Results for 'fluorescence'

92 found
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  1.  27
    Fluorescence correlation spectroscopy.Jonas Ries & Petra Schwille - 2012 - Bioessays 34 (5):361-368.
    Fluorescence correlation spectroscopy (FCS) is a powerful technique to measure concentrations, mobilities, and interactions of fluorescent biomolecules. It can be applied to various biological systems such as simple homogeneous solutions, cells, artificial, or cellular membranes and whole organisms. Here, we introduce the basic principle of FCS, discuss its application to biological questions as well as its limitations and challenges, present an overview of novel technical developments to overcome those challenges, and conclude with speculations about the future applications of (...) fluctuation spectroscopy. (shrink)
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  2.  51
    Fluorescent proteins for FRET microscopy: Monitoring protein interactions in living cells.Richard N. Day & Michael W. Davidson - 2012 - Bioessays 34 (5):341-350.
    The discovery and engineering of novel fluorescent proteins (FPs) from diverse organisms is yielding fluorophores with exceptional characteristics for live‐cell imaging. In particular, the development of FPs for fluorescence (or Förster) resonance energy transfer (FRET) microscopy is providing important tools for monitoring dynamic protein interactions inside living cells. The increased interest in FRET microscopy has driven the development of many different methods to measure FRET. However, the interpretation of FRET measurements is complicated by several factors including the high (...) background, the potential for photoconversion artifacts and the relatively low dynamic range afforded by this technique. Here, we describe the advantages and disadvantages of four methods commonly used in FRET microscopy. We then discuss the selection of FPs for the different FRET methods, identifying the most useful FP candidates for FRET microscopy. The recent success in expanding the FP color palette offers the opportunity to explore new FRET pairs. (shrink)
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  3.  37
    Phototoxicity in live fluorescence microscopy, and how to avoid it.Jaroslav Icha, Michael Weber, Jennifer C. Waters & Caren Norden - 2017 - Bioessays 39 (8):1700003.
    Phototoxicity frequently occurs during live fluorescence microscopy, and its consequences are often underestimated. Damage to cellular macromolecules upon excitation light illumination can impair sample physiology, and even lead to sample death. In this review, we explain how phototoxicity influences live samples, and we highlight that, besides the obvious effects of phototoxicity, there are often subtler consequences of illumination that are imperceptible when only the morphology of samples is examined. Such less apparent manifestations of phototoxicity are equally problematic, and can (...)
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  4.  20
    Image analysis in fluorescence microscopy: Bacterial dynamics as a case study.Sven van Teeffelen, Joshua W. Shaevitz & Zemer Gitai - 2012 - Bioessays 34 (5):427-436.
    Fluorescence microscopy is the primary tool for studying complex processes inside individual living cells. Technical advances in both molecular biology and microscopy have made it possible to image cells from many genetic and environmental backgrounds. These images contain a vast amount of information, which is often hidden behind various sources of noise, convoluted with other information and stochastic in nature. Accessing the desired biological information therefore requires new tools of computational image analysis and modeling. Here, we review some of (...)
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  5.  26
    Fluorescence correlation spectroscopy for the detection and study of single molecules in biology.Miguel Ángel Medina & Petra Schwille - 2002 - Bioessays 24 (8):758-764.
    The recent development of single molecule detection techniques has opened new horizons for the study of individual macromolecules under physiological conditions. Conformational subpopulations, internal dynamics and activity of single biomolecules, parameters that have so far been hidden in large ensemble averages, are now being unveiled. Herein, we review a particular attractive solution‐based single molecule technique, fluorescence correlation spectroscopy (FCS). This time‐averaging fluctuation analysis which is usually performed in Confocal setups combines maximum sensitivity with high statistical confidence. FCS has proven (...)
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  6. Fluorescent tags of protein function in living cells.Michael Whitaker - 2000 - Bioessays 22 (2):180-187.
    A cell's biochemistry is now known to be the biochemistry of molecular machines, that is, protein complexes that are assembled and dismantled in particular locations within the cell as needed. One important element in our understanding has been the ability to begin to see where proteins are in cells and what they are doing as they go about their business. Accordingly, there is now a strong impetus to discover new ways of looking at the workings of proteins in living cells. (...)
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  7.  10
    White Fluorescent Light.Justin H. Price - 2016 - Journal of Medical Humanities 37 (3):351-351.
