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113 results on '"Federation of European Biochemical Societies"'

4. Metallothionein‑3 promotes cisplatin chemoresistance remodelling in neuroblastoma

Author

European Commission, Czech Health Research Council, Czech Science Foundation, Federation of European Biochemical Societies, Ministry of Education, Youth and Sports (Czech Republic), Merlos Rodrigo, Miguel Angel [0000-0002-1920-0948], Strmiska, Vladislav [0000-0002-7036-1640], Casar, Berta [0000-0002-3058-5631], Crespo, Piero [0000-0003-2825-7783], de los Ríos, Vivian [0000-0001-5582-6879], Casal, J. Ignacio [0000-0003-1085-2840], Haddad, Yazan [0000-0002-7844-4336], Guran, Roman [0000-0002-2912-714X], Adam, Vojtech [0000-0002-8527-286X], Merlos Rodrigo, Miguel Angel, Michalkova, Hana, Strmiska, Vladislav, Casar, Berta, Crespo, Piero, Ríos, Vivian de los, Casal, J. Ignacio, Haddad, Yazan, Guran, Roman, Eckschlager, Tomas, Pokorná, Petra, Heger, Z., Adam, Vojtech, European Commission, Czech Health Research Council, Czech Science Foundation, Federation of European Biochemical Societies, Ministry of Education, Youth and Sports (Czech Republic), Merlos Rodrigo, Miguel Angel [0000-0002-1920-0948], Strmiska, Vladislav [0000-0002-7036-1640], Casar, Berta [0000-0002-3058-5631], Crespo, Piero [0000-0003-2825-7783], de los Ríos, Vivian [0000-0001-5582-6879], Casal, J. Ignacio [0000-0003-1085-2840], Haddad, Yazan [0000-0002-7844-4336], Guran, Roman [0000-0002-2912-714X], Adam, Vojtech [0000-0002-8527-286X], Merlos Rodrigo, Miguel Angel, Michalkova, Hana, Strmiska, Vladislav, Casar, Berta, Crespo, Piero, Ríos, Vivian de los, Casal, J. Ignacio, Haddad, Yazan, Guran, Roman, Eckschlager, Tomas, Pokorná, Petra, Heger, Z., and Adam, Vojtech

Abstract

Metallothionein-3 has poorly characterized functions in neuroblastoma. Cisplatin-based chemotherapy is a major regimen to treat neuroblastoma, but its clinical efficacy is limited by chemoresistance. We investigated the impact of human metallothionein-3 (hMT3) up-regulation in neuroblastoma cells and the mechanisms underlying the cisplatin-resistance. We confirmed the cisplatin-metallothionein complex formation using mass spectrometry. Overexpression of hMT3 decreased the sensitivity of neuroblastoma UKF-NB-4 cells to cisplatin. We report, for the first time, cisplatin-sensitive human UKF-NB-4 cells remodelled into cisplatin-resistant cells via high and constitutive hMT3 expression in an in vivo model using chick chorioallantoic membrane assay. Comparative proteomic analysis demonstrated that several biological pathways related to apoptosis, transport, proteasome, and cellular stress were involved in cisplatin-resistance in hMT3 overexpressing UKF-NB-4 cells. Overall, our data confirmed that up-regulation of hMT3 positively correlated with increased cisplatin-chemoresistance in neuroblastoma, and a high level of hMT3 could be one of the causes of frequent tumour relapses.

Published
2021

5. CTCF knockout in zebrafish induces alterations in regulatory landscapes and developmental gene expression

Author

European Commission, Ministerio de Economía y Competitividad (España), Fundación BBVA, Federation of European Biochemical Societies, Junta de Andalucía, Franke, Martin, Calle-Mustienes, Elisa de la, Neto, Ana, Almuedo-Castillo, María, Irastorza-Azcárate, Ibai, Acemel, Rafael D., Tena, Juan J., Santos-Pereira, José M., Gómez-Skarmeta, José Luis, European Commission, Ministerio de Economía y Competitividad (España), Fundación BBVA, Federation of European Biochemical Societies, Junta de Andalucía, Franke, Martin, Calle-Mustienes, Elisa de la, Neto, Ana, Almuedo-Castillo, María, Irastorza-Azcárate, Ibai, Acemel, Rafael D., Tena, Juan J., Santos-Pereira, José M., and Gómez-Skarmeta, José Luis

Abstract

Coordinated chromatin interactions between enhancers and promoters are critical for gene regulation. The architectural protein CTCF mediates chromatin looping and is enriched at the boundaries of topologically associating domains (TADs), which are sub-megabase chromatin structures. In vitro CTCF depletion leads to a loss of TADs but has only limited effects over gene expression, challenging the concept that CTCF-mediated chromatin structures are a fundamental requirement for gene regulation. However, how CTCF and a perturbed chromatin structure impacts gene expression during development remains poorly understood. Here we link the loss of CTCF and gene regulation during patterning and organogenesis in a ctcf knockout zebrafish model. CTCF absence leads to loss of chromatin structure and affects the expression of thousands of genes, including many developmental regulators. Our results demonstrate the essential role of CTCF in providing the structural context for enhancer-promoter interactions, thus regulating developmental genes.

Published
2021

6. Extending the applicability of In Ovo and Ex Ovo chicken chorioallantoic membrane assays to study cytostatic activity in neuroblastoma cells

Author

European Research Council, Czech Science Foundation, European Commission, Federation of European Biochemical Societies, Ministry of Education, Youth and Sports (Czech Republic), Ministerio de Ciencia, Innovación y Universidades (España), Agencia Estatal de Investigación (España), Merlos Rodrigo, Miguel Angel, Casar, Berta, Michalkova, Hana, Jiménez Jiménez, Ana María, Heger, Zbynek, Adam, Vojtech, European Research Council, Czech Science Foundation, European Commission, Federation of European Biochemical Societies, Ministry of Education, Youth and Sports (Czech Republic), Ministerio de Ciencia, Innovación y Universidades (España), Agencia Estatal de Investigación (España), Merlos Rodrigo, Miguel Angel, Casar, Berta, Michalkova, Hana, Jiménez Jiménez, Ana María, Heger, Zbynek, and Adam, Vojtech

Abstract

[Purpose]: The chick chorioallantoic membrane (CAM) assay can provide an alternative versatile, cost-effective, and ethically less controversial in vivo model for reliable screening of drugs. In the presented work, we demonstrate that CAM assay (in ovo and ex ovo) can be simply employed to delineate the effects of cisplatin (CDDP) and ellipticine (Elli) on neuroblastoma (Nbl) cells in terms of their growth and metastatic potential. [Methods]: The Nbl UKF-NB-4 cell line was established from recurrent bone marrow metastases of high-risk Nbl (stage IV, MYCN amplification, 7q21 gain). Ex ovo and in ovo CAM assays were optimized to evaluate the antimetastatic activity of CDDP and Elli. Immunohistochemistry, qRT-PCR, and DNA isolation were performed. [Results]: Ex ovo CAM assay was employed to study whether CDDP and Elli exhibit any inhibitory effects on growth of Nbl xenograft in ex ovo CAM assay. Under the optimal conditions, Elli and CDDP exhibited significant inhibition of the size of the primary tumor. To study the efficiency of CDDP and Elli to inhibit primary Nbl tumor growth, intravasation, and extravasation in the organs, we adapted the in ovo CAM assay protocol. In in ovo CAM assay, both studied compounds (CDDP and Elli) exhibited significant (p < 0.001) inhibitory activity against extravasation to all investigated organs including distal CAM. [Conclusions]: Taken together, CAM assay could be a helpful and highly efficient in vivo approach for high-throughput screening of libraries of compounds with expected anticancer activities.

