Your search keyword '"Alexander P. Golovanov"' showing total 88 results

51. The interaction of the cellular export adaptor protein Aly/REF with ICP27 contributes to the efficiency of herpes simplex virus 1 mRNA export

Author

Alexander P. Golovanov, Xiaochen Tian, Rozanne M. Sandri-Goldin, and G. V. Devi-Rao

Subjects

Small interfering RNA, viruses, Immunology, Blotting, Western, Active Transport, Cell Nucleus, Fluorescent Antibody Technique, RNA-binding protein, Herpesvirus 1, Human, Biology, Microbiology, Immediate early protein, Immediate-Early Proteins, Virology, Chlorocebus aethiops, Animals, Humans, Immunoprecipitation, RNA, Messenger, Nuclear protein, Vero Cells, In Situ Hybridization, DNA Primers, Messenger RNA, Gene knockdown, Signal transducing adaptor protein, RNA, Nuclear Proteins, RNA-Binding Proteins, Microarray Analysis, Molecular biology, Virus-Cell Interactions, Mutagenesis, Insect Science, HeLa Cells, Transcription Factors

Abstract

Herpes simplex virus 1 (HSV-1) protein ICP27 enables viral mRNA export by accessing the cellular mRNA export receptor TAP/NXF, which guides mRNA through the nuclear pore complex. ICP27 binds viral mRNAs and interacts with TAP/NXF, providing a link to the cellular mRNA export pathway. ICP27 also interacts with the mRNA export adaptor protein Aly/REF, which binds cellular mRNAs and also interacts with TAP/NXF. Studies using small interfering RNA (siRNA) knockdown indicated that Aly/REF is not required for cellular mRNA export, and similar knockdown studies during HSV-1 infection led us to conclude that Aly/REF may be dispensable for viral RNA export. Recently, the structural basis of the interaction of ICP27 with Aly/REF was elucidated at atomic resolution, and it was shown that three ICP27 residues, W105, R107, and L108, interface with the RNA recognition motif (RRM) domain of Aly/REF. Here, to determine the role the interaction of ICP27 and Aly/REF plays during infection, these residues were mutated to alanine, and a recombinant virus, WRL-A, was constructed. Virus production was reduced about 10-fold during WRL-A infection, and export of ICP27 protein and most viral mRNAs was less efficient. We conclude that interaction of ICP27 with Aly/REF contributes to efficient viral mRNA export.

Published

2013

52. Processing of heteronuclear NMR relaxation data with the new software DASHA

Author

V. Yu. Orekhov, Dmitry E. Nolde, Dmitry M. Korzhnev, Alexander P. Golovanov, and A. S. Arseniev

Subjects

Solid-state physics, Heteronuclear molecule, Spectrometer, Chemistry, Relaxation (NMR), Analytical chemistry, Spectral density, Rotational diffusion, Molecule, Thermodynamics, Anisotropy, Atomic and Molecular Physics, and Optics

Abstract

The new program DASHA is an efficient implementation of common data processing steps for the protein internal dynamic analysis. The “model-free” parameters and their uncertainties (Lipari G., Szabo A.: J. Am. Chem. Soc.104, 4546–4559 (1982) can be calculated from an arbitrary combination of experimental data sets (i.e. heteronuclear1H−15N or1H−13C relaxation times and NOE values at different spectrometer frequencies). Anisotropy of the molecular rotational diffusion could be also taken into account without introduction of the new adjustable parameters into the spectral density functionJ(ω), provided the structure of the molecule is known. Parameters of chemical (conformational) exchange can be estimated from the CPMG spin-lock frequency dependences (Bloomet al.: J. Chem. Phys.42, 1615–1624 (1965); Orekhovet al.: Eur. J. Biochem.219, 887–896 (1994). The program can be used both in the interactive and batch modes. It has sophisticated PostScript plotting facilities.

Published

1995

53. ChemInform Abstract: Fingerprinting Food: Current Technologies for the Detection of Food Adulteration and Contamination

Author

Alexander P. Golovanov, David I. Ellis, Warwick B. Dunn, Victoria L. Brewster, J. William Allwood, and Royston Goodacre

Subjects

Distribution system, Food security, Milk products, business.industry, Chemistry, Food products, Food processing, General Medicine, Contamination, Microbial contamination, business, Environmental planning

Abstract

Major food adulteration and contamination events seem to occur with some regularity, such as the widely publicised adulteration of milk products with melamine and the recent microbial contamination of vegetables across Europe for example. With globalisation and rapid distribution systems, these can have international impacts with far-reaching and sometimes lethal consequences. These events, though potentially global in the modern era, are in fact far from contemporary, and deliberate adulteration of food products is probably as old as the food processing and production systems themselves. This review first introduces some background into these practices, both historically and contemporary, before introducing a range of the technologies currently available for the detection of food adulteration and contamination. These methods include the vibrational spectroscopies: near-infrared, mid-infrared, Raman; NMR spectroscopy, as well as a range of mass spectrometry (MS) techniques, amongst others. This subject area is particularly relevant at this time, as it not only concerns the continuous engagement with food adulterers, but also more recent issues such as food security, bioterrorism and climate change. It is hoped that this introductory overview acts as a springboard for researchers in science, technology, engineering, and industry, in this era of systems-level thinking and interdisciplinary approaches to new and contemporary problems.

Published

2012

54. ¹H, ¹³C and ¹⁵N resonance assignment for the human K-Ras at physiological pH

Author

Uybach, Vo, Kevin J, Embrey, Alexander L, Breeze, and Alexander P, Golovanov

Subjects

Proto-Oncogene Proteins p21(ras), Carbon Isotopes, Nitrogen Isotopes, Proto-Oncogene Proteins, Molecular Sequence Data, ras Proteins, Humans, Amino Acid Sequence, Hydrogen-Ion Concentration, Protons, Guanosine Diphosphate, Nuclear Magnetic Resonance, Biomolecular, Sequence Alignment

Abstract

K-Ras, a member of the Ras family of small GTPases, is involved in cell growth, proliferation, differentiation and apoptosis and is frequently mutated in cancer. The activity of Ras is mediated by the inter-conversion between GTP- and GDP- bound states. This conversion is regulated by binding of effector proteins such as guanine nucleotide exchange factors and GTPase activating proteins. Previously, NMR signals from these effector-binding regions of Ras often remained unassigned and largely unobservable due to conformational exchange and polysterism inherent to this protein. In this paper, we report the complete backbone and C(β), as well as partial H(α), H(β) and C(γ), NMR assignment for human K-Ras (residues 1-166) in the GDP-bound form at a physiological pH of 7.4. These data thereby make possible detailed monitoring of the functional cycle of Ras and its interactions with nucleotides and effector proteins through the observation of fingerprint signals from all the functionally important regions of the protein.

Published

2012

55. Two-dimensional 1H-NMR study of the spatial structure of neurotoxin II from Naja naja oxiana

Author

Victor I. Tsetlin, Alexander S. Arseniev, Alexander P. Golovanov, Andrei L. Lomize, and Yuri N. Utkin

Subjects

Magnetic Resonance Spectroscopy, Protein Conformation, Stereochemistry, Chemistry, Molecular Sequence Data, Nuclear Overhauser effect, Nuclear magnetic resonance spectroscopy, Biochemistry, Cobra Neurotoxin Proteins, Homonuclear molecule, Proton NMR, Animals, Hydrogen–deuterium exchange, Amino Acid Sequence, Protein secondary structure, Two-dimensional nuclear magnetic resonance spectroscopy

Abstract

The spatial structure of neurotoxin II from the venom of the central Asian cobra Naja naja oxiana was determined by two-dimensional 1H-NMR techniques and computational analysis. Nearly complete proton resonance assignments for 61 amino acid residues have been made using two-dimensional (2D) homonuclear total correlated spectroscopy, 2D homonuclear double-quantum-filtered correlated spectroscopy and 2D homonuclear NOE spectroscopy (NOESY) experiments. The cross-peak volumes in NOESY spectra spin-spin coupling constants of vicinal protons NH-C alpha H and C alpha H-C beta H and the observation of slow deuterium exchange of amide protons were used to define local structure and a set of constraints for distance geometry program DIANA. The average root-mean-square deviations are 53 pm for backbone heavy atoms and 118 pm for all heavy atoms of 19 final neurotoxin II conformations. The spatial structure is characterized by a short double-stranded (residues 1-5 and 13-17) and a triple-stranded (residues 22-30, 33-41 and 50-54) antiparallel beta-sheets.

