

2017

112. Three-Dimensional Solution Structure and Stability of Thioredoxin m from Spinach

Author

José L. Neira, Carlos González, G. de Prat-Gay, C. Toiron, and M. Rico

Subjects

Models, Molecular, Guanidinium chloride, Protein Folding, Circular dichroism, Magnetic Resonance Spectroscopy, Molecular Sequence Data, Nuclear Overhauser effect, Crystallography, X-Ray, Biochemistry, Protein Structure, Secondary, chemistry.chemical_compound, Thioredoxins, Drug Stability, Spinacia oleracea, PROTEIN FOLDING, Denaturation (biochemistry), Amino Acid Sequence, biology, Otras Ciencias Químicas, Circular Dichroism, Ciencias Químicas, Active site, PROTEIN STRUCTURE, Nuclear magnetic resonance spectroscopy, Amides, Solutions, Crystallography, chemistry, THIOREDOXIN, biology.protein, Proton NMR, Thermodynamics, Protons, Thioredoxin, Crystallization, Dimerization, Oxidation-Reduction, CIENCIAS NATURALES Y EXACTAS

Abstract

Proton NMR spectral resonances of thioredoxin m from spinach have been assigned, and its solution structure has been determined on the basis of 1156 nuclear Overhauser effect- (NOE-) derived distance constraints by using restrained molecular dynamics calculations. The average pairwise root-mean-square deviation (RMSD) for the 25 best NMR structures for the backbone was 1.0 +/- 0.1, when the structurally well-defined residues were considered. The N- and C-terminal segments (1-13 and 118-119) and residues 41-49, comprising the active site, are highly disordered. At the time of concluding this work, a crystal structure of this protein was reported, in which thioredoxin m was found to crystallize as noncovalent dimers. Although the solution and crystal structures are very similar, no evidence was found about the existence of dimers in solution, thus confirming that dimerization is not needed for the regulatory activity of thioredoxin m. The spinach thioredoxin m does not unfold by heat in the range 25-85 degrees C, as revealed by thermal circular dichroic (CD) measurements. However, its unfolding free energy (9.1 +/- 0.8 kcal mol(-1), at pH 5.3 and 25 degrees C) could be determined by extrapolating the free energy values obtained at different concentrations of guanidinium chloride (GdmCl). The folding-unfolding process is two-state as indicated by the coincidence of the CD denaturation curves obtained at far and near UV. The H/D exchange behavior of backbone amide protons was analyzed. The slowest-exchanging protons, requiring a global-unfolding mechanism in order to exchange, are those from beta2, beta3, and beta4, the central strands of the beta-sheet, which constitute the main element of the core of the protein. The free energies obtained from exchange measurements of protons belonging to the alpha-helices are lower than those derived from GdmCl denaturation studies, indicating that those protons exchange by local-unfolding mechanisms. Fil: Neira, José L.. Universidad de Miguel Hernández; España Fil: González, Carlos. Consejo Superior de Investigaciones Científicas; España Fil: Toiron, Catherine. Consejo Superior de Investigaciones Científicas; España Fil: de Prat Gay, Gonzalo. Consejo Nacional de Investigaciones Científicas y Técnicas. Oficina de Coordinación Administrativa Parque Centenario. Instituto de Investigaciones Bioquímicas de Buenos Aires. Fundación Instituto Leloir. Instituto de Investigaciones Bioquímicas de Buenos Aires; Argentina. Consejo Nacional de Investigaciones Científicas y Técnicas. Oficina de Coordinación Administrativa Ciudad Universitaria. Instituto de Química Biológica de la Facultad de Ciencias Exactas y Naturales. Universidad de Buenos Aires. Facultad de Ciencias Exactas y Naturales. Instituto de Química Biológica de la Facultad de Ciencias Exactas y Naturales; Argentina Fil: Rico, Manuel. Consejo Superior de Investigaciones Científicas; España

Published

2001

113. Hydrogen exchange of the tetramerization domain of the human tumour suppressor p53 probed by denaturants and temperature

Author

José L. Neira and Mauricio G. Mateu

Subjects

Circular dichroism, Crystallography, Protein structure, Chemistry, Hydrogen bond, Beta sheet, Hydrogen–deuterium exchange, Protein folding, Biochemistry, Protein secondary structure, Alpha helix

Abstract

We have analysed the hydrogen/deuterium exchange of the tetramerization domain of human tumour suppressor p53 under mild chemical denaturation conditions, and at different temperatures. Exchange behaviour has been measured for 16 amide protons in the chemical-denaturation studies and for seven protons in the temperature-denaturation studies. The exchange rates are in the range observed for other proteins with similar elements of secondary structure. The slowest-exchange core includes contributions from residues in the alpha helix and the beta sheet. However, only some of the slowest-exchanging protons correspond to residues involved in native interactions in the transient intermediate detected during the folding of this domain. The guanidinium-chloride denaturation curves of all residues seem to merge together, although they are well below the main isotherm of global unfolding. Thus, there is no evidence for several subglobal unfolding units. The activation parameters obtained from the temperature-denaturation experiments are similar to those obtained for monomeric proteins, and well below the global unfolding enthalpy obtained by circular dichroism measurements. Thus, the exchange studies at different denaturant concentrations and temperatures indicate that no particular folding intermediate is populated under those conditions.

Published

2001

114. Human p8 Is a HMG-I/Y-like Protein with DNA Binding Activity Enhanced by Phosphorylation

Author

Eduardo T. Cánepa, Cynthia Mizyrycki, José M. González-Ros, José Antonio Encinar, Gustavo V. Mallo, José L. Neira, Manuel Rico, Juan L. Iovanna, Silvia N.J. Moreno, and Luciana E. Giono

Subjects

Circular dichroism, Molecular Sequence Data, Plasma protein binding, Biochemistry, DNA-binding protein, Protein Structure, Secondary, chemistry.chemical_compound, Spectroscopy, Fourier Transform Infrared, Basic Helix-Loop-Helix Transcription Factors, Humans, Amino Acid Sequence, HMGA1a Protein, Phosphorylation, Growth Substances, Protein kinase A, Nuclear Magnetic Resonance, Biomolecular, Molecular Biology, Peptide sequence, Protein secondary structure, Conserved Sequence, Sequence Homology, Amino Acid, Chemistry, Circular Dichroism, High Mobility Group Proteins, Cell Biology, Cyclic AMP-Dependent Protein Kinases, Neoplasm Proteins, Protein Structure, Tertiary, DNA-Binding Proteins, High-mobility group, DNA, Protein Binding, Transcription Factors

Abstract

We have studied the biochemical features, the conformational preferences in solution, and the DNA binding properties of human p8 (hp8), a nucleoprotein whose expression is affected during acute pancreatitis. Biochemical studies show that hp8 has properties of the high mobility group proteins, HMG-I/Y. Structural studies have been carried out by using circular dichroism (near- and far-ultraviolet), Fourier transform infrared, and NMR spectroscopies. All the biophysical probes indicate that hp8 is monomeric (up to 1 mm concentration) and partially unfolded in solution. The protein seems to bind DNA weakly, as shown by electrophoretic gel shift studies. On the other hand, hp8 is a substrate for protein kinase A (PKA). The phosphorylated hp8 (PKAhp8) has a higher content of secondary structure than the nonphosphorylated protein, as concluded by Fourier transform infrared studies. PKAhp8 binds DNA strongly, as shown by the changes in circular dichroism spectra, and gel shift analysis. Thus, although there is not a high sequence homology with HMG-I/Y proteins, hp8 can be considered as a HMG-I/Y-like protein.

Published

2001

115. Stability and folding of the protein complexes of barnase

Author

José L. Neira, Eugenio Vázquez, and Alan R. Fersht

Subjects

Barnase, Circular dichroism, Crystallography, biology, Chemistry, biology.protein, Protein folding, Denaturation (biochemistry), Phi value analysis, Nuclear magnetic resonance spectroscopy, Plasma protein binding, Cleavage (embryo), Biochemistry

Abstract

Native-like complexes of proteins, formed by the association of two complementary fragments comprising the entire sequence of the protein, can be used to gain insight into the stability and folding of the intact protein. We have studied the structural, thermodynamic and kinetic properties of four barnase complexes, with the cleavage site at different positions of the amino-acid chain (CB36, at position 36; CB56, at position 56; CB68, at position 68; and CB79, at position 79). The four barnase complexes have native-like structure as shown by fluorescence, far-and near-UV CD, size-exclusion chromatography and NMR. The NMR characterization indicated that the structural changes were mainly located in regions close to the cleavage site. The main core of the protein was fully formed and the overall structure was similar to that of intact barnase. The thermal and chemical denaturation showed that all complexes were substantially destabilized. CB56 displayed two denaturation transitions, probably because of the presence of partially folded conformations around the cleavage site. The rate constant for the association/folding of fragments decreased with the decreasing length of the C-terminal fragment. Thus, the larger the fragment (and, consequently, the larger the amount of residual native-like structure), the faster the association. These findings are consistent with the proposed model of barnase folding.

