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人死后大脑中信使核糖核酸的稳定性及人脑互补脱氧核糖核酸文库的构建

Stability of messenger RNA in postmortem human brains and construction of human brain cDNA libraries.

作者信息

Kobayashi H, Sakimura K, Kuwano R, Sato S, Ikuta F, Takahashi Y, Miyatake T, Tsuji S

机构信息

Department of Neurology, Niigata University, Japan.

出版信息

J Mol Neurosci. 1990;2(1):29-34. doi: 10.1007/BF02896923.

Abstract

We studied stabilities of poly(A)(+)-RNA in postmortem mouse and human brains for up to 12 hours. The yields of total RNA were not changed significantly during postmortem periods either in mouse brains or human brains. Cell-specific cDNA probes were used to evaluate postmortem stability of poly(A)(+)-RNA in each cell type in the central nervous system. We used neuron-specific enolase (NSE), S-100 beta (S-100), and myelin-associated glycoprotein (MAG) for molecular markers of neuron, astrocyte, and oligodendrocyte, respectively. There was no detectable degradation of mRNAs coding for NSE, S-100, and MAG during the postmortem periods on Northern blot hybridization analyses. These results indicate that intact mRNAs expressed in neuron, astrocyte, or oligodendrocyte can be isolated from postmortem brains for up to 12 hours after death. Using poly(A)(+)-RNA thus isolated from two postmortem human brains, we constructed directional cDNA libraries and demonstrated the presence of full-length cDNAs for NSE, S-100, and MAG on Southern blot hybridization analysis. The present data should encourage studies on altered gene expressions in human brain in various neurologic diseases.

摘要

我们研究了死后小鼠和人类大脑中聚腺苷酸(+)-RNA长达12小时的稳定性。在死后期间,无论是小鼠大脑还是人类大脑,总RNA的产量均无显著变化。使用细胞特异性cDNA探针评估中枢神经系统中每种细胞类型的聚腺苷酸(+)-RNA的死后稳定性。我们分别使用神经元特异性烯醇化酶(NSE)、S-100β(S-100)和髓鞘相关糖蛋白(MAG)作为神经元、星形胶质细胞和少突胶质细胞的分子标志物。在Northern印迹杂交分析中,在死后期间未检测到编码NSE、S-100和MAG的mRNA有降解。这些结果表明,在死后长达12小时内,可以从死后大脑中分离出在神经元、星形胶质细胞或少突胶质细胞中表达的完整mRNA。使用从两个死后人类大脑中分离得到的聚腺苷酸(+)-RNA,我们构建了定向cDNA文库,并在Southern印迹杂交分析中证明了存在NSE、S-100和MAG的全长cDNA。目前的数据应会促进对各种神经系统疾病中人类大脑基因表达改变的研究。

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