Stereochemistry‐Dependent Labeling of Organelles with a Near‐Infrared‐Emissive Phosphorus‐Bridged Rhodamine Dye in Live‐Cell Imaging

Author:

Wu Qian12,Taki Masayasu1ORCID,Tanaka Yoshiki3,Kesherwani Manish1,Phung Quan Manh1,Enoki Sawako4,Okada Yasushi4567ORCID,Tama Florence189ORCID,Yamaguchi Shigehiro1310ORCID

Affiliation:

1. Institute of Transformative Bio-Molecules (WPI-ITbM) Nagoya University Furo, Chikusa Nagoya 464-8601 Japan

2. Current address: State Key Laboratory of Medical Chemical Biology College of Pharmacy Nankai University 38 Tongyan Road, Jinnan District Tianjin 300350 P. R. China

3. Department of Chemistry Graduate School of Science Nagoya University Furo, Chikusa, Nagoya 464-8602 Japan

4. Department of Physics and Universal Biology Institute (UBI) Graduate School of Science The University of Tokyo Hongo, Tokyo 113-0033 Japan

5. Laboratory for Cell Polarity Regulation RIKEN Center for Biosystems Dynamics Research Suita Osaka 565-0874 Japan

6. Department of Cell Biology Graduate School of Medicine The University of Tokyo Hongo, Tokyo 113-0033 Japan

7. International Research Center for Neurointelligence (WPI-IRCN) The University of Tokyo Hongo, Tokyo 113-0033 Japan

8. Department of Physics Graduate School of Science Nagoya University Furo, Chikusa, Nagoya 464-8602 Japan

9. Center for Computational Science, RIKEN Kobe 650-0047 Japan

10. Integrated Research Consortium on Chemical Sciences (IRCCS) Nagoya University Furo, Chikusa, Nagoya 464-8602 Japan

Abstract

AbstractThe development of near‐infrared (NIR) fluorophores that have both excellent chemical stability and photostability, as well as efficient cell permeability, is highly demanded. In this study, we present phospha‐rhodamine (POR) dyes which display significantly improved performance for protein labeling. This is achieved by incorporating a 2‐carboxy‐3‐benzothiophenyl group at the 9‐position of the xanthene scaffold. The resulting cis and trans isomers were successfully isolated and structurally characterized using X‐ray diffraction. The HaloTag ligand conjugates of the two isomers exhibited different staining abilities in live cells. While the cis isomer showed non‐specific accumulation on the organelle membranes, the trans isomer selectively labeled the HaloTag‐fused proteins, enabling the long‐term imaging of cell division and the 5‐color imaging of cell organelles. Molecular dynamics simulations of the HaloTag ligand conjugates within the lipid membrane suggested that the cis isomer is more prone to forming oligomers in the membrane. In contrast, the oligomerization of the trans isomer is effectively suppressed by its interaction with the lipid molecules. By taking advantage of the superior labeling performance of the trans isomer and its NIR‐emissive properties, multi‐color time‐lapse super‐resolution 3D imaging, namely super‐resolution 5D‐imaging, of the interconnected network between the endoplasmic reticulum and microtubules was achieved in living cells.

Funder

Japan Society for the Promotion of Science

Core Research for Evolutional Science and Technology

Moonshot Research and Development Program

Publisher

Wiley

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