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  8.  18
    Fluorescent aporetics: Nicholas Rescher: Aporetics: rational deliberation in the face of inconsistency. University of Pittsburgh Press, Pittsburgh, 2009, 161 pp, £26.50 HB.Peter Vickers - 2010 - Metascience 19 (1):105-108.
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  9.  22
    Family of the green fluorescent protein: Journey to the end of the rainbow.Mikhail V. Matz, Konstantin A. Lukyanov & Sergey A. Lukyanov - 2002 - Bioessays 24 (10):953-959.
    Members of the family of the Green Fluorescent Protein (GFP) are the only known type of natural pigments that are essentially encoded by a single gene, since both the substrate for pigment biosynthesis and the necessary catalytic moieties are provided within a single polypeptide chain. In sharp contrast to the state of knowledge just three years ago when GFP was the only known protein of its kind, a whole family of related proteins, exhibiting striking diversity of features have now been (...)
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  10.  26
    Characterization of chromatin domains by 3D fluorescence microscopy: An automated methodology for quantitative analysis and nuclei screening.Sylvain Cantaloube, Kelly Romeo, Patricia Le Baccon, Geneviève Almouzni & Jean-Pierre Quivy - 2012 - Bioessays 34 (6):509-517.
    Fluorescence microscopy has provided a route to qualitatively analyze features of nuclear structures and chromatin domains with increasing resolution. However, it is becoming increasingly important to develop tools for quantitative analysis. Here, we present an automated method to quantitatively determine the enrichment of several endogenous factors, immunostained in pericentric heterochromatin domains in mouse cells. We show that this method permits an unbiased characterization of changes in the enrichment of several factors with statistical significance from a large number of nuclei. (...)
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  11.  7
    Fluorescence microscopy Methods in Cell Biology 29 Fluorescence microscopy of living cells in culture. Part A: Fluorescence analogs, labeling cells and basic microscopy (1989). Edited by Y.‐L. Wang & D. L. Taylor. Academic Press, New York. Pp 333. $59.00. [REVIEW]David M. Schotten - 1990 - Bioessays 12 (1):50-51.
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  12.  13
    Simultaneous measurement of fluorescence anisotropy and translational fluctuations by polarization-modulated MFICS.M. C. Fink & A. H. Marcus - 2008 - Philosophical Magazine 88 (33-35):3947-3951.
  13.  17
    Rapid detection of selected aneuploidies by quantitative fluorescent PCR.Matteo Adinolfi, Jon Sherlock & Barbara Pertl - 1995 - Bioessays 17 (7):661-664.
    Selected aneuploidies can be rapidly diagnosed by the analysis of fluorescent polymerase chain reaction (PCR) products of chromosome‐specific and highly polymorphic small tandem repeats (STRs). The quantitative STR patterns obtained from samples of normal individuals are markedly different from those seen when patients with aneuploidies involving chromosome X, or trisomies of chromosomes 21 and 18, are tested. For example, while samples from normal subjects – tested with a chromosome 21‐derived STR (D21S11) – show two fluorescent PCR peaks with similar activities (...)
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  14.  9
    Multifrequency cross‐correlation phase fluorometry of chlorophyll a fluorescence in thylakoid and psii‐enriched membranes. Covindjee, M. Van de Ven, J. Cao, C. Roye & E. Gratton - unknown
    — We prescnt here a comparative study on the decay of chlorophyll a fluorescence yield in thylakoid membranes and photosystem 11 ‐enriched samples, measured with multifrequency cross‐correlation phase fluorometry. These measurements confirm the general conclusions of Van Mieghem ef al., obtained with a flash method, on the effects of reduction of the primary quinone acceptor on ChI a fluorescence yield of PSI. Different states of the reaction centers of PSII were produced by: pretreatment with sodium dithionite and mcthyl (...)
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  15.  29
    Fluorescence microscopy revisited Fluorescence Microscopy of Living Cells in Culture_, Part B, _Quantitative Fluorescence Microscopy – Imaging and spectroscopy(1989). Edited by D. Lansing Taylor and YU‐LI Wang. Methods in Cell Biology 30. Academic Press: New York. 503pp. £94. [REVIEW]David M. Shotton - 1992 - Bioessays 14 (6):427-429.