Published

2000

116. The Helical Structure Propensity in the First Helix of the Histidine Phosphocarrier Protein of Streptomyces coelicolor

Author

Alicia Prieto, Estefanía Hurtado-Gómez, Marco Caprini, José L. Neira, Estefanía Hurtado-Gómez, Marco Caprini, Alicia Prieto, and José L. Neira

Subjects

Protein Folding, Molecular Sequence Data, Peptide, Streptomyces coelicolor, Phosphocarrier protein, macromolecular substances, Biochemistry, Protein Structure, Secondary, Diffusion, Protein structure, Bacterial Proteins, Structural Biology, Amino Acid Sequence, Phosphoenolpyruvate Sugar Phosphotransferase System, Peptide sequence, Polytetrafluoroethylene, chemistry.chemical_classification, biology, Circular Dichroism, Water, General Medicine, Protein engineering, PEP group translocation, biology.organism_classification, Magnetic Resonance Imaging, Peptide Fragments, chemistry, biology.protein, Mutagenesis, Site-Directed, Solvents, bacteria, Protein folding

Abstract

The bacterial phosphoenolpyruvate (PEP):sugar phosphotransferase system (PTS), formed by a cascade of several proteins, mediates the uptake and phosphorylation of carbohydrates, and it is also involved in signal transduction. Its uniqueness in bacteria makes the PTS a target for new antibacterial drugs. These drugs can be obtained from peptides or proteins fragments able to interfere the first step of the protein cascade: the phosphorylation of the HPr protein by the enzyme EI. We designed a peptide comprising the active site and the first α-helix of HPr of S. coelicolor; we also obtained a fragment of HPr by protein engineering methods, comprising the first forty-eight residues and thus, containing the amino acids of the shorter peptide. Both fragments were disordered in aqueous solution, with a similar percentage of helical structure (∼7 %), and an identical free energy of helix formation. In 40 % TFE, both fragments acquired native-like helical structure, stabilized by non-native hydrophobic interactions, as shown by the 2D-NMR assignments of the shorter peptide, and the presence of similar NOE contacts in both fragments. These findings, with the kinetic results in other members of the HPr family, highlight the importance of short- and long-range interactions during the folding reaction of HPr proteins. Based on the residual helical population, hypothesis about the inhibition capacity of the PTS by both fragments are discussed. © 2007 Bentham Science Publishers Ltd.

Published

2007

117. Acquisition of native-like interactions in C-terminal fragments of barnase 1 1Edited by J. Karn

Author

Alan R. Fersht and José L. Neira

Subjects

Barnase, Circular dichroism, biology, Chemistry, Fast protein liquid chromatography, Fluorescence, Protein tertiary structure, Folding (chemistry), Crystallography, Protein structure, Structural Biology, biology.protein, Protein folding, Molecular Biology

Abstract

We have characterised a series of C-terminal fragments of barnase by different biophysical techniques to find out when they acquire secondary and tertiary native-like structure. Fragments B96-110 (which comprises the last 15 residues of the intact protein) up to B37-110 (which involves most of the protein except the two first helices and a loop) were mainly disordered. Only fragment B23-110, which lacks alpha-helix1, showed native-like near and far-UV CD and fluorescence spectra. The intensities of these spectra were lower than those of the full-length protein, which suggests the absence of complete side-chain packing. Urea denaturation followed by fluorescence, far-UV CD and gel-filtration chromatography techniques indicated a co-operative transition only for B23-110. None of the fragments melted co-operatively with temperature. Thus, the formation of secondary and tertiary structure requires most of the polypeptide chain to be present, that is, secondary and tertiary structure are formed in parallel. This agrees with the proposed model for barnase folding, where the residual structure in small fragments is weak and flickering, and it is only consolidated when there are enough tertiary interactions. Thus, the development of structure in the series of C-terminal fragments follows a similar behaviour to that observed in the series of N-terminal fragments of barnase.

Published

1999

118. Exploring the Folding Funnel of a Polypeptide Chain by Biophysical Studies on Protein Fragments

Author

Alan R. Fersht and José L. Neira

Subjects

Protein Denaturation, Protein Folding, Magnetic Resonance Spectroscopy, Molecular Sequence Data, Phi value analysis, Protein Structure, Secondary, Ribonucleases, Bacterial Proteins, Structural Biology, Protein biosynthesis, Urea, Amino Acid Sequence, Folding funnel, Molecular Biology, Protein secondary structure, Barnase, biology, Chemistry, Circular Dichroism, Temperature, Hydrogen-Ion Concentration, GroEL, Peptide Fragments, Protein Structure, Tertiary, Crystallography, Spectrometry, Fluorescence, Chaperone (protein), Chromatography, Gel, biology.protein, Biophysics, Protein folding

Abstract

We are examining possible roles of native and non-native interactions in early events in protein folding by a systematic analysis of the structures of fragments of proteins whose folding pathways are well characterised. Seven fragments of the 110-residue protein barnase, corresponding to the progressive elongation from its N terminus, have been characterised by a battery of biophysical and spectroscopic methods. Barnase is a multi-modular protein that folds via an intermediate in which the C-terminal region of its major alpha-helix (alpha-helix1, residues Thr6-His18) is substantially formed as is also its anti-parallel beta-sheet, centred around a beta-hairpin (residues Ser92-Leu95). Fragments up to, and including, residues 1-95 (fragment B95), appeared to be mainly disordered, although a small amount of helical secondary structure in each was inferred from far-UV CD experiments, and fluorescence studies indicated some native-like tertiary interactions in B95. The largest fragment (residues 1-105, B105) is compactly folded. The secondary structure in alpha-helix1 in the seven fragments was found by NMR to increase with increasing chain length faster than the build-up of tertiary interactions, indicating that alpha-helix1 is being stabilised by non-native interactions. This behaviour contrasts with that in fragments of the 64-residue chymotrypsin inhibitor 2 (CI2), in which tertiary and secondary structures build up in parallel with increasing length. CI2 consists of a single module of structure that folds without a detectable intermediate. The largest fragment of barnase, B105, has interactions that resemble its folding intermediate, whereas one of the largest fragments of CI2 (residues 1-60) resembles the folding transition state. The folding pathways of both proteins are consistent with a scheme in which there are low levels of native-like secondary structure in the denatured state that become stabilised by long-range interactions as folding proceeds. Neither protein forms a stable fold when lacking the last ten residues at the C terminus. Since at least 20 amino acid residues are bound to the ribosome during protein biosynthesis, these small proteins do not fold until they have left the ribosome, and so the studies of the folding of such proteins in vitro may be relevant to their folding in vivo, especially as the molecular chaperone GroEL binds only weakly to denatured CI2 and does not discernibly alter the folding mechanism of barnase.

Published

1999

119. Hydrogen exchange in ribonuclease A and ribonuclease S: evidence for residual structure in the unfolded state under native conditions 1 1Edited by P. E. Wright

Author

José L. Neira, Marta Bruix, Manuel Rico, Margarita Menéndez, and Paz Sevilla

Subjects

Crystallography, Protein structure, Proton, Structural Biology, Chemistry, RNase P, Native state, Denaturation (biochemistry), Protein folding, Nuclear magnetic resonance spectroscopy, Molecular Biology, Equilibrium constant

Abstract

Two-dimensional NMR spectroscopy has been used to monitor the exchange of backbone amide protons in ribonuclease A (RNase A) and its subtilisin-cleaved form, ribonuclease S (RNase S). Exchange measurements at two different pH values (5.4 and 6.0) show that the exchange process occurs according to the conditions of the EX2 limit. Differential scanning calorimetry measurements have been carried out in 2H2O under conditions analogous to those used in the NMR experiments in order to determine the values of DeltaCp, DeltaHu and Tm, corresponding to the thermal denaturation of both proteins. For the amide protons of a large number of residues in RNase A, the free energies at 25 degreesC for exchange competent unfolding processes are much lower than the calorimetric denaturation free energies, thus showing that exchange occurs through local fluctuations in the native state. For 20 other protons, the cleavage reaction had approximately the same effect on the exchange rate constants than on the equilibrium constant for unfolding, indicating that those protons exchange by global unfolding. There is a good agreement between the residues to which these protons belong and those involved in the putative folding nucleation site identified by quench-flow NMR studies. The unfolding free energies of the slowest exchanging protons, DeltaGex, as evaluated from exchange data, are much larger than the calorimetric free energies of unfolding, DeltaGu. Given the agreement between DeltaDeltaGex(A-S), the difference in free energy from exchange for a given proton of the two proteins, and DeltaDeltaGu(A-S), the difference in the calorimetric free energy of the two proteins, the discrepancy indicates that the intrinsic exchange rates in the unfolded state of those protons cannot be approximated by those measured in short unstructured peptides and, consequently, exchange for those protons in RNase A and S must occur through a rather structured denatured state.

Published

1999

120. The isolated N terminus of Ring1B is a well-folded, monomeric fragment with native-like structure

Author

Julio Bacarizo, Ana Cámara-Artigas, José L. Neira, Sandra Villegas, Ana Isabel Martínez-Gómez, David Aguado-Llera, and Miguel Vidal

Subjects

Polycomb Repressive Complex 1, Protein Folding, biology, Stereochemistry, Chemistry, Protein Stability, Spectrum Analysis, Repressor, Bioengineering, macromolecular substances, Biochemistry, N-terminus, medicine.anatomical_structure, Ubiquitin, Histone H2A, biology.protein, Ring finger, medicine, Humans, Protein folding, PRC1, PRC2, Molecular Biology, Biotechnology

Abstract

The Polycomb group (PcG) proteins assemble into Polycomb repressive complexes (PRCs), PRC1 and PRC2, which act as general transcriptional repressors. PRC1 comprises a variety of biochemical entities endowed with histone H2A monoubiquitylation activity conferred by really interesting new gene (RING) finger E3 ubiquitin ligases Ring1A and Ring1B. All PRC1 complexes contain Ring1 proteins which are essential for Polycomb epigenetic regulation. We have been able to express the isolated N-terminal region of Ring1B, N-Ring1B, comprising the first 221 residues of the 334-residue-long Ring1B. This fragment contains the 41-residue-long RING finger motif, and flanking sequences that form an interacting platform for PcG and non-PcG proteins. We found that the N-Ring1B is a well-folded, monomeric fragment, with native-like structure which unfolds irreversibly. The protein is capable of binding to an ubiquitin-conjugase protein (with an 85% of sequence similarity to the Ring1B physiological partner) with moderate affinity. © The Author 2013.

