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首页> 外文期刊>Nucleic acids research >Gene2Oligo: oligonucleotide design for in vitro gene synthesis
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Gene2Oligo: oligonucleotide design for in vitro gene synthesis

机译:Gene2Oligo:用于体外基因合成的寡核苷酸设计

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There is substantial interest in implementing a bioinformatics tool that allows the design of oligonucleotides to support the development of in vitro gene synthesis. Current protocols to make long synthetic DNA molecules rely on the in vitro assembly of a set of short oligonucleotides, either by ligase chain reaction (LCR) or by assembly PCR. Ideally, such oligonucleotides should represent both strands of the final DNA molecule. They should be adjacent on the same strand and overlap the complementary oligonucleotides from the second strand to ensure good hybridization during assembly. This implies that the thermodynamic properties of each oligonucleotide have to be consistent across the set. Furthermore, any given oligonucleotide has to be totally specific to its target to avoid the creation of incorrectly assembled sequences. We have developed Gene2Oligo (http://berry.engin.umich.edu/gene2oligo/), a web-based tool that divides a long input DNA sequence into a set of adjacent oligonucleotides representing both DNA strands. The length of the oligonucleotides is dynamically optimized to ensure both the specificity and the uniform melting temperatures necessary for in vitro gene synthesis. We have successfully designed and used a set of oligonucleotides to synthesize the Saccharomyces cerevisiae cytochrome b5 by using both LCR and assembly PCR.
机译:人们对实现一种生物信息学工具非常感兴趣,该工具允许设计寡核苷酸以支持体外基因合成的发展。制备长的合成DNA分子的当前方案依赖于通过连接酶链反应(LCR)或通过组装PCR的一组短寡核苷酸的体外组装。理想地,此类寡核苷酸应代表最终DNA分子的两条链。它们应在同一条链上相邻,并与第二条链上的互补寡核苷酸重叠,以确保组装过程中的良好杂交。这意味着每个寡核苷酸的热力学性质必须在整个组中保持一致。此外,任何给定的寡核苷酸都必须对其靶标完全特异,以避免产生错误组装的序列。我们已经开发了Gene2Oligo(http://berry.engin.umich.edu/gene2oligo/),这是一种基于网络的工具,可将长输入DNA序列分成代表两条DNA链的一组相邻寡核苷酸。动态优化寡核苷酸的长度,以确保体外基因合成所需的特异性和均匀的解链温度。我们已经成功设计并使用了一组寡核苷酸,通过使用LCR和组装PCR来合成酿酒酵母细胞色素b5。

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