  16. Does indodicarbocyanine fluorescence reflect membrane potential of the sarcoplasmic reticulum in skeletal muscle.Hans Oetliker - 1981 - In G. Adam, I. Meszaros & E. I. Banyai (eds.), Advances in Physiological Science. pp. 5--345.
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  17.  30
    Affective and cognitive reactions to subliminal flicker from fluorescent lighting.Igor Knez - 2014 - Consciousness and Cognition 26:97-104.
    This study renews the classical concept of subliminal perception by investigating the impact of subliminal flicker from fluorescent lighting on affect and cognitive performance. It was predicted that low compared to high frequency lighting would evoke larger changes in affective states and also impair cognitive performance. Subjects reported high rather than low frequency lighting to be more pleasant, which, in turn, enhanced their problem solving performance. This suggests that sensory processing can take place outside of conscious awareness resulting in conscious (...)
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  18.  12
    The lipid raft hypothesis revisited – New insights on raft composition and function from super‐resolution fluorescence microscopy.Dylan M. Owen, Astrid Magenau, David Williamson & Katharina Gaus - 2012 - Bioessays 34 (9):739-747.
    Recently developed super‐resolution microscopy techniques are changing our understanding of lipid rafts and membrane organisation in general. The lipid raft hypothesis postulates that cholesterol can drive the formation of ordered domains within the plasma membrane of cells, which may serve as platforms for cell signalling and membrane trafficking. There is now a wealth of evidence for these domains. However, their study has hitherto been hampered by the resolution limit of optical microscopy, making the definition of their properties problematic and contentious. (...)
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  19.  21
    Microlight takes flight fluorescent and luminescent probes for biological activity: A practical guide to technology for quantitative real‐time analysis (1993). Edited by W. T. Mason. Series: “Biological Techniques”. Series Editor, D. B. Sattelle. Academic Press, London. 433 pp. £40. ISBN 0‐124‐77830‐5. [REVIEW]Roger B. Moreton - 1993 - Bioessays 15 (12):841-842.
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  20.  22
    Mobility of adsorbed Cry1Aa insecticidal toxin fromBacillus thuringiensis on montmorillonite measured by fluorescence recovery after photobleaching.Nordine Helassa, Gabrielle Daudin, Sylvie Noinville, Jean-Marc Janot, Philippe Déjardin, Siobhán Staunton & Hervé Quiquampoix - 2010 - Philosophical Magazine 90 (17-18):2365-2371.
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  21.  9
    18. Geochemical analysis using portable X-ray fluorescence.Kate Welham, Paul N. Cheetham & Rebecca J. S. Cannell - 2017 - In Dagfinn Skre (ed.), Avaldsnes - a Sea-Kings' Manor in First-Millennium Western Scandinavia. De Gruyter. pp. 421-454.
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  22.  20
    Fluorogenic Protein‐Based Strategies for Detection, Actuation, and Sensing.Arnaud Gautier & Alison G. Tebo - 2018 - Bioessays 40 (10):1800118.
    Fluorescence imaging has become an indispensable tool in cell and molecular biology. GFP‐like fluorescent proteins have revolutionized fluorescence microscopy, giving experimenters exquisite control over the localization and specificity of tagged constructs. However, these systems present certain drawbacks and as such, alternative systems based on a fluorogenic interaction between a chromophore and a protein have been developed. While these systems are initially designed as fluorescent labels, they also present new opportunities for the development of novel labeling and detection strategies. (...)
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  23.  18
    Single particle imaging of mRNAs crossing the nuclear pore: Surfing on the edge.Alexander F. Palazzo & Mathew Truong - 2016 - Bioessays 38 (8):744-750.
    Six years ago, the Singer lab published a landmark paper which described how individual mRNA particles cross the nuclear pore complex in mammalian tissue culture cells. This involved the simultaneous imaging of mRNAs, each labeled by a large number of tethered fluorescent proteins and fluorescently tagged nuclear pore components. Now two groups have applied this technique to the budding yeast Saccharomyces cerevisiae. Their results indicate that in the course of nuclear export, mRNAs likely engage complexes that are present on either (...)
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  24.  20
    Watching the embryo: Evolution of the microscope for the study of embryogenesis.Sharada Iyer, Sulagna Mukherjee & Megha Kumar - 2021 - Bioessays 43 (6):2000238.