Published

2013

121. Nuclear magnetic resonance spectroscopy to study virus structure

Author

José L, Neira

Subjects

Models, Molecular, Viruses, Animals, Humans, Nuclear Magnetic Resonance, Biomolecular

Abstract

Nuclear magnetic resonance (NMR) is a spectroscopic technique based in the absorption of radiofrequency radiation by atomic nuclei in the presence of an external magnetic field. NMR has followed a "bottom-up" approach to solve the structures of isolated domains of viral proteins, including capsid protein subunits. NMR has been instrumental to describe conformational changes in viral proteins and nucleic acids, showing the presence of dynamic equilibria which are thought to be important at different stages of the virus life cycle; in this sense, NMR is also the only technique currently available to describe, in atomic detail, the conformational preferences of natively unfolded viral proteins. NMR has also complemented X-ray crystallography and has been combined with electron microscopy to obtain pseudo-atomic models of entire virus capsids. Finally, the joint use of liquid and solid-state NMR has allowed the identification of conformational changes in intact viral capsids on insertion in host membranes.

Published

2013

122. Fluorescence, circular dichroism and mass spectrometry as tools to study virus structure

Author

José L, Neira

Subjects

Models, Molecular, Circular Dichroism, Viruses, Animals, Humans, Fluorescence, Mass Spectrometry

Abstract

Fluorescence and circular dichroism, as analytical spectroscopic techniques, and mass spectrometry as an analytical tool to determine the molecular mass, provide important biophysical approaches in structural virology. Although they do not provide atomic, or near-atomic, details as electron microscopy, X-ray crystallography or nuclear magnetic resonance spectroscopy can do, they do provide important insights into virus particle composition, structure, conformational stability and dynamics, assembly and maturation, and interactions with other viral and cellular biomolecules. They can be used also to investigate the molecular determinants of virus particle structure and properties, and the changes induced in them by external factors. In this chapter, I describe the physical bases of these three techniques, and some examples on how they have helped us to understand virus particle structure and physicochemical properties.

Published

2013

123. The histidine-phosphocarrier protein of the phosphoenolpyruvate: sugar phosphotransferase system of Bacillus sphaericus self-associates

Author

Claudio N. Cavasotto, Ana Isabel Díez-Peña, José García de la Torre, Julio Bacarizo, Ana Cámara-Artigas, José G. Hernández-Cifre, Sergio Martínez-Rodríguez, Adrián Velázquez-Campoy, José L. Neira, Rosa Doménech, Ministerio de Ciencia e Innovación (España), European Commission, Diputación General de Aragón, Junta de Andalucía, Agencia Nacional de Promoción Científica y Tecnológica (Argentina), and Instituto de Biocomputación y Física de Sistemas Complejos (España)

Subjects

Models, Molecular, Proteomics, BACILUS SPHAERICUS, Protein Denaturation, Protein Folding, Hot Temperature, lcsh:Medicine, Bacillus, Plasma protein binding, Bacillus sphaericus, Biochemistry, Protein Structure, Secondary, purl.org/becyt/ford/1 [https], Protein structure, ENZYME I, Macromolecular Structure Analysis, Phosphorylation, Biomacromolecule-Ligand Interactions, lcsh:Science, Multidisciplinary, biology, Physics, Streptomyces coelicolor, PEP group translocation, Bioquímica y Biología Molecular, Hydrogen-Ion Concentration, PROTEIN-PROTEIN INTERACTION, Thermodynamics, Phosphoenolpyruvate carboxykinase, CIENCIAS NATURALES Y EXACTAS, Protein Binding, Research Article, Protein Structure, Biophysics, Phosphocarrier protein, macromolecular substances, Calorimetry, Protein Chemistry, Ciencias Biológicas, Bacterial Proteins, Histidine, purl.org/becyt/ford/1.6 [https], Phosphoenolpyruvate Sugar Phosphotransferase System, Protein Interactions, Biology, lcsh:R, fungi, Proteins, Computational Biology, biology.organism_classification, carbohydrates (lipids), Spectrometry, Fluorescence, HISTIDINE-PHOSPHOCARRIER PROTEIN, biology.protein, Hydrodynamics, bacteria, lcsh:Q, Peptides

Abstract

15 pags, 7 figs, 1 tab, The phosphotransferase system (PTS) is involved in the use of carbon sources in bacteria. Bacillus sphaericus, a bacterium with the ability to produce insecticidal proteins, is unable to use hexoses and pentoses as the sole carbon source, but it has ptsHI genes encoding the two general proteins of the PTS: enzyme I (EI) and the histidine phosphocarrier (HPr). In this work, we describe the biophysical and structural properties of HPr from B. sphaericus, HPrbs, and its affinity towards EI of other species to find out whether there is inter-species binding. Conversely to what happens to other members of the HPr family, HPrbs forms several self-associated species. The conformational stability of the protein is low, and it unfolds irreversibly during heating. The protein binds to the N-terminal domain of EI from Streptomyces coelicolor, EINsc, with a higher affinity than that of the natural partner of EINsc, HPrsc. Modelling of the complex between EINsc and HPrbs suggests that binding occurs similarly to that observed in other HPr species. We discuss the functional implications of the oligomeric states of HPrbs for the glycolytic activity of B. sphaericus, as well as a strategy to inhibit binding between HPrsc and EINsc. © 2013 Doménech et al., This work was supported by the Spanish Ministerio de Ciencia e Innovación (MCINN) (CTQ2011-24393, and CSD2008-00005 to JLN; BIO2009-13261-C02- 01/02 and P09-CVI-5063, with Fondo Social Europeo (ESF) to ACA; and BFU2010-19451 to AVC), Diputación General de Aragón (PI044/09 to AVC), intramural BIFI 2011 projects (to AVC and JLN), Junta de Andalucía (BIO-328 to ACA), and by grants from the Agencia Nacional de Promoción Científica y Tecnológica Argentina (ANPCyT; PICT-2011-2778) (to CNC). SMR was supported by the CSD2008-00005. The stays of RD in the laboratory of AVC were supported by the Spanish Ministerio de Ciencia e Innovación (BFU2008-02302-BMC).

Published

2013

124. Protein folding and stability: a Prague cemetery

Author

José L. Neira

Subjects

Protein Folding, Biopolymers, Chemistry, Biophysics, Stability (learning theory), Proteins, Protein folding, Computational biology, Molecular Biology, Biochemistry

Published

2013

125. An NMR study on the β-hairpin region of barnase

Author

José L. Neira and Alan R. Fersht

Subjects

Models, Molecular, nucleation site, Protein Denaturation, Protein Folding, Magnetic Resonance Spectroscopy, Protein Conformation, Molecular Sequence Data, Nucleation, Biochemistry, Protein Structure, Secondary, Ribonucleases, Bacterial Proteins, tertiary interactions, unfolded states, Urea, Aromatic moiety, Amino Acid Sequence, Barnase, biology, Chemistry, Chemical shift, Intact protein, Protein engineering, Peptide Fragments, Crystallography, Docking (molecular), biology.protein, Thermodynamics, Molecular Medicine, Protein folding

Abstract

Backgound: The β -hairpin of barnase (residues Ser92–Leu95) has been proposed in theoretical and protein engineering studies to be an initiation site for folding [1]. There is evidence for residual structure in this region from NMR studies of the denatured protein under different denaturing conditions [2,3]. A more detailed analysis is possible by NMR studies of isolated fragments. Results: Protons of fragments B(80–110) and B(69–110) in 6 M urea have non-random chemical shifts. Non-native long-range and medium-range NOE contacts with the aromatic moiety of Trp94 indicate that it is involved in a β -turn-like or α -helix-like conformation. Also, the sidechains of Trp71, Tyr79, Phe82, Tyr90, Tyr97, His102, Tyr103 and Phe106 show non-native hydrophobic contacts. Non-random conformational shifts and sequential NN( i , i +1) NOE contacts are clustered to one of the β -strands and one of the loop regions. Conclusion: The hairpin region of barnase adopts β -turn-like or α -helix-like conformations, which are weakly populated even in 6 M urea. The hairpin region is a potential nucleation site in folding that may consolidate on docking with the first α -helix. The other residues that have conformational preferences form a β -strand and one of the loop regions in the native intact protein, but they do not constitute a nucleation site.

