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Ultra-high-speed DNA fragment separations using microfabricated capillary array electrophoresis chips.

机译:使用微型毛细管阵列电泳芯片进行超高速DNA片段分离。

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摘要

Capillary electrophoresis arrays have been fabricated on planar glass substrates by photolithographic masking and chemical etching techniques. The photolithographically defined channel patterns were etched in a glass substrate, and then capillaries were formed by thermally bonding the etched substrate to a second glass slide. High-resolution electrophoretic separations of phi X174 Hae III DNA restriction fragments have been performed with these chips using a hydroxyethyl cellulose sieving matrix in the channels. DNA fragments were fluorescently labeled with dye in the running buffer and detected with a laser-excited, confocal fluorescence system. The effects of variations in the electric field, procedures for injection, and sizes of separation and injection channels (ranging from 30 to 120 microns) have been explored. By use of channels with an effective length of only 3.5 cm, separations of phi X174 Hae II DNA fragments from approximately 70 to 1000 bp are complete in only 120 sec. We have also demonstrated high-speed sizing of PCR-amplified HLA-DQ alpha alleles. This work establishes methods for high-speed, high-throughput DNA separations on capillary array electrophoresis chips.
机译:已经通过光刻掩模和化学蚀刻技术在平面玻璃基板上制造了毛细管电泳阵列。在玻璃基板上蚀刻光刻定义的通道图案,然后通过将蚀刻的基板热粘合到第二玻璃载片上形成毛细管。使用这些芯片,在通道中使用羟乙基纤维素筛分基质,可以对phi X174 Hae III DNA限制性片段进行高分辨率电泳分离。 DNA片段在运行缓冲液中用染料进行荧光标记,并用激光激发的共聚焦荧光系统检测。已经研究了电场,注射程序以及分离和注射通道的尺寸(范围从30到120微米)变化的影响。通过使用有效长度仅为3.5 cm的通道,仅在120秒内即可完成大约70 bp至1000 bp的phi X174 Hae II DNA片段的分离。我们还证明了PCR扩增的HLA-DQα等位基因的高速大小。这项工作建立了在毛细管阵列电泳芯片上进行高速,高通量DNA分离的方法。

著录项

  • 作者

    Woolley, A T; Mathies, R A;

  • 作者单位
  • 年度 1994
  • 总页数
  • 原文格式 PDF
  • 正文语种 en
  • 中图分类

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