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本文引用的文献

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KINETICS OF HYPERPLASIA IN PSORIASIS.银屑病中增生的动力学
Arch Dermatol. 1963 Oct;88:373-81.
2
Metaplasia produced in cultures of chick ectoderm by high vitamin A.高维生素A在鸡外胚层培养物中产生的化生。
J Physiol. 1953 Mar;119(4):470-88. doi: 10.1113/jphysiol.1953.sp004860.
3
Tumorigenic keratinocyte lines requiring anchorage and fibroblast support cultured from human squamous cell carcinomas.从人鳞状细胞癌培养出的需要锚定和成纤维细胞支持的致瘤性角质形成细胞系。
Cancer Res. 1981 May;41(5):1657-63.
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Heterogeneity in epidermal basal keratinocytes: morphological and functional correlations.表皮基底角质形成细胞的异质性:形态与功能的相关性
Science. 1982 Mar 5;215(4537):1239-41. doi: 10.1126/science.7058342.
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The proteins of living psoriatic epidermis.活动性银屑病表皮的蛋白质
Biochim Biophys Acta. 1982 Jan 12;714(1):164-9. doi: 10.1016/0304-4165(82)90139-8.
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Retinoid effects on epidermal structure, differentiation, and permeability.维甲酸对表皮结构、分化及通透性的影响。
Lab Invest. 1981 Jun;44(6):531-40.
7
Regulation by vitamin A of envelope cross-linking in cultured keratinocytes derived from different human epithelia.维生素A对源自不同人类上皮组织的培养角质形成细胞包膜交联的调节作用。
Mol Cell Biol. 1982 Sep;2(9):1115-7. doi: 10.1128/mcb.2.9.1115-1117.1982.
8
Regulation of the expression of epidermal keratinocyte proliferation and differentiation by vitamin A analogs.维生素A类似物对表皮角质形成细胞增殖和分化表达的调控
Arch Dermatol Res. 1984;276(6):381-9. doi: 10.1007/BF00413359.
9
Cloning of cDNAs specifying vitamin A-responsive human keratins.
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10
Differences in keratin synthesis between normal epithelial cells and squamous cell carcinomas are mediated by vitamin A.正常上皮细胞与鳞状细胞癌之间角蛋白合成的差异由维生素A介导。
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使用视黄酸探究正常和恶性表皮细胞中与过度增殖相关的角蛋白和细胞增殖之间的关系。

The use of retinoic acid to probe the relation between hyperproliferation-associated keratins and cell proliferation in normal and malignant epidermal cells.

作者信息

Kopan R, Fuchs E

机构信息

Howard Hughes Medical Institute, Department of Molecular Genetics and Cell Biology, University of Chicago, Illinois 60637.

出版信息

J Cell Biol. 1989 Jul;109(1):295-307. doi: 10.1083/jcb.109.1.295.

DOI:10.1083/jcb.109.1.295
PMID:2473080
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC2115483/
Abstract

When cells from normal human epidermis and from the human squamous cell carcinoma line SCC-13 were seeded on floating rafts of collagen and fibroblasts, they stratified and underwent terminal differentiation. Although the program of differentiation in SCC-13 cells was morphologically abnormal, the cultures resembled normal epidermal raft cultures by expressing the terminal differentiation-specific keratins, K1/K10, and by restricting their proliferative capacity to the basal-like cells of the population. In addition, the differentiating cells of both normal and SCC-13 raft cultures expressed keratins K6 and K16, which are not normally expressed in epidermis, but are synthesized suprabasally during wound-healing and in various epidermal diseases associated with hyperproliferation. While the behavior of normal and SCC-13 rafts was quite similar when they were cultured over normal medium, significant biochemical differences began to emerge when the cultures were exposed to retinoic acid. Most notably, while the SCC-13 cultures still stratified extensively, they showed a marked inhibition of both abnormal (K6/K16) and normal (K1/K10) differentiation-associated keratins, concomitantly with an overall disappearance of differentiated phenotype. Surprisingly, the reduction in K6/K16 in retinoid-treated SCC-13 cultures was not accompanied by a decrease in cell proliferation. Using immunohistochemistry combined with [3H]thymidine labeling, we demonstrate that while the expression of K6 and K16 are often associated with hyperproliferation, these keratins are only produced in the nondividing, differentiating populations of proliferating cultures. Moreover, since their expression can be suppressed without a corresponding decrease in proliferation, the expression of these keratins cannot be essential to the nature of the hyperproliferative epidermal cell.

摘要

当将来自正常人表皮的细胞以及人鳞状细胞癌系SCC - 13的细胞接种到胶原蛋白和成纤维细胞的漂浮筏上时,它们会分层并经历终末分化。尽管SCC - 13细胞中的分化程序在形态上是异常的,但这些培养物通过表达终末分化特异性角蛋白K1/K10,并将其增殖能力限制在群体中基底样细胞,类似于正常表皮筏培养物。此外,正常和SCC - 13筏培养物的分化细胞均表达角蛋白K6和K16,这两种角蛋白在表皮中通常不表达,但在伤口愈合期间以及与过度增殖相关的各种表皮疾病中在基底上层合成。当正常和SCC - 13筏在正常培养基上培养时,它们的行为相当相似,但当培养物暴露于视黄酸时,显著的生化差异开始显现。最值得注意的是,虽然SCC - 13培养物仍广泛分层,但它们显示出对异常(K6/K16)和正常(K1/K10)分化相关角蛋白的明显抑制,同时分化表型总体消失。令人惊讶的是,在视黄酸处理的SCC - 13培养物中K6/K16的减少并未伴随着细胞增殖的降低。使用免疫组织化学结合[³H]胸苷标记,我们证明虽然K6和K16的表达通常与过度增殖相关,但这些角蛋白仅在增殖培养物的非分裂、分化群体中产生。此外,由于它们的表达可以被抑制而增殖没有相应降低,这些角蛋白的表达对于过度增殖的表皮细胞的性质并非必不可少。