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Semi-automated single-molecule microscopy screening of fast-dissociating specific antibodies directly from hybridoma cultures

Miyoshi, Takushi Zhang, Qianli Miyake, Takafumi Watanabe, Shin Ohnishi, Hiroe Chen, Jiji Vishwasrao, Harshad D. Chakraborty, Oisorjo Belyantseva, Inna A. Perrin, Benjamin J. Shroff, Hari Friedman, Thomas B. Omori, Koichi Watanabe, Naoki 京都大学 DOI:10.1016/j.celrep.2021.108708

2021.02

概要

Fast-dissociating, specific antibodies are single-molecule imaging probes that transiently interact with their targets and are used in biological applications including image reconstruction by integrating exchangeable single-molecule localization (IRIS), a multiplexable super-resolution microscopy technique. Here, we introduce a semi-automated screen based on single-molecule total internal reflection fluorescence (TIRF) microscopy of antibody-antigen binding, which allows for identification of fast-dissociating monoclonal antibodies directly from thousands of hybridoma cultures. We develop monoclonal antibodies against three epitope tags (FLAG-tag, S-tag, and V5-tag) and two F-actin crosslinking proteins (plastin and espin). Specific antibodies show fast dissociation with half-lives ranging from 0.98 to 2.2 s. Unexpectedly, fast-dissociating yet specific antibodies are not so rare. A combination of fluorescently labeled Fab probes synthesized from these antibodies and light-sheet microscopy, such as dual-view inverted selective plane illumination microscopy (diSPIM), reveal rapid turnover of espin within long-lived F-actin cores of inner-ear sensory hair cell stereocilia, demonstrating that fast-dissociating specific antibodies can identify novel biological phenomena.

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