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1. Selection and characterization of human scFvs targeting the SARS-CoV-2 nucleocapsid protein isolated from antibody libraries of COVID-19 patients

Author

Simonetta Lisi, Francesca Malerba, Paola Quaranta, Rita Florio, Ottavia Vitaloni, Elisa Monaca, Bruno Bruni Ercole, Angela Rachel Bitonti, Olga del Perugia, Marianna Mignanelli, Paola Perrera, Raffaele Sabbatella, Francesco Raimondi, Carmen Rita Piazza, Anna Moles, Caterina Alfano, Mauro Pistello, and Antonino Cattaneo

Subjects
Medicine, Science
Abstract

Abstract In 2019, the novel SARS-CoV-2 coronavirus emerged in China, causing the pneumonia named COVID-19. At the beginning, all research efforts were focused on the spike (S) glycoprotein. However, it became evident that the nucleocapsid (N) protein is pivotal in viral replication, genome packaging and evasion of the immune system, is highly immunogenic, which makes it another compelling target for antibody development alongside the spike protein. This study focused on the construction of single chain fragments variable (scFvs) libraries from SARS-CoV-2-infected patients to establish a valuable, immortalized and extensive antibodies source. We used the Intracellular Antibody Capture Technology to select a panel of scFvs against the SARS-CoV-2 N protein. The whole panel of scFv was expressed and characterized both as intrabodies and recombinant proteins. ScFvs were then divided into 2 subgroups: those that exhibited high binding activity to N protein when expressed in yeast or in mammalian cells as intrabodies, and those purified as recombinant proteins, displaying affinity for recombinant N protein in the nanomolar range. This panel of scFvs against the N protein represents a novel platform for research and potential diagnostic applications.

Published
2024
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3. In-silico guided chemical exploration of KDM4A fragments hits

Author

Jessica Lombino, Rosario Vallone, Maura Cimino, Maria Rita Gulotta, Giada De Simone, Maria Agnese Morando, Raffaele Sabbatella, Simona Di Martino, Mario Fogazza, Federica Sarno, Claudia Coronnello, Maria De Rosa, Chiara Cipollina, Lucia Altucci, Ugo Perricone, and Caterina Alfano

Subjects
Epigenetic regulation, Lysine demethylases, KDM4 inhibitors, Fragment-based drug discovery (FBDD), KDM4A, Rational drug design, Medicine, Genetics, QH426-470
Abstract

Abstract Background Lysine demethylase enzymes (KDMs) are an emerging class of therapeutic targets, that catalyse the removal of methyl marks from histone lysine residues regulating chromatin structure and gene expression. KDM4A isoform plays an important role in the epigenetic dysregulation in various cancers and is linked to aggressive disease and poor clinical outcomes. Despite several efforts, the KDM4 family lacks successful specific molecular inhibitors. Results Herein, starting from a structure-based fragments virtual screening campaign we developed a synergic framework as a guide to rationally design efficient KDM4A inhibitors. Commercial libraries were used to create a fragments collection and perform a virtual screening campaign combining docking and pharmacophore approaches. The most promising compounds were tested in-vitro by a Homogeneous Time-Resolved Fluorescence-based assay developed for identifying selective substrate-competitive inhibitors by means of inhibition of H3K9me3 peptide demethylation. 2-(methylcarbamoyl)isonicotinic acid was identified as a preliminary active fragment, displaying inhibition of KDM4A enzymatic activity. Its chemical exploration was deeply investigated by computational and experimental approaches which allowed a rational fragment growing process. The in-silico studies guided the development of derivatives designed as expansion of the primary fragment hit and provided further knowledge on the structure–activity relationship. Conclusions Our study describes useful insights into key ligand-KDM4A protein interaction and provides structural features for the development of successful selective KDM4A inhibitors.

Published
2023
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4. Author Correction: Selection and characterization of human scFvs targeting the SARS-CoV-2 nucleocapsid protein isolated from antibody libraries of COVID-19 patients

Author

Simonetta Lisi, Francesca Malerba, Paola Quaranta, Rita Florio, Ottavia Vitaloni, Elisa Monaca, Bruno Bruni Ercole, Angela Rachel Bitonti, Olga del Perugia, Marianna Mignanelli, Paola Perrera, Rafaele Sabbatella, Francesco Raimondi, Carmen Rita Piazza, Anna Moles, Caterina Alfano, Mauro Pistello, and Antonino Cattaneo

Subjects
Medicine, Science
Published
2024
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5. Solution structure of recombinant Pvfp-5β reveals insights into mussel adhesion

Author

Maria Agnese Morando, Francesca Venturella, Martina Sollazzo, Elisa Monaca, Raffaele Sabbatella, Valeria Vetri, Rosa Passantino, Annalisa Pastore, and Caterina Alfano

Subjects
Biology (General), QH301-705.5
Abstract

Solution structure of byssal plaque protein Pvfp-5β secreted by the Asian green mussel Perna viridis gives molecular insight into mussel adhesion on wet surfaces.

Published
2022
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6. Computational design and characterization of a multiepitope vaccine against carbapenemase-producing Klebsiella pneumoniae strains, derived from antigens identified through reverse vaccinology

Author

Nicola Cuscino, Ayesha Fatima, Vincenzo Di Pilato, Matteo Bulati, Caterina Alfano, Elisa Monaca, Giuseppina Di Mento, Daniele Di Carlo, Francesca Cardinale, Francesco Monaco, Gian Maria Rossolini, Asif M. Khan, Pier Giulio Conaldi, and Bruno Douradinha

Subjects
Klebsiella pneumoniae, Reverse vaccinology, Antimicrobial resistance, Carbapenems, Subunit vaccine, Bioinformatics, Biotechnology, TP248.13-248.65
Abstract

Klebsiella pneumoniae is a Gram-negative pathogen of clinical relevance, which can provoke serious urinary and blood infections and pneumonia. This bacterium is a major public health threat due to its resistance to several antibiotic classes. Using a reverse vaccinology approach, 7 potential antigens were identified, of which 4 were present in most of the sequences of Italian carbapenem-resistant K. pneumoniae clinical isolates. Bioinformatics tools demonstrated the antigenic potential of these bacterial proteins and allowed for the identification of T and B cell epitopes. This led to a rational design and in silico characterization of a multiepitope vaccine against carbapenem-resistant K. pneumoniae strains. As adjuvant, the mycobacterial heparin-binding hemagglutinin adhesin (HBHA), which is a Toll-like receptor 4 (TLR-4) agonist, was included, to increase the immunogenicity of the construct. The multiepitope vaccine candidate was analyzed by bioinformatics tools to assess its antigenicity, solubility, allergenicity, toxicity, physical and chemical parameters, and secondary and tertiary structures. Molecular docking binding energies to TLR-2 and TLR-4, two important innate immunity receptors involved in the immune response against K. pneumoniae infections, and molecular dynamics simulations of such complexes supported active interactions. A codon optimized multiepitope sequence cloning strategy is proposed, for production of recombinant vaccine in classical bacterial vectors. Finally, a 3 dose-immunization simulation with the multiepitope construct induced both cellular and humoral immune responses. These results suggest that this multiepitope construct has potential as a vaccination strategy against carbapenem-resistant K. pneumoniae and deserves further validation.

Published
2022
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7. Molecular network analysis of hormonal contraceptives side effects via database integration

Author

Manuela Petti, Caterina Alfano, and Lorenzo Farina

Subjects
Hormonal contraceptives, Multipartite graph, Network medicine, Side effect module, Precision medicine, Computer applications to medicine. Medical informatics, R858-859.7
Abstract

Hormonal contraceptives (HCs) have been shown to be safe and effective when used correctly and consistently, however, as other classes of drugs, they are also associated with adverse health outcomes. In this study, we aim to explain the occurrence of common and unexpected HCs side effects (SEs) integrating drug-target, drug-SE and protein-protein interaction (PPI) public databases. We created a tripartite network that includes three types of vertices: SEs, drugs, and targets. The three layers are linked by means of the inter-layer associations drug-target and drug-SE, whereas only the target layer is characterized also by intra-layer links (PPIs). We exploited the drug-mediated association SE-target to identify the side effect modules defined as a network connected component composed of target proteins plus the proteins needed to connect them. We found that module proteins are associated with diseases/phenotypes and/or KEGG pathways related to the SEs. In particular, in many cases, targets are not enriched in SE features, whereas investigating their neighborhood (here defined as the proteins that allow the targets' connection) we found SE-related pathways. These results show that HCs action can perturb the targets’ neighborhood inducing unwanted reaction and that the proposed approach can help to understand how, and through which molecular mechanisms, side effects can occur. The approach is general in its nature: it can be applied to other drugs categories providing a support in identifying a subject-specific therapy that takes into account comorbidities and lifestyle to reduce or avoid the most undesired side effects.

