Your search keyword '"Panjikar, Santosh"' showing total 14 results

1. Putative dioxygen-binding sites and recognition of tigecycline and minocycline in the tetracycline-degrading monooxygenase TetX.

Author

Volkers, Gesa, Damas, João M., Palm, Gottfried J., Panjikar, Santosh, Soares, Cláudio M., and Hinrichs, Winfried

Subjects

HYDROXYLASES, AEROBIC conditions (Biochemistry), DRUG resistance in bacteria, TETRACYCLINES, RIBOSOMES, X-ray crystallography, CRYSTAL structure

Abstract

Expression of the aromatic hydroxylase TetX under aerobic conditions confers bacterial resistance against tetracycline antibiotics. Hydroxylation inactivates and degrades tetracyclines, preventing inhibition of the prokaryotic ribosome. X-ray crystal structure analyses of TetX in complex with the second-generation and third-generation tetracyclines minocycline and tigecycline at 2.18 and 2.30 Å resolution, respectively, explain why both clinically potent antibiotics are suitable substrates. Both tetracyclines bind in a large tunnel-shaped active site in close contact to the cofactor FAD, pre-oriented for regioselective hydroxylation to 11a-hydroxytetracyclines. The characteristic bulky 9- tert-butylglycylamido substituent of tigecycline is solvent-exposed and does not interfere with TetX binding. In the TetX-minocycline complex a second binding site for a minocycline dimer is observed close to the active-site entrance. The pocket is formed by the crystal packing arrangement on the surface of two neighbouring TetX monomers. Crystal structure analysis at 2.73 Å resolution of xenon-pressurized TetX identified two adjacent Xe-binding sites. These putative dioxygen-binding cavities are located in the substrate-binding domain next to the active site. Molecular-dynamics simulations were performed in order to characterize dioxygen-diffusion pathways to FADH2 at the active site. [ABSTRACT FROM AUTHOR]

Published

2013

2. High-resolution structure of Bombyx mori lipoprotein 7: crystallographic determination of the identity of the protein and its potential role in detoxification.

Author

Pietrzyk, Agnieszka J., Panjikar, Santosh, Bujacz, Anna, Mueller-Dieckmann, Jochen, Lochynska, Malgorzata, Jaskolski, Mariusz, and Bujacz, Grzegorz

Subjects

*CRYSTAL structure, *SILKWORMS, *LIPOPROTEINS, *PROTEIN crystallography, *HEMOLYMPH, *AMINO acid sequence, *BINDING sites

Abstract

Three crystal structures of a lipoprotein (Bmlp7) of unknown function, a member of the 30 kDa lipoprotein family from mulberry silkworm ( Bombyx mori L.) haemolymph, have been determined. The 1.33 Å resolution structure is an excellent example of how a precise crystallographic study can contribute to protein identification. The correct sequence of this haemolymph-isolated protein was assigned thanks to superb-quality electron-density maps. Two unexpected cadmium cations were found in this crystal structure [Bmlp7-I(Cd)] and their presence may be connected to a detoxification mechanism in this insect. For a comparison of the metal-binding sites, the crystal structure of a platinum complex (Bmlp7-Pt) was also solved at 1.94 Å resolution. The third (2.50 Å resolution) structure, of the native protein harvested in a different season (Bmlp7-II), corresponds to a different polymorph with an altered pattern of intermolecular interactions and with a total absence of cadmium ions and highlights the possible involvement of Bmlp7 in the response to environmental pollution. The N-terminal domain of Bmlp7 has a fold resembling a clockwise spiral created by six helices and can be classified as a VHS domain. The C-terminal domain is folded as a β-trefoil. The biological function of Bmlp7 is unknown, but its structural homology to sugar-binding proteins suggests that, in analogy to other 30 kDa haemolymph lipoproteins, it could play a role as an anti-apoptotic factor or function in the immune response of the insect to fungal infections. [ABSTRACT FROM AUTHOR]

Published

2012

3. Formylglycinamide ribonucleotide amidotransferase from Salmonella typhimurium: role of ATP complexation and the glutaminase domain in catalytic coupling.

