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大鼠神经肿瘤RT4的克隆亚系与细胞分化。VI. 染色体分析。

Clonal sublines of rat neurotumor RT4 and cell differentiation. VI. Chromosome analysis.

作者信息

Haag M M, Soukup S W, Sueoka N

出版信息

Dev Biol. 1984 Jul;104(1):240-6. doi: 10.1016/0012-1606(84)90051-4.

Abstract

The RT4 neurotumor cell system consists of clonally derived cell lines where a stem cell type segregates in vitro into three biochemically and morphologically different cell types, one glial and two neuronal types. This process has been termed cell-type conversion (M. Imada and N. Sueoka, 1978, Dev. Biol. 66, 97-108). Detailed cytogenetic analysis of the RT4 cell lines are described. Giemsa-banding analysis of 12 independent clonal isolates of the four different RT4 cell types showed a relatively stable karyotype. The stem cell line, RT4-AC, is diploid and most stable, and it has one 4q+ marker chromosome in place of a normal No. 4. This 4q+ marker was identified in all cell types of the RT4 system and was not observed in other cell lines of BDIX origin. The 4q+, therefore, is a chromosomal marker of the RT4 system. Consistent chromosome rearrangement was not found in any one of the cell-type conversions of the RT4-AC cells into the three derivative cell types. The relative stability of the karyotype of the different clonal isolates gives the RT4 system an advantage in studies of genetic regulation and expression of cell-type conversion in vitro. Also the 4q+ marker can be used to identify RT4 cells in coculture experiments or to distinguish RT4 cells in cases of suspected cell-line contamination.

摘要

RT4神经肿瘤细胞系统由克隆衍生的细胞系组成,其中一种干细胞类型在体外分离为三种生化和形态不同的细胞类型,一种是神经胶质细胞类型,两种是神经元细胞类型。这个过程被称为细胞类型转换(M. 今田和N. 末冈,1978年,《发育生物学》66卷,97 - 108页)。本文描述了对RT4细胞系的详细细胞遗传学分析。对四种不同RT4细胞类型的12个独立克隆分离株进行吉姆萨带型分析,结果显示核型相对稳定。干细胞系RT4 - AC是二倍体且最稳定,它有一条4号染色体长臂增加的标记染色体取代了正常的4号染色体。这条4号染色体长臂增加的标记染色体在RT4系统的所有细胞类型中都能找到,而在源自BDIX的其他细胞系中未观察到。因此,4号染色体长臂增加是RT4系统的一个染色体标记。在RT4 - AC细胞向三种衍生细胞类型的任何一种细胞类型转换过程中,均未发现一致的染色体重排。不同克隆分离株核型的相对稳定性使RT4系统在体外细胞类型转换的遗传调控和表达研究中具有优势。此外,4号染色体长臂增加的标记可用于在共培养实验中鉴定RT4细胞,或在怀疑细胞系污染的情况下区分RT4细胞。

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