Published
2023
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10. Large-Scale Recombinant Production of the SARS-CoV-2 Proteome for High-Throughput and Structural Biology Applications

Author

Nadide Altincekic, Sophie Marianne Korn, Nusrat Shahin Qureshi, Marie Dujardin, Martí Ninot-Pedrosa, Rupert Abele, Marie Jose Abi Saad, Caterina Alfano, Fabio C. L. Almeida, Islam Alshamleh, Gisele Cardoso de Amorim, Thomas K. Anderson, Cristiane D. Anobom, Chelsea Anorma, Jasleen Kaur Bains, Adriaan Bax, Martin Blackledge, Julius Blechar, Anja Böckmann, Louis Brigandat, Anna Bula, Matthias Bütikofer, Aldo R. Camacho-Zarco, Teresa Carlomagno, Icaro Putinhon Caruso, Betül Ceylan, Apirat Chaikuad, Feixia Chu, Laura Cole, Marquise G. Crosby, Vanessa de Jesus, Karthikeyan Dhamotharan, Isabella C. Felli, Jan Ferner, Yanick Fleischmann, Marie-Laure Fogeron, Nikolaos K. Fourkiotis, Christin Fuks, Boris Fürtig, Angelo Gallo, Santosh L. Gande, Juan Atilio Gerez, Dhiman Ghosh, Francisco Gomes-Neto, Oksana Gorbatyuk, Serafima Guseva, Carolin Hacker, Sabine Häfner, Bing Hao, Bruno Hargittay, K. Henzler-Wildman, Jeffrey C. Hoch, Katharina F. Hohmann, Marie T. Hutchison, Kristaps Jaudzems, Katarina Jović, Janina Kaderli, Gints Kalniņš, Iveta Kaņepe, Robert N. Kirchdoerfer, John Kirkpatrick, Stefan Knapp, Robin Krishnathas, Felicitas Kutz, Susanne zur Lage, Roderick Lambertz, Andras Lang, Douglas Laurents, Lauriane Lecoq, Verena Linhard, Frank Löhr, Anas Malki, Luiza Mamigonian Bessa, Rachel W. Martin, Tobias Matzel, Damien Maurin, Seth W. McNutt, Nathane Cunha Mebus-Antunes, Beat H. Meier, Nathalie Meiser, Miguel Mompeán, Elisa Monaca, Roland Montserret, Laura Mariño Perez, Celine Moser, Claudia Muhle-Goll, Thais Cristtina Neves-Martins, Xiamonin Ni, Brenna Norton-Baker, Roberta Pierattelli, Letizia Pontoriero, Yulia Pustovalova, Oliver Ohlenschläger, Julien Orts, Andrea T. Da Poian, Dennis J. Pyper, Christian Richter, Roland Riek, Chad M. Rienstra, Angus Robertson, Anderson S. Pinheiro, Raffaele Sabbatella, Nicola Salvi, Krishna Saxena, Linda Schulte, Marco Schiavina, Harald Schwalbe, Mara Silber, Marcius da Silva Almeida, Marc A. Sprague-Piercy, Georgios A. Spyroulias, Sridhar Sreeramulu, Jan-Niklas Tants, Kaspars Tārs, Felix Torres, Sabrina Töws, Miguel Á. Treviño, Sven Trucks, Aikaterini C. Tsika, Krisztina Varga, Ying Wang, Marco E. Weber, Julia E. Weigand, Christoph Wiedemann, Julia Wirmer-Bartoschek, Maria Alexandra Wirtz Martin, Johannes Zehnder, Martin Hengesbach, and Andreas Schlundt

Subjects
COVID-19, SARS-CoV-2, nonstructural proteins, structural proteins, accessory proteins, intrinsically disordered region, Biology (General), QH301-705.5
Abstract

The highly infectious disease COVID-19 caused by the Betacoronavirus SARS-CoV-2 poses a severe threat to humanity and demands the redirection of scientific efforts and criteria to organized research projects. The international COVID19-NMR consortium seeks to provide such new approaches by gathering scientific expertise worldwide. In particular, making available viral proteins and RNAs will pave the way to understanding the SARS-CoV-2 molecular components in detail. The research in COVID19-NMR and the resources provided through the consortium are fully disclosed to accelerate access and exploitation. NMR investigations of the viral molecular components are designated to provide the essential basis for further work, including macromolecular interaction studies and high-throughput drug screening. Here, we present the extensive catalog of a holistic SARS-CoV-2 protein preparation approach based on the consortium’s collective efforts. We provide protocols for the large-scale production of more than 80% of all SARS-CoV-2 proteins or essential parts of them. Several of the proteins were produced in more than one laboratory, demonstrating the high interoperability between NMR groups worldwide. For the majority of proteins, we can produce isotope-labeled samples of HSQC-grade. Together with several NMR chemical shift assignments made publicly available on covid19-nmr.com, we here provide highly valuable resources for the production of SARS-CoV-2 proteins in isotope-labeled form.

Published
2021
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11. Thrombopoietin mutation in congenital amegakaryocytic thrombocytopenia treatable with romiplostim

Author

Alessandro Pecci, Iman Ragab, Valeria Bozzi, Daniela De Rocco, Serena Barozzi, Tania Giangregorio, Heba Ali, Federica Melazzini, Mohamed Sallam, Caterina Alfano, Annalisa Pastore, Carlo L Balduini, and Anna Savoia

Subjects
congenital amegakaryocytic thrombocytopenia, MPL, mutation, romiplostim, thrombopoietin, Medicine (General), R5-920, Genetics, QH426-470
Abstract

Abstract Congenital amegakaryocytic thrombocytopenia (CAMT) is an inherited disorder characterized at birth by thrombocytopenia with reduced megakaryocytes, which evolves into generalized bone marrow aplasia during childhood. Although CAMT is genetically heterogeneous, mutations of MPL, the gene encoding for the receptor of thrombopoietin (THPO), are the only known disease‐causing alterations. We identified a family with three children affected with CAMT caused by a homozygous mutation (p.R119C) of the THPO gene. Functional studies showed that p.R119C affects not only ability of the cytokine to stimulate MPL but also its release, which is consistent with the relatively low serum THPO levels measured in patients. In all the three affected children, treatment with the THPO‐mimetic romiplostim induced trilineage hematological responses, remission of bleeding and infections, and transfusion independence, which were maintained after up to 6.5 years of observation. Recognizing patients with THPO mutations among those with juvenile bone marrow failure is essential to provide them with appropriate substitutive therapy and prevent the use of invasive and unnecessary treatments, such as hematopoietic stem cell transplantation or immunosuppression.

Published
2017
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12. An optimized strategy to measure protein stability highlights differences between cold and hot unfolded states

Author

Caterina Alfano, Domenico Sanfelice, Stephen R. Martin, Annalisa Pastore, and Piero Andrea Temussi

Subjects
Science
Abstract

Crowding effects—important when considering cellular environments—greatly influence protein stability. Here the authors study the impact of macromolecular crowders on high and low temperature protein unfolding, and show that volume exclusion effects are larger when the protein and crowder volumes are similar.

