Your search keyword '"Linda Cerofolini"' showing total 64 results

1. Epitope Mapping and Binding Assessment by Solid-State NMR Provide a Way for the Development of Biologics under the Quality by Design Paradigm

Author

Domenico Rizzo, Linda Cerofolini, Stefano Giuntini, Luisa Iozzino, Carlo Pergola, Francesca Sacco, Angelo Palmese, Enrico Ravera, Claudio Luchinat, Fabio Baroni, and Marco Fragai

Subjects

Biological Products, Magnetic Resonance Spectroscopy, Colloid and Surface Chemistry, Antibodies, Epitope Mapping, Proteins, General Chemistry, Biochemistry, Catalysis

Abstract

Multispecific biologics are an emerging class of drugs, in which antibodies and/or proteins designed to bind pharmacological targets are covalently linked or expressed as fusion proteins to increase both therapeutic efficacy and safety. Epitope mapping on the target proteins provides key information to improve the affinity and also to monitor the manufacturing process and drug stability. Solid-state NMR has been here used to identify the pattern of the residues of the programmed cell death ligand 1 (PD-L1) ectodomain that are involved in the interaction with a new multispecific biological drug. This is possible because the large size and the intrinsic flexibility of the complexes are not limiting factors for solid-state NMR.

Published

2022

2. Cerebrospinal fluid lipoproteins inhibit α-synuclein aggregation by interacting with oligomeric species in seed amplification assays

Author

Giovanni Bellomo, Silvia Paciotti, Luis Concha-Marambio, Domenico Rizzo, Anna Lidia Wojdaƚa, Davide Chiasserini, Leonardo Gatticchi, Linda Cerofolini, Stefano Giuntini, Chiara Maria Giulia De Luca, Yihua Ma, Carly M. Farris, Giuseppe Pieraccini, Sara Bologna, Marta Filidei, Enrico Ravera, Moreno Lelli, Fabio Moda, Marco Fragai, Lucilla Parnetti, and Claudio Luchinat

Subjects

Cellular and Molecular Neuroscience, Neurology (clinical), Molecular Biology

Abstract

Background Aggregation of α-synuclein (α-syn) is a prominent feature of Parkinson’s disease (PD) and other synucleinopathies. Currently, α-syn seed amplification assays (SAAs) using cerebrospinal fluid (CSF) represent the most promising diagnostic tools for synucleinopathies. However, CSF itself contains several compounds that can modulate the aggregation of α-syn in a patient-dependent manner, potentially undermining unoptimized α-syn SAAs and preventing seed quantification. Methods In this study, we characterized the inhibitory effect of CSF milieu on detection of α-syn aggregates by means of CSF fractionation, mass spectrometry, immunoassays, transmission electron microscopy, solution nuclear magnetic resonance spectroscopy, a highly accurate and standardized diagnostic SAA, and different in vitro aggregation conditions to evaluate spontaneous aggregation of α-syn. Results We found the high-molecular weight fraction of CSF (> 100,000 Da) to be highly inhibitory on α-syn aggregation and identified lipoproteins to be the main drivers of this effect. Direct interaction between lipoproteins and monomeric α-syn was not detected by solution nuclear magnetic resonance spectroscopy, on the other hand we observed lipoprotein-α-syn complexes by transmission electron microscopy. These observations are compatible with hypothesizing an interaction between lipoproteins and oligomeric/proto-fibrillary α-syn intermediates. We observed significantly slower amplification of α-syn seeds in PD CSF when lipoproteins were added to the reaction mix of diagnostic SAA. Additionally, we observed a decreased inhibition capacity of CSF on α-syn aggregation after immunodepleting ApoA1 and ApoE. Finally, we observed that CSF ApoA1 and ApoE levels significantly correlated with SAA kinetic parameters in n = 31 SAA-negative control CSF samples spiked with preformed α-syn aggregates. Conclusions Our results describe a novel interaction between lipoproteins and α-syn aggregates that inhibits the formation of α-syn fibrils and could have relevant implications. Indeed, the donor-specific inhibition of CSF on α-syn aggregation explains the lack of quantitative results from analysis of SAA-derived kinetic parameters to date. Furthermore, our data show that lipoproteins are the main inhibitory components of CSF, suggesting that lipoprotein concentration measurements could be incorporated into data analysis models to eliminate the confounding effects of CSF milieu on α-syn quantification efforts.

Published

2023

3. Automated Determination of Nuclear Magnetic Resonance Chemical Shift Perturbations in Ligand Screening Experiments: The PICASSO Web Server

Author

Kevin Haubrich, Marco Fragai, Linda Cerofolini, Andrea Giachetti, Vincenzo Laveglia, Antonio Rosato, and Alessio Ciulli

Subjects

Web server, Magnetic Resonance Spectroscopy, web server, Computer science, General Chemical Engineering, Library and Information Sciences, Ligands, 010402 general chemistry, Tracking (particle physics), computer.software_genre, 01 natural sciences, Spectral line, 03 medical and health sciences, Protein sequencing, Nuclear magnetic resonance, medicinal chemistry, Application Note, Humans, structural biology, Amino Acid Sequence, drug screening, Nuclear Magnetic Resonance, Biomolecular, 030304 developmental biology, 0303 health sciences, Chemical shift, Proteins, Experimental data, General Chemistry, Small molecule, NMR, 0104 chemical sciences, Computer Science Applications, Identification (information), computer, Algorithms

Abstract

Nuclear magnetic resonance (NMR) is an effective, commonly used experimental approach to screen small organic molecules against a protein target. A very popular method consists of monitoring the changes of the NMR chemical shifts of the protein nuclei upon addition of the small molecule to the free protein. Multidimensional NMR experiments allow the interacting residues to be mapped along the protein sequence. A significant amount of human effort goes into manually tracking the chemical shift variations, especially when many signals exhibit chemical shift changes and when many ligands are tested. Some computational approaches to automate the procedure are available, but none of them as a web server. Furthermore, some methods require the adoption of a fairly specific experimental setup, such as recording a series of spectra at increasing small molecule:protein ratios. In this work, we developed a tool requesting a minimal amount of experimental data from the user, implemented it as an open-source program, and made it available as a web application. Our tool compares two spectra, one of the free protein and one of the small molecule:protein mixture, based on the corresponding peak lists. The performance of the tool in terms of correct identification of the protein-binding regions has been evaluated on different protein targets, using experimental data from interaction studies already available in the literature. For a total of 16 systems, our tool achieved between 79% and 100% correct assignments, properly identifying the protein regions involved in the interaction.

Published

2021

4. Functionalized Hyaluronic Acid for 'iIn Situ/i' Matrix Metalloproteinase Inhibition: A Bioactive Material to Treat the Dry Eye Sydrome

Author

Susi Burgalassi, Marco Fragai, Oscar Francesconi, Linda Cerofolini, Daniela Monti, Gemma Leone, Stefania Lamponi, Giuseppe Greco, Agnese Magnani, and Cristina Nativi

Subjects

Polymers and Plastics, Bioactive Material, Functionalized Hyaluronic Acid, Organic Chemistry, Hyaluronoglucosaminidase, Functionalized Hyaluronic Acid, Metalloproteinase, Bioactive Material, Dry Eye Sydrome, Matrix Metalloproteinases, Inorganic Chemistry, Dry Eye Sydrome, Polysaccharides, Materials Chemistry, Humans, Dry Eye Syndromes, Hyaluronic Acid, Metalloproteinase

Abstract

Hyaluronic acid (HA) is a naturally occurring polysaccharide with many molecular functions, including maintaining the structure and physiology of the tissues, tissue remodeling, and inflammation. HA is found naturally in physiological tear fluid, possesses excellent mucus-layer-adhesive properties, and is successfully employed in the treatment of dry eye syndrome (DES). However, HA has as major drawback: its rapidiin vivo/idegradation by hyaluronidase. We report on a unique material, namely, HA-b3/b, obtained by the functionalization of HA with the metalloproteinase inhibitorb3/b(MMPI). This material is characterized by an increased resistance to hyaluronidase degradation, associated with MMP inhibition properties. The ability of HA-b3/bto prevent dehydration of human corneal epithelial cellsiin vitro/iandiin vivo/imay accelerate the development of more efficient DES treatment and broaden the application of HA in human diseases.

Published

2022

5. Cerebrospinal fluid lipoproteins inhibit α-synuclein aggregation by interacting with oligomeric species in seed amplification assays

Author

Giovanni Bellomo, Silvia Paciotti, Luis Concha-Marambio, Domenico Rizzo, Leonardo Gatticchi, Linda Cerofolini, Stefano GIuntini, Chiara Maria Giulia De Luca, Yihua Ma, Carly M. Farris, Giuseppe Pieraccini, Sara Bologna, Marta Filidei, Enrico Ravera, Moreno Lelli, Fabio Moda, Marco Fragai, Lucilla Parnetti, and Claudio Luchinat

Abstract

Background: Aggregation of α-synuclein (α-syn) is a prominent feature of Parkinson’s disease (PD) and other synucleinopathies. In these diseases, the extracellular spreading of misfolded α-syn significantly contributes to the cell-to-cell propagation of the α-syn misfolding pathology in a prion-like fashion. Therefore, extracellular α-syn aggregates are considered primary targets both for diagnostics and for novel disease modifying therapies. Currently, α-syn seed amplification assays (SAAs) using cerebrospinal fluid (CSF) represent the most promising diagnostic tools for synucleinopathies. However, CSF itself contains several compounds that can modulate the aggregation of α-syn in a patient-dependent manner, potentially sabotaging unoptimized α-syn SAAs and preventing seed quantification. Methods: In this study, we characterized the inhibitory effect of CSF on in vitro α-syn aggregation by means of CSF fractionation, mass spectrometry, dot-blot, Western blot, transmission electron microscopy, solution nuclear magnetic resonance spectroscopy, a highly accurate and standardized diagnostic SAA, and different in vitro aggregation conditions to evaluate spontaneous aggregation of α-syn. Results: We found the high-molecular weight fraction of CSF (>100,000 Da) to be highly inhibitory and identified lipoproteins to be the main drivers of this effect. We evaluated direct interaction between lipoprotein and α-syn and observed lipoprotein-α-syn complexes by transmission electron microscopy. Direct interaction between lipoproteins and monomeric α-syn was not detected by solution nuclear magnetic resonance spectroscopy, suggesting interaction between lipoproteins and oligomeric/proto-fibrillary α-syn intermediates instead. Lastly, we observed significantly slower amplification of α-syn seeds in PD CSF when lipoproteins were added to the reaction mix of a highly accurate diagnostic SAA. Conclusions: Our results describe a novel interaction between lipoproteins and α-syn aggregates that inhibits the formation of α-syn fibrils and could have relevant biological and translational implications. Indeed, the donor-specific inhibition of CSF on α-syn aggregation explains the lack of quantitative results so far obtained by the analysis of SAA-derived kinetic parameters. Furthermore, our data show that apolipoproteins are the main inhibitory components of CSF, suggesting that lipoprotein concentration measurements could be incorporated into data analysis models to eliminate the confounding effects of CSF milieu on α-syn quantification efforts.

