Preparation and immunolabeling of mice epidermal sheets.

Mice of defined ages, ranging from E14 to P7, were sacrificed. Ventral skin was dissected, cut into 1 × 1–cm pieces, and placed dermal side down on PBS 20 mM EDTA for 2 h at 37°C. The epidermis was then peeled off the dermis. For E14 fetuses, whole skin was processed. To prepare epidermal sheets from adult mice (4–14 wk old), the ventral and dorsal halves of ears were split. To separate the epidermis and dermis, both halves were placed dermal side down on PBS 0.2% trypsin (Invitrogen) for 25 min at 37°C. In some experiment, PBS 0.5 M ammonium thiocyanate (Sigma-Aldrich) was used to separate the epidermis and dermis with a 40-min incubation at 37°C.

The epidermal sheets were fixed with PBS 3% paraformaldehyde, washed, and permeabilized in PBS 0.5% Triton X-100 (Sigma-Aldrich) for 15 min. Sheets were blocked by normal goat IgG (Invitrogen) in PBS 0.5% Triton X-100 (staining buffer) for 30 min before overnight labeling with rat anti–mouse Ki67 (clone TEC-3; Dako), CD45 (clone 30-F11; BD), langerin (clone 929F3.01; Dendritics), I-A/I-E (clone 2G9; BD), or rat anti–hamster CD11c (clone HL3; BD) antibodies. Samples were washed and incubated with Cy3-conjugated goat anti–rat or Cy3-conjugated goat anti–hamster antibodies (Jackson ImmunoResearch Laboratories, Inc.). To avoid antibody cross-reactions, sheets were blocked with staining buffer supplemented with normal rat IgG (Invitrogen) and further labeled with either rabbit anti-eGFP (Invitrogen) or rabbit antilangerin (clone M-200; Santa Cruz Biotechnology, Inc.). Samples were washed and labeled with Alexa Fluor 488–conjugated goat anti–rabbit (Invitrogen). Sheets were mounted in mounting medium (Vector Laboratories) complemented with DAPI (diluted 1:1,000; Invitrogen) for nuclei staining.

For hematoxylin and eosin (H&E) staining, whole embryos were fixed for 1 wk in neutral buffer formalin (Genta Medical) before paraffin embedding. 6-µm sections were labeled with H&E. After mounting, embryo sections were imaged using a microscope (Axiophot; Carl Zeiss, Inc.).

Preparation and immunostaining of human epidermal sheet.

6-mm punch skin biopsies from four healthy donors and two AD patients (non–steroid treated) were obtained after informed consent and approved by the St. Thomas' Hospital Research Ethics Committee (reference number 06/Q0702/138), and were incubated for 2 h at 37°C in PBS containing 20 mM EDTA. The epidermis was separated from the underlying dermis using forceps and washed several times in PBS. Epidermal sheets were fixed in PBS with 4% formaldehyde at 4°C for 45 min and subsequently washed in PBS. Sheets were stained overnight at room temperature in 500 µl PBS 0.25% Triton X-100 with anti-Ki67 antibody (diluted 1:500; Abcam) and anti–human langerin-PE antibody (diluted 1/10; Coulter Immunotech). Samples were washed twice in PBS 0.1% Tween and incubated for an additional 2 h at room temperature in 300 µl PBS 0.25% Triton X-100 with goat anti–rabbit Alexa Fluor 488 antibody (diluted 1:300; Invitrogen) and donkey anti–mouse IgG1 Cy3 (diluted 1:300; Jackson ImmunoResearch Laboratories, Inc.) before mounting.

Image acquisition and quantitative analysis.

All Z-stack acquisitions were done using a confocal microscope (SP5; Leica) with 20× and 40× lenses. The number of LCs per square millimeter of epidermis was determined by acquiring Z-stacks of immunolabeled epidermal sheets. A minimum of four Z-stacks (0.56 mm²/Z-stack) were acquired per epidermal sheet. The number of cells per Z-stack was enumerated and represented as cells per square millimeter. The distance between a langerin-GFP⁺ cell and its closest GFP⁺ neighbor (Ki67⁺ or Ki67⁻) was measured on a maximal intensity projection of Z-stacks of immunolabeled epidermal sheets. All image quantification and rendering was performed on MetaMorph (MDS Analytical Technologies) and Imaris (Bitplane) software.

Intravital microscopy.