Published
2017
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13. Clinical and pathogenic features of ETV6-related thrombocytopenia with predisposition to acute lymphoblastic leukemia

Author

Federica Melazzini, Flavia Palombo, Alessandra Balduini, Daniela De Rocco, Caterina Marconi, Patrizia Noris, Chiara Gnan, Tommaso Pippucci, Valeria Bozzi, Michela Faleschini, Serena Barozzi, Michael Doubek, Christian A. Di Buduo, Katerina Stano Kozubik, Lenka Radova, Giuseppe Loffredo, Sarka Pospisilova, Caterina Alfano, Marco Seri, Carlo L. Balduini, Alessandro Pecci, and Anna Savoia

Subjects
Diseases of the blood and blood-forming organs, RC633-647.5
Abstract

ETV6-related thrombocytopenia is an autosomal dominant thrombocytopenia that has been recently identified in a few families and has been suspected to predispose to hematologic malignancies. To gain further information on this disorder, we searched for ETV6 mutations in the 130 families with inherited thrombocytopenia of unknown origin from our cohort of 274 consecutive pedigrees with familial thrombocytopenia. We identified 20 patients with ETV6-related thrombocytopenia from seven pedigrees. They have five different ETV6 variants, including three novel mutations affecting the highly conserved E26 transformation-specific domain. The relative frequency of ETV6-related thrombocytopenia was 2.6% in the whole case series and 4.6% among the families with known forms of inherited thrombocytopenia. The degree of thrombocytopenia and bleeding tendency of the patients with ETV6-related thrombocytopenia were mild, but four subjects developed B-cell acute lymphoblastic leukemia during childhood, resulting in a significantly higher incidence of this condition compared to that in the general population. Clinical and laboratory findings did not identify any particular defects that could lead to the suspicion of this disorder from the routine diagnostic workup. However, at variance with most inherited thrombocytopenias, platelets were not enlarged. In vitro studies revealed that the maturation of the patients’ megakaryocytes was defective and that the patients have impaired proplatelet formation. Moreover, platelets from patients with ETV6-related thrombocytopenia have reduced ability to spread on fibrinogen. Since the dominant thrombocytopenias due to mutations in RUNX1 and ANKRD26 are also characterized by normal platelet size and predispose to hematologic malignancies, we suggest that screening for ETV6, RUNX1 and ANKRD26 mutations should be performed in all subjects with autosomal dominant thrombocytopenia and normal platelet size.

Published
2016
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14. Solution structure of the SGTA dimerisation domain and investigation of its interactions with the ubiquitin-like domains of BAG6 and UBL4A.

Author

John F Darby, Ewelina M Krysztofinska, Peter J Simpson, Aline C Simon, Pawel Leznicki, Newran Sriskandarajah, David S Bishop, Lisa R Hale, Caterina Alfano, Maria R Conte, Santiago Martínez-Lumbreras, Arjun Thapaliya, Stephen High, and Rivka L Isaacson

Subjects
Medicine, Science
Abstract

The BAG6 complex resides in the cytosol and acts as a sorting point to target diverse hydrophobic protein substrates along their appropriate paths, including proteasomal degradation and ER membrane insertion. Composed of a trimeric complex of BAG6, TRC35 and UBL4A, the BAG6 complex is closely associated with SGTA, a co-chaperone from which it can obtain hydrophobic substrates.SGTA consists of an N-terminal dimerisation domain (SGTA_NT), a central tetratricopeptide repeat (TPR) domain, and a glutamine rich region towards the C-terminus. Here we solve a solution structure of the SGTA dimerisation domain and use biophysical techniques to investigate its interaction with two different UBL domains from the BAG6 complex. The SGTA_NT structure is a dimer with a tight hydrophobic interface connecting two sets of four alpha helices. Using a combination of NMR chemical shift perturbation, isothermal titration calorimetry (ITC) and microscale thermophoresis (MST) experiments we have biochemically characterised the interactions of SGTA with components of the BAG6 complex, the ubiquitin-like domain (UBL) containing proteins UBL4A and BAG6. We demonstrate that the UBL domains from UBL4A and BAG6 directly compete for binding to SGTA at the same site. Using a combination of structural and interaction data we have implemented the HADDOCK protein-protein interaction docking tool to generate models of the SGTA-UBL complexes.This atomic level information contributes to our understanding of the way in which hydrophobic proteins have their fate decided by the collaboration between SGTA and the BAG6 complex.

Published
2014
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17. Oxidation effects in antiaggregogenic properties of Epigallocatechingallate

Author

Daniele Gulli, Giuseppe Sancataldo, Caterina Alfano, Bruno Pignataro, Valeria Vetri, and Daniele Gulli, Giuseppe Sancataldo, Caterina Alfano, Bruno Pignataro, Valeria Vetri

Subjects
Protein aggregation, electrostatics, EGCG-Protein interaction, EGCG Oxidation
Abstract

Epigallocatechin-gallate (EGCG), the most abundant flavonoid in green tea, has been extensively studied for its potential in the treatment of amyloid related disorders. This molecule was found to modulate abnormal protein self-assembly, reducing resulting cellular toxicity. EGCG is known to suppress or to slow down the aggregation processes of several proteins, thus supporting the idea that general mechanisms regulate its anti-aggregogenic effects and, interestingly, in the oxidised form it demonstrated an higher efficiency in reducing protein aggregation with respect to intact molecule. We here investigate the effects of intact and oxidized EGCG the thermal aggregation pathway of Bovine Serum Albumin (BSA), a well-known model protein whose aggregation processes are known in details. By means of different spectroscopic methods, we evaluate similarities and differences of the two molecules during protein aggregation. Different solution conditions are investigated, close and away from the isoelectric point of the protein, with the aim of eliciting the role of electrostatics in the observed EGCG-Protein interaction and in the supramolecular assembly which are dramatically dependent on solution conditions.

Published
2021

18. Quantifying the thermodynamics of protein unfolding using 2D NMR spectroscopy

Author

Piero Andrea Temussi, Stephen F. Martin, Rita Puglisi, Oliver Brylski, Caterina Alfano, and Annalisa Pastore

Subjects
0301 basic medicine, Materials science, Protein core, Amide proton, General Chemistry, Nuclear magnetic resonance spectroscopy, 010402 general chemistry, 01 natural sciences, Biochemistry, Measure (mathematics), Stability (probability), Article, 0104 chemical sciences, lcsh:Chemistry, 03 medical and health sciences, 030104 developmental biology, lcsh:QD1-999, Materials Chemistry, Environmental Chemistry, Spectroscopy, Biological system, Two-dimensional nuclear magnetic resonance spectroscopy
Abstract

A topic that has attracted considerable interest in recent years is the possibility to perform thermodynamic studies of proteins directly in-cell or in complex environments which mimic the cellular interior. Nuclear magnetic resonance (NMR) could be an attractive technique for these studies but its applicability has so far been limited by technical issues. Here, we demonstrate that 2D NMR methods can be successfully applied to measure thermodynamic parameters provided that a suitable choice of the residues used for the calculation is made. We propose a new parameter, named RAD, which reflects the level of protection of a specific amide proton in the protein core and can guide through the selection of the resonances. We also suggest a way to calibrate the volumes to become independent of technical limitations. The methodology we propose leads to stability curves comparable to that calculated from CD data and provides a new tool for thermodynamic measurements in complex environments. Multidimensional NMR spectroscopy can provide insight into the unfolding of proteins in cells, but may be sensitive to the choice of residue used as a reference. Here 2D 1H-15N NMR is used to obtain thermodynamic parameters of unfolding of Yfh1, relying on an internal standard to normalise peak volumes.

Published
2020

20. Networks as Biomarkers: Uses and Purposes

Author

Manuela Petti, Lorenzo Farina, and Caterina Alfano

Subjects
Genetics, Genetics (clinical)
Abstract

Networks-based approaches are often used to analyze gene expression data or protein–protein interactions but are not usually applied to study the relationships between different biomarkers. Given the clinical need for more comprehensive and integrative biomarkers that can help to identify personalized therapies, the integration of biomarkers of different natures is an emerging trend in the literature. Network analysis can be used to analyze the relationships between different features of a disease; nodes can be disease-related phenotypes, gene expression, mutational events, protein quantification, imaging-derived features and more. Since different biomarkers can exert causal effects between them, describing such interrelationships can be used to better understand the underlying mechanisms of complex diseases. Networks as biomarkers are not yet commonly used, despite being proven to lead to interesting results. Here, we discuss in which ways they have been used to provide novel insights into disease susceptibility, disease development and severity.