Published
2021

7. gNOMO: a multi-omics pipeline for integrated host and microbiome analysis of non-model organisms

Author

European Commission, Agencia Estatal de Investigación (España), Ministerio de Ciencia, Innovación y Universidades (España), German Research Foundation, Generalitat Valenciana, Research Foundation - Flanders, Federation of European Biochemical Societies, Muñoz-Benavent, Maria, Hartkopf, Felix, Van Den Bossche, Tim, Piro, Vitor C., García-Ferris, Carlos, Latorre, Amparo, Renard, Bernhard Y., Muth, Thilo, European Commission, Agencia Estatal de Investigación (España), Ministerio de Ciencia, Innovación y Universidades (España), German Research Foundation, Generalitat Valenciana, Research Foundation - Flanders, Federation of European Biochemical Societies, Muñoz-Benavent, Maria, Hartkopf, Felix, Van Den Bossche, Tim, Piro, Vitor C., García-Ferris, Carlos, Latorre, Amparo, Renard, Bernhard Y., and Muth, Thilo

Abstract

The study of bacterial symbioses has grown exponentially in the recent past. However, existing bioinformatic workflows of microbiome data analysis do commonly not integrate multiple meta-omics levels and are mainly geared toward human microbiomes. Microbiota are better understood when analyzed in their biological context; that is together with their host or environment. Nevertheless, this is a limitation when studying non-model organisms mainly due to the lack of well-annotated sequence references. Here, we present gNOMO, a bioinformatic pipeline that is specifically designed to process and analyze non-model organism samples of up to three meta-omics levels: metagenomics, metatranscriptomics and metaproteomics in an integrative manner. The pipeline has been developed using the workflow management framework Snakemake in order to obtain an automated and reproducible pipeline. Using experimental datasets of the German cockroach Blattella germanica, a non-model organism with very complex gut microbiome, we show the capabilities of gNOMO with regard to meta-omics data integration, expression ratio comparison, taxonomic and functional analysis as well as intuitive output visualization. In conclusion, gNOMO is a bioinformatic pipeline that can easily be configured, for integrating and analyzing multiple meta-omics data types and for producing output visualizations, specifically designed for integrating paired-end sequencing data with mass spectrometry from non-model organisms.

Published
2020

8. Differential Interactome and Innate Immune Response Activation of Two Structurally Distinct Misfolded Protein Oligomers

Author

Agencia Estatal de Investigación (España), Federation of European Biochemical Societies, EMBO, Società Italiana di Biochimica e Biologia Molecolare, Ministerio de Economía y Competitividad (España), Instituto de Salud Carlos III, Ministerio de Ciencia, Innovación y Universidades (España), Universidad de Sevilla, University of Cambridge, Mannini, Benedetta, Vecchi, Giulia, Labrador-Garrido, Adahir, Fabre, Bertrand, Fani, Giulia, Franco, Jaime M., Lilley, Kathryn, Pozo, David, Vendruscolo, Michele, Chiti, Fabrizio, Dobson, Christopher M., Roodveldt, Cintia, Agencia Estatal de Investigación (España), Federation of European Biochemical Societies, EMBO, Società Italiana di Biochimica e Biologia Molecolare, Ministerio de Economía y Competitividad (España), Instituto de Salud Carlos III, Ministerio de Ciencia, Innovación y Universidades (España), Universidad de Sevilla, University of Cambridge, Mannini, Benedetta, Vecchi, Giulia, Labrador-Garrido, Adahir, Fabre, Bertrand, Fani, Giulia, Franco, Jaime M., Lilley, Kathryn, Pozo, David, Vendruscolo, Michele, Chiti, Fabrizio, Dobson, Christopher M., and Roodveldt, Cintia

Abstract

The formation of misfolded protein oligomers during early stages of amyloid aggregation and the activation of neuroinflammatory responses are two key events associated with neurodegenerative diseases. Although it has been established that misfolded oligomers are involved in the neuroinflammatory process, the links between their structural features and their functional effects on the immune response remain unknown. To explore such links, we took advantage of two structurally distinct soluble oligomers (type A and B) of protein HypF-N and compared the elicited microglial inflammatory responses. By using confocal microscopy, protein pull-down, and high-throughput mass spectrometry, we found that, even though both types bound to a common pool of microglial proteins, type B oligomers - with a lower solvent-exposed hydrophobicity - showed enhanced protein binding, correlating with the observed inflammatory response. Furthermore, the interactome associated with inflammatory-mediated neurodegeneration revealed previously unidentified receptors and signaling molecules likely to be involved in the oligomer-elicited innate immune response.

Published
2019

9. Compartmentalization of ER-bound chaperone confines protein deposit formation to the aging yeast cell

Author

European Commission, Federation of European Biochemical Societies, Finnish Cultural Foundation, Federal Institute of Technology Zurich, Saarikangas, Juha, Caudron, Fabrice, Prasad, Rupali, Moreno, David F., Bolognesi, Alessio, Aldea, Marti, Barral, Yves, European Commission, Federation of European Biochemical Societies, Finnish Cultural Foundation, Federal Institute of Technology Zurich, Saarikangas, Juha, Caudron, Fabrice, Prasad, Rupali, Moreno, David F., Bolognesi, Alessio, Aldea, Marti, and Barral, Yves

Abstract

In order to produce rejuvenated daughters, dividing budding yeast cells confine aging factors, including protein aggregates, to the aging mother cell. The asymmetric inheritance of these protein deposits is mediated by organelle and cytoskeletal attachment and by cell geometry. Yet it remains unclear how deposit formation is restricted to the aging lineage. Here, we show that selective membrane anchoring and the compartmentalization of the endoplasmic reticulum (ER) membrane confine protein deposit formation to aging cells during division. Supporting the idea that the age-dependent deposit forms through coalescence of smaller aggregates, two deposits rapidly merged when placed in the same cell by cell-cell fusion. The deposits localized to the ER membrane, primarily to the nuclear envelope (NE). Strikingly, weakening the diffusion barriers that separate the ER membrane into mother and bud compartments caused premature formation of deposits in the daughter cells. Detachment of the Hsp40 protein Ydj1 from the ER membrane elicited a similar phenotype, suggesting that the diffusion barriers and farnesylated Ydj1 functioned together to confine protein deposit formation to mother cells during division. Accordingly, fluorescence correlation spectroscopy measurements in dividing cells indicated that a slow-diffusing, possibly client-bound Ydj1 fraction was asymmetrically enriched in the mother compartment. This asymmetric distribution depended on Ydj1 farnesylation and intact diffusion barriers. Taking these findings together, we propose that ER-anchored Ydj1 binds deposit precursors and prevents them from spreading into daughter cells during division by subjecting them to the ER diffusion barriers. This ensures that the coalescence of precursors into a single deposit is restricted to the aging lineage.

