大鼠睾丸和角膜全贴装制剂中背根神经节神经元和相关“伤害感受器”细轴突的凝集素和神经肽标记。

J D Silverman, L Kruger
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引用次数: 209

摘要

作为探索各种外周区域中与痛觉受体相关的薄感觉轴突神经支配模式的计划的一部分,我们在大鼠睾丸膜血管和角膜的整个支架中标记了降钙素基因相关肽免疫反应(CGRP-IR)神经纤维。为了可视化具有重要数字意义的含氟酸性磷酸酶(FRAP)的轴突种群,研究人员进行了努力,由于目前可用的酸性磷酸酶方法的技术限制,这些轴突的末梢迄今仍无法证明。研究了与FRAP共定位于背根神经节(DRG)和脊髓的各种组织化学标记物,发现一种植物凝集素Griffonia simplicifolia I-B4不仅选择性地标记了脊髓的FRAP(+)感觉神经节细胞和中央终末,而且在睾丸和角膜全坐骨中对大量的细轴突进行了差异染色。细长的凝集素标记纤维在角膜中丰富,分布在与血管无关的血管膜中。相比之下,CGRP-IR轴突与血管模式保持紧密结合,外观上更粗糙和静脉曲张。因此,凝集素染色为外周FRAP(+)轴突的可视化提供了第一种实用和特定的方法,主要由感觉C纤维组成,但可能包括少量无髓鞘的自主轴突。现在,使用来自不同外周伤害感受器神经支配组织的单个整片制剂来检查肽能纤维和FRAP(+)纤维的分布应该是可行的,它们共同构成了绝大多数薄感觉轴突。这样就有可能将观察到的解剖模式与有关相应生理特征的感受野的特性的知识联系起来。
本文章由计算机程序翻译,如有差异,请以英文原文为准。
Lectin and neuropeptide labeling of separate populations of dorsal root ganglion neurons and associated "nociceptor" thin axons in rat testis and cornea whole-mount preparations.

As part of a program to explore patterns of innervation by nociceptor-related thin sensory axons in a variety of peripheral regions, we have labeled calcitonin gene-related peptide immunoreactive (CGRP-IR) nerve fibers in whole mounts of rat testicular tunica vasculosa and cornea. Efforts were undertaken to visualize the numerically significant fluoride-resistant acid phosphatase (FRAP)-containing axon population, whose peripheral endings have heretofore remained undemonstrable due to technical limitations of currently available acid phosphatase methods. Various histochemical markers that colocalize with FRAP in dorsal root ganglion (DRG) and spinal cord were examined, and a plant lectin, Griffonia simplicifolia I-B4, has been identified that not only selectively labels FRAP(+) sensory ganglion cells and central terminals in spinal cord, but also differentially stains a large number of thin axons in testicular and corneal whole mounts. Slender lectin-labeled fibers are abundant in cornea, and are distributed throughout tunica vasculosa preparations unrelated to blood vessels. CGRP-IR axons, in contrast, maintain close adherence to vascular patterns and are more coarse and varicose in appearance. Lectin staining therefore provides the first practical and specific method for visualization of peripheral FRAP(+) axons consisting principally of sensory C fibers but possibly including a small number of unmyelinated autonomic axons. It should now be feasible, using individual whole-mount preparations from various peripheral nociceptor-innervated tissues, to examine the distributions of both peptidergic and FRAP(+) fibers, which together comprise the vast majority of thin sensory axons. It may then be possible to correlate the observed anatomical patterns with knowledge regarding properties of corresponding physiologically characterized receptive fields.

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