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Ultrasound-targeted microbubbles combined with a peptide nucleic acid binding nuclear localization signal mediate transfection of exogenous genes by improving cytoplasmic and nuclear import

机译:超声靶向微泡与肽核酸结合核定位信号通过改善细胞质和核进口来介导外源基因的转染

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摘要

The development of an efficient delivery system is critical for the successful treatment of cardiovascular diseases using non-viral gene therapies. Cytoplasmic and nuclear membrane barriers reduce delivery efficiency by impeding the transfection of foreign genes. Thus, a gene delivery system capable of transporting exogenous genes may improve gene therapy. The present study used a novel strategy involving ultrasound-targeted microbubbles and peptide nucleic acid (PNA)-binding nuclear localization signals (NLS). Ultrasound-targeted microbubble destruction (UTMD) and PNA-binding NLS were used to improve the cytoplasmic and nuclear importation of the plasmid, respectively. Experiments were performed using antibody-targeted microbubbles (AT-MCB) that specifically recognize the SV40T antigen receptor expressed on the membranes of 293T cells, resulting in the localization of ultrasound microbubbles to 293T cell membranes. Furthermore, PNA containing NLS was inserted into the enhanced green fluorescent protein (EGFP)-N3 plasmid DNA (NLS-PNA-DNA), which increased nuclear localization. The nuclear import and gene expression efficiency of the AT-MCB with PNA-binding NLS were compared with AT-MCB alone or a PNA-binding NLS. The effect of the AT-MCB containing PNA-binding NLS on transfection was investigated. The ultrasound and AT-MCB delivery significantly enhanced the cytoplasmic intake of exogenous genes and maintained high cell viability. The nuclear import and gene expression of combined microbubble-and PNA-transfected cells were significantly greater compared with cells that were transfected with AT-MCB or DNA with only PNA-binding NLS. The quantity of EGFP-N3 plasmids in the nuclei was increased by 5.0-fold compared with control microbubbles (CMCB) and NLS-free plasmids. The gene expression was similar to 1.7-fold greater compared with NLS-free plasmids and 1.3-fold greater compared with control microbubbles. In conclusion, UTMD combined with AT-MCB and a PNA-binding NLS plasmid significantly improved transfection efficiency by increasing cytoplasmic and nuclear DNA import. This method is a promising strategy for the noninvasive and effective delivery of target genes or drugs for the treatment of cardiovascular diseases.
机译:高效交付系统的发展对于使用非病毒基因疗法成功治疗心血管疾病的成功态度至关重要。细胞质和核膜屏障通过阻碍外源基因的转染来降低输送效率。因此,能够传送外源基因的基因递送系统可以改善基因治疗。本研究使用了一种新的策略,涉及超声靶向微泡和肽核酸(PNA) - 耦合核定位信号(NLS)。超声靶向微泡破坏(UTMD)和PAN结合NLS分别用于改善质粒的细胞质和核进口。使用特异性识别在293T细胞膜上表达的SV40T抗原受体的抗体靶向微泡(AT-MCB)进行实验,导致超声微泡的定位到293T细胞膜。此外,将含有N1的PNA插入增强的绿色荧光蛋白(EGFP)-N3质粒DNA(NLS-PNA-DNA)中,这增加了核定位。将AT-MCB的核进口和基因表达效率与单独的AT-MCB或PNA结合NL进行比较。研究了含有PNA结合NLS对转染的AT-MCB的效果。超声和MCB递送显着增强了外源基因的细胞质摄入并保持了高细胞活力。与仅用于PNA结合NLS转染的细胞相比,将微泡和PNA转染的细胞组合的核进口和基因表达明显更大。与对照微泡(CMCB)和无铅质粒相比,核中核中的EGFP-N3质粒的数量增加。5.0倍。与对照微泡相比,基因表达类似于1.7倍,与无铅质粒相比,1.3倍更大。总之,UTMD结合AT-MCB和PNA结合NLS质粒通过增加细胞质和核DNA进口,显着提高了转染效率。该方法是非侵入性和有效递送靶基因或药物治疗心血管疾病的有希望的策略。

著录项

  • 来源
    《Molecular medicine reports》 |2017年第2期|共7页
  • 作者单位

    Wuhan Univ Renmin Hosp Dept Ultrasound Imaging 238 Jiefang Rd Wuhan 430060 Hubei Peoples R;

    Wuhan Univ Renmin Hosp Dept Ultrasound Imaging 238 Jiefang Rd Wuhan 430060 Hubei Peoples R;

    Wuhan Univ Renmin Hosp Dept Ultrasound Imaging 238 Jiefang Rd Wuhan 430060 Hubei Peoples R;

    Wuhan Univ Renmin Hosp Dept Ultrasound Imaging 238 Jiefang Rd Wuhan 430060 Hubei Peoples R;

    Wuhan Univ Renmin Hosp Dept Ultrasound Imaging 238 Jiefang Rd Wuhan 430060 Hubei Peoples R;

    Wuhan Univ Renmin Hosp Dept Ultrasound Imaging 238 Jiefang Rd Wuhan 430060 Hubei Peoples R;

    Wuhan Univ Renmin Hosp Dept Ultrasound Imaging 238 Jiefang Rd Wuhan 430060 Hubei Peoples R;

  • 收录信息
  • 原文格式 PDF
  • 正文语种 eng
  • 中图分类 基础医学;
  • 关键词

    ultrasound; microbubbles; peptide nucleic acid; nuclear localization signals; gene transfection;

    机译:超声波;微泡;肽核酸;核定位信号;基因转染;

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