Published

1996

126. Towards the complete structural characterization of a protein folding pathway: the structures of the denatured, transition and native states for the association/folding of two complementary fragments of cleaved chymotrypsin inhibitor 2. Direct evidence for a nucleation-condensation mechanism

Author

José L Neira, Ben Davis, Andreas G Ladurner, Ashley M Buckle, Gonzalo de Prat Gay, and Alan R Fersht

Subjects

Models, Molecular, Protein Denaturation, Protein Folding, Magnetic Resonance Spectroscopy, Protein Conformation, Molecular Sequence Data, Phi value analysis, Crystallography, X-Ray, Protein Engineering, Biochemistry, Protein Structure, Secondary, medicine, Chymotrypsin, Amino Acid Sequence, Protein secondary structure, X-ray crystallography, Plant Proteins, Molecular Structure, Chemistry, nucleus, Nuclear magnetic resonance spectroscopy, Protein engineering, Contact order, NMR, Peptide Fragments, Molten globule, Solutions, Crystallography, medicine.anatomical_structure, Molecular Medicine, Phi-value, Crystallization, Peptides, Ground state, Nucleus

Abstract

Backgound: Single-module proteins, such as chymotrypsin inhibitor 2 (CI2), fold as a single cooperative unit. To solve its folding pathway, we must characterize, under conditions that favour folding, its denatured state, its transition state, and its final folded structure. To obtain a ‘denatured state' that can readily be thus characterized, we have used a trick of cleaving CI2 into two complementary fragments that associate and fold in a similar way to intact protein. Results: Fragment CI2(1–40) – which contains the sequence of the single α -helix, spanning residues 12–24 – and CI2(41–64), and mutants thereof, were analyzed by NMR spectroscopy, the transition state for association/folding was characterized by the protein engineering method, and the structure of the complex was solved by NMR and X-ray crystallography. Both isolated fragments are largely disordered. The transition state for association/folding is structured around a nucleus of a nearly fully formed α -helix, as is the transition state for the folding of intact CI2, from residues Ser12 to Leu21. Ala16, a residue from the helix whose sidechain is buried in the hydrophobic core, makes interactions with Leu49 and Ile57 in the other fragment. Ala16 makes its full interaction energy in the transition state for the association/folding reaction, just as found during the folding of the intact protein. Conclusion: The specific contacts in the transition state form a nucleus that extends from one fragment to the next, but the nucleus is only ‘flickeringly' present in the denatured state. This is direct evidence for the nucleation-condensation mechanism in which the nucleus is only weakly formed in the ground state and develops in the transition state. The low conformational preferences in the denatured state are not enough to induce significant local secondary structure, but are reinforced by tertiary interactions during the rapid condensation around the nucleus.

Published

1996

127. The HIV-1 capsid protein as a drug target: recent advances and future prospects

Author

Rosa Doménech and José L. Neira

Subjects

Models, Molecular, Anti-HIV Agents, viruses, Drug target, Molecular Sequence Data, Morphogenesis, Human immunodeficiency virus (HIV), HIV Infections, Cleavage (embryo), medicine.disease_cause, Biochemistry, Small Molecule Libraries, Retrovirus, medicine, Humans, Amino Acid Sequence, Molecular Targeted Therapy, Molecular Biology, biology, Chemistry, Gag Polyprotein, Cell Biology, General Medicine, biology.organism_classification, Cell biology, Protein Structure, Tertiary, Capsid, Drug Design, HIV-1, Capsid Proteins, CTD, Peptides

Abstract

HIV-1, the agent responsible for AIDS, belongs to the retrovirus family. Assembly of the immature HIV-1 capsid occurs through the controlled polymerization of the Gag polyprotein, which is transported to the plasma membrane of infected cells, where morphogenesis of the immature, non-infectious virion occurs. Moreover, the mature capsid of HIV-1 is formed by the assembly of copies of the capsid protein (CA), which results, among other proteins, from cleavage of Gag. The C-terminal domain of CA (CTD) can homodimerize, and most of the dimerization interface is formed by a single α-helix from each monomer. Assembly of the HIV-1 capsid critically depends on CA-CA interactions, including CTD interaction with itself and with the N-terminal domain of CA (NTD). This review will report on recent advances for the search of small organic compounds and peptides that have been designed in the last four years to hamper CA assembly. Most of the molecules have been proved to interact with CA; such molecules aim to disrupt and/or alter the oligomerization capability of CTD and/or NTD.

Published

2013

128. Fluorescence, Circular Dichroism and Mass Spectrometry as Tools to Study Virus Structure

Author

José L. Neira

Subjects

chemistry.chemical_classification, Quantitative Biology::Biomolecules, Circular dichroism, Particle composition, chemistry, Molecular mass, Biomolecule, Biophysics, Virus Structure, Nuclear magnetic resonance spectroscopy, Mass spectrometry, Fluorescence

Abstract

Fluorescence and circular dichroism, as analytical spectroscopic techniques, and mass spectrometry as an analytical tool to determine the molecular mass, provide important biophysical approaches in structural virology. Although they do not provide atomic, or near-atomic, details as electron microscopy, X-ray crystallography or nuclear magnetic resonance spectroscopy can do, they do provide important insights into virus particle composition, structure, conformational stability and dynamics, assembly and maturation, and interactions with other viral and cellular biomolecules. They can be used also to investigate the molecular determinants of virus particle structure and properties, and the changes induced in them by external factors. In this chapter, I describe the physical bases of these three techniques, and some examples on how they have helped us to understand virus particle structure and physicochemical properties.

Published

2013

129. BRMS151-98 and BRMS151-84 are crystal oligomeric coiled coils with different oligomerization states, which behave as disordered protein fragments in solution

Author

Jerónimo Bravo, Antonio A. Romero, José L. Neira, José Rivera, Mercedes Spínola-Amilibia, and Miguel Ortiz-Lombardía

Subjects

Coiled coil, Models, Molecular, Magnetic Resonance Spectroscopy, Chemistry, Protein Conformation, BRMS1, biophysical features, Antiparallel (biochemistry), Crystallography, X-Ray, NMR, Neoplasm Proteins, Repressor Proteins, X-ray, Crystallography, Structural Biology, Cytoplasm, Biophysics, Protein Multimerization, Coiled coils, Nuclear export signal, Molecular Biology, Oligopeptides, Dynamic equilibrium, Heteronuclear single quantum coherence spectroscopy, Cellular localization

Abstract

17 páginas, 9 figuras, 1 tabla., The breast cancer metastasis suppressor 1 (BRMS1) gene suppresses metastasis without affecting the primary tumor growth. Cellular localization of BRMS1 appears to be important for exerting its effects on metastasis inhibition. We recently described a nucleo-cytoplasmic shuttling for BRMS1 and identified a nuclear export signal within the N-terminal coiled coil. The structure of these regions shows an antiparallel coiled coil capable of oligomerizing, which compromises the accessibility to the nuclear export signal consensus residues. We have studied the structural and biophysical features of this region to further understand the contribution of the N-terminal coiled coil to the biological function of BRMS1. We have observed that residues 85 to 98 might be important in defining the oligomerization state of the BRMS1 N-terminal coiled coil. The fragments are mainly disordered in solution, with evidence of residual structure. In addition, we report the presence of a conformational dynamic equilibrium (oligomeric folded species ↔ oligomeric unfolded) in solution in the BRMS1 N-terminal coiled coil that might facilitate the nuclear export of BRMS1 to the cytoplasm., Work at the J.L.N. laboratory was supported by the Spanish Ministerio de Ciencia e Innovación (CTQ2011-24393, CSD2008-00005) and intramural BIFI 2011 grant. Work at the J.B. laboratory was supported by Ministerio de Ciencia e Innovación (SAF2008-04048-E, SAF2009-10667, and SAF2012-31405), Conselleria de Sanitat, Generalitat Valenciana AP-001/10, CSIC (200820I020), and Fundación Mutua Madrileña, Spain.

Published

2013

130. Spectroscopic Parameters in Nuclear Magnetic Resonance

Author

Rodrigo J. Carbajo and José L. Neira

Subjects

Coupling constant, Physics, Relaxometry, Electron nuclear double resonance, Nuclear magnetic resonance, Solid-state nuclear magnetic resonance, Relaxation (NMR), Spin echo, Condensed Matter::Strongly Correlated Electrons, Nuclear Overhauser effect, Two-dimensional nuclear magnetic resonance spectroscopy

Abstract

In common with other spectroscopic techniques, NMR measures the intensities of the nuclear spin transitions versus the frequencies at which these transitions happen. In this chapter, the spectroscopic parameters of NMR will be described, some of which are shared by other spectroscopies while others are unique to the technique, arising from the properties described in the previous chapter. The origin and physical characteristics of the chemical shift, the spin–spin scalar coupling and the nuclear Overhauser effect (NOE) will be introduced here.

Published

2013

131. Basic NMR Experiments

Author

Rodrigo J. Carbajo and José L. Neira

Subjects

Theoretical physics, Heteronuclear molecule, Multiple quantum, Scalar (physics), Fluorine-19 NMR, Homonuclear molecule

Abstract

In this chapter we shall describe basic NMR experiments used in the fields of Chemistry, Biochemistry and Biology. The topics of acquisition and processing of simple 1D-NMR spectra will be introduced, as well as the fundamental principles behind n-dimensional NMR experiments. For 2D-NMR, some homonuclear and heteronuclear shift correlation experiments based on scalar couplings are shown. The basis of the population transfer that is at the root of heteronuclear experiments is described. The chapter ends with the most relevant nuclear correlations via dipolar couplings, based on the NOE effect.

Published

2013

132. Nuclear Magnetic Resonance Spectroscopy to Study Virus Structure

Author

José L. Neira

Subjects

Membrane, Viral life cycle, Capsid, Chemistry, viruses, Chemical shift, Nucleic acid, Biophysics, Nuclear magnetic resonance spectroscopy, Virus, Protein–protein interaction

Abstract

Nuclear magnetic resonance (NMR) is a spectroscopic technique based in the absorption of radiofrequency radiation by atomic nuclei in the presence of an external magnetic field. NMR has followed a “bottom-up” approach to solve the structures of isolated domains of viral proteins, including capsid protein subunits. NMR has been instrumental to describe conformational changes in viral proteins and nucleic acids, showing the presence of dynamic equilibria which are thought to be important at different stages of the virus life cycle; in this sense, NMR is also the only technique currently available to describe, in atomic detail, the conformational preferences of natively unfolded viral proteins. NMR has also complemented X-ray crystallography and has been combined with electron microscopy to obtain pseudo-atomic models of entire virus capsids. Finally, the joint use of liquid and solid-state NMR has allowed the identification of conformational changes in intact viral capsids on insertion in host membranes.

