FAST AXOPLASMIC TRANSPORT OF ACETYLCHOLINESTERASE IN MAMMALIAN NERVE FIBRES

Abstract— Acetylcholinesterase (acetylcholine acetyl-hydrolase, EC 3.1.1.7) is carried down mammalian nerve fibres by the fast axoplasmic transport system. This conclusion was derived from experiments involving the ligation of cat sciatic nerves at two sites placed 83.5 mm apart. The enzyme accumulated in segments of nerve proximal to the upper ligation in a linear fashion over a period of at least 20 h. At approximately 5 h the accumulation of enzyme ceased in the nerve segment proximal to the distal ligation within the isolated length of nerve, an observation indicating that the portion of AChE free to move within the isolated nerve had been depleted during this period of time. The freely moving fraction of AChE was estimated to be 15% of the total enzyme activity present in the nerve (10% in the proximo-distal direction and 5% in the retrograde direction). The rate of AChE downflow (as estimated from the intercept of the curve plotting accumulation with the line denoting when depletion started) was 431 mm/day within a 95% confidence interval of 357–543 mm/day. In view of the variability, our results demonstrated that AChE was being carried by the fast axoplasmic transport system, which in earlier studies was estimated to have a characteristic rate close to 410 mm/day.
An accumulation of AChE was also found on the distal side of the ligations that represented a movement of AChE in the distal-proximal direction in the fibres. This retrograde transport was smaller in amount (about one-half) than the proximo-distal rate of transport, or close to 220 mm/day. The rate of AChE transport was discussed in relation to the 'transport filament' hypothesis of fast axoplasmic transport.     

DEPENDENCE OF FAST AXOPLASMIC TRANSPORT IN NERVE ON OXIDATIVE METABOLISM

—A crest of labelled activity moving down the sciatic nerve at 401 ± 35 mm/day after injection of the L7 dorsal root ganglion of the cat with L-[³H]leucine characterizes fast axoplasmic transport of materials and has been studied with regard to its dependence on oxidative metabolism. Transport of labelled materials in vitro occurred if the nerve was supplied with O₂ or 95 % O₂+ 5 % CO₂. Transport was not dependent upon continuity of the fibres with the ganglionic soma. Asphyxiation (N₂) rapidly blocked fast transport in vitro. Likewise NaCN or dinitrophenol in an O₂ atmosphere both effectively block fast transport within 15 min. Tetrodotoxin and procaine, agents which block excitation of the membrane, had no effect on fast transport. The inference is that oxidative metabolism supplies the energy required by the molecular mechanism underlying fast axoplasmic transport.     

FAST AXOPLASMIC TRANSPORT OF A CALCIUM-BINDING PROTEIN IN MAMMALIAN NERVE

Abstract— Calcium is transported at a fast rate of 410 mm/day in cat sciatic nerve on injection of ⁴⁵Ca²⁺ into the L7 dorsal root ganglia. Nerve segments corresponding to the crest and the plateau regions of transported activity were analyzed by column chromatography on Sephadex G-100 and Biogel A 5m columns and the fast transported ⁴⁵Ca²⁺ found to be bound to a protein of 15,000 dalton. Using [³H]leucine as a precursor, a labeled calcium binding protein (CaBP) was found located at the same position in elution volumes from the columns as was the protein-bound ⁴⁵Ca^{2 +}. The level of [³H]-labeled CaBP in the crest and plateau regions were compared using column chromatography and polyacrylamide gel electrophoresis techniques and approx 3×4 times more [³H]-labeled activity was found in the crest as compared to the plateau. These findings indicate that Ca²⁺ is fast transported in association with the CaBP. The relation of CaBP to the transport filament model of axoplasmic transport and its possible role in nerve are discussed.     

MONOAMINES AS POSSIBLE MEDIATORS IN THE REGULATION OF FAST AXOPLASMIC FLOW

—The effect of drugs which have been shown to alter monoamines in the CNS on the rate of fast axoplasmic flow of [³H]leucine labelled material in the rat sciatic nerve was examined. Drugs which deplete monoamines led to a decrease while those which increase the level of monoamines led to an increase in the rate of fast axoplasmic flow. Monoaminergic drugs were also found to alter the amount of [³H]leucine incorporated into spinal cord.     

SLOW AXONAL TRANSPORT OF LABELLED PROTEINS IN SENSORY FIBRES OF RABBIT VAGUS NERVE

Both rapid (415 mm/day) and slow (24 mm/day) rates of axonal transport of proteins were found in sensory fibres of rabbit vagus nerve after injection of [³H]leucine into the nodose ganglion in vivo. The slow phase of transport was dependent on contact between the cell bodies and the nerve trunk, and did not continue under in vivro conditions. The results suggest some difference between the mechanisms of fast and slow transport.     

