Protocol to study immunodynamics in the tumor microenvironment using a tyramide signal amplification-based immunofluorescent multiplex panel

Jane Siu-Fan Li; Philip Chiu-Tsun Tang; Chun Kit K Choi; Alex Siu-Wing Chan; Calvin Sze-Hang Ng; Ka-Fai To; Patrick Ming-Kuen Tang

doi:10.1016/j.xpro.2023.102823

Protocol to study immunodynamics in the tumor microenvironment using a tyramide signal amplification-based immunofluorescent multiplex panel

Jane Siu-Fan Li, Philip Chiu-Tsun Tang, Chun Kit K Choi, Alex Siu-Wing Chan, Calvin Sze-Hang Ng, Ka-Fai To, Patrick Ming-Kuen Tang^*

^*Corresponding author for this work

Academy of Wellness and Human Development

Research output: Contribution to journal › Journal article › peer-review

Abstract

Immunodynamics in the tumor microenvironment can be precisely examined by using multiple antigen identification approaches. Here, we present a protocol for capturing expression levels of multiple target proteins in the same specimen at single-cell resolution using a tyramide signal amplification-based immunofluorescent multiplexing system. We describe steps for tumor tissue microarray preparation, multiplex immunohistochemistry staining, image acquisition, and quantification. This protocol can quantify immune cells in tissues from patients or experimental disease models at a protein level. For complete details on the use and execution of this protocol, please refer to Chung et al. (2023), 1 Tang et al. (2022), 2 and Tang et al. (2022). 3.

Original language	English
Article number	102823
Number of pages	17
Journal	STAR Protocols
Volume	5
Issue number	1
DOIs	https://doi.org/10.1016/j.xpro.2023.102823
Publication status	Published - 15 Mar 2024

User-Defined Keywords

Humans
Tumor Microenvironment
Coloring Agents
Histological Techniques

UN SDGs

This output contributes to the following UN Sustainable Development Goals (SDGs)

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10.1016/j.xpro.2023.102823

Cite this

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title = "Protocol to study immunodynamics in the tumor microenvironment using a tyramide signal amplification-based immunofluorescent multiplex panel",

abstract = "Immunodynamics in the tumor microenvironment can be precisely examined by using multiple antigen identification approaches. Here, we present a protocol for capturing expression levels of multiple target proteins in the same specimen at single-cell resolution using a tyramide signal amplification-based immunofluorescent multiplexing system. We describe steps for tumor tissue microarray preparation, multiplex immunohistochemistry staining, image acquisition, and quantification. This protocol can quantify immune cells in tissues from patients or experimental disease models at a protein level. For complete details on the use and execution of this protocol, please refer to Chung et al. (2023), 1 Tang et al. (2022), 2 and Tang et al. (2022). 3. ",

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AU - Li, Jane Siu-Fan

AU - Tang, Philip Chiu-Tsun

AU - Choi, Chun Kit K

AU - Chan, Alex Siu-Wing

AU - Ng, Calvin Sze-Hang

AU - To, Ka-Fai

AU - Tang, Patrick Ming-Kuen

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N2 - Immunodynamics in the tumor microenvironment can be precisely examined by using multiple antigen identification approaches. Here, we present a protocol for capturing expression levels of multiple target proteins in the same specimen at single-cell resolution using a tyramide signal amplification-based immunofluorescent multiplexing system. We describe steps for tumor tissue microarray preparation, multiplex immunohistochemistry staining, image acquisition, and quantification. This protocol can quantify immune cells in tissues from patients or experimental disease models at a protein level. For complete details on the use and execution of this protocol, please refer to Chung et al. (2023), 1 Tang et al. (2022), 2 and Tang et al. (2022). 3.

AB - Immunodynamics in the tumor microenvironment can be precisely examined by using multiple antigen identification approaches. Here, we present a protocol for capturing expression levels of multiple target proteins in the same specimen at single-cell resolution using a tyramide signal amplification-based immunofluorescent multiplexing system. We describe steps for tumor tissue microarray preparation, multiplex immunohistochemistry staining, image acquisition, and quantification. This protocol can quantify immune cells in tissues from patients or experimental disease models at a protein level. For complete details on the use and execution of this protocol, please refer to Chung et al. (2023), 1 Tang et al. (2022), 2 and Tang et al. (2022). 3.

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KW - Coloring Agents

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DO - 10.1016/j.xpro.2023.102823

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Protocol to study immunodynamics in the tumor microenvironment using a tyramide signal amplification-based immunofluorescent multiplex panel

Abstract

User-Defined Keywords

UN SDGs

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