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纤连蛋白、胶原蛋白和整合素表达的微阵列评估以及纤连蛋白-胶原蛋白包被在正常、SV40 T抗原永生化和恶性人口腔角质形成细胞生长中的作用

Microarray assessment of fibronectin, collagen and integrin expression and the role of fibronectin-collagen coating in the growth of normal, SV40 T-antigen-immortalised and malignant human oral keratinocytes.

作者信息

Sarang Zsolt, Haig Ylva, Hansson Annette, Vondracek Martin, Wärngård Lars, Grafström Roland

机构信息

Division of Biochemical Toxicology and Experimental Cancer Research, Institute of Environmental Medicine, Karolinska Institute, 171 77 Stockholm, Sweden.

出版信息

Altern Lab Anim. 2003 Dec;31(6):575-85. doi: 10.1177/026119290303100606.

DOI:10.1177/026119290303100606
PMID:15560747
Abstract

Extracellular matrix proteins affect the growth and survival of epithelial tissues. Accordingly, surface coating with fibronectin and collagen is a common practice for promoting keratinocyte culture. In this study, the expression of fibronectin and collagen-related factors, including integrins, by normal (NOK), SV40 T-antigen-immortalised (SVpgC2a) and malignant (SqCC/Y1) human oral keratinocytes, under standardised, serum-free conditions, was investigated by using microarray analysis. Cell growth was also studied in the presence and absence of a matrix consisting of human fibronectin and bovine collagen type I (FN-COL). Fibronectin transcripts were abundant in all cells, whereas 16 of 29 collagen chains and 14 of 24 integrin subunits were variably detected. With regard to both the expression level and the number of transcripts, higher collagen and lower integrin expression was observed in SVpgC2a cells than in NOKs and SqCC/Y1 cells. The cell types differed with regard to colony-forming efficiency and the rate and kinetics of growth at high cell density. For all cell types, FN-COL coating consistently stimulated cell migration, without influencing growth in mass culture or clonal density. The results demonstrate the transcription of genes associated with the formation and function of fibronectin and collagen in oral epithelium, and variably altered expression patterns in transformed states, and show that keratinocyte lines can be successfully transferred without the stimulus from extracellular FN-COL.

摘要

细胞外基质蛋白影响上皮组织的生长和存活。因此,用纤连蛋白和胶原蛋白进行表面包被是促进角质形成细胞培养的常用方法。在本研究中,通过微阵列分析,研究了正常(NOK)、SV40 T抗原永生化(SVpgC2a)和恶性(SqCC/Y1)人口腔角质形成细胞在标准化无血清条件下纤连蛋白和胶原蛋白相关因子(包括整合素)的表达。还研究了在存在和不存在由人纤连蛋白和I型牛胶原蛋白(FN-COL)组成的基质的情况下细胞的生长情况。纤连蛋白转录本在所有细胞中都很丰富,而29条胶原蛋白链中的16条和24个整合素亚基中的14条被不同程度地检测到。就表达水平和转录本数量而言,SVpgC2a细胞中的胶原蛋白表达高于NOK细胞和SqCC/Y1细胞,而整合素表达则较低。不同细胞类型在集落形成效率以及高细胞密度下的生长速率和动力学方面存在差异。对于所有细胞类型,FN-COL包被始终能刺激细胞迁移,而不影响大规模培养或克隆密度下的生长。结果表明了口腔上皮中与纤连蛋白和胶原蛋白的形成及功能相关的基因转录情况,以及在转化状态下表达模式的不同变化,并且表明角质形成细胞系可以在没有细胞外FN-COL刺激的情况下成功传代。

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