大鼠和猫脊髓注射氚化氨基酸后背根神经节神经元的逆行标记。

P Barbaresi, A Rustioni, M Cuénod
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引用次数: 27

摘要

目前的实验是基于这样的证据,即神经元可以选择性地在其末端吸收并逆行运输它们用作神经递质或其类似物的相同化学物质。为了鉴定使用谷氨酸作为神经递质的背根神经节(DRG)神经元,我们选择[3H] d -天冬氨酸([3H]D-Asp)作为标记物,因为它是一种代谢惰性氨基酸,已知与l -天冬氨酸和l -谷氨酸具有相同的亲和力机制。成年大鼠和猫在颈节(C3 ~ C6)背角注射50 nl ~ 1.5微升[3H]D-Asp (500 microCi/微升)。注射后9 ~ 48小时,所有动物灌注5%戊二醛。切片处理后进行放射自显影,选取代表性病例中离注射部位最近的DRG神经元,计算切片平面上标记和未标记的有核仁的核周核的数量和截面积。在大鼠中,约4%的DRG神经元样本被放射自标记,这些神经元的平均核周面积约为未标记的核周面积的两倍。在猫中,标记的外核的百分比在抽样种群的6.5%到13.27%之间。标记神经元的平均核周面积与未标记神经元的核周面积之比在1.6 ~ 2.5之间。在C7注射[3H]脯氨酸的对照猫,C7 DRG的所有核周均被放射自显影标记。然而,注射[3H] γ -氨基丁酸([3H]GABA)观察到选择性逆行标记。在大鼠体内的定量数据显示,注射该氨基酸后,C6水平标记的核周虫约占C6 DRG样品总数的8%。标记核周与未标记核周的大小之比为2.02。在尾侧C3注射[3H]GABA的一只猫中,C4 DRG标记的核外体数量最多,占样本总数的5.32%。标记核周与未标记核周的大小之比为1.57。注射[3H]D-Asp的结果可能与部分DRG神经元使用谷氨酸和/或天冬氨酸作为神经递质的观点一致。(摘要删节为400字)
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Retrograde labeling of dorsal root ganglion neurons after injection of tritiated amino acids in the spinal cord of rats and cats.

The present experiments are based upon evidence that neurons may selectively take up at their terminals, and retrogradely transport, the same chemical they use as a neurotransmitter or its analogues. In an attempt to identify dorsal root ganglion (DRG) neurons that use glutamic acid as a neurotransmitter, [3H]D-aspartate ([3H]D-Asp) was chosen as a marker, since it is a metabolically inert amino acid known to be taken up by the same affinity mechanism as L-aspartate and L-glutamate. Adult rats and cats received injections of 50 nl to 1.5 microliter of [3H]D-Asp (500 microCi/microliter) in the dorsal horn of cervical segments (C3 to C6). At 9 to 48 hr after injection, all animals were perfused with 5% glutaraldehyde. After sections were processed for autoradiography, the DRG neurons situated most closely to the injection site were chosen from representative cases, and the number and cross-sectional area of labeled and unlabeled perikarya with a nucleolus in the plane of the section were calculated. In rats, about 4% of the sampled DRG neurons were autoradiographically labeled, and the mean perikaryal area of these neurons was about twice that of unlabeled perikarya. In cats, the percentage of labeled perikarya ranged between 6.5% and 13.27% of the sampled population. The ratio of the mean perikaryal area of labeled neurons to that of unlabeled neurons ranged between 1.6 and 2.5. In a control cat injected with [3H]proline at C7, all perikarya in the C7 DRG were autoradiographically labeled. However, with injection of [3H]gamma-aminobutyric acid ([3H]GABA) selective retrograde labeling was observed. Quantitative data in rat showed that perikarya labeled at the C6 level after injection of this amino acid constituted about 8% of the sample population in C6 DRG. The ratio of the size of labeled to unlabeled perikarya was 2.02. In one cat injected with [3H]GABA at caudal C3, the largest number of labeled perikarya were in C4 DRG and comprised up to 5.32% of the sampled population. The ratio of the size of labeled to unlabeled perikarya was 1.57. The results in cases of injection with [3H]D-Asp may be interpreted as consistent with the idea that a fraction of DRG neurons use glutamate and/or aspartate as neurotransmitter(s).(ABSTRACT TRUNCATED AT 400 WORDS)

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