Journal ArticleDOI
Specific Covalent Labeling of Recombinant Protein Molecules Inside Live Cells
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TLDR
This system provides a recipe for slightly modifying a target protein so that it can be singled out from the many other proteins inside live cells and fluorescently stained by small nonfluorescent dye molecules added from outside the cells.Abstract:
Recombinant proteins containing four cysteines at the i , i + 1, i + 4, and i + 5 positions of an α helix were fluorescently labeled in living cells by extracellular administration of 4′,5′-bis(1,3,2-dithioarsolan-2-yl)fluorescein. This designed small ligand is membrane-permeant and nonfluorescent until it binds with high affinity and specificity to the tetracysteine domain. Such in situ labeling adds much less mass than does green fluorescent protein and offers greater versatility in attachment sites as well as potential spectroscopic and chemical properties. This system provides a recipe for slightly modifying a target protein so that it can be singled out from the many other proteins inside live cells and fluorescently stained by small nonfluorescent dye molecules added from outside the cells.read more
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Activation Biosensor for G Protein-Coupled Receptors: A FRET-Based m1 Muscarinic Activation Sensor That Regulates Gq
Seungwoo Chang,Elliott M. Ross +1 more
TL;DR: A fluorescence sensor to measure activation by agonist of the m1 muscarinic cholinergic receptor, a prototypical class I Gq-coupled receptor, and the strategies used to increase the agonist-driven change in FRET while simultaneously maintaining regulatory interactions with Gαq are described.
Journal ArticleDOI
Tuning the Structure, Stability, and Responsivity of Polymeric Arsenical Nanoparticles Using Polythiol Cross-Linkers
Joji Tanaka,Guillaume Moriceau,Alexander B. Cook,Andrew Kerr,Junliang Zhang,Raoul Peltier,Sébastien Perrier,Thomas P. Davis,Paul Wilson +8 more
TL;DR: The use of organic arsenicals in polymer chemistry and biomaterials science is limited despite the distinctive and versatile chemistry of arsenic as discussed by the authors, despite the interchangeable oxidation states of arsenic an...
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Photons in - numbers out: Perspectives in quantitative fluorescence microscopy for in situ protein counting
TL;DR: In this article, important requirements of an ideal quantitative microscopy approach of general usability are outlined and discussed in the context of existing methods including sample preparation and labeling quality which are essential for the robustness and reliability of the methods and future applications in cell biology.
Journal ArticleDOI
Targetable fluorescent sensors for advanced cell function analysis
TL;DR: The original protein labeling technique, which enables fluorogenic labeling as an advanced technology, was introduced and the first discussed strategy is based on the intrinsic properties of small molecules for localization at specific organelles, such as mitochondria, nuclei, and lysosomes.
Journal ArticleDOI
All the small things: How virus-like particles and liposomes modulate allergic immune responses.
TL;DR: The “pros and cons” of inducing anti‐cytokine, anti‐IgE, or anti‐FcεR antibodies in the host are discussed and the various technical advances in VNP‐ and liposome‐research are put into (pre‐)clinical context by referring and critically discussing the relevant studies performed to treat allergic diseases.
References
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Journal ArticleDOI
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Fluorescent indicators for Ca2+based on green fluorescent proteins and calmodulin
Atsushi Miyawaki,Juan Llopis,Roger Heim,J. Michael McCaffery,Joseph A. Adams,Mitsuhiko Ikura,Mitsuhiko Ikura,Roger Y. Tsien +7 more
TL;DR: New fluorescent indicators for Ca2+ that are genetically encoded without cofactors and are targetable to specific intracellular locations are constructed and dubbed ‘cameleons’.
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TL;DR: The green fluorescent protein (GFP) from the Pacific Northwest jellyfish Aequorea victoria has generated intense interest as a marker for gene expression and localization of gene products.
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Roger Heim,Roger Y. Tsien +1 more
TL;DR: The results demonstrate that the production of more and better GFP variants is possible and worthwhile, and facilitates multicolor imaging of differential gene expression, protein localization or cell fate.
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