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体内组装多基因途径文库的重复重组。

Reiterative Recombination for the in vivo assembly of libraries of multigene pathways.

机构信息

Department of Chemistry, Columbia University, 550 West 120th Street, MC 4854, New York, NY 10027, USA.

出版信息

Proc Natl Acad Sci U S A. 2011 Sep 13;108(37):15135-40. doi: 10.1073/pnas.1100507108. Epub 2011 Aug 26.

Abstract

The increasing sophistication of synthetic biology is creating a demand for robust, broadly accessible methodology for constructing multigene pathways inside of the cell. Due to the difficulty of rationally designing pathways that function as desired in vivo, there is a further need to assemble libraries of pathways in parallel, in order to facilitate the combinatorial optimization of performance. While some in vitro DNA assembly methods can theoretically make libraries of pathways, these techniques are resource intensive and inherently require additional techniques to move the DNA back into cells. All previously reported in vivo assembly techniques have been low yielding, generating only tens to hundreds of constructs at a time. Here, we develop "Reiterative Recombination," a robust method for building multigene pathways directly in the yeast chromosome. Due to its use of endonuclease-induced homologous recombination in conjunction with recyclable markers, Reiterative Recombination provides a highly efficient, technically simple strategy for sequentially assembling an indefinite number of DNA constructs at a defined locus. In this work, we describe the design and construction of the first Reiterative Recombination system in Saccharomyces cerevisiae, and we show that it can be used to assemble multigene constructs. We further demonstrate that Reiterative Recombination can construct large mock libraries of at least 10(4) biosynthetic pathways. We anticipate that our system's simplicity and high efficiency will make it a broadly accessible technology for pathway construction and render it a valuable tool for optimizing pathways in vivo.

摘要

合成生物学的日益复杂,对在细胞内构建多基因途径的强大、广泛可及的方法提出了需求。由于在体内理性设计按预期功能运行的途径具有挑战性,因此还需要并行组装途径文库,以促进性能的组合优化。虽然一些体外 DNA 组装方法理论上可以构建途径文库,但这些技术资源密集,并且固有地需要其他技术将 DNA 转移回细胞。以前报道的所有体内组装技术产量都很低,一次只能生成数十到数百个构建体。在这里,我们开发了“重复重组”,这是一种在酵母染色体中直接构建多基因途径的强大方法。由于其使用内切核酸酶诱导的同源重组与可回收标记相结合,重复重组为在定义的基因座处顺序组装数量不定的 DNA 构建体提供了一种高效、技术简单的策略。在这项工作中,我们描述了第一个在酿酒酵母中重复重组系统的设计和构建,并展示了它可用于组装多基因构建体。我们进一步证明重复重组可以构建至少 10(4)个生物合成途径的大型模拟文库。我们预计,我们的系统的简单性和高效率将使其成为一种广泛可及的途径构建技术,并使其成为优化体内途径的有价值的工具。

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