    Embryos and microscopes share a long, remarkable history and biologists have always been intrigued to watch how embryos develop under the microscope. Here we discuss the advances in microscopy which have greatly influenced our current understanding of embryogenesis. We highlight the evolution of microscopes and the optical technologies that have been instrumental in studying various developmental processes. These imaging modalities provide mechanistic insights into the dynamic cellular and molecular events which drive lineage commitment and morphogenetic changes in the developing embryo. (...)
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  25.  11
    What precision‐protein‐tuning and nano‐resolved single molecule sciences can do for each other.Sigrid Milles & Edward A. Lemke - 2013 - Bioessays 35 (1):65-74.
    While innovations in modern microscopy, spectroscopy, and nanoscopy techniques have made single molecule observation a standard in many laboratories, the actual design of meaningful fluorescence reporter systems now hinders major scientific breakthroughs. Even though the field of chemical biology is supercharging the fluorescence toolbox, surprisingly few strategies exist that make the transition from model systems to biologically relevant applications. At the same time, the number of microscopy techniques is growing dramatically. We explain our view on how the impact (...)
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  26.  10
    Single‐molecule pull‐down (SiMPull) for new‐age biochemistry.Vasudha Aggarwal & Taekjip Ha - 2014 - Bioessays 36 (11):1109-1119.
    Macromolecular interactions play a central role in many biological processes. Protein‐protein interactions have mostly been studied by co‐immunoprecipitation, which cannot provide quantitative information on all possible molecular connections present in the complex. We will review a new approach that allows cellular proteins and biomolecular complexes to be studied in real‐time at the single‐molecule level. This technique is called single‐molecule pull‐down (SiMPull), because it integrates principles of conventional immunoprecipitation with the powerful single‐molecule fluorescence microscopy. SiMPull is used to count how (...)
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  27.  19
    Reading the invisible: the role of optical investigations in the study of the Herculaneum papyri.Sveva Longo, Sabrina Samela, Claudia Caliri, Danilo Paolo Pavone, Francesco Paolo Romano, Francesca Rosi, Graziano Ranocchia & Costanza Miliani - unknown
    Herculaneum papyri found during the discovery of the Villa dei Papiri in the XVIII century are our only knowledge about Greek philosophical schools. Unfortunately, the original manuscripts are in a precarious state of conservation and the currently available editions of them have largely been made obsolete by the latest technological progress. The aim of the Advanced Grant ERC project ‘Greekschools’ is to provide a new protocol based on optical methods to increase the text reading and thus allow for a new (...)
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  28.  20
    FRET microscopy in the living cell: Different approaches, strengths and weaknesses.Sergi Padilla-Parra & Marc Tramier - 2012 - Bioessays 34 (5):369-376.
    New imaging methodologies in quantitative fluorescence microscopy, such as Förster resonance energy transfer (FRET), have been developed in the last few years and are beginning to be extensively applied to biological problems. FRET is employed for the detection and quantification of protein interactions, and of biochemical activities. Herein, we review the different methods to measure FRET in microscopy, and more importantly, their strengths and weaknesses. In our opinion, fluorescence lifetime imaging microscopy (FLIM) is advantageous for detecting inter‐molecular interactions (...)
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  29.  13
    SHG nanoprobes: Advancing harmonic imaging in biology.William P. Dempsey, Scott E. Fraser & Periklis Pantazis - 2012 - Bioessays 34 (5):351-360.
    Second harmonic generating (SHG) nanoprobes have recently emerged as versatile and durable labels suitable for in vivo imaging, circumventing many of the inherent drawbacks encountered with classical fluorescent probes. Since their nanocrystalline structure lacks a central point of symmetry, they are capable of generating second harmonic signal under intense illumination – converting two photons into one photon of half the incident wavelength – and can be detected by conventional two‐photon microscopy. Because the optical signal of SHG nanoprobes is based on (...)
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  30.  21
    Single Pair Förster Resonance Energy Transfer: A Versatile Tool To Investigate Protein Conformational Dynamics.Lena Voith von Voithenberg & Don C. Lamb - 2018 - Bioessays 40 (3):1700078.
    Conformational changes of proteins and other biomolecules play a fundamental role in their functional mechanism. Single pair Förster resonance energy transfer offers the possibility to detect these conformational changes and dynamics, and to characterize their underlying kinetics. Using spFRET on microscopes with different modes of detection, dynamic timescales ranging from nanoseconds to seconds can be quantified. Confocal microscopy can be used as a means to analyze dynamics in the range of nanoseconds to milliseconds, while total internal reflection fluorescence microscopy (...)
