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人白血病细胞系K562中珠蛋白和血型糖蛋白基因表达对血红素的不同反应。

Differing responses of globin and glycophorin gene expression to hemin in the human leukemia cell line K562.

作者信息

Tonkonow B L, Hoffman R, Burger D, Elder J T, Mazur E M, Murnane M J, Benz E J

出版信息

Blood. 1982 Apr;59(4):738-46.

PMID:7037071
Abstract

The human leukemia cell line, K562, produces embryonic and fetal hemoglobins and glycophorin A, proteins normally associated only with erythroid cells. Hemoglobin accumulation is enhanced by exposure of the cells to 0.05 mM hemin. We have examined K562 cells before and after exposure to hemin to determine whether expression of these erythroid proteins was shared by all cells or confined to specific subpopulations. Globin gene expression was examined by quantitation of globin mRNA sequences, using a 3H-globin cDNA molecular hybridization probe. Constitutive cells produced globin mRNA, the content of which was increased 3-4-fold by hemin. Cell-to-cell distribution of globin mRNA was determined by in situ hybridization of 3H-globin cDNA to constitutive and hemin-treated K562 cells. Virtually all cells in the culture exhibited grain counts above background, indicating globin gene expression by all cells, rather than a confined subpopulation. Virtually all hemin-treated cells had 3-5-fold higher grain counts, indicating uniformly increased globin gene expression. The glycophorin content of K562 cells was estimated by fluorescence-activated cell sorting (FACS) of cells labeled with fluorescein-labeled antiglycophorin antiserum. The vast majority of constitutive cells contained glycophorin, but exhibited to apparent increase in glycophorin accumulation after hemin exposure. Thus, glycophorin and globin genes exhibited differential responses to hemin. These differences could reflect normal differences in the patterns of specialized gene expression in stem cells. Alternatively, different aberrations of gene expression could be occurring in response to the determinants of the neoplastic properties of K562.

摘要

人白血病细胞系K562能产生胚胎和胎儿血红蛋白以及血型糖蛋白A,这些蛋白通常仅与红细胞相关。将细胞暴露于0.05 mM的血红素中可增强血红蛋白的积累。我们检测了暴露于血红素前后的K562细胞,以确定这些红细胞蛋白的表达是所有细胞都具有还是局限于特定亚群。通过使用3H-珠蛋白cDNA分子杂交探针定量珠蛋白mRNA序列来检测珠蛋白基因的表达。组成型细胞产生珠蛋白mRNA,血红素可使其含量增加3至4倍。通过将3H-珠蛋白cDNA原位杂交到组成型和经血红素处理的K562细胞来确定珠蛋白mRNA的细胞间分布。培养物中的几乎所有细胞的颗粒计数均高于背景值,表明所有细胞都有珠蛋白基因表达,而不是局限于特定亚群。几乎所有经血红素处理的细胞的颗粒计数都高3至5倍,表明珠蛋白基因表达均匀增加。通过对用荧光素标记的抗血型糖蛋白抗血清标记的细胞进行荧光激活细胞分选(FACS)来估计K562细胞的血型糖蛋白含量。绝大多数组成型细胞含有血型糖蛋白,但在血红素暴露后血型糖蛋白的积累没有明显增加。因此,血型糖蛋白和珠蛋白基因对血红素表现出不同的反应。这些差异可能反映了干细胞中特殊基因表达模式的正常差异。或者,可能是由于K562肿瘤特性的决定因素而发生了不同的基因表达异常。

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