Published

1993

56. ChemInform Abstract: 2D-NMR for 3D-Structure of Membrane Spanning Polypeptides: Gramacidin A and Fragments of Bacteriorhodopsin

Author

A. L. Lomize, Igor L. Barsukov, A.G. Sobol, Alexander P. Golovanov, Vladimir F. Bystrov, Innokenty V. Maslennikov, Galina V. Abdulaeva, and A. S. Arsen'ev

Subjects

Crystallography, Membrane, biology, Chemistry, biology.protein, Bacteriorhodopsin, General Medicine, Two-dimensional nuclear magnetic resonance spectroscopy

Published

2010

57. Graphene as a transparent conductive support for studying biological molecules by transmission electron microscopy

Author

J. R. Blake, Peter Blake, Andre K. Geim, S. Anissimova, Rahul R. Nair, Recep Zan, Kostya S. Novoselov, Tatiana Latychevskaia, Sergey V. Morozov, Alexander P. Golovanov, Ursel Bangert, and University of Zurich

Subjects

Materials science, Physics and Astronomy (miscellaneous), 530 Physics, FOS: Physical sciences, Nanotechnology, 10192 Physics Institute, 02 engineering and technology, 010402 general chemistry, 01 natural sciences, law.invention, law, Mesoscale and Nanoscale Physics (cond-mat.mes-hall), 3101 Physics and Astronomy (miscellaneous), Electrical conductor, chemistry.chemical_classification, Condensed Matter - Materials Science, High contrast, Condensed Matter - Mesoscale and Nanoscale Physics, Graphene, Biomolecule, Materials Science (cond-mat.mtrl-sci), 021001 nanoscience & nanotechnology, 0104 chemical sciences, Membrane, chemistry, Transmission electron microscopy, 0210 nano-technology

Abstract

We demonstrate the application of graphene as a support for imaging individual biological molecules in transmission electron microscope (TEM). A simple procedure to produce free-standing graphene membranes has been designed. Such membranes are extremely robust and can support practically any sub-micrometer object. Tobacco mosaic virus has been deposited on graphene samples and observed in a TEM. High contrast has been achieved even though no staining has been applied.

Published

2010

58. Simultaneous measurement of residual dipolar couplings for proteins in complex using the isotopically discriminated NMR approach

Author

Elena N. Tkach, A.G. Sobol, Alexander P. Golovanov, and Wolfgang Bermel

Subjects

Models, Molecular, Quantitative Biology::Biomolecules, Chemistry, Quantitative Biology::Molecular Networks, Proteins, General Chemistry, Orientation (graph theory), Residual, Biochemistry, Catalysis, Magnetic field, Quantitative Biology::Subcellular Processes, Dipole, chemistry.chemical_compound, Colloid and Surface Chemistry, Nuclear magnetic resonance, Chemical physics, Residual dipolar coupling, Amide, Nuclear Magnetic Resonance, Biomolecular

Abstract

One-bond residual dipolar couplings (RDCs) measured for the amide groups of proteins partially aligned in a magnetic field provide valuable information regarding the relative orientation of protein units. In order for RDCs obtained for individual proteins to be useful in the structure determination of heterodimer complexes, they should be measured for exactly the same alignment of the complex. Here, an isotopically discriminated IDIS-RDC-TROSY NMR experiment is proposed, which enables the measurement of HN RDCs for two proteins simultaneously and independently, but in the same sample, while they are part of the same complex. The signals for both proteins, one of which should be labeled with (15)N and the other with (15)N and (13)C, are observed in different subspectra, thus reducing spectral overlap. The approach uniquely ensures that RDCs measured for both proteins relate to exactly the same alignment tensor, allowing accurate measurement of the relative angle between the two proteins. The method is also applicable for complexes containing three or more protein components. The experiment can speed up and lead to automation of protein-protein docking on the basis of angular restraints.

Published

2009

59. The divalent cation-binding sites of gramicidin A transmembrane ion-channel

Author

Vladimir F. Bystrov, Alexander S. Arseniev, Igor L. Barsukov, Alexander P. Golovanov, Stanislav V. Sukhanov, and Barsukov Li

Subjects

Models, Molecular, inorganic chemicals, Magnetic Resonance Spectroscopy, Dimer, Biophysics, Analytical chemistry, Synthetic membrane, Biochemistry, Ion Channels, Divalent, Ion, Biomaterials, chemistry.chemical_compound, Cations, Electrochemistry, Sodium dodecyl sulfate, Ion channel, chemistry.chemical_classification, Manganese, Binding Sites, Membranes, Organic Chemistry, Gramicidin, General Medicine, Crystallography, Membrane, chemistry, Hydrate

Abstract

The conductance of the gramicidin A single channels in glycerolmonooleate membranes is strongly reduced in the presence of Mn2+ cations. The nmr experiments were performed for N-terminal to N-terminal gramicidin A dimer formed by two right-handed single-stranded helixes incorporated into the sodium dodecyl sulfate micelles in the presence of Mn2+ ions. Dependence of the nonselective spin-lattice relaxation rates of the gramicidin A protons on Mn2+ concentration was analyzed to determine coordinates of the divalent cation binding sites. It is inferred that Mn2+ ions are bound at the channel mouths at distances of 6.4, 8.6, and 8.8 A (+/- 2 A) from the oxygen atoms of exposed carbonyl groups of D-Leu 12, 14, and 10, respectively. The bounded Mn2+ retains its hydrate shell, the size of which (approximately 6 A) exceeds the inner pore diameter (approximately 4 A). That makes the gramicidin A channel impermeable for divalent cations.

Published

1991

60. Increasing the sensitivity of cryoprobe protein NMR experiments by using the sole low-conductivity arginine glutamate salt

Author

Alexander P. Golovanov and Guillaume M. Hautbergue

Subjects

chemistry.chemical_classification, Nuclear and High Energy Physics, Chromatography, Magnetic Resonance Spectroscopy, Proton, Microchemistry, Biophysics, Analytical chemistry, Arginine glutamate, Electric Conductivity, Salt (chemistry), Proteins, Reproducibility of Results, Dipeptides, Conductivity, Protein aggregation, Condensed Matter Physics, Biochemistry, Sensitivity and Specificity, Cold Temperature, chemistry.chemical_compound, chemistry, Electrical resistivity and conductivity, Sensitivity (control systems), Protein solubility

Abstract

Decrease in experimental sensitivity of cryoprobe experiments for salty samples, attributed to increased sample conductivity, has been a long-standing issue in protein NMR. Salt concentration can not be simply reduced as this often leads to protein aggregation. A simple and inexpensive solution to this problem is demonstrated here. We show that even for proteins prone to aggregation, the traditional solubilizing salt, 100mM NaCl, can be completely replaced by 50mM l-Arg and l-Glu. This replacement simultaneously reduces the sample conductivity and improves protein solubility. Up to a 6-fold overall increase in experimental sensitivity was achieved, in comparison with the traditional salty buffer. At constant protein concentration up to 2-fold increase in sensitivity was observed. The lengths of the proton pi/2 pulses were also significantly decreased, up to the level typical for non-salty samples in water.

Published

2007

61. Quantification of casein phosphorylation with conformational interpretation using Raman spectroscopy

Author

Ewan W. Blanch, Royston Goodacre, Roger M. Jarvis, James Screen, and Alexander P. Golovanov

Subjects

inorganic chemicals, Magnetic Resonance Spectroscopy, Protein Conformation, Analytical chemistry, macromolecular substances, Spectrum Analysis, Raman, Biochemistry, Analytical Chemistry, Chemometrics, symbols.namesake, Casein, Partial least squares regression, Electrochemistry, Environmental Chemistry, Animals, Least-Squares Analysis, Phosphorylation, Spectroscopy, Spectroscopy, Near-Infrared, Chemistry, Caseins, Near infrared raman spectroscopy, Calibration, symbols, Cattle, Raman optical activity, Raman spectroscopy, Quantitative analysis (chemistry)

Abstract

Raman spectroscopy is emerging as a powerful method for obtaining both quantitative and qualitative information from biological samples. One very interesting area of research, for which the technique has rarely been used, is the detection, quantification and structural analysis of post-translational modifications (PTMs) on proteins. Since Raman spectra can be used to address both of these questions simultaneously, we have developed near infrared Raman spectroscopy with appropriate chemometric approaches (partial least squares regression) to quantify low concentration (4 microM) mixtures of phosphorylated and dephosphorylated bovine alpha(s)-casein. In addition, we have used these data in conjunction with Raman optical activity (ROA) spectra and NMR to assess the structural changes that occur upon phosphorylation.

