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使用合成寡核苷酸探针在大鼠下丘脑进行加压素mRNA的原位杂交。

In situ hybridization of the vasopressin mRNA in the rat hypothalamus by use of a synthetic oligonucleotide probe.

作者信息

Nojiri H, Sato M, Urano A

出版信息

Neurosci Lett. 1985 Jul 4;58(1):101-5. doi: 10.1016/0304-3940(85)90336-2.

Abstract

A 22mer oligonucleotide complementary to the rat vasopressin (AVP) mRNA was synthesized, radioactively labeled with 32P, and was applied to in situ hybridization with the mRNA on paraffin sections of the rat hypothalamus. The AVP mRNA in magnocellular neurosecretory neurons of the paraventricular and the supraoptic nuclei was demonstrated by use of this synthetic probe. Specificity of the autoradiographic signals was confirmed by a competition test using an excess amount of unlabeled probe and an absorption test using a synthetic template of the probe. Further, the mRNA of vasotocin, the ancestral molecule of AVP, was hybridized weakly with the probe, showing that the present probe can discriminate a few base substitutions. Autoradiographic signals representing hybrids of the probe and the AVP mRNA were rarely found in the region rich in oxytocin neurons whose mRNA is homologous to the AVP mRNA. These results show that the in situ hybridization method using synthetic oligonucleotide probes can be a powerful and specific tool for the study of gene expression in the central nervous system.

摘要

合成了一段与大鼠血管加压素(AVP)mRNA互补的22聚体寡核苷酸,用32P进行放射性标记,并将其应用于大鼠下丘脑石蜡切片上与mRNA的原位杂交。使用该合成探针证实了室旁核和视上核的大细胞神经分泌神经元中的AVP mRNA。通过使用过量未标记探针的竞争试验和使用探针合成模板的吸收试验,证实了放射自显影信号的特异性。此外,AVP的原始分子血管紧张素的mRNA与该探针杂交较弱,表明本探针能够区分少数碱基取代。在富含与AVP mRNA同源的催产素神经元的区域中,很少发现代表探针与AVP mRNA杂交体的放射自显影信号。这些结果表明,使用合成寡核苷酸探针的原位杂交方法可以成为研究中枢神经系统基因表达的强大而特异的工具。

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