Author

Tanwar, Ajay Singh, Morar, Marya, Panjikar, Santosh, and Anand, Ruchi

Subjects

GLYCINAMIDE, RIBONUCLEOTIDES, TRANSFERASES, SALMONELLA typhimurium, ADENOSINE triphosphate, GLUTAMINASES

Abstract

Formylglycinamide ribonucleotide (FGAR) amidotransferase (FGAR-AT) takes part in purine biosynthesis and is a multidomain enzyme with multiple spatially separated active sites. FGAR-AT contains a glutaminase domain that is responsible for the generation of ammonia from glutamine. Ammonia is then transferred via a channel to a second active site located in the synthetase domain and utilized to convert FGAR to formylglycinamidine ribonucleotide (FGAM) in an adenosine triphosphate (ATP) dependent reaction. In some ammonia-channelling enzymes ligand binding triggers interdomain signalling between the two diverse active centres and also assists in formation of the ammonia channel. Previously, the structure of FGAR-AT from Salmonella typhimurium containing a glutamyl thioester intermediate covalently bound in the glutaminase active site was determined. In this work, the roles played by various ligands of FGAR-AT in inducing catalytic coupling are investigated. Structures of FGAR-AT from S. typhimurium were determined in two different states: the unliganded form and the binary complex with an ATP analogue in the presence of the glutamyl thioester intermediate. The structures were compared in order to decipher the roles of these two states in interdomain communication. Using a process of elimination, the results indicated that binding of FGAR is most likely to be the major mechanism by which catalytic coupling occurs. This is because conformational changes do not occur either upon formation of the glutamyl thioester intermediate or upon subsequent ATP complexation. A model of the FGAR-bound form of the enzyme suggested that the loop in the synthetase domain may be responsible for initiating catalytic coupling via its interaction with the N-terminal domain. [ABSTRACT FROM AUTHOR]

Published

2012

4. On the routine use of soft X-rays in macromolecular crystallography. Part V. Molecular replacement and anomalous scattering.

Author

Unge, Johan, Mueller-Dieckmann, Christoph, Panjikar, Santosh, Tucker, Paul A., Lamzin, Victor S., and Weiss, Manfred S.

Subjects

SCATTERING amplitude (Physics), X-ray crystallography, MACROMOLECULES, MICROSTRUCTURE, MORPHOLOGY

Abstract

The article demonstrates the beneficial use of the combined anomalous differences and structure-factor amplitudes in molecular replacement (MR) in analyzing macromolecular structures. The study indicates that anomalous intensity differences can be utilized to enhance the performance of molecular replacement to study macromolecular structures. It demonstrates that this combined method is a promising approach to macromolecular structure studies.

Published

2011

5. Single isomorphous replacement phasing of selenomethionine-containing proteins using UV-induced radiation damage.

Author

Panjikar, Santosh, Mayerhofer, Hubert, Tucker, Paul A., Mueller-Dieckmann, Jochen, and De Sanctis, Daniele

Subjects

*PROTEINS, *ULTRAVIOLET radiation, *SELENIUM, *CRYSTALS, *X-rays

Abstract

The article discusses a research study on the phasing of selenomethionine-containing proteins with single isomorphous replacement through the use of inhouse ultraviolet (UV)-induced radiation damage. Experimental procedure include the use of three selenium-labelled proteins, simulation of protein crystal penetration depths and measurement UV absorption spectrum with the data collected on European Synchrotron Radiation Facility (ESRF). Conclusions indicated that UV can bring changes to protein crystals more than X-ray.

Published

2011

6. On the combination of molecular replacement and single-wavelength anomalous diffraction phasing for automated structure determination.

Author

Panjikar, Santosh, Parthasarathy, Venkataraman, Lamzin, Victor S., Weiss, Manfred S., and Tucker, Paul A.

Subjects

*X-ray diffraction, *MOLECULAR structure, *MATHEMATICAL models, *OPTICAL diffraction, *DATABASES

Abstract

A combination of molecular replacement and single-wavelength anomalous diffraction phasing has been incorporated into the automated structure-determination platform Auto-Rickshaw. The complete MRSAD procedure includes molecular replacement, model refinement, experimental phasing, phase improvement and automated model building. The improvement over the standard SAD or MR approaches is illustrated by ten test cases taken from the JCSG diffraction data-set database. Poor MR or SAD phases with phase errors larger than 70° can be improved using the described procedure and a large fraction of the model can be determined in a purely automatic manner from X-ray data extending to better than 2.6 Å resolution. [ABSTRACT FROM AUTHOR]

Published

2009

7. Structure of the C-terminal domain of nsp4 from feline coronavirus.

Author

Manolaridis, Ioannis, Wojdyla, Justyna A., Panjikar, Santosh, Snijder, Eric J., Gorbalenya, Alexander E., Berglind, Hanna, Nordlund, Pär, Coutard, Bruno, and Tucker, Paul A.