Published

2022

6. Elucidating the concentration-dependent effects of thiocyanate binding to carbonic anhydrase

Author

José Malanho Silva, Linda Cerofolini, Ana Luísa Carvalho, Enrico Ravera, Marco Fragai, Giacomo Parigi, Anjos L. Macedo, Carlos F.G.C. Geraldes, and Claudio Luchinat

Subjects

Inorganic Chemistry, Biochemistry

Published

2023

7. Identification and Characterization of an RRM-Containing, RNA Binding Protein in

Author

Caterina, Ciani, Anna, Pérez-Ràfols, Isabelle, Bonomo, Mariachiara, Micaelli, Alfonso, Esposito, Chiara, Zucal, Romina, Belli, Vito Giuseppe, D'Agostino, Irene, Bianconi, Vito, Calderone, Linda, Cerofolini, Orietta, Massidda, Michael Bernard, Whalen, Marco, Fragai, and Alessandro, Provenzani

Subjects

Acinetobacter baumannii, Proteome, Animals, Humans, RNA, RNA-Binding Proteins, Carrier Proteins, RNA Recognition Motif, Protein Binding

Published

2022

8. Interhelical interactions within the STIM1 CC1 domain modulate CRAC channel activation

Author

Linda Cerofolini, Matthias Bechmann, Petr Rathner, Marc Fahrner, Norbert Müller, Herwig Grabmayr, Ferdinand Horvath, Marco Fragai, Agrim Gupta, Christoph Romanin, Thomas Renger, Enrico Ravera, Claudio Luchinat, and Heinrich Krobath

Subjects

inorganic chemicals, Models, Molecular, Magnetic Resonance Spectroscopy, Patch-Clamp Techniques, ORAI1 Protein, Migraine Disorders, Mutant, chemistry.chemical_element, Erythrocytes, Abnormal, Calcium, Article, Dyslexia, 03 medical and health sciences, Humans, Patch clamp, Stromal Interaction Molecule 1, Cloning, Molecular, Molecular Biology, 030304 developmental biology, 0303 health sciences, C-terminus, Endoplasmic reticulum, Calcium channel, 030302 biochemistry & molecular biology, HEK 293 cells, Ichthyosis, STIM1, Cell Biology, Miosis, Calcium Release Activated Calcium Channels, Neoplasm Proteins, HEK293 Cells, chemistry, Muscle Fatigue, Mutation, Biophysics, Nucleic Acid Conformation, Blood Platelet Disorders, Spleen

Abstract

The calcium release activated calcium channel is activated by the endoplasmic reticulum-resident calcium sensor protein STIM1. On activation, STIM1 C terminus changes from an inactive, tight to an active, extended conformation. A coiled-coil clamp involving the CC1 and CC3 domains is essential in controlling STIM1 activation, with CC1 as the key entity. The nuclear magnetic resonance-derived solution structure of the CC1 domain represents a three-helix bundle stabilized by interhelical contacts, which are absent in the Stormorken disease-related STIM1 R304W mutant. Two interhelical sites between the CC1α1 and CC1α2 helices are key in controlling STIM1 activation, affecting the balance between tight and extended conformations. Nuclear magnetic resonance-directed mutations within these interhelical interactions restore the physiological, store-dependent activation behavior of the gain-of-function STIM1 R304W mutant. This study reveals the functional impact of interhelical interactions within the CC1 domain for modifying the CC1-CC3 clamp strength to control the activation of STIM1.

Published

2020

9. Small-Molecule Ebselen Binds to YTHDF Proteins Interfering with the Recognition of

Author

Mariachiara, Micaelli, Andrea, Dalle Vedove, Linda, Cerofolini, Jacopo, Vigna, Denise, Sighel, Sara, Zaccara, Isabelle, Bonomo, Georgios, Poulentzas, Emanuele Filiberto, Rosatti, Giulia, Cazzanelli, Laura, Alunno, Romina, Belli, Daniele, Peroni, Erik, Dassi, Shino, Murakami, Samie R, Jaffrey, Marco, Fragai, Ines, Mancini, Graziano, Lolli, Alessandro, Quattrone, and Alessandro, Provenzani

Abstract

YTHDF proteins bind the

Published

2022

10. Solid-state NMR methods for the characterization of bioconjugations and protein-material interactions

Author

Linda Cerofolini, Giacomo Parigi, Enrico Ravera, Marco Fragai, and Claudio Luchinat

Subjects

Nuclear and High Energy Physics, Magnetic Resonance Spectroscopy, Radiation, Proteins, General Chemistry, Magnetic Resonance Imaging, Instrumentation

Abstract

Protein solid-state NMR has evolved dramatically over the last two decades, with the development of new hardware and sample preparation methodologies. This technique is now ripe for complex applications, among which one can count bioconjugation, protein chemistry and functional biomaterials. In this review, we provide our account on this aspect of protein solid-state NMR.

Published

2022

11. Mixing Aβ(1–40) and Aβ(1–42) peptides generates unique amyloid fibrils

Author

Annett Böddrich, Domenico Rizzo, Iryna Benilova, Bettina Purfürst, Sara Bologna, Claudio Luchinat, Linda Cerofolini, Bart De Strooper, Leonardo Gonnelli, Gianluca Gallo, Erich E. Wanker, Marco Fragai, Thomas Wiglenda, Enrico Ravera, and Magdalena Korsak

Subjects

Models, Molecular, macromolecular substances, Protein aggregation, 010402 general chemistry, Fibril, 01 natural sciences, Protein Structure, Secondary, Catalysis, Protein Aggregates, 03 medical and health sciences, Protein structure, Materials Chemistry, Mixing (physics), 030304 developmental biology, 0303 health sciences, Amyloid beta-Peptides, Chemistry, Metals and Alloys, General Chemistry, Amyloid fibril, Peptide Fragments, 0104 chemical sciences, Surfaces, Coatings and Films, Electronic, Optical and Magnetic Materials, Ceramics and Composites, Biophysics, Technology Platforms, Function and Dysfunction of the Nervous System

Abstract

Recent structural studies show distinct morphologies for the fibrils of Aβ(1-42) and Aβ(1-40), which are believed not to co-fibrillize. We describe here a novel, structurally-uniform 1 : 1 mixed fibrillar species, which differs from both pure fibrils. It forms preferentially even when Aβ(1-42) : Aβ(1-40) peptides are mixed in a non-stoichiometric ratio.

Published

2020

12. Insights into telomeric G-quadruplex DNA recognition by HMGB1 protein

Author

Claudio Luchinat, Antonio Rosato, Jussara Amato, Ettore Novellino, Annamaria Biroccio, Linda Cerofolini, Stefano Giuntini, Bruno Pagano, Antonio Randazzo, Diego Brancaccio, Marco Fragai, Sara Iachettini, Pasquale Zizza, Nunzia Iaccarino, Amato, J., Cerofolini, L., Brancaccio, D., Giuntini, S., Iaccarino, N., Zizza, P., Iachettini, S., Biroccio, A., Novellino, E., Rosato, A., Fragai, M., Luchinat, C., Randazzo, A., and Pagano, B.

Subjects

Cell biology, DNA repair, DNA damage, chemical and pharmacologic phenomena, Biology, G-quadruplex, 03 medical and health sciences, chemistry.chemical_compound, 0302 clinical medicine, Structural Biology, Transcription (biology), Escherichia coli, Genetics, Humans, Gene silencing, HMGB1 Protein, Telomerase, 030304 developmental biology, 0303 health sciences, DNA, Telomere, G-Quadruplexes, chemistry, Nucleic acid, 030220 oncology & carcinogenesis, Magnetic Resonance Spectroscopy, Protein, K+ SOLUTION, BINDING, DOMAIN, CELLS, BOXES, D(TTAGGGT)(4), POLYMORPHISM, EXTENSION, COMPLEX, Nucleic Acid Conformation

Abstract

HMGB1 is a ubiquitous non-histone protein, which biological effects depend on its expression and subcellular location. Inside the nucleus, HMGB1 is engaged in many DNA events such as DNA repair, transcription and telomere maintenance. HMGB1 has been reported to bind preferentially to bent DNA as well as to noncanonical DNA structures like 4-way junctions and, more recently, to G-quadruplexes. These are four-stranded conformations of nucleic acids involved in important cellular processes, including telomere maintenance. In this frame, G-quadruplex recognition by specific proteins represents a key event to modulate physiological or pathological pathways. Herein, to get insights into the telomeric G-quadruplex DNA recognition by HMGB1, we performed detailed biophysical studies complemented with biological analyses. The obtained results provided information about the molecular determinants for the interaction and showed that the structural variability of human telomeric G-quadruplex DNA may have significant implications in HMGB1 recognition. The biological data identified HMGB1 as a telomere-associated protein in both telomerase-positive and -negative tumor cells and showed that HMGB1 gene silencing in such cells induces telomere DNA damage foci. Altogether, these findings provide a deeper understanding of telomeric G-quadruplex recognition by HMGB1 and suggest that this protein could actually represent a new target for cancer therapy.

Published

2019

13. Nanoparticles for the multivalent presentation of a TnThr mimetic and as tool for solid state NMR coating investigation

Author

Linda Cerofolini, Cristina Nativi, Francesco Papi, Marco Fragai, Claudio Luchinat, and Giulia Targetti

Subjects

Tumor-Associated Carbohydrate Antigens, 010405 organic chemistry, Chemistry, General Chemical Engineering, Synthetic antigen, Nanoparticle, 02 engineering and technology, General Chemistry, engineering.material, 021001 nanoscience & nanotechnology, 01 natural sciences, Combinatorial chemistry, 0104 chemical sciences, Silica nanoparticles, chemistry.chemical_compound, Solid-state nuclear magnetic resonance, Coating, engineering, 0210 nano-technology, Iron oxide nanoparticles

Abstract

The fully characterization of tumor associated antigens (TAAs) and of tumor associated carbohydrate antigens (TACAs) have opened the avenue of cancer immunotherapy. The intrinsic poor immunogenicity of TACAs, however, spotlighted the importance of multivalent presentation of the antigen(s) to trigger an immune response. Nanoparticles are excellent scaffolds for this purpose. Here we reported on the easy glycosylation of iron-based and biocompatible dextran-based nanoparticles with 1, a mimetic of the TnThr antigen. The multivalent presentation of 1 induced the induction of TNF-α and IL-6/IL10, respectively. The multivalent glycosylation of silica nanoparticles (GSiNPs) was also performed and saccharide loading qualitative assessed by solid state NMR. Our results offer the proof of concept that biomolecules coating can also be investigated on solid system by NMR.

Published

2019

14. An Integrative Approach to Understand the Effect of Sodium Thiocyanate on Human Carbonic Anhydrase 2

Author

Marta Cação, Ana P. Carvalho, Linda Cerofolini, Anjos L. Macedo, José Roberto Lapa e Silva, Enrico Ravera, Carlos F. G. C. Geraldes, Claudio Luchinat, and Giacomo Parigi

Subjects

chemistry.chemical_compound, biology, Biochemistry, Chemistry, Carbonic anhydrase, Genetics, biology.protein, Sodium thiocyanate, Molecular Biology, Biotechnology

Published

2021

15. Characterization of lanthanoid-binding proteins using NMR spectroscopy

Author

Enrico, Ravera, Linda, Cerofolini, Marco, Fragai, Giacomo, Parigi, and Claudio, Luchinat

Subjects

Magnetic Resonance Spectroscopy, Protein Conformation, Proteins, Carrier Proteins, Lanthanoid Series Elements, Nuclear Magnetic Resonance, Biomolecular

Abstract

The variety of magnetic properties exhibited by paramagnetic lanthanoids provides outstanding information in NMR-based structural biology and therefore can be a very useful tool for characterizing lanthanoid-binding proteins. Because of their dependence on the relative positions of the protein nuclei and of the lanthanoid ion, the paramagnetic restraints (PCS, PRDC and PRE) provide information on structure and dynamics of proteins. In this Chapter, we cover the use of lanthanoids in structural biology including protein sample preparation, NMR experiments and data interpretation.