Published
2023

22. Recombinant mussel protein Pvfp-5β: A potential tissue bioadhesive

Author

Alessandro Sicorello, Fabrizio Dal Piaz, Annalisa Pastore, Francesca Venturella, Caterina Alfano, Daniela Giacomazza, Estella Rao, Radha Santonocito, Maria Agnese Morando, Pier Luigi San Biagio, Maria Assunta Costa, Rosa Passantino, Alessia Provenzano, and Donatella Bulone

Subjects
0301 basic medicine, medicine.disease_cause, Biochemistry, epidermal growth factor (EGF), law.invention, Mice, Cell Movement, law, biophysics, structural biology, recombinant, Cells, Cultured, biology, Chemistry, Marine proteins, Adhesion, Recombinant Proteins, adhesion, Protein Structure and Folding, Recombinant DNA, adhesion proteins, biomaterials, Perna, Cell Survival, Surface Properties, Bioadhesive, mussel, 03 medical and health sciences, medicine, Animals, Humans, Molecular Biology, Escherichia coli, Cell Proliferation, Tissue Engineering, 030102 biochemistry & molecular biology, Proteins, Cell Biology, Mussel, biology.organism_classification, EGF-like motifs, 030104 developmental biology, Structural biology, Cell culture, NIH 3T3 Cells, Biophysics, Tissue Adhesives, HeLa Cells, Perna viridis
Abstract

During their lifecycle, many marine organisms rely on natural adhesives to attach to wet surfaces for movement and self-defence in aqueous tidal environments. Adhesive proteins from mussels are biocompatible and elicit only minimal immune responses in humans. Therefore these proteins have received increased attention for their potential applications in medicine, biomaterials and biotechnology. The Asian green mussel Perna viridis secretes several byssal plaque proteins, molecules that help anchor the mussel to surfaces. Among these proteins, protein-5β (Pvfp-5β) initiates interactions with the substrate, displacing interfacial water molecules before binding to the surface. Here, we established the first recombinant expression in Escherichia coli of Pvfp-5β. We characterized recombinant Pvfp-5β, finding that despite displaying a CD spectrum consistent with features of a random coil, the protein is correctly folded as indicated by MS and NMR analyses. Pvfp-5β folds as a β-sheet–rich protein as expected for an epidermal growth factor (EGF)-like module. We examined the effects of Pvfp-5β on cell viability and adhesion capacity in NIH-3T3 and HeLa cell lines, revealing that Pvfp-5β has no cytotoxic effects at the protein concentrations used and provides good cell-adhesion strength on both glass and plastic plates. Our findings suggest that the adhesive properties of recombinant Pvfp-5β make it an efficient surface coating material, potentially suitable for biomedical applications including regeneration of damaged tissues.

Published
2019

23. RNA as a key factor in driving or preventing self-assembly of the TAR DNA-binding protein 43

Author

Gian Gaetano Tartaglia, Caterina Alfano, Natalia Sanchez de Groot, Stephen R. Martin, Elsa Zacco, Annalisa Pastore, Ricardo Graña-Montes, Zacco, Elsa, Graña-Montes, Ricardo, Martin, Stephen R, de Groot, Natalia Sanchez, Alfano, Caterina, Tartaglia, Gian Gaetano, and Pastore, Annalisa

Subjects
Models, Molecular, RNA-binding, amyotrophic lateral sclerosis, frontotemporal dementia, neurodegeneration, protein aggregation, Amyloid, Demència frontotemporal, TAR DNA-Binding Protein 43, Protein aggregation, Protein Aggregation, Pathological, Article, 03 medical and health sciences, 0302 clinical medicine, Structural Biology, mental disorders, medicine, Agregació de proteïnes, Humans, amyotrophic lateral sclerosi, Molecular Biology, 030304 developmental biology, Chemical Biology & High Throughput, 0303 health sciences, Chemistry, Neurodegeneration, nutritional and metabolic diseases, RNA, Translation (biology), Frontotemporal lobar degeneration, medicine.disease, nervous system diseases, Cell biology, DNA-Binding Proteins, RNA splicing, Sistema nerviós -- Degeneració, Esclerosi lateral amiotròfica, 030217 neurology & neurosurgery, Protein Binding, Structural Biology & Biophysics, Frontotemporal dementia
Abstract

Amyotrophic lateral sclerosis and frontotemporal lobar degeneration are incurable motor neuron diseases associated with muscle weakness, paralysis and respiratory failure. Accumulation of TAR DNA-binding protein 43 (TDP-43) as toxic cytoplasmic inclusions is one of the hallmarks of these pathologies. TDP-43 is an RNA-binding protein responsible for regulating RNA transcription, splicing, transport and translation. Aggregated TDP-43 does not retain its physiological function. Here, we exploit the ability of TDP-43 to bind specific RNA sequences to validate our hypothesis that the native partners of a protein can be used to interfere with its ability to self-assemble into aggregates. We propose that binding of TDP-43 to specific RNA can compete with protein aggregation. This study provides a solid proof of concept to the hypothesis that natural interactions can be exploited to increase protein solubility and could be adopted as a more general rational therapeutic strategy. This work was supported by a Newton International Fellowship (Royal Society) and the European Research Council (ERC, Ribomylome)

Published
2019

24. Investigation on a MMACHC mutant from cblC disease: The c.394C>T variant

Author

Rosa Passantino, Maria Rosalia Mangione, Maria Grazia Ortore, Maria Assunta Costa, Alessia Provenzano, Heinz Amenitsch, Raffaele Sabbatella, Caterina Alfano, Vincenzo Martorana, Silvia Vilasi, Passantino, Rosa, Mangione, Maria Rosalia, Ortore, Maria Grazia, Costa, Maria Assunta, Provenzano, Alessia, Amenitsch, Heinz, Sabbatella, Raffaele, Alfano, Caterina, Martorana, Vincenzo, and Vilasi, Silvia

Subjects
Vitamin B12 (cobalamin), Structure-function relationship, Biophysics, Biochemistry, Analytical Chemistry, Vitamin B 12, Mutation, MMACHC protein, Humans, Methylmalonic aciduria and homocystinuria cblC type, Homocystinuria, Carrier Proteins, Child, Oxidoreductases, Amino Acid Metabolism, Inborn Errors, Molecular Biology
Abstract

The cblC disease is an inborn disorder of the vitamin B12 (cobalamin, Cbl) metabolism characterized by methylmalonic aciduria and homocystinuria. The clinical consequences of this disease are devastating and, even when early treated with current therapies, the affected children manifest symptoms involving vision, growth, and learning. The illness is caused by mutations in the gene codifying for MMACHC, a 282aa protein that transports and transforms the different Cbl forms. Here we present data on the structural properties of the truncated protein p.R132X resulting from the c.394C > T mutation that, along with c.271dupA and c.331C > T, is among the most common mutations in cblC. Although missing part of the Cbl binding domain, p.R132X is associated to late-onset symptoms and, therefore, it is supposed to retain residual function. However, to our knowledge structuralfunctional studies on c.394C > T mutant aimed at verifying this hypothesis are still lacking. By using a biophysical approach including Circular Dichroism, fluorescence, Small Angle X-ray Scattering, and Molecular Dynamics, we show that the mutant protein MMACHC-R132X retains secondary structure elements and remains compact in solution, partly preserving its binding affinity for Cbl. Insights on the fragile stability of MMACHCR132X-Cbl are provided.

Published
2022

25. Backbone chemical shift spectral assignments of SARS coronavirus-2 non-structural protein nsp9

Author

Andreas Schlundt, Erika F. Dudás, Harald Schwalbe, Caterina Alfano, Elisa Monaca, Annalisa Pastore, Rita Puglisi, Maria Laura Bellone, Geoff Kelly, Fabrizio Dal Piaz, and Sophie Marianne Korn

Subjects
Models, Molecular, Stereochemistry, viruses, Crystal structure, Viral Nonstructural Proteins, 010402 general chemistry, medicine.disease_cause, 01 natural sciences, Biochemistry, Protein Structure, Secondary, Article, Virus, Imaging, Analytical Ultracentrifugation, 03 medical and health sciences, Dynamic light scattering, Structural Biology, medicine, Nuclear Magnetic Resonance, Biomolecular, 030304 developmental biology, Coronavirus, Solution NMR, 0303 health sciences, SARS-CoV-2, Chemistry, Protein, RNA-Binding Proteins, Covid-19 NMR, Structure, RNA, Hydrogen-Ion Concentration, Small molecule, 3. Good health, 0104 chemical sciences, Viral replication, Structural Biology & Biophysics
Abstract

As part of an International consortium aiming at the characterization by NMR of the proteins of the SARS-CoV-2 virus, we have obtained the virtually complete assignment of the backbone atoms of the non-structural protein nsp9. This small (12 kDa) protein is encoded by ORF1a, binds to RNA and seems to be essential for viral RNA synthesis. The crystal structures of the SARS-CoV-2 protein and other homologues suggest that the protein is dimeric as also confirmed by analytical ultracentrifugation and dynamic light scattering. Our data constitute the prerequisite for further NMR-based characterization, and provide the starting point for the identification of small molecule lead compounds that could interfere with RNA binding and prevent viral replication.

