Your search keyword '"Cegarra C"' showing total 8 results

1. Additional file 3 of Exploring ITM2A as a new potential target for brain delivery

Author

Cegarra, C��line, Chaves, C., D��on, C., Do, T. M., Dumas, B., Frenzel, A., Kuhn, P., Roudieres, V., Guillemot, J. C., and Lesuisse, D.

Abstract

Additional file 3: Figure S3. Western Blot membranes of ITM2A relative quantification expression in new born mice. Signal was detected by antibody anti-ITM2A AF4876. HEK293 ITM2A mouse GFP is used as control. On the left a-tubulin T9026 detection on the right anti-ITM2A AF4876. Detection with primary antibody was followed by HRP coupled with appropriate antibody. Then, luminescence was quantified.

Published

2022

2. Additional file 4 of Exploring ITM2A as a new potential target for brain delivery

Author

Cegarra, C��line, Chaves, C., D��on, C., Do, T. M., Dumas, B., Frenzel, A., Kuhn, P., Roudieres, V., Guillemot, J. C., and Lesuisse, D.

Abstract

Additional file 4: Figure S4. Detection limit of mouse ITM2A by western blot in HEK293 overexpressing mITM2A. Signal is quantified with MultiGauge v3.0. Housekeeping protein is ��-tubulin in orange and protein of interest is ITM2A in blue.

Published

2022

3. Additional file 2 of Exploring ITM2A as a new potential target for brain delivery

Author

Cegarra, C��line, Chaves, C., D��on, C., Do, T. M., Dumas, B., Frenzel, A., Kuhn, P., Roudieres, V., Guillemot, J. C., and Lesuisse, D.

Abstract

Additional file 2: Figure S2. Western Blot membrane of relative quantification of ITM2A protein expression in different cells type. Signal was detected by antibody anti-ITM2A AF4876 followed by HRP coupled anti-sheep antibody. Then, luminescence was quantified.

Published

2022

4. Additional file 1 of Exploring ITM2A as a new potential target for brain delivery

Author

Cegarra, C��line, Chaves, C., D��on, C., Do, T. M., Dumas, B., Frenzel, A., Kuhn, P., Roudieres, V., Guillemot, J. C., and Lesuisse, D.

Subjects

food and beverages, human activities

Abstract

Additional file 1: Figure S1. Clonal selection of stable HEK293 overexpressing ITM2A. After fluorescence selection, better clones were confirmed by Western Blot. Clones with higher expression and higher luminescent signal were selected. Selected clones are circled in red. A HEK293 ITM2A human C-Ter and Nter GFP clone selection. B HEK293 ITM2A murin Nter GFP clone selection. C HEK293 ITM2A murin C-Ter GFP clone selection. D HEK293 ITM2A human C-Ter HA clone selection. E HEK293 ITM2A human N-Ter HA and WT clone selection.

Published

2022

5. An innovative strategy to identify new targets for delivering antibodies to the brain has led to the exploration of the integrin family.

Author

Cegarra C, Cameron B, Chaves C, Dabdoubi T, Do TM, Genêt B, Roudières V, Shi Y, Tchepikoff P, and Lesuisse D

Subjects

Activated-Leukocyte Cell Adhesion Molecule, Animals, Antibodies metabolism, Brain metabolism, Integrin beta1 metabolism, Mice, Endothelial Cells metabolism, Integrins metabolism

Abstract

Background: Increasing brain exposure of biotherapeutics is key to success in central nervous system disease drug discovery. Accessing the brain parenchyma is especially difficult for large polar molecules such as biotherapeutics and antibodies because of the blood-brain barrier. We investigated a new immunization strategy to identify novel receptors mediating transcytosis across the blood-brain barrier., Method: We immunized mice with primary non-human primate brain microvascular endothelial cells to obtain antibodies. These antibodies were screened for their capacity to bind and to be internalized by primary non-human primate brain microvascular endothelial cells and Human Cerebral Microvascular Endothelial Cell clone D3. They were further evaluated for their transcytosis capabilities in three in vitro blood-brain barrier models. In parallel, their targets were identified by two different methods and their pattern of binding to human tissue was investigated using immunohistochemistry., Results: 12 antibodies with unique sequence and internalization capacities were selected amongst more than six hundred. Aside from one antibody targeting Activated Leukocyte Cell Adhesion Molecule and one targeting Striatin3, most of the other antibodies recognized β1 integrin and its heterodimers. The antibody with the best transcytosis capabilities in all blood-brain barrier in vitro models and with the best binding capacity was an anti-αnβ1 integrin. In comparison, commercial anti-integrin antibodies performed poorly in transcytosis assays, emphasizing the originality of the antibodies derived here. Immunohistochemistry studies showed specific vascular staining on human and non-human primate tissues., Conclusions: This transcytotic behavior has not previously been reported for anti-integrin antibodies. Further studies should be undertaken to validate this new mechanism in vivo and to evaluate its potential in brain delivery., Competing Interests: All authors are Sanofi employees and may hold shares and/or stock options in the company This does not alter our adherence to PLOS ONE policies on sharing data and materials.

