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Development of a Quenchbody for the Detection and Imaging of the Cancer-Related Tight-Junction-Associated Membrane Protein Claudin
Author(s) -
HeeJin Jeong,
Takuya Kawamura,
Manami Iida,
Yumi Kawahigashi,
Mutsumi Takigawa,
Yuki OhmuroMatsuyama,
Chan-I Chung,
Jinhua Dong,
Masuo Kondoh,
Hiroshi Ueda
Publication year - 2017
Publication title -
analytical chemistry
Language(s) - English
Resource type - Journals
SCImago Journal Rank - 2.117
H-Index - 332
eISSN - 1520-6882
pISSN - 0003-2700
DOI - 10.1021/acs.analchem.7b02047
Subject(s) - claudin , chemistry , fluorescence , cancer cell , tight junction , antibody , in vivo , in vitro , cancer , biophysics , microbiology and biotechnology , recombinant dna , membrane , cls upper limits , green fluorescent protein , biochemistry , gene , biology , immunology , physics , quantum mechanics , genetics , medicine , optometry
Claudins (CLs) are membrane proteins found in tight junctions and play a major role in establishing the intercellular barrier. However, some CLs are abnormally overexpressed on tumor cells and are valid clinical biomarkers for cancer diagnosis. Here, we constructed antibody Fab fragment-based Quenchbodies (Q-bodies) as effective and reliable fluorescent sensors for detecting and visualizing CLs on live tumor cells. The variable region genes for anti-CL1 and anti-CL4 antibodies were used to express recombinant Fab fragments, and clones recognizing CL4 with high affinity were selected for making Q-bodies. When two fluorescent dyes were conjugated to the N-terminal tags attached to the Fab, the fluorescent signal was significantly increased after adding nanomolar-levels of purified CL4. Moreover, addition of the Q-body to CL4-expressing cells including CL4-positive cancer cells led to a clear fluorescence signal with low background, even without washing steps. Our findings suggested that such Q-bodies would serve as a potent tool for specifically illuminating membrane targets expressed on cancer cells, both in vitro and in vivo.

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