Published

2007

62. Isotopically discriminated NMR spectroscopy: a tool for investigating complex protein interactions in vitro

Author

Johanna M. Avis, Richard T. Blankley, Wolfgang Bermel, and Alexander P. Golovanov

Subjects

Stereochemistry, Allosteric regulation, Titrimetry, Proteins, Nuclear magnetic resonance spectroscopy, General Chemistry, Biochemistry, Sensitivity and Specificity, Spectral line, In vitro, Catalysis, Protein–protein interaction, chemistry.chemical_compound, Colloid and Surface Chemistry, Complex protein, chemistry, Isotopes, Amide, Molecule, Computer Simulation, Peptides, Nuclear Magnetic Resonance, Biomolecular

Abstract

A new NMR approach is presented for observing in vitro multicomponent protein-protein-ligand(s) interactions, which should help to understand how cellular networks of protein interactions operate on a molecular level and how they can be controlled with drugs. The method uniquely allows at least two polypeptide components of the mixture to be simultaneously closely monitored in a single sample, without increased signal overlap, and can be used to study complex (e.g., sequential, competitive, cooperative, allosteric, induced, etc.) binding events, witnessed by two polypeptides independently. One polypeptide is uniformly labeled with 15N and another with 15N and 13C. The 1H-15N correlation spectra are recorded for each of these molecules separately, discriminated on the basis of the type of 13C'/12C' atom attached to the amide group nitrogen. Any changes to the state of the two differently isotopically labeled molecules will be reported individually by fingerprint signals from amide groups, e.g., as unlabeled ligands are added. To our knowledge, no other technique currently exists which can monitor complex binding events in similar detail. The proposed method can be combined easily with traditional protein NMR techniques and incorporated in a variety of applications.

Published

2007

63. Assignment of 1H, 13C, and 15N resonances for the PilP pilot protein from Neisseria meningitidis

Author

Lu-Yun Lian, Jeremy P. Derrick, Benjamin T. Goult, Alexander P. Golovanov, Seetha V. Balasingham, Tone Tønjum, Christos Tzitzilonis, and Håvard Homberset

Subjects

Carbon Isotopes, Nitrogen Isotopes, Chemistry, Neisseria meningitidis, medicine.disease_cause, Gram-Positive Bacteria, Biochemistry, Microbiology, Bacterial protein, Bacterial Proteins, Fimbriae, Bacterial, medicine, Amino Acid Sequence, Fimbriae Proteins, Nuclear Magnetic Resonance, Biomolecular, Spectroscopy, Hydrogen

Published

2006

64. The solution structure of a domain from the Neisseria meningitidis lipoprotein PilP reveals a new beta-sandwich fold

Author

Benjamin T. Goult, Tone Tønjum, Jeremy P. Derrick, Alexander P. Golovanov, Seetha V. Balasingham, Håvard Homberset, Lu-Yun Lian, and Christos Tzitzilonis

Subjects

Models, Molecular, Beta-sandwich, Protein Folding, Lipoproteins, Molecular Sequence Data, Biology, Neisseria meningitidis, Pilus, Protein Structure, Secondary, Protein structure, Structural Biology, Amino Acid Sequence, Binding site, Molecular Biology, Peptide sequence, Nuclear Magnetic Resonance, Biomolecular, Binding Sites, Recombinant Proteins, Protein Structure, Tertiary, Solutions, Biochemistry, Protein folding, Fimbriae Proteins, Bacterial outer membrane, Hydrophobic and Hydrophilic Interactions, Heteronuclear single quantum coherence spectroscopy

Abstract

Type IV pili are long, thin fibres, which extend from the surface of the bacterial pathogen Neisseria meningitidis; they play a key role in adhesion and colonisation of host cells. PilP is a lipoprotein, suggested to be involved in the assembly and stabilization of an outer membrane protein, PilQ, which is required for pilus formation. Here we describe the expression of a recombinant fragment of PilP, spanning residues 20 to 181, and determination of the solution structure of a folded domain, spanning residues 85 to 163, by NMR. The N-terminal third of the protein, from residues 20 to 84, is apparently unfolded. Protease digestion yielded a 113 residue fragment that contained the folded domain. The domain adopts a simple beta-sandwich type fold, consisting of a three-stranded beta-sheet packed against a four-stranded beta-sheet. There is also a short segment of 3(10) helix at the N-terminal part of the folded domain. We were unable to identify any other proteins that are closely related in structure to the PilP domain, although the fold appears to be distantly related to the lipocalin family. Over 40 homologues of PilP have been identified in Gram-negative bacteria and the majority of conserved residues lie within the folded domain. The fourth beta-strand and adjacent loop regions contain a high proportion of conserved residues, including three glycine residues, which seem to play a role in linking the two beta-sheets. The two beta-sheets pack together to form a crevice, lined with conserved hydrophobic residues: we suggest that this feature could act as a binding site for a small ligand. The results show that PilP and its homologues have a conserved, folded domain at the C-terminal end of the protein that may be involved in mediating binding to hydrophobic ligands.

Published

2006

65. Distinct domains of small Tims involved in subunit interaction and substrate recognition

Author

Pierre Luciano, Lu-Yun Lian, Felicity Alcock, Alexander P. Golovanov, Catherine Baud, Maïlys A. S. Vergnolle, and Kostas Tokatlidis

Subjects

Saccharomyces cerevisiae Proteins, Protein subunit, Complex formation, Subunit interaction, Substrate recognition, Saccharomyces cerevisiae, Mitochondrion, Biology, Mitochondrial Membrane Transport Proteins, Mitochondrial Proteins, Structural Biology, Mitochondrial Precursor Protein Import Complex Proteins, Inner mitochondrial membrane, DNA, Fungal, Molecular Biology, Nuclear Magnetic Resonance, Biomolecular, Base Sequence, Membrane Proteins, Membrane Transport Proteins, Surface Plasmon Resonance, Cell biology, Mitochondria, Protein Structure, Tertiary, Crystallography, Protein Subunits, Multiprotein Complexes

Abstract

Tim9 and Tim10 belong to the small Tim family of mitochondrial ATP-independent chaperones. They are organised in a specific hetero-oligomeric complex (TIM10) that escorts polytopic proteins into the mitochondrial inner membrane. The contributions of the individual subunits to the assembly and function of the TIM10 complex remain poorly understood. Here, we show that substrate recognition and assembly of the complex are mediated by distinct domains of the subunits. These are unrelated to the characteristic “twin CX3C” motif that is present in all small Tims and ensures proper folding of the unassembled subunits. Specifically, we show that substrate recognition is achieved by the Tim10 subunit, whilst Tim9 serves a more structural role. The N-terminal domain of Tim10 is a substrate sensor whilst its C-terminal part is essential for complex formation. By contrast, both N and C-terminal domains of Tim9 are involved in the stability of the complex.

Published

2005

66. The structure and dynamics of tandem WW domains in a negative regulator of notch signaling, Suppressor of deltex

Author

Oleg Y. Fedoroff, Alexander P. Golovanov, Johanna M. Avis, Martin Baron, and Sharon A. Townson

Subjects

Models, Molecular, DNA, Complementary, Magnetic Resonance Spectroscopy, Phenylalanine, Ubiquitin-Protein Ligases, Molecular Sequence Data, Regulator, Notch signaling pathway, NEDD4, Ligands, Biochemistry, law.invention, WW domain, law, Animals, Drosophila Proteins, Amino Acid Sequence, Molecular Biology, Genetics, biology, Receptors, Notch, Sequence Homology, Amino Acid, Tryptophan, Membrane Proteins, Cell Biology, Ligand (biochemistry), Cell biology, Protein Structure, Tertiary, Drosophila melanogaster, Spectrometry, Fluorescence, Domain (ring theory), biology.protein, Suppressor, Drosophila, Peptides, Linker, Protein Binding

Abstract

WW domains mediate protein recognition, usually though binding to proline-rich sequences. In many proteins, WW domains occur in tandem arrays. Whether or how individual domains within such arrays cooperate to recognize biological partners is, as yet, poorly characterized. An important question is whether functional diversity of different WW domain proteins is reflected in the structural organization and ligand interaction mechanisms of their multiple domains. We have determined the solution structure and dynamics of a pair of WW domains (WW3-4) from a Drosophila Nedd4 family protein called Suppressor of deltex (Su(dx)), a regulator of Notch receptor signaling. We find that the binding of a type 1 PPPY ligand to WW3 stabilizes the structure with effects propagating to the WW4 domain, a domain that is not active for ligand binding. Both WW domains adopt the characteristic triple-stranded beta-sheet structure, and significantly, this is the first example of a WW domain structure to include a domain (WW4) lacking the second conserved Trp (replaced by Phe). The domains are connected by a flexible linker, which allows a hinge-like motion of domains that may be important for the recognition of functionally relevant targets. Our results contrast markedly with those of the only previously determined three-dimensional structure of tandem WW domains, that of the rigidly oriented WW domain pair from the RNA-splicing factor Prp40. Our data illustrate that arrays of WW domains can exhibit a variety of higher order structures and ligand interaction mechanisms.

