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Literature DB >> 20830362

Turn-on fluorescence switch involving aggregation and elimination processes for β-lactamase-tag.

Kalyan K Sadhu¹, Shin Mizukami, Shuji Watanabe, Kazuya Kikuchi.

Abstract

The targeted protein of interest is fused with genetically modified β-lactamase enzyme, which reacts with the probe in physiological conditions to break the aggregated interaction between the fluorophore and quencher. This alliance-separation technique is new for protein labeling and is probed in vitro and in live cell imaging studies.

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Year: 2010 PMID： 20830362 DOI： 10.1039/c0cc02432e

Source DB: PubMed Journal: Chem Commun (Camb) ISSN： 1359-7345 Impact factor: 6.222

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Cited

4 in total

1. Dual-colour imaging of RNAs using quencher- and fluorophore-binding aptamers.

Authors: Ankita Arora; Murat Sunbul; Andres Jäschke
Journal: Nucleic Acids Res Date: 2015-07-14 Impact factor: 16.971

Review 2. Development of an effective protein-labeling system based on smart fluorogenic probes.

Authors: Shahi Imam Reja; Masafumi Minoshima; Yuichiro Hori; Kazuya Kikuchi
Journal: J Biol Inorg Chem Date: 2019-05-31 Impact factor: 3.358

3. Development of cyanine probes with dinitrobenzene quencher for rapid fluorogenic protein labelling.

Authors: Yuichiro Hori; Shinya Hirayama; Kazuya Kikuchi
Journal: Philos Trans A Math Phys Eng Sci Date: 2017-11-28 Impact factor: 4.226

4. Fluorogenic probes reveal a role of GLUT4 N-glycosylation in intracellular trafficking.

Authors: Shinya Hirayama; Yuichiro Hori; Zsolt Benedek; Tadashi Suzuki; Kazuya Kikuchi
Journal: Nat Chem Biol Date: 2016-08-22 Impact factor: 15.040

4 in total