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一种培养秀丽隐杆线虫胚胎细胞的方法。

A method for culturing embryonic C. elegans cells.

作者信息

Sangaletti Rachele, Bianchi Laura

机构信息

Department of Physiology and Biophysics, University of Miami.

出版信息

J Vis Exp. 2013 Sep 21(79):e50649. doi: 10.3791/50649.

Abstract

C. elegans is a powerful model system, in which genetic and molecular techniques are easily applicable. Until recently though, techniques that require direct access to cells and isolation of specific cell types, could not be applied in C. elegans. This limitation was due to the fact that tissues are confined within a pressurized cuticle which is not easily digested by treatment with enzymes and/or detergents. Based on early pioneer work by Laird Bloom, Christensen and colleagues developed a robust method for culturing C. elegans embryonic cells in large scale. Eggs are isolated from gravid adults by treatment with bleach/NaOH and subsequently treated with chitinase to remove the eggshells. Embryonic cells are then dissociated by manual pipetting and plated onto substrate-covered glass in serum-enriched media. Within 24 hr of isolation cells begin to differentiate by changing morphology and by expressing cell specific markers. C. elegans cells cultured using this method survive for up 2 weeks in vitro and have been used for electrophysiological, immunochemical, and imaging analyses as well as they have been sorted and used for microarray profiling.

摘要

秀丽隐杆线虫是一个强大的模型系统,在其中遗传和分子技术很容易应用。然而直到最近,需要直接接触细胞并分离特定细胞类型的技术还无法在秀丽隐杆线虫中应用。这种限制是由于组织被限制在一个加压的角质层内,而用酶和/或去污剂处理不易将其消化。基于莱尔德·布鲁姆早期的开创性工作,克里斯蒂安森及其同事开发了一种大规模培养秀丽隐杆线虫胚胎细胞的可靠方法。通过用漂白剂/氢氧化钠处理从怀孕成虫中分离出卵,随后用几丁质酶处理以去除卵壳。然后通过手动移液将胚胎细胞解离,并接种到富含血清的培养基中覆盖有底物的玻璃上。分离后24小时内,细胞开始通过改变形态和表达细胞特异性标记物进行分化。使用这种方法培养的秀丽隐杆线虫细胞在体外可存活长达2周,并已用于电生理、免疫化学和成像分析,以及它们已被分选并用于微阵列分析。

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