Published

2021

16. Interfering with the Tumor-Immune Interface: Making Way for Triazine-Based Small Molecules as Novel PD-L1 Inhibitors

Author

Linda Cerofolini, Gerolama Condorelli, Giovanna Polcaro, Daniela Arosio, Vincenzo Maria D'Amore, Stefano Pepe, Riccardo Scaglia, Marco Fragai, E. Novellino, Giulia Assoni, Luciana Marinelli, Pasquale Russomanno, Stefano Giuntini, Jussara Amato, Diego Brancaccio, Francesco Sabbatino, Marianna Falzoni, Valeria La Pietra, Greta Donati, Paolo Orlando, Pierfausto Seneci, Cristina Quintavalle, Martina Pedrini, Bruno Pagano, Russomanno, P., Assoni, G., Amato, J., D'Amore, V. M., Scaglia, R., Brancaccio, D., Pedrini, M., Polcaro, G., La Pietra, V., Orlando, P., Falzoni, M., Cerofolini, L., Giuntini, S., Fragai, M., Pagano, B., Donati, G., Novellino, E., Quintavalle, C., Condorelli, G., Sabbatino, F., Seneci, P., Arosio, D., Pepe, S., and Marinelli, L.

Subjects

Models, Molecular, medicine.drug_class, Immune Checkpoint Inhibitor, B7-H1 Antigen, Calorimetry, Differential Scanning, Cell Line, Tumor, Coculture Techniques, Humans, Immune Checkpoint Inhibitors, Neoplasms, Small Molecule Libraries, Structure-Activity Relationship, Triazines, Calorimetry, Monoclonal antibody, Differential Scanning, Peripheral blood mononuclear cell, PD-1/PD-L1, Cell Line, 03 medical and health sciences, 0302 clinical medicine, Immune system, Small Molecule Librarie, Models, PD-L1, Drug Discovery, medicine, Cytotoxicity, Coculture Technique, immune checkpoint, 030304 developmental biology, 0303 health sciences, Tumor, biology, Chemistry, Molecular, Small molecule, 3. Good health, Triazine, Apoptosis, 030220 oncology & carcinogenesis, Cancer cell, Cancer research, biology.protein, Molecular Medicine, Neoplasm, Human

Abstract

The inhibition of the PD-1/PD-L1 axis by monoclonal antibodies has achieved remarkable success in treating a growing number of cancers. However, a novel class of small organic molecules, with BMS-202 (1) as the lead, is emerging as direct PD-L1 inhibitors. Herein, we report a series of 2,4,6-tri- and 2,4-disubstituted 1,3,5-triazines, which were synthesized and assayed for their PD-L1 binding by NMR and homogeneous time-resolved fluorescence. Among them, compound 10 demonstrated to strongly bind with the PD-L1 protein and challenged it in a co-culture of PD-L1 expressing cancer cells (PC9 and HCC827 cells) and peripheral blood mononuclear cells enhanced antitumor immune activity of the latter. Compound 10 significantly increased interferon γ release and apoptotic induction of cancer cells, with low cytotoxicity in healthy cells when compared to 1, thus paving the way for subsequent preclinical optimization and medical applications.

Published

2021

17. Evaluation of the Higher Order Structure of Biotherapeutics Embedded in Hydrogels for Bioprinting and Drug Release

Author

Anna Pérez-Ràfols, Stefano Giuntini, Claudio Luchinat, Enrico Ravera, Domenico Rizzo, Linda Cerofolini, Marco Fragai, and Fabio Baroni

Subjects

Tissue Engineering, Tissue Scaffolds, Chemistry, Bioprinting, Hydrogels, Nanotechnology, 02 engineering and technology, 010402 general chemistry, 021001 nanoscience & nanotechnology, Biocompatible material, 01 natural sciences, Article, 0104 chemical sciences, Analytical Chemistry, Drug Liberation, Printing, Three-Dimensional, Tissue scaffolds, Tissue engineering, Three-Dimensional, Self-healing hydrogels, Drug release, Printing, 0210 nano-technology, Higher Order Structure

Abstract

Biocompatible hydrogels for tissue regeneration/replacement and drug release with specific architectures can be obtained by three-dimensional bioprinting techniques. The preservation of the higher order structure of the proteins embedded in the hydrogels as drugs or modulators is critical for their biological activity. Solution nuclear magnetic resonance (NMR) experiments are currently used to investigate the higher order structure of biotherapeutics in comparability, similarity, and stability studies. However, the size of pores in the gel, protein–matrix interactions, and the size of the embedded proteins often prevent the use of this methodology. The recent advancements of solid-state NMR allow for the comparison of the higher order structure of the matrix-embedded and free isotopically enriched proteins, allowing for the evaluation of the functionality of the material in several steps of hydrogel development. Moreover, the structural information at atomic detail on the matrix–protein interactions paves the way for a structure-based design of these biomaterials.

Published

2021

18. Characterization of lanthanoid-binding proteins using NMR spectroscopy

Author

Linda Cerofolini, Claudio Luchinat, Giacomo Parigi, Enrico Ravera, and Marco Fragai

Subjects

Lanthanide, Paramagnetism, Crystallography, Structural biology, Chemistry, Relaxation (NMR), Sample preparation, Nuclear magnetic resonance spectroscopy, Magnetic susceptibility, Characterization (materials science)

Abstract

The variety of magnetic properties exhibited by paramagnetic lanthanoids provides outstanding information in NMR-based structural biology and therefore can be a very useful tool for characterizing lanthanoid-binding proteins. Because of their dependence on the relative positions of the protein nuclei and of the lanthanoid ion, the paramagnetic restraints (PCS, PRDC and PRE) provide information on structure and dynamics of proteins. In this Chapter, we cover the use of lanthanoids in structural biology including protein sample preparation, NMR experiments and data interpretation.

Published

2021

19. CXCR4 antagonism sensitizes cancer cells to novel indole-based MDM2/4 inhibitors in glioblastoma multiforme

Author

Claudia Martini, Valeria La Pietra, Romano Silvestri, Linda Cerofolini, Simona Daniele, Michela Puxeddu, Sabrina Taliani, Chiara Cavallini, Martina Pedrini, Stefano Giuntini, Marianna Nalli, Vincenzo Maria D'Amore, Luciana Marinelli, Marco Fragai, Claudio Luchinat, Ettore Novellino, Deborah Pietrobono, Rebecca Piccarducci, Giuseppe La Regina, Pasquale Russomanno, Daniele, S., La Pietra, V., Piccarducci, R., Pietrobono, D., Cavallini, C., D'Amore, V. M., Cerofolini, L., Giuntini, S., Russomanno, P., Puxeddu, M., Nalli, M., Pedrini, M., Fragai, M., Luchinat, C., Novellino, E., Taliani, S., La Regina, G., Silvestri, R., Martini, C., and Marinelli, L.

Subjects

0301 basic medicine, p53, Benzylamines, Indoles, Cell Cycle Proteins, Cyclams, CXCR4, Benzylamine, 0302 clinical medicine, Cell Movement, Cell Cycle Protein, Antineoplastic Combined Chemotherapy Protocols, Proto-Oncogene Protein, CXCR4 antagonist, biology, Chemistry, GBM stem-Like cells (GSCs), Brain Neoplasms, Drug Synergism, Proto-Oncogene Proteins c-mdm2, Cyclam, Neoplastic Stem Cells, Mdm2, Stem cell, Human, Signal Transduction, Receptors, CXCR4, Neurogenesis, Brain Neoplasm, 03 medical and health sciences, MDM4, Downregulation and upregulation, MDM2, Glioma, Neurosphere, Cell Line, Tumor, Proto-Oncogene Proteins, Spheroids, Cellular, medicine, Humans, Neoplasm Invasiveness, Cell Proliferation, Pharmacology, Neoplasm Invasivene, Glioblastoma multiforme (GBM), Antineoplastic Combined Chemotherapy Protocol, medicine.disease, 030104 developmental biology, Indole, Cancer cell, biology.protein, Cancer research, Neurogenesi, Neoplastic Stem Cell, Tumor Suppressor Protein p53, Glioblastoma, 030217 neurology & neurosurgery

Abstract

Glioblastoma Multiforme (GBM) is a highly invasive primary brain tumour characterized by chemo- and radio-resistance and poor overall survival. GBM can present an aberrant functionality of p53, caused by the overexpression of the murine double minute 2 protein (MDM2) and its analogue MDM4, which may influence the response to conventional therapies. Moreover, tumour resistance/invasiveness has been recently attributed to an overexpression of the chemokine receptor CXCR4, identified as a pivotal mediator of glioma neovascularization. Notably, CXCR4 and MDM2-4 cooperate in promoting tumour invasion and progression. Although CXCR4 actively promotes MDM2 activation leading to p53 inactivation, MDM2-4 knockdown induces the downregulation of CXCR4 gene transcription. Our study aimed to assess if the CXCR4 signal blockade could enhance glioma cells' sensitivity to the inhibition of the p53-MDMs axis. Rationally designed inhibitors of MDM2/4 were combined with the CXCR4 antagonist, AMD3100, in human GBM cells and GBM stem-like cells (neurospheres), which are crucial for tumour recurrence and chemotherapy resistance. The dual MDM2/4 inhibitor RS3594 and the CXCR4 antagonist AMD3100 reduced GBM cell invasiveness and migration in single-agent treatment and mainly in combination. AMD3100 sensitized GBM cells to the antiproliferative activity of RS3594. It is noteworthy that these two compounds present synergic effects on cancer stem components: RS3594 inhibited the growth and formation of neurospheres, AMD3100 induced differentiation of neurospheres while enhancing RS3594 effectiveness preventing their proliferation/clonogenicity. These results confirm that blocking CXCR4/MDM2/4 represents a valuable strategy to reduce GBM proliferation and invasiveness, acting on the stem cell component too.

Published

2020

20. Single Peptide Backbone Surrogate Mutations to Regulate Angiotensin GPCR Subtype Selectivity

Author

Mark P. Del Borgo, Ibai E. Valverde, Linda Cerofolini, Alba Mascarin, Hamidreza Shaye, Adina T. Michael-Titus, Claudio Luchinat, Vadim Cherezov, Francesca Magnani, Essam Ghazaly, Patrick N. Pallier, Marco Fragai, Andreas G. Tzakos, Thomas L. Mindt, Nelofer Syed, Marie-Isabel Aguilar, Eirinaios I. Vrettos, Nathalie M. Grob, Evgenios Κ. Stylos, Tim Crook, Robert E Widdop, Nick Bekas, Emal Waqif, Baydaa Hirmiz, Giacomo Parigi, Institut de Chimie Moléculaire de l'Université de Bourgogne [Dijon] (ICMUB), Centre National de la Recherche Scientifique (CNRS)-Université de Bourgogne (UB)-Institut de Chimie du CNRS (INC), Barrow Foundation UK, Brain Tumour Research Campaign, and Brain Tumour Research

Subjects

Peptidomimetic, Stereochemistry, Chemistry, Multidisciplinary, [SDV]Life Sciences [q-bio], G-protein-coupled receptors, Peptide, [CHIM.THER]Chemical Sciences/Medicinal Chemistry, Ligands, Click chemistry, Competition-binding experiments, Neurotrophic effects, Peptidomimetics, 010402 general chemistry, 01 natural sciences, Catalysis, Substrate Specificity, neurotrophic effects, competition-binding experiments, Animals, Humans, Peptide bond, Amino Acids, ComputingMilieux_MISCELLANEOUS, G protein-coupled receptor, chemistry.chemical_classification, Receptors, Angiotensin, Science & Technology, Angiotensin II receptor type 1, 010405 organic chemistry, [CHIM.ORGA]Chemical Sciences/Organic chemistry, Angiotensin II, Organic Chemistry, General Chemistry, 0104 chemical sciences, Amino acid, Chemistry, HEK293 Cells, chemistry, peptidomimetics, Mutation, Physical Sciences, click chemistry, Peptides, 03 Chemical Sciences, Two-dimensional nuclear magnetic resonance spectroscopy

