首页> 外文期刊>Biological & pharmaceutical bulletin >Creation of novel cell-penetrating peptides for intracellular drug delivery using systematic phage display technology originated from Tat transduction domain.
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Creation of novel cell-penetrating peptides for intracellular drug delivery using systematic phage display technology originated from Tat transduction domain.

机译:使用系统化的噬菌体展示技术,从Tat转导结构域创建用于细胞内药物递送的新型细胞穿透肽。

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摘要

Many biologically active proteins need to be delivered intracellularly to exert their therapeutic action inside the cytoplasm. Cell penetrating peptides (CPPs) have been developed to efficiently deliver a wide variety of cargo in a fully biological active form into a range of cell types for the treatment of multiple preclinical disease models. To further develop this methodology, we established a systematic approach to identify novel CPPs using phage display technology. Firstly, we screened a phage peptide library for peptides that bound to the cell membrane. Secondly, to assess functionality as intracellular carriers, we recombined cDNAs of binding peptides with protein synthesis inhibitory factor (PSIF) to create fusion proteins. Randomly chosen clones were cultured and expression of peptide-PSIF fusion proteins induced, followed by screening of protein synthesis activity in cells. Using this systematic approach, novel and effective CPPs were rapidly identified. We suggest that these novel cell-penetrating peptides can utilized as drug delivery tools for protein therapy or an analytical tool to study mechanisms of protein transduction into the cytoplasm.
机译:许多生物活性蛋白需要在细胞内传递,以在细胞质内发挥其治疗作用。已经开发出细胞穿透肽(CPPs),以将具有完全生物活性形式的多种货物有效地递送到多种细胞类型中,以治疗多种临床前疾病模型。为了进一步开发这种方法,我们建立了一种系统的方法来使用噬菌体展示技术鉴定新型CPP。首先,我们筛选了噬菌体肽库中与细胞膜结合的肽。其次,为了评估作为细胞内载体的功能,我们将结合肽的cDNA与蛋白质合成抑制因子(PSIF)重组以产生融合蛋白。培养随机选择的克隆并诱导肽-PSIF融合蛋白的表达,然后筛选细胞中的蛋白合成活性。使用这种系统的方法,可以迅速识别出新颖有效的CPP。我们建议这些新的细胞穿透肽可以用作蛋白质治疗的药物传递工具或研究蛋白质转导进入细胞质的机制的分析工具。

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