Freeman J A, Manis P B, Snipes G J, Mayes B N, Samson P C, Wikswo J P, Freeman D B
J Neurosci Res. 1985;13(1-2):257-83. doi: 10.1002/jnr.490130118.
The rate and direction of neurite growth have been shown in a number of studies to be determined by the distribution of adhesive sites on the growth cone. Recent evidence showing that the application of extrinsic electric fields can redistribute membrane molecules and alter both the rate and direction of neurite growth have raised the question whether endogenous electric fields might be produced by steady currents in growth cones. To investigate this question, we have devised a novel circularly vibrating microprobe capable of measuring current densities in the range of 5 nA/cm2 (near the theorectical limit of sensitivity), with a spatial resolution of 2 micron. The design of this device and the development of a novel algorithm for computing current vectors on-line is described. Using this probe we have found that cultured goldfish retinal ganglion cell growth cones generate steady inward currents at their tips. The measured currents, in the range of 10-100 nA/cm2, appear to flow into the filopodia at their tips and back outward near the junctures of the filopodia and the growth cone. The currents appear to be produced only during active growth. Ion substitution experiments support the conclusion that the majority of this current is carried by Ca2+ ions, which we postulate flow through a population of activated voltage-sensitive Ca2+ channels located on the filopodial tips. Calculation of the transmembrane current density (4 X 10(-6) nA/cm2) leads to an estimate of channel density (10 channels/micron2) in close agreement with the measured density of Ca2+ channels in other systems. The assumption that calcium channel proteins are conveyed to nerve terminals by active transport, whereas sodium channel proteins are conveyed passively by a slower somatofugal diffusion process [Strichartz et al, 1984], would explain why developing neurons tend to display Ca2+-sensitive electrogenesis at their growing tips, and Na+-sensitive action potentials later in development. In order to gain some insight into the possible role of these steady growth currents, we estimated the membrane depolarization and axial voltage gradient they produce. It is likely that the currents produce sufficient membrane depolarization (approximately equal to 4 mV) to cause autogenous activation of ion channel permeabilities. Similarly, the axial voltage gradient (approximately equal to 4 mV/cm) would be expected to move intracytoplasmic vesicles by electrophoresis at a rate (20-40 microns/hr) very close to that at which the filopodia are observed to grow.(ABSTRACT TRUNCATED AT 400 WORDS)
许多研究表明,神经突生长的速率和方向由生长锥上黏附位点的分布所决定。最近有证据显示,施加外部电场可使膜分子重新分布,并改变神经突生长的速率和方向,这就引发了一个问题:生长锥中的稳定电流是否可能产生内源性电场。为了研究这个问题,我们设计了一种新型的圆形振动微探针,它能够测量5 nA/cm2范围内的电流密度(接近理论灵敏度极限),空间分辨率为2微米。本文描述了该装置的设计以及一种用于在线计算电流矢量的新算法的开发。使用这个探针,我们发现培养的金鱼视网膜神经节细胞生长锥在其尖端产生稳定的内向电流。测量到的电流在10 - 100 nA/cm2范围内,似乎在其尖端流入丝状伪足,并在丝状伪足与生长锥的交界处附近向外回流。这些电流似乎仅在活跃生长期间产生。离子替代实验支持了这样的结论:大部分这种电流由Ca2+离子携带,我们推测这些Ca2+离子流经位于丝状伪足尖端的一群激活的电压敏感Ca2+通道。跨膜电流密度(4×10(-6) nA/cm2)的计算得出通道密度(10个通道/微米2)的估计值,这与在其他系统中测量到的Ca2+通道密度非常一致。钙通道蛋白通过主动运输被输送到神经末梢,而钠通道蛋白通过较慢的向胞体扩散过程被动输送的假设[斯特里查兹等人,1984年],可以解释为什么发育中的神经元在其生长尖端倾向于表现出对Ca2+敏感的电发生,而在发育后期表现出对Na+敏感的动作电位。为了深入了解这些稳定生长电流的可能作用,我们估计了它们产生的膜去极化和轴向电压梯度。这些电流很可能产生足够的膜去极化(约等于4 mV),从而导致离子通道通透性的自身激活。同样,轴向电压梯度(约等于4 mV/cm)预计会以非常接近观察到的丝状伪足生长速率(20 - 40微米/小时)通过电泳移动胞浆内的囊泡。(摘要截断于400字)
