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神经生长因子可防止无血清培养基中克隆性PC12嗜铬细胞瘤细胞死亡,并刺激其神经元分化。

Nerve growth factor prevents the death and stimulates the neuronal differentiation of clonal PC12 pheochromocytoma cells in serum-free medium.

作者信息

Greene L A

出版信息

J Cell Biol. 1978 Sep;78(3):747-55. doi: 10.1083/jcb.78.3.747.

Abstract

The PC12 clone is a noradrenergic cell line derived from a rat pheochromocytoma. In culture medium containing horse serum, PC12 cells undergo mitosis; when nerve growth factor (NGF) is included in the medium, the cells cease multiplication and extend neuritis. It is shown here: (a) that PC12 cells are not viable in serum-free medium. When serum is withdrawn, 90 percent of the cells die within 4-6 days and 99 percent by 2-3 wk. (b) If NGF is added at the time of serum withdrawal, the cells undergo one doubling and remain viable for at least 1 mo. (c) Addition of NGF to cultures after more than 2 days in serum-free conditions results in maintenance of surviving cells, but not in an increase in cell number. (d) NGD also induces neurite outgrowth from PC12 cells in serum-free medium. (e) NGF-treated cells exhibit much less cell-cell and neurite-neurite aggregation in the absence than in the presence of serum. (f) The apparent minimum level of 2.5S NGF required for PC12 survival and morphological differentiation in serum-free medium is about 10 ng/ml (approximately 0.4 nM). (g) Withdrawal of NGF in serum-free conditions results in degeneration of neurites and loss of cell viability. (h) Experiments with campotothecin demonstrate that the effects of NGF on survival and neurite outgrowth may be uncoupled and suggest that the survival effects are transcriptionally independent. The present results also suggest that PC12 cells have a requirement for NGF (similar to that of normal sympathetic neurons) and that serum may substitute for this requirement. In addition, the present system of maintaining a highly differentiated cell line in a chemically defined medium suggests certain experimental opportunities.

摘要

PC12 克隆是一种源自大鼠嗜铬细胞瘤的去甲肾上腺素能细胞系。在含有马血清的培养基中,PC12 细胞进行有丝分裂;当培养基中加入神经生长因子(NGF)时,细胞停止增殖并长出神经突。此处显示:(a)PC12 细胞在无血清培养基中无法存活。去除血清后,90%的细胞在 4 - 6 天内死亡,2 - 3 周内 99%的细胞死亡。(b)如果在去除血清时添加 NGF,细胞会进行一次倍增并至少存活 1 个月。(c)在无血清条件下培养超过 2 天后向培养物中添加 NGF 可维持存活细胞,但细胞数量不会增加。(d)NGD 也可在无血清培养基中诱导 PC12 细胞长出神经突。(e)与有血清存在时相比,在无血清情况下,经 NGF 处理的细胞表现出少得多的细胞 - 细胞和神经突 - 神经突聚集。(f)在无血清培养基中,PC12 细胞存活和形态分化所需的 2.5S NGF 的表观最低水平约为 10 ng/ml(约 0.4 nM)。(g)在无血清条件下去除 NGF 会导致神经突退化和细胞活力丧失。(h)喜树碱实验表明,NGF 对存活和神经突生长的影响可能是解偶联的,提示存活效应在转录上是独立的。目前的结果还表明,PC12 细胞对 NGF 有需求(类似于正常交感神经元),血清可能替代这种需求。此外,在化学成分明确的培养基中维持高度分化细胞系的当前系统提示了某些实验机会。

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Proc Natl Acad Sci U S A. 1970 May;66(1):160-7. doi: 10.1073/pnas.66.1.160.
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Effects of camptothecin on RNA synthesis in leukemia L1210 cells.喜树碱对白血病L1210细胞中RNA合成的影响。
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Pheochromocytoma.嗜铬细胞瘤
Cancer. 1972 Feb;29(2):327-31. doi: 10.1002/1097-0142(197202)29:2<327::aid-cncr2820290210>3.0.co;2-3.
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Nerve growth factor.神经生长因子
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