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一种从尾和趾外植体建立用于澳大利亚蜥蜴(有鳞目:鬣蜥科)细胞遗传学研究的原代细胞系的简单非侵入性方案。

A simple non-invasive protocol to establish primary cell lines from tail and toe explants for cytogenetic studies in Australian dragon lizards (Squamata: Agamidae).

机构信息

Comparative Genomics Group, Research School of Biological Sciences, The Australian National University, GPO Box 475, Canberra, ACT, 2601, Australia,

出版信息

Cytotechnology. 2008 Nov;58(3):135-9. doi: 10.1007/s10616-009-9182-3. Epub 2009 Feb 6.

Abstract

Primary cell lines were established from cultures of tail and toe clips of five species of Australian dragon lizards: Tympanocryptis pinguicolla, Tympanocryptis sp., Ctenophorus fordi, Amphibolurus norrisi and Pogona vitticeps. The start of exponential cell growth ranged from 1 to 5 weeks. Cultures from all specimens had fibroblastic morphology. Cell lines were propagated continuously up to ten passages, cryopreserved and recovered successfully. We found no reduction in cell viability after short term (<6 months) storage at -80 degrees C. Mitotic metaphase chromosomes were harvested from these cell lines and used in differential staining, banding and fluorescent in situ hybridisation. Cell lines maintained normal diploidy in all species. This study reports a simple non-invasive method for establishing primary cell lines from Australian dragon lizards without sacrifice. The method is likely to be applicable to a range of species. Such cell lines provide a virtually unlimited source of material for cytogenetic, evolutionary and genomic studies.

摘要

从澳大利亚五种蜥蜴的尾和趾夹培养物中建立了原代细胞系

鼓膜爬蜥、鼓膜爬蜥属、福氏棱蜥、短尾棱蜥和圆鼻巨蜥。指数细胞生长的开始时间范围为 1 至 5 周。所有标本的培养物均呈成纤维细胞形态。细胞系连续传代达 10 代,成功冷冻保存并复苏。我们发现,在-80°C 下短期(<6 个月)储存后,细胞活力没有降低。从这些细胞系中收获有丝分裂中期染色体,并用于差异染色、带型分析和荧光原位杂交。所有物种的细胞系均保持正常的二倍体。本研究报告了一种简单的非侵入性方法,无需牺牲即可从澳大利亚蜥蜴中建立原代细胞系。该方法可能适用于多种物种。这样的细胞系为细胞遗传学、进化和基因组研究提供了几乎无限的材料来源。

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