Published
2021
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26. The Wide World of Coacervates: From the Sea to Neurodegeneration

Author

Emanuele Astoricchio, Annalisa Pastore, Piero Andrea Temussi, Lawrence Rajendran, and Caterina Alfano

Subjects
marine organisms, 0303 health sciences, Coacervate, Origin of Life, Polychaeta, cellular compartmentalization, Biochemistry, Bivalvia, Cell Compartmentation, Solutions, 03 medical and health sciences, 0302 clinical medicine, Chemical physics, confinement, Phase (matter), liquid–liquid phase transition, Animals, Colloids, membraneless particles, Molecular Biology, 030217 neurology & neurosurgery, 030304 developmental biology
Abstract

The formation of immiscible liquid phases or coacervates is a phenomenon widely observed in biology. Marine organisms, for instance, use liquid–liquid phase separation (LLPS) as the precursor phase to form various fibrillar or crustaceous materials that are essential for surface adhesion. More recently, the importance of LLPS has been realized in the compartmentalization of living cells and in obtaining ordered but dynamic partitions that can be reversed according to necessity. Here, we compare the properties, features, and peculiarities of intracellular and extracellular coacervates, drawing parallels and learning from the differences. A more general view of the phenomenon may in the future inform new studies to allow a better comprehension of its laws.

Published
2020

27. A novel RNA polymerase‐binding protein that interacts with a sigma‐factor docking site

Author

Ann Hochschild, Caterina Alfano, Ewelina M. Krysztofinska, Rivka L. Isaacson, Cinthia P. Garcia, Anna F. Wang Erickson, Padraig Deighan, Kelsey Barrasso, Santiago Martínez-Lumbreras, Richard Losick, Arjun Thapaliya, Amy H. Camp, and Shanshan Chen

Subjects
0301 basic medicine, Transcription, Genetic, Anti-sigma factors, Sigma Factor, RNA polymerase II, Microbiology, Article, 03 medical and health sciences, chemistry.chemical_compound, Bacterial Proteins, Sigma factor, RNA polymerase, Journal Article, RNA polymerase I, Molecular Biology, RNA polymerase II holoenzyme, Spores, Bacterial, biology, General transcription factor, RNA-Binding Proteins, DNA-Directed RNA Polymerases, Gene Expression Regulation, Bacterial, Molecular biology, Protein Structure, Tertiary, Cell biology, 030104 developmental biology, chemistry, biology.protein, Transcription factor II D, Bacillus subtilis, Protein Binding, Transcription Factors
Abstract

Sporulation in Bacillus subtilis is governed by a cascade of alternative RNA polymerase sigma factors. We previously identified a small protein Fin that is produced under the control of the sporulation sigma factor σ(F) to create a negative feedback loop that inhibits σ(F) -directed gene transcription. Cells deleted for fin are defective for spore formation and exhibit increased levels of σ(F) -directed gene transcription. Based on pull-down experiments, chemical crosslinking, bacterial two-hybrid experiments, and nuclear magnetic resonance chemical shift analysis, we now report that Fin binds to RNA polymerase and specifically to the coiled-coil region of the β' subunit. The coiled-coil is a docking site for sigma factors on RNA polymerase, and evidence is presented that the binding of Fin and σ(F) to RNA polymerase is mutually exclusive. We propose that Fin functions by a mechanism distinct from that of classic sigma factor antagonists (anti-σ factors), which bind directly to a target sigma factor to prevent its association with RNA polymerase, and instead functions to inhibit σ(F) by competing for binding to the β' coiled-coil. This article is protected by copyright. All rights reserved.

Published
2017

28. The missing links to link ubiquitin: Methods for the enzymatic production of polyubiquitin chains

Author

Caterina Alfano, Serena Faggiano, Annalisa Pastore, Faggiano, Serena, Alfano, Caterina, and Pastore, Annalisa

Subjects
0301 basic medicine, Biophysics, Computational biology, Ubiquitin-conjugating enzyme, Biochemistry, 03 medical and health sciences, Ubiquitinating enzyme, Ubiquitin, Production (economics), Polyubiquitin, Link (knot theory), Ligation, Molecular Biology, Ubiquitinating enzymes, Flexibility (engineering), biology, Chemistry, Ubiquitination, Cell Biology, Protein purification, 030104 developmental biology, Post-translational modification, Enzymatic ubiquitination, Biophysic, Structural biology, Ubiquitin-Conjugating Enzymes, Mutagenesis, Site-Directed, biology.protein, Posttranslational modification
Abstract

Attachment of ubiquitin (Ub) as monoUb and polyUb chains of different lengths and linkages to proteins plays a dominant role in very different regulatory mechanisms. Therefore, the study of polyUb chains has assumed a central interest in biochemistry and structural biology. An essential step necessary to allow in vitro biochemical and structural studies of polyUbs is the production of their chains in high quantities and purity. This is not always an easy task and can be achieved both enzymatically and chemically. Previous reviews have covered chemical cross-linking exhaustively. In this review, we concentrate on the different approaches developed so far for the enzymatic production of different Ub chains. These strategies permit a certain flexibility in the production of chains with various linkages and lengths. We critically describe the available methods and comment on advantages and limitations. It is clear that the field is mature to study most of the possible links, but some more work needs to be done to complete the picture and to exploit the current methodologies for understanding in full the Ub code.

Published
2016

29. Gray platelet syndrome: Novel mutations of the NBEAL2 gene

Author

Debora Bertaggia-Calderara, Elena Nicchia, Lorenzo Alberio, Caterina Alfano, Annalisa Pastore, Ana C. Glembotsky, Paula G. Heller, Anna Savoia, Guillermo Arbesú, Roberta Bottega, Michel A. Duchosal, and Bettina Bisig

Subjects
Genetics, Mutation, Hematology, 030204 cardiovascular system & hematology, Biology, Platelet membrane glycoprotein, medicine.disease_cause, medicine.disease, Gray platelet syndrome, 03 medical and health sciences, 0302 clinical medicine, Genotype, Gene expression, Cancer research, medicine, Platelet, Allele, Gene, 030215 immunology
Published
2017

30. Thrombopoietin mutation in congenital amegakaryocytic thrombocytopenia treatable with romiplostim

Author

Serena Barozzi, Annalisa Pastore, Mohamed Sallam, Heba Ibrahim Ali, Iman A. Ragab, Daniela De Rocco, Federica Melazzini, Caterina Alfano, Anna Savoia, Tania Giangregorio, Carlo L. Balduini, Valeria Bozzi, Alessandro Pecci, Pecci, Alessandro, Ragab, Iman, Bozzi, Valeria, De Rocco, Daniela, Barozzi, Serena, Giangregorio, Tania, Ali, Heba, Melazzini, Federica, Sallam, Mohamed, Alfano, Caterina, Pastore, Annalisa, Balduini, Carlo L, and Savoia, Anna

Subjects
0301 basic medicine, Medicine (General), MPL, medicine.medical_treatment, Bone Marrow Aplasia, Hematopoietic stem cell transplantation, QH426-470, 03 medical and health sciences, 0302 clinical medicine, R5-920, Genetics, Medicine, thrombopoietin, Thrombopoietin, Romiplostim, business.industry, Genetic heterogeneity, Bone marrow failure, Immunosuppression, romiplostim, medicine.disease, congenital amegakaryocytic thrombocytopenia, 030104 developmental biology, Immunology, Congenital amegakaryocytic thrombocytopenia, Molecular Medicine, mutation, business, 030215 immunology, medicine.drug
Abstract

Congenital amegakaryocytic thrombocytopenia (CAMT) is an inherited disorder characterized at birth by thrombocytopenia with reduced megakaryocytes, which evolves into generalized bone marrow aplasia during childhood. Although CAMT is genetically heterogeneous, mutations of MPL , the gene encoding for the receptor of thrombopoietin (THPO), are the only known disease‐causing alterations. We identified a family with three children affected with CAMT caused by a homozygous mutation (p.R119C) of the THPO gene. Functional studies showed that p.R119C affects not only ability of the cytokine to stimulate MPL but also its release, which is consistent with the relatively low serum THPO levels measured in patients. In all the three affected children, treatment with the THPO‐mimetic romiplostim induced trilineage hematological responses, remission of bleeding and infections, and transfusion independence, which were maintained after up to 6.5 years of observation. Recognizing patients with THPO mutations among those with juvenile bone marrow failure is essential to provide them with appropriate substitutive therapy and prevent the use of invasive and unnecessary treatments, such as hematopoietic stem cell transplantation or immunosuppression.

