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C.M. Taisne

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The composition, conformation, and function of most macromolecular complexes depend on their cellular context and must be studied inside cells. Few cells are sufficiently thin to permit direct imaging with cryoelectron microscopy (cryo-EM). Focused ion beam milling enables cryo-EM to visualize macromolecules in cells at high resolution by generating thin sections of frozen-hydrated cells. We show how thin cellular sections can be prepared in a controlled fashion using an integrated light microscope coincident with electron and ion beams. The procedure provides live feedback on the thickness and uniformity of the prepared lamella, reducing complexity and increasing the success rate. Combined with its ability for fluorescence-based targeting, our procedure paves the way toward an automated workflow that allows for control over lamella quality, thickness, and target inclusion, facilitating the routine fabrication of frozen-hydrated cellular sections. ...
Guanylate-binding proteins (GBPs) are interferon-inducible guanosine triphosphate hydrolases (GTPases) mediating host defense against intracellular pathogens. Their antimicrobial activity hinges on their ability to self-associate and coat pathogen-associated compartments or cytosolic bacteria. Coat formation depends on GTPase activity but how nucleotide binding and hydrolysis prime coat formation remains unclear. Here, we report the cryo-electron microscopy structure of the full-length human GBP1 dimer in its guanine nucleotide-bound state and describe the molecular ultrastructure of the GBP1 coat on liposomes and bacterial lipopolysaccharide membranes. Conformational changes of the middle and GTPase effector domains expose the isoprenylated C terminus for membrane association. The α-helical middle domains form a parallel, crossover arrangement essential for coat formation and position the extended effector domain for intercalation into the lipopolysaccharide layer of gram-negative membranes. Nucleotide binding and hydrolysis create oligomeric scaffolds with contractile abilities that promote membrane extrusion and fragmentation. Our data offer a structural and mechanistic framework for understanding GBP1 effector functions in intracellular immunity. ...
Journal article (2023) - Radim Skoupý, Daan B. Boltje, Miroslav Slouf, Kateřina Mrázová, Tomáš Láznička, Clémence M. Taisne, Vladislav Krzyžánek, Jacob P. Hoogenboom, Arjen J. Jakobi
A quantitative four-dimensional scanning transmission electron microscopy (4D-STEM) imaging technique (q4STEM) for local thickness estimation across amorphous specimen such as obtained by focused ion beam (FIB)-milling of lamellae for (cryo-)TEM analysis is presented. This study is based on measuring spatially resolved diffraction patterns to obtain the angular distribution of electron scattering, or the ratio of integrated virtual dark and bright field STEM signals, and their quantitative evaluation using Monte Carlo simulations. The method is independent of signal intensity calibrations and only requires knowledge of the detector geometry, which is invariant for a given instrument. This study demonstrates that the method yields robust thickness estimates for sub-micrometer amorphous specimen using both direct detection and light conversion 2D-STEM detectors in a coincident FIB-SEM and a conventional SEM. Due to its facile implementation and minimal dose reauirements, it is anticipated that this method will find applications for in situ thickness monitoring during lamella fabrication of beam-sensitive materials. ...