豚鼠眶外肌中快肌与慢肌纤维的小终板电流

豚鼠眶外肌中有两类不同电活动模式的肌纤维。一类纤维有动作电位,小终板电位时程较短并且较一致;另一类纤维不能产生动作电位,小终板电位时程较长而且多变。用电泳注射普胺天蓝分别标记这两类纤维各6条,并结合胆碱酯酶染色,结果表明,前一类肌纤维都是只有一个神经肌肉接头的快纤维;而另一类肌纤维都是有多个接头的慢纤维。根据双微电极电庄箱位实验结果,计算了上述决、慢肌纤维小终板电流下降相时间常数τ及其电压系数A。实验表明:(1)在静息电位附近,慢肌纤维小终板电流的τ值大于快肌纤维的;(2)慢肌纤维的A值比快肌纤维的小的多,即τ值较少随膜电位变化。本文对上述不同曾加以讨论。     

FAST AXOPLASMIC TRANSPORT IN MAMMALIAN NERVE IN VITRO AFTER BLOCK OF GLYCOLYSIS WITH IODOACETIC ACID

Abstract— Fast axoplasmic transport of components incorporating L-[³H]leucine in cat sciatic nerve occurred in vitro at a rate of 407 ± 21 (S.D.) mm/day. Although fast transport had earlier been shown to be blocked within 10 to 15 min by asphyxiation with nitrogen or by agents such as NaCN or dinitrophenol that interfere with oxidative phosphorylation, interruption of glycolysis by application of iodoacetate resulted in a gradually diminishing transport with a complete block in about 2 h. This block characteristically showed a sloping front instead of the usual crest of activity found in the nerve after the 3 h period usually allowed for in vitro downflow. The declining slope of radioactivity in the nerve seen after exposure to iodoacetate was not the result of a delayed entry of iodoacetate into the nerve fibres. We consider it to be the consequence of a limited and diminishing supply of endogenous metabolites entering the tricarboxylic acid cycle below the site of glycolytic block by iodoacetate. When either pyruvate or L-lactate was supplied to the iodoacetate-blocked nerve, recovery of the normal pattern and distance of flow was effected. Pyruvate partially reversed the iodoacetate block at concentrations as low as 2 mM, with almost complete recovery at approximately 25 mM. A concentration of L-lactate approx. 20 times that of pyruvate was required for a comparable degree of reversal of iodoacetate block.     

AXOPLASMIC TRANSPORT IN THE OPTIC NERVE AND TRACT OF THE RABBIT

The axonal transport of labelled proteins was studied in the optic system of adult rabbits after an intraocular injection of [³H]Ieucine. It was demonstrated that the precursor was incorporated into protein, which was transported along the axons of the retinal ganglion cells. Intraocularly injected puromycin inhibited protein synthesis in the retina and markedly inhibited the appearance of labelled protein in the optic nerve and tract. It was further demonstrated by intracisternal injection of [³H]leucine that an intraocular injection of puromycin did not affect the local protein synthesis in the optic nerve and tract. Cell fractionation studies of the optic nerve and tract showed that the rapidly migrating component, previously described as moving at an average rate of 110-150 mm/day, was largely associated with the microsomal fraction. About 40 per cent of the total protein-bound radioactivity in this component was found in the microsomal fraction and about 15 per cent was recovered in the soluble protein fraction. Most of the labelled material moving at a rate of 1-5-2 mm/day was soluble protein. The specific radioactivity of this component was about ten times greater than that of the fast one. In the slow component about 50 per cent of the radioactivity was found in the soluble protein fraction and about 10 per cent of the radioactivity was recovered in the microsomal fraction. Radioautography demonstrated incorporated label in the neuropil structures in the lateral geniculate body as early as 4-8 hr after intraocular injection. The labelling of the neuropil increased markedly during the first week, and could be observed after 3 weeks.     

FAST AND SLOW COMPONENTS IN AXONAL TRANSPORT OF PROTEIN

(a) After injection of labeled leucine into the eye of goldfish, radioactive protein rapidly accumulates in the contralateral optic tectum in the layer containing the synaptic endings of the optic fibers. This material reaches the tectum 6–12 hr after the isotope injection, a fact which indicates that the rate of transport is at least 40 mm per day. (b) This rapidly transported material has been shown to consist exclusively of protein, in which the label remains attached to leucine. (c) Inhibition of protein synthesis in the retina prevents the appearance of the transported protein in the tectum, but inhibition of protein synthesis in the tectum does not. Substances having some of the same properties as leucine, such as cycloleucine and norepinephrine, are not transported to the tectum. These experiments all indicate that the transported protein is synthesized in the retina. However, inhibition of retinal protein synthesis after this protein has been formed does not interfere with the transport mechanism itself. (d) The fast component consists of about 85% particulate material. It may be distinguished from a slowly moving component, transported at 0.4 mm per day, which contains about 5 times as much radioactivity as the fast component, and which consists of 60% particulate matter and 40% soluble protein.     