Published
2018

31. Expression and Purification of ZASP Subdomains and Clinically Important Isoforms: High-Affinity Binding to G-Actin

Author

Yotam Blech-Hermoni, Annalisa Pastore, Norman R. Watts, Ira Palmer, Altaira D. Dearborn, Xiaolei Zhuang, Ami Mankodi, Joshua D. Kaufman, Paul T. Wingfield, Stephen Coscia, Caterina Alfano, Watts Norman, R, Zhuang, Xiaolei, Kaufman Joshua, D, Palmer Ira, W, Dearborn Altaira, D, Coscia, Stephen, Blech-Hermoni, Yotam, Alfano, Caterina, Pastore, Annalisa, Mankodi, Ami, and Wingfield Paul, T

Subjects
0301 basic medicine, Gene isoform, Sarcomeres, Protein domain, PDZ domain, Gene Expression, Plasma protein binding, Biology, Biochemistry, Article, 03 medical and health sciences, Structure-Activity Relationship, 0302 clinical medicine, Protein Domains, Escherichia coli, Humans, Protein Isoforms, Binding site, Actin, LIM domain, Adaptor Proteins, Signal Transducing, Binding Sites, Alternative splicing, Osmolar Concentration, Exons, LIM Domain Proteins, Actins, Introns, Recombinant Proteins, Cell biology, Alternative Splicing, 030104 developmental biology, Mutation, 030217 neurology & neurosurgery, Protein Binding
Abstract

Z-disc-associated, alternatively spliced, PDZ motif-containing protein (ZASP) is a principal component of the sarcomere. The three prevalent isoforms of ZASP in skeletal muscle are generated by alternative splicing of exons 9 and 10. The long isoforms, either having (ZASP-L) or lacking exon 10 (ZASP-LΔex10), include an N-terminal PDZ domain, an actin-binding region (ABR) with a conserved motif (ZM), and three C-terminal LIM domains. The short isoform (ZASP-S) lacks the LIM domains. Mutations, A147T and A165V, within the ZM of ZASP-LΔex10 cause myofibrillar myopathy, but the mechanism is unknown. We have prepared these proteins, their ABR, and the respective mutant variants in recombinant form, characterized them biophysically, and analyzed their actin-binding properties by surface plasmon resonance and electron microscopy. All the proteins were physically homogeneous and monomeric and had circular dichroic spectra consistent with partially folded conformations. Comparison of the NMR HSQC spectra of ZASP-S and the PDZ domain showed that the ABR is unstructured. ZASP-S and its mutant variants and ZASP-LΔex10 all bound to immobilized G-actin with high affinity (K(d) ≈ 10(−8) to 10(−9) M). Constructs of the isolated actin-binding region missing exon 10 (ABRΔ10) bound with lower affinity (K(d) ≈ 10(−7) M), but those retaining exon 10 (ABR+10) did so only weakly (K(d) ≈ 10(−5) M). ZASP-S, and the ABRΔ10, also induced F-actin and array formation, even in conditions of low ionic strength and in the absence of KCl and Mg(2+) ions. Interestingly, the ZM mutations A147T and A165V did not affect any of the results described above.

Published
2017

32. The Ball and Chain of Polyubiquitin Structures

Author

Caterina Alfano, Serena Faggiano, Annalisa Pastore, Alfano, Caterina, Faggiano, Serena, and Pastore, Annalisa

Subjects
Protein Conformation, alpha-Helical, 0301 basic medicine, Proteasome Endopeptidase Complex, NEDD8 Protein, Amino Acid Motifs, Plasma protein binding, macromolecular substances, 010402 general chemistry, 01 natural sciences, Biochemistry, proteasomal pathway, 03 medical and health sciences, Ubiquitin, Small Ubiquitin-Related Modifier Proteins, biophysics, Endopeptidases, ubiquitin, post-translational modifications, Animals, Humans, Moiety, Protein Interaction Domains and Motifs, structure, Binding site, signalling, Polyubiquitin, Ubiquitins, Molecular Biology, Binding Sites, biology, Lysine, C-terminus, Ubiquitination, 0104 chemical sciences, Cell biology, 030104 developmental biology, Biophysic, Covalent bond, biology.protein, Protein Conformation, beta-Strand, Post-translational modification, Hydrophobic and Hydrophilic Interactions, Protein Processing, Post-Translational, Protein Binding, Signal Transduction
Abstract

Ubiquitylation is a post-translational modification implicated in several different cellular pathways. The possibility of forming chains through covalent crosslinking between any of the seven lysines, or the initial methionine, and the C terminus of another moiety provides ubiquitin (Ub) with special flexibility in its function in signalling. Here, we review the knowledge accumulated over the past several years about the functions and structural features of polyUb chains. This analysis reveals the need to understand further the functional role of some of the linkages and the structural code that determines recognition of polyUbs by protein partners.

Published
2016

33. Clinical and pathogenic features of ETV6-related thrombocytopenia with predisposition to acute lymphoblastic leukemia

Author

Serena Barozzi, Giuseppe Loffredo, Carlo L. Balduini, Chiara Gnan, Alessandra Balduini, Caterina Marconi, Michael Doubek, Lenka Radová, Christian A. Di Buduo, Federica Melazzini, Caterina Alfano, Anna Savoia, Daniela De Rocco, Valeria Bozzi, Tommaso Pippucci, Flavia Palombo, Marco Seri, Michela Faleschini, Katerina Stano Kozubik, Patrizia Noris, Šárka Pospíšilová, Alessandro Pecci, Melazzini, Federica, Palombo, Flavia, Balduini, Alessandra, DE ROCCO, Daniela, Marconi, Caterina, Noris, Patrizia, Gnan, Chiara, Pippucci, Tommaso, Bozzi, Valeria, Faleschini, Michela, Barozzi, Serena, Doubek, Michael, Di Buduo, Christian A., Kozubik, Katerina Stano, Radova, Lenka, Loffredo, Giuseppe, Pospisilova, Sarka, Alfano, Caterina, Seri, Marco, Balduini, Carlo L., Pecci, Alessandro, Savoia, Anna, De Rocco, Daniela, Di Buduo, Christian A, Stano Kozubik, Katerina, and Balduini, Carlo L

Subjects
0301 basic medicine, Fibrinogen, 0302 clinical medicine, hemic and lymphatic diseases, Medicine, Platelet, platelet disorders, inherited thrombocytopenia, Child, inherited thrombocytopenias, education.field_of_study, Hematology, Incidence (epidemiology), Nuclear Proteins, Middle Aged, Precursor Cell Lymphoblastic Leukemia-Lymphoma, Pedigree, 3. Good health, Cell Transformation, Neoplastic, Child, Preschool, Core Binding Factor Alpha 2 Subunit, Cohort, Intercellular Signaling Peptides and Proteins, medicine.drug, Adult, Platelets, medicine.medical_specialty, Adolescent, Platelet disorder, Population, Article, Young Adult, 03 medical and health sciences, Internal medicine, Humans, Family, Genetic Predisposition to Disease, education, Proto-Oncogene Proteins c-ets, business.industry, Infant, Newborn, Infant, Thrombocytopenia, Repressor Proteins, ETV6, 030104 developmental biology, Mutation, Immunology, business, 030215 immunology
Abstract