Published
2017

10. Role of cannabinoid receptor CB2 in HER2 pro-oncogenic signaling in breast cancer

Author

Comunidad de Madrid, GW Pharmaceuticals, Fundación Mutua Madrileña, Centro de Investigación Biomédica en Red Enfermedades Raras (España), Fundación Científica Asociación Española Contra el Cáncer, Federation of European Biochemical Societies, European Commission, Ministerio de Economía y Competitividad (España), Instituto de Salud Carlos III, Pérez-Gómez, Eduardo, Andradas, Clara, Caffarel, María M., Villa-Morales, María, Martín-Villar, Ester, Flores, Juana María, Megías, Diego, Moreno-Bueno, Gema, Quintanilla, Miguel, Fernández-Piqueras, José, Sánchez, Cristina, Comunidad de Madrid, GW Pharmaceuticals, Fundación Mutua Madrileña, Centro de Investigación Biomédica en Red Enfermedades Raras (España), Fundación Científica Asociación Española Contra el Cáncer, Federation of European Biochemical Societies, European Commission, Ministerio de Economía y Competitividad (España), Instituto de Salud Carlos III, Pérez-Gómez, Eduardo, Andradas, Clara, Caffarel, María M., Villa-Morales, María, Martín-Villar, Ester, Flores, Juana María, Megías, Diego, Moreno-Bueno, Gema, Quintanilla, Miguel, Fernández-Piqueras, José, and Sánchez, Cristina

Abstract

[Background]: Pharmacological activation of cannabinoid receptors elicits antitumoral responses in different cancer models. However, the biological role of these receptors in tumor physio-pathology is still unknown. [Methods]: We analyzed CB2 cannabinoid receptor protein expression in two series of 166 and 483 breast tumor samples operated in the University Hospitals of Kiel, Tübingen, and Freiburg between 1997 and 2010 and CB2 mRNA expression in previously published DNA microarray datasets. The role of CB2 in oncogenesis was studied by generating a mouse line that expresses the human V-Erb-B2 Avian Erythroblastic Leukemia Viral Oncogene Homolog 2 (HER2) rat ortholog (neu) and lacks CB2 and by a variety of biochemical and cell biology approaches in human breast cancer cells in culture and in vivo, upon modulation of CB2 expression by si/shRNAs and overexpression plasmids. CB2-HER2 molecular interaction was studied by colocalization, coimmunoprecipitation, and proximity ligation assays. Statistical tests were two-sided. [Results]: We show an association between elevated CB2 expression in HER2+ breast tumors and poor patient prognosis (decreased overall survival, hazard ratio [HR] = 0.29, 95% confidence interval [CI] = 0.09 to 0.71, P = .009) and higher probability to suffer local recurrence (HR = 0.09, 95% CI = 0.049 to 0.54, P = .003) and to develop distant metastases (HR = 0.33, 95% CI = 0.13 to 0.75, P = .009). We also demonstrate that genetic inactivation of CB2 impairs tumor generation and progression in MMTV-neu mice. Moreover, we show that HER2 upregulates CB2 expression by activating the transcription factor ELK1 via the ERK cascade and that an increased CB2 expression activates the HER2 pro-oncogenic signaling at the level of the tyrosine kinase c-SRC. Finally, we show HER2 and CB2 form heteromers in cancer cells. [Conclusions]: Our findings reveal an unprecedented role of CB2 as a pivotal regulator of HER2 pro-oncogenic signaling in breast cancer, and they

Published
2015

11. Structure of the yeast mitochondrial large ribosomal subunit

Author

Medical Research Council (UK), Agouron Institute, Louis Jeantet Foundation, European Research Council, Human Frontier Science Program, Federation of European Biochemical Societies, Llácer, José Luis [0000-0001-5304-1795], Amunts, Alexey, Brown, Alan, Bai, Xiao-chen, Llácer, José Luis, Hussain, Tanweer, Emsley, Paul, Long, Fei, Murshudov, Garib, Scheres, Sjors H.W., Ramakrishnan, V., Medical Research Council (UK), Agouron Institute, Louis Jeantet Foundation, European Research Council, Human Frontier Science Program, Federation of European Biochemical Societies, Llácer, José Luis [0000-0001-5304-1795], Amunts, Alexey, Brown, Alan, Bai, Xiao-chen, Llácer, José Luis, Hussain, Tanweer, Emsley, Paul, Long, Fei, Murshudov, Garib, Scheres, Sjors H.W., and Ramakrishnan, V.

Abstract

Mitochondria have specialized ribosomes that have diverged from their bacterial and cytoplasmic counterparts. We have solved the structure of the yeast mitoribosomal large subunit using single-particle cryo-electron microscopy. The resolution of 3.2 angstroms enabled a nearly complete atomic model to be built de novo and refined, including 39 proteins, 13 of which are unique to mitochondria, as well as expansion segments of mitoribosomal RNA. The structure reveals a new exit tunnel path and architecture, unique elements of the E site, and a putative membrane docking site.

Published
2014

12. VARP is recruited on to endosomes by direct interaction with retromer, where together they function in export to the cell surface

Author

Canadian Institutes of Health Research, Federation of European Biochemical Societies, European Molecular Biology Laboratory, Medical Research Council (UK), Wellcome Trust, Engineering and Physical Sciences Research Council (UK), Cambridge Biomedical Research Centre, ., Hesketh, Geoffrey G., Pérez-Dorado, Inmaculada, Jackson, Lauren P., Wartosch, Lena, Schäfer, Ingmar B., Gray, Sally R., McCoy, Airlie J., Zeldin, Oliver B., Garman, Elspeth F., Harbour, Michael E., Evans, Philip R., Seaman, Matthew N. J., Luzio, J. Paul, Owen, David J., Canadian Institutes of Health Research, Federation of European Biochemical Societies, European Molecular Biology Laboratory, Medical Research Council (UK), Wellcome Trust, Engineering and Physical Sciences Research Council (UK), Cambridge Biomedical Research Centre, ., Hesketh, Geoffrey G., Pérez-Dorado, Inmaculada, Jackson, Lauren P., Wartosch, Lena, Schäfer, Ingmar B., Gray, Sally R., McCoy, Airlie J., Zeldin, Oliver B., Garman, Elspeth F., Harbour, Michael E., Evans, Philip R., Seaman, Matthew N. J., Luzio, J. Paul, and Owen, David J.

