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刚性、共轭、荧光标记的三磷酸胸苷:合成及聚合酶介导掺入DNA类似物

Rigid, conjugated, fluoresceinated thymidine triphosphates: syntheses and polymerase mediated incorporation into DNA analogues.

作者信息

Thoresen Lars H, Jiao Guan-Sheng, Haaland Wade C, Metzker Michael L, Burgess Kevin

机构信息

Texas A & M University, Chemistry Department, P. O. Box 30012, College Station, TX 77842, USA.

出版信息

Chemistry. 2003 Oct 6;9(19):4603-10. doi: 10.1002/chem.200304944.

DOI:10.1002/chem.200304944
PMID:14566865
Abstract

Syntheses of a unique set of energy transfer dye labeled nucleoside triphosphates, compounds 1-3, are described. Attempts to prepare these compounds were only successful if the triphosphorylation reaction was performed before coupling the dye to the nucleobase, and not the other way around. Compounds were prepared as both the 2'-deoxy (a) and 2',3'-dideoxy- (b) forms. They feature progressively longer rigid conjugated linkers connecting the nucleobase and the hydroxyxanthone moiety. UV spectra of the parent nucleosides 12-14 show that as the length of the linker increases so does the absorption of the donor in the 320-330 nm region, but with relatively little red-shift of the maxima. Fluorescence spectra of the same compounds show that radiation in the 320-330 nm region results in predominant emission from the fluorescein. When the linker is irradiated at 320 nm, the only significant emission observed corresponds to the hydroxyxanthone part of the molecules at 520 nm; this corresponds to an effective Stokes' shift of 200 nm. As the absorption at 320-330 nm by the linker increases with length, so does the intensity of the fluorescein emission. A gel assay was used to gauge relative incorporation efficiencies of compounds 1-3, dTTP, ddTTP, and 6-TAMRA-ddTTP. Throughout, the thermostable polymerase TaqFS was used, as it is the one most widely applied in high throughput DNA sequencing. This assay showed that only compounds 3 were incorporated efficiently; these have the longest linkers. Of these, the 2'-deoxy nucleoside 3 a was incorporated and did not prevent the polymerase from extending the chain further. The 2',3'-dideoxy nucleoside 3 b was incorporated only about 430 times less efficiently than ddTTP under the same conditions, and caused chain termination. The implications of these studies on modified sequencing protocols are discussed.

摘要

本文描述了一组独特的能量转移染料标记的三磷酸核苷(化合物1 - 3)的合成方法。只有在将染料与核碱基偶联之前进行三磷酸化反应,而不是反过来,制备这些化合物的尝试才会成功。化合物制备成了2'-脱氧(a)和2',3'-二脱氧(b)两种形式。它们的特点是连接核碱基和羟基氧杂蒽部分的刚性共轭连接子逐渐变长。母体核苷12 - 14的紫外光谱表明,随着连接子长度的增加,供体在320 - 330 nm区域的吸收也增加,但最大值的红移相对较小。相同化合物的荧光光谱表明,在320 - 330 nm区域的辐射导致主要是荧光素的发射。当连接子在320 nm处照射时,观察到的唯一显著发射对应于分子在520 nm处的羟基氧杂蒽部分;这对应于200 nm的有效斯托克斯位移。随着连接子在320 - 330 nm处的吸收随长度增加,荧光素发射的强度也增加。使用凝胶分析来评估化合物1 - 3、dTTP、ddTTP和6 - TAMRA - ddTTP的相对掺入效率。在整个过程中,使用了热稳定聚合酶TaqFS,因为它是在高通量DNA测序中应用最广泛的一种。该分析表明只有化合物3被有效掺入;这些化合物具有最长的连接子。其中,2'-脱氧核苷3 a被掺入且没有阻止聚合酶进一步延伸链。在相同条件下,2',3'-二脱氧核苷3 b的掺入效率仅比ddTTP低约430倍,并导致链终止。讨论了这些研究对改进测序方案的意义。

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