Subjects

CORONAVIRUSES, VIRUSES, PATHOGENIC microorganisms, GENOMES, PROTEINS

Abstract

Coronaviruses are a family of positive-stranded RNA viruses that includes important pathogens of humans and other animals. The large coronavirus genome (26-31 kb) encodes 15-16 nonstructural proteins (nsps) that are derived from two replicase polyproteins by autoproteolytic processing. The nsps assemble into the viral replication-transcription complex and nsp3, nsp4 and nsp6 are believed to anchor this enzyme complex to modified intracellular membranes. The largest part of the coronavirus nsp4 subunit is hydrophobic and is predicted to be embedded in the membranes. In this report, a conserved C-terminal domain (~100 amino-acid residues) has been delineated that is predicted to face the cytoplasm and has been isolated as a soluble domain using library-based construct screening. A prototypical crystal structure at 2.8 Å resolution was obtained using nsp4 from feline coronavirus. Unmodified and SeMet-substituted proteins were crystallized under similar conditions, resulting in tetragonal crystals that belonged to space group P43. The phase problem was initially solved by single isomorphous replacement with anomalous scattering (SIRAS), followed by molecular replacement using a SIRAS-derived composite model. The structure consists of a single domain with a predominantly α-helical content displaying a unique fold that could be engaged in protein-protein interactions. [ABSTRACT FROM AUTHOR]

Published

2009

8. The F4 fimbrial chaperone FaeE is stable as a monomer that does not require self-capping of its pilin-interactive surfaces.

Author

Van Molle, Inge, Moonens, Kristof, Buts, Lieven, Garcia-Pino, Abel, Panjikar, Santosh, Wyns, Lode, De Greve, Henri, and Bouckaert, Julie

Subjects

PILI (Microbiology), GRAM-negative bacteria, CELLS, ESCHERICHIA coli, CRYSTALS, DIMERS

Abstract

Many Gram-negative bacteria use the chaperone-usher pathway to express adhesive surface structures, such as fimbriae, in order to mediate attachment to host cells. Periplasmic chaperones are required to shuttle fimbrial subunits or pilins through the periplasmic space in an assembly-competent form. The chaperones cap the hydrophobic surface of the pilins through a donor-strand complementation mechanism. Face is the periplasmic chaperone required for the assembly of the F4 fimbriae of enterotoxigenic Escherichia coli. The FacE crystal structure shows a dimer formed by interaction between the pilin-binding interfaces of the two monomers. Dimerization and tetramerization have been observed previously in crystal structures of fimbrial chaperones and have been suggested to serve as a self-capping mechanism that protects the pilin-interactive surfaces in solution in the absence of the pilins. However, thermodynamic and biochemical data show that Face occurs as a stable monomer in solution. Other lines of evidence indicate that self-capping of the pilin-interactive interfaces is not a mechanism that is conservedly applied by all periplasmic chaperones, but is rather a case-specific solution to cap aggregation-prone surfaces. [ABSTRACT FROM AUTHOR]

Published

2009

9. On the routine use of soft X-rays in macromolecular crystallography. Part IV. Efficient determination of anomalous substructures in biomacromolecules using longer X-ray wavelengths.

Author

Kuper, Jochen, Panjikar, Santosh, Schmidt, Andrea, Mueller, Simone, Geerlof, Arie, Wilmanns, Matthias, Mueller-Dieckmann, Christoph, Singh, Rajesh K., Tucker, Paul A., and Weiss, Manfred S.

Subjects

*GRENZ rays, *CRYSTAL field theory, *BIOMACROMOLECULES, *OPTICAL diffraction, *WAVELENGTHS, *BUFFER solutions, *METAL refining, *CRYSTALLOGRAPHY

Abstract

23 different crystal forms of 19 different biological macromolecules were examined with respect to their anomalously scattering substructures using diffraction data collected at a wavelength of 2.0 Å (6.2 keV). In more than 90% of the cases the substructure was found to contain more than just the protein S atoms. The data presented suggest that chloride, sulfate, phosphate or metal ions from the buffer or even from the purification protocol are frequently bound to the protein molecule and that these ions are often overlooked, especially if they are not bound at full occupancy. Thus, in order to fully describe the macromolecule under study, it seems desirable that any structure determination be complemented with a long-wavelength data set. [ABSTRACT FROM AUTHOR]

Published

2007

10. On the routine use of soft X-rays in macromolecular crystallography. Part III. The optimal data-collection wavelength.

Author

Mueller-Dieckmann, Christoph, Panjikar, Santosh, Tucker, Paul A., and Weiss, Manfred S.

