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BEGIN:VEVENT
DTSTART;TZID=UTC:20151217T190000
DTEND;TZID=UTC:20151217T190000
DTSTAMP:20260426T115936
CREATED:20151130T155937Z
LAST-MODIFIED:20151130T155937Z
UID:95884-1450378800-1450378800@ibecbarcelona.eu
SUMMARY:IBEC Christmas Party 2015
DESCRIPTION:We’re delighted to invite all IBECers to the biggest\, best IBEC Christmas Party Ever! \nThis year\, there’ll be a chance to take part in a charity event to raise money for some very good causes. If you take part\, you’ll be in with a chance of winning a fabulous prize provided by our sponsors\, such as a food hamper\, a digital camera\, a tablet\, or a weekend break. If you’d like to suggest your favourite charity to be a beneficiary of this fundraising\, fill in the form in i-Box in the intranet (deadline 9th December)). \nWith all this\, plus food\, drink\, music and some fun surprises\, the IBEC Christmas Party promises to be a fabulous way to kick-start the festive season!\n\nRegistration here.
URL:https://ibecbarcelona.eu/event/ibec-christmas-party-2015-2/
LOCATION:Fifteen Restaurant\, PCB
CATEGORIES:Social / Internal / PhD Committee
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151211T120000
DTEND;TZID=UTC:20151211T130000
DTSTAMP:20260426T115936
CREATED:20151029T093053Z
LAST-MODIFIED:20151029T093053Z
UID:19457-1449835200-1449838800@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Roberto de la Rica
DESCRIPTION:Bioplasmonics in nanofabrication\, biosensing and nanomedicine\nRoberto de la Rica\, University of Strathclyde\nIn this talk I will show several bio-enabled and bio-inspired approaches for growing and assembling plasmonic nanoparticles and their applications in biosensing and nanomedicine. I will explain how to use enzyme nanoreactors to guide the growth of plasmonic nanoparticles with different morphologies\, an approach that can be used to design ultrasensitive biosensors and new nanolithography tools. [1-4] \nI will also show a method for assembling nanoparticle superstructures with crystallographically aligned building blocks5 that possess improved plasmonic properties derived from their 3D organization. When assembled on magnetic supports these plasmonic superstructures can be used for as multifunctional intracellular sensors as well as for heat generation in thermal therapy. \n[1] Nat. Mater. 11\, 604 (2012);[2] Nat. Nanotechnol. 7\, 821\, 2012; [3] Nat. Protocol. 8\, 1759 (2013); [4] Adv. Funct. Mater. 24\, 3692 (2104); [5] JACS 133\, 2875 (2011)
URL:https://ibecbarcelona.eu/event/ibec-seminar-roberto-de-la-rica/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151211T120000
DTEND;TZID=UTC:20151211T130000
DTSTAMP:20260426T115936
CREATED:20151029T093053Z
LAST-MODIFIED:20151029T093053Z
UID:95876-1449835200-1449838800@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Roberto de la Rica
DESCRIPTION:Bioplasmonics in nanofabrication\, biosensing and nanomedicine\nRoberto de la Rica\, University of Strathclyde\nIn this talk I will show several bio-enabled and bio-inspired approaches for growing and assembling plasmonic nanoparticles and their applications in biosensing and nanomedicine. I will explain how to use enzyme nanoreactors to guide the growth of plasmonic nanoparticles with different morphologies\, an approach that can be used to design ultrasensitive biosensors and new nanolithography tools. [1-4] \nI will also show a method for assembling nanoparticle superstructures with crystallographically aligned building blocks5 that possess improved plasmonic properties derived from their 3D organization. When assembled on magnetic supports these plasmonic superstructures can be used for as multifunctional intracellular sensors as well as for heat generation in thermal therapy. \n[1] Nat. Mater. 11\, 604 (2012);[2] Nat. Nanotechnol. 7\, 821\, 2012; [3] Nat. Protocol. 8\, 1759 (2013); [4] Adv. Funct. Mater. 24\, 3692 (2104); [5] JACS 133\, 2875 (2011)
URL:https://ibecbarcelona.eu/event/ibec-seminar-roberto-de-la-rica-2/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151209T110000
DTEND;TZID=UTC:20151209T130000
DTSTAMP:20260426T115936
CREATED:20151117T133654Z
LAST-MODIFIED:20151117T133811Z
UID:19772-1449658800-1449666000@ibecbarcelona.eu
SUMMARY:PhD Thesis defence: Ernest Moles
DESCRIPTION:“Development of polyvalent erythrocyte- and parasitized erythrocyte-targeted nanovectors as novel site-specific drug delivery approaches for Plasmodium falciparum malaria chemotherapy”\nErnest Moles\, Nanomalaria joint unit\nErnest will be defending his PhD thesis on Wednesday 9th December at 11:00 in the Aula Magna of the Faculty of Pharmacy\, University of Barcelona. \nEverybody is welcome to attend. \n—\nIf you’re an IBEC PhD student and would like to advertise your PhD defence on the IBEC calendar\, please contact vleigh@ibecbarcelona.eu
URL:https://ibecbarcelona.eu/event/phd-thesis-defence-ernest-moles/
LOCATION:Aula Magna\, Faculty of Pharmacy\, Av. Joan XXIII s/n\, Barcelona\, Spain
CATEGORIES:PhD Thesis Defence
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151209T110000
DTEND;TZID=UTC:20151209T130000
DTSTAMP:20260426T115936
CREATED:20151117T133654Z
LAST-MODIFIED:20151117T133654Z
UID:95880-1449658800-1449666000@ibecbarcelona.eu
SUMMARY:PhD Thesis defence: Ernest Moles
DESCRIPTION:“Development of polyvalent erythrocyte- and parasitized erythrocyte-targeted nanovectors as novel site-specific drug delivery approaches for Plasmodium falciparum malaria chemotherapy”\nErnest Moles\, Nanomalaria joint unit\nErnest will be defending his PhD thesis on Wednesday 9th December at 11:00 in the Aula Magna of the Faculty of Pharmacy\, University of Barcelona. \nEverybody is welcome to attend. \n—\nIf you’re an IBEC PhD student and would like to advertise your PhD defence on the IBEC calendar\, please contact vleigh@ibecbarcelona.eu
URL:https://ibecbarcelona.eu/event/phd-thesis-defence-ernest-moles-2/
LOCATION:Aula Magna\, Faculty of Pharmacy\, Av. Joan XXIII s/n\, Barcelona\, Spain
CATEGORIES:PhD Thesis Defence
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151203T100000
DTEND;TZID=UTC:20151203T230000
DTSTAMP:20260426T115936
CREATED:20151126T075237Z
LAST-MODIFIED:20151126T075237Z
