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整合素α(6)β(1)表达唾液腺移植细胞的分离与培养:一种用于人工唾液腺的模型

Isolation and cultivation of integrin alpha(6)beta(1)-expressing salivary gland graft cells: a model for use with an artificial salivary gland.

作者信息

David Ran, Shai Ela, Aframian Doron J, Palmon Aaron

机构信息

Institute of Dental Sciences, Faculty of Dental Medicine, Hebrew University-Hadassah School of Dental Medicine, Jerusalem, Israel.

出版信息

Tissue Eng Part A. 2008 Feb;14(2):331-7. doi: 10.1089/tea.2007.0122.

Abstract

Regeneration of the salivary glands' (SGs) normal function for patients with cancer of the head and neck treated with irradiation would be a major contribution to their quality of life. This could be accomplished by re-implantation of autologous SG cells into the residual irradiated tissue or by implantation of tissue-engineered artificial SGs. Both methods depend on the isolation of cells able to propagate and differentiate into SG epithelial cells. Recently, it has been shown that SG integrin alpha(6)beta(1)-expressing (SGIE) cells have stem cell capabilities, but these cells could be isolated only after duct ligation insult requiring surgical intervention. Because such an invasive procedure is not clinically acceptable for these patients, our aim in the present study was to explore the use of immuno-magnetic separation of untreated and short heat stress-conditioned rats as a less-insulting methodology for enhancement of these cells. Our results show that submandibular SGIE cells could be isolated and cultivated from untreated animals. However, short heat stress (HS) increased the number of isolated SGIE cells 4.7-fold and their proliferation and clonal capability 4.6-fold and 3 fold, respectively. We believe that SGIE graft cells may be suitable candidates for future tissue-engineered SGs that have been damaged by irradiation in patients with head and neck cancer.

摘要

对头颈部癌症患者进行放射治疗后,使其唾液腺(SGs)的正常功能得以恢复,将对其生活质量有重大贡献。这可以通过将自体SG细胞重新植入残留的受辐照组织,或植入组织工程化人工唾液腺来实现。这两种方法都依赖于分离出能够增殖并分化为唾液腺上皮细胞的细胞。最近的研究表明,表达唾液腺整合素α(6)β(1)的细胞(SGIE细胞)具有干细胞能力,但这些细胞只有在进行需要手术干预的导管结扎损伤后才能分离出来。由于这种侵入性手术对这些患者来说在临床上是不可接受的,因此我们在本研究中的目的是探索采用免疫磁珠分选法,从未经处理和短期热应激预处理的大鼠中分离这些细胞,作为一种损伤较小的方法来富集这些细胞。我们的结果表明,可从未经处理的动物中分离并培养下颌下腺SGIE细胞。然而,短期热应激(HS)使分离出的SGIE细胞数量增加了4.7倍,其增殖能力和克隆能力分别提高了4.6倍和3倍。我们认为,对于头颈部癌症患者中因放疗而受损的唾液腺,SGIE移植细胞可能是未来组织工程化唾液腺的合适候选细胞。

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