ETV6-related thrombocytopenia is an autosomal dominant thrombocytopenia that has been recently identified in a few families and has been suspected to predispose to hematologic malignancies. To gain further information on this disorder, we searched for ETV6 mutations in the 130 families with inherited thrombocytopenia of unknown origin from our cohort of 274 consecutive pedigrees with familial thrombocytopenia. We identified 20 patients with ETV6-related thrombocytopenia from seven pedigrees. They have five different ETV6 variants, including three novel mutations affecting the highly conserved E26 transformation-specific domain. The relative frequency of ETV6-related thrombocytopenia was 2.6% in the whole case series and 4.6% among the families with known forms of inherited thrombocytopenia. The degree of thrombocytopenia and bleeding tendency of the patients with ETV6-related thrombocytopenia were mild, but four subjects developed B-cell acute lymphoblastic leukemia during childhood, resulting in a significantly higher incidence of this condition compared to that in the general population. Clinical and laboratory findings did not identify any particular defects that could lead to the suspicion of this disorder from the routine diagnostic workup. However, at variance with most inherited thrombocytopenias, platelets were not enlarged. In vitro studies revealed that the maturation of the patients' megakaryocytes was defective and that the patients have impaired proplatelet formation. Moreover, platelets from patients with ETV6-related thrombocytopenia have reduced ability to spread on fibrinogen. Since the dominant thrombocytopenias due to mutations in RUNX1 and ANKRD26 are also characterized by normal platelet size and predispose to hematologic malignancies, we suggest that screening for ETV6, RUNX1 and ANKRD26 mutations should be performed in all subjects with autosomal dominant thrombocytopenia and normal platelet size.

Published
2016

34. Synergic interplay of the La motif, RRM1 and the interdomain linker of LARP6 in the recognition of collagen mRNA expands the RNA binding repertoire of the La module

Author

Luigi, Martino, Simon, Pennell, Geoff, Kelly, Baptiste, Busi, Paul, Brown, R Andrew, Atkinson, Nicholas J H, Salisbury, Zi-Hao, Ooi, Kang-Wei, See, Stephen J, Smerdon, Caterina, Alfano, Tam T T, Bui, and Maria R, Conte

Subjects
Models, Molecular, Ribonucleoproteins, Structural Biology, Amino Acid Motifs, Molecular Sequence Data, Mutation, Humans, Amino Acid Sequence, Collagen, 5' Untranslated Regions, Autoantigens, Sequence Alignment, Protein Binding
Abstract

The La-related proteins (LARPs) form a diverse group of RNA-binding proteins characterized by the possession of a composite RNA binding unit, the La module. The La module comprises two domains, the La motif (LaM) and the RRM1, which together recognize and bind to a wide array of RNA substrates. Structural information regarding the La module is at present restricted to the prototypic La protein, which acts as an RNA chaperone binding to 3′ UUUOH sequences of nascent RNA polymerase III transcripts. In contrast, LARP6 is implicated in the regulation of collagen synthesis and interacts with a specific stem-loop within the 5′ UTR of the collagen mRNA. Here, we present the structure of the LaM and RRM1 of human LARP6 uncovering in both cases considerable structural variation in comparison to the equivalent domains in La and revealing an unprecedented fold for the RRM1. A mutagenic study guided by the structures revealed that RNA recognition requires synergy between the LaM and RRM1 as well as the participation of the interdomain linker, probably in realizing tandem domain configurations and dynamics required for substrate selectivity. Our study highlights a considerable complexity and plasticity in the architecture of the La module within LARPs.

Published
2014

35. Solution Structure of the SGTA Dimerisation Domain and Investigation of Its Interactions with the Ubiquitin-Like Domains of BAG6 and UBL4A

Author

Aline C. Simon, Pawel Leznicki, Peter Simpson, Santiago Martínez-Lumbreras, Lisa R. Hale, David S. Bishop, Arjun Thapaliya, John F. Darby, Ewelina M. Krysztofinska, Rivka L. Isaacson, Newran Sriskandarajah, Stephen High, Caterina Alfano, and Maria R. Conte

Subjects
Models, Molecular, Magnetic Resonance Spectroscopy, Cell Membranes, lcsh:Medicine, Bioinformatics, Biochemistry, Protein structure, Protein Interaction Mapping, lcsh:Science, RETICULUM-ASSOCIATED DEGRADATION, Cellular Stress Responses, CHAPERONE, Multidisciplinary, biology, PROLIFERATION, Multidisciplinary Sciences, Solutions, Tetratricopeptide, Cell Processes, Endoplasmic Reticulum Stress Response, Science & Technology - Other Topics, Cellular Structures and Organelles, Research Article, Protein Binding, EXPRESSION, General Science & Technology, Protein domain, ENDOPLASMIC-RETICULUM, INSERTION, Structural Characterization, Research and Analysis Methods, Binding, Competitive, Protein–protein interaction, MD Multidisciplinary, RETROTRANSLOCATION, Animals, Humans, Protein Interactions, Ubiquitins, Science & Technology, COMPLEX, Binding Sites, Ubiquitin, Microscale thermophoresis, lcsh:R, Biology and Life Sciences, Proteins, Membrane Proteins, MICROSCALE THERMOPHORESIS, Computational Biology, Isothermal titration calorimetry, Cell Biology, Chaperone Proteins, Protein Structure, Tertiary, Transmembrane Proteins, Protein-Protein Interactions, Multiprotein Complexes, Chaperone (protein), biology.protein, Biophysics, lcsh:Q, Protein Multimerization, Carrier Proteins, ANCHORED MEMBRANE-PROTEINS, Software, Alpha helix, Molecular Chaperones
Abstract

Background The BAG6 complex resides in the cytosol and acts as a sorting point to target diverse hydrophobic protein substrates along their appropriate paths, including proteasomal degradation and ER membrane insertion. Composed of a trimeric complex of BAG6, TRC35 and UBL4A, the BAG6 complex is closely associated with SGTA, a co-chaperone from which it can obtain hydrophobic substrates. Methodology and Principal Findings SGTA consists of an N-terminal dimerisation domain (SGTA_NT), a central tetratricopeptide repeat (TPR) domain, and a glutamine rich region towards the C-terminus. Here we solve a solution structure of the SGTA dimerisation domain and use biophysical techniques to investigate its interaction with two different UBL domains from the BAG6 complex. The SGTA_NT structure is a dimer with a tight hydrophobic interface connecting two sets of four alpha helices. Using a combination of NMR chemical shift perturbation, isothermal titration calorimetry (ITC) and microscale thermophoresis (MST) experiments we have biochemically characterised the interactions of SGTA with components of the BAG6 complex, the ubiquitin-like domain (UBL) containing proteins UBL4A and BAG6. We demonstrate that the UBL domains from UBL4A and BAG6 directly compete for binding to SGTA at the same site. Using a combination of structural and interaction data we have implemented the HADDOCK protein-protein interaction docking tool to generate models of the SGTA-UBL complexes. Significance This atomic level information contributes to our understanding of the way in which hydrophobic proteins have their fate decided by the collaboration between SGTA and the BAG6 complex.