Langerin-GFP CCR2^+/− or CCR2^−/− mice of various ages (P2–P7) were anesthetized using 25 mg/kg ketamine, 5 mg/kg xylazine, and 0.8 mg/kg acepromazine injected intraperitoneally. Mice were kept at 37°C with oxygen (0.5 liter/min). Mice abdomens were placed on a custom-made tray-stage insert with a circular 2.5-cm hole covered with a coverslip. Images were acquired using an inverted confocal microscope (LSM 510; Carl Zeiss, Inc.) equipped with a 20×/0.75 Plan Apochromat objective. A thermostated chamber (Carl Zeiss, Inc.) was used to keep the microscope, mouse, tray, and objective at 37°C during the experiment. Z-stacks (with 1-µm Z-spacing) were acquired on the ventral skin (at least seven Z-stacks per mouse, 0.22 mm²/Z-stack), and the number of langerin-GFP⁺ cells per square millimeter was determined.

LC isolation, PI staining, and cell-cycle analysis.

Skin from langerin-GFP neonates (P4 and P7) and split ears of 10-wk-old mice were incubated in PBS 0.2% trypsin at 37°C for either 1 h or 25 min, respectively. The epidermis was peeled from the dermis and reincubated for 2 h in PBS with 1 mg/ml collagenase D (Roche). An epidermal cell suspension was obtained by mechanical dissociation of epidermal sheets on a 100-µm cell strainer (BD). GFP-expressing LCs were sorted (FACSAria II; BD). Sorted cells were washed with PBS and fixed in 70% ethanol at 4°c for 30 min. After washes, samples were stained with 50 µg/ml PI (Invitrogen) complemented with 50 µg/ml RNaseA (Sigma-Aldrich) at 37°C for 20 min. Samples were analyzed by flow cytometry (FACSAria II). The sorting and cell-cycle analyses were performed as described in Fig. S4.

Antibodies used for flow cytometry.

The following purified or conjugated antibodies were purchased from BD: purified anti-FcγRIII/II (CD32/16; clone 2.4G2), PECy7- or biotin-labeled anti-CD11b (M1/70), allophycocyanin (APC)-labeled anti-CD117 (c-kit; 2B8), biotin-labeled anti-NK1.1 (PK136), biotin- or APC-labeled anti-CD11c (HL3), PECy7- and biotin-labeled anti-CD3 (145-2C11), PECy7- and biotin-labeled anti-CD19 (MB19-1), biotin-labeled anti–I-A/I-E (2G9), PE-labeled anti–I-A^b(AF6-120.1), and biotin-labeled anti-Lyc6 (AL-21). The following antibodies were purchased from eBioscience: PE-labeled anti-Flt3 (A2F10), PE- or biotin-labeled anti-CD115 (AFS98), and PECy7- and biotin-labeled anti-CD127 (A7R34). Antibodies used for depletion, including TER-119 (erythrocytes) and RB6-8C5 (Ly6-C/G), were supernatants of hybridomas donated by B. Rocha (Institut Fédératif de Recherche Necker, Paris, France). Streptavidin Pacific blue was purchased from Invitrogen.

Phenotyping of bone marrow MDPs and CDPs, and epidermal CX₃CR1-GFP⁺ and langerin-GFP⁺ cells.

BM cells from femurs and tibias of CX₃CR1-GFP Rag^−/− γc^−/− mice aged 6–8 wk were flushed with serum-free RPMI 1640. For isolation of MDPs and CDPs, BM granulocytes and erythrocytes were labeled with RB6-8C5 and TER-119, respectively, and depleted using sheep anti–rat Dynabeads (Invitrogen). Fc receptors were blocked with antibody to FcγRIII/II (2.4G2), and cells were labeled using antibodies against lineage markers (IL-7Rα, CD11b, NK1.1, CD3, and CD19), CD117, CD115, CD135, CD11c, and I-A.

Epidermal cells from E18 CX₃CR1-GFP Rag2^−/− γc^−/− embryos and 8-wk-old langerin-GFP mice were isolated with a similar protocol. Fc receptors were blocked with antibody to FcγRIII/II (2.4G2), and cells were labeled using antibodies against CD11b, CD117, CD115, CD135, CD11c, I-A, and Lyc6. MDPs (defined as GFP⁺ [CX₃CR1] lineage⁻ CD117⁺), CDPs (defined as lineage⁻ CD135⁺ CD117^low), and epidermal CX₃CR1-GFP⁺ and langerin-GFP⁺ cells were analyzed by flow cytometry using a FACSAria II. Flow cytometry data were analyzed using Summit software (version 4.3; Dako).

In vivo induction of AD.

Induction of AD by topical application of MC903 (a low calcemic analogue of vitamin D) was performed as previously described (Li et al., 2006; Li et al., 2009). In summary, 10–14-wk-old mice were treated every other day with 1 nmol of MC903 diluted in 25 µl ethanol on the right ear and treated with the same volume of ethanol on the left ear as a control. Immunolabeled epidermis were then analyzed after 4 and 14 d of treatment.