Published

2004

67. ParG, a protein required for active partition of bacterial plasmids, has a dimeric ribbon-helix-helix structure

Author

Alexander P, Golovanov, Daniela, Barillà, Marina, Golovanova, Finbarr, Hayes, and Lu-Yun, Lian

Subjects

DNA, Bacterial, Models, Molecular, Molecular Sequence Data, Protein Structure, Secondary, Protein Structure, Tertiary, DNA-Binding Proteins, Bacterial Proteins, Genes, Bacterial, Amino Acid Sequence, Protein Structure, Quaternary, Dimerization, Nuclear Magnetic Resonance, Biomolecular, Sequence Alignment, Plasmids

Abstract

The ParG protein (8.6 kDa) is an essential component of the DNA partition complex of multidrug resistance plasmid TP228. ParG is a dimer in solution, interacts with DNA sequences upstream of the parFG genes and also with the ParF partition protein both in the absence and presence of target DNA. Here, the solution nuclear magnetic resonance structure of ParG is reported. The ParG dimer is composed of a folded domain formed by two closely intertwined C-terminal parts (residues 33-76), and two highly mobile tails consisting of N-terminal regions (residues 1-32). The folded part of ParG has the ribbon-helix-helix (RHH) architecture similar to that of the Arc/MetJ superfamily of DNA-binding transcriptional repressors, although the primary sequence similarity is very low. ParG interacts with DNA predominantly via its folded domain; this interaction is coupled with ParG oligomerization. The dimeric RHH structure of ParG suggests that it binds to DNA by inserting the double-stranded beta-sheet into the major groove of DNA, in a manner similar to transcriptional repressors from the Arc/MetJ superfamily, and that ParG can function as a transcriptional repressor itself. A new classification of proteins belonging to the Arc/MetJ superfamily and ParG homologues is proposed, based on the location of a conserved positively charged residue at either the beginning or at the end of the beta-strand which forms part of the DNA recognition motif.

Published

2003

68. Competitive and Cooperative Interactions Mediate RNA Transfer from Herpesvirus Saimiri ORF57 to the Mammalian Export Adaptor ALYREF

Author

Richard B. Tunnicliffe, Priti Kalra, Stuart A. Wilson, Alexander P. Golovanov, and Guillaume M. Hautbergue

Subjects

Macromolecular Assemblies, Viral Diseases, RNA-binding protein, Biochemistry, RNA Transport, NXF1, Biomacromolecule-Ligand Interactions, lcsh:QH301-705.5, 0303 health sciences, 030302 biochemistry & molecular biology, Nuclear Proteins, RNA-Binding Proteins, Signal transducing adaptor protein, Herpesviridae Infections, 3. Good health, Cell biology, Nucleic acids, Infectious Diseases, Transfer RNA, RNA, Viral, Medicine, Research Article, lcsh:Immunologic diseases. Allergy, Protein Structure, Immunology, Active Transport, Cell Nucleus, Biophysics, RNA transport, Repressor, Biology, Microbiology, Herpesvirus 2, Saimiriine, Host-Parasite Interactions, 03 medical and health sciences, Virology, Genetics, Humans, Protein Structure, Quaternary, Protein Interactions, Molecular Biology, 030304 developmental biology, Messenger RNA, Proteins, RNA, Herpes Simplex, Molecular biology, Repressor Proteins, Tumor Virus Infections, lcsh:Biology (General), Trans-Activators, Parasitology, lcsh:RC581-607, Transcription Factors

Abstract

The essential herpesvirus adaptor protein HVS ORF57, which has homologs in all other herpesviruses, promotes viral mRNA export by utilizing the cellular mRNA export machinery. ORF57 protein specifically recognizes viral mRNA transcripts, and binds to proteins of the cellular transcription-export (TREX) complex, in particular ALYREF. This interaction introduces viral mRNA to the NXF1 pathway, subsequently directing it to the nuclear pore for export to the cytoplasm. Here we have used a range of techniques to reveal the sites for direct contact between RNA and ORF57 in the absence and presence of ALYREF. A binding site within ORF57 was characterized which recognizes specific viral mRNA motifs. When ALYREF is present, part of this ORF57 RNA binding site, composed of an α-helix, binds preferentially to ALYREF. This competitively displaces viral RNA from the α-helix, but contact with RNA is still maintained by a flanking region. At the same time, the flexible N-terminal domain of ALYREF comes into contact with the viral RNA, which becomes engaged in an extensive network of synergistic interactions with both ALYREF and ORF57. Transfer of RNA to ALYREF in the ternary complex, and involvement of individual ORF57 residues in RNA recognition, were confirmed by UV cross-linking and mutagenesis. The atomic-resolution structure of the ORF57-ALYREF interface was determined, which noticeably differed from the homologous ICP27-ALYREF structure. Together, the data provides the first site-specific description of how viral mRNA is locked by a herpes viral adaptor protein in complex with cellular ALYREF, giving herpesvirus access to the cellular mRNA export machinery. The NMR strategy used may be more generally applicable to the study of fuzzy protein-protein-RNA complexes which involve flexible polypeptide regions., Author Summary Herpes viruses invade cells, hijacking cellular components to sustain their lifecycle and replicate. A critical step of infection is the export of viral mRNA from the nucleus to the cytoplasm, where the molecular machinery to produce proteins is located. To provide a link between their mRNA and cellular components of the mRNA export pathway, all herpesviruses use special adaptor proteins. These adaptor proteins specifically select viral mRNAs from the mixture present in the nucleus, and introduce them to cellular mRNA export factors, such as ALYREF. How these viral adaptors manage to trick ALYREF to accept foreign genetic material has not been understood on a molecular level. In this study we reveal how a typical viral adaptor protein ORF57 recognizes specific viral RNA motifs, and also how it binds to the cellular protein ALYREF. We uncover details of how ORF57 transfers the viral RNA to ALYREF, locking it in the cooperative ternary complex. We also describe the atomic-resolution structure of ORF57-ALYREF interaction interface. Together the data provides the first molecular insight of how viral mRNA is transferred between viral and cellular proteins, thus helping virus to hijack a cell.

Published

2014

69. Structural consequences of site-directed mutagenesis in flexible protein domains: NMR characterization of the L(55,56)S mutant of RhoGDI

Author

Gary M. Bokoch, Gordon C. K. Roberts, Igor L. Barsukov, Dawn Hawkins, Alexander P. Golovanov, Ramin Badii, and Lu-Yun Lian

Subjects

Models, Molecular, rac1 GTP-Binding Protein, Protein Folding, Magnetic Resonance Spectroscopy, Guanine, Protein Conformation, Mutant, Protein domain, RAC1, Biochemistry, Protein–protein interaction, chemistry.chemical_compound, Cytosol, rho-Specific Guanine Nucleotide Dissociation Inhibitors, Site-directed mutagenesis, Guanine Nucleotide Dissociation Inhibitors, Cell Membrane, Binding constant, Recombinant Proteins, Protein Structure, Tertiary, chemistry, Mutation, Biophysics, Mutagenesis, Site-Directed

Abstract

The guanine dissociation inhibitor RhoGDI consists of a folded C-terminal domain and a highly flexible N-terminal region, both of which are essential for biological activity, that is, inhibition of GDP dissociation from Rho GTPases, and regulation of their partitioning between membrane and cytosol. It was shown previously that the double mutation L55S/L56S in the flexible region of RhoGDI drastically decreases its affinity for Rac1. In the present work we study the effect of this double mutation on the conformational and dynamic properties of RhoGDI, and describe the weak interaction of the mutant with Rac1 using chemical shift mapping. We show that the helical content of the region 45–56 of RhoGDI is greatly reduced upon mutation, thus increasing the entropic penalty for the immobilization of the helix, and contributing to the loss of binding. In contrast to wild-type RhoGDI, no interaction with Rac1 could be identified for amino-acid residues of the flexible domain of the mutant RhoGDI and only very weak binding was observed for the folded domain of the mutant. The origins of the effect of the L55S/L56S mutation on the binding constant (decreased by at least three orders of magnitude relative to wild-type) are discussed with particular reference to the flexibility of this part of the protein.

