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Oligo-L-lysine-, dextran-, and alkyl- derivatives of polyethylenimine for the development of novel gene transfection vectors.

机译:聚乙烯亚胺的寡聚-L-赖氨酸,葡聚糖和烷基衍生物,用于开发新型基因转染载体。

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Synthesis of a dendrimer for a proposed non-viral vector has been taken with the following attributes: an inner polycationic polyethylenimine (PEI) core (to help lyse endosomes by osmotic effects) linked to a hydrophobic shell (to lyse endocytotic vesicles by lipid depletion) linked to an outer shell of oligoamines (which binds DNA and the cell surface) by means of acid labile linkers designed to be disrupted by changing pH conditions inside the endocytotic vesicle. The synthesis of the proposed dendrimer will take place in a part convergent, part divergent method, to minimize the handling of the acid labile linker. The hydrophobic shell has been added to the PEI core in a divergent mode. This reaction proceeds by alkyl iodide displacement on the PEI amines. The terminal functionality of the alkyl groups consists of a homocysteine thiolactone ring where upon treatment with base reveals a thiol functionality. This thiol reacts readily with homo-bifunctional acid labile maleimide linkers. In the last step, a convergent synthesis approach will be used to couple the PEI-hydrophobic shell to the linker-oligoamine, via a thioether bond. The outer shell will consist of short oligoamines such as spermidine, and low molecular weight polyethylenimine. This oligoamine shell will be attached through acid labile linkers, which will allow detachment of the complexed DNA-Oligoamines once inside the acidic endocytotic environment. The dendrimeric vectors were analyzed using dynamic and static laser light scattering to characterize the vectors and their complexes with plasmid DNA. Flow cytometry was employed to quantify the reporter protein (enhanced green fluorescent protein) and cytotoxicity of the dendrimeric vector/pEGFP complexes. Dextran and oligo-L-lysine polyethylenimine derivatives were also synthesized and characterized in regards to their potential as gene delivery vectors.
机译:已针对拟议的非病毒载体合成了树枝状大分子,其具有以下属性:内聚阳离子聚乙烯亚胺(PEI)核心(通过渗透作用帮助溶解内体)与疏水壳连接(通过脂质消耗来溶解内吞性囊泡)通过酸不稳定的连接子连接至寡胺的外壳(其结合DNA和细胞表面),酸不稳定的连接子设计为通过改变内吞小泡内的pH条件而被破坏。提出的树枝状聚合物的合成将以部分收敛,部分发散的方法进行,以最大程度地减少对酸不稳定的接头的处理。疏水壳已以发散模式添加到PEI核中。该反应通过在PEI胺上置换烷基碘来进行。烷基的末端官能团由高半胱氨酸硫代内酯环组成,其中在用碱处理后揭示出硫醇官能团。该硫醇容易与均双功能酸不稳定的马来酰亚胺连接基反应。在最后一步中,将使用收敛合成方法将PEI-疏水性壳通过硫醚键偶联至连接子-低聚胺。外壳将由短寡胺(如亚精胺)和低分子量聚乙烯亚胺组成。该低聚胺壳将通过酸不稳定的接头连接,一旦进入酸性内吞环境,该复合物将允许复合的DNA-低聚胺的分离。使用动态和静态激光散射分析树枝状载体,以表征载体及其与质粒DNA的复合物。流式细胞仪用于定量报告蛋白(增强型绿色荧光蛋白)和树状载体/ pEGFP复合物的细胞毒性。还合成了葡聚糖和低聚-L-赖氨酸聚亚乙基亚胺衍生物,并就它们作为基因递送载体的潜力进行了表征。

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