UID:95882-1449136800-1449183600@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Alexandre Perera
DESCRIPTION:Data evaluation in Metabolomics\, preprocessing\, analysis and biological enrichment\nAlexandre Perera\, B2SLab Bioinformatics and Biomedical Signals Laboratory\, UPC\nThis talk will depict the last efforts by the B2Slab on the processing of LC/MS metabolomics data. First\, we describe a new method to solve known issues of peak intensity drifts in metabolomics datasets. This method is based on a two-step approach in which intensity drift effects are modelled through Common Principal Components Analysis and removed from original data. Secondly\, we propose a new processing workflow based on peak aggregation techniques. We show that the predictive power of the data is improved when the peak aggregation techniques are used regardless of the prediction technique used. We also describe a new computational tool to perform end-to-end analysis (MAIT) coded under the R environment. MAIT package is highly modular and programmable which allow the users to perform their personalised LC/MS data analysis workflows. MAIT is able to take the raw output files from an LC/MS instrument as an input and\, by applying a set of functions\, provide a metabolite identification table as a result. Finally\, we introduce FELLA\, a set of algorithms for biological interpretation of metabolomic data in light of existing knowledge extracted from annotation databases\, extending the concept of pathway enrichment into metabolomics. FELLA is based on diffusion process on a graph representation of a knowledge base\, while statistically testing solutions against analytical null diffusion distributions. Results are provided comparing the tools with sate of the art methods on different network types.\n\n[1] Fernández-Albert F.\, Llorach R.\, Andrés-Lacueva C.\, Perera-Lluna A. Peak Aggregation as an Innovative Strategy for Improving the Predictive Power of LC-MS Metabolomic Profiles. Analytical Chemistry 86 (5)\, 2320–5 (2014).\n[2] Fernández-Albert F.\, Llorach R.\, Andrés-Lacueva C.\, Perera-Lluna A. An R package to analyse LC/MS metabolomic data: MAIT (Metabolite Automatic Identification Toolkit). Bioinformatics 30(13):1937-9 (2014).\n[3] Fernández-Albert F.\, Llorach R.\, Garcia-Aloy M\, Ziyatdinov A\, Andrés-Lacueva C.\, Perera-Lluna A. Intensity drift removal in LC/MS metabolomics by Common Variance Compensation. Bioinformatics 30(20)\, 2898-2905 (2014)\n[4] Domingo-Almenara\, X.\, Perera\, A.\, Ramírez\, N.\, Cañellas\, N.\, Correig\, X.\, & Brezmes\, J. (2015). Compound identification in gas chromatography/mass spectrometry-based metabolomics by blind source separation. Journal of Chromatography A\, 1409\, 226-233\n[5] Ziyatdinov\, A.; Marco\, S.; Chaudry\, A.; Persaud\, K.; Caminal\, P.; Perera\, A. Drift compensation of gas sensor array data by common principal component analysis. Sensors and Actuators B: Chemical 146\, 460-5 (2010).
URL:https://ibecbarcelona.eu/event/ibec-seminar-alexandre-perera-2/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151203T100000
DTEND;TZID=UTC:20151203T230000
DTSTAMP:20260426T115936
CREATED:20151126T075237Z
LAST-MODIFIED:20151126T075237Z
UID:19883-1449136800-1449183600@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Alexandre Perera
DESCRIPTION:Data evaluation in Metabolomics\, preprocessing\, analysis and biological enrichment\nAlexandre Perera\, B2SLab Bioinformatics and Biomedical Signals Laboratory\, UPC\nThis talk will depict the last efforts by the B2Slab on the processing of LC/MS metabolomics data. First\, we describe a new method to solve known issues of peak intensity drifts in metabolomics datasets. This method is based on a two-step approach in which intensity drift effects are modelled through Common Principal Components Analysis and removed from original data. Secondly\, we propose a new processing workflow based on peak aggregation techniques. We show that the predictive power of the data is improved when the peak aggregation techniques are used regardless of the prediction technique used. We also describe a new computational tool to perform end-to-end analysis (MAIT) coded under the R environment. MAIT package is highly modular and programmable which allow the users to perform their personalised LC/MS data analysis workflows. MAIT is able to take the raw output files from an LC/MS instrument as an input and\, by applying a set of functions\, provide a metabolite identification table as a result. Finally\, we introduce FELLA\, a set of algorithms for biological interpretation of metabolomic data in light of existing knowledge extracted from annotation databases\, extending the concept of pathway enrichment into metabolomics. FELLA is based on diffusion process on a graph representation of a knowledge base\, while statistically testing solutions against analytical null diffusion distributions. Results are provided comparing the tools with sate of the art methods on different network types.\n\n[1] Fernández-Albert F.\, Llorach R.\, Andrés-Lacueva C.\, Perera-Lluna A. Peak Aggregation as an Innovative Strategy for Improving the Predictive Power of LC-MS Metabolomic Profiles. Analytical Chemistry 86 (5)\, 2320–5 (2014).\n[2] Fernández-Albert F.\, Llorach R.\, Andrés-Lacueva C.\, Perera-Lluna A. An R package to analyse LC/MS metabolomic data: MAIT (Metabolite Automatic Identification Toolkit). Bioinformatics 30(13):1937-9 (2014).\n[3] Fernández-Albert F.\, Llorach R.\, Garcia-Aloy M\, Ziyatdinov A\, Andrés-Lacueva C.\, Perera-Lluna A. Intensity drift removal in LC/MS metabolomics by Common Variance Compensation. Bioinformatics 30(20)\, 2898-2905 (2014)\n[4] Domingo-Almenara\, X.\, Perera\, A.\, Ramírez\, N.\, Cañellas\, N.\, Correig\, X.\, & Brezmes\, J. (2015). Compound identification in gas chromatography/mass spectrometry-based metabolomics by blind source separation. Journal of Chromatography A\, 1409\, 226-233\n[5] Ziyatdinov\, A.; Marco\, S.; Chaudry\, A.; Persaud\, K.; Caminal\, P.; Perera\, A. Drift compensation of gas sensor array data by common principal component analysis. Sensors and Actuators B: Chemical 146\, 460-5 (2010).