Published

2022

6. Exploring ITM2A as a new potential target for brain delivery.

Author

Cegarra C, Chaves C, Déon C, Do TM, Dumas B, Frenzel A, Kuhn P, Roudieres V, Guillemot JC, and Lesuisse D

Subjects

Animals, Blood-Brain Barrier metabolism, Brain metabolism, HEK293 Cells, Humans, Membrane Proteins metabolism, Mice, Endothelial Cells metabolism, Proteomics

Abstract

Background: Integral membrane protein 2A (ITM2A) is a transmembrane protein expressed in a variety of tissues; little is known about its function, particularly in the brain. ITM2A was found to be highly enriched in human brain versus peripheral endothelial cells by transcriptomic and proteomic studies conducted within the European Collaboration on the Optimization of Macromolecular Pharmaceutical (COMPACT) Innovative Medicines Initiative (IMI) consortium. Here, we report the work that was undertaken to determine whether ITM2A could represent a potential target for delivering drugs to the brain., Methods: A series of ITM2A constructs, cell lines and specific anti-human and mouse ITM2A antibodies were generated. Binding and internalization studies in Human Embryonic Kidney 293 (HEK293) cells overexpressing ITM2A and in brain microvascular endothelial cells from mouse and non-human primate (NHP) were performed with these tools. The best ITM2A antibody was evaluated in an in vitro human blood brain barrier (BBB) model and in an in vivo mouse pharmacokinetic study to investigate its ability to cross the BBB., Results: Antibodies specifically recognizing extracellular parts of ITM2A or tags inserted in its extracellular domain showed selective binding and uptake in ITM2A-overexpressing cells. However, despite high RNA expression in mouse and human microvessels, the ITM2A protein was rapidly downregulated when endothelial cells were grown in culture, probably explaining why transcytosis could not be observed in vitro. An attempt to directly demonstrate in vivo transcytosis in mice was inconclusive, using either a cross-reactive anti-ITM2A antibody or in vivo phage panning of an anti-ITM2A phage library., Conclusions: The present work describes our efforts to explore the potential of ITM2A as a target mediating transcytosis through the BBB, and highlights the multiple challenges linked to the identification of new brain delivery targets. Our data provide evidence that antibodies against ITM2A are internalized in ITM2A-overexpressing HEK293 cells, and that ITM2A is expressed in brain microvessels, but further investigations will be needed to demonstrate that ITM2A is a potential target for brain delivery., (© 2022. The Author(s).)

Published

2022

7. Non-Human Primate Blood-Brain Barrier and In Vitro Brain Endothelium: From Transcriptome to the Establishment of a New Model.

Author

Chaves C, Do TM, Cegarra C, Roudières V, Tolou S, Thill G, Rocher C, Didier M, and Lesuisse D

Abstract

The non-human primate (NHP)-brain endothelium constitutes an essential alternative to human in the prediction of molecule trafficking across the blood-brain barrier (BBB). This study presents a comparison between the NHP transcriptome of freshly isolated brain microcapillaries and in vitro-selected brain endothelial cells (BECs), focusing on important BBB features, namely tight junctions, receptors mediating transcytosis (RMT), ABC and SLC transporters, given its relevance as an alternative model for the molecule trafficking prediction across the BBB and identification of new brain-specific transport mechanisms. In vitro BECs conserved most of the BBB key elements for barrier integrity and control of molecular trafficking. The function of RMT via the transferrin receptor (TFRC) was characterized in this NHP-BBB model, where both human transferrin and anti-hTFRC antibody showed increased apical-to-basolateral passage in comparison to control molecules. In parallel, eventual BBB-related regional differences were investigated in seven-day in vitro-selected BECs from five brain structures: brainstem, cerebellum, cortex, hippocampus, and striatum. Our analysis retrieved few differences in the brain endothelium across brain regions, suggesting a rather homogeneous BBB function across the brain parenchyma. The presently established NHP-derived BBB model closely mimics the physiological BBB, thus representing a ready-to-use tool for assessment of the penetration of biotherapeutics into the human CNS., Competing Interests: All authors are Sanofi employees, and may hold shares and/or stock options in the company. The company had no role in the design of the study; in the collection, analyses, or interpretation of data; in the writing of the manuscript, or in the decision to publish the results. The authors declare no other conflict of interest.

Published

2020

8. Development of a novel NURR1/NOT agonist from hit to lead and candidate for the potential treatment of Parkinson's disease.

Author

Lesuisse D, Malanda A, Peyronel JF, Evanno Y, Lardenois P, De-Peretti D, Abécassis PY, Barnéoud P, Brunel P, Burgevin MC, Cegarra C, Auger F, Dommergue A, Lafon C, Even L, Tsi J, Luc TPH, Almario A, Olivier A, Castel MN, Taupin V, Rooney T, and Vigé X

Subjects

Animals, Cell Line, Cricetinae, Drug Discovery, Gene Expression Regulation drug effects, Homeodomain Proteins metabolism, Interleukin-1beta genetics, Interleukin-1beta metabolism, Mice, Microglia drug effects, Molecular Structure, Neurons drug effects, Nuclear Receptor Subfamily 4, Group A, Member 2 genetics, Rats, Retinoid X Receptors genetics, Retinoid X Receptors metabolism, Neuroprotective Agents chemical synthesis, Neuroprotective Agents pharmacology, Nuclear Receptor Subfamily 4, Group A, Member 2 metabolism, Parkinson Disease drug therapy

Abstract

In the course of a programme aimed at identifying Nurr1/NOT agonists for potential treatment of Parkinson's disease, a few hits from high throughput screening were identified and characterized. A combined optimization pointed to a very narrow and stringent structure activity relationship. A comprehensive program of optimization led to a potent and safe candidate drug displaying neuroprotective and anti-inflammatory activity in several in vitro and in vivo models., (Copyright © 2019 Elsevier Ltd. All rights reserved.)

Published

2019