Abstract

VARP is a Rab32/38 effector that also binds to the endosomal/lysosomal R-SNARE VAMP7. VARP binding regulates VAMP7 participation in SNARE complex formation and can therefore influence VAMP7-mediated membrane fusion events. Mutant versions of VARP that cannot bind Rab32:GTP, designed on the basis of the VARP ankyrin repeat/Rab32:GTP complex structure described here, unexpectedly retain endosomal localization, showing that VARP recruitment is not dependent on Rab32 binding. We show that recruitment of VARP to the endosomal membrane is mediated by its direct interaction with VPS29, a subunit of the retromer complex, which is involved in trafficking from endosomes to the TGN and the cell surface. Transport of GLUT1 from endosomes to the cell surface requires VARP, VPS29, and VAMP7 and depends on the direct interaction between VPS29 and VARP. Finally, we propose that endocytic cycling of VAMP7 depends on its interaction with VARP and, consequently, also on retromer.

Published
2014

13. BRAF inhibitors induce metastasis in RAS mutant or inhibitor-resistant melanoma cells by reactivating MEK and ERK signaling

Author

Cancer Research UK, European Commission, Wenner-Gren Foundation, Federation of European Biochemical Societies, National Health Service (UK), Lloyd's Register Foundation, International Agency for Research on Cancer, Manchester Biomedical Research Centre, Royal Marsden NHS Foundation Trust, Sánchez-Laorden, Berta, Viros, Amaya, Girotti, Maria Romina, Pedersen, Malin, Saturno, Grazia, Zambon, Alfonso, Niculescu-Duvaz, Dan, Turajlic, Samra, Hayes, Andrew, Gore, Martin, Larkin, James, Lorigan, Paul, Cook, Martin, Springer, Caroline, Marais, Richard, Cancer Research UK, European Commission, Wenner-Gren Foundation, Federation of European Biochemical Societies, National Health Service (UK), Lloyd's Register Foundation, International Agency for Research on Cancer, Manchester Biomedical Research Centre, Royal Marsden NHS Foundation Trust, Sánchez-Laorden, Berta, Viros, Amaya, Girotti, Maria Romina, Pedersen, Malin, Saturno, Grazia, Zambon, Alfonso, Niculescu-Duvaz, Dan, Turajlic, Samra, Hayes, Andrew, Gore, Martin, Larkin, James, Lorigan, Paul, Cook, Martin, Springer, Caroline, and Marais, Richard

Abstract

Melanoma is a highly metastatic and lethal form of skin cancer. The protein kinase BRAF is mutated in about 40% of melanomas, and BRAF inhibitors improve progression-free and overall survival in these patients. However, after a relatively short period of disease control, most patients develop resistance because of reactivation of the RAF-ERK (extracellular signal-regulated kinase) pathway, mediated in many cases by mutations in RAS. We found that BRAF inhibition induces invasion and metastasis in RAS mutant melanoma cells through a mechanism mediated by the reactivation of the MEK (mitogen-activated protein kinase kinase)-ERK pathway, increased expression and secretion of interleukin 8, and induction of protease-dependent invasion. These events were accompanied by a cell morphology switch from predominantly rounded to predominantly elongated cells. We also observed similar responses in BRAF inhibitor-resistant melanoma cells. These data show that BRAF inhibitors can induce melanoma cell invasion and metastasis in tumors that develop resistance to these drugs.

Published
2014

14. Histamine production by human neutrophils

Author

Junta de Andalucía, Fundación de la Sociedad Española de Alergia e Inmunología Clínica, Instituto de Salud Carlos III, Red de Investigación de Reacciones Adversas a Alérgenos y Fármacos (España), Fundación Alergol, Ministerio de Ciencia y Tecnología (España), Federation of European Biochemical Societies, Ministerio de Educación y Ciencia (España), Marie Curie Fellows Association, Alcañiz, Lorena, Vega, Antonio, Chacón, Pedro J., El Bekay, Rajaa, Ventura, Inmaculada, Aroca, Rocío, Blanca, Miguel, Bergstralh, Dan T., Monteseirín, Javier, Junta de Andalucía, Fundación de la Sociedad Española de Alergia e Inmunología Clínica, Instituto de Salud Carlos III, Red de Investigación de Reacciones Adversas a Alérgenos y Fármacos (España), Fundación Alergol, Ministerio de Ciencia y Tecnología (España), Federation of European Biochemical Societies, Ministerio de Educación y Ciencia (España), Marie Curie Fellows Association, Alcañiz, Lorena, Vega, Antonio, Chacón, Pedro J., El Bekay, Rajaa, Ventura, Inmaculada, Aroca, Rocío, Blanca, Miguel, Bergstralh, Dan T., and Monteseirín, Javier

Abstract

Histamine is an important mediator in the development of allergic reactions. Only a small subset of human cell types is able to produce histamine. No previous studies have shown that human neutrophils are among them. The present work was undertaken to analyze whether human neutrophils produce histamine, and to determine what agonists are involved in histamine production by human neutrophils. The expression of histidine decarboxylase in human neutrophils was established by quantitative PCR, Western blotting, and flow cytometry analysis. The activity of the enzyme was determined by ELISA, which measured histamine in the culture supernatant of neutrophils stimulated with a set of classical agonists. Human neutrophils are bona fide histamine-producing cells. Neutrophils store ∼0.29 pg/cell and release ∼50% of the histamine content in an antigen-dependent manner and on stimulation with other neutrophil agonists. Basal expression of histidine decarboxylase, the rate-limiting enzyme in histamine production, is higher in neutrophils from patients with allergies than from healthy donors. Our results cannot be ascribed to cell contamination for several reasons. LPS failed to induce histamine release by basophils, whereas it induced histamine release by neutrophils; and we did not detect basophils, monocytes, or lymphocytes in our neutrophil preparations. Eosinophils, albeit detected, were only 0.001-0.004% of the final cell population, and they did not store or release histamine on antigen or LPS stimulation. Antigens to which patients with allergies were sensitized stimulated release of histamine from neutrophils. These observations represent a novel view of neutrophils as possible source of histamine in the allergic diseases. © FASEB.

Published
2013

15. A genetic progression model of BrafV600E-induced intestinal tumorigenesis reveals targets for therapeutic intervention

Author

Wellcome Trust, Helmholtz Association, German Research Foundation, Federation of European Biochemical Societies, Human Frontier Science Program, Rad, Roland, Varela, Ignacio, Calvanese, Vincenzo, Bradley, Allan, Wellcome Trust, Helmholtz Association, German Research Foundation, Federation of European Biochemical Societies, Human Frontier Science Program, Rad, Roland, Varela, Ignacio, Calvanese, Vincenzo, and Bradley, Allan

Abstract

We show that BRAFV600E initiates an alternative pathway to colorectal cancer (CRC), which progresses through a hyperplasia/adenoma/carcinoma sequence. This pathway underlies significant subsets of CRCs with distinctive pathomorphologic/genetic/epidemiologic/clinical characteristics. Genetic and functional analyses in mice revealed a series of stage-specific molecular alterations driving different phases of tumor evolution and uncovered mechanisms underlying this stage specificity. We further demonstrate dose-dependent effects of oncogenic signaling, with physiologic BrafV600E expression being sufficient for hyperplasia induction, but later stage intensified Mapk-signaling driving both tumor progression and activation of intrinsic tumor suppression. Such phenomena explain, for example, the inability of p53 to restrain tumor initiation as well as its importance in invasiveness control, and the late stage specificity of its somatic mutation. Finally, systematic drug screening revealed sensitivity of this CRC subtype to targeted therapeutics, including Mek or combinatorial PI3K/Braf inhibition. © 2013 Elsevier Inc.