Published

2001

70. Structure-activity relationships in flexible protein domains: regulation of rho GTPases by RhoGDI and D4 GDI

Author

Tsung-Hsien Chuang, Gary M. Bokoch, Ramin Badii, Gordon C. K. Roberts, Céline DerMardirossian, Igor L. Barsukov, Alexander P. Golovanov, Lu-Yun Lian, and Dawn Hawkins

Subjects

Models, Molecular, rac1 GTP-Binding Protein, rho GTP-Binding Proteins, Guanine, Protein domain, Molecular Sequence Data, Guanosine, RAC1, GTPase, Transfection, Guanosine Diphosphate, Dissociation (chemistry), Protein Structure, Secondary, chemistry.chemical_compound, Structure-Activity Relationship, rho Guanine Nucleotide Dissociation Inhibitor beta, Structural Biology, Humans, rho-Specific Guanine Nucleotide Dissociation Inhibitors, Amino Acid Sequence, Cloning, Molecular, Pliability, Molecular Biology, Nuclear Magnetic Resonance, Biomolecular, Guanine Nucleotide Dissociation Inhibitors, Sequence Deletion, rho Guanine Nucleotide Dissociation Inhibitor alpha, Binding Sites, Hydrolysis, NADPH Oxidases, Amides, In vitro, Protein Structure, Tertiary, chemistry, Biochemistry, Solvents, Guanosine Triphosphate, rhoA GTP-Binding Protein, Sequence Alignment, Heteronuclear single quantum coherence spectroscopy, HeLa Cells, Protein Binding

Abstract

The guanine dissociation inhibitors RhoGDI and D4GDI inhibit guanosine 5′-diphosphate dissociation from Rho GTPases, keeping these small GTPases in an inactive state. The GDIs are made up of two domains: a flexible N-terminal domain of about 70 amino acid residues and a folded 134-residue C-terminal domain. Here, we characterize the conformation of the N-terminal regions of both RhoGDI and D4GDI using a series of NMR experiments which include 15 N relaxation and amide solvent accessibility measurements. In each protein, two regions with tendencies to form helices are identified: residues 36 to 58 and 9 to 20 in RhoGDI, and residues 36 to 57 and 20 to 25 in D4GDI. To examine the functional roles of the N-terminal domain of RhoGDI, in vitro and in vivo functional assays have been carried out with N-terminally truncated proteins. These studies show that the first 30 amino acid residues are not required for inhibition of GDP dissociation but appear to be important for GTP hydrolysis, whilst removal of the first 41 residues completely abolish the ability of RhoGDI to inhibit GDP dissociation. The combination of structural and functional studies allows us to explain why RhoGDI and D4GDI are able to interact in similar ways with the guanosine 5′-diphosphate-bound GTPase, but differ in their ability to regulate GTP-bound forms; these functional differences are attributed to the conformational differences of the N-terminal domains of the guanosine 5′-diphosphate dissociation inhibitors. Therefore, the two transient helices, appear to be associated with different biological effects of RhoGDI, providing a clear example of structure-activity relationships in a flexible protein domain.

Published

2000

71. Recognizing misfolded and distorted protein structures by the assumption-based similarity score

Author

P.E. Volynsky, Alexander P. Golovanov, A. S. Arseniev, and S.B. Ermakova

Subjects

Protein Folding, Models, Statistical, Databases, Factual, Chemistry, Structure (category theory), Bioengineering, Biochemistry, Models, Biological, Mean squared displacement, Set (abstract data type), Folding (chemistry), Molecular dynamics, Crystallography, Protein structure, Similarity (network science), Confidence Intervals, Statistical physics, Symmetry (geometry), Molecular Biology, Biotechnology

Abstract

A new similarity score (sigma-score) is proposed which is able to find the correct protein structure among the very close alternatives and to distinguish between correct and deliberately misfolded structures. This score is based on the general principle 'similar likes similar', and it favors hydrophobic and hydrophilic contacts, and disfavors hydrophobic-to-hydrophilic contacts in proteins. The values of sigma-scores calculated for the high-resolution protein structures from the representative set are compared with those of alternatives: (i) very close alternatives which are only slightly distorted by conformational energy minimization in vacuo; (ii) alternatives with subsequently growing distortions, generated by molecular dynamics simulations in vacuo; (iii) structures derived by molecular dynamics simulation in solvent at 300 K; (iv) deliberately misfolded protein models. In nearly all tested cases the similarity score can successfully distinguish between experimental structure and its alternatives, even if the root mean square displacement of all heavy atoms is less than 1 A. The confidence interval of the similarity score was estimated using the high-resolution X-ray structures of domain pairs related by non-crystallographic symmetry. The similarity score can be used for the evaluation of the general quality of the protein models, choosing the correct structures among the very close alternatives, characterization of models simulating folding/unfolding, etc.

Published

1999

72. A new method to characterize hydrophobic organization of proteins: application to rational protein engineering of barnase

Author

Gérard Vergoten, Victor A. Jaravine, Roman G. Efremov, Mikhail P. Kirpichnikov, Alexander S. Arseniev, and Alexander P. Golovanov

Subjects

Models, Molecular, Stereochemistry, Protein Conformation, Molecular Sequence Data, Protein Engineering, Hydrophobic effect, Ribonucleases, Bacterial Proteins, Structural Biology, Enzyme Stability, Amino Acid Sequence, Amino acid residue, Amino Acids, Molecular Biology, Hydrophobicity scales, Barnase, biology, Chemistry, Spatial structure, General Medicine, Protein engineering, Crystallography, Mutation, biology.protein, Algorithms, Software

Abstract

We present a new algorithm for characterization of protein spatial structure basing on the molecular hydrophobicity potential approach. The method is illustrated by the analysis of three-dimensional structure of barnase and barnase-barstar complex. Current approach enables identification of amino acid residues situated in unfavorable environment (these residues may be "active" for binding), and to map quantitatively hydrophobic, hydrophilic and unfavorable hydrophobic-hydrophilic intra- and inter-molecular contacts involving backbone and side-chain segments of amino acid residues. Calculation of individual contributions of amino acid residues to such contacts permits identification of structurally-important residues. The contact plots obtained with molecular hydrophobicity potential calculations, provide easy rules to choose sites for mutations, which can increase a strength of intra- or inter-molecular hydrophobic interactions. The unfavorable hydrophobic-hydrophilic contact can be mutated to favorable hydrophobic, and already existing weak hydrophobic contact can be strengthen by increasing hydrophobicity of residues in contact. Basing on the analysis of the contact plots, we suggest several mutations of barnase which are supposed to increase intramolecular hydrophobic interactions, and thus might lead to increased stability of the protein. Part of these mutations was studied previously experimentally, and indeed stabilized barnase. The other of predicted mutations were not studied experimentally yet. Several new mutations of barnase and barstar are also proposed to enhance the hydrophobic interactions on their binding interface.

Published

1998

73. Detailed assessment of spatial hydrophobic and electrostatic properties of 2D NMR-derived models of neurotoxin II

Author

Alexander S. Arseniev, Roman G. Efremov, Alexander P. Golovanov, Gérard Vergoten, Victor I. Tsetlin, and Alain J.P. Alix

Subjects

Protein Folding, Magnetic Resonance Spectroscopy, Stereochemistry, Protein Conformation, Molecular Sequence Data, Neurotoxins, Protein Structure, Secondary, Protein structure, Structural Biology, Electrochemistry, Neurotoxin, Animals, Computer Simulation, Receptors, Cholinergic, Amino Acid Sequence, Elapidae, Amino Acids, Cobra Neurotoxin Proteins, Molecular Biology, chemistry.chemical_classification, Aqueous solution, Chemistry, Hydrogen bond, Intermolecular force, Water, General Medicine, Amino acid, Nicotinic acetylcholine receptor, Two-dimensional nuclear magnetic resonance spectroscopy, Algorithms

Abstract

2D NMR-derived spatial structures of neurotoxin II (NtII) and several homologous toxins in solution were assessed by comparison with their own amino acid sequences using a three-dimensional (3D) profile method [1]. 3D profiles of all the toxin models match the sequences well and, therefore, the method of 3D profile was demonstrated to work correctly for these well-resolved NMR structures in aqueous solution. At the same time, the profile window plots reveal low scores in the bottom tip of loop II (residues 22–34 in NtII) and in βstrand of loop III (residues 49–52). Some residues in the first poor-scoring region are of functional importance being involved in binding with nicotinic acetylcholine receptor (AChR). Furthermore, the second segment participates in intermolecular hydrogen bonding upon dimerization of postsynaptic neurotoxins in solution resulting in increasing of the 3D_1D score for residues at the interface between monomers. Therefore, the 3D profile method can be useful for detection functionally-important regions in well-resolved protein structures.

