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3-D human epidermal tissue cultures bulk RNA-Seq expression

dataset
posted on 2024-06-26, 21:07 authored by Johann GudjonssonJohann Gudjonsson, Alex Tsoi, Meri OlivaMeri Oliva, Bridget Riley-GillisBridget Riley-Gillis

This dataset corresponds to gene expression changed occurring in the formation of 3-D human epidermal raft cultures. Normal human epidermal keratinocytes were isolated from epidermis (n=3) and grown using J2-3T3 mouse fibroblasts as a feeder layer originally described by Rheinwald and Green53. 3-D human epidermal raft cultures seeded in collagen hydrogels were prepared using three distinct donor pools as described previously54 and grown at an air-liquid interface for 12 days in E-Medium (DMEM/DMEM-F12 (1:1), 5% Fetal Bovine Serum, adenine (180µM), Bovine pancreatic insulin (5µg/ml), Human apo- transferrin (5µg/ml), triiodothyronine (5µg/ml), L-Glutamine (4mM), Cholera toxin (10ng/ml), Gentamicin (10µg/ml), Amphotericin B (0.25µg/ml)). At day 9 at an air-liquid-interface to allow for epidermal maturation, the epidermal rafts (RHE) were treated with 0.1% BSA/phosphate-buffered saline (Sigma Aldrich, St Louis, MO) for 72 Hrs. Epidermal tissues were separated at the stages from Sub-confluent stage to 3-D raft on day 12 (Sub-confluent, Day 0-Confluent, Day 3-Confluent, Day 3-Raft, Day 6-Raft, Day 9-Raft, Day 12-Raft) from the collagen scaffold and lysed in QIAzol for RNA isolation. RNA samples were sent to the University of Michigan Advanced Genomics Core for RNA sequencing. Libraries for RNA-Seq were generated from polyadenylated RNA and sequenced at six libraries per lane on the Illumina Genome Analyzer IIx. We used Tophat2 to align RNA-seq reads to the human genome, using annotations of GENCODE as gene model. HTSeq was used to quantify gene expression levels. Normalization was performed by DESeq2.

Funding

University of Michigan Skin Biology and Diseases Resource-based Center

National Institute of Arthritis and Musculoskeletal and Skin Diseases

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Research Institution(s)

AbbVie Inc. University of Michigan

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Competing Interest Statement

BRG, MO, are or were employees of AbbVie. AbbVie participated in the design, study conduct, interpretation of data, review, and approval of the publication. JEG has received research support from AbbVie, Janssen, Almirall, Prometheus Biosciences/Merck, BMS/Celgene, Boehringer Ingelheim, Galderma, Eli Lilly, and advisor to Sanofi, Eli Lilly, Galderma, BMS, Boehringer Ingelheim. The remaining authors declare no competing interests.

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