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  31.  10
    Fish technology in chromosome and genome research.Henry H. Q. Heng, Barbara Spyropoulos & Peter B. Moens - 1997 - Bioessays 19 (1):75-84.
    Fluorescent in situ hybridization technology is one of the most exciting and versatile research tools to be developed in recent years. It has enabled research to progress at a phenomenal rate in diverse areas of basic research as well as in clinical medicine. Fluorescent in situ hybridization has applications in physical mapping, the study of nuclear architecture and chromatin packaging, and the investigation of fundamental principles of biology such as DNA replication, RNA processing, gene amplification, gene integration and chromatin elimination. (...)
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  32.  7
    New approaches for low phototoxicity imaging of living cells and tissues.Wiktoria Kasprzycka, Wiktoria Szumigraj, Przemysław Wachulak & Elżbieta Anna Trafny - 2024 - Bioessays 46 (5):2300122.
    Fluorescence microscopy is a powerful tool used in scientific and medical research, but it is inextricably linked to phototoxicity. Neglecting phototoxicity can lead to erroneous or inconclusive results. Recently, several reports have addressed this issue, but it is still underestimated by many researchers, even though it can lead to cell death. Phototoxicity can be reduced by appropriate microscopic techniques and carefully designed experiments. This review focuses on recent strategies to reduce phototoxicity in microscopic imaging of living cells and tissues. (...)
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  33.  18
    Raman spectroscopy is a powerful tool in molecular paleobiology: An analytical response to Alleon et al. (https://doi.org/10.1002/bies.202000295). [REVIEW]Jasmina Wiemann & Derek E. G. Briggs - 2022 - Bioessays 44 (2):2100070.
    A recent article argued that signals from conventional Raman spectroscopy of organic materials are overwhelmed by edge filter and fluorescence artefacts. The article targeted a subset of Raman spectroscopic investigations of fossil and modern organisms and has implications for the utility of conventional Raman spectroscopy in comparative tissue analytics. The inferences were based on circular reasoning centered around the unconventional analysis of spectra from just two samples, one modern, and one fossil. We validated the disputed signals with in situ (...)
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  34.  29
    Other People's Stories.Nell Burger Kirst - 2011 - Hastings Center Report 41 (5):9-10.
    There is a bustling, fluorescent clamor that governs hospital hallways during the day and so fills the air that any sound wanting attention has to vie for it, each alarm louder and more cacophonous than the last. But at night, an altogether different temper settles over the hospital. A restrained, low-lit quiet descends, transforming those long corridors into a space that seems smaller and almost comforting. Almost any sound stands out at night. I was once trudging down one of those (...)
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  35.  17
    Luminescent sensing and imaging of oxygen: Fierce competition to the Clark electrode.Otto S. Wolfbeis - 2015 - Bioessays 37 (8):921-928.
    Luminescence‐based sensing schemes for oxygen have experienced a fast growth and are in the process of replacing the Clark electrode in many fields. Unlike electrodes, sensing is not limited to point measurements via fiber optic microsensors, but includes additional features such as planar sensing, imaging, and intracellular assays using nanosized sensor particles. In this essay, I review and discuss the essentials of (i) common solid‐state sensor approaches based on the use of luminescent indicator dyes and host polymers; (ii) fiber optic (...)
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  36.  44
    Materiality and sublimation in Dan Flavin's luminous minimalism.Vangelis Giannakakis - 2021 - Zeitschrift für Ästhetik Und Allgemeine Kunstwissenschaft (Special issue / Sonderheft 19):313-330.
    Modern aesthetic Minimalism is neither a flight to abstract spirituality, nor an extracting process of a primordial essence. It is concerned, rather, with the aesthetic object as pure refiguration and the production of “concrete universality”, of form as content and possibility of itself. This becomes especially apparent in the Minimalism of the 1960s. The main focus of this paper will be on Dan Flavin’s luminous minimalism. The latter is characterised by a style that, though simple in appearance, introduced a higher (...)
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  37.  15
    The Lab in the Museum. Or, Using New Scientific Instruments to Look at Old Scientific Instruments.Boris Jardine & Joshua Nall - 2023 - Centaurus 65 (2):261-289.
