Genomic DNA from normotrophic scar fibroblasts from patient 5 data from: Methylation profiling by genome tiling array

Experiment type: Methylation profiling by genome tiling array Summary: 3mm punch biopsies were taken from a healed normotrophic scar and a contralateral matched control site in burn patients with a scar at least 1 year old. Fibroblasts were cultured from explants to passage 2 and DNA was extracted and run on methylation arrays to examine differences in scar and control fibroblast gene expression Normotrophic scar maintains its abnormal scar phenotype for the rest of the patients life, long after the injury has healed. Differences in gene expression may reaveal target genes that can be modulated to improve scar appearance. Overall design: 6 patients had normotrophic scar and matched control fibroblasts extracted and compared. Sample type genomic Source name Patient 5 Scar Organism Homo sapiens Characteristics Sex: Male age (years): 25 time since injury (years): 5 Treatment protocol There were no treatments applied to the scar and control cells in vitro. DNA was bisulfite treated prior to processing on the chip Growth protocol 3mm punch biopsies were taken from the forearm scar site and a matched site on the uninjured forearm by the attendant physician. Tissue was transported to the lab where it was placed in a petri dish and sliced into three equal sized potions. Pieces of the biopsy were then placed dermis side down in a T-25 (25 cm2) (Greiner Bio-One, Germany) culture flask without any media, and a drop of 100% foetal bovine serum (FBS) added to the surface of each piece. They were then cultured in DMEM with 10% FBS and 5% pen/strep until passage 2, at which point DNA and RNA was extracted. Extracted molecule genomic DNA Extraction protocol Genomic DNA was extracted using either the Promega Wizard SV Genomic DNA system (Patients 1 and 2, Promega, USA) or the QIAamp DNA mini kit system (Patients 3-6, Qiagen, Netherlands) as per manufacturer’s instructions Label Cy3 and Cy5 Label protocol Standard Illumina protocol Hybridization protocol bisulphite converted DNA was amplified, fragmented and hybridised to Illumina Infinium Human Methylation27 Beadchip using standard Illumina protocol Scan protocol Arrays were imaged using BeadArray Reader using standard recommended Illumina scanner setting Description Normotrophic Scar Fibroblast DNA Data processing Methylation data was imported from the raw files using Illumina® GenomeStudio and analysed using R statistics software, using the RnBeads package

实验类型：基于基因组平铺阵列的甲基化谱分析 研究概述：从瘢痕形成至少1年的烧伤患者身上，分别采集愈合后稳定的正常肥厚性瘢痕（normotrophic scar）及对侧匹配对照部位的组织样本。从组织外植体中培养成纤维细胞至第2代，提取DNA后进行甲基化芯片检测，以分析瘢痕组织与对照成纤维细胞的基因表达差异。 正常肥厚性瘢痕会在患者余生中持续保持异常瘢痕表型，即便损伤早已愈合。基因表达差异的解析可揭示可被调控以改善瘢痕外观的靶基因。 实验设计：共纳入6名患者，分别提取其正常肥厚性瘢痕及匹配对照的成纤维细胞并进行对比分析。 样本类型：基因组样本 样本来源名称：患者5瘢痕组织 生物来源：智人（Homo sapiens） 样本特征：性别：男；年龄（岁）：25；损伤后时间（年）：5 处理方案：体外实验中未对瘢痕及对照细胞施加任何处理。DNA在芯片上机前进行亚硫酸氢盐转化处理。 培养方案：由主治医师从前臂瘢痕部位及未损伤前臂的匹配部位采集3mm直径穿刺活检样本。样本被运送至实验室后置于培养皿中，切分为三等份。将活检组织块真皮侧朝下放置于T-25（25 cm²，Greiner Bio-One，德国）培养瓶中，不添加培养基，并在每块组织表面滴加100%胎牛血清（FBS）。随后将组织置于含10% FBS及5%青链霉素的DMEM培养基中培养至第2代，此时提取DNA与RNA。 提取分子：基因组DNA 提取方案：基因组DNA提取分别采用Promega Wizard SV基因组DNA提取试剂盒（患者1、2，Promega，美国）或QIAamp DNA迷你试剂盒（患者3-6，Qiagen，荷兰），操作严格遵循制造商说明书。 标记物：Cy3与Cy5 标记流程：采用标准Illumina标记方案 杂交方案：将亚硫酸氢盐转化后的DNA进行扩增、片段化，随后采用标准Illumina流程与Illumina Infinium Human Methylation27 Beadchip进行杂交。 扫描方案：采用BeadArray阅读器，按照Illumina官方推荐的标准扫描仪设置对芯片进行成像。 样本描述：正常肥厚性瘢痕成纤维细胞DNA 数据处理：甲基化数据通过Illumina® GenomeStudio从原始文件中导入，并使用R统计软件及RnBeads包进行分析。