Published

1995

74. Fingerprinting food: current technologies for the detection of food adulteration and contamination

Author

David I. Ellis, Warwick B. Dunn, Royston Goodacre, J. William Allwood, Alexander P. Golovanov, and Victoria L. Brewster

Subjects

Food security, Chemistry(all), business.industry, Spectrum Analysis, Food Contamination, General Chemistry, Microbial contamination, Contamination, Food Analysis, Distribution system, Environmental chemistry, Food products, Food processing, Animals, Humans, business, Environmental planning, Food contaminant

Abstract

Major food adulteration and contamination events seem to occur with some regularity, such as the widely publicised adulteration of milk products with melamine and the recent microbial contamination of vegetables across Europe for example. With globalisation and rapid distribution systems, these can have international impacts with far-reaching and sometimes lethal consequences. These events, though potentially global in the modern era, are in fact far from contemporary, and deliberate adulteration of food products is probably as old as the food processing and production systems themselves. This review first introduces some background into these practices, both historically and contemporary, before introducing a range of the technologies currently available for the detection of food adulteration and contamination. These methods include the vibrational spectroscopies: near-infrared, mid-infrared, Raman; NMR spectroscopy, as well as a range of mass spectrometry (MS) techniques, amongst others. This subject area is particularly relevant at this time, as it not only concerns the continuous engagement with food adulterers, but also more recent issues such as food security, bioterrorism and climate change. It is hoped that this introductory overview acts as a springboard for researchers in science, technology, engineering, and industry, in this era of systems-level thinking and interdisciplinary approaches to new and contemporary problems. © The Royal Society of Chemistry 2012.

Published

2012

75. Structural Basis for the Recognition of Cellular mRNA Export Factor REF by Herpes Viral Proteins HSV-1 ICP27 and HVS ORF57

Author

Richard B. Tunnicliffe, Priti Kalra, Stuart A. Wilson, Alexander P. Golovanov, Adrian Whitehouse, Guillaume M. Hautbergue, and Brian R. Jackson

Subjects

viruses, Computational Biology/Macromolecular Structure Analysis, Herpesvirus 1, Human, Plasma protein binding, Biophysics/Macromolecular Assemblies and Machines, Protein Interaction Mapping, DNA-(Apurinic or Apyrimidinic Site) Lyase, Nuclear pore, lcsh:QH301-705.5, Biochemistry/Biomacromolecule-Ligand Interactions, Peptide sequence, Biochemistry/Experimental Biophysical Methods, 0303 health sciences, 030302 biochemistry & molecular biology, 3. Good health, Cell biology, Biochemistry/Macromolecular Assemblies and Machines, Molecular Biology/mRNA Transport and Localization, RNA, Viral, Molecular Biology/RNA-Protein Interactions, Research Article, Protein Binding, lcsh:Immunologic diseases. Allergy, Molecular Sequence Data, Immunology, Repressor, Biology, Microbiology, Immediate early protein, Immediate-Early Proteins, 03 medical and health sciences, Virology, Genetics, Humans, Amino Acid Sequence, RNA, Messenger, Binding site, Nuclear export signal, Molecular Biology, 030304 developmental biology, Binding Sites, Phosphoproteins, Molecular biology, Repressor Proteins, Exodeoxyribonucleases, lcsh:Biology (General), Trans-Activators, Biophysics/Biomacromolecule-Ligand Interactions, Parasitology, lcsh:RC581-607

Abstract

The herpesvirus proteins HSV-1 ICP27 and HVS ORF57 promote viral mRNA export by utilizing the cellular mRNA export machinery. This function is triggered by binding to proteins of the transcription-export (TREX) complex, in particular to REF/Aly which directs viral mRNA to the TAP/NFX1 pathway and, subsequently, to the nuclear pore for export to the cytoplasm. Here we have determined the structure of the REF-ICP27 interaction interface at atomic-resolution and provided a detailed comparison of the binding interfaces between ICP27, ORF57 and REF using solution-state NMR. Despite the absence of any obvious sequence similarity, both viral proteins bind on the same site of the folded RRM domain of REF, via short but specific recognition sites. The regions of ICP27 and ORF57 involved in binding by REF have been mapped as residues 104–112 and 103–120, respectively. We have identified the pattern of residues critical for REF/Aly recognition, common to both ICP27 and ORF57. The importance of the key amino acid residues within these binding sites was confirmed by site-directed mutagenesis. The functional significance of the ORF57-REF/Aly interaction was also probed using an ex vivo cytoplasmic viral mRNA accumulation assay and this revealed that mutants that reduce the protein-protein interaction dramatically decrease the ability of ORF57 to mediate the nuclear export of intronless viral mRNA. Together these data precisely map amino acid residues responsible for the direct interactions between viral adaptors and cellular REF/Aly and provide the first molecular details of how herpes viruses access the cellular mRNA export pathway., Author Summary When invading host cells, herpes viruses highjack cellular components to allow them to replicate. It has been long recognized that each herpes virus has a specific signature adaptor protein which, among other functions, inserts viral mRNA into the cellular mRNA nuclear export pathway, enabling production of viral proteins by the host cell. This process has been extensively studied in vivo and in vitro, but despite many efforts, the molecular and structural mechanisms of key interactions between viral adaptors and cellular mRNA export factors have not been described. Here we present the first atomic-resolution structure of the key complex between the archetypal viral adaptor ICP27 (from Herpes simplex virus 1) and the cellular mRNA export factor REF, responsible for introducing viral mRNA into the cellular nuclear export pathway. We demonstrate that despite the absence of obvious sequence similarity, the adaptor protein ORF57 from a different herpes virus (Herpesvirus saimiri) binds REF in the same site and in a similar way. We have identified and studied amino acid residues responsible for REF recognition. Together the data provide the first molecular insight into how herpesviral signature proteins recognize cellular proteins, obtaining access to the cellular mRNA export machinery.

Published

2011

76. Assignment of 1H, 13C, and 15N resonances for the REF2-I mRNA export factor

Author

Guillaume M. Hautbergue, Stuart A. Wilson, Alexander P. Golovanov, and Lu-Yun Lian

Subjects

Carbon Isotopes, Messenger RNA, Nitrogen Isotopes, Transcription, Genetic, Chemistry, RNA-Binding Proteins, Computational biology, Biochemistry, Peptide Fragments, RNA, Messenger, Nuclear export signal, Nuclear Magnetic Resonance, Biomolecular, Spectroscopy, Hydrogen

Published

2006

77. Quantification of casein phosphorylation with conformational interpretation using Raman spectroscopy.

Author

Roger M. Jarvis, Ewan W. Blanch, Alexander P. Golovanov, James Screen, and Royston Goodacre

Subjects

PHOSPHORYLATION, CASEINS, POST-translational modification, RAMAN spectroscopy

Abstract

Raman spectroscopy is emerging as a powerful method for obtaining both quantitative and qualitative information from biological samples. One very interesting area of research, for which the technique has rarely been used, is the detection, quantification and structural analysis of post-translational modifications (PTMs) on proteins. Since Raman spectra can be used to address both of these questions simultaneously, we have developed near infrared Raman spectroscopy with appropriate chemometric approaches (partial least squares regression) to quantify low concentration (4 µM) mixtures of phosphorylated and dephosphorylated bovine αs-casein. In addition, we have used these data in conjunction with Raman optical activity (ROA) spectra and NMR to assess the structural changes that occur upon phosphorylation. [ABSTRACT FROM AUTHOR]

Published

2007

78. The Effect of Point Mutations on the Biophysical Properties of an Antimicrobial Peptide: Development of a Screening Protocol for Peptide Stability Screening

Author

Günther H.J. Peters, Sowmya Indrakumar, Alexander P. Golovanov, Pernille Harris, Inas El Bialy, Werner Streicher, Matja Zalar, Allan Noergaard, Wolfgang Friess, and Christin Pohl