Abstract

Mutating the side-chains of amino acids in a peptide ligand, with unnatural amino acids, aiming to mitigate its short half-life is an established approach. However, it is hypothesized that mutating specific backbone peptide bonds with bioisosters can be exploited not only to enhance the proteolytic stability of parent peptides, but also to tune its receptor subtype selectivity. Towards this end, four [Y]6-Angiotensin II analogues are synthesized where amide bonds have been replaced by 1,4-disubstituted 1,2,3-triazole isosteres in four different backbone locations. All the analogues possessed enhanced stability in human plasma in comparison with the parent peptide, whereas only two of them achieved enhanced AT2R/AT1R subtype selectivity. This diversification has been studied through 2D NMR spectroscopy and unveiled a putative more structured microenvironment for the two selective ligands accompanied with increased number of NOE cross-peaks. The most potent analogue, compound 2, has been explored regarding its neurotrophic potential and resulted in an enhanced neurite growth with respect to the established agent C21. © 2020 Wiley-VCH Verlag GmbH & Co. KGaA, Weinheim. ISSN:0947-6539 ISSN:1521-3765

Published

2020

21. Fucosylated Ubiquitin and Orthogonally Glycosylated Mutant A28C: Conceptually New Ligands for Burkholderia Ambifaria Lectin (BambL)†

Author

Grazia Lombardi, Marco Fragai, Silvia Fallarini, Sakonwan Kuhaudomlarp, Cristina Nativi, Anne Imberty, Linda Cerofolini, Alessandro Dondoni, Carolina Valori, Stefano Giuntini, Emilie Gillon, Maxime Denis, Sabrina Santarsia, Centre de Recherches sur les Macromolécules Végétales (CERMAV), Institut de Chimie du CNRS (INC)-Centre National de la Recherche Scientifique (CNRS)-Université Grenoble Alpes (UGA), Consorzio Interuniversitario Risonanze Magnetiche di Metallo Proteine (CIRMMP), and Università degli Studi di Siena = University of Siena (UNISI)-Università degli Studi di Firenze = University of Florence [Firenze] (UNIFI)-University of Bologna-Partenaires INRAE

Subjects

chemistry.chemical_classification, Scaffold protein, biology, 010405 organic chemistry, Rhamnose, Chemistry, Mutant, Glycoside, Lectin, Burkholderia ambifaria, General Chemistry, 010402 general chemistry, biology.organism_classification, 01 natural sciences, 0104 chemical sciences, 3. Good health, chemistry.chemical_compound, Residue (chemistry), Immune system, Structural biology, Biochemistry, Ubiquitin, biology.protein, [CHIM]Chemical Sciences

Abstract

Two orthogonal, metal free click reactions, enabled to glycosylate ubiquitin and its mutant A28C forming two protein scaffolds with high affinity for BambL, a lectin from the human pathogen Burkholderia ambifaria. A new fucoside analogue, with high affinity with BambL, firstly synthetized and co-crystallized with the protein target, provided the insights for sugar determinants grafting onto ubiquitin. Three ubiquitin-based glycosides were thus assembled. Fuc-Ub, presented several copies of the fucoside analogue, with proper geometry for multivalent effect; Rha-A28C, displayed one thio-rhamnose, known for its ability to tuning the immunological response; finally, Fuc-Rha-A28C, included both multiple fucoside analogs and the rhamnose residue. Fuc-Ub and Fuc-Rha-A28C ligands proved high affinity for BambL and unprecedented immune modulatory properties towards macrophages activation., Metal free click reactions used to glycosylate ubiquitin and its mutant A28C afforded two protein scaffolds with high affinity for Burkholderia ambifaria lectin (BambL).

Published

2020

22. Orientation of immobilized antigens on common surfaces by a simple computational model: Exposition of SARS-CoV-2 Spike protein RBD epitopes

Author

Linda Cerofolini, Enrico Ravera, Claudio Luchinat, and Marco Fragai

Subjects

Models, Molecular, Surface Properties, Severe acute respiratory syndrome coronavirus 2 (SARS-CoV-2), Protein domain, Biophysics, Molecular Docking Simulation, Biochemistry, Epitope, Article, Betacoronavirus, Epitopes, Antigen, Protein Domains, Simple (abstract algebra), Antigens, Protein-surface interaction, Bioconjugation, Orientation (computer vision), Chemistry, SARS-CoV-2, Organic Chemistry, United residue model, Silicon Dioxide, Spike Glycoprotein, Coronavirus, Immunosensing, Biological system

Abstract

The possibility of immobilizing a protein with antigenic properties on a solid support offers significant possibilities in the development of immunosensors and vaccine formulations. For both applications, the orientation of the antigen should ensure ready accessibility of the antibodies to the epitope. However, an experimental assessment of the orientational preferences necessarily proceeds through the preparation/isolation of the antigen, the immobilization on different surfaces and one or more biophysical characterization steps. To predict a priori whether favorable orientations can be achieved or not would allow one to select the most promising experimental routes, partly mitigating the time cost towards the final product. In this manuscript, we apply a simple computational model, based on united-residue modelling, to the prediction of the orientation of the receptor binding domain of the SARS-CoV-2 spike protein on surfaces commonly used in lateral-flow devices. These calculations can account for the experimental observation that direct immobilization on gold gives sufficient exposure of the epitope to obtain a response in immunochemical assays., Graphical abstract Unlabelled Image, Highlights • Protein immobilization is a crucial in preparing immunosensors. • Immobilization must ensure exposition of the epitope. • A simple computational model can help predicting the exposition.

Published

2020

23. Characterization of PEGylated Asparaginase: New Opportunities from NMR Analysis of Large PEGylated Therapeutics

Author

Enrico Ravera, Giacomo Parigi, Azzurra Carlon, Claudio Luchinat, Stefano Giuntini, Marco Fragai, Linda Cerofolini, and Vito Calderone

Subjects

Magnetic Resonance Spectroscopy, Combinatorial chemistry, Hydrolase, Computational biology, PEGylation, biopharmaceuticals, protein modifications, protein structures, structural biology, 010402 general chemistry, 01 natural sciences, Catalysis, Polyethylene Glycols, Protein structure, Coated Materials, Biocompatible, Asparaginase, 010405 organic chemistry, Chemistry, Organic Chemistry, Rational design, General Chemistry, Integrated approach, 0104 chemical sciences, 3. Good health, Characterization (materials science), Structural biology, Pegylated asparaginase, Protein Multimerization, Peg coating

Abstract

Resonance assignment and structural characterization of pharmacologically relevant proteins promise to improve understanding and safety of these proteins by rational design. However, the PEG coating that is used to evade the immune system also causes these molecules to "evade" the standard structural biology methodologies. We here demonstrate that it is possible to obtain the resonance assignment and a reliable structural model of large PEGylated proteins through an integrated approach encompassing NMR and X-ray crystallography.

Published

2019

24. HOPPI-NMR: Hot-Peptide-Based Screening Assay for Inhibitors of Protein–Protein Interactions by NMR

Author

Stefano Tomassi, Salvatore Di Maro, Claudio Luchinat, Stefano Giuntini, Ettore Novellino, Alfonso Carotenuto, Pasquale Russomanno, Marco Fragai, Linda Cerofolini, Antonio Limatola, Diego Brancaccio, Francesco Merlino, Brancaccio, Diego, Di Maro, Salvatore, Cerofolini, Linda, Giuntini, Stefano, Fragai, Marco, Luchinat, Claudio, Tomassi, Stefano, Limatola, Antonio, Russomanno, Pasquale, Merlino, Francesco, Novellino, Ettore, Carotenuto, Alfonso, Brancaccio, D, Di Maro, S, Cerofolini, L, Giuntini, S, Fragai, M, Luchinat, C, Tomassi, S, Limatola, A, Russomanno, P, Merlino, F, Novellino, E, and Carotenuto, A.

Subjects

chemistry.chemical_classification, 010405 organic chemistry, Chemistry, Organic Chemistry, Cancer, Screening assay, Peptide, macromolecular substances, Computational biology, medicine.disease, 01 natural sciences, Biochemistry, NMR, 0104 chemical sciences, Protein–protein interaction, 010404 medicinal & biomolecular chemistry, Drug Discovery, medicine

Abstract

[Image: see text] Protein–protein interactions (PPIs) contribute to the onset and/or progression of several diseases, especially cancer, and this discovery has paved the way for considering disruption of the PPIs as an attractive anti-tumor strategy. In this regard, simple and efficient biophysical methods for detecting the interaction of the inhibitors with the protein counterpart are still in high demand. Herein, we describe a convenient NMR method for the screening of putative PPI inhibitors based on the use of “hot peptides” (HOPPI-NMR). As a case study, HOPPI-NMR was successful applied to the well-known p53/MDM2 system. Our outcomes highlight the main advantages of the method, including the use of a small amount of unlabeled proteins, the minimization of the risk of protein aggregation, and the ability to identify weak binders. The last leaves open the possibility for application of HOPPI-NMR in tandem with fragment-based drug discovery as a valid strategy for the identification of novel chemotypes acting as PPI inhibitors.

Published

2020

25. Non-crystallographic symmetry in proteins: Jahn–Teller-like and Butterfly-like effects?

Author

Linda Cerofolini, Anjos L. Macedo, Marco Fragai, Enrico Ravera, Claudio Luchinat, José Malanho Silva, Stefano Giuntini, Vito Calderone, and Carlos F. G. C. Geraldes

Subjects

Models, Molecular, Protein Conformation, Jahn–Teller effect, media_common.quotation_subject, Crystallography, X-Ray, 010402 general chemistry, Carbonic Anhydrase II, 01 natural sciences, Biochemistry, Asymmetry, Inorganic Chemistry, Crystal, Nickel, Humans, Molecule, media_common, Crystallographic point group, Binding Sites, biology, 010405 organic chemistry, Chemistry, Active site, Symmetry (physics), 0104 chemical sciences, Crystallography, X-ray crystallography, biology.protein

Abstract

Partial symmetry, i.e., the presence of more than one molecule in the asymmetric unit of a crystal, is a relatively rare phenomenon in small-molecule crystallography, but is quite common in protein crystallography, where it is typically known as non-crystallographic symmetry (NCS). Several papers in literature propose molecular determinants such as crystal contacts, thermal factors, or TLS parameters as an explanation for the phenomenon of intrinsic asymmetry among molecules that are in principle equivalent. Nevertheless, are all of the above determinants the cause or are they rather the effect? In the general frame of the NCS often observed in crystals of biomolecules, this paper deals with nickel(II)-substituted human carbonic anhydrase(II) (hCAII) and its SAD structure determination at the nickel edge. The structure revealed two non-equivalent molecules in the asymmetric unit, the presence of a secondary nickel-binding site at the N-terminus of both molecules (which had never been found before in the nickel-substituted enzyme) and two different coordination geometries of the active site nickel (hexa-coordinated in one molecule and mainly penta-coordinated in the other). The above-mentioned standard molecular crystallographic determinants of this asymmetry are analyzed and presented in detail for this particular case. From these considerations, we speculate on the existence of a fundamental, although yet unknown, common cause for the partial symmetry that is so often encountered in X-ray structures of biomolecules.