Published
2013

16. A rationally designed six-residue swap generates comparability in the aggregation behavior of α-synuclein and β-synuclein

Author

Wellcome Trust, Leverhulme Trust, EMBO, Royal Society (UK), Ministerio de Sanidad, Servicios Sociales e Igualdad (España), Instituto de Salud Carlos III, European Commission, Federation of European Biochemical Societies, Ministerio de Ciencia e Innovación (España), Roodveldt, Cintia, Labrador-Garrido, Adahir, Dobson, Christopher M., Vendruscolo, Michele, Wellcome Trust, Leverhulme Trust, EMBO, Royal Society (UK), Ministerio de Sanidad, Servicios Sociales e Igualdad (España), Instituto de Salud Carlos III, European Commission, Federation of European Biochemical Societies, Ministerio de Ciencia e Innovación (España), Roodveldt, Cintia, Labrador-Garrido, Adahir, Dobson, Christopher M., and Vendruscolo, Michele

Abstract

The aggregation process of α-synuclein, a protein closely associated with Parkinson's disease, is highly sensitive to sequence variations. It is therefore of great importance to understand the factors that define the aggregation propensity of specific mutational variants as well as their toxic behavior in the cellular environment. In this context, we investigated the extent to which the aggregation behavior of α-synuclein can be altered to resemble that of β-synuclein, an aggregation-resistant homologue of α-synuclein not associated with disease, by swapping residues between the two proteins. Because of the vast number of possible swaps, we have applied a rational design procedure to single out a mutational variant, called α2β, in which two short stretches of the sequence in the NAC region have been replaced in α-synuclein from β-synuclein. We find not only that the aggregation rate of α2β is close to that of β-synuclein, being much lower than that of α-synuclein, but also that α2β effectively changes the cellular toxicity of α-synuclein to a value similar to that of β-synuclein upon exposure of SH-SY5Y cells to preformed oligomers. Remarkably, control experiments on the corresponding mutational variant of β-synuclein, called β2α, confirmed that the mutations that we have identified also shift the aggregation behavior of this protein toward that of α-synuclein. These results demonstrate that it is becoming possible to control in quantitative detail the sequence code that defines the aggregation behavior and toxicity of α-synuclein. © 2012 American Chemical Society.

Published
2012

17. Sequence determinants of a microtubule tip localization signal (MtLS)

Author

Swiss National Science Foundation, European Commission, Federation of European Biochemical Societies, EMBO, Ministerio de Ciencia e Innovación (España), Martínez Buey, Rubén, Pereda, José M. de, Steinmetz, Michel O., Swiss National Science Foundation, European Commission, Federation of European Biochemical Societies, EMBO, Ministerio de Ciencia e Innovación (España), Martínez Buey, Rubén, Pereda, José M. de, and Steinmetz, Michel O.

Abstract

Microtubule plus-end-tracking proteins (+TIPs) specifically localize to the growing plus-ends of microtubules to regulate microtubule dynamics and functions. A large group of +TIPs contain a short linear motif, SXIP, which is essential for them to bind to end-binding proteins (EBs) and target microtubule ends. The SXIP sequence site thus acts as a widespread microtubule tip localization signal (MtLS). Here we have analyzed the sequence-function relationship of a canonical MtLS. Using synthetic peptide arrays on membrane supports, we identified the residue preferences at each amino acid position of the SXIP motif and its surrounding sequence with respect to EB binding. We further developed an assay based on fluorescence polarization to assess the mechanism of the EB-SXIP interaction and to correlate EB binding and microtubule tip tracking of MtLS sequences from different +TIPs. Finally, we investigated the role of phosphorylation in regulating the EB-SXIP interaction. Together, our results define the sequence determinants of a canonical MtLS and provide the experimental data for bioinformatics approaches to carry out genome-wide predictions of novel +TIPs in multiple organisms.

Published
2012

18. Sumoylation regulates nuclear localization of repressor DREAM

Author

Ministerio de Ciencia e Innovación (España), Centro Investigación Biomédica en Red Enfermedades Neurodegenerativas (España), Comunidad de Madrid, Fundació La Marató de TV3, Fundación la Caixa, Federation of European Biochemical Societies, Palczewska, Małgorzata, Casafont, Íñigo, Ghimire, Kedar, Rojas Mendoza, Ana M., Valencia, Alfonso, Lafarga, Miguel, Mellström, Britt, Naranjo, José Ramón, Ministerio de Ciencia e Innovación (España), Centro Investigación Biomédica en Red Enfermedades Neurodegenerativas (España), Comunidad de Madrid, Fundació La Marató de TV3, Fundación la Caixa, Federation of European Biochemical Societies, Palczewska, Małgorzata, Casafont, Íñigo, Ghimire, Kedar, Rojas Mendoza, Ana M., Valencia, Alfonso, Lafarga, Miguel, Mellström, Britt, and Naranjo, José Ramón

Abstract

DREAM is a Ca2+-binding protein with specific functions in different cell compartments. In the nucleus, DREAM acts as a transcriptional repressor, although the mechanism that controls its nuclear localization is unknown. Yeast two-hybrid assay revealed the interaction between DREAM and the SUMO-conjugating enzyme Ubc9 and bioinformatic analysis identified four sumoylation-susceptible sites in the DREAM sequence. Single K-to-R mutations at positions K26 and K90 prevented in vitro sumoylation of recombinant DREAM. DREAM sumoylation mutants retained the ability to bind to the DRE sequence but showed reduced nuclear localization and failed to regulate DRE-dependent transcription. In PC12 cells, sumoylated DREAM is present exclusively in the nucleus and neuronal differentiation induced nuclear accumulation of sumoylated DREAM. In fully differentiated trigeminal neurons, DREAM and SUMO-1 colocalized in nuclear domains associated with transcription. Our results show that sumoylation regulates the nuclear localization of DREAM in differentiated neurons. This article is part of a Special Issue entitled: 11th European Symposium on Calcium.

