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基于序列的毛细管电泳中单链 DNA 的核苷酸分离:重点是磷酸。

Sequence-based separation of single-stranded DNA using nucleotides in capillary electrophoresis: focus on phosphate.

机构信息

Department of Chemistry and Chemical Biology, 321 Cogswell Laboratory, Rensselaer Polytechnic Institute, Troy, NY 12180, USA.

出版信息

Electrophoresis. 2013 Jun;34(12):1778-86. doi: 10.1002/elps.201200683.

Abstract

DNA analysis has widespread applicability in biology, medicine, biotechnology, and forensics. DNA separation by length is readily achieved using sieving gels in electrophoresis. Separation by sequence is less simple, generally requiring adequate differences in native or induced conformation or differences in thermal or chemical stability of the strands that are hybridized prior to measurement. We previously demonstrated separation of four single-stranded DNA 76-mers that differ by only a few A-G substitutions based solely on sequence using guanosine-5'-monophosphate (GMP) in the running buffer. We attributed separation to the unique self-assembly of GMP to form higher order structures. Here, we examine an expanded set of 76-mers designed to probe the mechanism of the separation and effects of experimental conditions. We were surprised to find that other ribonucleotides achieved the similar separation to GMP, and that some separation was achieved using sodium phosphate instead of GMP. Potassium phosphate achieved almost as good separations as the ribonucleotides. This suggests that the separation medium provides a physicochemical environment for the DNA that effects strand migration in a sequence-selective manner. Further investigation is needed to determine whether the mechanism involves specific interactions between the phosphates and the DNA strands or is a result of other properties of the separation medium. Phosphate generally has been avoided in DNA separations by capillary gel electrophoresis because its high ionic strength exacerbates Joule heating. Our results suggest that phosphate compounds should be examined for separation of DNA based on sequence.

摘要

DNA 分析在生物学、医学、生物技术和法医学中具有广泛的应用。在电泳中,通过筛分凝胶可以轻松实现 DNA 按长度分离。按序列分离则不那么简单,通常需要天然或诱导构象的充分差异,或者在测量之前杂交的链的热或化学稳定性的差异。我们之前证明,仅基于序列,使用运行缓冲液中的鸟苷-5'-单磷酸 (GMP) 就可以分离出仅相差几个 A-G 取代的四个单链 DNA 76 -mer。我们将分离归因于 GMP 独特的自组装形成高级结构。在这里,我们研究了一组扩展的 76-mer,旨在探索分离的机制和实验条件的影响。我们惊讶地发现,其他核苷酸也能像 GMP 一样实现类似的分离,并且使用磷酸钠而不是 GMP 也能实现一些分离。磷酸钾的分离效果几乎与核苷酸一样好。这表明分离介质为 DNA 提供了一种理化环境,以序列选择性的方式影响链迁移。需要进一步研究以确定分离机制是否涉及磷酸根与 DNA 链之间的特定相互作用,还是分离介质的其他特性的结果。由于磷酸盐的高离子强度会加剧焦耳加热,因此在毛细管凝胶电泳中通常避免使用磷酸盐进行 DNA 分离。我们的结果表明,应该根据序列检查磷酸盐化合物是否可用于 DNA 分离。

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