A type of human skin dendritic cell marked by CD5 is associated with the development of inflammatory skin disease
Daniel Korenfeld, Laurent Gorvel, Adiel Munk, Joshua Man, Andras Schaffer, Thomas Tung, Caroline Mann, Eynav Klechevsky
Daniel Korenfeld, Laurent Gorvel, Adiel Munk, Joshua Man, Andras Schaffer, Thomas Tung, Caroline Mann, Eynav Klechevsky
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Research Article Immunology Inflammation

A type of human skin dendritic cell marked by CD5 is associated with the development of inflammatory skin disease

Abstract

Dendritic cells (DCs) are important in regulating immunity and tolerance and consist of functionally distinct subsets that differentially regulate T lymphocyte function. The underlying basis for this subset specificity is lacking, particularly in humans, where the classification of tissue DCs is currently incomplete. Examination of healthy human epidermal Langerhans cells and dermal skin cells revealed a tissue CD5-expressing DC subtype. The CD5+ DCs were potent inducers of cytotoxic T cells and Th22 cells. The products of these T cells, IL-22 and IFN-γ, play a key role in the pathogenesis of psoriasis. Remarkably, CD5+ DCs were significantly enriched in lesional psoriatic skin compared with distal tissues, suggesting their involvement in the disease. We show that CD5+ DCs can be differentiated from hematopoietic progenitor cells independently of the CD5– DCs. A progenitor population found in human cord blood and in the dermal skin layer, marked as CD34–CD123+CD117dimCD45RA+, was an immediate precursor of these CD11c+CD1c+CD5+ DCs. Overall, our discovery of the CD5-expressing DC subtype suggests that strategies to regulate their composition or function in the skin will represent an innovative approach for the treatment of immune-mediated disorders in and beyond the skin.

Authors

Daniel Korenfeld, Laurent Gorvel, Adiel Munk, Joshua Man, Andras Schaffer, Thomas Tung, Caroline Mann, Eynav Klechevsky

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Figure 2

Dermal CD5+ DCs are more efficient than their CD5 counterparts at priming CTLs.

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Dermal CD5+ DCs are more efficient than their CD5– counterparts at primi...
(A) Allogeneic naive CD8+ T cells primed with sorted CD40L-activated skin dermal CD5+ or CD5 CD1adim DCs, dermal CD1adimCD141+ DCs, or dermal CD14+ DCs at ratio 1:40 for 7 days. The graph shows the percentage of proliferating (CFSElo) CD3+CD8+ T cells (n = 15). Mean ± SD ± SEM for CD5+: 53.7% ± 26.6% ± 6.8%, CD5: 36.4% ± 20.7% ± 5.3%, CD141+ DCs: 20.2% ± 16.1% ± 5.3%, CD14+ DCs: 15.1% ± 17% ± 5.6%. (B) Allogeneic CFSE-labeled naive CD8+ T cells primed for 7 days by each dermal skin mDC subset were stained and analyzed by flow cytometry for the expression of granzyme B. The percentage of cells that diluted CFSE and expressed granzyme B is shown. One of 8 experiments is shown. (C) The plot shows the percentage of cells primed by each of the mDC subsets and expressed granzyme B (n = 8). (D) The plots show the expression of IFN-γ and TNF-α by naive CD8+ T cells that were primed by either dermal CD5+ or CD5 DCs. CD8+ T cells primed by the dermal CD14+ DCs are shown as a control. One of 5 experiments is shown. (E) CFSEloCD8+ T cells that were primed by either dermal CD1adimCD5+ or CD5 DCs were reactivated by anti-CD3 and anti-CD28 mAbs for 18 hours. IFN-γ was measured in the culture supernatant by a Luminex magnetic bead assay. The graph shows the pooled results of 4 experiments. Data represent mean ± SEM; **P < 0.01, ****P < 0.0001 by paired Student’s t tests (A, C, and E).