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拓扑定义的线性和环状DNA瓶刷聚合物的生成:一种接枝法。

Generation of topologically defined linear and cyclic DNA bottle brush polymers a graft-to approach.

作者信息

Pierini Nicholas G, Paiva Wynter A, Durant Owen C, Dobbins Aubrianna M, Wheeler Ben B, Currier Matthew E, Vesenka James, Oldenhuis Nathan J

机构信息

Department of Chemistry, College of Engineering and Physical Science, University of New Hampshire 23 Academic Way Parsons Hall Durham NH 03824 USA

School of Molecular and Physical Sciences, University of New England 11 Hills Beach Road Biddeford ME 04005 USA.

出版信息

Polym Chem. 2025 May 1. doi: 10.1039/d5py00082c.

Abstract

Herein, we report a graft-to approach for synthesizing linear and circular double-stranded DNA (dsDNA) bottlebrush polymers (BBPs). Using a bioreactor, plasmid DNA (pDNA) serves as an inexpensive and abundant source of circular, biodegradable, and unimolecular polymers. pDNA is easily converted to the linear isoform through enzymatic restriction, providing access to polymeric backbones with distinct topological states. DNA is grafted with polyethylene glycol monomethyl ether chloroethylamines (mPEGCEA) to yield DNA BBPs. Importantly this PEGylation occurs rapidly under ambient conditions in aqueous buffer. By varying the molecular weight of mPEGCEA ( = 750, 2000, 5000 Da) and the concentration relative to μmol of nucleotides, different brush arm densities and lengths were achieved with both linear and macrocyclic DNA backbones. Analysis of the DNA BBPs was achieved through agarose gel electrophoresis, which showed graft densities of up to ~68% and ~74% for linear and ring DNA respectively. The grafting process does not alter base pairing or circularity as determined using atomic force microscopy. Shear rheology was used to compare the mechanical response of 1% wt/wt solutions of the ring and linear DNA BBPs to their un-alkylated forms. Linear DNA BBPs exhibited a lower shear modulus linear DNA, which is expected due to the increased persistence length and decreased ability to interpenetrate associated with the attachment of polymer arms. However, the circular DNA BBPs exhibited a universally higher shear modulus the un-alkylated sample suggesting an increase in interchain interaction addition of polymer arms. Finally, the increased steric encumbrance of the DNA BBPs slows enzymatic degradation, potentially providing a general method to increase stability of DNA constructs towards nuclease.

摘要

在此,我们报道了一种用于合成线性和环状双链DNA(dsDNA)瓶刷聚合物(BBP)的接枝法。使用生物反应器,质粒DNA(pDNA)作为环状、可生物降解且单分子聚合物的廉价且丰富的来源。通过酶切限制,pDNA可轻松转化为线性异构体,从而获得具有不同拓扑状态的聚合物主链。DNA与聚乙二醇单甲醚氯乙胺(mPEGCEA)接枝以产生DNA BBP。重要的是,这种聚乙二醇化在水性缓冲液的环境条件下迅速发生。通过改变mPEGCEA的分子量( = 750、2000、5000 Da)以及相对于核苷酸μmol的浓度,使用线性和大环DNA主链均可实现不同的刷臂密度和长度。通过琼脂糖凝胶电泳对DNA BBP进行分析,结果表明线性和环状DNA的接枝密度分别高达约68%和约74%。如使用原子力显微镜所确定的,接枝过程不会改变碱基配对或环状结构。使用剪切流变学来比较环状和线性DNA BBP的1% wt/wt溶液与其未烷基化形式的力学响应。线性DNA BBP表现出较低的剪切模量 线性DNA,这是预期的,因为聚合物臂的附着导致持久长度增加且相互渗透能力降低。然而,环状DNA BBP表现出普遍高于未烷基化样品的剪切模量,表明聚合物臂的添加增加了链间相互作用。最后,DNA BBP增加的空间位阻减缓了酶促降解,这可能提供了一种提高DNA构建体对核酸酶稳定性的通用方法。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/f61f/12070894/05d8fd3315cf/d5py00082c-f1.jpg

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