URL:https://ibecbarcelona.eu/event/ibec-seminar-alexandre-perera/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151127T120000
DTEND;TZID=UTC:20151127T130000
DTSTAMP:20260426T115936
CREATED:20151106T080207Z
LAST-MODIFIED:20151123T092950Z
UID:19561-1448625600-1448629200@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Chia-Fu Chou
DESCRIPTION:Low-copy number biomolecular analysis with dielectrophoretic enrichment /trapping via molecular dam and plasmonic electrode nanogaps\nChia-Fu Chou\, Senior Research Fellow/Professor\, Institute of Physics\, Academia Sinica\, Taiwan\nNanoscale structures\, such as electrode nanogap and nanofluidic confinement\, given its simplicity in geometry\, nevertheless offer unique platforms for the study of molecular and cellular biophysics\, with the potential for bioanalytical applications [1-5]. For low-copy number molecule detection\, we developed two versatile analysis platforms for the manipulation and sensing of biomolecules. In the first scenario\, sub-30 nm insulating nanoconstriction operating under the balance of negative dielectrophoresis (DEP)\, electrophoresis\, and electroosmosis\, serves as molecular dam\, enables protein enrichment of 105-fold in 20 seconds [6]\, which can then be coupled with graphene-modified electrode for sensitive electrochemical detection of proteins and peptides [7\, 8]. In the second scenario\, an array of Ti/Au electrode nanogaps with sub-10 nm gap size function as templates for AC DEP-based molecular trapping\, plasmonic hot spots for surface-enhanced Raman spectroscopy as well as electronic measurements\, and fluorescence imaging. During molecular trapping\, recorded Raman spectra\, conductance measurements across the nanogaps and fluorescence imaging show unambiguously the presence and characteristics of the trapped molecules\, demonstrated with R-phycoerythrin [9] and Alzheimer’s disease associated biomarkers A-beta 40 and 42 peptides. Our platforms open up simple ways for multifunctional low-concentration heterogeneous sample analysis.\n[1] L.J. Guo\, X. Cheng\, C.F. Chou\, Nano Lett. 4\, 69 (2004).\n[2] J. Gu\, R. Gupta\, C.F. Chou\, Q. Wei\, F. Zenhausern\, Lab Chip 7\, 1198 (2007).\n[3] J.W. Yeh\, A. Taloni\, Y.L. Chen\, C.F. Chou\, Nano Lett. 12\, 1597 (2012). [Research Highlights\, Nature 482\, 442 (2012)].\n[4] J.P. Shen and C.F. Chou\, Biomicrofluidics 8\, 041103 (2014).\n[5] K.K. Sriram\, J.W. Yeh\, Y.L. Lin\, Y.R. Chang\, C.F. Chou\, Nucleic Acids Res. 42\, e85 (2014).\n[6] K.T. Liao\, C.F. Chou\, J. Am. Chem. Soc. 134\, 8742 (2012). [JACS Spotlights: JACS 134\, 10307 (2012)]\n[7] B. Sanghavi\, W. Varhue\, J. Chávez\, C.F. Chou\, N. S. Swami\, Anal. Chem. 86\, 4120 (2014\,).\n[8] B.J. Sanghavi\, W. Varhue\, A. Rohani\, K.T. Liao\, L. Bazydlo\, C.F. Chou\, N. S. Swami\, Lab Chip 2015\, DOI: 10.1039/c5lc00840a.\n[9] L. Lesser-Rojas\, P. Ebbinghaus\, G. Vasan\, M.L. Chu\, A. Erbe\, C.F. Chou\, Nano Lett. 14\, 2242 (2014).
URL:https://ibecbarcelona.eu/event/ibec-seminar-chia-fu-chou/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151127T120000
DTEND;TZID=UTC:20151127T130000
DTSTAMP:20260426T115936
CREATED:20151106T080207Z
LAST-MODIFIED:20151106T080207Z
UID:95877-1448625600-1448629200@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Chia-Fu Chou
DESCRIPTION:Low-copy number biomolecular analysis with dielectrophoretic enrichment /trapping via molecular dam and plasmonic electrode nanogaps\nChia-Fu Chou\, Senior Research Fellow/Professor\, Institute of Physics\, Academia Sinica\, Taiwan\nNanoscale structures\, such as electrode nanogap and nanofluidic confinement\, given its simplicity in geometry\, nevertheless offer unique platforms for the study of molecular and cellular biophysics\, with the potential for bioanalytical applications [1-5]. For low-copy number molecule detection\, we developed two versatile analysis platforms for the manipulation and sensing of biomolecules. In the first scenario\, sub-30 nm insulating nanoconstriction operating under the balance of negative dielectrophoresis (DEP)\, electrophoresis\, and electroosmosis\, serves as molecular dam\, enables protein enrichment of 105-fold in 20 seconds [6]\, which can then be coupled with graphene-modified electrode for sensitive electrochemical detection of proteins and peptides [7\, 8]. In the second scenario\, an array of Ti/Au electrode nanogaps with sub-10 nm gap size function as templates for AC DEP-based molecular trapping\, plasmonic hot spots for surface-enhanced Raman spectroscopy as well as electronic measurements\, and fluorescence imaging. During molecular trapping\, recorded Raman spectra\, conductance measurements across the nanogaps and fluorescence imaging show unambiguously the presence and characteristics of the trapped molecules\, demonstrated with R-phycoerythrin [9] and Alzheimer’s disease associated biomarkers A-beta 40 and 42 peptides. Our platforms open up simple ways for multifunctional low-concentration heterogeneous sample analysis.\n[1] L.J. Guo\, X. Cheng\, C.F. Chou\, Nano Lett. 4\, 69 (2004).\n[2] J. Gu\, R. Gupta\, C.F. Chou\, Q. Wei\, F. Zenhausern\, Lab Chip 7\, 1198 (2007).\n[3] J.W. Yeh\, A. Taloni\, Y.L. Chen\, C.F. Chou\, Nano Lett. 12\, 1597 (2012). [Research Highlights\, Nature 482\, 442 (2012)].\n[4] J.P. Shen and C.F. Chou\, Biomicrofluidics 8\, 041103 (2014).\n[5] K.K. Sriram\, J.W. Yeh\, Y.L. Lin\, Y.R. Chang\, C.F. Chou\, Nucleic Acids Res. 42\, e85 (2014).\n[6] K.T. Liao\, C.F. Chou\, J. Am. Chem. Soc. 134\, 8742 (2012). [JACS Spotlights: JACS 134\, 10307 (2012)]\n[7] B. Sanghavi\, W. Varhue\, J. Chávez\, C.F. Chou\, N. S. Swami\, Anal. Chem. 86\, 4120 (2014\,).\n[8] B.J. Sanghavi\, W. Varhue\, A. Rohani\, K.T. Liao\, L. Bazydlo\, C.F. Chou\, N. S. Swami\, Lab Chip 2015\, DOI: 10.1039/c5lc00840a.\n[9] L. Lesser-Rojas\, P. Ebbinghaus\, G. Vasan\, M.L. Chu\, A. Erbe\, C.F. Chou\, Nano Lett. 14\, 2242 (2014).
