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通过定向标签PCR消减技术分离大鼠纹状体特异性mRNA的克隆

Isolation of clones of rat striatum-specific mRNAs by directional tag PCR subtraction.

作者信息

Usui H, Falk J D, Dopazo A, de Lecea L, Erlander M G, Sutcliffe J G

机构信息

Department of Molecular Biology, Scripps Research Institute, La Jolla, California 92037.

出版信息

J Neurosci. 1994 Aug;14(8):4915-26. doi: 10.1523/JNEUROSCI.14-08-04915.1994.

DOI:10.1523/JNEUROSCI.14-08-04915.1994
PMID:8046460
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC6577190/
Abstract

We report an improved subtractive cDNA cloning procedure, named "directional tag PCR subtraction," for isolating clones of mRNAs enriched in a target tissue compared to a second tissue, the driver. In this method, the target and driver are prepared from directional cDNA libraries constructed in different vectors, and the target cDNA contains tag sequences at both its 5' and 3' ends for PCR amplification. This method avoids several limitations of previous subtraction procedures, and was demonstrated to be technically easy and efficient. Using the directional tag PCR subtraction and improved screening procedures, cDNA clones corresponding to mRNAs expressed in the striatum but not in the cerebellum of the rat brain were efficiently isolated, including mRNAs encoding calmodulin-dependent phosphodiesterase, a transcriptional regulatory protein, and several previously uncharacterized species. Our data suggest that approximately 1% of the striatal polyA+ RNA mass potentially encoding more than 300 distinct proteins corresponds to RNA species reduced in concentration or absent from the cerebellum, of which about one-third are expressed prominently only in the striatum. This unexpected finding suggests that the striatum has a unique biochemical character within the brain, and that characterization of these mRNAs will be important for understanding the biochemical basis of striatal function.

摘要

我们报道了一种改进的消减cDNA克隆方法,名为“定向标签PCR消减”,用于分离与第二种组织(驱动组织)相比在目标组织中富集的mRNA克隆。在该方法中,目标组织和驱动组织由构建于不同载体的定向cDNA文库制备而来,并且目标cDNA在其5'和3'末端均含有用于PCR扩增的标签序列。该方法避免了先前消减程序的几个局限性,并且被证明在技术上简便且高效。使用定向标签PCR消减和改进的筛选程序,高效分离出了对应于在大鼠脑纹状体中表达但在小脑不表达的mRNA的cDNA克隆,包括编码钙调蛋白依赖性磷酸二酯酶、一种转录调节蛋白以及几个先前未鉴定的mRNA的克隆。我们的数据表明,潜在编码超过300种不同蛋白质的纹状体多聚腺苷酸加尾RNA群体中约1%对应于在小脑中浓度降低或不存在的RNA种类,其中约三分之一仅在纹状体中显著表达。这一意外发现表明纹状体在脑内具有独特的生化特征,并且对这些mRNA的表征对于理解纹状体功能的生化基础将具有重要意义。

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