Your search keyword '"Biophysical assays"' showing total 27 results

1. Optimizing the affinity selection mass spectrometry workflow for efficient identification and ranking of potent USP1 inhibitors

Author

Yi Zhao, Meixian Liu, Tian Qin, Yongqiang Peng, Guang Lin, Chao Che, and Zhendong Zhu

Subjects

High throughput mass spec (HTMS), Affinity selection MS (AS-MS), USP1 inhibitors, Protein immobilization, Drug discovery technology, Biophysical assays, Biotechnology, TP248.13-248.65, Medical technology, R855-855.5

Abstract

An optimized Affinity Selection-Mass Spectrometry (AS-MS) workflow has been developed for the efficient identification of potent USP1 inhibitors. USP1 was immobilized on agarose beads, ensuring low small molecule retention, efficient protein capture, and protein stability. The binding affinity of 49 compounds to USP1 was evaluated using the optimized AS-MS method, calculating binding index (BI) values for each compound. Biochemical inhibition assays validated the AS-MS results, revealing a potential correlation between higher BI values and lower IC50 values. This optimized workflow enables rapid identification of high-quality USP1 inhibitor hits, facilitating structure-activity relationship studies and accelerating the discovery of potential cancer therapeutics.

Published

2024

2. Molecular mechanisms of the influenza fusion peptide: insights from experimental and simulation studies

Author

Diana Lousa and Cláudio M. Soares

Subjects

biophysical assays, hemagglutinin, influenza, membrane fusion, molecular dynamics simulation, virus, Biology (General), QH301-705.5

Abstract

A key step in infections by enveloped viruses, such as influenza, is the fusion between the viral envelope and the host cell membrane, which allows the virus to insert its genetic material into the host cell and replicate. The influenza virus fusion process is promoted by hemagglutinin (HA), a glycoprotein that contains three identical monomers composed of two polypeptide chains (HA1 and HA2). Early studies on this protein revealed that HA‐mediated fusion involves the insertion of the HA2 N‐terminal segment into the host membrane and that this segment, known as the fusion peptide, is a key player in the fusion process. This mini‐review highlights the main findings that have been obtained by experimental and computational studies on the HA fusion peptide, which give us a glimpse of its mode of action.

Published

2021

3. Applied Biophysics for Bromodomain Drug Discovery

Author

Pomerantz, William C. K., Johnson, Jorden A., Ycas, Peter D., Bernstein, Peter R., Series Editor, Garner, Amanda L., Series Editor, Georg, Gunda I., Series Editor, Lowe, John A., Series Editor, Meanwell, Nicholas A., Series Editor, Saxena, Anil Kumar, Series Editor, Supuran, Claudiu T., Series Editor, Zhang, Ao, Series Editor, and Mai, Antonello, editor

Published

2020

4. Molecular mechanisms of the influenza fusion peptide: insights from experimental and simulation studies.

Author

Lousa, Diana and Soares, Cláudio M.

Subjects

MEMBRANE fusion, INFLUENZA, VIRAL envelopes, VIRUS diseases, INFLUENZA viruses, INFLUENZA A virus

Abstract

A key step in infections by enveloped viruses, such as influenza, is the fusion between the viral envelope and the host cell membrane, which allows the virus to insert its genetic material into the host cell and replicate. The influenza virus fusion process is promoted by hemagglutinin (HA), a glycoprotein that contains three identical monomers composed of two polypeptide chains (HA1 and HA2). Early studies on this protein revealed that HA‐mediated fusion involves the insertion of the HA2 N‐terminal segment into the host membrane and that this segment, known as the fusion peptide, is a key player in the fusion process. This mini‐review highlights the main findings that have been obtained by experimental and computational studies on the HA fusion peptide, which give us a glimpse of its mode of action. [ABSTRACT FROM AUTHOR]

Published

2021

5. Optimizing the affinity selection mass spectrometry workflow for efficient identification and ranking of potent USP1 inhibitors.

Author

Zhao Y, Liu M, Qin T, Peng Y, Lin G, Che C, and Zhu Z

Subjects

Humans, Workflow, Ubiquitin-Specific Proteases antagonists & inhibitors, Ubiquitin-Specific Proteases metabolism, Protein Binding, Mass Spectrometry methods, Enzyme Inhibitors pharmacology, Enzyme Inhibitors chemistry

Abstract

An optimized Affinity Selection-Mass Spectrometry (AS-MS) workflow has been developed for the efficient identification of potent USP1 inhibitors. USP1 was immobilized on agarose beads, ensuring low small molecule retention, efficient protein capture, and protein stability. The binding affinity of 49 compounds to USP1 was evaluated using the optimized AS-MS method, calculating binding index (BI) values for each compound. Biochemical inhibition assays validated the AS-MS results, revealing a potential correlation between higher BI values and lower IC 50 values. This optimized workflow enables rapid identification of high-quality USP1 inhibitor hits, facilitating structure-activity relationship studies and accelerating the discovery of potential cancer therapeutics., Competing Interests: Declaration of competing interest The authors declare that they have no known competing financial interests or personal relationships that could have appeared to influence the work reported in this paper., (Copyright © 2024 The Author(s). Published by Elsevier Inc. All rights reserved.)

Published

2024

6. Molecular recognition of a single-chain Fv antibody specific for GA-pyridine, an advanced glycation end-product (AGE), elucidated using biophysical techniques and synthetic antigen analogues.

