Single‐cell RNA sequencing reveals a high‐resolution cell atlas of xylem in Populus

Abstract High‐throughput single‐cell RNA sequencing (scRNA‐seq) has advantages over traditional RNA‐seq to explore spatiotemporal information on gene dynamic expressions in heterogenous tissues. We performed Drop‐seq, a method for the dropwise sequestration of single cells for sequencing, on protoplasts from the differentiating xylem of Populus alba × Populus glandulosa . The scRNA‐seq profiled 9,798 cells, which were grouped into 12 clusters. Through characterization of differentially expressed genes in each cluster and RNA in situ hybridizations, we identified vessel cells, fiber cells, ray parenchyma cells and xylem precursor cells. Diffusion pseudotime analyses revealed the differentiating trajectory of vessels, fiber cells and ray parenchyma cells and indicated a different differentiation process between vessels and fiber cells, and a similar differentiation process between fiber cells and ray parenchyma cells. We identified marker genes for each cell type (cluster) and key candidate regulators during developmental stages of xylem cell differentiation. Our study generates a high‐resolution expression atlas of wood formation at the single cell level and provides valuable information on wood formation.