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锤头状核酶的作用机制及其体内应用:利用新型杂交核酶文库在后基因组时代快速鉴定功能基因。

Mechanism of action of hammerhead ribozymes and their applications in vivo: rapid identification of functional genes in the post-genome era by novel hybrid ribozyme libraries.

作者信息

Takagi Y, Suyama E, Kawasaki H, Miyagishi M, Taira K

机构信息

Gene Function Research Laboratory, National Institute of Advanced Industrial Science and Technology (AIST), Central 4, 1-1-1 Higashi, Tsukuba Science City 305-8562, Japan.

出版信息

Biochem Soc Trans. 2002 Nov;30(Pt 6):1145-9. doi: 10.1042/bst0301145.

DOI:10.1042/bst0301145
PMID:12440992
Abstract

A hammerhead ribozyme was demonstrated to be a metalloenzyme. By controlling the metal-binding ability of the hammerhead ribozyme in the presence or absence of a specific sequence of interest, we engineered an allosterically controllable ribozyme, designated the maxizyme. Hybrid ribozymes were then constructed by coupling the site-specific cleavage activity of a hammerhead ribozyme with the unwinding activity of an endogenous RNA helicase. This leads to extremely efficient cleavage of target mRNA, not only in vitro, but also in vivo, and eliminates one of the major problems arising in the application of ribozymes for cleavage of mRNA in vivo : that many target sites on the RNA were previously inaccessible to cleavage owing to secondary and/or tertiary structure formation. Since hybrid ribozymes can efficiently attack target sites within mRNA, libraries were made of hybrid ribozymes with randomized binding arms, which were then introduced into cells. This procedure made it possible to readily identify the relevant genes associated with a specific phenotype, such as in apoptosis and cancer metastasis pathways. This application of a randomized library of hybrid ribozymes represents a simple, yet powerful, method for the identification of genes associated with specific phenotypes in the post-genome era. Moreover, vector-based siRNA (short-interfering RNA for RNA interference, RNAi) can also be used for the creation of the libraries and for the subsequent confirmation of the identified genes, relevant in the examined phenotype.

摘要

锤头状核酶被证明是一种金属酶。通过在存在或不存在特定目标序列的情况下控制锤头状核酶的金属结合能力,我们构建了一种变构可控核酶,命名为最大核酶。然后通过将锤头状核酶的位点特异性切割活性与内源性RNA解旋酶的解旋活性偶联,构建了杂交核酶。这不仅在体外,而且在体内都能导致对靶mRNA的极其高效的切割,并消除了核酶在体内切割mRNA应用中出现的一个主要问题:由于二级和/或三级结构的形成,RNA上的许多靶位点以前无法被切割。由于杂交核酶能够有效地攻击mRNA内的靶位点,因此构建了具有随机结合臂的杂交核酶文库,然后将其导入细胞。这一过程使得能够轻松识别与特定表型相关的相关基因,如在细胞凋亡和癌症转移途径中。杂交核酶随机文库的这种应用代表了一种简单但强大的方法,用于在后基因组时代识别与特定表型相关的基因。此外,基于载体的小干扰RNA(用于RNA干扰的短干扰RNA,RNAi)也可用于构建文库以及随后对在所研究表型中相关的已鉴定基因进行确认。

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