Sternini C, Anderson K
Center for Ulcer Research and Education/Digestive Disease Center, Department of Veterans Affairs VA Medical Center West Los Angeles, California 90073.
Somatosens Mot Res. 1992;9(1):45-59. doi: 10.3109/08990229209144762.
In the enteric nervous system, calcitonin gene-related peptide (CGRP) immunoreactivity is localized to a substantial number of capsaicin-sensitive afferent fibers and to intrinsic neurons and processes. CGRP immunoreactivity detected by immunohistochemistry represents the expression of two distinct genes, the calcitonin/alpha-CGRP and the beta-CGRP genes, which have different tissue distributions. In the present study, we used (1) in situ hybridization histochemistry and ribonucleic acid (RNA) blot hybridization with RNA probes complementary to the divergent sequences of alpha- and beta-CGRP messenger RNAs (mRNAs) to differentiate which CGRP gene was expressed in enteric and afferent neurons; and (2) axonal transport approaches in combination with CGRP immunohistochemistry to define the location of CGRP-containing afferent neurons supplying the digestive system. In situ hybridization histochemistry with [35S]-labeled RNA probes indicated that in the gastrointestinal tract beta-CGRP mRNA, but not alpha-CGRP mRNA, was expressed in enteric neurons confined to the myenteric and submucous plexuses of the small and large intestine. In dorsal root and vagal sensory ganglia, mRNAs for alpha-CGRP and beta-CGRP were both present in a vast population of neurons, with an overlapping pattern, even though the alpha-CGRP signal appeared more intense. RNA blot hybridization analysis showed a single band of hybridization at 1.2 Kb with the beta-CGRP RNA probe in RNA extracts from muscle layer-myenteric plexus and submucosal layer preparations of the ileum, and from dorsal root ganglia; it also showed a single band at 1.3 Kb with the alpha-CGRP RNA probe in extracts from dorsal root ganglia, but not from the intestine. These findings further support the differential expression of alpha- and beta-CGRP mRNAs. Retrograde transport of fast blue or fluorogold coupled with CGRP immunohistochemistry demonstrated that the vast majority of CGRP-containing afferent neurons supplying the stomach, proximal duodenum, and pancreas were located in dorsal root ganglia at the middle and lower thoracic and at the upper lumbar levels, and represented a major component of the afferent innervation of these viscera (up to 89%). Approximately 50% of CGRP-immunoreactive afferent neurons also expressed tachykinin (TK) immunoreactivity, as shown by triple labeling. Only a minor component of the afferent innervation of the stomach, duodenum, and pancreas derived from vagal CGRP-containing neurons (less than 8%). A large portion of these neurons (an average of 62%) also contained TK immunoreactivity.(ABSTRACT TRUNCATED AT 400 WORDS)
在肠神经系统中,降钙素基因相关肽(CGRP)免疫反应性定位于大量对辣椒素敏感的传入纤维以及内在神经元和突起。通过免疫组织化学检测到的CGRP免疫反应性代表了两个不同基因的表达,即降钙素/α-CGRP基因和β-CGRP基因,它们具有不同的组织分布。在本研究中,我们使用:(1)原位杂交组织化学和核糖核酸(RNA)印迹杂交,采用与α-和β-CGRP信使核糖核酸(mRNA)的不同序列互补的RNA探针,以区分在肠神经元和传入神经元中表达的是哪个CGRP基因;(2)轴突运输方法结合CGRP免疫组织化学,来确定供应消化系统的含CGRP传入神经元的位置。用[35S]标记的RNA探针进行原位杂交组织化学表明,在胃肠道中,β-CGRP mRNA而非α-CGRP mRNA在局限于小肠和大肠肌间神经丛和黏膜下神经丛的肠神经元中表达。在背根神经节和迷走神经感觉神经节中,α-CGRP和β-CGRP的mRNA在大量神经元中均有表达,呈重叠模式,尽管α-CGRP信号显得更强。RNA印迹杂交分析显示,在回肠的肌层-肌间神经丛和黏膜下层制剂以及背根神经节的RNA提取物中,β-CGRP RNA探针在1.2 Kb处出现单一条带的杂交信号;在背根神经节提取物中,α-CGRP RNA探针在1.3 Kb处出现单一条带,但在肠提取物中未出现。这些发现进一步支持了α-和β-CGRP mRNA的差异表达。快速蓝色染料或荧光金的逆行运输结合CGRP免疫组织化学表明,供应胃、十二指肠近端和胰腺的绝大多数含CGRP传入神经元位于胸段中下部和腰段上部的背根神经节,是这些内脏传入神经支配的主要组成部分(高达89%)。如三重标记所示,约50%的CGRP免疫反应性传入神经元也表达速激肽(TK)免疫反应性。胃、十二指肠和胰腺的传入神经支配中,只有一小部分来自含迷走神经CGRP的神经元(不到8%)。这些神经元中的很大一部分(平均62%)也含有TK免疫反应性。(摘要截于400字)
