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Literature DB >> 30381437

New observations in neuroscience using superresolution microscopy.

Michihiro Igarashi¹, Motohiro Nozumi², Ling-Gang Wu³, Francesca Cella Zanacchi⁴, István Katona⁵, László Barna⁶, Pingyong Xu^7,8,9, Mingshu Zhang^7,8, Fudong Xue^7,8, Edward Boyden¹⁰.

Abstract

Superresolution microscopy (SM) techniques are among the revolutionary methods for molecular and cellular observations in the 21st century. SM techniques overcome optical limitations, and several new observations using SM lead us to expect these techniques to have a large impact on neuroscience in the near future. Several types of SM have been developed, including structured illumination microscopy (SIM), stimulated emission depletion microscopy (STED), and photoactivated localization microscopy (PALM)/stochastic optical reconstruction microscopy (STORM), each with special features. In this Minisymposium, experts in these different types of SM discuss the new structural and functional information about specific important molecules in neuroscience that has been gained with SM. Using these techniques, we have revealed novel mechanisms of endocytosis in nerve growth, fusion pore dynamics, and described quantitative new properties of excitatory and inhibitory synapses. Additional powerful techniques, including single molecule-guided Bayesian localization SM (SIMBA) and expansion microscopy (ExM), alone or combined with super-resolution observation, are also introduced in this session.

Mesh：

Year: 2018 PMID： 30381437 PMCID： PMC6209844 DOI： 10.1523/JNEUROSCI.1678-18.2018

Source DB: PubMed Journal: J Neurosci ISSN： 0270-6474 Impact factor: 6.167

40 in total

1. Super-resolution imaging reveals that AMPA receptors inside synapses are dynamically organized in nanodomains regulated by PSD95.

Authors: Deepak Nair; Eric Hosy; Jennifer D Petersen; Audrey Constals; Gregory Giannone; Daniel Choquet; Jean-Baptiste Sibarita
Journal: J Neurosci Date: 2013-08-07 Impact factor: 6.167

Review 2. Exocytosis and endocytosis: modes, functions, and coupling mechanisms.

Authors: Ling-Gang Wu; Edaeni Hamid; Wonchul Shin; Hsueh-Cheng Chiang
Journal: Annu Rev Physiol Date: 2013-11-20 Impact factor: 19.318

3. Coordinated Movement of Vesicles and Actin Bundles during Nerve Growth Revealed by Superresolution Microscopy.

Authors: Motohiro Nozumi; Fubito Nakatsu; Kaoru Katoh; Michihiro Igarashi
Journal: Cell Rep Date: 2017-02-28 Impact factor: 9.423

4. Increased spatiotemporal resolution reveals highly dynamic dense tubular matrices in the peripheral ER.

Authors: Jonathon Nixon-Abell; Christopher J Obara; Aubrey V Weigel; Dong Li; Wesley R Legant; C Shan Xu; H Amalia Pasolli; Kirsten Harvey; Harald F Hess; Eric Betzig; Craig Blackstone; Jennifer Lippincott-Schwartz
Journal: Science Date: 2016-10-27 Impact factor: 47.728

5. Cell-specific STORM super-resolution imaging reveals nanoscale organization of cannabinoid signaling.

Authors: Barna Dudok; László Barna; Marco Ledri; Szilárd I Szabó; Eszter Szabadits; Balázs Pintér; Stephen G Woodhams; Christopher M Henstridge; Gyula Y Balla; Rita Nyilas; Csaba Varga; Sang-Hun Lee; Máté Matolcsi; Judit Cervenak; Imre Kacskovics; Masahiko Watanabe; Claudia Sagheddu; Miriam Melis; Marco Pistis; Ivan Soltesz; István Katona
Journal: Nat Neurosci Date: 2014-12-08 Impact factor: 24.884

6. Live cell single molecule-guided Bayesian localization super resolution microscopy.

Authors: Fan Xu; Mingshu Zhang; Wenting He; Renmin Han; Fudong Xue; Zhiyong Liu; Fa Zhang; Jennifer Lippincott-Schwartz; Pingyong Xu
Journal: Cell Res Date: 2016-12-30 Impact factor: 25.617