Published

2018

26. Characterization of the Conjugation Pattern in Large Polysaccharide–Protein Conjugates by NMR Spectroscopy

Author

Francesco Berti, Linda Cerofolini, Enrico Ravera, Evita Balducci, Stefano Giuntini, Claudio Luchinat, and Marco Fragai

Subjects

0301 basic medicine, Glycoconjugate, drug design, carbohydrate-based vaccines, protein modifications, solid-state NMR spectroscopy, structural biology, Catalysis, Chemistry (all), Conjugated system, 010402 general chemistry, 01 natural sciences, Epitope, 03 medical and health sciences, Antigen, Structural Biology, chemistry.chemical_classification, Bioconjugation, 010405 organic chemistry, Communication, General Chemistry, Nuclear magnetic resonance spectroscopy, General Medicine, Communications, 3. Good health, 0104 chemical sciences, 030104 developmental biology, Structural biology, chemistry, Biochemistry, Conjugate

Abstract

Carbohydrate‐based vaccines are among the safest and most effective vaccines and represent potent tools for prevention of life‐threatening bacterial infectious diseases, like meningitis and pneumonia. The chemical conjugation of a weak antigen to protein as a source of T‐cell epitopes generates a glycoconjugate vaccine that results more immunogenic. Several methods have been used so far to characterize the resulting polysaccharide–protein conjugates. However, a reduced number of methodologies has been proposed for measuring the degree of saccharide conjugation at the possible protein sites. Here we show that detailed information on large proteins conjugated with large polysaccharides can be achieved by a combination of solution and solid‐state NMR spectroscopy. As a test case, a large protein assembly, l‐asparaginase II, has been conjugated with Neisseria meningitidis serogroup C capsular polysaccharide and the pattern and degree of conjugation were determined.

Published

2017

27. High-Resolution Solid-State NMR Characterization of Ligand Binding to a Protein Immobilized in a Silica Matrix

Author

Linda Cerofolini, Alexandra Louka, Enrico Ravera, Stefano Giuntini, Marco Fragai, and Claudio Luchinat

Subjects

Immobilized enzyme, Protein Conformation, High resolution, Ligands, 010402 general chemistry, Carbonic Anhydrase II, 01 natural sciences, Physical and Theoretical Chemistry, Bioinspired materials, medicinal chemistry, drug screening, Materials Chemistry, Humans, Organic chemistry, Nuclear Magnetic Resonance, Biomolecular, chemistry.chemical_classification, 010405 organic chemistry, Drug discovery, Biomolecule, Proteins, A protein, Silicon Dioxide, Combinatorial chemistry, Recombinant Proteins, 3. Good health, 0104 chemical sciences, Surfaces, Coatings and Films, Characterization (materials science), Immobilized Proteins, chemistry, Solid-state nuclear magnetic resonance, Silica matrix, Protein Binding

Abstract

Solid-state NMR is becoming a powerful tool to detect atomic-level structural features of biomolecules even when they are bound to (or trapped in) solid systems that lack long-range three-dimensional order. We here demonstrate that it is possible to probe protein-ligand interactions from a protein-based perspective also when the protein is entrapped in silica, thus translating into biomolecular solid-state NMR all of the considerations that are usually made to understand the chemical nature of the interaction of a protein with its ligands. This work provides a proof of concept that also immobilized enzymes can be used for protein-based NMR protein-ligand interactions for drug discovery.

Published

2017

28. NMR of Immobilized Enzymes

Author

Linda, Cerofolini, Enrico, Ravera, Marco, Fragai, and Claudio, Luchinat

Subjects

Models, Molecular, Immobilized Proteins, Protein Conformation, Enzymes, Immobilized, Nuclear Magnetic Resonance, Biomolecular

Abstract

Solid-state NMR has become the method of choice for the assessment of protein structure for insoluble objects lacking long-range order. In this context, it is apparent that solid-state NMR is also perfectly poised toward the characterization of immobilized proteins. For these systems, it is possible to understand at the atomic level which perturbations, if any, are occurring as a result of the functionalization. Here we describe how it is possible to accomplish the NMR characterization of enzymes that have been immobilized through different approaches, and we introduce the reader to the choice of the experimental strategy that can be useful in different cases. An outlook on the level of information that can be attained is also given, in view of recent methodological advancements.

Published

2020

29. NMR of Immobilized Enzymes

Author

Linda Cerofolini, Enrico Ravera, Claudio Luchinat, and Marco Fragai

Subjects

Immobilized enzyme, 010405 organic chemistry, Chemistry, Context (language use), Nanotechnology, Nuclear magnetic resonance spectroscopy, 010402 general chemistry, 01 natural sciences, Enzyme structure, 0104 chemical sciences, Characterization (materials science), Experimental strategy, Protein structure, Solid-state nuclear magnetic resonance

Abstract

Solid-state NMR has become the method of choice for the assessment of protein structure for insoluble objects lacking long-range order. In this context, it is apparent that solid-state NMR is also perfectly poised toward the characterization of immobilized proteins. For these systems, it is possible to understand at the atomic level which perturbations, if any, are occurring as a result of the functionalization. Here we describe how it is possible to accomplish the NMR characterization of enzymes that have been immobilized through different approaches, and we introduce the reader to the choice of the experimental strategy that can be useful in different cases. An outlook on the level of information that can be attained is also given, in view of recent methodological advancements.

Published

2020

30. How Do Nuclei Couple to the Magnetic Moment of a Paramagnetic Center? A New Theory at the Gauntlet of the Experiments

Author

Giacomo Parigi, Linda Cerofolini, Carlos F. G. C. Geraldes, Jose Silva, Claudio Luchinat, Maurizio Romanelli, Marco Fragai, Enrico Ravera, and Anjos L. Macedo

Subjects

Physics, Magnetic moment, Condensed matter physics, 010405 organic chemistry, 010402 general chemistry, 01 natural sciences, Quantum chemistry, Magnetic susceptibility, 0104 chemical sciences, Paramagnetism, General Materials Science, Center (algebra and category theory), Physical and Theoretical Chemistry, Anisotropy

Abstract

The recent derivation, based on pure quantum chemistry (QC) first-principles, of the pseudocontact shifts (PCSs) caused by a paramagnetic metal center on far away nuclei has cast doubts on the validity of the semiempirical (SE) theory, predicting PCSs to arise from the metal magnetic susceptibility anisotropy. The SE theory has been used and applied countless times, especially in the last 2 decades, to obtain structural information on proteins containing paramagnetic metal ions. We show here that the QC and SE predictions can be directly tested against experiments, provided a suitable macromolecular system is used. The SE approach yields a good prediction of the experimental PCSs while the QC one does not. It appears that the classic theory is able to grasp satisfactorily the underlying physics.

Published

2019

31. Structural characterization of a protein adsorbed on aluminum hydroxide adjuvant in vaccine formulation

Author

Linda Cerofolini, Stefano Giuntini, Marco Fragai, Enrico Ravera, Francesco Berti, and Claudio Luchinat

Subjects

lcsh:Immunologic diseases. Allergy, medicine.medical_treatment, Immunology, Biologics, Vaccines, Chemical interaction, 010402 general chemistry, 01 natural sciences, lcsh:RC254-282, Article, 03 medical and health sciences, chemistry.chemical_compound, Immune system, Antigen, medicine, Pharmacology (medical), 030304 developmental biology, Pharmacology, 0303 health sciences, Chemistry, Alum, A protein, lcsh:Neoplasms. Tumors. Oncology. Including cancer and carcinogens, 3. Good health, 0104 chemical sciences, Infectious Diseases, Biochemistry, Hydroxide, Inorganic matrix, lcsh:RC581-607, Adjuvant

Abstract

The heterogeneous composition of vaccine formulations and the relatively low concentration make the characterization of the protein antigens extremely challenging. Aluminum-containing adjuvants have been used to enhance the immune response of several antigens over the last 90 years and still remain the most commonly used. Here, we show that solid-state NMR and isotope labeling methods can be used to characterize the structural features of the protein antigen component of vaccines and to investigate the preservation of the folding state of proteins adsorbed on Alum hydroxide matrix, providing the way to identify the regions of the protein that are mainly affected by the presence of the inorganic matrix. l-Asparaginase from E. coli has been used as a pilot model of protein antigen. This methodology can find application in several steps of the vaccine development pipeline, from the antigen optimization, through the design of vaccine formulation, up to stability studies and manufacturing process., Quality control: Assessing how adjuvants affect vaccine antigens Aluminum salts are the most frequently used adjuvants in vaccines, but they may negatively affect the antigens in suspension via chemical interactions that could reduce antigen quality and stability. Marco Fragai from the University of Florence and colleagues now report a method based on solid-state nuclear magnetic resonance, to characterize the structure of the model antigen L-asparaginase when adsorbed to the adjuvant aluminum hydroxide in a vaccine suspension. The researchers identify the antigen motifs that interact with the adjuvant directly, and are able to shed light on the antigen’s folding when in complex with the aluminum adjuvant in suspension. This approach could help identify antigen misfolding as a consequence of interactions with chemical adjuvants and may provide useful information during multiple stages of vaccine manufacturing, from antigen optimization to the vaccine manufacturing process, to ultimately improve vaccine quality.

Published

2019

32. Dissecting the Interactions between Human Serum Albumin and α-Synuclein: New Insights on the Factors Influencing α-Synuclein Aggregation in Biological Fluids

Author

Linda Cerofolini, Leonardo Gatticchi, Giovanni Bellomo, Sara Bologna, Lucilla Parnetti, Enrico Ravera, Claudio Luchinat, Silvia Paciotti, and Marco Fragai

Subjects

Models, Molecular, Serum albumin, Serum Albumin, Human, Plasma protein binding, Protein aggregation, Hydrophobic effect, Protein Aggregates, Materials Chemistry, medicine, Humans, Physical and Theoretical Chemistry, biology, Chemistry, Albumin, Human serum albumin, nervous system diseases, Surfaces, Coatings and Films, Body Fluids, body regions, Proteostasis, nervous system, Ionic strength, embryonic structures, biology.protein, Biophysics, alpha-Synuclein, medicine.drug, Protein Binding

Abstract

α-Synuclein (α-syn) is found to be naturally present in biofluids such as cerebrospinal fluid (CSF) and serum. Human serum albumin (HSA) is the most abundant protein found in these biofluids, which, beyond transporting hormones and drugs, also exerts a chaperone-like activity binding other proteins in blood and inhibiting their aggregation. Contrasting results are reported in the literature about the effects of albumin on α-syn aggregation. We characterized the binding region of HSA on α-syn by high-field solution NMR spectroscopy and the effect of HSA on α-syn aggregation by thioflavin-T (ThT) fluorescence under both low-ionic-strength and physiological conditions at the albumin concentration in serum and CSF. We found that HSA, at the concentration found in human serum, slows the aggregation of α-syn significantly. α-Syn interacts with HSA in an ionic strength- and pH-dependent manner. The binding is driven by hydrophobic interactions at the N-terminus under physiological experimental conditions and by electrostatic interactions at the C-terminus at low ionic strength. This work provides novel information about the proteostasis of α-syn in biofluids and supports the hypothesis of a chaperone-like behavior of HSA.

