Red Light-Activated Reversible Inhibition of Protein Functions by Assembled Trap

Peng Zhou; Yongkang Jia; Tianyu Zhang; Abasi Abudukeremu; Xuan He; Xiaozhong Zhang; Chao Liu; Wei Li; Zengpeng Li; Ling Sun; Shouhong Guang; Zhongcheng Zhou; Zhiheng Yuan; Xiaohua Lu; Yang Yu

doi:10.1021/acssynbio.4c00585

Red Light-Activated Reversible Inhibition of Protein Functions by Assembled Trap

Peng Zhou^*, Yongkang Jia, Tianyu Zhang, Abasi Abudukeremu, Xuan He, Xiaozhong Zhang, Chao Liu, Wei Li, Zengpeng Li, Ling Sun, Shouhong Guang, Zhongcheng Zhou, Zhiheng Yuan, Xiaohua Lu^*, Yang Yu^*

^*Corresponding author for this work

Research output: Contribution to journal › Article › peer-review

Abstract

Red light, characterized by superior tissue penetration and minimal phototoxicity, represents an ideal wavelength for optogenetic applications. However, the existing tools for reversible protein inhibition by red light remain limited. Here, we introduce R-LARIAT (red light-activated reversible inhibition by assembled trap), a novel optogenetic system enabling precise spatiotemporal control of protein function via 660 nm red-light-induced protein clustering. Our system harnesses the rapid and reversible binding of engineered light-dependent binders (LDBs) to the bacterial phytochrome DrBphP, which utilizes the endogenous mammalian biliverdin chromophore for red light absorption. By fusing LDBs with single-domain antibodies targeting epitope-tagged proteins (e.g., GFP), R-LARIAT enables the rapid sequestration of diverse proteins into light-responsive clusters. This approach demonstrates high light sensitivity, clustering efficiency, and sustained stability. As a proof of concept, R-LARIAT-mediated sequestration of tubulin inhibits cell cycle progression in HeLa cells. This system expands the optogenetic toolbox for studying dynamic biological processes with high spatial and temporal resolution and holds the potential for applications in living tissues.

Original language	English
Journal	ACS Synthetic Biology
DOIs	https://doi.org/10.1021/acssynbio.4c00585
Publication status	Accepted/In press - 2025
Externally published	Yes

Keywords

DrBphP
LARIAT
LDB
nanobody
optogenetics
red light

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10.1021/acssynbio.4c00585

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@article{be966f32347b49f68214adde67437128,

title = "Red Light-Activated Reversible Inhibition of Protein Functions by Assembled Trap",

abstract = "Red light, characterized by superior tissue penetration and minimal phototoxicity, represents an ideal wavelength for optogenetic applications. However, the existing tools for reversible protein inhibition by red light remain limited. Here, we introduce R-LARIAT (red light-activated reversible inhibition by assembled trap), a novel optogenetic system enabling precise spatiotemporal control of protein function via 660 nm red-light-induced protein clustering. Our system harnesses the rapid and reversible binding of engineered light-dependent binders (LDBs) to the bacterial phytochrome DrBphP, which utilizes the endogenous mammalian biliverdin chromophore for red light absorption. By fusing LDBs with single-domain antibodies targeting epitope-tagged proteins (e.g., GFP), R-LARIAT enables the rapid sequestration of diverse proteins into light-responsive clusters. This approach demonstrates high light sensitivity, clustering efficiency, and sustained stability. As a proof of concept, R-LARIAT-mediated sequestration of tubulin inhibits cell cycle progression in HeLa cells. This system expands the optogenetic toolbox for studying dynamic biological processes with high spatial and temporal resolution and holds the potential for applications in living tissues.",

keywords = "DrBphP, LARIAT, LDB, nanobody, optogenetics, red light",

author = "Peng Zhou and Yongkang Jia and Tianyu Zhang and Abasi Abudukeremu and Xuan He and Xiaozhong Zhang and Chao Liu and Wei Li and Zengpeng Li and Ling Sun and Shouhong Guang and Zhongcheng Zhou and Zhiheng Yuan and Xiaohua Lu and Yang Yu",

