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建立具有从无毛囊皮肤诱导毛囊能力的大鼠真皮乳头细胞系。

Establishment of rat dermal papilla cell lines that sustain the potency to induce hair follicles from afollicular skin.

作者信息

Inamatsu M, Matsuzaki T, Iwanari H, Yoshizato K

机构信息

Yoshizato MorphoMatrix Project, ERATO, Japan Science and Technology Corporation, Higashihiroshima, Hiroshima.

出版信息

J Invest Dermatol. 1998 Nov;111(5):767-75. doi: 10.1046/j.1523-1747.1998.00382.x.

Abstract

Dermal papilla cells in culture show a lower proliferative capacity compared with dermal fibroblasts, and lose their in situ potency to induce hair follicles in the epidermis at more than 10 passage numbers. This study overcomes these limitations of cultured papilla cells and for the first time demonstrates that papilla cells can be serially cultured for a long period without losing their hair-inductive potency. Outgrowth and the ensuing proliferation of papilla cells were markedly stimulated when explants of rat vibrissa papillae were cultured with rat sole-derived keratinocytes. Such feeder effects of the keratinocytes could be replaced to some extent with conditioned medium of the cells. Serial cultivation of papilla cells was established by maintaining them in the conditioned medium in which they were subcultured for more than 90 passages with an approximate population doubling time of 30 h, a value similar to that of rat dermal fibroblasts. During the subculture, they showed morphologic characteristics and phenotypic expressions of original papilla cells. Even after at least 70 passages, papilla cells sustained the innate hair follicle inductive ability at a level comparable with that of intact dermal papillae. The established cell lines did not show tumorigenicity when they were subcutaneously implanted into nude mice. The culture method developed in this study should facilitate the search for a biochemical entity of dermal papilla cells.

摘要

与真皮成纤维细胞相比,培养的毛乳头细胞增殖能力较低,并且在传代超过10次后会丧失其在表皮中诱导毛囊的原位能力。本研究克服了培养的乳头细胞的这些局限性,首次证明乳头细胞可以长期连续培养而不丧失其毛发诱导能力。当用大鼠足底来源的角质形成细胞培养大鼠触须乳头外植体时,乳头细胞的生长及随后的增殖受到显著刺激。角质形成细胞的这种饲养层效应在一定程度上可用细胞条件培养基替代。通过将乳头细胞维持在条件培养基中建立了乳头细胞的连续培养,在该条件培养基中它们传代培养超过90次,群体倍增时间约为30小时,这一数值与大鼠真皮成纤维细胞相似。在传代培养过程中,它们表现出原始乳头细胞的形态特征和表型表达。即使在至少70次传代后,乳头细胞仍保持与完整真皮乳头相当的固有毛囊诱导能力。当将建立的细胞系皮下植入裸鼠时,未显示出致瘤性。本研究中开发的培养方法应有助于寻找毛乳头细胞的生化实体。

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