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微粒上的DNA杂交:确定捕获探针密度和平衡解离常数。

DNA hybridization on microparticles: determining capture-probe density and equilibrium dissociation constants.

作者信息

Wilkins Stevens P, Henry M R, Kelso D M

机构信息

Department of Biomedical Engineering, Robert R. McCormick School of Engineering and Applied Science, Northwestern University, 2145 Sheridan Road, Evanston, IL 60208, USA.

出版信息

Nucleic Acids Res. 1999 Apr 1;27(7):1719-27. doi: 10.1093/nar/27.7.1719.

DOI:10.1093/nar/27.7.1719
PMID:10076004
原文链接:https://pmc.ncbi.nlm.nih.gov/articles/PMC148376/
Abstract

Many DNA-probe assays utilize oligonucleotide-coated microparticles for capture of complementary nucleic acids from solution. During development of these assays, as well as in other particle-based nucleic acid applications, it is useful to know both the amount of duplex formation expected under various experimental conditions and the coating density of the capture oligonucleotide on the particle surface. We examined the simplest form of a DNA-probe microparticle assay: hybridization of a particle-bound capture oligonucleotide to its solution-phase complement. Fluorescein-labeled solution-phase oligonucleotide was hybridized to varying amounts of particles, and the amount of labeled oligonucleotide remaining in solution at equilibrium was measured. We present a simple two-state, all-or-none model for bimolecular hybridization of non-self-complementary sequences that can be used to calculate the equilibrium dissociation constant ( Kd ) from hybridization data. With experimental conditions where both the Kd value and the concentration of capture probe in the reaction are small relative to the concentration of labeled complementary oligonucleotide in the reaction, density of the capture probe on the particle's surface can also be determined. Kd values for particle-based hybridization were different from those obtained from solution-phase thermodynamic parameters. At higher temperatures, hybridization on particles was more efficient than hybridization in solution.

摘要

许多DNA探针检测方法利用包被有寡核苷酸的微粒从溶液中捕获互补核酸。在这些检测方法的开发过程中,以及在其他基于微粒的核酸应用中,了解在各种实验条件下预期的双链体形成量以及微粒表面捕获寡核苷酸的包被密度是很有用的。我们研究了DNA探针微粒检测方法的最简单形式:颗粒结合的捕获寡核苷酸与其溶液相互补物的杂交。将荧光素标记的溶液相寡核苷酸与不同量的微粒杂交,并测量平衡时溶液中剩余的标记寡核苷酸量。我们提出了一个简单的两态、全或无模型,用于非自互补序列的双分子杂交,该模型可用于根据杂交数据计算平衡解离常数(Kd)。在实验条件下,如果Kd值和反应中捕获探针的浓度相对于反应中标记的互补寡核苷酸的浓度都较小,也可以确定微粒表面捕获探针的密度。基于微粒的杂交的Kd值与从溶液相热力学参数获得的Kd值不同。在较高温度下,微粒上的杂交比溶液中的杂交更有效。