CD62LhiCD44lo and CD62LhiCD44hi T cells were almost exclusively CD27+CCR6? in both pLN and mLN (Fig.?1b). lymphoid organs (SLOs) until they encounter their cognate antigens and differentiate into effector T cells that preferentially migrate into non-lymphoid tissues. After the effector phase, T cells can differentiate into classically defined memory subsets Serlopitant as central memory (TCM), which circulates between SLOs, effector memory (TEM), which circulates between spleen and non-lymphoid tissues and resident memory (TRM), which stays in non-lymphoid tissues without circulation. Diversity in T cell migratory behavior is realized by specific combinations of chemokine receptors, integrins and selectins, as well as other homing factors. For example, both TCM and na?ve T cells express high levels of L-selectin (CD62L), CCR7 and S1PR1 which facilitates their circulation through Slc7a7 lymph nodes (LNs)1,2. On the other hand, TRM cells generally express low levels of these molecules, which contributes to their recruitment to and residency in non-lymphoid tissues1,2. T cells of the vertebrate immune system can be divided into and T cells based on their T cell receptor (TCR) chains and T cells are further classified as CD4+ helper and CD8+ cytotoxic T cells. Although T cells represent only 1C2% of all T cells in LNs of human and mice, their frequency can be significantly higher in non-lymphoid tissues such as gut epithelium and skin epidermis3C6. Interestingly, T cells expressing certain and/or chains are enriched in specific non-lymphoid organs, which is suggested to be due to specific retention and/or migration3C8. Most studies addressing migratory subsets of T cells focus on T cells and less is known about circulation characteristics of T cells. This is partially due to their low frequency in LNs, poorly understood differentiation pathways, heterogeneity in their TCR activation mechanisms and limitations of conventional experimental approaches3C6. Recently, photoconversion-based cell tracking methods emerged as powerful tools to investigate T cell migration tracking of T cells10C12. To overcome this limitation, we previously generated a histone-fused green-to-red photoconvertible protein (H2B-Dendra2) which dramatically increased the half-life of the native Dendra2 protein15. By using bone-marrow chimeras that express H2B-Dendra2, we identified resident populations of CD4+ T cells in lymphoid organs15. Here, we Serlopitant extend the long-term tracking of T cells to CD8+ and T cells using a transgenic mouse model that expresses a Serlopitant stabilized photoconvertible protein. We show that T cells in LNs can be classified into subsets with different migratory characteristics that resemble those of CD8+ T cells. Moreover, we identified resident populations of CD8+ and T cells in both skin and gut draining LNs that stayed in LNs without circulation or proliferation. Our results suggest that CD4+ and CD8+ T cells as well as T cells show highly congruent migratory patterns. Results T cell subsets express different levels of migration-related genes CD62L and CD44 are commonly used to discriminate T cells with different migratory properties in mice1,2. For CD8+ T cells, the CD62LloCD44hi population contains TEM, TRM and recently activated T cells whereas the CD62LhiCD44hi and CD62LhiCD44lo populations represent TCM and na?ve T cells, respectively. To explore the suitability of this classification to stratify populations of T cells, we stained T cells (CD19?CD3+TCR?TCR+) from LNs of unmanipulated wild type mice for CD62L and CD44. Similar to CD8+ T cells (CD19?CD3+TCR?TCR+CD4?CD8+), we observed three major populations of T cells (Fig.?1a,b). Frequency of CD62LloCD44hi T cells was higher in skin-draining peripheral LNs (pLN) compared to gut-draining mesenteric LNs (mLN) and these cells expressed higher levels of CD44 in pLN, indicating site-specific accumulation of different subsets T cells (Fig.?1a). Open in a separate window Figure 1 T cells in LNs can be divided into distinct subsets using CD62L and CD44 expression. (a) CD62L and CD44 expression in CD8+ and T cells.