Author

Kobashigawa, Yoshihiro, Ohara, Toshiya, Morita, Kosuke, Toyota, Yuya, Nakamura, Teruya, Kotani, Shunsuke, Arimori, Takao, Yamauchi, Soichiro, Liu, Chenjiang, Kitazaki, Masaya, Wakeyama-Miyazaki, Yukari, Suwa, Yoshiaki, Uchida-Kamekura, Makiyo, Fukuda, Natsuki, Sato, Takashi, Nakajima, Makoto, Takagi, Junichi, Yamagata, Yuriko, and Morioka, Hiroshi

Subjects

*MOLECULAR recognition, *ADVANCED glycation end-products, *CHEMICAL biology, *IMMUNE recognition, *ANTIGENS

Abstract

Advanced glycation end-products (AGEs) are a heterogeneous group of compounds formed by non-enzymatic reaction between reducing-sugar and Arg/Lys in proteins and are involved in various diabetic complications. GA-pyridine is derived from glycolaldehyde and is one of the most cytotoxic AGEs. Here, we established a single-chain Fv (scFv) antibody against GA-pyridine, 73MuL9-scFv, and examined the details of its specificity and antigen recognition by using various techniques involving biophysics, chemical biology and structural biology. We also synthesized several compounds that differ slightly in regard to the position and number of GA-pyridine substituent groups, and revealed that GA-pyridine was specifically bound to 73MuL9-scFv. Thermodynamic analysis revealed that the association of GA-pyridine to 73MuL9-scFv was an exothermic and enthalpy driven reaction, and thus that the antigen recognition involved multiple specific interactions. Crystallographic analysis of the Fv fragment of 73MuL9-scFv revealed that several CH-π and hydrogen bond interactions took place between the Fv-fragment and GA-pyridine, which was consistent with the results of thermodynamic analysis. Further studies using 73MuL9-scFv as a tool to clarify the relevance of GA-pyridine to diabetic complications are warranted. [ABSTRACT FROM AUTHOR]

Published

2021

7. Aptamers as Functional Modules for DNA Nanostructures

Author

Shiu, Simon Chi-Chin, Kinghorn, Andrew B., Guo, Wei, Slaughter, Liane Siu, Ji, Danyang, Mo, Xiaoyong, Wang, Lin, Tran, Ngoc Chau, Kwok, Chun Kit, Shum, Anderson Ho Cheung, Tse, Edmund Chun Ming, Tanner, Julian A., Shiu, Simon Chi-Chin, Kinghorn, Andrew B., Guo, Wei, Slaughter, Liane Siu, Ji, Danyang, Mo, Xiaoyong, Wang, Lin, Tran, Ngoc Chau, Kwok, Chun Kit, Shum, Anderson Ho Cheung, Tse, Edmund Chun Ming, and Tanner, Julian A.

Abstract

Watson-Crick base-pairing of DNA allows the nanoscale fabrication of biocompatible synthetic nanostructures for diagnostic and therapeutic biomedical purposes. DNA nanostructure design elicits exquisite control of shape and conformation compared to other nanoparticles. Furthermore, nucleic acid aptamers can be coupled to DNA nanostructures to allow interaction and response to a plethora of biomolecules beyond nucleic acids. When compared to the better-known approach of using protein antibodies for molecular recognition, nucleic acid aptamers are bespoke with the underlying DNA nanostructure backbone and have various other stability, synthesis, and cost advantages. Here, we provide detailed methodologies to synthesize and characterize aptamer-enabled DNA nanostructures. The methods described can be generally applied to various designs of aptamer-enabled DNA nanostructures with a wide range of applications both within and beyond biomedical nanotechnology. © 2023, Springer Science+Business Media, LLC, part of Springer Nature.

Published

2023

8. Structural changes in hemoglobin and glycation.

Author

Nascimento ALA, Guimarães AS, Rocha TDS, Goulart MOF, Xavier JA, and Santos JCC

Subjects

Humans, Glycosylation, Glycated Hemoglobin metabolism, Protein Conformation, Animals, Hemoglobins metabolism, Hemoglobins chemistry

Abstract

Hemoglobin (Hb) is a hemeprotein found inside erythrocytes and is crucial in transporting oxygen and carbon dioxide in our bodies. In erythrocytes (Ery), the main energy source is glucose metabolized through glycolysis. However, a fraction of Hb can undergo glycation, in which a free amine group from the protein spontaneously binds to the carbonyl of glucose in the bloodstream, resulting in the formation of glycated hemoglobin (HbA1c), widely used as a marker for diabetes. Glycation leads to structural and conformational changes, compromising the function of proteins, and is intensified in the event of hyperglycemia. The main changes in Hb include structural alterations to the heme group, compromising its main function (oxygen transport). In addition, amyloid aggregates can form, which are strongly related to diabetic complications and neurodegenerative diseases. Therefore, this chapter discusses in vitro protocols for producing glycated Hb, as well as the main techniques and biophysical assays used to assess changes in the protein's structure before and after the glycation process. This more complete understanding of the effects of glycation on Hb is fundamental for understanding the complications associated with hyperglycemia and for developing more effective prevention and treatment strategies., (Copyright © 2024. Published by Elsevier Inc.)

