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基于热力学的 DNA 嵌段共聚物理性设计用于通过亲和毛细管电泳定量检测单核苷酸多态性。

Thermodynamics-based rational design of DNA block copolymers for quantitative detection of single-nucleotide polymorphisms by affinity capillary electrophoresis.

机构信息

Bioengineering Laboratory, RIKEN , 2-1 Hirosawa, Wako, Saitama 351-0198, Japan.

出版信息

Anal Chem. 2014 Nov 18;86(22):11425-33. doi: 10.1021/ac503522f. Epub 2014 Nov 6.

DOI:10.1021/ac503522f
PMID:25358129
Abstract

Diblock copolymers composed of allele-specific oligodeoxyribonucleotide (ODN) and poly(ethylene glycol) (PEG) are used as an affinity probe of free-solution capillary electrophoresis to quantitatively detect single-base substitutions in genetic samples. During electrophoresis, the probe binds strongly to a wild-type single-stranded DNA analyte (WT) through hybridization, while it binds weakly to its single-base-mutated DNA analyte (MT) due to a mismatch. Complex formation with the probe augments the hydrodynamic friction of either analyte, thereby retarding its migration. The difference in affinity strength leads to separation of the WT, MT, and contaminants, including the PCR primers used for sample preparation. The optimal sequence of the probe's ODN segment is rationally determined in such a way that the binding constant between the ODN segment and MT at the capillary temperature is on the order of 10(6) M(-1). The validity of this guideline is verified using various chemically synthesized DNA analytes, as well as those derived from a bacterial genome. The peak area ratio of MT agrees well with its feed ratio, suggesting the prospective use of the present method in SNP allele frequency estimation.

摘要

由等位特异性寡脱氧核苷酸 (ODN) 和聚乙二醇 (PEG) 组成的两亲嵌段共聚物被用作自由溶液毛细管电泳的亲和探针,用于定量检测遗传样品中的单碱基替换。在电泳过程中,探针通过杂交与野生型单链 DNA 分析物 (WT) 强烈结合,而由于碱基错配,与单碱基突变的 DNA 分析物 (MT) 的结合较弱。与探针形成复合物会增加任一个分析物的流体动力摩擦,从而减缓其迁移。亲和力强度的差异导致 WT、MT 和污染物(包括用于样品制备的 PCR 引物)的分离。以这样的方式合理确定探针的 ODN 片段的最佳序列,即 ODN 片段与毛细管温度下的 MT 之间的结合常数约为 10(6) M(-1)。使用各种化学合成的 DNA 分析物以及源自细菌基因组的分析物验证了这一准则的有效性。MT 的峰面积比与其进料比吻合较好,表明该方法有望用于 SNP 等位基因频率估计。

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