Published

2019

33. Active-Site Targeting Paramagnetic Probe for Matrix Metalloproteinases

Author

Marco Fragai, Barbara Richichi, Cristina Nativi, Claudio Luchinat, Veronica Baldoneschi, Andrea Storai, Elisa Dragoni, and Linda Cerofolini

Subjects

0301 basic medicine, chemistry.chemical_classification, biology, Stereochemistry, Active site, General Chemistry, Matrix metalloproteinase, 010402 general chemistry, 01 natural sciences, 0104 chemical sciences, Sulfonamide, 03 medical and health sciences, chemistry.chemical_compound, 030104 developmental biology, chemistry, Metalloprotein, biology.protein, Organic chemistry, DOTA, Moiety, Molecular probe, neoplasms, Linker

Abstract

The design and synthesis of the Ln3+ complexes of a DOTA-containing (DOTA=1,4,7,10-tetraazacyclododecane-1,4,7,10-tetraacetic acid) inhibitor of matrix metalloproteinases are reported. The tight binding of the sulfonamide scaffold to the catalytic domain of the investigated matrix metalloproteinase is not impaired by the presence of the Ln3+ -DOTA moiety. The paramagnetic properties of the Ln3+ complex are exploited to obtain insights into the structural features of the ligand-protein interactions and to evaluate the influence of the linker length on the quality of the paramagnetic restraints.

Published

2016

34. Cover Feature: Single Peptide Backbone Surrogate Mutations to Regulate Angiotensin GPCR Subtype Selectivity (Chem. Eur. J. 47/2020)

Author

Robert E Widdop, Nick Bekas, Emal Waqif, Baydaa Hirmiz, Evgenios Κ. Stylos, Nathalie M. Grob, Vadim Cherezov, Nelofer Syed, Andreas G. Tzakos, Mark P. Del Borgo, Eirinaios I. Vrettos, Thomas L. Mindt, Marco Fragai, Essam Ghazaly, Alba Mascarin, Hamidreza Shaye, Marie-Isabel Aguilar, Claudio Luchinat, Tim Crook, Linda Cerofolini, Adina T. Michael-Titus, Francesca Magnani, Giacomo Parigi, Patrick N. Pallier, and Ibai E. Valverde

Subjects

Peptide backbone, Chemistry, Stereochemistry, Feature (computer vision), Peptidomimetic, Organic Chemistry, Renin–angiotensin system, Click chemistry, Subtype selectivity, Cover (algebra), General Chemistry, Catalysis, G protein-coupled receptor

Published

2020

35. Cover Feature: The Photocatalyzed Thiol‐ene reaction: A New Tag to Yield Fast, Selective and reversible Paramagnetic Tagging of Proteins (ChemPhysChem 9/2020)

Author

Charlotte A Softley, Linda Cerofolini, Stefano Giuntini, Maxime Denis, Grzegorz M. Popowicz, Michael Sattler, Giacomo Parigi, Enrico Ravera, Marco Fragai, Matteo Gentili, Claudio Luchinat, and Cristina Nativi

Subjects

Paramagnetism, Thiol-ene reaction, Feature (computer vision), Chemistry, Yield (chemistry), Cover (algebra), Physical and Theoretical Chemistry, Photochemistry, Atomic and Molecular Physics, and Optics

Published

2020

36. Metal centers in biomolecular solid-state NMR

Author

Vito Calderone, Anjos L. Macedo, Linda Cerofolini, Giacomo Parigi, Carlos F. G. C. Geraldes, Enrico Ravera, Marco Fragai, Claudio Luchinat, José Malanho Silva, and Stefano Giuntini

Subjects

Models, Molecular, Magnetic Resonance Spectroscopy, Materials science, Protein Conformation, Iron, Nanotechnology, Electronic structure, Metal, Biosolids, Paramagnetic NMR, Resolution, Sensitivity, Structural Biology, 03 medical and health sciences, Paramagnetism, Nickel, Metalloproteins, Organometallic Compounds, Nuclear Magnetic Resonance, Biomolecular, 030304 developmental biology, Electronic properties, chemistry.chemical_classification, 0303 health sciences, Biomolecule, 030302 biochemistry & molecular biology, Characterization (materials science), Solid-state nuclear magnetic resonance, chemistry, Metals, visual_art, visual_art.visual_art_medium, Copper

Abstract

Solid state NMR (SSNMR) has earned a substantial success in the characterization of paramagnetic systems over the last decades. Nowadays, the resolution and sensitivity of solid state NMR in biological molecules has improved significantly and these advancements can be translated into the study of paramagnetic biomolecules. However, the electronic properties of different metal centers affect the quality of their SSNMR spectra differently, and not all systems turn out to be equally easy to approach by this technique. In this review we will try to give an overview of the properties of different paramagnetic centers and how they can be used to increase the chances of experimental success.

Published

2019

37. Integrative Approaches in Structural Biology: A More Complete Picture from the Combination of Individual Techniques

Author

Linda Cerofolini, Ludovic Renault, Christoph A. Diebolder, Enrico Ravera, Vito Calderone, and Marco Fragai

Subjects

Models, Molecular, Molecular model, Cryo-electron microscopy, Integrative structural biology, X-ray crystallography, solution NMR, SSNMR, SAXS, cryo-EM, lcsh:QR1-502, Review, 010402 general chemistry, Crystallography, X-Ray, 01 natural sciences, Biochemistry, lcsh:Microbiology, Polyethylene Glycols, X-Ray Diffraction, 0103 physical sciences, Scattering, Small Angle, Asparaginase, Molecular Biology, Nuclear Magnetic Resonance, Biomolecular, integrative structural biology, Flexibility (engineering), 010304 chemical physics, Small-angle X-ray scattering, Mechanism (biology), Cryoelectron Microscopy, A protein, 0104 chemical sciences, Complement (complexity), Structural biology, Technology Platforms, Biological system

Abstract

With the recent technological and computational advancements, structural biology has begun to tackle more and more difficult questions, including complex biochemical pathways and transient interactions among macromolecules. This has demonstrated that, to approach the complexity of biology, one single technique is largely insufficient and unable to yield thorough answers, whereas integrated approaches have been more and more adopted with successful results. Traditional structural techniques (X-ray crystallography and Nuclear Magnetic Resonance (NMR)) and the emerging ones (cryo-electron microscopy (cryo-EM), Small Angle X-ray Scattering (SAXS)), together with molecular modeling, have pros and cons which very nicely complement one another. In this review, three examples of synergistic approaches chosen from our previous research will be revisited. The first shows how the joint use of both solution and solid-state NMR (SSNMR), X-ray crystallography, and cryo-EM is crucial to elucidate the structure of polyethylene glycol (PEG)ylated asparaginase, which would not be obtainable through any of the techniques taken alone. The second deals with the integrated use of NMR, X-ray crystallography, and SAXS in order to elucidate the catalytic mechanism of an enzyme that is based on the flexibility of the enzyme itself. The third one shows how it is possible to put together experimental data from X-ray crystallography and NMR restraints in order to refine a protein model in order to obtain a structure which simultaneously satisfies both experimental datasets and is therefore closer to the ‘real structure’.

Published

2019

38. Real-Time Insights into Biological Events: In-Cell Processes and Protein-Ligand Interactions

Author

Anna Codina, Enrico Luchinat, Letizia Barbieri, Enrico Ravera, Lucia Banci, Marco Fragai, Matteo Pennestri, Stefano Giuntini, Linda Cerofolini, Cerofolini, Linda, Giuntini, Stefano, Barbieri, Letizia, Pennestri, Matteo, Codina, Anna, Fragai, Marco, Banci, Lucia, Luchinat, Enrico, and Ravera, Enrico

Subjects

Magnetic Resonance Spectroscopy, Nuclear Magnetic Resonance, Biophysics, Ligand, Plasma protein binding, Protein ligand, Carbonic Anhydrase II, Biochemistry, bioreactor, 03 medical and health sciences, 0302 clinical medicine, Bioreactors, Drug Discovery, Humans, Closed tube, Enzyme Inhibitors, Biology, Volume concentration, 030304 developmental biology, 0303 health sciences, Active volume, in-cell NMR, Chemistry, Superoxide Dismutase, HEK 293 cells, in-cell NMR, Nuclear Magnetic Resonance, bioreactor, protein-ligand interactions, flowNMR, Articles, Ligand (biochemistry), protein-ligand interaction, flowNMR, HEK293 Cells, Batch Cell Culture Techniques, Cell, Dialysis (biochemistry), 030217 neurology & neurosurgery, Protein Binding

Abstract

FlowNMR has the aim of continuously monitoring processes that occur in conditions that are not compatible with being carried out within a closed tube. However, it is sample intensive and not suitable for samples, such as proteins or living cells, that are often available in limited volumes and possibly low concentrations. We here propose a dialysis-based modification of a commercial flowNMR setup that allows for recycling the medium while confining the sample (proteins and cells) within the active volume of the tube. This approach is demonstrated in the specific cases of in-cell NMR and protein-based ligand studies.

Published

2018

39. Protein Glycosylation through Sulfur Fluoride Exchange (SuFEx) Chemistry: The Key Role of a Fluorosulfate Thiolactoside

Author

Elisa Crescenzo, Marco Martinucci, Claudio Luchinat, Alessandro Dondoni, Alberto Marra, Linda Cerofolini, Cristina Nativi, Jiajia Dong, Stefano Giuntini, Marco Fragai, and Ma Tiancheng

Subjects

Proteases, Glycosylation, biology, 010405 organic chemistry, Chemistry, Stereochemistry, Organic Chemistry, Lysine, chemistry.chemical_element, General Chemistry, Carbohydrate, 010402 general chemistry, 01 natural sciences, Sulfur, Catalysis, 0104 chemical sciences, Folding (chemistry), chemistry.chemical_compound, Ubiquitin, biology.protein, Reactivity (chemistry)

Abstract

Protein glycosylation is the most complex post-translational modification process. More than 50 % of human cells proteins are glycosylated, whereas bacteria such as E. coli do not have this modification machinery. Indeed, the carbohydrate residues in natural proteins affect their folding, immunogenicity, and stability toward proteases, besides controlling biological properties and activities. It is therefore important to introduce such structural modification in bioengineered proteins lacking the presence of carbohydrate residues. This is not trivial as it requires reagents and conditions compatible with the protein's stability and reactivity. This work reports on the introduction of lactose moieties in two natural proteins, namely ubiquitin (Ub) and l-asparaginase II (ANSII). The synthetic route employed is based on the sulfur(VI) fluoride exchange (SuFEx) coupling of a lactose tethered arylfluorosulfate (Lact-Ar-OSO2 F) with the ϵ-NH2 group of lysine residues of the proteins. This metal-free click SuFEx reaction relies on the properties of the fluorosulfate employed, which is easily prepared in multigram scale from available precursors and reacts chemoselectively with the ϵ-NH2 group of lysine residues under mild conditions. Thus, iterative couplings of Lact-Ar-OSO2 F to Ub and ANSII, afforded multiple glycosylations of these proteins so that up to three and four Lact-Ar-OSO2 groups were introduced in Ub and ANSII, respectively, via the formation of a sulfamoyl (OSO2 -NH) linkage.