Published
2014

36. A new mutant of Bovine Seminal Ribonuclease with a reversed swapping propensity

Author

Carmine Ercole, Teodorico Tancredi, Delia Picone, Roberta Spadaccini, Caterina Alfano, Ercole, Carmine, R., Spadaccini, C., Alfano, T., Tancredi, and Picone, Delia

Subjects
Models, Molecular, Circular dichroism, Protein Conformation, RNase P, Stereochemistry, Mutant, Mutagenesis (molecular biology technique), Sequence (biology), Crystallography, X-Ray, Bovine pancreatic ribonuclease, Biochemistry, Evolution, Molecular, BS-RNase, Protein structure, Endoribonucleases, Enzyme Stability, Animals, Ribonuclease, Nuclear Magnetic Resonance, Biomolecular, biology, Chemistry, Circular Dichroism, Temperature, domain swapping, hinge peptide, protein engineering, Ribonuclease, Pancreatic, NMR, Protein Structure, Tertiary, flexibility, Crystallography, Mutagenesis, Site-Directed, biology.protein, Cattle, Dimerization
Abstract

Bovine seminal ribonuclease (BS-RNase) is made up of two identical subunits bridged through two disulfide bonds. In solution, it exists as a 2:1 equilibrium mixture between two forms, with (MxM) and without swapping (M=M) of the N-terminal arms. The swapping endows BS-RNase with some special biological functions, including antitumor activity, since MxM retains a dimeric structure even under reducing conditions, thus evading the cytosolic ribonuclease inhibitor. To investigate the structural basis of domain swapping in BS-RNase, we have obtained several mutants by replacing selected residues with the corresponding ones of its monomeric counterpart, bovine pancreatic ribonuclease (RNase A). We have already shown that, in contrast with all other cases of swapped proteins, the swapping propensity of BS-RNase does not depend on the specific sequence of the 16-22 hinge loop, which connects the main body to the dislocating arm. In this paper we report the design, the expression, and the structural characterization of two mutants obtained by replacing Arg80 with Ser either in BS-RNase or in the mutant already containing the 16-22 hinge sequence of RNase A. NMR and circular dichroism data indicate that, in the monomeric form of the latter mutant, Ser80 acts as a switch for the conformation of the hinge region. Accordingly, in the dimeric form of the same mutant the MxM:M=M equilibrium ratio is inverted to 1:2. Overall, these data suggest that the presence of Arg80 triggers the swapping of N-terminal ends and plays a relevant role in the stability of the swapped form of BS-RNase.

Published
2007

37. Structural analysis of cooperative RNA binding by the La motif and central RRM domain of human La protein

Author

Geoff Kelly, Maria R. Conte, Stephen Curry, Amanda Jacks, Caterina Alfano, Jeffrey J. Babon, and Domenico Sanfelice

Subjects
Riboswitch, Models, Molecular, Magnetic Resonance Spectroscopy, Stereochemistry, Molecular Sequence Data, Biology, Autoantigens, RNA polymerase III, Protein Structure, Secondary, Structural Biology, Animals, Humans, Amino Acid Sequence, Molecular Biology, Conserved Sequence, Ribonucleoprotein, Binding Sites, RNA recognition motif, Sequence Homology, Amino Acid, Oligonucleotide, RNA, Cooperative binding, Molecular biology, Protein Structure, Tertiary, Ribonucleoproteins, Sequence motif, Sequence Alignment
Abstract

The La protein is a conserved component of eukaryotic ribonucleoprotein complexes that binds the 3' poly(U)-rich elements of nascent RNA polymerase III (pol III) transcripts to assist folding and maturation. This specific recognition is mediated by the N-terminal domain (NTD) of La, which comprises a La motif and an RNA recognition motif (RRM). We have determined the solution structures of both domains and show that the La motif adopts an alpha/beta fold that comprises a winged-helix motif elaborated by the insertion of three helices. Chemical shift mapping experiments show that these insertions are involved in RNA interactions. They further delineate a distinct surface patch on each domain-containing both basic and aromatic residues-that interacts with RNA and accounts for the cooperative binding of short oligonucleotides exhibited by the La NTD.

Published
2004

39. The swapping of terminal arms in ribonucleases: comparison of the solution structure of monomeric bovine seminal and pancreatic ribonucleases

Author

Francesca Avitabile, Delia Picone, Giuseppe D’Alessio, Teodorico Tancredi, Orlando Crescenzi, Anna Maria D'Ursi, Roberta Spadaccini, Caterina Alfano, Avitabile, F, Alfano, C., Spadaccini, R, Crescenzi, O, D'Ursi, Am, D'Alessio, G, Tancredi, T, Picone, Delia, Alfano, C, Spadaccini, Roberta, Crescenzi, Orlando, and D'Alessio, Giuseppe

Subjects
Models, Molecular, Magnetic Resonance Spectroscopy, Proline, Stereochemistry, RNase P, Protein Conformation, Peptide, Bovine pancreatic ribonuclease, Biochemistry, Protein Structure, Secondary, Diffusion, chemistry.chemical_compound, Hydrolase, Endoribonucleases, Escherichia coli, Animals, Ribonuclease, Protein secondary structure, chemistry.chemical_classification, biology, Temperature, Hydrogen Bonding, Ribonuclease, Pancreatic, Hydrogen-Ion Concentration, Protein Structure, Tertiary, Crystallography, Monomer, chemistry, Heteronuclear molecule, biology.protein, Mutagenesis, Site-Directed, Cattle, Dimerization, Protein Binding
Abstract

Bovine seminal ribonuclease (BS-RNase), the only dimeric protein among the pancreatic-like ribonucleases, is endowed with special structural features and with biological functions beyond enzymatic activity. In solution, the protein exists as an equilibrium mixture of two forms, with or without exchange (or swapping) of the N-terminal arms. After selective reduction and alkylation of the two intrachain disulfide bridges, the dimeric protein can be transformed into a monomeric derivative that has a ribonuclease activity higher than that of the parent dimeric protein but is devoid of the special biological functions. A detailed investigation of the structural features of this protein in solution, in comparison with those of other monomeric ribonucleases, may help unveil the structural details which induce swapping of the N-terminal arms of BS-RNase. The solution structure of the recombinant monomeric form of BS-RNase, as determined by 3D heteronuclear NMR, shows close similarity with that of bovine pancreatic ribonuclease (RNase A) in all regions characterized by regular elements of secondary structure. However, significant differences are present in the flexible regions, which could account for the different behavior of the two proteins. To characterize in detail these regions, we have measured H/D exchange rate constants, temperature coefficients and heteronuclear NOEs of backbone amides for both RNase A and monomeric BS-RNase. The results indicate a large difference in the backbone flexibility of the hinge peptide segment 16-22 of the two proteins, which could provide the molecular basis to explain the ability of BS-RNase subunits to swap their N-terminal arms.

Published
2003

40. [Untitled]

Author

Jeffrey J. Babon, Stephen Curry, Geoff Kelly, Caterina Alfano, and Maria R. Conte

Subjects
Nuclear magnetic resonance, Terminal (electronics), Fragment (computer graphics), Stereochemistry, Chemistry, Resonance, La Protein, LA antigen, Biochemistry, Protein secondary structure, Spectroscopy
Published
2003

41. Electrostatics regulate Epigallocatechin-Gallate effects on Bovine Serum Albumin aggregation

Author

Daniele Gulli, Giuseppe Sancataldo, Caterina Alfano, Bruno Giuseppe Pignataro, Valeria Vetri, and Daniele Gulli, Giuseppe Sancataldo, Caterina Alfano, Bruno Giuseppe Pignataro, Valeria Vetri

Subjects
BSA, Isoelectric point, electrostatic interaction, protein charge, Settore FIS/07 - Fisica Applicata(Beni Culturali, Ambientali, Biol.e Medicin)
Abstract

Protein aggregation processes are complex phenomena often involved in the etiology of several pathologies. It is now assessed that all proteins, in suitable conditions, may undergo supramolecular assembly. Aggregation pathways are known to be controlled by solution conditions which regulate protein-protein and protein-solvent interactions affecting binding mechanisms, morphology and inherent toxicity of the aggregate species. In this context, the presence of small molecules was indicated as a promising method to modulate protein-protein interactions reducing pathogenic aggregation. In the light of the idea that common mechanisms regulate anti-aggregogenic properties of small molecules, we here investigate Epigallocatechin-Gallate (EGCG) effects on the thermal aggregation pathway of Bovine Serum Albumin (BSA), a well-known model protein. EGCG is a small molecule extracted from green tea, which is known to reduce aggregation of key proteins involved in neurodegenerative diseases [1]. Fundamental mechanisms which regulate EGCG effectiveness as therapeutic molecule are still not clearly elucidated. The interaction of EGCG with BSA and its effects on thermal aggregation pathway were investigated by means of spectroscopic methods and Isothermal Titration calorimetry as a function of solution conditions. Results show that electrostatic forces modulated by pH play a key role in regulating EGCG interactions with BSA. Data shows that close to the isoelectric point of the protein, EGCG is found to promote the supramolecular assembly, whilst away from the isoelectric point, EGCG is found to reduce aggregation mechanisms increasing protein conformational stability. These results reveal the large impact of electrostatics in small molecules effects on the protein aggregation phenomena requiring larger investigation aimed at rationalizing their effects on related pathogenic mechanisms.

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