Searched for: author%3A%22Jakobi%2C+A.%22
(1 - 12 of 12)
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Huber, S. (author), Jakobi, A. (author)
Gas vesicles mediate buoyancy-based motility in aquatic bacteria and archaea and are the only protein-based structures known to enclose a gas-filled volume. Their unique physicochemical properties and ingenious architecture rank them among the most intriguing macromolecular assemblies characterised to date. This review covers the 60-year...
review 2024
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Huber, S. (author), Terwiel, D. (author), Evers, W.H. (author), Maresca, D. (author), Jakobi, A. (author)
Gas vesicles are gas-filled nanocompartments that allow a diverse group of bacteria and archaea to control their buoyancy. The molecular basis of their properties and assembly remains unclear. Here, we report the 3.2 Å cryo-EM structure of the gas vesicle shell made from the structural protein GvpA that self-assembles into hollow helical...
journal article 2023
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Skoupý, R. (author), Boltje, D.B. (author), Slouf, Miroslav (author), Mrázová, Kateřina (author), Láznička, Tomáš (author), Taisne, C.M. (author), Krzyžánek, Vladislav (author), Hoogenboom, J.P. (author), Jakobi, A. (author)
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...
journal article 2023
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Wang, W. (author), Jakobi, A. (author), Wu, Yu-Le (author), Ries, Jonas (author), Stallinga, S. (author), Rieger, B. (author)
Single molecule localization microscopy offers resolution nearly down to the molecular level with specific molecular labelling, and is thereby a promising tool for structural biology. In practice, however, the actual value to this field is limited primarily by incomplete fluorescent labelling of the structure. This missing information can be...
journal article 2023
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Wang, W. (author), Jakobi, A. (author), Wu, Yu‑Le ‑L (author), Ries, Jonas (author), Stallinga, S. (author), Rieger, B. (author)
Correction to: Scientific Reports, published online 16 August 2023 The original version of this Article contained an error in the upper inset of Figure 4, where the atomic model was missing. The original Figure 4 and accompanying legend appear below. (Figure presented.) Overlay of the fluorophore positions from the SMLM particle fusion data ...
journal article 2023
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Bharadwaj, A. (author), Jakobi, A. (author)
Resolution-dependent loss of contrast in cryo-EM maps may obscure features at high resolution that are critical for map interpretation. Post-processing of cryo-EM maps can improve the interpretability by adjusting the resolution-dependence of structure factor amplitudes through map sharpening. Traditionally this has been done by rescaling the...
journal article 2022
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Huber, S. (author), Sarajlic, Edin (author), Huijink, Roeland (author), Weis, Felix (author), Evers, W.H. (author), Jakobi, A. (author)
Cryogenic electron microscopy has become an essential tool for structure determination of biological macromolecules. In practice, the difficulty to reliably prepare samples with uniform ice thickness still represents a barrier for routine high-resolution imaging and limits the current throughput of the technique. We show that a nanofluidic...
journal article 2022
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Maan, R. (author), Reese, L. (author), Volkov, V. (author), King, M.R. (author), van der Sluis, E.O. (author), Andrea, N. (author), Evers, W.H. (author), Jakobi, A. (author), Dogterom, A.M. (author)
Growing microtubule ends organize end-tracking proteins into comets of mixed composition. Here using a reconstituted fission yeast system consisting of end-binding protein Mal3, kinesin Tea2 and cargo Tip1, we found that these proteins can be driven into liquid-phase droplets both in solution and at microtubule ends under crowding conditions....
journal article 2022
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Boltje, D.B. (author), Hoogenboom, J.P. (author), Jakobi, A. (author), Jensen, Grant J. (author), Jonker, C.T.H. (author), Kaag, Max J. (author), de Agrela Pinto, C. (author), van der Wee, E.B. (author), Hoedt, Sander Den (author)
Cryogenic electron tomography (cryo-ET) combined with sub-tomogram averaging, allows in-situ visualization and structure determination of macromolecular complexes at sub-nanometre resolution. Cryogenic focused ion beam (cryo-FIB) micromachining is used to prepare a thin lamella-shaped sample out of a frozen-hydrated cell for cryo-ET imaging,...
journal article 2022
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Joseph, Agnel Praveen (author), Lagerstedt, Ingvar (author), Jakobi, A. (author), Burnley, Tom (author), Patwardhan, Ardan (author), Topf, Maya (author), Winn, Martyn (author)
Cryogenic electron microscopy (cryo-EM) is a powerful technique for determining structures of multiple conformational or compositional states of macromolecular assemblies involved in cellular processes. Recent technological developments have led to a leap in the resolution of many cryo-EM data sets, making atomic model building more common...
journal article 2020
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Jakobi, A. (author)
Transformative technological advances have propelled cryogenic electron microscopy (cryo-EM) to take center stage in elucidating the intricacies of the nanoscale molecular machinery of viruses, bacteria and eukaryotic cells. Continued developments hold exciting promise for structural biophysicists to move closer to their dream of visualising...
journal article 2020
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Koiwai, Kotaro (author), Tsukimoto, Jun (author), Higashi, Tetsuya (author), Mafuné, Fumitaka (author), Miyajima, Ken (author), Nakane, Takanori (author), Matsugaki, Naohiro (author), Kato, Ryuichi (author), Jakobi, A. (author)
In cellulo crystallization is a developing technique to provide crystals for protein structure determination, particularly for proteins that are difficult to prepare by in vitro crystallization. This method has a key advantage: It requires neither a protein purification step nor a crystallization step. However, there is still no systematic...
journal article 2019
Searched for: author%3A%22Jakobi%2C+A.%22
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