Single-molecule imaging in vivo: The dancing building blocks of the cell

Coelho, Miguel; Maghelli, Nicola; Tolić- Norrelykke, Iva Marija

izvor podataka: crosbi !

Single-molecule imaging in vivo: The dancing building blocks of the cell (CROSBI ID 209366)

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Coelho, Miguel ; Maghelli, Nicola ; Tolić- Norrelykke, Iva Marija Single-molecule imaging in vivo: The dancing building blocks of the cell // Integrative Biology, 5 (2013), 5; 748-758. doi: 10.1039/c3ib40018b

Podaci o odgovornosti

Autori

Coelho, Miguel ; Maghelli, Nicola ; Tolić- Norrelykke, Iva Marija

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Jezik

engleski

Naslov

Single-molecule imaging in vivo: The dancing building blocks of the cell

Sažetak

A cell can be viewed as a dynamic puzzle, where single pieces shuffle in space, change their conformation to fit different partners, and new pieces are generated while old ones are destroyed. Microscopy has become capable of directly observing the pieces of the puzzle, which are single molecules. Single-molecule microscopy in vivo provides new insights into the molecular processes underlying the physiology of a cell, allowing not only for visualizing how molecules distribute with nanometer resolution in the cellular environment, but also for characterizing their movement with high temporal precision. This approach reveals molecular behaviors normally invisible in ensemble measurements. Depending on the molecule, the process, and the cellular region studied, single molecules can be followed by conventional epifluorescence microscopy, or by illuminating only a thin region of the cell, as in Total Internal Reflection Fluorescence (TIRF) and Selective Plane Illumination Microscopy (SPIM), and by limiting the amount of detectable molecules, as in Fluorescence Speckle Microscopy (FSM) and Photo-Activation (PA). High spatial resolution can be obtained by imaging only a fraction of the molecules at a time, as in Photo- Activated Localization Microscopy (PALM) and Stochastic Optical Reconstruction Microscopy (STORM), or by de-exciting molecules in the periphery of the detection region as in Stimulated Emission-Depletion (STED) microscopy. Single- molecule techniques in vivo are becoming widespread ; however, it is important to choose the most suited technique for each biological question or sample. Here we review single-molecule microscopy techniques, describe their basic principles, advantages for in vivo application, and discuss the lessons that can be learned from live single-molecule imaging.

Ključne riječi

internal-reflection fluorescence ; individual influenza-viruses ; living cells ; messenger-rna ; live cells ; protein ; microscopy ; tracking ; organization ; movements

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Jezik

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Naslov

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Sažetak

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Ključne riječi

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Napomena

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Podaci o izdanju

Časopis

Integrative Biology

Volumen (broj)

5 (5)

Godina

2013.

Stranice rada

748-758

Status objave rada

objavljeno

ISSN

1757-9694

e-ISSN

1757-9708

DOI

10.1039/c3ib40018b

Povezanost rada

Povezane osobe

Iva Marija Tolić (autor/i)

Područje

Biologija

Poveznice

doi.org

academic.oup.com

doi.org

Indeksiranost

Scopus

Medline

Web of Science Core Collection, Science Citation Index Expanded (WoSCC-SCI-Exp)

Web of Science Core Collection, SCI-Exp, SSCI & A&HCI (WoSCC-SCI-Exp, SSCI, A&HCI)