    This paper explores the use of new scientific techniques to examine collections of historic scientific apparatus and other technological artefacts. One project under discussion uses interferometry to examine the history of lens development, while another uses X-ray fluorescence to discover the kinds of materials used to make early mathematical and astronomical instruments. These methods lead to surprising findings: instruments turn out to be fake, and lens makers turn out to have been adept at solving the riddle of aperture. Although (...)
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  38.  69
    Media ethics on a higher order of magnitude.Clifford G. Christians - 2008 - Journal of Mass Media Ethics 23 (1):3 – 14.
    Between Summits I and II, media ethics established its legitimacy, summarized into recommendations for the field's future fluorescence. This history points to the challenges through which media ethics moves to another order of magnitude. A historical map of media ethics scholarship since 1980 divides into 5 domains, and each is introduced: theory, social philosophy, religious ethics, technology, and truth. From this content analysis of the literature, an agenda emerges for research and academic study that can raise media ethics to (...)
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  39.  34
    Molecular bioelectricity in developmental biology: New tools and recent discoveries.Michael Levin - 2012 - Bioessays 34 (3):205-217.
    Significant progress in the molecular investigation of endogenous bioelectric signals during pattern formation in growing tissues has been enabled by recently developed techniques. Ion flows and voltage gradients produced by ion channels and pumps are key regulators of cell proliferation, migration, and differentiation. Now, instructive roles for bioelectrical gradients in embryogenesis, regeneration, and neoplasm are being revealed through the use of fluorescent voltage reporters and functional experiments using well‐characterized channel mutants. Transmembrane voltage gradients (Vmem) determine anatomical polarity and function as (...)
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  40.  14
    Autism and the Right to a Hypersensitivity-Friendly Workspace.Bouke de Vries - 2021 - Public Health Ethics 14 (3):281-287.
    Many individuals on the autism spectrum are hypersensitive to certain sensory stimuli. For this group, as well as for non-autistic individuals with sensory processing disorders, being exposed to e.g. fluorescent lights, perfume odours, and various sounds and noises can be real torment. In this article, I consider the normative implications of such offence for the design of office spaces, which is a topic that has not received any attention from philosophers. After identifying different ways in which the senses of hypersensitive (...)
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  41.  20
    Computing with Synthetic Protocells.Angélique Stéphanou & Nicolas Glade - 2015 - Acta Biotheoretica 63 (3):309-323.
    In this article we present a new kind of computing device that uses biochemical reactions networks as building blocks to implement logic gates. The architecture of a computing machine relies on these generic and composable building blocks, computation units, that can be used in multiple instances to perform complex boolean functions. Standard logical operations are implemented by biochemical networks, encapsulated and insulated within synthetic vesicles called protocells. These protocells are capable of exchanging energy and information with each other through transmembrane (...)
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  42.  48
    Engineering Novel Proteins with Orthogonal tRNA: Artificial Causes that make a Difference.Janella Baxter - manuscript
    Model organisms, the use of green fluorescent proteins, and orthogonal transfer RNA are examples of artificial causes being used in biology. Recent work characterizing the research interests of biologists in terms of a common set of values has ruled out artificial causes as biologically interesting. For instance, Kenneth Waters argues that biologists are primarily interested in causes that actually obtain. Similarly, Marcel Weber argues that biologists are primarily concerned with biologically normal interventions. Both views express a widely received attitude about (...)
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  43.  37
    Flow cytometric analysis of the cell cycle: Mathematical modeling and biological interpretation.José Pierrez & Xavier Ronot - 1992 - Acta Biotheoretica 40 (2-3):131-137.
    Estimation of the repartition of asynchronous cells in the cell cycle can be explained by two hypotheses:– - the cells are supposed to be distributed into three groups: cells with a 2c DNA content (G0/1 phase), cells with a 4c DNA content (G2+M phase) and cells with a DNA content ranging from 2c to 4c (S phase); – - there is a linear relationship between the amount of fluorescence emitted by the fluorescent probe which reveals the DNA and the (...)
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  44. A methodological approach for pattern recognition system using discriminant analysis and artificial neural networks.Anna Pérez-Méndez, Elizabeth Torres-Rivas, Francklin Rivas-Echeverría & Ronald Maldonado-Rodríguez - 2005 - Cognitive Science 13 (14):15.