note = "Publisher Copyright: {\textcopyright} 2025 American Chemical Society.",

year = "2025",

doi = "10.1021/acssynbio.4c00585",

language = "English",

journal = "ACS Synthetic Biology",

issn = "2161-5063",

publisher = "American Chemical Society",

}

TY - JOUR

T1 - Red Light-Activated Reversible Inhibition of Protein Functions by Assembled Trap

AU - Zhou, Peng

AU - Jia, Yongkang

AU - Zhang, Tianyu

AU - Abudukeremu, Abasi

AU - He, Xuan

AU - Zhang, Xiaozhong

AU - Liu, Chao

AU - Li, Wei

AU - Li, Zengpeng

AU - Sun, Ling

AU - Guang, Shouhong

AU - Zhou, Zhongcheng

AU - Yuan, Zhiheng

AU - Lu, Xiaohua

AU - Yu, Yang

PY - 2025

Y1 - 2025

N2 - Red light, characterized by superior tissue penetration and minimal phototoxicity, represents an ideal wavelength for optogenetic applications. However, the existing tools for reversible protein inhibition by red light remain limited. Here, we introduce R-LARIAT (red light-activated reversible inhibition by assembled trap), a novel optogenetic system enabling precise spatiotemporal control of protein function via 660 nm red-light-induced protein clustering. Our system harnesses the rapid and reversible binding of engineered light-dependent binders (LDBs) to the bacterial phytochrome DrBphP, which utilizes the endogenous mammalian biliverdin chromophore for red light absorption. By fusing LDBs with single-domain antibodies targeting epitope-tagged proteins (e.g., GFP), R-LARIAT enables the rapid sequestration of diverse proteins into light-responsive clusters. This approach demonstrates high light sensitivity, clustering efficiency, and sustained stability. As a proof of concept, R-LARIAT-mediated sequestration of tubulin inhibits cell cycle progression in HeLa cells. This system expands the optogenetic toolbox for studying dynamic biological processes with high spatial and temporal resolution and holds the potential for applications in living tissues.

AB - Red light, characterized by superior tissue penetration and minimal phototoxicity, represents an ideal wavelength for optogenetic applications. However, the existing tools for reversible protein inhibition by red light remain limited. Here, we introduce R-LARIAT (red light-activated reversible inhibition by assembled trap), a novel optogenetic system enabling precise spatiotemporal control of protein function via 660 nm red-light-induced protein clustering. Our system harnesses the rapid and reversible binding of engineered light-dependent binders (LDBs) to the bacterial phytochrome DrBphP, which utilizes the endogenous mammalian biliverdin chromophore for red light absorption. By fusing LDBs with single-domain antibodies targeting epitope-tagged proteins (e.g., GFP), R-LARIAT enables the rapid sequestration of diverse proteins into light-responsive clusters. This approach demonstrates high light sensitivity, clustering efficiency, and sustained stability. As a proof of concept, R-LARIAT-mediated sequestration of tubulin inhibits cell cycle progression in HeLa cells. This system expands the optogenetic toolbox for studying dynamic biological processes with high spatial and temporal resolution and holds the potential for applications in living tissues.

KW - DrBphP

KW - LARIAT

KW - LDB

KW - nanobody

KW - optogenetics

KW - red light

UR - http://www.scopus.com/inward/record.url?scp=105004075020&partnerID=8YFLogxK

U2 - 10.1021/acssynbio.4c00585

DO - 10.1021/acssynbio.4c00585

M3 - Article

AN - SCOPUS:105004075020

SN - 2161-5063

JO - ACS Synthetic Biology

JF - ACS Synthetic Biology

ER -

Red Light-Activated Reversible Inhibition of Protein Functions by Assembled Trap

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Keywords

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