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中国生物工程杂志

CHINA BIOTECHNOLOGY
中国生物工程杂志  2006, Vol. 26 Issue (0): 82-86    
专稿     
鸡成纤维细胞的分离与体外培养
王娟
滨洲医学院基础医学部生物技术教研室
Dissociation and in vitro culture and of Chicken Fibroblasts
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摘要:

探讨鸡成纤维细胞的体外培养体系。在比较组织块法和消化法分离培养鸡皮肤成纤维细胞的基础上,发现酶消化培养的成纤维细胞原代生长快,约2天便可形成单层。两种方法传代细胞的生长速度相似,仅需2~3d就可形成单层。用0.25%的胰酶消化鸡胚组织,可获得足够原代培养的细胞量。使用酶消化法和反复贴壁法,经3~4代后,可获得纯化的成纤维细胞。成纤维细胞经冷冻复苏后有75%~80%存活。分离纯化的胚胎和皮肤成纤维细胞的生长曲线都正常。成纤维细胞可传至12代,传代后染色体数目不变。

Abstract:

The objective of this study was to develop a practical in vitro culture system of chicken fibroblasts to facilitate further studies on the feeder cells of chicken embryonic stem cells. Explant techniques and monolayer culture in culturing chicken fibroblasts were compared, the primary chichen fibroblasts derived from tissue explant culture grown slowly and confluented together by 6~7 days of culture, while cells derived from enzymatic digestion grown faster and confluented together by 5 days of culture. However the growing speed of passaged fibrlblasts derived from the two methods was similar, which could confluent within 2 to 3 days of culture. Chicken embryonic tissue digested by 0.25% trypsin provided a high yield of viable proliferating for primary culture. Homogeneous fibroblasts could be obtained after the mixture of fibroblasts and epithelial cells were treated by the combined use of typsin digestion and repeated attachment method for three or four subcultures. There were 75%-80% of cells survived after frozen and thawed. The growth curves of fetal and skin fibroblasts were normal and similar. Chicken embryonic and skin fibroblasts could subculture 12th generation and still retained the normal chromosome content.

收稿日期: 2006-03-07 出版日期: 2006-06-15
通讯作者: 王娟   
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引用本文:

王娟. 鸡成纤维细胞的分离与体外培养[J]. 中国生物工程杂志, 2006, 26(0): 82-86.

. Dissociation and in vitro culture and of Chicken Fibroblasts. China Biotechnology, 2006, 26(0): 82-86.

链接本文:

https://manu60.magtech.com.cn/biotech/CN/        https://manu60.magtech.com.cn/biotech/CN/Y2006/V26/I0/82

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