Subjects

protein characterization, Pore Forming Cytotoxic Proteins, Biophysics, Pharmaceutical Science, Peptide, 02 engineering and technology, Protein aggregation, 030226 pharmacology & pharmacy, protein aggregation, Protein–protein interaction, Protein Aggregates, 03 medical and health sciences, pharmaceutical screening, 0302 clinical medicine, Dynamic light scattering, Drug Discovery, medicine, Point Mutation, Thermal stability, chemistry.chemical_classification, Calorimetry, Differential Scanning, Protein Stability, Chemistry, Point mutation, protein engineering, Protein engineering, Hydrogen-Ion Concentration, Plectasin, 021001 nanoscience & nanotechnology, Dynamic Light Scattering, aggregation assessment, peptide screening, Molecular Medicine, protein−protein interactions, Peptides, 0210 nano-technology, medicine.drug

Abstract

Therapeutic peptides and proteins show enormous potential in the pharmaceutical market, but high costs in discovery and development are limiting factors so far. Single or multiple point mutations are commonly introduced in protein drugs to increase their binding affinity or selectivity. They can also induce adverse properties, which might be overlooked in a functional screen, such as a decreased colloidal or thermal stability, leading to problems in later stages of the development. In this study, we address the effect of point mutations on the stability of the 4.4 kDa antimicrobial peptide plectasin, as a case study. We combined a systematic high-throughput biophysical screen of the peptide thermal and colloidal stability using dynamic light scattering and differential scanning calorimetry with structure-based methods including small-angle X-ray scattering, analytical ultracentrifugation, and nuclear magnetic resonance spectroscopy. Additionally, we applied molecular dynamics simulations to link obtained protein stability parameters to the protein's molecular structure. Despite their predicted structural similarities, all four plectasin variants showed substantially different behavior in solution. We observed an increasing propensity of plectasin to aggregate at a higher pH, and the introduced mutations influenced the type of aggregation. Our strategy for systematically assessing the stability and aggregation of protein drugs is generally applicable and is of particular relevance, given the increasing number of protein drugs in development.

79. Amino acid residue: is it structural or functional?

Author

Victor A. Jaravine, Roman G. Efremov, Gérard Vergoten, Alexander P. Golovanov, and Alexander S. Arseniev

Subjects

Cardiotoxin, Stereochemistry, Molecular Sequence Data, Neurotoxins, Biophysics, Cardiotoxins, Biochemistry, Protein Structure, Secondary, Hydrophobic effect, Protein structure, Structural Biology, Genetics, Amino Acid Sequence, Amino Acids, Amino acid residue, Molecular Biology, Sequence Homology, Amino Acid, Chemistry, Proteins, Cell Biology, Protein engineering, Hydrophilic Interactions, Intramolecular force, Hydrophobic interactions, Neurotoxin, Snake Venoms

Abstract

A new approach is suggested for delineating the structural and functional amino acid residues in proteins with known three-dimensional structure, basing on the involvement of residues in intramolecular hydrophobic and hydrophilic interactions and additional information about the conservativity of the residues. The approach is applied to the families of homologous neurotoxins and cardiotoxins. The results obtained concerning the role of amino acid residues in both families of toxins accord well with the similarity of their fold, but different mechanisms of action. Current approach can be used for detailed characterization of protein spatial structures, as well as for rational protein engineering.

80. Mapping the binding site for the GTP-binding protein Rac-1 on its inhibitor RhoGDI-1

Author

Igor L. Barsukov, Lu-Yun Lian, Ramin Badii, Gary M. Bokoch, Kong-Hung Sze, Alexander P. Golovanov, Nicholas H. Keep, Dawn Hawkins, and Gordon C. K. Roberts

Subjects

Models, Molecular, rac1 GTP-Binding Protein, Protein Folding, Conformational change, Magnetic Resonance Spectroscopy, Protein Conformation, Molecular Sequence Data, GTPase, Plasma protein binding, In Vitro Techniques, 03 medical and health sciences, Protein structure, Structural Biology, Animals, Humans, rho-Specific Guanine Nucleotide Dissociation Inhibitors, Amino Acid Sequence, Binding site, Molecular Biology, Guanine Nucleotide Dissociation Inhibitors, 030304 developmental biology, rho Guanine Nucleotide Dissociation Inhibitor alpha, 0303 health sciences, Binding Sites, Sequence Homology, Amino Acid, Chemistry, C-terminus, 030302 biochemistry & molecular biology, Dissociation inhibitor, RhoGDI, Recombinant Proteins, Protein Structure, Tertiary, Rac, Biochemistry, Mutagenesis, Site-Directed, Biophysics, Thermodynamics, Protein folding, Protein Binding

Abstract

Background: Members of the Rho family of small GTP-binding proteins, such as Rho, Rac and Cdc42, have a role in a wide range of cell responses. These proteins function as molecular switches by virtue of a conformational change between the GTP-bound (active) and GDP-bound (inactive) forms. In addition, most members of the Rho and Rac subfamilies cycle between the cytosol and membrane. The cytosolic guanine nucleotide dissociation inhibitors, RhoGDIs, regulate both the GDP/GTP exchange cycle and the membrane association/dissociation cycle. Results: We have used NMR spectroscopy and site-directed mutagenesis to identify the regions of human RhoGDI-1 that are involved in binding Rac-1. The results emphasise the importance of the flexible regions of both proteins in the interaction. At least one specific region (residues 46–57) of the flexible N-terminal domain of RhoGDI, which has a tendency to form an amphipathic helix in the free protein, makes a major contribution to the binding energy of the complex. In addition, the primary site of Rac-1 binding on the folded domain of RhoGDI involves the β4–β5 and β6–β7 loops, with a slight movement of the 3 10 helix accompanying the interaction. This binding site is on the same face of the protein as the binding site for the isoprenyl group of post-translationally modified Rac-1, but is distinct from this site. Conclusions: Isoprenylated Rac-1 appears to interact with three distinct sites on RhoGDI. The isoprenyl group attached to the C terminus of Rac-1 binds in a pocket in the folded domain of RhoGDI. This is distinct from the major site on this domain occupied by Rac-1 itself, which involves two loops at the opposite end to the isoprenyl-binding site. It is probable that the flexible C-terminal region of Rac-1 extends from the site at which Rac-1 contacts the folded domain of RhoGDI to allow the isoprenyl group to bind in the pocket at the other end of the RhoGDI molecule. Finally, the flexible N terminus of RhoGDI-1, and particularly residues 48–58, makes a specific interaction with Rac-1 which contributes substantially to the binding affinity.

81. New Disulphide Bond in Cystatin-Based Protein Scaffold Prevents Domain-Swap-Mediated Oligomerization and Stabilizes the Functionally Active Form

Author

Alexander P. Golovanov and Matja Zalar

Subjects

chemistry.chemical_classification, Scaffold protein, 0303 health sciences, General Chemical Engineering, Dimer, Aptamer, 030302 biochemistry & molecular biology, Mutagenesis, Peptide, General Chemistry, Article, Turn (biochemistry), Chemistry, 03 medical and health sciences, chemistry.chemical_compound, Monomer, chemistry, Biophysics, Molecule, QD1-999, 030304 developmental biology

Abstract

Peptide aptamers built using engineered scaffolds are a valuable alternative to monoclonal antibodies in many research applications because of their smaller size, versatility, specificity for chosen targets, and ease of production. However, inserting peptides needed for target binding may affect the aptamer structure, in turn compromising its activity. We have shown previously that a stefin A-based protein scaffold with AU1 and Myc peptide insertions (SQT-1C) spontaneously forms dimers and tetramers and that inserted loops mediate this process. In the present study, we show that SQT-1C forms tetramers by self-association of dimers and determine the kinetics of monomer–dimer and dimer–tetramer transitions. Using site-directed mutagenesis, we show that while slow domain swapping defines the rate of dimerization, conserved proline P80 is involved in the tetramerization process. We also demonstrate that the addition of a disulphide bond at the base of the engineered loop prevents domain swapping and dimer formation, also preventing subsequent tetramerization. Formation of SQT-1C oligomers compromises the presentation of inserted peptides for target molecule binding, diminishing aptamer activity; however, the introduction of the disulphide bond locking the monomeric state enables maximum specific aptamer activity, while also increasing its thermal and colloidal stability. We conclude that stabilizing scaffold proteins by adding disulphide bonds at peptide insertion sites might be a useful approach in preventing binding-epitope-driven oligomerization, enabling creation of very stable aptamers with maximum binding activity.