    In this work it is presented a methodology for the development of a pattern recognition system using classification methods as discriminant analysis and artificial neural networks. In this methodology, the statistical analysis is contemplated, with the purpose of retaining the observations and the important characteristics that can produce an appropriate classification, and allows, as well, to detect outliers’ observations, multicolinearity between variables, among other things. Chlorophyll a fluorescence OJIP signals measured from Pisum sativum leaves belonging to different drought stress (...)
     
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  45.  21
    Hello, We're Philosophy in the Wild.Zachary Agoff, Mike Gadomski & Maja Sidzinska - 2023 - Philosophy in the Wild Collection.
    This article introduces the Philosophy in the Wild collection. Philosophy in the Wild asks how ways of doing philosophy impact the kinds of philosophy being done and the kinds of philosophical engagement that are possible. We think that taking philosophy outside of its usual fluorescent, wired context would open up new ways of theorizing our relation to the world, as well as create new ways of engaging with philosophy. Thus Philosophy in the Wild hosts outdoor and technology-free conferences and workshops. (...)
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  46.  16
    Genome analysis with gene expression microarrays.Mark Schena - 1996 - Bioessays 18 (5):427-431.
    Advances in biochemistry, chemistry and engineering have enabled the development of a new gene expression assay. This ‘chip‐based’ approach utilizes microscopic arrays of cDNAs printed on glass as high‐density hybridization targets. Fluorescent probe mixtures derived from total cellular messenger RNA (mRNA) hybridize to cognate elements on the array, allowing accurate measurement of the expression of the corresponding genes. Array densities of >1,000 cDNAs per cm2 enable quantitative expression monitoring of a large number of genes in a single hybridization. A two‐color (...)
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  47.  46
    Trusting in the 'efficacy of beauty': A kalocentric approach to moral philosophy.Brian G. Henning - 2009 - Ethics and the Environment 14 (1):pp. 101-128.
    Although debates over carbon taxes and trading schemes, over carbon offsets and compact fluorescents are important, our efforts to address the environmental challenges that we face will fall short unless and until we also set about the difficult work of reconceiving who we are and how we are related to our processive cosmos. What is needed, I argue, are new ways of thinking and acting grounded in new ways of understanding ourselves and our relationship to the world, ways of understanding (...)
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  48.  46
    The potential of 3D‐FISH and super‐resolution structured illumination microscopy for studies of 3D nuclear architecture.Yolanda Markaki, Daniel Smeets, Susanne Fiedler, Volker J. Schmid, Lothar Schermelleh, Thomas Cremer & Marion Cremer - 2012 - Bioessays 34 (5):412-426.
    Three‐dimensional structured illumination microscopy (3D‐SIM) has opened up new possibilities to study nuclear architecture at the ultrastructural level down to the ∼100 nm range. We present first results and assess the potential using 3D‐SIM in combination with 3D fluorescence in situ hybridization (3D‐FISH) for the topographical analysis of defined nuclear targets. Our study also deals with the concern that artifacts produced by FISH may counteract the gain in resolution. We address the topography of DAPI‐stained DNA in nuclei before and (...)
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  49.  29
    Learning in the Open Air.Amanda Corris - 2022 - Public Philosophy Journal 4.
    The typical college lecture hall is a highly artificial environment: windowless, fluorescent-lit, and technology-heavy. It all but necessitates treating students as mental receptacles, where learning is a matter of passive absorption of knowledge, and where it is increasingly difficult to hold students’ attention. Natural environments, such as forests and public parks, provide a striking comparison—they free us from technological distractions, invigorate our senses, and encourage physical in addition to mental exploration. What’s more, research in environmental psychology suggests that natural environments (...)
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  50.  21
    Change in the graphics of journal articles in the life sciences field: analysis of figures and tables in the journal “Cell”.Kana Ariga & Manabu Tashiro - 2022 - History and Philosophy of the Life Sciences 44 (3):1-34.
    The purpose of this study is to examine how trends in the use of images in modern life science journals have changed since the spread of computer-based visual and imaging technology. To this end, a new classification system was constructed to analyze how the graphics of a scientific journal have changed over the years. The focus was on one international peer-reviewed journal in life sciences, Cell, which was founded in 1974, whereby 1725 figures and 160 tables from the research articles (...)
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