Doubling multiplexed imaging capability via spatial expression pattern-guided protein pairing and computational unmixing.

Three-dimensional multiplexed fluorescence imaging is an indispensable technique in neuroscience. For two-dimensional multiplexed imaging, cyclic immunofluorescence, which involves repeating staining, imaging, and signal removal over multiple cycles, has been widely used. However, the application of cyclic immunofluorescence to three dimensions poses challenges, as a single staining process can take more than 12 hours for thick specimens, and repeating this process for multiple cycles can be prohibitively long. Here, we propose SEPARATE (Spatial Expression PAttern-guided paiRing And unmixing of proTEins), a method that reduces the number of cycles by half by imaging two proteins using a single fluorophore. This is achieved by labeling two proteins with the same fluorophores and unmixing their signals based on their three-dimensional spatial expression patterns, using a neural network. We employ a feature extraction network to quantify the spatial distinction between proteins, with these quantified values, termed feature-based distances, used to identify protein pairs. We then validate the feature extraction network with ten proteins, showing a high correlation between spatial pattern distinction and signal unmixing performance. We finally demonstrate the volumetric multiplexed imaging of six proteins using three fluorophores, pairing them based on feature-based distances and unmixing their signals through protein separation networks.