URL:https://ibecbarcelona.eu/event/ibec-seminar-chia-fu-chou-2/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151127T100000
DTEND;TZID=UTC:20151127T110000
DTSTAMP:20260426T115936
CREATED:20151027T093619Z
LAST-MODIFIED:20151119T152104Z
UID:19436-1448618400-1448622000@ibecbarcelona.eu
SUMMARY:PhD Discussions Session: Maria Chiara Biagi and Roger Oria
DESCRIPTION:Nanoscale dielectric characterization of single bacterial cells at microwave frequency\nMaria Chiara Biagi\, Nanoscale Bioelectrical Characterization group\nInformation on the microwave electromagnetic properties of cell suspensions and tissues has already led to important application in therapeutic and diagnostic. In recent years\, a new microscopy technique has appeared\, able to resolve the electromagnetic response at GHz even further down\, at nanoscale spatial resolution: Scanning Microwave Microscope (SMM). Its application to single cells would possibly allow not just to scale down the existing medical and biological techniques\, but would also give rise to a new class of label-free imaging methods based on dielectric contrast. Yet\, the quantification of the intrinsic dielectric properties (i.e. complex permittivity) of non-planar irregular shaped objects like single cells from the standard SMM images remains a challenge\, because the experimental signal is greatly affected by the huge presence of non-local contributions. \nWe developed a methodology to quantify and remove them\, which consequently enables to obtain images related only to the intrinsic dielectric response of the sample. These images are then suitable for a quantitative analysis and\, in combination with 3D finite element numerical calculations\, a map of the complex permittivity of the cell can be obtained.\nWe have applied this procedure to a single bacterial cell (E. coli) and quantified for the first time its complex permittivity at ~19 GHz\, in dry and humid conditions. \n  \nInterplay between integrin expression\, clustering\, and substrate rigidity in cell mechanical response\nRoger Oria\, Cellular and respiratory biomechanics group\nEssential cell functions such as proliferation\, differentiation\, or migration are determined by the rigidity and composition of the extracellular matrix (ECM). Understanding this interaction requires a precise control of ECM mechanical properties and molecular distribution of cell-ECM ligands\, as well as the ability to measure the mechanical forces transmitted at the cell-ECM interface. To address this issue\, we have developed an approach based on polyacrylamide substrates of tunable rigidity decorated with nanometric regular hexagonal patterns of RGD ligands\, which serve as binding sites for single integrins. By using this system\, we have systematically analysed cell response in terms of force transmission\, rearward flow and integrin recruitment after varying (i) gel rigidity\, (ii) spacing and spatial distribution between RGD ligands\, and (iii) integrin expression levels. Our results show that cell response and force generation are critically dependent on all factors. We also demonstrate the counter-intuitive fact that at specific ECM rigidities cells increase force transmission as the spacing between integrins increases from 50 to 100 nm. Our findings indicate that mechanical homeostasis can be tuned by cells using strategies based on integrin expression\, clustering of ECM ligands\, or ECM rigidity\, and that an in-depth understanding of cell mechanical responses requires the consideration of all those factors. \n 
URL:https://ibecbarcelona.eu/event/phd-discussions-session-maria-chiara-and-roger-oria/
CATEGORIES:PhD Discussions Session
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151127T100000
DTEND;TZID=UTC:20151127T110000
DTSTAMP:20260426T115936
CREATED:20151027T093619Z
LAST-MODIFIED:20151027T093619Z
UID:95874-1448618400-1448622000@ibecbarcelona.eu
SUMMARY:PhD Discussions Session: Maria Chiara Biagi and Roger Oria
DESCRIPTION:Nanoscale dielectric characterization of single bacterial cells at microwave frequency\nMaria Chiara Biagi\, Nanoscale Bioelectrical Characterization group\nInformation on the microwave electromagnetic properties of cell suspensions and tissues has already led to important application in therapeutic and diagnostic. In recent years\, a new microscopy technique has appeared\, able to resolve the electromagnetic response at GHz even further down\, at nanoscale spatial resolution: Scanning Microwave Microscope (SMM). Its application to single cells would possibly allow not just to scale down the existing medical and biological techniques\, but would also give rise to a new class of label-free imaging methods based on dielectric contrast. Yet\, the quantification of the intrinsic dielectric properties (i.e. complex permittivity) of non-planar irregular shaped objects like single cells from the standard SMM images remains a challenge\, because the experimental signal is greatly affected by the huge presence of non-local contributions. \nWe developed a methodology to quantify and remove them\, which consequently enables to obtain images related only to the intrinsic dielectric response of the sample. These images are then suitable for a quantitative analysis and\, in combination with 3D finite element numerical calculations\, a map of the complex permittivity of the cell can be obtained.\nWe have applied this procedure to a single bacterial cell (E. coli) and quantified for the first time its complex permittivity at ~19 GHz\, in dry and humid conditions. \n  \nInterplay between integrin expression\, clustering\, and substrate rigidity in cell mechanical response\nRoger Oria\, Cellular and respiratory biomechanics group\nEssential cell functions such as proliferation\, differentiation\, or migration are determined by the rigidity and composition of the extracellular matrix (ECM). Understanding this interaction requires a precise control of ECM mechanical properties and molecular distribution of cell-ECM ligands\, as well as the ability to measure the mechanical forces transmitted at the cell-ECM interface. To address this issue\, we have developed an approach based on polyacrylamide substrates of tunable rigidity decorated with nanometric regular hexagonal patterns of RGD ligands\, which serve as binding sites for single integrins. By using this system\, we have systematically analysed cell response in terms of force transmission\, rearward flow and integrin recruitment after varying (i) gel rigidity\, (ii) spacing and spatial distribution between RGD ligands\, and (iii) integrin expression levels. Our results show that cell response and force generation are critically dependent on all factors. We also demonstrate the counter-intuitive fact that at specific ECM rigidities cells increase force transmission as the spacing between integrins increases from 50 to 100 nm. Our findings indicate that mechanical homeostasis can be tuned by cells using strategies based on integrin expression\, clustering of ECM ligands\, or ECM rigidity\, and that an in-depth understanding of cell mechanical responses requires the consideration of all those factors. \n 
