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Quantitative comparison between poly(L-arginine) and poly(L-lysine) at each step of polyplex-based gene transfection using a microinjection technique

机译:使用显微注射技术对基于多重复合体的基因转染的每个步骤中的聚L-精氨酸和聚L-赖氨酸进行定量比较

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摘要

Among the well-studied polypeptide-type gene carriers, transfection efficiency is empirically known to be higher for poly(L-arginine) (PR) than poly(L-lysine) (PK). The big difference between PR and PK should be determined at one of the intracellular trafficking steps based on the different charge densities, structures or PKa values. However, the endosomal escape and the intranuclear transcription efficiency in living cells have not been clarified yet. In this study, a novel method for quantifying the intranuclear transcription efficiency and the nuclear transport of the polyplex is established based on the nuclear and the cytosolic microinjection technique, and the results for PK and PR with different molecular weights (MWs) are compared in living cells. The intranuclear transcription efficiency is the same in PR and PK and it decreases rapidly with increasing MW, in spite of the commonly measured transfection efficiency. The transcription efficiency is strongly suppressed at high MW and strongly correlates with the polyplex forming ability expressed as a critical ratio of the number of polypeptide cationic groups to the number of pDNA anionic groups. When considered with the results of the cellular uptake and in vitro transfection with or without chloroquine, the rate-limiting step for their gene transfer is the buffering effect-independent endosomal escape.
机译:在经过充分研究的多肽类型基因载体中,根据经验已知,聚(L-精氨酸)(PR)的转染效率高于聚(L-赖氨酸)(PK)。 PR和PK之间的较大差异应根据不同的电荷密度,结构或PKa值在细胞内运输步骤之一中确定。然而,活细胞中的内体逃逸和核内转录效率尚未阐明。在这项研究中,基于核和胞质显微注射技术,建立了一种定量多聚体核内转录效率和核转运的新方法,并比较了不同分子量(MW)的PK和PR的结果。细胞。尽管通常测定了转染效率,但PR和PK中的核内转录效率是相同的,并且随着MW的增加,核内转录效率会迅速下降。在高分子量下,转录效率被强烈抑制,并且与多聚体形成能力密切相关,多聚体形成能力以多肽阳离子基团数目与pDNA阴离子基团数目的临界比率表示。当考虑细胞吸收和体外转染的结果(有或没有氯喹)时,其基因转移的限速步骤是不依赖缓冲作用的内体逃逸。

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