Published
2011

19. Directed evolution of a DD-Peptidase into a Beta-lactamase

Author

UCL - SST/ISV - Institut des sciences de la vie, UCL - SST/IMCN - Institute of Condensed Matter and Nanosciences, Trabelsi, Heykel, Soumillion, Patrice, 35th Congress of the Federation-of-European-Biochemical-Societies, UCL - SST/ISV - Institut des sciences de la vie, UCL - SST/IMCN - Institute of Condensed Matter and Nanosciences, Trabelsi, Heykel, Soumillion, Patrice, and 35th Congress of the Federation-of-European-Biochemical-Societies

Published
2010

20. beta/delta-Agatoxins are unique modulators of voltage-gated sodium channels

Author

UCL - Autre, Nikolsky, A., Billen, B., Vassilevski, A., Tytgat, J., Grishin, E., 35th Congress of the Federation-of-European-Biochemical-Societies, UCL - Autre, Nikolsky, A., Billen, B., Vassilevski, A., Tytgat, J., Grishin, E., and 35th Congress of the Federation-of-European-Biochemical-Societies

Abstract

Search of natural polypeptide molecules that affect the nervous systems of humans and animals with high selectivity and efficiency is one of the most important tasks of modern biochemistry and therefore has practical value to pharmacy, medicine and biotechnology. This work is devoted to identification and investigation of a new family of peptide components from Agelena orientalis (Agelenidae) spider venom designated b/d-agatoxins that modulate the activity of insect sodium channels. Complete amino acid sequences of all peptides (36– 38 residues) were established by automated Edman degradation. Purified toxins are characterized by a high degree of similarity with each other (up to 97%) and with some other toxins such as l-agatoxins, curtatoxins and d-palutoxins. b/d-Agatoxins were tested on Xenopus laevis oocytes expressing genes of insect sodium channel proteins using the two-electrode voltage clamp technique. Application of all studied compounds at concentrations of ~ 100 nM evoked a modulating effect on the fruit fly Drosophila melanogaster voltage-gated sodium channels (DmNav1), i.e. inhibition of inactivation (the socalled a-effect) and a shift of channel activation voltage dependence (b-effect). This peculiar ‘double’ effect of polypeptide toxins on sodium channels can be used for structure and function investigations. Moreover, b/d-agatoxins are characterized by a high specificity towards channels of insects, being totally ineffective on their mammalian counterparts. Such selectivity of the peptides provides a basis for creating new highly effective and safe insecticides.

Published
2010

21. Phenotypic, genotypic and proteomic characterization of J774 macrophages upon chronic exposure to fluoroquinolone antibiotics

Author

UCL - MD/FARM - Ecole de pharmacie, Marquez, B., Caceres, Nancy, Aerts, M., Vallet, Coralie M., Mingeot-Leclercq, Marie-Paule, Tulkens, Paul M., Devreese, B., Van Bambeke, Françoise, 34th Congress of the Federation-of-European-Biochemical-Societies, UCL - MD/FARM - Ecole de pharmacie, Marquez, B., Caceres, Nancy, Aerts, M., Vallet, Coralie M., Mingeot-Leclercq, Marie-Paule, Tulkens, Paul M., Devreese, B., Van Bambeke, Françoise, and 34th Congress of the Federation-of-European-Biochemical-Societies

Published
2009

22. Natural and directed evolution, the beta-lactamase model

Author

UCL - SC/CHIM - Département de chimie, Fastrez, Jacques, 31st Congress of the Federation-of-European-Biochemical-Societies (FEBS), UCL - SC/CHIM - Département de chimie, Fastrez, Jacques, and 31st Congress of the Federation-of-European-Biochemical-Societies (FEBS)

Published
2006

23. The presence of four iron-containing superoxide dismutase isozymes in Trypanosomatidae: characterization and subcellular localization in Trypanosoma brucei

Author

UCL - MD/BICL - Département de biochimie et de biologie cellulaire, Opperdoes, Frederik, Yernaux, Cédric, Gerbod, D, Viscogliosi, E, 30th Congress of the Federation-of-European-Biochemical-Societies (FEBS)/9th IUBMB Conference, UCL - MD/BICL - Département de biochimie et de biologie cellulaire, Opperdoes, Frederik, Yernaux, Cédric, Gerbod, D, Viscogliosi, E, and 30th Congress of the Federation-of-European-Biochemical-Societies (FEBS)/9th IUBMB Conference

Published
2005

24. An NMR view of the folding process of a CheY mutant at the residue level

Author

Federation of European Biochemical Societies, Consejo Superior de Investigaciones Científicas (España), García, P., Serrano, Luis, Rico, Manuel, Bruix, M., Federation of European Biochemical Societies, Consejo Superior de Investigaciones Científicas (España), García, P., Serrano, Luis, Rico, Manuel, and Bruix, M.

Abstract

The folding of CheY mutant F14N/V83T was studied at 75 residues by NMR. Fluorescence, NMR, and sedimentation equilibrium studies at different urea and protein concentrations reveal that the urea-induced unfolding of this CheY mutant includes an on-pathway molten globule-like intermediate that can associate off-pathway. The populations of native and denatured forms have been quantified from a series of 15N-1H HSQC spectra recorded under increasing concentrations of urea. A thermodynamic analysis of these data provides a detailed picture of the mutant's unfolding at the residue level: (1) the transition from the native state to the molten globule-like intermediate is highly cooperative, and (2) the unfolding of this state is sequential and yields another intermediate showing a collapsed N-terminal domain and an unfolded C-terminal tail. This state presents a striking similarity to the kinetic transition state of the CheY folding pathway.

Published
2002

25. Blood antioxidant parameters in subjects from Azorean populations with different socio-cultural profile

Author

27th meeting of the Federation of European Biochemical Societies (30 juin-5 juillet 2001: Lisbonne, Portugal), Pavao, M. L., Antonio, S., Figueiredo, T., Santos, Maria Cristina, Neve, Jean, Viegas Crespo, J., 27th meeting of the Federation of European Biochemical Societies (30 juin-5 juillet 2001: Lisbonne, Portugal), Pavao, M. L., Antonio, S., Figueiredo, T., Santos, Maria Cristina, Neve, Jean, and Viegas Crespo, J.