Subjects

*X-rays, *ELECTROMAGNETIC waves, *IONIZING radiation, *RADIATION, *CRYSTALLOGRAPHY, *PHYSICAL sciences

Abstract

Complete and highly redundant data sets were collected at different wavelengths between 0.80 and 2.65 Å for a total of ten different protein and DNA model systems. The magnitude of the anomalous signal-to-noise ratio as assessed by the quotient Ranom/Rr.i.m. was found to be influenced by the data-collection wavelength and the nature of the anomalously scattering substructure. By utilizing simple empirical correlations, for instance between the estimated ΔF/F and the expected Ranom or the data-collection wavelength and the expected Rr.i.m., the wavelength at which the highest anomalous signal-to-noise ratio can be expected could be estimated even before the experiment. Almost independent of the nature of the anomalously scattering substructure and provided that no elemental X-ray absorption edge is nearby, this optimal wavelength is 2.1 Å. [ABSTRACT FROM AUTHOR]

Published

2005

11. Auto-Rickshaw: an automated crystal structure determination platform as an efficient tool for the validation of an X-ray diffraction experiment.

Author

Panjikar, Santosh, Parthasarathy, Venkataraman, Lamzin, Victor S., Weiss, Manfred S., and Tucker, Paul A.

Subjects

*CRYSTALS, *CRYSTALLOGRAPHY, *X-rays, *OPTICAL diffraction, *PHYSICAL sciences

Abstract

The EMBL-Hamburg Automated Crystal Structure Determination Platform is a sys-tem that combines a number of existing macromolecular crystallographic computer programs and several decision-makers into a software pipeline for automated and efficient crystal structure determination. The pipeline can be invoked as soon as X-ray data from derivatized protein crystals have been collected and processed. It is controlled by a web-based graphical user interface for data and parameter input, and for monitoring the progress of structure determination. A large number of possible structure-solution paths are encoded in the system and the optimal path is selected by the decision-makers as the structure solution evolves. The processes have been optimized for speed so that the pipeline can be used effectively for validating the X-ray experiment at a synchrotron beamline. [ABSTRACT FROM AUTHOR]

Published

2005

12. On the routine use of soft X-rays in macromolecular crystallography. Part II. Data-collection wavelength and scaling models.

Author

Mueller-Dieckmann, Christoph, Polentarutti, Maurizio, Carugo, Kristina Djinovic, Panjikar, Santosh, Tucker, Paul A., and Weiss, Manfred S.

Subjects

MACROMOLECULES, CRYSTALLOGRAPHY, HELIUM, GRENZ rays, AIR analysis, SCALING laws (Statistical physics)

Abstract

Complete and highly redundant data sets were collected at nine different wavelengths between 0.80 and 2.65 Å on a xenon derivative of porcine pancreatic elastase in both air and helium atmospheres. The magnitude of the anomalous signal, as assessed by the xenon-peak height in the anomalous difference Patterson synthesis, is affected by the wavelength of data collection as well as by the scaling model used. For data collected at wavelengths longer than 1.7 Å, the use of a three-dimensional scaling protocol is essential in order to obtain the highest possible anomalous signal. Based on the scaling protocols currently available, the optimal wavelength range for data collection appears to be between 2.1 and 2.4 Å. Beyond that, any further increase in signal will be compensated for or even superseded by a concomitant increase in noise, which cannot be fully corrected for. Data collection in a helium atmosphere yields higher I/σ(I) values, but not significantly better anomalous differences, than data collection in air. [ABSTRACT FROM AUTHOR]

Published

2004

13. Metal binding to porcine pancreatic elastase: calcium or not calcium.

Author

Weiss, Manfred S., Panjikar, Santosh, Nowak, Elzbieta, and Tucker, Paul A.

Subjects

*DIGESTIVE enzymes, *HYDROGEN-ion concentration

Abstract

Investigates the crystallization of porcine pancreatic elastase (PPE) at acidic hydrogen-ion concentration. Detection of calcium ion in the metal-binding site of PPE; Coordination distance of the metal ions; Structure of PPE.

Published

2002

14. Xenon derivatization of halide-soaked protein crystals.

Author

Panjikar, Santosh and Tucker, Paul A.

Subjects

*XENON, *CRYSTALLOIDS (Botany)

Abstract

Investigates the xenon (Xe) derivatization of halide-soaked protein crystals. Use of Xe sites in determining the bromide substructure; Refinement of the bromide-containing structures; Crystallization of porcine pancreatic elastase.

Published

2002