URL:https://ibecbarcelona.eu/event/phd-discussions-session-maria-chiara-and-roger-oria-2/
CATEGORIES:PhD Discussions Session
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151123T150000
DTEND;TZID=UTC:20151123T170000
DTSTAMP:20260426T115936
CREATED:20151119T115401Z
LAST-MODIFIED:20151119T115612Z
UID:19829-1448290800-1448298000@ibecbarcelona.eu
SUMMARY:PhD Thesis defence: Lorena De Oñate
DESCRIPTION:“Research on cardiac differentiation from human pluripotent stem cells: how to get beating cells in a dish”\nLorena De Oñate\, Pluripotent Stem Cells and Activation of Endogenous Tissue Programs for Organ Regeneration group\nLorena will be defending her PhD thesis on Monday 23rd November at 15:00 in the Ramón y Cajal Room at the Parc de Recerca Biomèdica (PRBB).  \nEverybody is welcome to attend. \n—\nIf you’re an IBEC PhD student and would like to advertise your PhD defence on the IBEC calendar\, please contact vleigh@ibecbarcelona.eu
URL:https://ibecbarcelona.eu/event/phd-thesis-defence-lorena-de-onate/
LOCATION:Sala Ramón y Cajal\, Parc de Recerca Biomèdica (PRBB)\, Barcelona\, Spain
CATEGORIES:PhD Thesis Defence
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151123T150000
DTEND;TZID=UTC:20151123T170000
DTSTAMP:20260426T115936
CREATED:20151119T115401Z
LAST-MODIFIED:20151119T115401Z
UID:95881-1448290800-1448298000@ibecbarcelona.eu
SUMMARY:PhD Thesis defence: Lorena De Oñate
DESCRIPTION:“Research on cardiac differentiation from human pluripotent stem cells: how to get beating cells in a dish”\nLorena De Oñate\, Pluripotent Stem Cells and Activation of Endogenous Tissue Programs for Organ Regeneration group\nLorena will be defending her PhD thesis on Monday 23rd November at 15:00 in the Ramón y Cajal Room at the Parc de Recerca Biomèdica (PRBB).  \nEverybody is welcome to attend. \n—\nIf you’re an IBEC PhD student and would like to advertise your PhD defence on the IBEC calendar\, please contact vleigh@ibecbarcelona.eu
URL:https://ibecbarcelona.eu/event/phd-thesis-defence-lorena-de-onate-2/
LOCATION:Sala Ramón y Cajal\, Parc de Recerca Biomèdica (PRBB)\, Barcelona\, Spain
CATEGORIES:PhD Thesis Defence
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151119T120000
DTEND;TZID=UTC:20151119T130000
DTSTAMP:20260426T115936
CREATED:20151109T154810Z
LAST-MODIFIED:20151113T074152Z
UID:19587-1447934400-1447938000@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Luis de Lecea
DESCRIPTION:Optogenetic control of arousal\nLuis de Lecea\, Department of Psychiatry and Behavioral Sciences\, Stanford University School of Medicine\nChanges in arousal states are at the core of most neuropsychiatric disorders. Several groups of monoaminergic neurons have long been known to facilitate arousal state transitions. Here we will review the role of hypocretin/orexin neurons in the dynamics of sleep-to-wake transitions. I will also show data demonstrating that dopaminergic neurons of the ventral tegmental area (VTA) directly and causally control the generation and maintenance of electrocortical and behavioral arousal. Combining chemogenetic and optogenetic tools with polysomnographic recordings in mice\, we show that activity in VTA-dopaminergic neurons is necessary for arousal\, and that their chemogenetic inhibition suppresses wakefulness to promote both non-rapid eye movement (NREM) and REM sleep. Moreover\, chemogenetic inhibition of VTA-dopaminergic neurons suppresses wakefulness even in the face of highly salient stimuli related to reproduction\, feeding and predation. Nevertheless\, prior to inducing sleep\, chemogenetic inhibition of VTA-dopaminergic neurons promotes goal-directed and sleep-related nest building behavior. Optogenetic stimulation\, in contrast\, initiates and maintains long-term wakefulness and suppresses sleep and sleep-related nesting behavior. We further show that the nucleus accumbens (NAc) circuit\, and not the medial prefrontal cortex (mPFC)\, mediates most of VTA-dopaminergic effects on arousal. After collecting data from multiple brain structures involved in arousal states\, we propose a computational model that assigns probabilities to optogenetically-induced arousal state transitions in individual brain structures. We identify feedback\, redundancy\, and gating hierarchy as three fundamental aspects of this model. Incorporation of conductance-based models of neuronal ensembles into this model and existing models of cortical excitability will provide more comprehensive insight into arousal state dynamics as well as arousal-related disorders.
URL:https://ibecbarcelona.eu/event/ibec-seminar-luis-de-lecea/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151119T120000
DTEND;TZID=UTC:20151119T130000
DTSTAMP:20260426T115936
CREATED:20151109T154810Z
LAST-MODIFIED:20151109T154810Z
UID:95878-1447934400-1447938000@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Luis de Lecea
DESCRIPTION:Optogenetic control of arousal\nLuis de Lecea\, Department of Psychiatry and Behavioral Sciences\, Stanford University School of Medicine\nChanges in arousal states are at the core of most neuropsychiatric disorders. Several groups of monoaminergic neurons have long been known to facilitate arousal state transitions. Here we will review the role of hypocretin/orexin neurons in the dynamics of sleep-to-wake transitions. I will also show data demonstrating that dopaminergic neurons of the ventral tegmental area (VTA) directly and causally control the generation and maintenance of electrocortical and behavioral arousal. Combining chemogenetic and optogenetic tools with polysomnographic recordings in mice\, we show that activity in VTA-dopaminergic neurons is necessary for arousal\, and that their chemogenetic inhibition suppresses wakefulness to promote both non-rapid eye movement (NREM) and REM sleep. Moreover\, chemogenetic inhibition of VTA-dopaminergic neurons suppresses wakefulness even in the face of highly salient stimuli related to reproduction\, feeding and predation. Nevertheless\, prior to inducing sleep\, chemogenetic inhibition of VTA-dopaminergic neurons promotes goal-directed and sleep-related nest building behavior. Optogenetic stimulation\, in contrast\, initiates and maintains long-term wakefulness and suppresses sleep and sleep-related nesting behavior. We further show that the nucleus accumbens (NAc) circuit\, and not the medial prefrontal cortex (mPFC)\, mediates most of VTA-dopaminergic effects on arousal. After collecting data from multiple brain structures involved in arousal states\, we propose a computational model that assigns probabilities to optogenetically-induced arousal state transitions in individual brain structures. We identify feedback\, redundancy\, and gating hierarchy as three fundamental aspects of this model. Incorporation of conductance-based models of neuronal ensembles into this model and existing models of cortical excitability will provide more comprehensive insight into arousal state dynamics as well as arousal-related disorders.