Published

2024

9. Cellular Models and Assays to Study NLRP3 Inflammasome Biology

Author

Giovanni Zito, Marco Buscetta, Maura Cimino, Paola Dino, Fabio Bucchieri, and Chiara Cipollina

Subjects

NLRP3, inflammasome, NLRP3 inhibitors, cell models, biochemical assays, biophysical assays, Biology (General), QH301-705.5, Chemistry, QD1-999

Abstract

The NLRP3 inflammasome is a multi-protein complex that initiates innate immunity responses when exposed to a wide range of stimuli, including pathogen-associated molecular patterns (PAMPs) and danger-associated molecular patterns (DAMPs). Inflammasome activation leads to the release of the pro-inflammatory cytokines interleukin (IL)-1β and IL-18 and to pyroptotic cell death. Over-activation of NLRP3 inflammasome has been associated with several chronic inflammatory diseases. A deep knowledge of NLRP3 inflammasome biology is required to better exploit its potential as therapeutic target and for the development of new selective drugs. To this purpose, in the past few years, several tools have been developed for the biological characterization of the multimeric inflammasome complex, the identification of the upstream signaling cascade leading to inflammasome activation, and the downstream effects triggered by NLRP3 activation. In this review, we will report cellular models and cellular, biochemical, and biophysical assays that are currently available for studying inflammasome biology. A special focus will be on those models/assays that have been used to identify NLRP3 inhibitors and their mechanism of action.

Published

2020

10. A Biophysical Approach to the Identification of Novel ApoE Chemical Probes

Author

Lucas Kraft, Louise C. Serpell, and John R. Atack

Subjects

ApoE, Alzheimer’s disease, drug discovery, high-throughput screening, chemical probes, biophysical assays, Microbiology, QR1-502

Abstract

Alzheimer’s disease (AD) is the most common type of dementia and, after age, the greatest risk factor for developing AD is the allelic variation of apolipoprotein E (ApoE), with homozygote carriers of the ApoE4 allele having an up to 12-fold greater risk of developing AD than noncarriers. Apolipoprotein E exists as three isoforms that differ in only two amino acid sites, ApoE2 (Cys112/Cys158), ApoE3 (Cys112/Arg158), and ApoE4 (Arg112/Arg158). These amino acid substitutions are assumed to alter ApoE structure and function, and be responsible for the detrimental effects of ApoE4 via a mechanism that remains unclear. The hypothesis that a structural difference between ApoE4 and ApoE3 (and ApoE2) is the cause of the ApoE4-associated increased risk for AD forms the basis of a therapeutic approach to modulate ApoE4 structure, and we were therefore interested in screening to identify new chemical probes for ApoE4. In this regard, a high-yield protocol was developed for the expression and purification of recombinant full-length ApoE, and three diverse biophysical screening assays were established and characterized; an optical label-free assay (Corning Epic) for hit identification and microscale thermophoresis (MST) and isothermal titration calorimetry (ITC) as orthogonal assays for hit confirmation. The 707 compounds in the National Institute of Health clinical collection were screened for binding to ApoE4, from which six confirmed hits, as well as one analogue, were identified. Although the compounds did not differentiate between ApoE isoforms, these data nevertheless demonstrate the feasibility of using a biophysical approach to identifying compounds that bind to ApoE and that, with further optimization, might differentiate between isoforms to produce a molecule that selectively alters the function of ApoE4.

Published

2019

11. Complexes of Pro-Apoptotic siRNAs and Carbosilane Dendrimers: Formation and Effect on Cancer Cells

Author

Olga A. Krasheninina, Evgeny K. Apartsin, Elena Fuentes, Aleksandra Szulc, Maksim Ionov, Alya G. Venyaminova, Dzmitry Shcharbin, F. Javier de la Mata, Maria Bryszewska, and Rafael Gόmez

Subjects

carbosilane, dendrimers, anticancer siRNA, nucleic acids, dendriplexes, complexation, transfection, cytotoxicity, biophysical assays, Pharmacy and materia medica, RS1-441

Abstract

This paper examines the complexation of anti-cancer small interfering RNAs (siRNAs) by cationic carbosilane dendrimers, and the interaction of the formed complexes with HeLa and HL-60 cancer cells. Stepwise formation of the complexes accompanied by the evolution of their properties has been observed through the increase of the charge ratio (dendrimer/siRNA). The complexes decrease the viability of both “easy-to-transfect” cells (HeLa) and “hard-to transfect” ones (HL-60), indicating a high potential of the cationic carbosilane dendrimers for siRNA delivery into tumor cells.

Published

2019

12. Molecular mechanisms of the influenza fusion peptide: insights from experimental and simulation studies

Author

Cláudio M. Soares and Diana Lousa

Subjects

Models, Molecular, QH301-705.5, Protein Conformation, membrane fusion, Hemagglutinin (influenza), Reviews, Review, virus, General Biochemistry, Genetics and Molecular Biology, Insert (molecular biology), Virus, biophysical assays, Viral envelope, Influenza, Human, Humans, hemagglutinin, Biology (General), Viral Fusion Protein Inhibitors, chemistry.chemical_classification, Host cell membrane, Fusion, Membranes, biology, Chemistry, Lipid bilayer fusion, Hydrogen-Ion Concentration, Cell biology, molecular dynamics simulation, Influenza A virus, biology.protein, Glycoprotein, Peptides, influenza, Viral Fusion Proteins

Abstract

A key step in infections by enveloped viruses, such as influenza, is the fusion between the viral envelope and the host cell membrane, which allows the virus to insert its genetic material into the host cell and replicate. The influenza virus fusion process is promoted by hemagglutinin (HA), a glycoprotein that contains three identical monomers composed of two polypeptide chains (HA1 and HA2). Early studies on this protein revealed that HA‐mediated fusion involves the insertion of the HA2 N‐terminal segment into the host membrane and that this segment, known as the fusion peptide, is a key player in the fusion process. This mini‐review highlights the main findings that have been obtained by experimental and computational studies on the HA fusion peptide, which give us a glimpse of its mode of action., A key step in influenza infection is the fusion of the viral and host membranes, promoted by the protein hemagglutinin, which contains a fusion peptide that inserts and destabilizes the host membrane. This review highlights the major findings of experimental and computational studies, which analyzed the properties of this peptide, including the role of key residues for its fusogenic activity.

