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用于持续超特异性杂交的模拟引导DNA探针设计

Simulation-guided DNA probe design for consistently ultraspecific hybridization.

作者信息

Wang Juexiao Sherry, Zhang David Yu

机构信息

1] Systems, Synthetic, and Physical Biology, Rice University, Houston, Texas 77030, USA [2] Department of Bioengineering, Rice University, Houston, Texas 77030, USA.

出版信息

Nat Chem. 2015 Jul;7(7):545-53. doi: 10.1038/nchem.2266. Epub 2015 May 25.

Abstract

Hybridization of complementary sequences is one of the central tenets of nucleic acid chemistry; however, the unintended binding of closely related sequences limits the accuracy of hybridization-based approaches to analysing nucleic acids. Thermodynamics-guided probe design and empirical optimization of the reaction conditions have been used to enable the discrimination of single-nucleotide variants, but typically these approaches provide only an approximately 25-fold difference in binding affinity. Here we show that simulations of the binding kinetics are both necessary and sufficient to design nucleic acid probe systems with consistently high specificity as they enable the discovery of an optimal combination of thermodynamic parameters. Simulation-guided probe systems designed against 44 sequences of different target single-nucleotide variants showed between a 200- and 3,000-fold (median 890) higher binding affinity than their corresponding wild-type sequences. As a demonstration of the usefulness of this simulation-guided design approach, we developed probes that, in combination with PCR amplification, detect low concentrations of variant alleles (1%) in human genomic DNA.

摘要

互补序列的杂交是核酸化学的核心原则之一;然而,密切相关序列的意外结合限制了基于杂交的核酸分析方法的准确性。热力学指导的探针设计和反应条件的经验优化已被用于区分单核苷酸变体,但通常这些方法仅提供约25倍的结合亲和力差异。在这里,我们表明结合动力学模拟对于设计具有始终如一的高特异性的核酸探针系统既是必要的也是充分的,因为它们能够发现热力学参数的最佳组合。针对44个不同目标单核苷酸变体序列设计的模拟指导探针系统显示,其结合亲和力比相应的野生型序列高200至3000倍(中位数为890倍)。作为这种模拟指导设计方法实用性的证明,我们开发了与PCR扩增相结合可检测人类基因组DNA中低浓度变体等位基因(1%)的探针。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/073f/4479422/72c4ac4f3f5b/nihms683310f1.jpg

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