URL:https://ibecbarcelona.eu/event/ibec-seminar-luis-de-lecea-2/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151118T171500
DTEND;TZID=UTC:20151118T203000
DTSTAMP:20260426T115936
CREATED:20151110T131625Z
LAST-MODIFIED:20151110T131625Z
UID:95879-1447866900-1447878600@ibecbarcelona.eu
SUMMARY:Setmana de la Ciència 2015
DESCRIPTION:Setmana de la Ciència 2015\nParc Científic de Barcelona\, Sala Dolors Aleu\nEl dimecres 18 de novembre a la tarda\, en el context de la celebració de la SETMANA DE LA CIÈNCIA\, volem que ens acompanyis en una jornada científica singular. \nPodràs visitar els laboratoris per conèixer la recerca més puntera en bioenginyeria\, i sota el títol “Fem visibles les forces cel·lulars”\, el Professor Xavier Trepat explicarà com i perquè estudien les forces que fan les cèl·lules. \nA més a més\, per celebrar que aquest any és l’Any Internacional de la llum\, finalitzarem la visita amb un brindis i un petit concert amb inspiració científica.\nAquesta activitat és gratuïta\, està dirigida a majos de 16 anys i les places són limitades\, per tant cal INSCRIURE’S
URL:https://ibecbarcelona.eu/event/setmana-de-la-ciencia-2015-2/
LOCATION:Sala Dolors Aleu\, Cluster II\, Parc Científic de Barcelona\, Barcelona\, Spain
CATEGORIES:Outreach / Fair / Festival
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151118T171500
DTEND;TZID=UTC:20151118T203000
DTSTAMP:20260426T115936
CREATED:20151110T131625Z
LAST-MODIFIED:20170801T131002Z
UID:19592-1447866900-1447878600@ibecbarcelona.eu
SUMMARY:Setmana de la Ciència 2015
DESCRIPTION:Setmana de la Ciència 2015\nParc Científic de Barcelona\, Sala Dolors Aleu\nEl dimecres 18 de novembre a la tarda\, en el context de la celebració de la SETMANA DE LA CIÈNCIA\, volem que ens acompanyis en una jornada científica singular. \nPodràs visitar els laboratoris per conèixer la recerca més puntera en bioenginyeria\, i sota el títol “Fem visibles les forces cel·lulars”\, el Professor Xavier Trepat explicarà com i perquè estudien les forces que fan les cèl·lules. \nA més a més\, per celebrar que aquest any és l’Any Internacional de la llum\, finalitzarem la visita amb un brindis i un petit concert amb inspiració científica.\nAquesta activitat és gratuïta\, està dirigida a majos de 16 anys i les places són limitades\, per tant cal INSCRIURE’S
URL:https://ibecbarcelona.eu/event/setmana-de-la-ciencia-2015/
LOCATION:Sala Dolors Aleu\, Cluster II\, Parc Científic de Barcelona\, Barcelona\, Spain
CATEGORIES:Outreach / Fair / Festival
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151111T110000
DTEND;TZID=UTC:20151111T130000
DTSTAMP:20260426T115936
CREATED:20151021T082429Z
LAST-MODIFIED:20151021T082429Z
UID:19399-1447239600-1447246800@ibecbarcelona.eu
SUMMARY:PhD Thesis Defense:  Rosa Letizia Zaffino
DESCRIPTION:“Development of a nano-sensor for the direct electrical free-label detection of DNA’s hybridisation and single nucleotide polymorphism”\nRosa Letizia Zaffino\, Nanobioengineering group\nRosa will be defending her PhD thesis on Wednesday 11th November at 11:00 in the Sala de Grados (A01S)\, Faculty of Physics.  \nEverybody is welcome to attend. \n—\nIf you’re an IBEC PhD student and would like to advertise your PhD defense on the IBEC calendar\, please contact vleigh@ibecbarcelona.eu
URL:https://ibecbarcelona.eu/event/phd-thesis-defense-rosa-letizia-zaffino/
LOCATION:Sala de Grados (A01S)\, Faculty of Physics\, UB\, Barcelona
CATEGORIES:PhD Thesis Defence
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151111T110000
DTEND;TZID=UTC:20151111T130000
DTSTAMP:20260426T115936
CREATED:20151021T082429Z
LAST-MODIFIED:20151021T082429Z
UID:95873-1447239600-1447246800@ibecbarcelona.eu
SUMMARY:PhD Thesis Defense:  Rosa Letizia Zaffino
DESCRIPTION:“Development of a nano-sensor for the direct electrical free-label detection of DNA’s hybridisation and single nucleotide polymorphism”\nRosa Letizia Zaffino\, Nanobioengineering group\nRosa will be defending her PhD thesis on Wednesday 11th November at 11:00 in the Sala de Grados (A01S)\, Faculty of Physics.  \nEverybody is welcome to attend. \n—\nIf you’re an IBEC PhD student and would like to advertise your PhD defense on the IBEC calendar\, please contact vleigh@ibecbarcelona.eu
URL:https://ibecbarcelona.eu/event/phd-thesis-defense-rosa-letizia-zaffino-2/
LOCATION:Sala de Grados (A01S)\, Faculty of Physics\, UB\, Barcelona
CATEGORIES:PhD Thesis Defence
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151027T113000
DTEND;TZID=UTC:20151027T133000
DTSTAMP:20260426T115936
CREATED:20151021T064210Z
LAST-MODIFIED:20151021T064210Z
UID:19388-1445945400-1445952600@ibecbarcelona.eu
SUMMARY:PhD Thesis Defense: Andrés Arcentales Viteri
DESCRIPTION:“Análisis de la interacción cardíaca y respiratoria en pacientes con cardiomiopatía y pacientes en proceso de extubación”\nAndrés Arcentales Viteri\, Biomedical Signal Processing and Interpretation group\nAndrés will be defending his PhD thesis on Tuesday 27th October at 11:30 in the Sala d’Actes de la Facultat de Matemàtica i Estadística (FME)\, C. Pau Gargallo\, 5\, 08028 Barcelona.  \nEverybody is welcome to attend. \n—\nIf you’re an IBEC PhD student and would like to advertise your PhD defense on the IBEC calendar\, please contact vleigh@ibecbarcelona.eu
URL:https://ibecbarcelona.eu/event/phd-thesis-defense-andres-arcentales-viteri/
LOCATION:Sala d’Actes de la Facultat de Matemàtica i Estadística (FME)\, C. Pau Gargallo\, 5\, Barcelona\, 08028
CATEGORIES:PhD Thesis Defence
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151027T113000
DTEND;TZID=UTC:20151027T133000
DTSTAMP:20260426T115936
CREATED:20151021T064210Z
LAST-MODIFIED:20151021T064210Z
UID:95872-1445945400-1445952600@ibecbarcelona.eu
SUMMARY:PhD Thesis Defense: Andrés Arcentales Viteri
DESCRIPTION:“Análisis de la interacción cardíaca y respiratoria en pacientes con cardiomiopatía y pacientes en proceso de extubación”\nAndrés Arcentales Viteri\, Biomedical Signal Processing and Interpretation group\nAndrés will be defending his PhD thesis on Tuesday 27th October at 11:30 in the Sala d’Actes de la Facultat de Matemàtica i Estadística (FME)\, C. Pau Gargallo\, 5\, 08028 Barcelona.  \nEverybody is welcome to attend. \n—\nIf you’re an IBEC PhD student and would like to advertise your PhD defense on the IBEC calendar\, please contact vleigh@ibecbarcelona.eu
URL:https://ibecbarcelona.eu/event/phd-thesis-defense-andres-arcentales-viteri-2/
LOCATION:Sala d’Actes de la Facultat de Matemàtica i Estadística (FME)\, C. Pau Gargallo\, 5\, Barcelona\, 08028
CATEGORIES:PhD Thesis Defence
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=Europe/Madrid:20151023T100000
DTEND;TZID=Europe/Madrid:20151023T110000
DTSTAMP:20260426T115936
CREATED:20150803T123423Z
LAST-MODIFIED:20150803T123423Z
UID:95866-1445594400-1445598000@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Miquel Bosch Pita
DESCRIPTION:The molecular mechanisms of memory persistence: imaging how single synapses learn in real time\nMiquel Bosch Pita\, Nanoprobes and nanoswitches group\, IBEC\nMemories are stored in our brain through the ability of synaptic connections to modify their structure and function in a long-lasting way. However\, nobody has ever observed how these changes occur in a single synapse in real time.\nI will explain how we used a new combination of optical technologies to reveal the molecular remodeling that takes place inside a synapse during the creation of a memory. We used two-photon microscopy to stimulate individual synapses and to visualize protein trafficking in real time. We identified a unique protein that is rapidly and persistently captured in potentiated synapses\, forming a new macromolecule that could serve as a memory tag. We developed a novel photo-marking technique that allowed us to localize the same synapses under both two-photon and electron microscopies. This way we observed how different synaptic structures evolve asynchronously in three temporal phases during synaptic potentiation.