Published

2021

13. Lessons from snake venom: new insights into the structural and functional aspects of factor V and factor X

Author

Verhoef, D., Reitsma, P.H., Bos, M.H.A., Versteeg, H.H., Meijer, A.B., Castoldi, E., and Leiden University

Subjects

Clotting assays, Snake venom, Thrombin generation, Coagulation factor X, Coagulation factor V, Protein engineering, Blood coagulation, Biophysical assays, complex mixtures, Biochemistry, Enzymatic inhibitors

Abstract

The venom of the Australian snake Pseudonaja textilis contains coagulation factors V (five) and X (ten) which have been adapted to derail the blood clotting system of its prey. Snake venom factor V is unique in that is constitutively active, unlike its human counterpart. The snake liver transcriptome was found to contain alternatively spliced factor V mRNA that encoded for either the activated protein or its quiescent form. A potential pre-mRNA splicing mechanism was uncovered that may yield the active protein. Snake venom factor V is also particularly stable due to several modifications to its molecular structure. These modifications have been investigated in detail by engineering chimeras of human and snake venom factor V. The snake venom factor X molecule was also investigated in more detail. It was discovered that this enzyme is insensitive to the action of certain anticoagulant drugs (Factor Xa inhibitors) due to a unique molecular modification. A Human factor X can be modified in similar fashion, so that it is no longer sensitive to the action of Factor Xa inhibitors. This finding could make an important contribution to acute care for patients who experience life-threatening bleeding after the use of FXa inhibitors.

Published

2021

14. [Untitled]

Author

Reitsma, P.H., Bos, M.H.A., Versteeg, H.H., Meijer, A.B., Castoldi, E., and Leiden University

Subjects

Clotting assays, Snake venom, Thrombin generation, Coagulation factor X, Coagulation factor V, Protein engineering, Blood coagulation, Biophysical assays, Biochemistry, Enzymatic inhibitors

Abstract

The venom of the Australian snake Pseudonaja textilis contains coagulation factors V (five) and X (ten) which have been adapted to derail the blood clotting system of its prey. Snake venom factor V is unique in that is constitutively active, unlike its human counterpart. The snake liver transcriptome was found to contain alternatively spliced factor V mRNA that encoded for either the activated protein or its quiescent form. A potential pre-mRNA splicing mechanism was uncovered that may yield the active protein. Snake venom factor V is also particularly stable due to several modifications to its molecular structure. These modifications have been investigated in detail by engineering chimeras of human and snake venom factor V. The snake venom factor X molecule was also investigated in more detail. It was discovered that this enzyme is insensitive to the action of certain anticoagulant drugs (Factor Xa inhibitors) due to a unique molecular modification. A Human factor X can be modified in similar fashion, so that it is no longer sensitive to the action of Factor Xa inhibitors. This finding could make an important contribution to acute care for patients who experience life-threatening bleeding after the use of FXa inhibitors.

Published

2021

15. Biophysical and Computational Approaches to Study Ternary Complexes: A 'Cooperative Relationship' to Rationalize Targeted Protein Degradation.

Author

Ward JA, Perez-Lopez C, and Mayor-Ruiz C

Subjects

Proteolysis, Ubiquitination, Protein Binding, Ubiquitin-Protein Ligases metabolism, Proteome metabolism

Abstract

Degraders have illustrated that compound-induced proximity to E3 ubiquitin ligases can prompt the ubiquitination and degradation of disease-relevant proteins. Hence, this pharmacology is becoming a promising alternative and complement to available therapeutic interventions (e. g., inhibitors). Degraders rely on protein binding instead of inhibition and, hence, they hold the promise to broaden the druggable proteome. Biophysical and structural biology approaches have been the cornerstone of understanding and rationalizing degrader-induced ternary complex formation. Computational models have now started to harness the experimental data from these approaches with the aim to identify and rationally help design new degraders. This review outlines the current experimental and computational strategies used to study ternary complex formation and degradation and highlights the importance of effective crosstalk between these approaches in the advancement of the targeted protein degradation (TPD) field. As our understanding of the molecular features that govern drug-induced interactions grows, faster optimizations and superior therapeutic innovations for TPD and other proximity-inducing modalities are sure to follow., (© 2023 Wiley-VCH GmbH.)

Published

2023

16. Aptamers as Functional Modules for DNA Nanostructures.

Author

Shiu SC, Kinghorn AB, Guo W, Slaughter LS, Ji D, Mo X, Wang L, Tran NC, Kwok CK, Shum AHC, Tse ECM, and Tanner JA

Subjects

DNA chemistry, Nanotechnology methods, Nucleic Acid Conformation, Aptamers, Nucleotide chemistry, Nanostructures chemistry, Nucleic Acids chemistry

Abstract

Watson-Crick base-pairing of DNA allows the nanoscale fabrication of biocompatible synthetic nanostructures for diagnostic and therapeutic biomedical purposes. DNA nanostructure design elicits exquisite control of shape and conformation compared to other nanoparticles. Furthermore, nucleic acid aptamers can be coupled to DNA nanostructures to allow interaction and response to a plethora of biomolecules beyond nucleic acids. When compared to the better-known approach of using protein antibodies for molecular recognition, nucleic acid aptamers are bespoke with the underlying DNA nanostructure backbone and have various other stability, synthesis, and cost advantages. Here, we provide detailed methodologies to synthesize and characterize aptamer-enabled DNA nanostructures. The methods described can be generally applied to various designs of aptamer-enabled DNA nanostructures with a wide range of applications both within and beyond biomedical nanotechnology., (© 2023. Springer Science+Business Media, LLC, part of Springer Nature.)