轴浆转运在神经再生中的作用

夹伤坐骨神经阻断标记蛋白在轴浆中的快、慢转运。3天后转运再现。第14天的转运距离与对照相似,说明再生神经的转运动能基本恢复。用快、慢转运测出的14天平均再生速度分别为1.77±0.14与1.96±0.07mm/d,比对照神经的正常生长速度快6.3—7倍,提示再生需要更多的转运物质。进一步发现再生神经中某些标记蛋白(慢转运波W1)的转运速度为10.25±0.66mm/d,约比对照快1倍,因此这些标记蛋白可能包含适应再生需要而加速转运的结构和功能物质。     

CONDUCTION IN NERVE FIBRES

Data by E. A. Blair and Erlanger on the voltage-capacity curves and the nerve impulse velocities of each of several fibres in the same nerve trunk are related to Rashevsky''s equation for the velocity of transmission in nerve. The results lend support to Rashevsky''s analysis. Other empirical relations between the velocity and the parameters of the excitation equations indicate the correctness of the hypothesis that the action current is the primary factor in transmission, which process is carried on by the electrical excitation of successive regions of the nerve fibre by means of its action current according to the ordinary laws of electrical excitation.     

SUBCELLULAR DISTRIBUTION AND TRANSPORT OF ACETYLCHOLINE IN CAT VENTRAL ROOTS AND SCIATIC NERVE

Abstract— The axonal transport of radioactive ACh, which was labelled by injecting radioactive choline into the ventral horn of the cat, was studied. Radioactivity analysed as ACh was transported in the nerves at a rate of 20–25 cm/24 h from the place of injection. Morphological and biochemical analysis after density gradient centrifugation revealed that endogenous ACh was principally distributed in three fractions-(a) a soluble fraction (provided homogenization was carried out in the presence of eserine), (b) a vesicular fraction (diameter 600–1600 A) in the 0.4M-sucrose layer of the density gradient, and (c) a fraction containing very small structures (size 90–100 A) in the 0.8–1.0 M-sucrose interphase. The radioactive ACh, however, was exclusively found in the soluble fraction (supernatant) after density gradient centrifugation. Analysis of ACh metabolites showed that radioactive ACh may have been formed locally in the nerves after transport of its precursor. Thus the morphologic and metabolic results do not support the hypothesis that ACh is transported in vesicles.     

神经元胞浆转运的两相流模型

提出神经元胞浆转运的两相流模型,对胞浆快转运和慢转运进行统一的流体力学描述,给出微粒转运与胞浆流动的定量关系。     

RAPID AXOPLASMIC TRANSPORT OF PROTEINS IN REGENERATING SENSORY NERVE FIBERS

Abstract— Utilizing an in vitro labeling procedure, the proteins carried by rapid axoplasmic transport in normal and regenerating sensory fibers of the rat sciatic nerve were compared. No statistically significant differences were found when the total amount of transported protein was compared in control and sectioned nerves at times from 2 to 76 days following axotomy. Fractionation of labeled proteins on polyacrylamide slab gels enabled the identification of some 25 individual transported proteins. By this criterion, no differences were detectable in the composition of proteins synthesized in the dorsal root ganglia from which sectioned vs control sciatic nerves project. When the electrophoretic distributions of transported proteins from control and sectioned nerves were compared, significant' differences were observed. The appearance and disappearance of two proteins were temporally related to chromatolytic changes in the nerve cell body. In addition, the composition of transported proteins in undamaged control nerves contralateral to the sectioned nerves exhibited changes which were not observed in either normal control nerves or sectioned nerves. Changes in the composition of transported proteins as a function of time following the onset of chromatolysis may be involved in controlling nerve regeneration in sensory nerve fibers.     

A RAPID METHOD FOR SELECTIVE SILVER STAINING OF NERVE FIBRES AND NERVE ENDINGS IN MOUNTED PARAFFIN SECTIONS

Abstract The staining described in this paper fundamentally is performed by two manipulations, namely (1) the treatment of deparaffinized sections for about fifteen minutes in a solution containing 15 per cent silver nitrate, 10 per cent potassium nitrate and 0.05 per cent glycine, and (2) the reduction for one minute in a solution of 1 per cent pyrogallol, 55 per cent ethyl alcohol and a trace (0.002 per cent) of nitric acid. After toning, dehydrating and mounting in the usual manner the sections generally are ready for examinations within less than an hour. The method is available for specimens fixed in the ordinary fixatives but those containing oxidizing metal compounds. The procedure is discussed from a theoretical point of view and some results are shown in photomicrographs.     

鸡的快肌在切碎移植并受到慢神经支配后的组织化学观察

使用出壳后3星期的鸡,把后背阔肌(快,α型纤维)切碎然后使之占据前背阔肌(慢-紧张,α’和β’型纤维)的空缺位置,并在前背阔肌神经的支配下生成新肌,新生肌肉象正常前背阔肌一样具有 ATP-ase 淡染的性质,但它也与前背阔肌不同,它具有酸不稳定性,而这后一性质却是碎肉源(后背阔肌)的性质。另外,把前背阔肌切碎然后把它放归原位,则由此新生的肌肉在上述两个方面都象正常的前背阔肌。以上实验证明在出生后3星期的鸡的横纹肌中的卫星细胞已带有向某种类型发育的倾向,以致于这些细胞经繁殖、融合后所产生的肌纤维仍带有肉源肌肉的某些性质。