Published

2013

133. The Basis of Nuclear Magnetic Resonance Spectroscopy

Author

Rodrigo J. Carbajo and José L. Neira

Subjects

education.field_of_study, Relaxometry, Nuclear magnetic resonance, Solid-state nuclear magnetic resonance, Population, Relaxation (NMR), Spin echo, Nuclear magnetic resonance spectroscopy, education, Two-dimensional nuclear magnetic resonance spectroscopy, Nuclear magnetic resonance decoupling

Abstract

Nuclear magnetic resonance (NMR) has transformed the research areas of Chemistry, Biochemistry and Medicine, but much of its fundamentals remain obscure for the non-initiated. NMR is a technique based on the absorption of radiofrequency radiation by atomic nuclei in the presence of an external magnetic field. In this chapter, we describe the physical basis of phenomena within NMR spectroscopy from both a quantum-theory perspective and a classical view, to provide any prospective user the basic concepts underlying the technique. The spectroscopic notion of energy level population is described, as well as a basic introduction to the theory and mechanisms of spin relaxation. The application of radiofrequency pulses to produce the NMR signal, its conversion to the frequency domain by Fourier Transform and the typical instrumental set-up of magnetic resonance are also covered.

Published

2013

134. Biomolecular NMR

Author

Rodrigo J. Carbajo and José L. Neira

Published

2013

135. Turbulent times in southern European science

Author

José L. Neira and Francisco N. Barrera

Subjects

Meteorology, Turbulence, Political science, Research, Humans, General Medicine

Published

2012

136. The C-terminal sterile alpha motif (SAM) domain of human p73 is a highly dynamic protein, which acquires high thermal stability through a decrease in backbone flexibility

Author

José L. Neira, Paz Sevilla, and Francisco García-Blanco

Subjects

Models, Molecular, Time Factors, Movement, General Physics and Astronomy, chemistry.chemical_compound, Residue (chemistry), Amide, Molecule, Humans, Thermal stability, Physical and Theoretical Chemistry, Guanidine, Nuclear Magnetic Resonance, Biomolecular, Thermostability, Protein Stability, C-terminus, Tumor Suppressor Proteins, Temperature, Nuclear Proteins, Tumor Protein p73, Protein Structure, Tertiary, DNA-Binding Proteins, Crystallography, chemistry, Sterile alpha motif

Abstract

The α-splice variant of p73 (p73α), a homologue of the tumour suppressor p53, has close to its C terminus a sterile alpha motif (SAM), SAMp73, that is involved in protein-biomolecule interactions. The conformational stability of SAMp73 is low (∼5 kcal mol(-1)), although its thermal stability is high. To explain this high thermostability, we studied the dynamics of SAMp73 over a wide range of GdmCl (guanidine hydrochloride) concentrations and temperatures by NMR relaxation, NMR hydrogen-exchange (HX) and fluorescence lifetime approaches. The slowest exchanging residues of SAMp73 belong to the helical regions, and they did exchange by a global unfolding process. Moreover, SAMp73 was very flexible, with most of its amide protons affected by slow μs-ms conformational exchange. Within this time scale, the residues of SAMp73 with the largest exchange rates (R(ex)) were involved in binding with other molecules; therefore, the flexibility in the μs-ms range was associated with biological functions. As the [GdmCl] increased, the pico-to-nanosecond flexibility of the backbone amide protons raised, but it did so differently depending on the residue. We were able to obtain, for the first time, the linear [GdmCl]-variation of the local conformational entropies, m(S(i)), which ranged from 5.3 to 0.3 cal mol(-1) K(-1) M(-1), similar to those measured by using macroscopic techniques in other proteins. Conversely, the temperature dependence of the pico-to-nanosecond dynamics of the backbone amide protons of SAMp73 indicates that the flexibility of some residues decreased with the temperature; these results explain the high thermostability of the protein.

Published

2012

137. Stability and binding of the phosphorylated species of the N-terminal domain of enzyme I and the histidine phosphocarrier protein from the Streptomyces coelicolor phosphoenolpyruvate:sugar phosphotransferase system

Author

Adrián Velázquez-Campoy, Ana Isabel Martínez-Gómez, Sergio Martínez-Rodríguez, Josefa María Clemente-Jiménez, José L. Neira, Rosa Doménech, and David Aguado-Llera

Subjects

Biophysics, Streptomyces coelicolor, macromolecular substances, Phosphocarrier protein, Biochemistry, Serine, Bacterial Proteins, Catalytic Domain, Enzyme Stability, Phosphorylation, Phosphoenolpyruvate Sugar Phosphotransferase System, Molecular Biology, Histidine, biology, Permease, Hydrogen Bonding, PEP group translocation, biology.organism_classification, Phosphoproteins, carbohydrates (lipids), Mutation, biology.protein, Mutagenesis, Site-Directed, bacteria, Thermodynamics, Phosphoenolpyruvate carboxykinase

Abstract

The phosphotransferase system (PTS) is involved in the use of carbon sources in bacteria. It is formed by two general proteins: enzyme I (EI) and the histidine phosphocarrier (HPr), and various sugar-specific permeases. EI is formed by two domains, with the N-terminal domain (EIN) being responsible for the binding to HPr. In low-G+C Gram-positive bacteria, HPr becomes phosphorylated not only by phosphoenolpyruvate (PEP) at the active-site histidine, but also by ATP at a serine. In this work, we have characterized: (i) the stability and binding affinities between the active-site-histidine phosphorylated species of HPr and the EIN from Streptomyces coelicolor; and (ii) the stability and binding affinities of the species involving the phosphorylation at the regulatory serine of HPr(sc). Our results show that the phosphorylated active-site species of both proteins are less stable than the unphosphorylated counterparts. Conversely, the Hpr-S47D, which mimics phosphorylation at the regulatory serine, is more stable than wild-type HPr(sc) due to helical N-capping effects, as suggested by the modeled structure of the protein. Binding among the phosphorylated and unphosphorylated species is always entropically driven, but the affinity and the enthalpy vary widely.

Published

2012

138. Mutation of Ser-50 and Cys-66 in Snapin modulates protein structure and stability

Author

Jesús Prieto, Blanca López-Méndez, José L. Neira, Oscar Millet, Aaron Navarro, David Aguado-Llera, Antonio Ferrer-Montiel, José Antonio Encinar, José M. González-Ros, Luis Alfonso Martínez-Cruz, Javier Gómez, and Gregorio Fernández-Ballester

Subjects

Protein Conformation, Protein Stability, Protein subunit, Wild type, Vesicular Transport Proteins, Biology, Biochemistry, Protein Structure, Secondary, Protein structure, Mutation, Spectroscopy, Fourier Transform Infrared, Biophysics, Serine, Protein oligomerization, Cysteine, Protein kinase A, Protein Dimerization, SNARE complex, SNARE Proteins, Protein secondary structure

Abstract

Snapin is a 15 kDa protein present in neuronal and non-neuronal cells that has been implicated in the regulation of exocytosis and endocytosis. Protein kinase A (PKA) phosphorylates Snapin at Ser-50, modulating its function. Likewise, mutation of Cys-66, which mediates protein dimerization, impairs its cellular activity. Here, we have investigated the impact of mutating these two positions on protein oligomerization, structure, and thermal stability, along with the interaction with SNARE proteins. We found that recombinant purified Snapin in solution appears mainly as dimers in equilibrium with tetramers. The protein exhibits modest secondary structure elements and notable thermal stability. Mutation of Cys-66 to Ser abolished subunit dimerization, but not higher-order oligomers. This mutant augmented the presence of α-helical structure and slightly increased the protein thermal stability. Similarly, the S50A mutant, mimicking the unphosphorylated protein, also exhibited a higher helical secondary structure content than the wild type, along with greater thermal stability. In contrast, replacement of Ser-50 with Asp (S50D), emulating the protein-phosphorylated state, produced a loss of α-helical structure, concomitant with a decrease in protein thermal stability. In vitro, the wild type and mutants weakly interacted with SNAP-25 and the reconstituted SNARE complex, although S50D exhibited the strongest binding to the SNARE complex, consistent with the observed higher cellular activity of PKA-phosphorylated Snapin. Our observations suggest that the stronger binding of S50D to SNAREs might be due to a destabilization of tetrameric assemblies of Snapin that favor the interaction of protein dimers with the SNARE proteins. Therefore, phosphorylation of Ser-50 has an important impact on the protein structure and stability that appears to underlie its functional modulation.

