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125I-神经生长因子在分隔培养的大鼠交感神经元中的逆行运输和稳态分布

Retrograde transport and steady-state distribution of 125I-nerve growth factor in rat sympathetic neurons in compartmented cultures.

作者信息

Ure D R, Campenot R B

机构信息

Department of Cell Biology and Anatomy, University of Alberta, Edmonton, Alberta, Canada T6G 2H7.

出版信息

J Neurosci. 1997 Feb 15;17(4):1282-90. doi: 10.1523/JNEUROSCI.17-04-01282.1997.

Abstract

We have used compartmented cultures of rat sympathetic neurons to quantitatively examine the retrograde transport of 125I-nerve growth factor (NGF) supplied to distal axons and to characterize the cellular events that maintain steady-state levels of NGF in cell bodies. In cultures allowed to reach steady-state 125I-NGF transport, cell bodies contained only 5-30% of the total neuron-associated 125I-NGF, whereas 70-95% remained associated with the distal axons. This was true over an 8 pM to 1.5 nM 125I-NGF concentration range, indicating that saturation of high affinity receptors could not account for the large fraction of 125I-NGF remaining in axons. Dissociation assays indicated that 85% of 125I-NGF associated with distal axons was surface-bound. At steady-state, only 2-25% of the distal axon-associated 125I-NGF was retrogradely transported each hour, with higher transport rates associated with younger cultures and lower 125I-NGF concentrations. The velocity of 125I-NGF retrograde transport was estimated at 10-20 mm/hr. However, as in a previous report, almost no 125I-NGF transport was observed during the first hour after 125I-NGF administration, indicating a significant lag between receptor binding and loading onto the retrograde transport system. During 125I-NGF transport through axons spanning an intermediate compartment in five-compartment cultures, little or no 125I-NGF was degraded or released from the axons. After transport, 125I-NGF was degraded with a half-life of 3 hr. In summary, although some cellular events promoted NGF accumulation in cell bodies, distal axons represented by far the principal site of NGF-receptor interaction at steady-state as a result of a low retrograde transport rate.

摘要

我们利用大鼠交感神经元的分隔培养来定量检测供应给远端轴突的125I-神经生长因子(NGF)的逆行运输,并描述维持细胞体中NGF稳态水平的细胞事件。在达到125I-NGF运输稳态的培养物中,细胞体仅含有与神经元相关的总125I-NGF的5%-30%,而70%-95%仍与远端轴突相关。在8 pM至1.5 nM的125I-NGF浓度范围内均是如此,这表明高亲和力受体的饱和不能解释大部分125I-NGF仍留在轴突中的现象。解离分析表明,与远端轴突相关的125I-NGF中有85%是表面结合的。在稳态时,每小时只有2%-25%与远端轴突相关的125I-NGF被逆行运输,运输速率较高与较年轻的培养物以及较低的125I-NGF浓度相关。125I-NGF逆行运输的速度估计为10-20毫米/小时。然而,正如之前的一份报告中所述,在给予125I-NGF后的第一个小时内几乎没有观察到125I-NGF的运输,这表明受体结合与装载到逆行运输系统之间存在显著延迟。在125I-NGF通过五分隔培养物中跨越中间隔室的轴突运输过程中,很少或没有125I-NGF从轴突中降解或释放。运输后,125I-NGF以3小时的半衰期降解。总之,尽管一些细胞事件促进了NGF在细胞体中的积累,但由于逆行运输速率较低,在稳态时远端轴突是NGF-受体相互作用的主要部位。

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