Table 13.
Cell type | Phenotypic identitya) | Positive transcriptomic signatureb) | Negative transcriptomic signaturec) | Key functions that can be tested in vitro | Additional characteristics | References |
---|---|---|---|---|---|---|
cDC1 | HLA-DR+ CD11c+ CD33+ CD141+ CLEC9A+ XCR1+ CADM1+ BTLAhi | C1orf54, CADM1, CLEC9A, CLNK, CPNE3, GCSAM, NAAA, WDFY4, RAB32, XCR1, BATF3, BTLA, HLA-DOB, ID2, IDO1, IRF8 | NN | • IFN-III production upon TLR3 stimulation. • IL-12p70 production upon TLR8 stimulation. • High efficacy for cross-presentation of (dead-) cell-associated Ag. |
• BATF3- and IRF8-dependent differentiation. | [78, 89, 95, 96, 106–110] |
cDC2 | HLA-DR+ CD11c+ CD33+ CD1c+ CLEC10A+ FCER1A+ CD5lo_to_hi BTLAlo_to_hi CD14– CD163− CX3CR1+ CD88− | CD1C, CD1E, CLEC10A, FCER1A, BTLA, CD5, FLT3, HLA-DOB, IRF4 | C3AR1, C5AR1, CD14, CD163, S100A8, S100A9, FCN1, VCAN | • IL-12p70 production upon triggering of CD40 and TLR8, IL-23 production. • Functional polarization of CD4+ T cells toward Th17 or Th2? |
• IRF8-dependent differentiation. | [96, 101, 105, 107–111] |
DC3 | HLA-DR+ CD11c+ CD33+ CD1c+ CD163+ CD14lo_to_hi CD5– BTLA− CD88− | CD14, CD163, CD1C, CLEC10A, FCER1A, S100A8, S100A9, CDKN1A, CLEC4E, F13A1, FCN1, LMNA, VCAN | C1QA, C1QB, C1QC, C3AR1, C5AR1, MERTK | • TGFβ and IL-1β production. • TRM differentiation. |
• Differentiation does not require as high IRF8 expression as for cDC2. | [101, 111, 112] |
ASDC | HLA-DR+ CD11clow/+ CD33+ CD123low/+ CLEC4C+ SIGLEC6+ AXL+ CX3CR1+ CD2+ CD5+ | AXL, CD123, SIGLEC1, SIGLEC6, TCF4, BCL11A, KLF12, LYZ | GZMB, LILRA4, NLRP7, PACSIN1 | • Lack of IFN-I/III production upon TLR7 or TLR9 stimulation • High antigen presentation capacity, similar to that of cDC |
• Dendritic morphology • TCF4-dependent differentiation. • High susceptibility to HIV-1 infection |
[107–109, 113] |
pDC | HLA-DR+ CD11c− CD33− CD123+ CLEC4C+ CD2− CD5− | CD123, CLEC4C, GZMB, IRF7, LILRA4, NLRP7, PACSIN1, TCF4, TLR7, TLR9, BCL11A, EPHB1, PTPRS, RUNX2, SPIB | ZBTB46 | • IFN-I/III production upon TLR7 or TLR9 stimulation. • Lower steady state antigen presentation capacity than cDC, but that is strongly boosted upon adequate stimulation. |
• Plasmacytoid morphology. • TCF4-dependent differentiation. |
[95, 105, 107–109, 114, 115] |
MoDC | HLA-DR+ CD11chi CD11bhi CD172ahi CD163− CD1a+ CD206low/+ CD209low/+ | CD1A, CD1C, CD209, FCER1A, FCER2, FCGR2A, FCGR2B, FCGR2C, FCGR3A, IRF4, ITGAM, LILRB2, MRC1, S100A8, S100A9, SIRPA, STAB1, TLR2, TLR4, VCAN, CD14, CD226, CD68, CLEC10A, CSF1R, EBI3, LAMP3, MMP12 | C1QA, C1QB, C1QC, CD163, FLT3, MERTK | • Production of high levels of TNF, CXCL1, CCL7 and IL-10 in response to TLR4 triggering. • IL-23 production upon CD40 triggering. • Functional polarization of CD4+ T cells toward Th17 or Tfh (or Th2?). |
• Dendritic morphology • IRF4-dependent differentiation. |
[30, 85, 89, 105, 116, 117] |
LC | HLA-DR+ CD11chi CD11b+ CD1a+ CD207+ E-Cad+ | CD207, EPCAM, ABCC4, AXIN2, BMPR1A, MICAL2, MYO6, TJP1 | NN | • High efficacy for CD8+ T cell priming. | • Birbeck granules. | [87, 106] |
CD14+ DDC | HLA-DR+ CD11c+ CD11bhi CD1a− CD14hi CD207− E-Cad− | CD14, CEBPB, MAFB, MSR1, TLR4 | • Functional polarization of CD4+ T cells toward Tfh. | • Dendritic morphology. | [87, 106] | |
cMo | CD88+ CD11bhi CD172ahi CD14+ CD163− CD206− | CD14, CEBPB, FCN1, LYZ, S100A8, S100A9, VCAN | C1QA, C1QB, C1QC, CD163, FLT3, MERTK, ZBTB46 | • Direct B cell stimulation. • Low phagocytosis compared to macrophages • Low antigen presentation ability compared to cDC |
• Non-dendritic and non foamy morphology | [105, 110] |
MoMac | CD88+ CD11bhi CD172ahi CD16+ CD163+ CD206+ CD1a− | APOE, C1QA, C1QB, C1QC, C3AR1, C5AR1, CD163, FCGR3A, FOLR2, MERTK | NN | • High phagocytosis. • Production of high levels of TNF in response to TLR4 triggering. |
• Foam cell morphology. • MAFB-dependent differentiation. |
[30, 85, 105, 110] |
The minimal set of phenotypic markers recommended to identify the cell types is highlighted in bold. – −
The minimal set of positive marker genes recommended to identify the cell types is highlighted in bold.
The minimal set of negative marker gene recommended to discriminate the target cell type from the other types of mononuclear phagocytes that harbor the closest gene expression profiles is highlighted in bold. NN, not necessary, the use of negative marker genes is not necessary.