Published

2012

139. Biophysical characterization of the isolated C-terminal region of the transient receptor potential vanilloid 1

Author

Ana Cámara-Artigas, Francisco J. Taberner, José L. Neira, Lucia Gregorio-Teruel, Julio Bacarizo, and David Aguado-Llera

Subjects

Protein Denaturation, Calmodulin, Stereochemistry, Biophysics, TRPV1, TRPV Cation Channels, Biochemistry, TRPV, Fluorescence, Biophysical Phenomena, Protein–protein interaction, Transient receptor potential channel, Structural Biology, Genetics, Animals, Binding site, Molecular Biology, Ion channel, Protein Unfolding, Binding Sites, biology, Chemistry, musculoskeletal, neural, and ocular physiology, Circular Dichroism, Folding, Cell Biology, Protein Structure, Tertiary, Rats, Transmembrane domain, nervous system, Oligomer, biology.protein, lipids (amino acids, peptides, and proteins), psychological phenomena and processes

Abstract

Transient receptor potential (TRP) proteins are sensory-related cation channels. TRPV subfamily responds to vanilloids, generating a Ca2+ current. TRPV1, a thermal-sensitive non-selective ion channel, possesses six transmembrane helices and the intracellular N- and C-terminal domains. The latter contains the PIP2 and calmodulin binding sites, the TRP domain and a temperature-responding flexible region. Although the function of C-TRPV1 is known, there are no experimental reports on its structural features. Here, we describe the conformational features of C-TRVP1, by using spectroscopic and biophysical approaches. Our results show that C-TRVP1 is an oligomeric protein, which shows features of natively unfolded proteins. Structured summary of protein interactions C-TRPV1 and C-TRPV1 bind by dynamic light scattering ( View interaction ) C-TRPV1 and C-TRPV1 bind by static light scattering ( View interaction ) C-TRPV1 and C-TRPV1 bind by cross-linking study ( View interaction ) C-TRPV1 and C-TRPV1 bind by comigration in non-denaturing gel electrophoresis ( View interaction )

Published

2012

140. The inactivating factor of glutamine synthetase IF17 is an intrinsically disordered protein, which folds upon binding to its target

Author

Carla V. Galmozzi, Lorena Saelices, M. Isabel Muro-Pastor, José L. Neira, and Francisco J. Florencio

Subjects

Cyanobacteria, Protein Denaturation, Protein Conformation, Biochemistry, chemistry.chemical_compound, Bacterial Proteins, Glutamate-Ammonia Ligase, Glutamate synthase, Glutamine synthetase, Ammonium, Protein Interaction Domains and Motifs, Nuclear Magnetic Resonance, Biomolecular, biology, Chemistry, Protein Stability, Circular Dichroism, Synechocystis, biology.organism_classification, Recombinant Proteins, Kinetics, Synechocystis sp, Spectrometry, Fluorescence, biology.protein, bacteria, Protein Processing, Post-Translational

Abstract

In cyanobacteria, ammonium is incorporated into carbon skeletons by the sequential action of glutamine synthetase and glutamate synthase (GOGAT). The activity of Synechocystis sp. PCC 6803 glutamine synthetase type I (GS) is controlled by a post-transcriptional process involving protein-protein interactions with two inactivating factors: the 65-residue-long protein (IF7) and the 149-residue-long one (IF17). The sequence of the C terminus of IF17 is similar to IF7; IF7 is an intrinsically disordered protein (IDP). In this work, we study the structural propensities and affinity for GS of IF17 and a chimera protein, IF17N/IF7 (constructed by fusing the first 82 residues of IF17 with the whole IF7) by fluorescence, CD, and NMR. IF17 and IF17N/IF7 are IDPs with residual non-hydrogen-bonded structure, probably formed by α-helical, turn-like, and PPII conformations; several theoretical predictions support these experimental findings. IF17 seems to fold upon binding to GS, as suggested by CD thermal denaturations and steady-state far-UV spectra. The apparent affinity of IF17 for GS, as measured by fluorescence, is slightly smaller (K(D) ~1 μM) than that measured for IF7 (~0.3 μM). The K(D)s determined by CD are similar to those measured by fluorescence, but slightly larger, suggesting possible conformational rearrangements in the IFs and/or GS upon binding. Further, the results with IFN17/IF7 suggest that (i) binding of IF17 to the GS is modulated not only by its C-terminal region but also by its N-terminus and (ii) there are weakly structured (that is, "fuzzy") complexes in the ternary GS-IF system.

Published

2011

141. Biochemical and mutational studies of the Bacillus cereus CECT 5050T formamidase support the existence of a C-E-E-K tetrad in several members of the nitrilase superfamily

Author

Montserrat Andújar-Sánchez, José L. Neira, Josefa María Clemente-Jiménez, Ana Isabel Martínez-Gómez, Felipe Rodríguez-Vico, Francisco Javier Las Heras-Vázquez, Sergio Martínez-Rodríguez, and Pablo Soriano-Maldonado

Subjects

Subfamily, Sequence analysis, Molecular Sequence Data, Bacillus cereus, Glutamic Acid, Sequence alignment, Applied Microbiology and Biotechnology, Nitrilase, Catalysis, Protein Structure, Secondary, Amidase, Amidohydrolases, Substrate Specificity, Bacterial Proteins, Aminohydrolases, Escherichia coli, Homology modeling, Cloning, Molecular, Enzymology and Protein Engineering, Chromatography, High Pressure Liquid, Phylogeny, Enzyme Assays, Genetics, Ecology, biology, Base Sequence, Sequence Homology, Amino Acid, Circular Dichroism, biology.organism_classification, Recombinant Proteins, Enzyme Activation, Biochemistry, Mutation, Chromatography, Gel, Mutagenesis, Site-Directed, Formamidase, Sequence Alignment, Food Science, Biotechnology

Abstract

Formamidases (EC 3.5.1.49) are poorly characterized proteins. In spite of this scarce knowledge, ammonia has been described as playing a central role in the pathogenesis of human pathogens such as Helicobacter pylori , for which formamidase has been shown to participate in the nitrogen metabolic pathway. Sequence analysis has revealed that at least two different groups of formamidases are classified as EC 3.5.1.49: on the one hand, the derivatives of the FmdA-AmdA superfamily, which are the best studied to date, and on the other hand, the derivatives of Helicobacter pylori AmiF. Here we present the cloning, purification, and characterization of a recombinant formamidase from Bacillus cereus CECT 5050T (BceAmiF), the second member of the AmiF subfamily to be characterized, showing new features of the enzyme further supporting its relationship with aliphatic amidases. We also present homology modeling-based mutational studies confirming the importance of the Glu140 and Tyr191 residues in the enzymatic activities of the AmiF family. Moreover, we can conclude that a second glutamate residue is critical in several members of the nitrilase superfamily, meaning that what has consistently been identified as a C-E-K triad is in fact a C-E-E-K tetrad.

Published

2011

142. The isolated major homology region of the HIV capsid protein is mainly unfolded in solution and binds to the intact protein

Author

Rebeca Bocanegra, Rosa Doménech, José L. Neira, and Adrián Velázquez-Campoy

Subjects

Models, Molecular, Protein Folding, viruses, Biophysics, Peptide, Biology, Crystallography, X-Ray, Biochemistry, Virus, Analytical Chemistry, Protein structure, Humans, Amino Acid Sequence, Molecular Biology, Peptide sequence, chemistry.chemical_classification, Sequence Homology, Amino Acid, C-terminus, Virus Assembly, Virology, Peptide Fragments, Protein Structure, Tertiary, Solutions, Capsid, chemistry, HIV-1, Protein folding, Capsid Proteins, Protein Multimerization, Heteronuclear single quantum coherence spectroscopy, Protein Binding

Abstract

Assembly of the mature human immunodeficiency virus type 1 (HIV-1) capsid involves the oligomerization of the capsid protein, CA. During retroviral maturation, the CA protein undergoes structural changes and forms exclusive intermolecular interfaces in the mature capsid shell, different from those in the immature precursor. The most conserved region of CA, the major homology region (MHR), is located in the C-terminal domain of CA (CTD). The MHR is involved in both immature and mature virus assembly; however, its exact function during both assembly stages is unknown. To test its conformational preferences and to provide clues on its role during CA assembly, we have used a minimalist approach by designing a peptide comprising the whole MHR (MHRpep, residues Asp152 to Ala174). Isolated MHRpep is mainly unfolded in aqueous solution, with residual structure at its C terminus. MHRpep binds to monomeric CTD with an affinity of ~30μM (as shown by fluorescence and ITC); the CTD binding region comprises residues belonging to α-helices 10 and 11. In the immature virus capsid, the MHR and α-helix 11 regions of two CTD dimers also interact [Briggs JAG, Riches JD, Glass B, Baratonova V, Zanetti G and Krausslich H-G (2009) Proc. Natl. Acad. Sci. USA 106, 11090-11095]. These results can be considered a proof-of-concept that the conformational preferences and binding features of isolated peptides derived from virus proteins could be used to mimic early stages of virus assembly.

Published

2011

143. The structure of BRMS1 nuclear export signal and SNX6 interacting region reveals a hexamer formed by antiparallel coiled coils

Author

Mercedes Spínola-Amilibia, José L. Neira, Miguel Ortiz-Lombardía, Jerónimo Bravo, Antonio A. Romero, and José Rivera

Subjects

Coiled coil domain, Protein Conformation, Molecular Sequence Data, Protein Data Bank (RCSB PDB), metastasis suppressors, Random hexamer, Antiparallel (biochemistry), Crystallography, X-Ray, Structural Biology, Humans, Amino Acid Sequence, Nuclear export signal, X-Ray diffraction, Molecular Biology, Nuclear Magnetic Resonance, Biomolecular, Sorting Nexins, Cellular localization, Coiled coil, Nuclear Export Signals, Sequence Homology, Amino Acid, Chemistry, BRMS1, Structure, Neoplasm Proteins, Repressor Proteins, Crystallography, Biophysics, Hydrodynamics, Protein quaternary structure, Ultracentrifugation, Metastasis Suppressor Protein

Abstract

14 páginas, 3 tablas, 3 figuras. PMID:21777593[PubMed] Coordinates and structure factors have been deposited in the PDB with accession number 2XUS, We present here the first structural report derived from breast cancer metastasis suppressor 1 (BRMS1), a member of the metastasis suppressor protein group, which, during recent years, have drawn much attention since they suppress metastasis without affecting the growth of the primary tumor. The relevance of the predicted N-terminal coiled coil on the molecular recognition of some of the BRMS1 partners, on its cellular localization and on the role of BRMS1 biological functions such as transcriptional repression prompted us to characterize its three-dimensional structure by X-ray crystallography. The structure of BRMS1 N-terminal region reveals that residues 51-98 form an antiparallel coiled-coil motif and, also, that it has the capability of homo-oligomerizing in a hexameric conformation by forming a trimer of coiled-coil dimers. We have also performed hydrodynamic experiments that strongly supported the prevalence in solution of this quaternary structure for BRMS1(51-98). This work explores the structural features of BRMS1 N-terminal region to help clarify the role of this area in the context of the full-length protein. Our crystallographic and biophysical results suggest that the biological function of BRMS1 may be affected by its ability to promote molecular clustering through its N-terminal coiled-coil region., This work was supported by Ministerio de Ciencia e Innovación (SAF2008-04048-E and SAF2009-10667); Conselleria de Sanitat, Generalitat Valenciana (AP-001/10); Consejo Superior de Investigaciones Científicas (200820I020); and Fundación Mutua Madrileña, Spain. Work in JLN laboratory was supported by Ministerio de Ciencia e Innovacion (CSD2008-00005, SAF2008-05742-C2-01), Generalitat Valenciana (ACOMP2011/113) and Fundación para la investigación y prevención del SIDA en España, FIPSE, (36557/06).

