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阐明一种无模板依赖性聚合酶中的序列-功能关系,以实现新的 DNA 记录应用。

Elucidating sequence-function relationships in a template-independent polymerase to enable novel DNA recording applications.

机构信息

Department of Chemical and Biological Engineering, Northwestern University, Evanston, Illinois, USA.

Center for Synthetic Biology, Northwestern University, Evanston, Illinois, USA.

出版信息

Biotechnol Bioeng. 2024 Dec;121(12):3808-3821. doi: 10.1002/bit.28838. Epub 2024 Sep 14.

DOI:10.1002/bit.28838
PMID:39275897
Abstract

Harnessing DNA as a high-density storage medium for information storage and molecular recording of signals has been of increasing interest in the biotechnology field. Recently, progress in enzymatic DNA synthesis, DNA digital data storage, and DNA-based molecular recording has been made by leveraging the activity of the template-independent DNA polymerase, terminal deoxynucleotidyl transferase (TdT). TdT adds deoxyribonucleotides to the 3' end of single-stranded DNA, generating random sequences of single-stranded DNA. TdT can use several divalent cations for its enzymatic activity and exhibits shifts in deoxyribonucleotide incorporation frequencies in response to changes in its reaction environment. However, there is limited understanding of sequence-structure-function relationships regarding these properties, which in turn limits our ability to modulate TdT to further advance TdT-based tools. Most TdT literature to-date explores the activity of murine, bovine or human TdTs; studies probing TdT sequence and structure largely focus on strictly conserved residues that are functionally critical to TdT activity. Here, we explore non-conserved TdT sequence space by surveying the natural diversity of TdT. We characterize a diverse set of TdT homologs from different organisms and identify several TdT residues/regions that confer differences in TdT behavior between homologs. The observations in this study can design rules for targeted TdT libraries, in tandem with a screening assay, to modulate TdT properties. Moreover, the data can be useful in guiding further studies of potential residues of interest. Overall, we characterize TdTs that have not been previously studied in the literature, and we provide new insights into TdT sequence-function relationships.

摘要

利用 DNA 作为高密度存储介质来存储信息,并对信号进行分子记录,这在生物技术领域引起了越来越多的兴趣。最近,通过利用无模板依赖性 DNA 聚合酶末端脱氧核苷酸转移酶(TdT)的活性,在酶促 DNA 合成、DNA 数字数据存储和基于 DNA 的分子记录方面取得了进展。TdT 将脱氧核糖核苷酸添加到单链 DNA 的 3' 端,生成单链 DNA 的随机序列。TdT 可以使用几种二价阳离子进行酶促反应,并表现出在其反应环境发生变化时,脱氧核糖核苷酸掺入频率的变化。然而,对于这些特性的序列-结构-功能关系,我们的理解有限,这反过来又限制了我们调节 TdT 的能力,以进一步推进基于 TdT 的工具。迄今为止,大多数 TdT 文献都探讨了鼠、牛或人 TdT 的活性;研究 TdT 序列和结构的研究主要集中在对 TdT 活性具有功能重要性的严格保守残基上。在这里,我们通过研究 TdT 的自然多样性来探索非保守的 TdT 序列空间。我们从不同的生物体中表征了一组多样化的 TdT 同源物,并确定了几个 TdT 残基/区域,这些残基/区域导致了同源物之间 TdT 行为的差异。本研究中的观察结果可以为靶向 TdT 文库设计规则,与筛选测定相结合,以调节 TdT 特性。此外,这些数据可以在指导对潜在感兴趣的残基的进一步研究中发挥作用。总的来说,我们对以前文献中未研究过的 TdT 进行了表征,并提供了关于 TdT 序列-功能关系的新见解。

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