Published

2018

40. Engineering l-asparaginase for spontaneous formation of calcium phosphate bioinspired microreactors

Author

Alexandra Louka, Andrea Cavallo, Gil Goobes, Marco Fragai, Enrico Ravera, Ayyalusamy Ramamoorthy, Irina Matlahov, Stefano Giuntini, Linda Cerofolini, Claudio Luchinat, Serena Pillozzi, and Annarosa Arcangeli

Subjects

Materials science, Magnetic Resonance Spectroscopy, Surface Properties, Composite number, General Physics and Astronomy, chemistry.chemical_element, Nanotechnology, Biocompatible Materials, 02 engineering and technology, Calcium, 010402 general chemistry, Protein Engineering, 01 natural sciences, L asparaginase, X-Ray Diffraction, Cell Line, Tumor, Materials Testing, Escherichia coli, Asparaginase, Humans, Amino Acid Sequence, Physical and Theoretical Chemistry, Topology (chemistry), chemistry.chemical_classification, Protein Stability, Biomolecule, Escherichia coli Proteins, 021001 nanoscience & nanotechnology, ddc, 0104 chemical sciences, Durapatite, chemistry, Microscopy, Electron, Scanning, Inorganic matrix, Microreactor, 0210 nano-technology, L-asparaginase, microreactors

Abstract

Active bioinspired materials are appealing biotechnological targets, and their study is gaining momentum. These materials, which comprise of an inorganic matrix and one or more biomolecules, are extremely variable and therefore may result difficult to characterize in their intimate structure. In this work we have prepared a hydroxyapatite–L-asparaginase composite, with the perspective of using it in acute leukemia treatment. We demonstrate that the use of electron microscopy and powder X-ray diffraction, combined with the atomic-resolution information coming from solid-state NMR, allows us to understand the topology of the material and how the different components interplay to obtain an active composite.

Published

2018

41. Solid-State NMR of PEGylated Proteins

Author

Tommaso Martelli, Tatiana Kozyreva, Claudio Luchinat, Silvia Ciambellotti, Marco Fragai, Linda Cerofolini, Stefano Giuntini, Enrico Ravera, Caterina Bernacchioni, and Paola Turano

Subjects

Magnetic Resonance Spectroscopy, 010405 organic chemistry, Chemistry, Proteins, Structural integrity, General Medicine, General Chemistry, Nuclear magnetic resonance spectroscopy, 010402 general chemistry, 01 natural sciences, Combinatorial chemistry, Catalysis, Polyethylene Glycols, 0104 chemical sciences, NMR spectra database, Protein structure, Solid-state nuclear magnetic resonance, Posttranslational modification

Abstract

PEGylated proteins are widely used in biomedicine but, in spite of their importance, no atomic-level information is available since they are generally resistant to structural characterization approaches. PEGylated proteins are shown here to yield highly resolved solid-state NMR spectra, which allows assessment of the structural integrity of proteins when PEGylated for therapeutic or diagnostic use.

Published

2016

42. Probing the interaction of distamycin A with S100β: the 'unexpected' ability of S100β to bind to DNA-binding ligands

Author

Linda Cerofolini, Marco Fragai, Valentina Borsi, Bruno Pagano, Antonio Randazzo, and Jussara Amato

Subjects

chemistry.chemical_classification, Stereochemistry, Lexitropsin, Nuclear magnetic resonance spectroscopy, In vitro, DNA sequencing, chemistry.chemical_compound, chemistry, Biochemistry, Structural Biology, Docking (molecular), Non-covalent interactions, DISTAMYCIN A, Molecular Biology, DNA

Abstract

DNA-minor-groove-binding ligands are potent antineoplastic molecules. The antibiotic distamycin A is the prototype of one class of these DNA-interfering molecules that have been largely used in vitro. The affinity of distamycin A for DNA is well known, and the structural details of the complexes with some B-DNA and G-quadruplex-forming DNA sequences have been already elucidated. Here, we show that distamycin A binds S100β, a protein involved in the regulation of several cellular processes. The reported affinity of distamycin A for the calcium(II)-loaded S100β reinforces the idea that some biological activities of the DNA-minor-groove-binding ligands arise from the binding to cellular proteins. Copyright © 2015 John Wiley & Sons, Ltd.

Published

2015

43. Interfering with HuR-RNA Interaction: Design, Synthesis and Biological Characterization of Tanshinone Mimics as Novel, Effective HuR Inhibitors

Author

Luciana Marinelli, Preet Lal, Emiliano Biasini, Chiara Zucal, Alessandro Provenzani, Vito Giuseppe D'Agostino, Pierfausto Seneci, Vanessa Baj, Natthakan Thongon, Saioa R. Elezgarai, Danilo Di Maio, Linda Cerofolini, Claudio Luchinat, Leonardo Manzoni, Ettore Novellino, Marta Brambilla, Marco Fragai, Marco Miceli, Isabelle Bonomo, Manzoni, Leonardo, Zucal, Chiara, Maio, Danilo Di, D'Agostino, Vito G, Thongon, Natthakan, Bonomo, Isabelle, Lal, Preet, Miceli, Marco, Baj, Vanessa, Brambilla, Marta, Cerofolini, Linda, Elezgarai, Saioa, Biasini, Emiliano, Luchinat, Claudio, Novellino, Ettore, Fragai, Marco, Marinelli, Luciana, Provenzani, Alessandro, and Seneci, Pierfausto

Subjects

0301 basic medicine, ELAV-Like Protein 1, RNA-binding protein, Plasma protein binding, Molecular Dynamics Simulation, medicine.disease_cause, Cell Line, 03 medical and health sciences, Structure-Activity Relationship, 0302 clinical medicine, human antigen R , HuR, dihydrotanshinone-I , DHTS, 1, Drug Discovery, medicine, HuR inhibitors, Structure–activity relationship, Humans, RNA, Messenger, Hur-mRNA, Drug Discovery, Chemistry Medicinal, RNA, Protein, Magnetic Resonance Spectroscopy, Chemistry, Molecular Mimicry, mimetics, Quinones, RNA, RNA-Binding Proteins, Cell biology, Molecular mimicry, 030104 developmental biology, Cell culture, 030220 oncology & carcinogenesis, Drug Design, Abietanes, Tanshinone, Molecular Medicine, Function (biology), Protein Binding

Abstract

The human antigen R (HuR) is an RNA-binding protein known to modulate the expression of target mRNA coding for proteins involved in inflammation, tumorigenesis, and stress responses and is a valuable drug target. We previously found that dihydrotanshinone-I (DHTS, 1) prevents the association of HuR with its RNA substrate, thus imparing its function. Herein, inspired by DHTS structure, we designed and synthesized an array of ortho-quinones (tanshinone mimics) using a function-oriented synthetic approach. Among others, compound 6a and 6n turned out to be more effective than 1, showing a nanomolar Ki and disrupting HuR binding to RNA in cells. A combined approach of NMR titration and molecular dynamics (MD) simulations suggests that 6a stabilizes HuR in a peculiar closed conformation, which is incompatible with RNA binding. Alpha screen and RNA-electrophoretic mobility shift assays (REMSA) data on newly synthesized compounds allowed, for the first time, the generation of structure activity relationships (SARs), thus providing a solid background for the generation of highly effective HuR disruptors.

Published

2018

44. Simultaneous Targeting of RGD-Integrins and Dual Murine Double Minute Proteins in Glioblastoma Multiforme

Author

Ettore Novellino, Diego Brancaccio, Sabrina Taliani, Rebecca Piccarducci, Stefano Tomassi, Stefano Giuntini, Salvatore Di Maro, Francesco Saverio Di Leva, Claudia Martini, Chiara Cavallini, Luciana Marinelli, Horst Kessler, Barbara Costa, Linda Cerofolini, Marco Fragai, Simona Daniele, Francesco Merlino, Valeria La Pietra, Florian Reichart, Federico Da Settimo, Claudio Luchinat, Merlino, Francesco, Daniele, Simona, La Pietra, Valeria, Di Maro, Salvatore, Di Leva, Francesco Saverio, Brancaccio, Diego, Tomassi, Stefano, Giuntini, Stefano, Cerofolini, Linda, Fragai, Marco, Luchinat, Claudio, Reichart, Florian, Cavallini, Chiara, Costa, Barbara, Piccarducci, Rebecca, Taliani, Sabrina, Da Settimo, Federico, Martini, Claudia, Kessler, Horst, Novellino, Ettore, and Marinelli, Luciana

Subjects

0301 basic medicine, Models, Molecular, Protein Conformation, Cell, Integrin, 03 medical and health sciences, Mice, 0302 clinical medicine, Proto-Oncogene Proteins c-mdm2, Glioma, Cell Line, Tumor, Drug Discovery, medicine, Animals, Molecular Targeted Therapy, neoplasms, biology, Chemistry, Drug Discovery3003 Pharmaceutical Science, Cell cycle, medicine.disease, Integrin alphaVbeta3, 030104 developmental biology, medicine.anatomical_structure, Molecular Medicine, Apoptosis, Cell culture, 030220 oncology & carcinogenesis, Cancer research, biology.protein, Mdm2, Peptidomimetics, Glioblastoma, Oligopeptides, Integrin alpha5beta1

Abstract

In the fight against Glioblastoma Multiforme, recent literature data have highlighted that integrin alpha 5 beta 1 and p53 are part of convergent pathways in the control of glioma apoptosis. This observation prompted us to seek a molecule able to simultaneously modulate both target families. Analyzing the results of a previous virtual screening against murine double minute 2 protein (MDM2), we envisaged that Arg-Gly-Asp (RGD)-mimetic molecules could be inhibitors of MDM2/4. Herein, we present the discovery of compound 7, which inhibits both MDM2/4 and alpha 5 beta 1/alpha v beta 3 integrins. A lead optimization campaign was carried out on 7 with the aim to preserve the activities on integrins while improving those on MDM proteins. Compound 9 turned out to be a potent MDM2/4 and alpha 5 beta 1/alpha v beta 3 blocker. In p53 -wild type glioma cells, 9 arrested cell cycle and proliferation and strongly reduced cell invasiveness, emerging as the first molecule of a novel class of integrin/MDM inhibitors, which might be especially useful in subpopulations of patients with glioblastoma expressing a functional p53 concomitantly with a high level of alpha 5 beta 1 integrin.

Published

2018

45. Atomic structural details of a protein grafted onto gold nanoparticles

Author

Claudio Luchinat, Stefano Giuntini, Marco Fragai, Linda Cerofolini, and Enrico Ravera

Subjects

Materials science, Magnetic Resonance Spectroscopy, Multidisciplinary, lcsh:R, Nanoparticle, A protein, Metal Nanoparticles, lcsh:Medicine, Nanotechnology, 02 engineering and technology, Conjugated system, 010402 general chemistry, 021001 nanoscience & nanotechnology, 01 natural sciences, Article, 0104 chemical sciences, Polyethylene Glycols, Heteronuclear molecule, Colloidal gold, Molecule, Asparaginase, lcsh:Q, Gold, 0210 nano-technology, lcsh:Science

Abstract

The development of a methodology for the structural characterization at atomic detail of proteins conjugated to nanoparticles would be a breakthrough in nanotechnology. Solution and solid-state NMR spectroscopies are currently used to investigate molecules and peptides grafted onto nanoparticles, but the strategies used so far fall short in the application to proteins, which represent a thrilling development in theranostics. We here demonstrate the feasibility of highly-resolved multidimensional heteronuclear spectra of a large protein assembly conjugated to PEGylated gold nanoparticles. The spectra have been obtained by direct proton detection under fast MAS and allow for both a fast fingerprinting for the assessment of the preservation of the native fold and for resonance assignment. We thus demonstrate that the structural characterization and the application of the structure-based methodologies to proteins bound to gold nanoparticles is feasible and potentially extensible to other hybrid protein-nanomaterials.

