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与小鼠神经母细胞瘤细胞中的颗粒相关的局部儿茶酚胺储存。

Localized catecholamine storage associated with granules in murine neuroblastoma cells.

作者信息

Breakfield X O, Neale E A, Neale J H, Jacobowitz D M

出版信息

Brain Res. 1975 Jul 11;92(2):237-56. doi: 10.1016/0006-8993(75)90273-5.

DOI:10.1016/0006-8993(75)90273-5
PMID:240485
Abstract

Catecholamine storage was examined in cultures of the murine neuroblastoma cell line, N-TD6, using histofluorescence, electron microscopic, isotopic and radioautographic criteria. This line was originally derived from uncloned, C1300 tumor cells by selection in tyrosine deficient medium. N-TD6 cells possess both tyrosine hydroxylase (tyrosine-3-monooxygenase, EC 1.14.16.2) and dopamine beta-hydroxylase (dopamine beta-monooxygenase, EC 1.14.17.1) activities. When examined for paraformaldehyde-induced histofluorescence, a small percentage of cells in the population show intense catecholamine fluorescence, often localized within discrete regions of the cellular processes. Electron microscopic examination of these cells reveals both electron lucent vesicles and more frequent, electron dense granules, 50-70 nm and 100-300 nm in diameter, respectively. The distribution of these granules and vesicles varies, but they appear most numerous near the cell surface, along processes and within process endings. By labeling cells with [3H]dopamine and then allowing the cells to release unbound label in the presence of unlabeled dopamine, the localization of catecholamine stores was visualized by radioautographic techniques. While a variety of intracellular distribution of radioactivity were observed, the most prominent concentrations were found in the processes and their terminals; no labeled material was retained when reserpine was present during uptake. The topographic coincidence of granules, catecholamine fluorescence and [3H]dopamine retention in these neuroblastoma cells suggests that catecholamines are stored within these granules in a manner analogous to that observed in normal adrenergic neurons.

摘要

利用组织荧光、电子显微镜、同位素和放射自显影标准,对小鼠神经母细胞瘤细胞系N-TD6的培养物中的儿茶酚胺储存情况进行了检测。该细胞系最初是通过在酪氨酸缺乏培养基中筛选从未克隆的C1300肿瘤细胞中获得的。N-TD6细胞同时具有酪氨酸羟化酶(酪氨酸-3-单加氧酶,EC 1.14.16.2)和多巴胺β-羟化酶(多巴胺β-单加氧酶,EC 1.14.17.1)的活性。当检测多聚甲醛诱导的组织荧光时,群体中的一小部分细胞显示出强烈的儿茶酚胺荧光,通常定位于细胞突起的离散区域内。对这些细胞的电子显微镜检查发现了电子透明囊泡和更常见的电子致密颗粒,其直径分别为50-70纳米和100-300纳米。这些颗粒和囊泡的分布各不相同,但它们在细胞表面附近、沿着突起以及在突起末端似乎最为丰富。通过用[3H]多巴胺标记细胞,然后在未标记多巴胺存在的情况下让细胞释放未结合的标记物,利用放射自显影技术观察到了儿茶酚胺储存的定位。虽然观察到了放射性的多种细胞内分布,但最显著的浓度出现在突起及其末端;摄取过程中存在利血平时,没有保留标记物质。这些神经母细胞瘤细胞中颗粒、儿茶酚胺荧光和[3H]多巴胺保留的地形学一致性表明,儿茶酚胺以类似于正常肾上腺素能神经元中观察到的方式储存在这些颗粒中。

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