Published

2011

144. The conformational stability and biophysical properties of the eukaryotic thioredoxins of Pisum sativum are not family-conserved

Author

David Aguado-Llera, Ana Chueca, José L. Neira, Jesús Prieto, Ana Isabel Martínez-Gómez, Marco Marenchino, Javier Gómez, and José A. Traverso

Subjects

Protein Denaturation, Protein Structure, Protein Folding, Protein Conformation, Molecular Sequence Data, Biophysics, lcsh:Medicine, Biology, Biochemistry, Protein Chemistry, Biophysical Phenomena, Protein–protein interaction, Conserved sequence, Protein structure, Thioredoxins, Denaturation (biochemistry), Amino Acid Sequence, lcsh:Science, Peptide sequence, Conserved Sequence, Multidisciplinary, Sequence Homology, Amino Acid, Protein Stability, lcsh:R, Peas, Proteins, Subcellular localization, Eukaryotic Cells, Multigene Family, Biophysical Process, Hydrodynamics, lcsh:Q, Thioredoxin, Protein Multimerization, Acids, Research Article

Abstract

Thioredoxins (TRXs) are ubiquitous proteins involved in redox processes. About forty genes encode TRX or TRX-related proteins in plants, grouped in different families according to their subcellular localization. For instance, the h-type TRXs are located in cytoplasm or mitochondria, whereas f-type TRXs have a plastidial origin, although both types of proteins have an eukaryotic origin as opposed to other TRXs. Herein, we study the conformational and the biophysical features of TRXh1, TRXh2 and TRXf from Pisum sativum. The modelled structures of the three proteins show the well-known TRX fold. While sharing similar pH-denaturations features, the chemical and thermal stabilities are different, being PsTRXh1 (Pisum sativum thioredoxin h1) the most stable isoform; moreover, the three proteins follow a three-state denaturation model, during the chemical-denaturations. These differences in the thermal- and chemical-denaturations result from changes, in a broad sense, of the several ASAs (accessible surface areas) of the proteins. Thus, although a strong relationship can be found between the primary amino acid sequence and the structure among TRXs, that between the residue sequence and the conformational stability and biophysical properties is not. We discuss how these differences in the biophysical properties of TRXs determine their unique functions in pea, and we show how residues involved in the biophysical features described (pH-titrations, dimerizations and chemical-denaturations) belong to regions involved in interaction with other proteins. Our results suggest that the sequence demands of protein-protein function are relatively rigid, with different protein-binding pockets (some in common) for each of the three proteins, but the demands of structure and conformational stability per se (as long as there is a maintained core), are less so.

Published

2011

145. Rationally designed interfacial peptides are efficient in vitro inhibitors of HIV-1 capsid assembly with antiviral activity

Author

Miguel Angel Martinez, Rebeca Bocanegra, Inmaculada López, Alicia Rodríguez-Huete, Maria Nevot, Mauricio G. Mateu, Javier Gómez, Olga Abian, Adrián Velázquez-Campoy, Claudio N. Cavasotto, Rosa Doménech, José L. Neira, UAM. Departamento de Biología Molecular, Generalitat Valenciana, Comunidad de Madrid, Ministerio de Ciencia e Innovación (España), and Fundación para la Investigación y la Prevención del Sida en España

Subjects

Models, Molecular, Macromolecular Assemblies, lcsh:Medicine, Peptide, Biochemistry, Protein Structure, Secondary, Immunodeficiency Viruses, Drug Discovery, Biomacromolecule-Ligand Interactions, lcsh:Science, Peptide sequence, chemistry.chemical_classification, Multidisciplinary, Antivirals, Biología y Biomedicina / Biología, Capsid, Structural Proteins, Research Article, Biotechnology, Signal peptide, Protein Structure, Anti-HIV Agents, Molecular Sequence Data, Biophysics, Viral Structure, Microbiology, Cell Line, Virology, Viruslike Particles, Amino Acid Sequence, Binding site, Protein Interactions, Biology, Binding Sites, lcsh:R, Rational design, Proteins, Molecular biology, In vitro, Peptide Fragments, Protein Structure, Tertiary, chemistry, Solubility, Drug Design, Helix, HIV-1, Capsid Proteins, lcsh:Q, Protein Multimerization

Abstract

Virus capsid assembly constitutes an attractive target for the development of antiviral therapies; a few experimental inhibitors of this process for HIV-1 and other viruses have been identified by screening compounds or by selection from chemical libraries. As a different, novel approach we have undertaken the rational design of peptides that could act as competitive assembly inhibitors by mimicking capsid structural elements involved in intersubunit interfaces. Several discrete interfaces involved in formation of the mature HIV-1 capsid through polymerization of the capsid protein CA were targeted. We had previously designed a peptide, CAC1, that represents CA helix 9 (a major part of the dimerization interface) and binds the CA C-terminal domain in solution. Here we have mapped the binding site of CAC1, and shown that it substantially overlaps with the CA dimerization interface. We have also rationally modified CAC1 to increase its solubility and CA-binding affinity, and designed four additional peptides that represent CA helical segments involved in other CA interfaces. We found that peptides CAC1, its derivative CAC1M, and H8 (representing CA helix 8) were able to efficiently inhibit the in vitro assembly of the mature HIV-1 capsid. Cocktails of several peptides, including CAC1 or CAC1M plus H8 or CAI (a previously discovered inhibitor of CA polymerization), or CAC1M+H8+CAI, also abolished capsid assembly, even when every peptide was used at lower, sub-inhibitory doses. To provide a preliminary proof that these designed capsid assembly inhibitors could eventually serve as lead compounds for development of anti-HIV-1 agents, they were transported into cultured cells using a cell-penetrating peptide, and tested for antiviral activity. Peptide cocktails that drastically inhibited capsid assembly in vitro were also able to efficiently inhibit HIV-1 infection ex vivo. This study validates a novel, entirely rational approach for the design of capsid assembly interfacial inhibitors that show antiviral activity. © 2011 Bocanegra et al., Fundacion para la Investigacion y Prevencion del SIDA en Espana (FIPSE Exp: 36557/06) to MGM, JLN and MAM, Spain’s Ministerio de Ciencia e Innovacion (BIO2009-10072 to MGM and SAF2008-05742-C02-01 and CSD20008-00005 to JLN and JG), Comunidad de Madrid (S-2009/MAT/1467 to MGM), Generalitat Valenciana (ACOMP2010/114 to JLN and JG)

Published

2011

146. Conformational Stability of Hepatitis C Virus NS3 Protease

Author

José L. Neira, Olga Abian, Sonia Vega, and Adrián Velázquez-Campoy

Subjects

Proteases, Protein Denaturation, Viral protein, medicine.medical_treatment, viruses, Population, Biophysics, chemistry.chemical_element, Zinc, Hepacivirus, Viral Nonstructural Proteins, medicine.disease_cause, Fluorescence, Protein Structure, Secondary, Enzyme Stability, medicine, education, Protein Unfolding, Serine protease, NS3, education.field_of_study, Protease, biology, Calorimetry, Differential Scanning, Chemistry, Protein, Temperature, biochemical phenomena, metabolism, and nutrition, Hydrogen-Ion Concentration, NS2-3 protease, Biochemistry, biology.protein

Abstract

The hepatitis C virus NS3 protease is responsible for the processing of the nonstructural region of viral precursor polyprotein in infected hepatic cells. NS3 has been considered a target for drug discovery for a long time. NS3 is a zinc-dependent serine protease. However, the zinc ion is not involved in the catalytic mechanism, because it is bound far away from the active site. Thus, zinc is essential for the structural integrity of the protein and it is considered to have a structural role. The first thermodynamic study on the conformational equilibrium and stability of NS3 and the effect of zinc on such equilibrium is presented here. In agreement with a previous calorimetric study on the binding of zinc to NS3, the global unfolding heat capacity is dominated by the zinc dissociation step, suggesting that the binding of zinc induces a significant structural rearrangement of the protein. In addition, contrary to other homologous zinc-dependent proteases, the zinc-free NS3 protease is not completely unstructured. It is apparent that the conformational landscape of hepatitis C virus NS3 protease is fairly complex due to its intrinsic plasticity, and to the interactions with its different effectors (zinc and the accessory viral protein NS4A) and their modulation of the population of the different conformational states.

