Literature DB >> 31403624

Optimization, Design and Avoiding Pitfalls in Manual Multiplex Fluorescent Immunohistochemistry.

Jenny Lazarus1, Yagiz Akiska1, Mirna Perusina Lanfranca1, Lawrence Delrosario1, Lei Sun1, Daniel Long2, Jiaqi Shi3, Howard Crawford2, Marina P Di Magliano1, Weiping Zou1, Timothy Frankel4.   

Abstract

Microenvironment evaluation of intact tissue for analysis of cell infiltration and spatial organization are essential in understanding the complexity of disease processes. The principle techniques used in the past include immunohistochemistry (IHC) and immunofluorescence (IF) which enable visualization of cells as a snapshot in time using between 1 and 4 markers. Both techniques have shortcomings including difficulty staining poorly antigenic targets and limitations related to cross-species reactivity. IHC is reliable and reproducible, but the nature of the chemistry and reliance on the visible light spectrum allows for only a few markers to be used and makes co-localization challenging. Use of IF broadens potential markers but typically relies on frozen tissue due to the extensive tissue autofluorescence following formalin fixation. Flow cytometry, a technique that enables simultaneous labeling of multiple epitopes, abrogates many of the deficiencies of IF and IHC, however, the need to examine cells as a single cell suspension loses the spatial context of cells discarding important biologic relationships. Multiplex fluorescent immunohistochemistry (mfIHC) bridges these technologies allowing for multi-epitope cellular phenotyping in formalin fixed paraffin embedded (FFPE) tissue while preserving the overall microenvironment architecture and spatial relationship of cells within intact undisrupted tissue. High fluorescent intensity fluorophores that covalently bond to the tissue epitope enables multiple applications of primary antibodies without worry of species specific cross-reactivity by secondary antibodies. Although this technology has been proven to produce reliable and accurate images for the study of disease, the process of creating a useful mfIHC staining strategy can be time consuming and exacting due to extensive optimization and design. In order to make robust images that represent accurate cellular interactions in-situ and to mitigate the optimization period for manual analysis, presented here are methods for slide preparation, optimizing antibodies, multiplex design as well as errors commonly encountered during the staining process.

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Year:  2019        PMID: 31403624      PMCID: PMC6786767          DOI: 10.3791/59915

Source DB:  PubMed          Journal:  J Vis Exp        ISSN: 1940-087X            Impact factor:   1.424


  13 in total

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Journal:  Lab Invest       Date:  2017-05-15       Impact factor: 5.662

2.  Eight-Color Multiplex Immunohistochemistry for Simultaneous Detection of Multiple Immune Checkpoint Molecules within the Tumor Microenvironment.

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Journal:  J Immunol       Date:  2017-11-15       Impact factor: 5.422

Review 3.  New flow cytometric assays for monitoring cell-mediated cytotoxicity.

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4.  Multispectral imaging reveals hyper active TGF-β signaling in colorectal cancer.

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Journal:  Cancer Biol Ther       Date:  2017-12-08       Impact factor: 4.742

5.  Multiplex Immunohistochemistry for Image Analysis of Tertiary Lymphoid Structures in Cancer.

Authors:  Keith E Steele; Charles Brown
Journal:  Methods Mol Biol       Date:  2018

Review 6.  Multiplexed immunohistochemistry, imaging, and quantitation: a review, with an assessment of Tyramide signal amplification, multispectral imaging and multiplex analysis.

Authors:  Edward C Stack; Chichung Wang; Kristin A Roman; Clifford C Hoyt
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7.  Spatial computation of intratumoral T cells correlates with survival of patients with pancreatic cancer.

Authors:  Julienne L Carstens; Pedro Correa de Sampaio; Dalu Yang; Souptik Barua; Huamin Wang; Arvind Rao; James P Allison; Valerie S LeBleu; Raghu Kalluri
Journal:  Nat Commun       Date:  2017-04-27       Impact factor: 14.919

8.  Validation of multiplex immunofluorescence panels using multispectral microscopy for immune-profiling of formalin-fixed and paraffin-embedded human tumor tissues.

Authors:  Edwin R Parra; Naohiro Uraoka; Mei Jiang; Pamela Cook; Don Gibbons; Marie-Andrée Forget; Chantale Bernatchez; Cara Haymaker; Ignacio I Wistuba; Jaime Rodriguez-Canales
Journal:  Sci Rep       Date:  2017-10-17       Impact factor: 4.379

9.  Topological analysis reveals a PD-L1-associated microenvironmental niche for Reed-Sternberg cells in Hodgkin lymphoma.

Authors:  Christopher D Carey; Daniel Gusenleitner; Mikel Lipschitz; Margaretha G M Roemer; Edward C Stack; Evisa Gjini; Xihao Hu; Robert Redd; Gordon J Freeman; Donna Neuberg; F Stephen Hodi; Xiaole Shirley Liu; Margaret A Shipp; Scott J Rodig
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Review 10.  A Functional Spatial Analysis Platform for Discovery of Immunological Interactions Predictive of Low-Grade to High-Grade Transition of Pancreatic Intraductal Papillary Mucinous Neoplasms.

Authors:  Souptik Barua; Luisa Solis; Edwin Roger Parra; Naohiro Uraoka; Mei Jiang; Huamin Wang; Jaime Rodriguez-Canales; Ignacio Wistuba; Anirban Maitra; Subrata Sen; Arvind Rao
Journal:  Cancer Inform       Date:  2018-06-28
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  3 in total

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Authors:  Weixian Hu
Journal:  Thorac Cancer       Date:  2019-11-12       Impact factor: 3.500

2.  Development of a Multiplex Immunohistochemistry Workflow to Investigate the Immune Microenvironment in Mouse Models of Inflammatory Bowel Disease and Colon Cancer.

Authors:  Lokman Pang; Matthias Ernst; Jennifer Huynh
Journal:  Int J Mol Sci       Date:  2021-10-12       Impact factor: 5.923

3.  Phenotypic heterogeneity driven by plasticity of the intermediate EMT state governs disease progression and metastasis in breast cancer.

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Journal:  Sci Adv       Date:  2022-08-03       Impact factor: 14.957

  3 in total

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