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体外成纤维细胞-角质形成细胞共培养:生长、形态测定及营养物质交换

Fibroblast-keratinocyte co-cultures in vitro: growth, morphometry and nutrient exchange.

作者信息

Parnigotto P P, Bassani V, Pastore S, Valenti F, Conconi M T

机构信息

Centro Interdipartimentale per lo Studio dei Cheratinociti: Applicazioni Farmaceutiche e Cliniche, Università di Padova.

出版信息

Ital J Anat Embryol. 1994 Jan-Mar;99(1):17-30.

PMID:7755444
Abstract

The interaction between fibroblasts and rat keratinocytes co-cultured in vitro was examined. The epidermal cells cultured with a basal medium or with a conditioning medium (derived from fibroblast cultures) presented a lower growth rate and significantly greater cellular dimensions than those cells grown in the presence of a feeder layer. Qualitative and quantitative differences in the keratin patterns of the cells grown in the three cultural conditions were found. Keratinocytes cultured with the feeder layer expressed seven keratin types (58, 57, 53, 52, 50, 48 and 45 kDa), those with conditioning medium, five types (58, 53, 52, 48 and 45 kDa) and those with basal medium, only one type (45 kDa). This data confirms the dependence of keratinocytes on fibroblasts. HPLC analysis of the culture media, suggested that a protein factor (MW approximately 65 kDa) was secreted by fibroblasts into the culture medium. This factor was added to the keratinocyte culture medium (conditioning medium), and, after a 48 hour culture, was apparently completely removed from the medium by the keratinocytes. Moreover, the keratinocytes cultured with the feeder layer and exposed to indomethacin, a cyclo-oxygenase inhibitor, showed a decrease in growth rate at drug concentrations of < or = 10 microM which did not induce a reduction in the viability of the fibroblasts and keratinocytes in separate cultures. This preliminary data suggests a relationship between fibroblast PGE2 secretion and keratinocyte growth.

摘要

研究了体外共培养的成纤维细胞与大鼠角质形成细胞之间的相互作用。用基础培养基或条件培养基(源自成纤维细胞培养物)培养的表皮细胞,与在饲养层存在下生长的细胞相比,生长速率较低且细胞尺寸明显更大。发现在三种培养条件下生长的细胞在角蛋白模式上存在定性和定量差异。用饲养层培养的角质形成细胞表达七种角蛋白类型(58、57、53、52、50、48和45 kDa),用条件培养基培养的角质形成细胞表达五种类型(58、53、52、48和45 kDa),而用基础培养基培养的角质形成细胞仅表达一种类型(45 kDa)。该数据证实了角质形成细胞对成纤维细胞的依赖性。对培养基的HPLC分析表明,成纤维细胞向培养基中分泌了一种蛋白质因子(分子量约为65 kDa)。将该因子添加到角质形成细胞培养基(条件培养基)中,培养48小时后,该因子显然被角质形成细胞从培养基中完全清除。此外,用饲养层培养并暴露于环氧化酶抑制剂吲哚美辛的角质形成细胞,在药物浓度≤10 microM时生长速率降低,而该浓度并未导致单独培养的成纤维细胞和角质形成细胞的活力下降。该初步数据表明成纤维细胞分泌的前列腺素E2与角质形成细胞生长之间存在关联。

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