Published

2010

147. Robust place recognition with stereo cameras

Author

Dorian Galvez-Lopez, Juan D. Tardós, José L. Neira, Cesar Cadena, and Fabio Ramos

Subjects

Stereopsis, Stereo cameras, business.industry, Computer science, Epipolar geometry, Feature extraction, ComputingMethodologies_IMAGEPROCESSINGANDCOMPUTERVISION, Computer vision, Artificial intelligence, Computational geometry, Visual appearance, business, Stereo camera

Abstract

Place recognition is a challenging task in any SLAM system. Algorithms based on visual appearance are becoming popular to detect locations already visited, also known as loop closures, because cameras are easily available and provide rich scene detail. These algorithms typically result in pairs of images considered depicting the same location. To avoid mismatches, most of them rely on epipolar geometry to check spatial consistency. In this paper we present an alternative system that makes use of stereo vision and combines two complementary techniques: bag-of-words to detect loop closing candidate images, and conditional random fields to discard those which are not geometrically consistent. We evaluate this system in public indoor and outdoor datasets from the Rawseeds project, with hundred-metre long trajectories. Our system achieves more robust results than using spatial consistency based on epipolar geometry.

Published

2010

148. Dendrimers as potential inhibitors of the dimerization of the capsid protein of HIV-1

Author

Ricardo Riguera, Juan Correa, Adrián Velázquez-Campoy, Eduardo Fernandez-Megia, Rosa Doménech, José L. Neira, Olga Abian, Ana Sousa-Herves, Rebeca Bocanegra, and Mauricio G. Mateu

Subjects

Models, Molecular, Circular dichroism, Dendrimers, Magnetic Resonance Spectroscopy, Polymers and Plastics, Stereochemistry, Anti-HIV Agents, viruses, Glycopolymer, Bioengineering, Calorimetry, environment and public health, Polyethylene Glycols, Biomaterials, chemistry.chemical_compound, Dendrimer, Gallic Acid, Materials Chemistry, Binding site, Circular Dichroism, Biological activity, Dissociation constant, enzymes and coenzymes (carbohydrates), Kinetics, Spectrometry, Fluorescence, Capsid, chemistry, HIV-1, Capsid Proteins, CTD, Dimerization

Abstract

Assembly of the mature human immunodeficiency virus type 1 capsid involves the oligomerization of the capsid protein, CA. The C-terminal domain of CA, CTD, participates both in the formation of CA hexamers and in the joining of hexamers through homodimerization. Intact CA and the isolated CTD are able to homodimerize in solution with similar affinity (dissociation constant in the order of 10 microM); CTD homodimerization involves mainly an alpha-helical region. In this work, we show that first-generation gallic acid-triethylene glycol (GATG) dendrimers bind to CTD. The binding region is mainly formed by residues involved in the homodimerization interface of CTD. The dissociation constant of the dendrimer-CTD complexes is in the range of micromolar, as shown by ITC. Further, the affinity for CTD of some of the dendrimers is similar to that of synthetic peptides capable of binding to the dimerization region, and it is also similar to the homodimerization affinity of both CTD and CA. Moreover, one of the dendrimers, with a relatively large hydrophobic moiety at the dendritic branching (a benzoate), was able to hamper the assembly in vitro of the human immunodeficiency virus capsid. These results open the possibility of considering dendrimers as lead compounds for the development of antihuman immunodeficiency virus drugs targeting capsid assembly.

Published

2010

149. The N-terminal domain of the enzyme I is a monomeric well-folded protein with a low conformational stability and residual structure in the unfolded state

Author

Usue Ariz, Erik Goormaghtigh, María L. Martínez-Chantar, José L. Neira, Manuel Romero-Beviar, Javier Gómez, Sergio Martínez-Rodríguez, and Jesús Prieto

Subjects

Circular dichroism, Protein Denaturation, Protein Folding, Multiprotein complex, Protein Conformation, Bioengineering, Streptomyces coelicolor, Biochemistry, chemistry.chemical_compound, Molecular recognition, Bacterial Proteins, Enzyme Stability, Spectroscopy, Fourier Transform Infrared, Escherichia coli, Phosphoenolpyruvate Sugar Phosphotransferase System, Molecular Biology, Nuclear Magnetic Resonance, Biomolecular, Histidine, chemistry.chemical_classification, biology, Circular Dichroism, Phosphotransferases (Nitrogenous Group Acceptor), PEP group translocation, Hydrogen-Ion Concentration, biology.organism_classification, Recombinant Proteins, Crystallography, Monomer, Enzyme, chemistry, Thermodynamics, Hydrophobic and Hydrophilic Interactions, Biotechnology

Abstract

The bacterial phosphoenolpyruvate-dependent sugar phosphotransferase system is a multiprotein complex that phosphorylates and, concomitantly, transports carbohydrates across the membrane into the cell. The first protein of the cascade is a multidomain protein so-called enzyme I (EI). The N-terminal domain of EI from Streptomyces coelicolor, EIN(sc), responsible for the binding to the second protein in the cascade (the histidine phosphocarrier, HPr), was cloned and successfully expressed and purified. We have previously shown that EI(sc) binds to HPr(sc) with smaller affinity than other members of the EI and HPr families [Hurtado-Gomez et al. (2008) Biophys. J., 95, 1336-1348]. We think that the study of the isolated binding HPr(sc) domain, that is EIN(sc), could shed light on the small affinity value measured. Therefore, in this work we present a detailed description of the structural features of the EIN domain, as a first step towards a complete characterization of the molecular recognition process between the two proteins. We show that EIN(sc) is a folded protein, with alpha-helix and beta-sheet structures and also random-coil conformations, as shown by circular dichroism (CD), FTIR and NMR spectroscopies. The acquisition of secondary and tertiary structures, and the burial of hydrophobic regions, occurred concomitantly at acidic pHs, but at very low pH, the domain acquired a molten-globule conformation. The EIN(sc) protein was not very stable, with an apparent conformational free energy change upon unfolding, DeltaG, of 4.1 +/- 0.4 kcal mol(-1), which was pH independent in the range explored (from pH 6.0 to 8.5). The thermal denaturation midpoint, which was also pH invariant, was similar to that measured in the isolated intact EI(sc). Although EIN(sc) shows thermal- and chemical denaturations that seems to follow a two-state mechanism, there is evidence of residual structure in the chemical and thermally unfolded states, as indicated by differential scanning calorimetry and CD measurements.

Published

2010

150. Structural characterisation of the natively unfolded enterocin EJ97

Author

Marina Sánchez-Hidalgo, Mercedes Maqueda, Lellys M. Contreras, José L. Neira, Manuel Rico, Manuel Martínez-Bueno, Olga Ruiz de los Paños, Junta de Andalucía, Ministerio de Ciencia e Innovación (España), Generalitat Valenciana, and Ministerio de Educación, Cultura y Deporte (España)

Subjects

Models, Molecular, Protein Denaturation, Protein Folding, Antiparasitic, medicine.drug_class, Protein Conformation, Molecular Sequence Data, Virulence, Bioengineering, Peptide, Biology, Biochemistry, Enterococcus faecalis, Microbiology, chemistry.chemical_compound, Bacteriocin, Bacteriocins, Spectroscopy, Fourier Transform Infrared, medicine, Computer Simulation, Amino Acid Sequence, Molecular Biology, Nuclear Magnetic Resonance, Biomolecular, chemistry.chemical_classification, Circular Dichroism, Computational Biology, Molecular Sequence Annotation, Hydrogen-Ion Concentration, biology.organism_classification, Antimicrobial, Spectrometry, Fluorescence, chemistry, Gramicidin, Bacteria, Biotechnology

Abstract

12 pags, 5 figs, 2 tabs, Bacteriocins belong to the wide variety of antimicrobial ribosomal peptides synthesised by bacteria. Enterococci are Gram-positive, catalase-negative bacteria that produce lactic acid as the major end product of glucose fermentation. Many enterococcal strains produce bacteriocins, named enterocins. We describe in this work, the structural characterisation of the 44 residues-long enterocin EJ97, produced by Enterococcus faecalis EJ97. To this end, we have used a combined theoretical and experimental approach. First, we have characterised experimentally the conformational properties of EJ97 in solution under different conditions by using a number of spectroscopic techniques, namely fluorescence, CD, FTIR and NMR. Then, we have used several bioinformatic tools as an aid to complement the experimental information about the conformational properties of EJ97. We have shown that EJ97 is monomeric in aqueous solution and that it appears to be chiefly unfolded, save some flickering helical- or turn-like structures, probably stabilised by hydrophobic clustering. Accordingly, EJ97 does not show a cooperative sigmoidal transition when heated or upon addition of GdmCl. These conformational features are essentially pH-independent, as shown by NMR assignments at pHs 5.9 and 7.0. The computational results were puzzling, since some algorithms revealed the natively unfolded character of EJ97 (FoldIndex, the mean scaled hydropathy), whereas some others suggested the presence of ordered structure in its central region (PONDR, RONN and IUPRED). A future challenge is to produce much more experimental results to aid the development of accurate software tools for predicting disorder in proteins. © 2010 The Author. Published by Oxford University Press. All rights reserved., This work was supported by Grupo de Investigación de la Junta de Andalucía (CIV 016 to M.S.-H.), by Spanish Ministerio de Ciencia e Innovación (SAF2008-05742-C02-01), FIPSE Foundation (Exp: 36557/06) and Generalitat Valenciana (ACOMP/2009/185) to J.L.N. M.S.-H. received a grant from the Spanish Ministry of Education, Culture and Sports

Published

2010