82. 2D-NMR for 3D-Structure of Membrane Spanning Polypeptides: Gramacidin A and Fragments of Bacteriorhodopsin

Author

Vladimir F. Bystrov, Galina V. Abdulaeva, A. L. Lomize, A. S. Arseniev, Innokenty V. Maslennikov, Igor L. Barsukov, A.G. Sobol, and Alexander P. Golovanov

Subjects

biology, Chemistry, Stereochemistry, Dimer, Bacteriorhodopsin, Nuclear magnetic resonance spectroscopy, Antiparallel (biochemistry), Transmembrane protein, chemistry.chemical_compound, Crystallography, Membrane, Helix, biology.protein, Two-dimensional nuclear magnetic resonance spectroscopy

Abstract

Spatial structures of gramicidin A (GA) and the bacteriorhodopsin (BR) fragments in membrane mimetic milieu have been determined by NMR spectroscopy. GA incorporated into SDS micelles adopts the conformation of the monovalent cation selective transmembrane channel, i.e. head-to-head dimer formed by two right-handed π6.3 LD-helices. Interaction of impermeable Mn(II) ions with the channel was studied by paramagnetic induced proton relaxation and their preferred binding sites were evaluated. Additional results on synthetic GA analogs reveal structure-functional relationships and mechanism of channel unfolding. In contrast to micelles, organic solvents induce formation of four distinct GA double helices (parallel and antiparallel) with 5.6 residues per turn. In organic solvent in the presence of caesium salt the right-handed antiparallel double helix with 7.2 residues per turn becomes a dominant species. Discrepancies and similarities with the results obtained by other techniques are discussed.

Published

1989

83. Crystal structures of (E)-5-(4-methylphenyl)-1-(pyridin-2-yl)pent-2-en-4-yn-1-one and [3,4-bis(phenylethynyl)cyclobutane-1,2-diyl]bis(pyridin-2-ylmethanone)

Author

Ivan E. Ushakov, Ivan S. Odin, Pavel A. Gloukhov, Alexander A. Golovanov, Pavel V. Dorovatovskii, and Anna V. Vologzhanina

Subjects

vinyl ketones with acetylene fragment, cyclobutane derivatives, photoreaction, crystal structure, Crystallography, QD901-999

Abstract

Recrystallization of (E)-5-phenyl-1-(pyridin-2-yl)pent-2-en-4-yn-1-one at room temperature from ethylene glycol in daylight afforded [3,4-bis(phenylethynyl)cyclobutane-1,2-diyl)bis(pyridin-2-ylmethanone], C32H22N2O2 (3), while (E)-5-(4-methylphenyl)-1-(pyridin-2-yl)pent-2-en-4-yn-1-one, C17H13NO (2), remained photoinert. This is the first experimental evidence that pentenynones can be photoreactive when fixed in nearly coplanar parallel positions. During the photoreaction, the bond lengths and angles along the pentenyne chain changed significantly, while the disposition of the pyridyl ring towards the keto group was almost unchanged. The cyclobutane ring adopts an rctt conformation.

Published

2020

84. Michael Addition of 3-Oxo-3-phenylpropanenitrile to Linear Conjugated Enynones: Approach to Polyfunctional δ-Diketones as Precursors for Heterocycle Synthesis

Author

Anastasiya V. Igushkina, Alexander A. Golovanov, and Aleksander V. Vasilyev

Subjects

conjugated enynones, 3-oxo-3-phenylpropanenitrile, Michael addition, δ-diketones, 1,2-diazepine, Organic chemistry, QD241-441

Abstract

Reaction of linear conjugated enynones, 1,5-diarylpent-2-en-4-yn-1-ones [Ar1C≡CCH=CHC(=O)Ar2], with 3-oxo-3-phenylpropanenitrile (NCCH2COPh) in the presence of sodium methoxide MeONa as a base in MeOH at room temperature for 4–26 h affords polyfunctional δ-diketones as a product of regioselective Michael addition to the double carbon–carbon bond of starting enynones. The δ-diketones have been formed as mixtures of two diastereomers in a ratio of 2.5:1 in good general yields of 53–98%. A synthetic potential of the obtained δ-diketones has been demonstrated by heterocyclization with hydrazine into substututed 5,6-dihydro-4H-1,2-diazepine.

Published

2022

85. Stereoselective Synthesis of Multisubstituted Cyclohexanes by Reaction of Conjugated Enynones with Malononitrile in the Presence of LDA

Author

Anastasiya V. Igushkina, Alexander A. Golovanov, Irina A. Boyarskaya, Ilya E. Kolesnikov, and Aleksander V. Vasilyev

Subjects

conjugated enynones, malononitrile, cyclohexanes, carbanionic reactions, photoluminescent compounds, Organic chemistry, QD241-441

Abstract

Reaction of linear conjugated enynones, 1,5-diarylpent-2-en-4-yn-1-ones, with malononitrile in the presence of lithium diisopropylamide LDA, as a base, in THF at room temperature for 3–7 h resulted in the formation of the product of dimerization, multisubstituted polyfunctional cyclohexanes, 4-aryl-2,6-bis(arylethynyl)-3-(aryloxomethyl)-4-hydroxycyclohexane-1,1-dicarbonitriles, in yields up to 60%. Varying the reaction conditions by decreasing time and temperature and changing the ratio of starting compounds (enynone and malononitrile) allowed isolating some intermediate compounds, which confirmed a plausible reaction mechanism. The relative stability of possible stereoisomers of such cyclohexanes was estimated by quantum chemical calculations (DFT method). The obtained cyclohexanes were found to possess photoluminescent properties.

Published

2020

86. Crystal structure of (2E,4E)-5-[bis(2-hydroxyethyl)amino]-1-(4-chlorophenyl)-5-phenylpenta-2,4-dien-1-one

Author

Alexander A. Golovanov, Anna V. Vologzhanina, Ivan S. Odin, Tat'yana P. Tret'yakova, and Sergey V. Naumov

Subjects

crystal structure, dienes, enamines, hydrogen bonding, C—H...π interactions, Crystallography, QD901-999

Abstract

In the title compound, C21H22ClNO3, the pentadiene unit is nearly planar [maximum deviation = 0.023 (1) Å], but the carbonyl O atom deviates significantly [by 0.304 (1) Å] from its mean plane, which is twisted with respect to the phenyl and chlorobenzene rings by 71.34 (13) and 46.40 (13)°, respectively. In the crystal, inversion-related molecules are linked by two pairs of O—H...O hydrogen bonds, forming chains propagating along [01-1], enclosing R22(16) and R22(22) ring motifs. The chains are linked via C—H...O hydrogen bonds and C—H...π interactions into a three-dimensional supramolecular architecture.

Published

2015

87. Crystal structure of (E)-1-(2,4-dinitrophenyl)-2-[(E)-5-phenyl-1-(p-tolyl)pent-2-en-4-yn-1-ylidene]hydrazine

Author

Alexander A. Golovanov, Anna V. Vologzhanina, Evgeniya D. Voronova, Vadim V. Bekin, and Sergey V. Naumov

Subjects

crystal structure, hydrazones, hydrazine, hydrogen bonding, C—H...π interactions, π–π interactions, Crystallography, QD901-999

Abstract

In the title compound, C24H18N4O4, the plane of the phenyl ring is inclined to those of the toluene ring and the dinitro-substituted benzene ring by 66.96 (19) and 47.06 (18)°, respectively, while the planes of the two benzene rings are inclined to one another by 36.26 (19)°. There is an intramolecular N—H...O hydrogen bond between the NH group and the O atom of a nitro group, forming an S(6) ring motif. In the crystal, molecules are linked by C—H...O hydrogen bonds and C—H...π interactions, forming a three-dimensional network. There are also weak π–π interactions present involving the phenyl ring and the dinitro-substituted benzene ring [inter-centroid distance = 3.741 (2) Å].

Published

2015

88. (E,Z)-1-(4-Chlorophenyl)-5-phenyl-5-(phenylsulfanyl)penta-2,4-dien-1-one

Author

Anna V. Vologzhanina, Dmitry M. Gusev, Alexander A. Golovanov, and Valentina S. Pisareva

Subjects

Crystallography, QD901-999

Abstract

The penta-2,4-dien-1-one fragment of the title compound, C23H17ClOS, is twisted by 20.0 (3)°, as measured by the dihedral angle between the planes of the carbonyl group and its attached C atom and the distant C=C double bond and its attached C atom. The 4-chlorophenyl group forms a dihedral angle of 4.0 (3)° with the adjacent carbonyl group. Conjugation between the phenyl ring and the C=C double bond is absent; the dihedral angle between the phenyl ring and the C—C=C fragment is 34.3 (2)°. In the crystal, molecules are linked via C—H...O hydrogen bonds, forming chains parallel to the b-axis direction.

Published

2013