Multiplex Immunofluorescence Staining Protocol

To prepare specimens for multiplex IF staining, tissue sections were cut at 4 μm from formalin-fixed paraffin-embedded blocks. All sections on slides were deparaffinized using the Bond ER2 Leica Biosystems AR9640, followed by staining with the Leica Bond RX autostainer. The slides were stained with - CD3 (1:50 SP7 Abcam ab16669), CD16 (1:50 2H7 CellSignaling Technologies 88251S), CD32b (1:2000 NovusBiologicals NBP2–89364), and CD68 (1:400 PGM-1 DAKO). Antibody binding was visualized using secondary anti-mouse/anti-rabbit polymer HRP followed with TSA-Opal reagents (Akoya NEL811001KT). Tissue slides were incubated with DAPI as a counterstain and coverslipped with VectaShield mounting media (Vector Labs). Control tissue samples were stained for each marker as positive controls.
Whole slide digital images were captured with the PhenoImager HT platform and analyzed with QuPath software^{24 (link)}. Tissue samples from consecutive slides were stained by conventional H&E and scanned with the Leica SCN400F platform. H&E slides in conjunction with Cytokeratin staining were used to annotate tumor regions within the whole slide image. Cells were segmented, phenotyped, and enumerated using the QuPath object classification algorithm.

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Knorr D., Leidner R., Jensen S., Meng R., Jones A., Ballesteros-Merino C., Bell R.B., Baez M., Sprott D., Bifulco C., Piening B., Dahan R., Fox B.A, & Ravetch J. (2023). FcyRIIB is a novel immune checkpoint in the tumor microenvironment limiting activity of Treg-targeting antibodies. bioRxiv.

Publication Preprint 2023

Bond ER2 PGM-1 TSA-Opal reagents VectaShield mounting media SCN400F platform

Antibody Cells Cytokeratin Dapi Formalin Mouse Opal Paraffin Polymer Rabbit Tissue Tumor Vector

Corresponding Organization : Memorial Sloan Kettering Cancer Center

Other organizations : Providence Portland Medical Center, Weizmann Institute of Science

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Variable analysis

independent variables

Tissue preparation method: formalin-fixed paraffin-embedded blocks, 4 μm sections, deparaffinization using Bond ER2 Leica Biosystems AR9640, staining with Leica Bond RX autostainer

dependent variables

Expression levels of CD3, CD16, CD32b, and CD68 markers in tissue samples

control variables

Staining conditions: antibody concentrations, secondary antibody, and visualization reagents
Tissue samples: control tissue samples stained for each marker as positive controls

controls

Positive controls: control tissue samples stained for each marker

Annotations

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