Abstract

info:eu-repo/semantics/nonPublished

Published
2001

26. Mining zebrafish microbiota reveals key community-level resistance against fish pathogen infection

Author

Valérie Briolat, Stevenn Volant, Sebastian Bruchmann, Susanne Häussler, Joaquín Bernal-Bayard, Franziska A. Stressmann, Bianca Audrain, Jean-Marc Ghigo, Amine Ghozlane, David Pérez-Pascual, Eric Duchaud, Jean-Pierre Levraud, Olaya Rendueles, Génétique des Biofilms - Genetics of Biofilms, Institut Pasteur [Paris] (IP)-Centre National de la Recherche Scientifique (CNRS), Génomique évolutive des Microbes / Microbial Evolutionary Genomics, Macrophages et Développement de l’Immunité, Helmholtz Centre for Infection Research (HZI), University of Cambridge [UK] (CAM), Hub Bioinformatique et Biostatistique - Bioinformatics and Biostatistics HUB, Virologie et Immunologie Moléculaires (VIM (UR 0892)), Université de Versailles Saint-Quentin-en-Yvelines (UVSQ)-Université Paris-Saclay-Institut National de Recherche pour l’Agriculture, l’Alimentation et l’Environnement (INRAE), This work was supported by the Institut Pasteur, the French Government’s Investissement d’Avenir program: Laboratoire d’Excellence ‘Integrative Biology of Emerging Infectious Diseases’ (grant no. ANR-10-LABX-62-IBEID to J.M.G.), the Fondation pour la Recherche Médicale (grant no. DEQ20180339185 to J.M.G.). F.S. was the recipient of a post-doctoral Marie Curie fellowship from the EU-FP7 programme, J.B.B. was the recipient of a long-term post-doctoral fellowship from the Federation of European Biochemical Societies(FEBS) and by the European Union’s Horizon 2020 research and innovation programme under the Marie Skłodowska-Curie grant agreement No 842629 D.P-P was supported by an Institut Carnot MS Postdoctoral fellowship., ANR-10-LABX-0062,IBEID,Integrative Biology of Emerging Infectious Diseases(2010), HZI,Helmholtz-Zentrum für Infektionsforschung GmbH, Inhoffenstr. 7,38124 Braunschweig, Germany., This work was supported by the Institut Pasteur, the French Government’s Investissement d’Avenir program: Laboratoire d’Excellence ‘Integrative Biology of Emerging Infectious Diseases’ (grant no. ANR-10-LABX-62-IBEID to J-MG.), the Fondation pour la Recherche Médicale (grant no. DEQ20180339185 to J-MG). FS was the recipient of a post-doctoral Marie Curie fellowship from the EU-FP7 program, JBB was the recipient of a long-term post-doctoral fellowship from the Federation of European Biochemical Societies (FEBS) and by the European Union’s Horizon 2020 research and innovation programme under the Marie Skłodowska-Curie grant agreement No 842629. DP-P was supported by an Institut Carnot MS Postdoctoral fellowship., European Project: 842629,Salmofish, and Institut Pasteur [Paris]-Centre National de la Recherche Scientifique (CNRS)

Subjects
Exogenous bacteria, Chryseobacterium, Colonisation resistance, Flavobacterium, [SDV.IMM.II]Life Sciences [q-bio]/Immunology/Innate immunity, Microbiology, Article, 03 medical and health sciences, medicine, MESH: Microbiota, Animals, MESH: Animals, MESH: Zebrafish, Pathogen, Zebrafish, Ecology, Evolution, Behavior and Systematics, 030304 developmental biology, 0303 health sciences, [SDV.BA.MVSA]Life Sciences [q-bio]/Animal biology/Veterinary medicine and animal Health, Innate immune system, biology, 030306 microbiology, Microbiota, fungi, Commensalism, biology.organism_classification, medicine.disease, [SDV.MP.BAC]Life Sciences [q-bio]/Microbiology and Parasitology/Bacteriology, MESH: Dysbiosis, Flavobacterium columnare, Dysbiosis, MESH: Flavobacterium / genetics, Bacteria
Abstract

The long-known resistance to pathogens provided by host-associated microbiota fostered the notion that adding protective bacteria could prevent or attenuate infection. However, the identification of endogenous or exogenous bacteria conferring such protection is often hindered by the complexity of host microbial communities. Here, we used zebrafish and the fish pathogen Flavobacterium columnare as a model system to study the determinants of microbiota-associated colonization resistance. We compared infection susceptibility in germ-free, conventional and re-conventionalized larvae and showed that a consortium of 10 culturable bacterial species are sufficient to protect zebrafish. Whereas survival to F. columnare infection does not rely on host innate immunity, we used antibiotic dysbiosis to alter zebrafish microbiota composition, leading to the identification of two different protection strategies. We first identified that the bacterium Chryseobacterium massiliae individually protects both larvae and adult zebrafish. We also showed that an assembly of 9 endogenous zebrafish species that do not otherwise protect individually confer a community-level resistance to infection. Our study therefore provides a rational approach to identify key endogenous protecting bacteria and promising candidates to engineer resilient microbial communities. It also shows how direct experimental analysis of colonization resistance in low-complexity in vivo models can reveal unsuspected ecological strategies at play in microbiota-based protection against pathogens.

Published
2020
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27. CTCF knockout in zebrafish induces alterations in regulatory landscapes and developmental gene expression

Author

Elisa de la Calle-Mustienes, Martin Franke, Ibai Irastorza-Azcarate, María Almuedo-Castillo, Juan J. Tena, José M. Santos-Pereira, José Luis Gómez-Skarmeta, Ana Neto, Rafael D. Acemel, European Commission, Ministerio de Economía y Competitividad (España), Fundación BBVA, Federation of European Biochemical Societies, and Junta de Andalucía

Subjects
CCCTC-Binding Factor, Embryo, Nonmammalian, Organogenesis, Science, General Physics and Astronomy, Development, Chromatin structure, General Biochemistry, Genetics and Molecular Biology, Article, 03 medical and health sciences, Gene Knockout Techniques, 0302 clinical medicine, Gene expression, Animals, RNA-Seq, Enhancer, Promoter Regions, Genetic, Gene, Zebrafish, 030304 developmental biology, Body Patterning, Regulation of gene expression, 0303 health sciences, Multidisciplinary, biology, Gene Expression Regulation, Developmental, Promoter, General Chemistry, Zebrafish Proteins, biology.organism_classification, Chromatin, Cell biology, Gene regulation, Enhancer Elements, Genetic, CTCF, CRISPR-Cas Systems, 030217 neurology & neurosurgery
Abstract

Coordinated chromatin interactions between enhancers and promoters are critical for gene regulation. The architectural protein CTCF mediates chromatin looping and is enriched at the boundaries of topologically associating domains (TADs), which are sub-megabase chromatin structures. In vitro CTCF depletion leads to a loss of TADs but has only limited effects over gene expression, challenging the concept that CTCF-mediated chromatin structures are a fundamental requirement for gene regulation. However, how CTCF and a perturbed chromatin structure impacts gene expression during development remains poorly understood. Here we link the loss of CTCF and gene regulation during patterning and organogenesis in a ctcf knockout zebrafish model. CTCF absence leads to loss of chromatin structure and affects the expression of thousands of genes, including many developmental regulators. Our results demonstrate the essential role of CTCF in providing the structural context for enhancer-promoter interactions, thus regulating developmental genes., J.L.G.-S. received funding from the ERC (Grant Agreement No. 740041), the Spanish Ministerio de Economía y Competitividad (Grant No. BFU2016-74961-P) and the institutional grant Unidad de Excelencia María de Maeztu (MDM-2016-0687). J.T. was funded by a 2019 Leonardo Grant for Researchers and Cultural Creators, BBVA Foundation. I.I.-A. acknowledges support from the Federation of European Biochemical Societies (FEBS Long-Term Fellowship). M.F. was funded by the European Union’s Horizon 2020 research and innovation program under the Marie Skłodowska-Curie grant agreement [#800396] and a Juan de la Cierva-Formación fellow from the Spanish Ministry of Science and Innovation (FJC2018-038233-I). JMS-P was funded by a postdoctoral fellowship from Junta de Andalucía (DOC_00512).