URL:https://ibecbarcelona.eu/event/ibec-seminar-miquel-bosch-pita-2/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=Europe/Madrid:20151023T100000
DTEND;TZID=Europe/Madrid:20151023T110000
DTSTAMP:20260426T115936
CREATED:20150803T123423Z
LAST-MODIFIED:20150803T123423Z
UID:18434-1445594400-1445598000@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Miquel Bosch Pita
DESCRIPTION:The molecular mechanisms of memory persistence: imaging how single synapses learn in real time\nMiquel Bosch Pita\, Nanoprobes and nanoswitches group\, IBEC\nMemories are stored in our brain through the ability of synaptic connections to modify their structure and function in a long-lasting way. However\, nobody has ever observed how these changes occur in a single synapse in real time.\nI will explain how we used a new combination of optical technologies to reveal the molecular remodeling that takes place inside a synapse during the creation of a memory. We used two-photon microscopy to stimulate individual synapses and to visualize protein trafficking in real time. We identified a unique protein that is rapidly and persistently captured in potentiated synapses\, forming a new macromolecule that could serve as a memory tag. We developed a novel photo-marking technique that allowed us to localize the same synapses under both two-photon and electron microscopies. This way we observed how different synaptic structures evolve asynchronously in three temporal phases during synaptic potentiation.
URL:https://ibecbarcelona.eu/event/ibec-seminar-miquel-bosch-pita/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151022T110000
DTEND;TZID=UTC:20151022T120000
DTSTAMP:20260426T115936
CREATED:20151013T090618Z
LAST-MODIFIED:20170801T131050Z
UID:19216-1445511600-1445515200@ibecbarcelona.eu
SUMMARY:Nanomalaria joint unit seminar: Konstantinos Mitsakakis\, University of Freiburg
DESCRIPTION:LabDisk\, a multi-purpose\, multi-target diagnostic platform for patient management and surveillance at the point-of-care\nDr. Konstantinos Mitsakakis\, Hahn-Schickard & IMTEK\, Department of Microsystems Engineering\, University of Freiburg\, Germany\nThe LabDisk is a CD-shaped microfluidic platform with all reagents integrated for on-site sample-to-answer diagnosis of single or multiple infectious diseases stemming from parasites\, bacteria\, viruses\, or co-infections of theirs. Through “composite” diagnosis\, by combining molecular diagnostics and protein biomarker detection\, the LabDisk offers increased reliability in pathogen species identification. Its modular nature enables the creation of a “disc library” for different sample matrices\, and the rapid adaptation to end-users’ requests (endemic needs\, sudden epidemics outbreaks). \nThe presentation will consist of two sections: (1) description of the LabDisk and its operating principle (modularity\, multiplexity\, fully integrated sample preparation); and (2) an overview of the current infectious disease-related applications\, in particular: neonatal sepsis\, respiratory tract infections\, antibiotic resistance\, febrile tropical infections (malaria\, dengue\, pneumonia\, typhoid)\, mosquito/vector control. \nDr. Mitsakakis has been invited by Xavier Fernàndez Busquets\, Head of Nanomalaria Joint Unit
URL:https://ibecbarcelona.eu/event/ibec-external-seminar-konstantinos-mitsakakis-university-of-freiburg/
LOCATION:Aula 6\, Faculty of Medicine\, Carrer de Casanova\, 143\, Barcelona
CATEGORIES:Joint seminar / workshop / symposium
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151022T110000
DTEND;TZID=UTC:20151022T120000
DTSTAMP:20260426T115936
CREATED:20151013T090618Z
LAST-MODIFIED:20151013T090618Z
UID:95870-1445511600-1445515200@ibecbarcelona.eu
SUMMARY:Nanomalaria joint unit seminar: Konstantinos Mitsakakis\, University of Freiburg
DESCRIPTION:LabDisk\, a multi-purpose\, multi-target diagnostic platform for patient management and surveillance at the point-of-care\nDr. Konstantinos Mitsakakis\, Hahn-Schickard & IMTEK\, Department of Microsystems Engineering\, University of Freiburg\, Germany\nThe LabDisk is a CD-shaped microfluidic platform with all reagents integrated for on-site sample-to-answer diagnosis of single or multiple infectious diseases stemming from parasites\, bacteria\, viruses\, or co-infections of theirs. Through “composite” diagnosis\, by combining molecular diagnostics and protein biomarker detection\, the LabDisk offers increased reliability in pathogen species identification. Its modular nature enables the creation of a “disc library” for different sample matrices\, and the rapid adaptation to end-users’ requests (endemic needs\, sudden epidemics outbreaks). \nThe presentation will consist of two sections: (1) description of the LabDisk and its operating principle (modularity\, multiplexity\, fully integrated sample preparation); and (2) an overview of the current infectious disease-related applications\, in particular: neonatal sepsis\, respiratory tract infections\, antibiotic resistance\, febrile tropical infections (malaria\, dengue\, pneumonia\, typhoid)\, mosquito/vector control. \nDr. Mitsakakis has been invited by Xavier Fernàndez Busquets\, Head of Nanomalaria Joint Unit
URL:https://ibecbarcelona.eu/event/ibec-external-seminar-konstantinos-mitsakakis-university-of-freiburg-2/
LOCATION:Aula 6\, Faculty of Medicine\, Carrer de Casanova\, 143\, Barcelona
CATEGORIES:Joint seminar / workshop / symposium
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151021T113000
DTEND;TZID=UTC:20151021T133000
DTSTAMP:20260426T115936
CREATED:20151015T111927Z
LAST-MODIFIED:20151015T111927Z
UID:19304-1445427000-1445434200@ibecbarcelona.eu
SUMMARY:PhD Thesis Defense: Ana Guaman