Published

2023

17. A cyclic GB virus C derived peptide with anti-HIV-1 activity targets the fusion peptide of HIV-1.

Author

Galatola, Ramona, Vasconcelos, Aimee, Pérez, Yolanda, Cruz, Antonio, Pujol, Montserrat, Alsina, María A., Gómara, María J., and Haro, Isabel

Subjects

*PEPTIDE analysis, *ANTI-HIV agents, *TARGETED drug delivery, *PEPTIDES, *CELL membranes

Abstract

The development of peptide fusion inhibitors based on short synthetic peptides represents a promising option in the fight against HIV-1 infection, especially in individuals infected with multiresistant HIV-1 strains. GBV-C has the beneficial effect of retarding the progression of AIDS in people who are co-infected with both the GBV-C and HIV viruses. In previous works, the E1(22–39) GBV-C sequence (E1P8lin) was found to be capable of inhibiting the interaction of HIV-1 FP with bilayers and its cyclic analogue (E1P8cyc) showed a higher anti-HIV-1 activity. In the present work, in an attempt to gain a better understanding of the interaction of E1P8 peptides with HIV-1 FP, we analyzed direct interactions between peptides at the molecular level. Our results support that E1P8cyc might be more potent at blocking HIV-1 entry than E1P8lin as a consequence of the structure induced in the complex formed with HIV-1 FP, which is able to modify the conformation adopted by this functional domain of the HIV-1 gp41 protein in target cell membranes. [ABSTRACT FROM AUTHOR]

Published

2014

18. Identification of a dual acting SARS-CoV-2 proteases inhibitor through in silico design and step-by-step biological characterization

Author

Mario Felice Tecce, Maria Carmina Scala, Robert Snoeck, Sara Novi, Vincenzo Vestuto, Pietro Campiglia, Gerardina Smaldone, Alessia Bertamino, Marina Sala, Francesca Di Matteo, Carmine Ostacolo, Veronica Di Sarno, Gianluigi Lauro, Ornella Moltedo, Graciela Andrei, Isabel Gomez-Monterrey, Tania Ciaglia, Simona Musella, Giuseppe Bifulco, Di Sarno, Veronica, Lauro, Gianluigi, Musella, Simona, Ciaglia, Tania, Vestuto, Vincenzo, Sala, Marina, Scala, Maria Carmina, Smaldone, Gerardina, Di Matteo, Francesca, Novi, Sara, Tecce, Mario Felice, Moltedo, Ornella, Bifulco, Giuseppe, Campiglia, Pietro, Gomez-Monterrey, Isabel M, Snoeck, Robert, Andrei, Graciela, Ostacolo, Carmine, and Bertamino, Alessia

Subjects

Drug, Proteases, media_common.quotation_subject, medicine.medical_treatment, In silico, Computational biology, Antiviral Agents, Article, Enzymatic assays, In-silico design, Drug Discovery, Chlorocebus aethiops, medicine, Animals, Computer Simulation, Protease Inhibitors, Pathogen, Vero Cells, Repurposing, Biophysical assays, Cellular characterization, SARS-CoV-2 proteases dual inhibitor, media_common, Pharmacology, Protease, Chemistry, SARS-CoV-2, Organic Chemistry, Enzymatic assay, General Medicine, Drug Design, Biophysical assay, Vero cell, Identification (biology)

Abstract

COVID-19 pandemic, starting from the latest 2019, and caused by SARS-CoV-2 pathogen, led to the hardest health-socio-economic disaster in the last century. Despite the tremendous scientific efforts, mainly focused on the development of vaccines, identification of potent and efficient anti-SARS-CoV-2 therapeutics still represents an unmet need. Remdesivir, an anti-Ebola drug selected from a repurposing campaign, is the only drug approved, so far, for the treatment of the infection. Nevertheless, WHO in later 2020 has recommended against its use in COVID-19. In the present paper, we describe a step-by-step in silico design of a small library of compounds as main protease (Mpro) inhibitors. All the molecules were screened by an enzymatic assay on Mpro and, then, cellular activity was evaluated using Vero cells viral infection model. The cellular screening disclosed compounds 29 and 34 as in-vitro SARS-CoV-2 replication inhibitors at non-toxic concentrations (0.32, Graphical abstract Image 1

Published

2021

19. Identification of a dual acting SARS-CoV-2 proteases inhibitor through in silico design and step-by-step biological characterization.

