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大致密核心囊泡中前神经肽Y的加工:利用腺病毒对交感神经元中激素原转化酶表达的操控

Proneuropeptide Y processing in large dense-core vesicles: manipulation of prohormone convertase expression in sympathetic neurons using adenoviruses.

作者信息

Paquet L, Massie B, Mains R E

机构信息

Department of Neuroscience, Johns Hopkins University School of Medicine, Baltimore, Maryland 21205-2185, USA.

出版信息

J Neurosci. 1996 Feb 1;16(3):964-73. doi: 10.1523/JNEUROSCI.16-03-00964.1996.

Abstract

The efficient delivery of foreign genes into postmitotic cells is becoming very important for studies of nervous system functions. Cultured sympathetic neurons synthesize neuropeptide Y (NPY) in addition to catecholamines, providing an experimental model for studying neuronal peptide biosynthesis. In this work, we have studied the biosynthetic processing of NPY in primary cultures of rat superior cervical ganglion (SCG) neurons. NPY activation is complex, requiring sequential actions of a prohormone convertase (PC), carboxypeptidase H, and peptidylglycine alpha-amidating mono-oxygenase. Northern analyses established that SCG neurons in the animal contain mRNAs for both PC1 and PC2, and simultaneous immunocytochemistry for NPY and PC1 or PC2 established a 1:1 correspondence between NPY and PC2 expression in two thirds of the neurons that express NPY, both in the animal and in tissue culture. Biosynthetic studies on proneuropeptide Y (pro-NPY) processing to mature NPY established a close similarity to the rates seen in endocrine cells expressing PC2 and established clear differences between the patterns in SCG neurons and in endocrine cells expressing PC1. Recombinant adenoviruses were used to increase the level of PC1 in the cultured neurons from negligible to a level comparable with the level of PC1 in the anterior pituitary, and pro-NPY processing was markedly accelerated. When the viruses were used to lower the endogenous PC2 levels, using an antisense construct, pro-NPY processing was retarded. Taken together, these results support a major role for PC2 as the pro-NPY converting enzyme, and they establish the cultured SCG neurons as a model to study neuronal peptide biosynthesis.

摘要

将外源基因高效导入有丝分裂后细胞对于神经系统功能研究变得非常重要。培养的交感神经元除了合成儿茶酚胺外,还合成神经肽Y(NPY),为研究神经元肽生物合成提供了一个实验模型。在这项工作中,我们研究了大鼠颈上神经节(SCG)神经元原代培养物中NPY的生物合成加工过程。NPY的激活过程很复杂,需要前激素转化酶(PC)、羧肽酶H和肽基甘氨酸α-酰胺化单加氧酶的顺序作用。Northern分析表明,动物体内的SCG神经元含有PC1和PC2的mRNA,同时对NPY和PC1或PC2进行免疫细胞化学分析发现,在动物和组织培养中,三分之二表达NPY的神经元中,NPY和PC2的表达呈1:1对应关系。对前神经肽Y(pro-NPY)加工成成熟NPY的生物合成研究表明,其速率与表达PC2的内分泌细胞中的速率非常相似,并且SCG神经元和表达PC1的内分泌细胞中的加工模式存在明显差异。重组腺病毒被用于将培养神经元中PC1的水平从可忽略不计提高到与垂体前叶中PC1的水平相当,pro-NPY的加工明显加速。当使用病毒通过反义构建体降低内源性PC2水平时,pro-NPY的加工受到阻碍。综上所述,这些结果支持PC2作为pro-NPY转化酶的主要作用,并将培养的SCG神经元确立为研究神经元肽生物合成的模型。

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