DESCRIPTION:“Multivariate Signal Processing for Quantitative and Qualitative analysis of Ion Mobility Spectrometry applied to Biomedical and Food Applications”\n \nAna Guaman\, Signal and information processing for sensing systems group\nAna will be defending her PhD thesis on Wednesday 21st October at 11:30 in the Sala de grados\, Facultad de Física\, UB.  \nEverybody is welcome to attend. \n—\nIf you’re an IBEC PhD student and would like to advertise your PhD defense on the IBEC calendar\, please contact vleigh@ibecbarcelona.eu
URL:https://ibecbarcelona.eu/event/phd-thesis-defense-ana-guaman/
LOCATION:Sala de Graus Eduard Fontseré\, Martí i Franquès\, 1-11\, Barcelona\, 08028
CATEGORIES:PhD Thesis Defence
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151021T113000
DTEND;TZID=UTC:20151021T133000
DTSTAMP:20260426T115936
CREATED:20151015T111927Z
LAST-MODIFIED:20151015T111927Z
UID:95871-1445427000-1445434200@ibecbarcelona.eu
SUMMARY:PhD Thesis Defense: Ana Guaman
DESCRIPTION:“Multivariate Signal Processing for Quantitative and Qualitative analysis of Ion Mobility Spectrometry applied to Biomedical and Food Applications”\n \nAna Guaman\, Signal and information processing for sensing systems group\nAna will be defending her PhD thesis on Wednesday 21st October at 11:30 in the Sala de grados\, Facultad de Física\, UB.  \nEverybody is welcome to attend. \n—\nIf you’re an IBEC PhD student and would like to advertise your PhD defense on the IBEC calendar\, please contact vleigh@ibecbarcelona.eu
URL:https://ibecbarcelona.eu/event/phd-thesis-defense-ana-guaman-2/
LOCATION:Sala de Graus Eduard Fontseré\, Martí i Franquès\, 1-11\, Barcelona\, 08028
CATEGORIES:PhD Thesis Defence
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151019T100000
DTEND;TZID=UTC:20151019T120000
DTSTAMP:20260426T115936
CREATED:20151006T054804Z
LAST-MODIFIED:20151006T054804Z
UID:95869-1445248800-1445256000@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Cell Imaging Day - Molecular Probes
DESCRIPTION:Cell Imaging Day – Molecular Probes\nClara Streiff\, Senior Technical Specialist · Molecular Probes – ThermoFisher Scientific\nSeminar:\n•	Marcaje de estructuras celulares en células vivas (Bacmam Cellight)\n•	Proliferación celular (Click-iT® EdU)\n•	Estrés oxidativo (CellROX®)\n•	Fagocitosis (PHrodo)\n•	Apoptosis (Cellevent Caspase 3 and 7)\n•	Mejorando la señal fluorescente en células vivas y fijadas (ReadyProbes reactivos “ready to use”)\n•	Ventajas de la citometría por focalización acústica (Attune®NxT acoustic focusing cytometer)  \nAl final del seminario podrás pasar tus muestras en el microscopio EVOS® FL AUTO y prueba nuestros reactivos ReadyProbes de Molecular Probes sin compromiso\, reactivos para imaging que permiten marcar tus células sin necesidad de hacer calculos\, diluciones ni pipetear.
URL:https://ibecbarcelona.eu/event/ibec-seminar-cell-imaging-day-molecular-probes-2/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=UTC:20151019T100000
DTEND;TZID=UTC:20151019T120000
DTSTAMP:20260426T115936
CREATED:20151006T054804Z
LAST-MODIFIED:20151006T054804Z
UID:19129-1445248800-1445256000@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Cell Imaging Day - Molecular Probes
DESCRIPTION:Cell Imaging Day – Molecular Probes\nClara Streiff\, Senior Technical Specialist · Molecular Probes – ThermoFisher Scientific\nSeminar:\n•	Marcaje de estructuras celulares en células vivas (Bacmam Cellight)\n•	Proliferación celular (Click-iT® EdU)\n•	Estrés oxidativo (CellROX®)\n•	Fagocitosis (PHrodo)\n•	Apoptosis (Cellevent Caspase 3 and 7)\n•	Mejorando la señal fluorescente en células vivas y fijadas (ReadyProbes reactivos “ready to use”)\n•	Ventajas de la citometría por focalización acústica (Attune®NxT acoustic focusing cytometer)  \nAl final del seminario podrás pasar tus muestras en el microscopio EVOS® FL AUTO y prueba nuestros reactivos ReadyProbes de Molecular Probes sin compromiso\, reactivos para imaging que permiten marcar tus células sin necesidad de hacer calculos\, diluciones ni pipetear.
URL:https://ibecbarcelona.eu/event/ibec-seminar-cell-imaging-day-molecular-probes/
CATEGORIES:IBEC Seminar
END:VEVENT
BEGIN:VEVENT
DTSTART;TZID=Europe/Madrid:20151016T100000
DTEND;TZID=Europe/Madrid:20151016T110000
DTSTAMP:20260426T115936
CREATED:20150713T060412Z
LAST-MODIFIED:20150713T060412Z
UID:95862-1444989600-1444993200@ibecbarcelona.eu
SUMMARY:IBEC Seminar: Lorenzo Albertazzi
DESCRIPTION:Nanoscopy for Nanomedicine: looking at nanomaterials in action one molecule at a time\nLorenzo Albertazzi\, IBEC\nThe use of nanomaterials for biomedical purposes such as drug or gene delivery is one of the key applications of nanotechnology. In this framework a variety of materials have been fabricated\, evaluated in cells and in vivo and\, in some cases\, successfully translated into clinical applications. A crucial factor limiting the design of effective nanocarriers is the lack of knowledge about materials-cell interactions that severely limit the rational design of nanosized devices.\nHere I’ll show how advanced optical microscopy techniques can shine a light on nanomaterials behavior in the biological environment\, helping us to understand structure-activity relationships and to design improved and more effective therapeutic devices. In particular I’ll discuss the ability of super resolution microscopy to image with nanometric resolution nanomaterials interactions with target cells. The potential and the applications of the technique will be discussed\, with particular emphasis on the study of self-assembled bio-inspired materials.
URL:https://ibecbarcelona.eu/event/ibec-seminar-lorenzo-albertazzi-2/
CATEGORIES:IBEC Seminar
END:VEVENT
END:VCALENDAR