7. Iterative expansion microscopy.

Authors: Jae-Byum Chang; Fei Chen; Young-Gyu Yoon; Erica E Jung; Hazen Babcock; Jeong Seuk Kang; Shoh Asano; Ho-Jun Suk; Nikita Pak; Paul W Tillberg; Asmamaw T Wassie; Dawen Cai; Edward S Boyden
Journal: Nat Methods Date: 2017-04-17 Impact factor: 28.547

8. Brain Slice Staining and Preparation for Three-Dimensional Super-Resolution Microscopy.

Authors: Christopher L German; Manasa V Gudheti; Annette E Fleckenstein; Erik M Jorgensen
Journal: Methods Mol Biol Date: 2017

9. Synaptic recruitment of gephyrin regulates surface GABAA receptor dynamics for the expression of inhibitory LTP.

Authors: Enrica Maria Petrini; Tiziana Ravasenga; Torben J Hausrat; Giuliano Iurilli; Umberto Olcese; Victor Racine; Jean-Baptiste Sibarita; Tija C Jacob; Stephen J Moss; Fabio Benfenati; Paolo Medini; Matthias Kneussel; Andrea Barberis
Journal: Nat Commun Date: 2014-06-04 Impact factor: 14.919

10. Protein-retention expansion microscopy of cells and tissues labeled using standard fluorescent proteins and antibodies.

Authors: Paul W Tillberg; Fei Chen; Kiryl D Piatkevich; Yongxin Zhao; Chih-Chieh Jay Yu; Brian P English; Linyi Gao; Anthony Martorell; Ho-Jun Suk; Fumiaki Yoshida; Ellen M DeGennaro; Douglas H Roossien; Guanyu Gong; Uthpala Seneviratne; Steven R Tannenbaum; Robert Desimone; Dawen Cai; Edward S Boyden
Journal: Nat Biotechnol Date: 2016-07-04 Impact factor: 54.908

18 in total

New observations in neuroscience using superresolution microscopy.

1. Super-resolution imaging reveals that AMPA receptors inside synapses are dynamically organized in nanodomains regulated by PSD95.

Review 2. Exocytosis and endocytosis: modes, functions, and coupling mechanisms.

3. Coordinated Movement of Vesicles and Actin Bundles during Nerve Growth Revealed by Superresolution Microscopy.

4. Increased spatiotemporal resolution reveals highly dynamic dense tubular matrices in the peripheral ER.

5. Cell-specific STORM super-resolution imaging reveals nanoscale organization of cannabinoid signaling.

6. Live cell single molecule-guided Bayesian localization super resolution microscopy.

7. Iterative expansion microscopy.

8. Brain Slice Staining and Preparation for Three-Dimensional Super-Resolution Microscopy.

9. Synaptic recruitment of gephyrin regulates surface GABAA receptor dynamics for the expression of inhibitory LTP.

10. Protein-retention expansion microscopy of cells and tissues labeled using standard fluorescent proteins and antibodies.

1. A Pictorial History of the Neuronal Cytoskeleton.

2. Quantification of trans-synaptic protein alignment: A data analysis case for single-molecule localization microscopy.

Review 3. Imaging the endocannabinoid signaling system.

4. STORM Super-Resolution Imaging of CB₁ Receptors in Tissue Preparations.

5. Assessing CB₁ Expression in the Brain by Immunohistochemical Methods: Light, Confocal, and Electron Microscopy.

Review 6. A Single-Neuron: Current Trends and Future Prospects.

Review 7. Molecular basis of the functions of the mammalian neuronal growth cone revealed using new methods.

8. Imaging tripartite synapses using super-resolution microscopy.

9. Super Resolution Microscopy of SUMO Proteins in Neurons.

10. Phosphorylation sites of microtubule-associated protein 1B (MAP 1B) are involved in axon growth and regeneration.