Figure 3.

PhenoCycler (CODEX) workflow. Tissue is labeled using oligonucleotide-conjugated antibodies to detect up to one hundred markers simultaneously. Initial antibody staining is followed by hybridization cycles with three reporter oligonucleotides containing spectrum-separable fluorophores, which hybridize with the unique antisense oligonucleotide conjugated to the primary antibody (left). After each cycle, a microscopy image is acquired (imaging with PhenoCycler). Next, reporters are removed; this is followed by the next reporter hybridization cycle. Images from all cycles are compiled and registered to generate multiplex data images. During imaging analysis, these images can be processed into single-cell expression data and downstream analysis is performed (e.g., cell type mapping, clustering, marker expression).