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培养的人鼓膜表皮角质形成细胞的转录和微小RNA分析

Transcription and microRNA Profiling of Cultured Human Tympanic Membrane Epidermal Keratinocytes.

作者信息

Aabel Peder, Utheim Tor Paaske, Olstad Ole Kristoffer, Rask-Andersen Helge, Dilley Rodney James, von Unge Magnus

机构信息

Department of Medical Biochemistry, Oslo University Hospital, Oslo, Norway.

Ear, Nose and Throat Department, Division of Surgery, Akershus University Hospital, Lørenskog, Norway.

出版信息

J Assoc Res Otolaryngol. 2018 Jun;19(3):243-260. doi: 10.1007/s10162-018-0660-1. Epub 2018 Apr 5.

Abstract

The human tympanic membrane (TM) has a thin outer epidermal layer which plays an important role in TM homeostasis and ear health. The specialised cells of the TM epidermis have a different physiology compared to normal skin epidermal keratinocytes, displaying a dynamic and constitutive migration that maintains a clear TM surface and assists in regeneration. Here, we characterise and compare molecular phenotypes in keratinocyte cultures from TM and normal skin. TM keratinocytes were isolated by enzymatic digestion and cultured in vitro. We compared global mRNA and microRNA expression of the cultured cells with that of human epidermal keratinocyte cultures. Genes with either relatively higher or lower expression were analysed further using the biostatistical tools g:Profiler and Ingenuity Pathway Analysis. Approximately 500 genes were found differentially expressed. Gene ontology enrichment and Ingenuity analyses identified cellular migration and closely related biological processes to be the most significant functions of the genes highly expressed in the TM keratinocytes. The genes of low expression showed a marked difference in homeobox (HOX) genes of clusters A and C, giving the TM keratinocytes a strikingly low HOX gene expression profile. An in vitro scratch wound assay showed a more individualised cell movement in cells from the tympanic membrane than normal epidermal keratinocytes. We identified 10 microRNAs with differential expression, several of which can also be linked to regulation of cell migration and expression of HOX genes. Our data provides clues to understanding the specific physiological properties of TM keratinocytes, including candidate genes for constitutive migration, and may thus help focus further research.

摘要

人类鼓膜(TM)有一层薄的外层表皮,这在鼓膜内环境稳定和耳部健康中起着重要作用。与正常皮肤表皮角质形成细胞相比,鼓膜表皮的特化细胞具有不同的生理学特性,表现出动态的、组成性的迁移,维持鼓膜表面清洁并协助再生。在此,我们对来自鼓膜和正常皮肤的角质形成细胞培养物中的分子表型进行表征和比较。通过酶消化分离鼓膜角质形成细胞并在体外培养。我们将培养细胞的整体mRNA和微小RNA表达与人类表皮角质形成细胞培养物的表达进行比较。使用生物统计学工具g:Profiler和 Ingenuity通路分析进一步分析表达相对较高或较低的基因。发现约500个基因差异表达。基因本体富集分析和Ingenuity分析确定细胞迁移及密切相关的生物学过程是鼓膜角质形成细胞中高表达基因的最显著功能。低表达基因在A簇和C簇的同源框(HOX)基因中表现出明显差异,使鼓膜角质形成细胞具有极低的HOX基因表达谱。体外划痕试验显示,鼓膜细胞的细胞运动比正常表皮角质形成细胞更具个体化。我们鉴定出10个差异表达的微小RNA,其中几个也可能与细胞迁移调节和HOX基因表达有关。我们的数据为理解鼓膜角质形成细胞的特定生理特性提供了线索,包括组成性迁移的候选基因,并可能有助于进一步研究的聚焦。

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本文引用的文献

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Epithelialization in Wound Healing: A Comprehensive Review.伤口愈合中的上皮化:综述
Adv Wound Care (New Rochelle). 2014 Jul 1;3(7):445-464. doi: 10.1089/wound.2013.0473.

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