Author

Di Sarno, Veronica, Lauro, Gianluigi, Musella, Simona, Ciaglia, Tania, Vestuto, Vincenzo, Sala, Marina, Scala, Maria Carmina, Smaldone, Gerardina, Di Matteo, Francesca, Novi, Sara, Tecce, Mario Felice, Moltedo, Ornella, Bifulco, Giuseppe, Campiglia, Pietro, Gomez-Monterrey, Isabel M., Snoeck, Robert, Andrei, Graciela, Ostacolo, Carmine, and Bertamino, Alessia

Subjects

*PROTEASE inhibitors, *SARS-CoV-2, *COVID-19 pandemic, *PROTEOLYTIC enzymes, *COVID-19, *VIRUS diseases

Abstract

COVID-19 pandemic, starting from the latest 2019, and caused by SARS-CoV-2 pathogen, led to the hardest health-socio-economic disaster in the last century. Despite the tremendous scientific efforts, mainly focused on the development of vaccines, identification of potent and efficient anti-SARS-CoV-2 therapeutics still represents an unmet need. Remdesivir, an anti-Ebola drug selected from a repurposing campaign, is the only drug approved, so far, for the treatment of the infection. Nevertheless, WHO in later 2020 has recommended against its use in COVID-19. In the present paper, we describe a step-by-step in silico design of a small library of compounds as main protease (Mpro) inhibitors. All the molecules were screened by an enzymatic assay on Mpro and, then, cellular activity was evaluated using Vero cells viral infection model. The cellular screening disclosed compounds 29 and 34 as in-vitro SARS-CoV-2 replication inhibitors at non-toxic concentrations (0.32 < EC 50 < 5.98 μM). To rationalize these results, additional in-vitro assays were performed, focusing on papain like protease (PLpro) and spike protein (SP) as potential targets for the synthesized molecules. This pharmacological workflow allowed the identification of compound 29 , as a dual acting SARS-CoV-2 proteases inhibitor featuring micromolar inhibitory potency versus Mpro (IC 50 = 1.72 μM) and submicromolar potency versus PLpro (IC 50 = 0.67 μM), and of compound 34 as a selective SP inhibitor (IC 50 = 3.26 μM). [Display omitted] • Indole based compounds were designed in-silico as SARS-CoV-2 main protease inhibitors. • Step-by-step optimization of the cognate compounds was performed by in-vitro assays. • Different compounds showed low μM potencies when challenged in SARS-CoV-2 transfected Vero cells. • Further investigations were performed over different SARS-CoV-2 targets. • A dual Mpro/PLpro inhibitor and a selective SP inhibitor were disclosed. [ABSTRACT FROM AUTHOR]

Published

2021

20. A biophysical approach to the identification of novel ApoE chemical probes

Author

John R. Atack, Lucas Kraft, and Louise C. Serpell

Subjects

0301 basic medicine, Gene isoform, Apolipoprotein E, High-throughput screening, lcsh:QR1-502, Biochemistry, high-throughput screening, lcsh:Microbiology, Article, law.invention, drug discovery, biophysical assays, 03 medical and health sciences, 0302 clinical medicine, chemical probes, Apolipoproteins E, law, mental disorders, Humans, Protein Isoforms, Allele, Molecular Biology, Genetics, chemistry.chemical_classification, Molecular Structure, Microscale thermophoresis, Drug discovery, Amino acid, 030104 developmental biology, chemistry, Molecular Probes, Recombinant DNA, lipids (amino acids, peptides, and proteins), Alzheimer’s disease, human activities, 030217 neurology & neurosurgery, ApoE

Abstract

Alzheimer&rsquo, s disease (AD) is the most common type of dementia and, after age, the greatest risk factor for developing AD is the allelic variation of apolipoprotein E (ApoE), with homozygote carriers of the ApoE4 allele having an up to 12-fold greater risk of developing AD than noncarriers. Apolipoprotein E exists as three isoforms that differ in only two amino acid sites, ApoE2 (Cys112/Cys158), ApoE3 (Cys112/Arg158), and ApoE4 (Arg112/Arg158). These amino acid substitutions are assumed to alter ApoE structure and function, and be responsible for the detrimental effects of ApoE4 via a mechanism that remains unclear. The hypothesis that a structural difference between ApoE4 and ApoE3 (and ApoE2) is the cause of the ApoE4-associated increased risk for AD forms the basis of a therapeutic approach to modulate ApoE4 structure, and we were therefore interested in screening to identify new chemical probes for ApoE4. In this regard, a high-yield protocol was developed for the expression and purification of recombinant full-length ApoE, and three diverse biophysical screening assays were established and characterized, an optical label-free assay (Corning Epic) for hit identification and microscale thermophoresis (MST) and isothermal titration calorimetry (ITC) as orthogonal assays for hit confirmation. The 707 compounds in the National Institute of Health clinical collection were screened for binding to ApoE4, from which six confirmed hits, as well as one analogue, were identified. Although the compounds did not differentiate between ApoE isoforms, these data nevertheless demonstrate the feasibility of using a biophysical approach to identifying compounds that bind to ApoE and that, with further optimization, might differentiate between isoforms to produce a molecule that selectively alters the function of ApoE4.

