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在合成膜上重建的人表皮:实验条件对终末分化的影响。

Human epidermis reconstructed on synthetic membrane: influence of experimental conditions on terminal differentiation.

作者信息

Noël-Hudson M S, Dusser I, Collober I, Muriel M P, Bonté F, Meybeck A, Font J, Wepierre J

机构信息

Laboratoire de Pharmacologie, Faculté de Pharmacie, Châtenay-Malabry, France.

出版信息

In Vitro Cell Dev Biol Anim. 1995 Jul-Aug;31(7):508-15. doi: 10.1007/BF02634028.

DOI:10.1007/BF02634028
PMID:8528499
Abstract

Cell suspensions of human keratinocytes seeded onto cell culture inserts may undergo terminal differentiation in the absence of fibroblasts. Among the parameters that control these morphogenic events, exposure to air and the composition of the culture medium were investigated. In the latter case, three media were considered DMEM:Ham's F12, MCDB 153, and keratinocyte SFM medium at equivalent calcium (1.5 mM) and fetal calf serum (5%) concentrations. Immunochemical methods and transmission electron microscopy show that cells cultured in DMEM:Ham's F12 medium, and then raised at the air-liquid interface, form a basal layer plus suprabasal cell layers corresponding to the stratum spinosum, stratum granulosum, and stratum corneum. The suprabasal keratinocyte layers show morphologies that resemble intact skin in which cells are connected by desmosomes and contain intermediate filaments and keratohyalin-filaggrin granules. When the cultures are kept submerged, the keratinocytes show occasional keratohyalin granules and are connected by fewer desmosomes. Additionally, no proper stratum corneum is formed. In keratinocyte SFM medium and MCDB 153, cultures raised at the air-liquid interface are not able to form an epithelium of normal architecture and do not express terminal differentiation markers. Differentiation is initiated, however, since desmosomes and bundles of keratin filaments appear; on the other hand, filaggrin is not expressed even after 28 d in culture. Membrane-bound transglutaminase is expressed throughout the entire suprabasal compartment in MCDB153 and DMEM:Ham's F12 media but never appears in keratinocyte SFM medium. These studies show the relative independence of epidermal differentiation program to the composition (including the calcium concentration) of the media contacting the dermis and filling the extracellular space.(ABSTRACT TRUNCATED AT 250 WORDS)

摘要

接种在细胞培养插入物上的人角质形成细胞悬液在没有成纤维细胞的情况下可能会发生终末分化。在控制这些形态发生事件的参数中,研究了暴露于空气和培养基的成分。在后一种情况下,考虑了三种培养基:DMEM:Ham's F12、MCDB 153和角质形成细胞SFM培养基,它们具有相同的钙(1.5 mM)和胎牛血清(5%)浓度。免疫化学方法和透射电子显微镜显示,在DMEM:Ham's F12培养基中培养,然后在气液界面培养的细胞形成了一个基底层加上对应于棘层、颗粒层和角质层的基底层以上细胞层。基底层以上的角质形成细胞层显示出类似于完整皮肤的形态,其中细胞通过桥粒连接,并含有中间丝和角蛋白透明颗粒-细丝聚集蛋白颗粒。当培养物保持浸没状态时,角质形成细胞偶尔会出现角蛋白透明颗粒,并且通过较少的桥粒连接。此外,没有形成适当的角质层。在角质形成细胞SFM培养基和MCDB 153中,在气液界面培养的培养物无法形成正常结构的上皮,也不表达终末分化标志物。然而,由于桥粒和角蛋白丝束出现,分化开始;另一方面,即使在培养28天后,细丝聚集蛋白也不表达。膜结合转谷氨酰胺酶在MCDB153和DMEM:Ham's F12培养基的整个基底层以上隔室中表达,但在角质形成细胞SFM培养基中从未出现。这些研究表明表皮分化程序相对于接触真皮并填充细胞外空间的培养基成分(包括钙浓度)具有相对独立性。(摘要截断于250字)

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本文引用的文献

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