Published

2017

46. HTS by NMR for the Identification of Potent and Selective Inhibitors of Metalloenzymes

Author

Linda Cerofolini, Claudio Luchinat, Maurizio Pellecchia, Carlo Baggio, and Marco Fragai

Subjects

0301 basic medicine, Peptide, 01 natural sciences, Biochemistry, FBLD, Medicinal and Biomolecular Chemistry, 03 medical and health sciences, chemistry.chemical_compound, Drug Discovery, Moiety, chemistry.chemical_classification, Hydroxamic acid, MMP, 010405 organic chemistry, Chemistry, Drug discovery, focused positional scanning libraries, Organic Chemistry, Pharmacology and Pharmaceutical Sciences, Nuclear magnetic resonance spectroscopy, Combinatorial chemistry, 0104 chemical sciences, 030104 developmental biology, Metal Chelating Agents, FBDD, HTS by NMR, Identification (biology)

Abstract

We have recently proposed a novel drug discovery approach based on biophysical screening of focused positional scanning libraries in which each element of the library contained a common binding moiety for the given target or class of targets. In this Letter, we report on the implementation of this approach to target metal containing proteins. In our implementation, we first derived a focused positional scanning combinatorial library of peptide mimetics (of approximately 100,000 compounds) in which each element of the library contained the metal-chelating moiety hydroxamic acid at the C-terminal. Screening of this library by nuclear magnetic resonance spectroscopy in solution allowed the identification of a novel and selective compound series targeting MMP-12. The data supported that our general approach, perhaps applied using other metal chelating agents or other initial binding fragments, may result very effective in deriving novel and selective agents against metalloenzyme.

Published

2017

47. G-triplex structure and formation propensity

Author

Jussara Amato, Antonio Randazzo, Linda Cerofolini, Claudio Luchinat, Marco Fragai, Michele Parrinello, Vittorio Limongelli, Andrea Giachetti, Ettore Novellino, Cerofolini, Linda, Amato, Jussara, Giachetti, Andrea, Limongelli, Vittorio, Novellino, Ettore, Parrinello, Michele, Fragai, Marco, Randazzo, Antonio, and Luchinat, Claudio

Subjects

Models, Molecular, Circular dichroism, Guanine, Biology, 010402 general chemistry, G-quadruplex, 01 natural sciences, 03 medical and health sciences, Differential scanning calorimetry, Structural Biology, G-Quadruplexe, Genetics, medicine, 030304 developmental biology, 0303 health sciences, Oligonucleotide, Hydrogen bond, Metadynamics, Triad (anatomy), DNA, Aptamers, Nucleotide, Cations, Monovalent, 0104 chemical sciences, G-Quadruplexes, Folding (chemistry), Crystallography, medicine.anatomical_structure, Biochemistry, Nucleic Acid Conformation

Abstract

The occurrence of a G-triplex folding intermediate of thrombin binding aptamer (TBA) has been recently predicted by metadynamics calculations, and experimentally supported by Nuclear Magnetic Resonance (NMR), Circular Dichroism (CD) and Differential Scanning Calorimetry (DSC) data collected on a 3′ end TBA-truncated 11-mer oligonucleotide (11-mer-3′-t-TBA). Here we present the solution structure of 11-mer-3′-t-TBA in the presence of potassium ions. This structure is the first experimental example of a G-triplex folding, where a network of Hoogsteen-like hydrogen bonds stabilizes six guanines to form two G:G:G triad planes. The G-triplex folding of 11-mer-3′-t-TBA is stabilized by the potassium ion and destabilized by increasing the temperature. The superimposition of the experimental structure with that predicted by metadynamics shows a great similarity, with only significant differences involving two loops. These new structural data show that 11-mer-3′-t-TBA assumes a G-triplex DNA conformation as its stable form, reinforcing the idea that G-triplex folding intermediates may occur in vivo in human guanine-rich sequences. NMR and CD screening of eight different constructs obtained by removing from one to four bases at either the 3′ and the 5′ ends show that only the 11-mer-3′-t-TBA yields a relatively stable G-triplex., Nucleic Acids Research, 42 (21), ISSN:1362-4962, ISSN:0301-5610

Published

2014

48. Examination of Matrix Metalloproteinase-1 in Solution

Author

Marco Fragai, Giacomo Parigi, Linda Cerofolini, João M.C. Teixeira, Enrico Ravera, Carlos F. G. C. Geraldes, Dmitri I. Svergun, Claudio Luchinat, and Gregg B. Fields

Subjects

0303 health sciences, Collagen degradation, Chemistry, Small-angle X-ray scattering, Cell Biology, Nuclear magnetic resonance spectroscopy, Matrix metalloproteinase, Matrix (biology), 010402 general chemistry, 01 natural sciences, Biochemistry, 0104 chemical sciences, Solvent, 03 medical and health sciences, Paramagnetism, Crystallography, Structural biology, Molecular Biology, 030304 developmental biology

Abstract

Catalysis of collagen degradation by matrix metalloproteinase 1 (MMP-1) has been proposed to critically rely on flexibility between the catalytic (CAT) and hemopexin-like (HPX) domains. A rigorous assessment of the most readily accessed conformations in solution is required to explain the onset of substrate recognition and collagenolysis. The present study utilized paramagnetic NMR spectroscopy and small angle x-ray scattering (SAXS) to calculate the maximum occurrence (MO) of MMP-1 conformations. The MMP-1 conformations with large MO values (up to 47%) are restricted into a relatively small conformational region. All conformations with high MO values differ largely from the closed MMP-1 structures obtained by x-ray crystallography. The MO of the latter is ∼20%, which represents the upper limit for the presence of this conformation in the ensemble sampled by the protein in solution. In all the high MO conformations, the CAT and HPX domains are not in tight contact, and the residues of the HPX domain reported to be responsible for the binding to the collagen triple-helix are solvent exposed. Thus, overall analysis of the highest MO conformations indicated that MMP-1 in solution was poised to interact with collagen and then could readily proceed along the steps of collagenolysis. Background: Matrix metalloproteinase-1 (MMP-1) collagenolysis relies on interdomain flexibility. Results: In all high maximum occurrence conformations, the MMP-1 hemopexin-like domain residues reported responsible for binding to the collagen triple-helix are solvent exposed. Conclusion: MMP-1 in solution is poised to interact with collagen and proceed along the steps of collagenolysis. Significance: The maximum occurrence approach can evaluate the predominant domain conformations for numerous multidomain enzymes.

Published

2013

49. Multivalent presentation of a hydrolytically stable GM3 lactone mimetic as modulator of melanoma cells motility and adhesion

Author

Alessandro Dondoni, Cristina Nativi, Lisa Moni, Alberto Marra, Paola Chiarugi, Linda Cerofolini, Barbara Richichi, Lucio Toma, Giuseppina Comito, Gabriele Gabrielli, Alice Pace, Lucia Pasquato, Richichi, B., Comito, G., Cerofolini, L., Gabrielli, G., Marra, A., Moni, L., Pace, A., Pasquato, Lucia, Chiarugi, P., Dondoni, A., Toma, L., and Nativi, C.

Subjects

Clinical Biochemistry, Pharmaceutical Science, Motility, Apoptosis, GM(3) ganglioside, Tumour antigen, Biochemistry, Biomimetic Materials, Cell Movement, Glycomimetic, Drug Discovery, Cell Adhesion, medicine, G(M3) Ganglioside, Humans, Mimetic, Melanoma, Adhesion, Anoikis, Cell adhesion, Molecular Biology, chemistry.chemical_classification, GM3 ganglioside, Chemistry, Organic Chemistry, medicine.disease, Cell biology, Molecular Medicine, Lactone

Abstract

A hydrolytically stable mimetic of the tumour antigen GM3 lactone is used to decorate multivalent scaffolds. Two of them positively interfere on melanoma cell adhesion, migration and resistance to apoptosis (anoikis). Notably, their ability to hamper melanoma-cells adhesion and reduce the metastatic potential is enhanced when the two scaffolds, presenting a different shape, are used in combination. © 2013 Elsevier Ltd.All rights reserved.

Published

2013

50. Computer-Aided Identification and Lead Optimization of Dual Murine Double Minute 2 and 4 Binders: Structure-Activity Relationship Studies and Pharmacological Activity

Author

Giuseppe La Regina, Claudio Luchinat, Sandro Cosconati, Linda Cerofolini, Diego Brancaccio, Mariateresa Giustiniano, Federico Da Settimo, Stefano Giuntini, Luciana Marinelli, Ettore Novellino, Anna Messere, Sveva Pelliccia, Simona Daniele, Claudia Martini, Deborah Pietrobono, Marco Fragai, Valeria La Pietra, Sabrina Taliani, Romano Silvestri, Giustiniano, Mariateresa, Daniele, Simona, Pelliccia, Sveva, La Pietra, Valeria, Pietrobono, Deborah, Brancaccio, Diego, Cosconati, Sandro, Messere, Anna, Giuntini, Stefano, Cerofolini, Linda, Fragai, Marco, Luchinat, Claudio, Taliani, Sabrina, La Regina, Giuseppe, Da Settimo, Federico, Silvestri, Romano, Martini, Claudia, Novellino, Ettore, and Marinelli, Luciana

Subjects

0301 basic medicine, High-Throughput Screening Assay, Models, Molecular, Magnetic Resonance Spectroscopy, Antineoplastic Agents, Apoptosis, neuroblastoma cells, Antineoplastic Agent, 03 medical and health sciences, Structure-Activity Relationship, 0302 clinical medicine, Proto-Oncogene Proteins, Cell Line, Tumor, Drug Discovery, Structure–activity relationship, Humans, Receptor, p53 protein, Cell Proliferation, Virtual screening, MDM2/MDM4 binders, Proto-Oncogene Protein, biology, Cell growth, Chemistry, Drug Discovery3003 Pharmaceutical Science, Apoptosi, Biological activity, Proto-Oncogene Proteins c-mdm2, Genes, p53, High-Throughput Screening Assays, 030104 developmental biology, Biochemistry, Docking (molecular), Cell culture, 030220 oncology & carcinogenesis, Drug Design, biology.protein, Neoplastic Stem Cells, Mdm2, Computer-Aided Design, Molecular Medicine, Neoplastic Stem Cell, Human

Abstract

The function of p53 protein, also known as "genome guardian", might be impaired by the overexpression of its primary cellular inhibitor, the murine double minute 2 protein (MDM2). However, the recent finding that MDM2-selective inhibitors induce high levels of its homologue MDM4, prompt us to identify, through a receptor-based virtual screening on an in house database, dual MDM2/MDM4 binders. Compound 1 turned out to possess an IC50 of 93.7 and of 4.6 nM on MDM2 and MDM4, respectively. A series of compounds were synthesized to optimize its activity on MDM2. As a result, compound 12 showed low nanomolar IC50 for both targets. NMR studies confirmed the pocket of binding of 12 as predicted by the Glide docking software. Notably, 12 was able to cause concentration-dependent inhibition of cell proliferation, yielding an IC50 value of 356 ± 21 nM in neuroblastoma SHSY5Y cells and proved even to efficiently block cancer stem cell growth. The function of p53 protein, also known as "genome guardian", might be impaired by the overexpression of its primary cellular inhibitor, the murine double minute 2 protein (MDM2). However, the recent finding that MDM2-selective inhibitors induce high levels of its homologue MDM4, prompt us to identify, through a receptor-based virtual screening on an in house database, dual MDM2/MDM4 binders. Compound 1 turned out to possess an IC50 of 93.7 and of 4.6 nM on MDM2 and MDM4, respectively. A series of compounds were synthesized to optimize its activity on MDM2. As a result, compound 12 showed low nanomolar IC50 for both targets. NMR studies confirmed the pocket of binding of 12 as predicted by the Glide docking software. Notably, 12 was able to cause concentration-dependent inhibition of cell proliferation, yielding an IC50 value of 356 ± 21 nM in neuroblastoma SHSY5Y cells and proved even to efficiently block cancer stem cell growth.

Published

2017