Published

2019

21. Complexes of Pro-Apoptotic siRNAs and Carbosilane Dendrimers: Formation and Effect on Cancer Cells

Author

Aleksandra Szulc, Rafael Gόmez, Alya G. Venyaminova, Evgeny K. Apartsin, Maksim Ionov, Elena Fuentes, F. Javier de la Mata, Dzmitry Shcharbin, Maria Bryszewska, and Olga A. Krasheninina

Subjects

Small interfering RNA, complexation, anticancer siRNA, Pharmaceutical Science, lcsh:RS1-441, carbosilane, 02 engineering and technology, 01 natural sciences, Article, dendrimers, biophysical assays, HeLa, lcsh:Pharmacy and materia medica, Dendrimer, Cytotoxicity, biology, 010405 organic chemistry, Chemistry, dendriplexes, Cationic polymerization, Transfection, 021001 nanoscience & nanotechnology, biology.organism_classification, 3. Good health, 0104 chemical sciences, nucleic acids, transfection, Apoptosis, Cancer cell, Biophysics, cytotoxicity, 0210 nano-technology

Abstract

This paper examines the complexation of anti-cancer small interfering RNAs (siRNAs) by cationic carbosilane dendrimers, and the interaction of the formed complexes with HeLa and HL-60 cancer cells. Stepwise formation of the complexes accompanied by the evolution of their properties has been observed through the increase of the charge ratio (dendrimer/siRNA). The complexes decrease the viability of both &ldquo, easy-to-transfect&rdquo, cells (HeLa) and &ldquo, hard-to transfect&rdquo, ones (HL-60), indicating a high potential of the cationic carbosilane dendrimers for siRNA delivery into tumor cells.

Published

2019

22. Cellular Models and Assays to Study NLRP3 Inflammasome Biology

Author

Chiara Cipollina, Marco Buscetta, Fabio Bucchieri, Maura Cimino, Paola Dino, Giovanni Zito, Zito G., Buscetta M., Cimino M., Dino P., Bucchieri F., and Cipollina C.

Subjects

Programmed cell death, 2019-20 coronavirus outbreak, Inflammasomes, Interleukin-1beta, Review, Biology, Biochemical assays, Models, Biological, Catalysis, Inflammasome, lcsh:Chemistry, Inorganic Chemistry, NLRP3, NLR Family, Pyrin Domain-Containing 3 Protein, Pyroptosis, medicine, Deep knowledge, Alarmins, Animals, Humans, Physical and Theoretical Chemistry, lcsh:QH301-705.5, Molecular Biology, Spectroscopy, Innate immune system, integumentary system, Cell models, Pathogen-Associated Molecular Pattern Molecules, Organic Chemistry, Interleukin-18, Interleukin, General Medicine, Biophysical assays, Immunity, Innate, Computer Science Applications, Cell biology, NLRP3 inhibitors, lcsh:Biology (General), lcsh:QD1-999, Mechanism of action, Read-outs, medicine.symptom, Inflammasome complex, Signal Transduction, medicine.drug

Abstract

The NLRP3 inflammasome is a multi-protein complex that initiates innate immunity responses when exposed to a wide range of stimuli, including pathogen-associated molecular patterns (PAMPs) and danger-associated molecular patterns (DAMPs). Inflammasome activation leads to the release of the pro-inflammatory cytokines interleukin (IL)-1β and IL-18 and to pyroptotic cell death. Over-activation of NLRP3 inflammasome has been associated with several chronic inflammatory diseases. A deep knowledge of NLRP3 inflammasome biology is required to better exploit its potential as therapeutic target and for the development of new selective drugs. To this purpose, in the past few years, several tools have been developed for the biological characterization of the multimeric inflammasome complex, the identification of the upstream signaling cascade leading to inflammasome activation, and the downstream effects triggered by NLRP3 activation. In this review, we will report cellular models and cellular, biochemical, and biophysical assays that are currently available for studying inflammasome biology. A special focus will be on those models/assays that have been used to identify NLRP3 inhibitors and their mechanism of action.

Published

2020

23. Using Microscale Thermophoresis to Characterize Hits from High-Throughput Screening: A European Lead Factory Perspective

Author

Julie M. Rainard, George C. Pandarakalam, and Stuart P. McElroy

Subjects

0301 basic medicine, assay development, Computer science, High-throughput screening, Biophysics, Review, 01 natural sciences, Biochemistry, high-throughput screening, Analytical Chemistry, drug discovery, biophysical assays, Small Molecule Libraries, 03 medical and health sciences, Lead (geology), Microscale thermophoresis, Drug discovery, Target engagement, Temperature, microscale thermophoresis, 0104 chemical sciences, High-Throughput Screening Assays, Europe, 010404 medicinal & biomolecular chemistry, 030104 developmental biology, Workflow, Drug Design, Molecular targets, Molecular Medicine, Factory (object-oriented programming), Biological Assay, Biochemical engineering, Biotechnology

Abstract

High-throughput screening (HTS) is a proven method for discovering new lead matter for drug discovery and chemical biology. To maximize the likelihood of identifying genuine binders to a molecular target, and avoid wasting resources following up compounds with unproductive/nonspecific mechanisms of action, it is important to employ a range of assays during an HTS campaign that build confidence of target engagement for hit compounds. Biophysical methods that measure direct target/compound engagement have established themselves as key techniques in generating this confidence, and they are now integral to the latter stages of HTS triage at the European Lead Factory (ELF). One relatively new technique that the ELF is using is microscale thermophoresis (MST), which measures the differences in rate of movement through a temperature gradient that are caused when single molecular species form complexes. Here we provide an overview of the MST assay development workflow that the ELF employs and a perspective of our experience to date of using MST to triage the output of HTS campaigns and how it compares and contrasts with the use of other biophysical techniques.