Published
2021

28. Determination of the structure and dynamics of the fuzzy coat of an amyloid fibril of IAPP using cryo-electron microscopy

Author

Z. Faidon Brotzakis, Thomas Löhr, Steven Truong, Samuel E. Hoff, Massimiliano Bonomi, Michele Vendruscolo, University of Cambridge [UK] (CAM), Département de Biologie structurale et Chimie - Department of Structural Biology and Chemistry, Institut Pasteur [Paris] (IP)-Université Paris Cité (UPCité), Centre National de la Recherche Scientifique (CNRS), Z.F.B. would like to acknowledge the Federation of European Biochemical Societies (FEBS) for financial support (LTF). M.B. and S.E.H. acknowledge the support of the French Agence Nationale de la Recherche (ANR), under grant ANR-20-CE45-0002 (project EMMI)., and ANR-20-CE45-0002,EMMI,Modélisation intégrative de la structure et de la dynamique des protéines avec la cryo-EM(2020)

Subjects
MEMMI, Structural Biology, IAPP, [SDV]Life Sciences [q-bio], macromolecular substances, Molecular Dynamics, Cryo-EM
Abstract

In recent years, major advances in cryo-electron microscopy (cryo-EM) have enabled the routine determination of complex biomolecular structures at atomic resolution. An open challenge for this approach, however, concerns large systems that exhibit continuous dynamics. To address this problem, we developed the metadynamic electron-microscopy metainference (MEMMI) method, which incorporates metadynamics, an enhanced conformational sampling approach, into the metainference method of integrative structural biology. MEMMI enables the simultaneous determination of the structure and dynamics of large heterogeneous systems by combining cryo-EM density maps with prior information through molecular dynamics, while at the same time modelling the different sources of error. To illustrate the method, we apply it to elucidate the dynamics of an amyloid fibril of the islet amyloid polypeptide (IAPP). The resulting conformational ensemble provides an accurate description of the structural variability of the disordered region of the amyloid fibril, known as fuzzy coat. The conformational ensemble also reveals that in nearly half of the structural core of this amyloid fibril the side-chains exhibit liquid-like dynamics despite the presence of the highly ordered network backbone of hydrogen bonds characteristic of the cross-β structure of amyloid fibrils.

Published
2022

37. Apoptosis: molecular regulation of cell death

Author

Hale, Annette J., Smith, Christopher A., Sutherland, Leslie C., Stoneman, Victoria E. A., Longthorne, Vanessa L., Culhane, Aedín C., Williams, Gwyn T., Federation of European Biochemical Societies, Christen, P., and Hofmann, E.

Published
1997
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45. Behavioral immune landscapes of inflammation

Author

Georgiana Crainiciuc, Miguel Palomino-Segura, Miguel Molina-Moreno, Jon Sicilia, David G. Aragones, Jackson Liang Yao Li, Rodrigo Madurga, José M. Adrover, Alejandra Aroca-Crevillén, Sandra Martin-Salamanca, Alfonso Serrano del Valle, Sandra D. Castillo, Heidi C. E. Welch, Oliver Soehnlein, Mariona Graupera, Fátima Sánchez-Cabo, Alexander Zarbock, Thomas E. Smithgall, Mauro Di Pilato, Thorsten R. Mempel, Pierre-Louis Tharaux, Santiago F. González, Angel Ayuso-Sacido, Lai Guan Ng, Gabriel F. Calvo, Iván González-Díaz, Fernando Díaz-de-María, Andrés Hidalgo, Ministerio de Ciencia e Innovación (España), Fundación La Caixa, Transatlantic Network of Excellence, Fondation Leducq, Unión Europea. Comisión Europea, Federation of European Biochemical Societies, European Molecular Biology Organization, Fundación ProCNIC, and Marie Curie

Subjects
Inflammation, Proteomics, Mice, Multidisciplinary, src-Family Kinases, Neutrophils, Proto-Oncogene Proteins, Leukocytes, Animals, Endothelium, Cell Shape, Article
Abstract

Transcriptional and proteomic profiling of individual cells have revolutionized interpretation of biological phenomena by providing cellular landscapes of healthy and diseased tissues1,2. These approaches, however, do not describe dynamic scenarios in which cells continuously change their biochemical properties and downstream 'behavioural' outputs3-5. Here we used 4D live imaging to record tens to hundreds of morpho-kinetic parameters describing the dynamics of individual leukocytes at sites of active inflammation. By analysing more than 100,000 reconstructions of cell shapes and tracks over time, we obtained behavioural descriptors of individual cells and used these high-dimensional datasets to build behavioural landscapes. These landscapes recognized leukocyte identities in the inflamed skin and trachea, and uncovered a continuum of neutrophil states inside blood vessels, including a large, sessile state that was embraced by the underlying endothelium and associated with pathogenic inflammation. Behavioural screening in 24 mouse mutants identified the kinase Fgr as a driver of this pathogenic state, and interference with Fgr protected mice from inflammatory injury. Thus, behavioural landscapes report distinct properties of dynamic environments at high cellular resolution. This study was supported by RTI2018-095497-B-I00 from Ministerio de Ciencia e Innovación (MCIN), HR17_00527 from Fundación La Caixa, Transatlantic Network of Excellence (TNE-18CVD04) from the Leducq Foundation, and FET-OPEN (no. 861878) from the European Commission to A.H. M.P-S. is supported by a Federation of European Biochemical Societies and the EMBO ALTF (no. 1142-2020) long-term fellowships. J.S. is supported by a fellowship (PRE2019-089130) from MICINN and A.A.-C. is supported by fellowship CF/BQ/ DR19/11740022 from La Caixa Foundation. J.L.Y.L. was supported by A*STAR and a Juan de la Cierva JCI-2017-33136 Fellowship from MICINN. S.D.C. is a recipient of a Marie Sklodowska-Curie fellowship (749731). M.G. is supported by SAF2017-89116R-P from MCIN and HR18_00120 from la Fundación La Caixa. T.R.M. is supported by grant NIH AI163223, L.G.N. is supported by SIgN core funding from A*STAR, and G.F.C. is supported by MCIN/ AEI/10.13039/501100011033 (grant PID2019-110895RB-I00) and by Junta de Comunidades de Castilla-La Mancha (SBPLY/19/180501/000211). F.S.-C. is supported by MCIN (grant RTI2018- 102084-B-I00), O.S. is supported by the Leducq Foundation (TNE-18CVD04), F.D.-d.-M. is supported by MCIN (TEC2017-84395-P), and T.E.S. is supported by the National Cancer Institute, NIH grant CA233576. The CNIC is supported by the MCIN and the Pro-CNIC Foundation. Sí

Published
2022

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