Your search keyword '"Jonathan B. Grimm"' showing total 3 results

1. Optimization of fluorophores for chemical tagging and immunohistochemistry of Drosophila neurons

Author

Rebecca M. Johnston, Sebastian Cachero, Luke D. Lavis, Jonathan B. Grimm, Gregory S.X.E. Jefferis, Ben Sutcliffe, Geoffrey W. Meissner, Julian Ng, Oz Malkesman, Apollo-University Of Cambridge Repository, Jefferis, Gregory [0000-0002-0587-9355], and Apollo - University of Cambridge Repository

Subjects

0301 basic medicine, Neuropil, lcsh:Medicine, Animals, Genetically Modified, chemistry.chemical_compound, 0302 clinical medicine, Signal quality, Animal Cells, Medicine and Health Sciences, lcsh:Science, Cross Reactivity, Neurons, Liquid Chromatography, Multidisciplinary, Tissue clearing, Microscopy, Confocal, biology, Molecular Structure, Chemistry, Drosophila Melanogaster, Chromatographic Techniques, Brain, Eukaryota, Esters, General Medicine, Animal Models, Immunohistochemistry, 3. Good health, Cell biology, Insects, Experimental Organism Systems, Optical Equipment, Physical Sciences, Engineering and Technology, Female, Drosophila, Drosophila melanogaster, Cellular Types, General Agricultural and Biological Sciences, Research Article, Fluorophore, Arthropoda, Transgene, education, Immunology, Equipment, Glial Cells, Research and Analysis Methods, General Biochemistry, Genetics and Molecular Biology, 03 medical and health sciences, Model Organisms, Animals, Drosophila (subgenus), Immunohistochemistry Techniques, Alexa Fluor, Fluorescent Dyes, Staining and Labeling, Lasers, lcsh:R, Organisms, Chemical Compounds, Biology and Life Sciences, Cell Biology, biology.organism_classification, Invertebrates, High Performance Liquid Chromatography, Histochemistry and Cytochemistry Techniques, 030104 developmental biology, Cellular Neuroscience, Immunologic Techniques, lcsh:Q, 030217 neurology & neurosurgery, Neuroscience

Abstract

The use of genetically encoded ‘self-labeling tags’ with chemical fluorophore ligands enables rapid labeling of specific cells in neural tissue. To improve the chemical tagging of neurons, we synthesized and evaluated new fluorophore ligands based on Cy, Janelia Fluor, Alexa Fluor, and ATTO dyes and tested these with recently improved Drosophila melanogaster transgenes. We found that tissue clearing and mounting in DPX substantially improves signal quality when combined with specific non-cyanine fluorophores. We compared and combined this labeling technique with standard immunohistochemistry in the Drosophila brain.

Published

2018

2. Correlative Photoactivated Localization and Scanning Electron Microscopy

Author

Harald F. Hess, Gleb Shtengel, David A. Clayton, Benjamin G. Kopek, and Jonathan B. Grimm

Subjects

Fluorescence-lifetime imaging microscopy, Fluorophore, Phalloidine, lcsh:Medicine, Context (language use), law.invention, Mice, chemistry.chemical_compound, Imaging, Three-Dimensional, law, Microscopy, Peroxisomes, Fluorescence microscope, Microtome, Animals, Photoactivated localization microscopy, lcsh:Science, Nuclear Lamina, Multidisciplinary, Staining and Labeling, Chemistry, lcsh:R, Microtomy, Actins, Mitochondria, Cell biology, Microscopy, Fluorescence, Microscopy, Electron, Scanning, NIH 3T3 Cells, Biophysics, lcsh:Q, Electron microscope, Cryoultramicrotomy, Research Article

Abstract

The ability to localize proteins precisely within subcellular space is crucial to understanding the functioning of biological systems. Recently, we described a protocol that correlates a precise map of fluorescent fusion proteins localized using three-dimensional super-resolution optical microscopy with the fine ultrastructural context of three-dimensional electron micrographs. While it achieved the difficult simultaneous objectives of high photoactivated fluorophore preservation and ultrastructure preservation, it required a super-resolution optical and specialized electron microscope that is not available to many researchers. We present here a faster and more practical protocol with the advantage of a simpler two-dimensional optical (Photoactivated Localization Microscopy (PALM)) and scanning electron microscope (SEM) system that retains the often mutually exclusive attributes of fluorophore preservation and ultrastructure preservation. As before, cryosections were prepared using the Tokuyasu protocol, but the staining protocol was modified to be amenable for use in a standard SEM without the need for focused ion beam ablation. We show the versatility of this technique by labeling different cellular compartments and structures including mitochondrial nucleoids, peroxisomes, and the nuclear lamina. We also demonstrate simultaneous two-color PALM imaging with correlated electron micrographs. Lastly, this technique can be used with small-molecule dyes as demonstrated with actin labeling using phalloidin conjugated to a caged dye. By retaining the dense protein labeling expected for super-resolution microscopy combined with ultrastructural preservation, simplifying the tools required for correlative microscopy, and expanding the number of useful labels we expect this method to be accessible and valuable to a wide variety of researchers.

Published

2013

3. Optimization of fluorophores for chemical tagging and immunohistochemistry of Drosophila neurons.

Author

Geoffrey W Meissner, Jonathan B Grimm, Rebecca M Johnston, Ben Sutcliffe, Julian Ng, Gregory S X E Jefferis, Sebastian Cachero, Luke D Lavis, and Oz Malkesman

Subjects

Medicine, Science

Abstract

The use of genetically encoded 'self-labeling tags' with chemical fluorophore ligands enables rapid labeling of specific cells in neural tissue. To improve the chemical tagging of neurons, we synthesized and evaluated new fluorophore ligands based on Cy, Janelia Fluor, Alexa Fluor, and ATTO dyes and tested these with recently improved Drosophila melanogaster transgenes. We found that tissue clearing and mounting in DPX substantially improves signal quality when combined with specific non-cyanine fluorophores. We compared and combined this labeling technique with standard immunohistochemistry in the Drosophila brain.

Published

2018