Published

2018

24. Cellular Models and Assays to Study NLRP3 Inflammasome Biology.

Author

Zito, Giovanni, Buscetta, Marco, Cimino, Maura, Dino, Paola, Bucchieri, Fabio, and Cipollina, Chiara

Subjects

*DRUG development, *BIOLOGY, *CELL death, *NATURAL immunity

Abstract

The NLRP3 inflammasome is a multi-protein complex that initiates innate immunity responses when exposed to a wide range of stimuli, including pathogen-associated molecular patterns (PAMPs) and danger-associated molecular patterns (DAMPs). Inflammasome activation leads to the release of the pro-inflammatory cytokines interleukin (IL)-1β and IL-18 and to pyroptotic cell death. Over-activation of NLRP3 inflammasome has been associated with several chronic inflammatory diseases. A deep knowledge of NLRP3 inflammasome biology is required to better exploit its potential as therapeutic target and for the development of new selective drugs. To this purpose, in the past few years, several tools have been developed for the biological characterization of the multimeric inflammasome complex, the identification of the upstream signaling cascade leading to inflammasome activation, and the downstream effects triggered by NLRP3 activation. In this review, we will report cellular models and cellular, biochemical, and biophysical assays that are currently available for studying inflammasome biology. A special focus will be on those models/assays that have been used to identify NLRP3 inhibitors and their mechanism of action. [ABSTRACT FROM AUTHOR]

Published

2020

25. A Biophysical Approach to the Identification of Novel ApoE Chemical Probes.

Author

Kraft, Lucas, Serpell, Louise C., and Atack, John R.

Subjects

*ALZHEIMER'S disease, *BIOPHYSICS, *ISOTHERMAL titration calorimetry, *APOLIPOPROTEIN E

Abstract

Alzheimer's disease (AD) is the most common type of dementia and, after age, the greatest risk factor for developing AD is the allelic variation of apolipoprotein E (ApoE), with homozygote carriers of the ApoE4 allele having an up to 12-fold greater risk of developing AD than noncarriers. Apolipoprotein E exists as three isoforms that differ in only two amino acid sites, ApoE2 (Cys112/Cys158), ApoE3 (Cys112/Arg158), and ApoE4 (Arg112/Arg158). These amino acid substitutions are assumed to alter ApoE structure and function, and be responsible for the detrimental effects of ApoE4 via a mechanism that remains unclear. The hypothesis that a structural difference between ApoE4 and ApoE3 (and ApoE2) is the cause of the ApoE4-associated increased risk for AD forms the basis of a therapeutic approach to modulate ApoE4 structure, and we were therefore interested in screening to identify new chemical probes for ApoE4. In this regard, a high-yield protocol was developed for the expression and purification of recombinant full-length ApoE, and three diverse biophysical screening assays were established and characterized; an optical label-free assay (Corning Epic) for hit identification and microscale thermophoresis (MST) and isothermal titration calorimetry (ITC) as orthogonal assays for hit confirmation. The 707 compounds in the National Institute of Health clinical collection were screened for binding to ApoE4, from which six confirmed hits, as well as one analogue, were identified. Although the compounds did not differentiate between ApoE isoforms, these data nevertheless demonstrate the feasibility of using a biophysical approach to identifying compounds that bind to ApoE and that, with further optimization, might differentiate between isoforms to produce a molecule that selectively alters the function of ApoE4. [ABSTRACT FROM AUTHOR]

Published

2019

26. Complexes of Pro-Apoptotic siRNAs and Carbosilane Dendrimers: Formation and Effect on Cancer Cells.

Author

Krasheninina, Olga A., Apartsin, Evgeny K., Fuentes, Elena, Szulc, Aleksandra, Ionov, Maksim, Venyaminova, Alya G., Shcharbin, Dzmitry, de la Mata, F. Javier, Bryszewska, Maria, and Gόmez, Rafael

Subjects

*DENDRIMERS, *NANOPARTICLES, *SMALL interfering RNA, *HELA cells, *APOPTOSIS

Abstract

This paper examines the complexation of anti-cancer small interfering RNAs (siRNAs) by cationic carbosilane dendrimers, and the interaction of the formed complexes with HeLa and HL-60 cancer cells. Stepwise formation of the complexes accompanied by the evolution of their properties has been observed through the increase of the charge ratio (dendrimer/siRNA). The complexes decrease the viability of both "easy-to-transfect" cells (HeLa) and "hard-to transfect" ones (HL-60), indicating a high potential of the cationic carbosilane dendrimers for siRNA delivery into tumor cells. [ABSTRACT FROM AUTHOR]

Published

2019

27. Using Microscale Thermophoresis to Characterize Hits from High-Throughput Screening: A European Lead Factory Perspective.

Author

Rainard JM, Pandarakalam GC, and McElroy SP

Subjects

Biophysics methods, Drug Design, Drug Discovery methods, Europe, Small Molecule Libraries chemistry, Temperature, Biological Assay methods, High-Throughput Screening Assays methods

Abstract

High-throughput screening (HTS) is a proven method for discovering new lead matter for drug discovery and chemical biology. To maximize the likelihood of identifying genuine binders to a molecular target, and avoid wasting resources following up compounds with unproductive/nonspecific mechanisms of action, it is important to employ a range of assays during an HTS campaign that build confidence of target engagement for hit compounds. Biophysical methods that measure direct target/compound engagement have established themselves as key techniques in generating this confidence, and they are now integral to the latter stages of HTS triage at the European Lead Factory (ELF). One relatively new technique that the ELF is using is microscale thermophoresis (MST), which measures the differences in rate of movement through a temperature gradient that are caused when single molecular species form complexes. Here we provide an overview of the MST assay development workflow that the ELF employs and a perspective of our experience to date of using MST to triage the output of HTS campaigns and how it compares and contrasts with the use of other biophysical techniques.

Published

2018