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用于微通道DNA测序的稀疏交联“纳米凝胶”

Sparsely cross-linked "nanogels" for microchannel DNA sequencing.

作者信息

Doherty Erin A S, Kan Cheuk Wai, Barron Annelise E

机构信息

Department of Chemical Engineering, Northwestern University, Evanston, IL 60208, USA.

出版信息

Electrophoresis. 2003 Dec;24(24):4170-80. doi: 10.1002/elps.200305702.

Abstract

We have developed sparsely cross-linked "nanogels", sub-colloidal polymer structures composed of covalently linked, linear polyacrylamide chains, as novel DNA sequencing matrices for capillary electrophoresis. The presence of covalent cross-links affords nanogel matrices with enhanced network stability relative to standard, linear polyacrylamide (LPA), improving the separation of large DNA fragments. Nanogels were synthesized via inverse emulsion (water-in-oil) copolymerization of acrylamide and N,N-methylenebisacrylamide (Bis). In order to retain the fluidity necessary in a replaceable polymer matrix for capillary array electrophoresis (CAE), a low percentage of the Bis cross-linker (< 10(-4) mol%) was used. Nanogels were characterized by multiangle laser light scattering and rheometry, and were tested for DNA sequencing by CAE with four-color laser-induced fluorescence (LIF) detection. The properties and performance of nanogel matrices were compared to those of a commercially available LPA network, which was matched for both weight-average molar mass (Mw) and extent of interchain entanglements (c/c*). Nanogels presented in this work have an average radius of gyration of 226 nm and a weight-average molar mass of 8.8 x 10(6) g/mol. At concentrations above the overlap threshold, nanogels form a clear, viscous solution, similar to the LPA matrix (Mw approximately 8.9 x 10(6) g/mol). The two matrices have similar flow and viscosity characteristics. However, because of the physical network stability provided by the internally cross-linked structure of the nanogels, a substantially longer read length ( approximately 63 bases, a 10.4% improvement) is obtained with the nanogel matrix at 98.5% accuracy of base-calling. The nanogel network provides higher-selectivity separation of ssDNA sequencing fragments longer than 375 bases. Moreover, nanogel matrices require 30% less polymer per unit volume than LPA. This is the first report of a sequencing matrix that provides better performance than LPA, in a side-by-side comparison of polymer matrices matched for Mw and extent of interchain entanglements.

摘要

我们已经开发出了稀疏交联的“纳米凝胶”,它是由共价连接的线性聚丙烯酰胺链组成的亚胶体聚合物结构,作为用于毛细管电泳的新型DNA测序基质。与标准的线性聚丙烯酰胺(LPA)相比,共价交联的存在使纳米凝胶基质具有更高的网络稳定性,从而改善了大DNA片段的分离效果。纳米凝胶是通过丙烯酰胺和N,N-亚甲基双丙烯酰胺(双丙烯酰胺)的反相乳液(油包水)共聚反应合成的。为了在用于毛细管阵列电泳(CAE)的可替换聚合物基质中保持必要的流动性,使用了低百分比的双丙烯酰胺交联剂(<10^(-4) mol%)。通过多角度激光光散射和流变学对纳米凝胶进行了表征,并通过CAE结合四色激光诱导荧光(LIF)检测对其进行了DNA测序测试。将纳米凝胶基质的性质和性能与市售的LPA网络进行了比较,该LPA网络在重均摩尔质量(Mw)和链间缠结程度(c/c*)方面均匹配。本文介绍的纳米凝胶的平均回转半径为226 nm,重均摩尔质量为8.8×10^6 g/mol。在高于重叠阈值的浓度下,纳米凝胶形成澄清、粘稠的溶液,类似于LPA基质(Mw约为8.9×10^6 g/mol)。这两种基质具有相似的流动和粘度特性。然而,由于纳米凝胶内部交联结构提供的物理网络稳定性,在碱基识别准确率为98.5%的情况下,纳米凝胶基质可获得显著更长的读取长度(约63个碱基,提高了10.4%)。纳米凝胶网络对长度超过375个碱基的单链DNA测序片段提供了更高选择性的分离。此外,纳米凝胶基质每单位体积所需的聚合物比LPA少30%。这是在对Mw和链间缠结程度相匹配的聚合物基质进行并排比较时,首次报道的一种性能优于LPA的测序基质。

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