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聚阳离子和脂质体介导的核酸传递机制:瞬时膜去稳定化的实时可视化,而无内涵体溶酶体的作用。

Mechanism of polyplex- and lipoplex-mediated delivery of nucleic acids: real-time visualization of transient membrane destabilization without endosomal lysis.

机构信息

Department of Cell Biology, University Medical Center Groningen, University of Groningen, A Deusinglaan 1, 9713 AV Groningen, The Netherlands.

出版信息

ACS Nano. 2013 May 28;7(5):3767-77. doi: 10.1021/nn3049494. Epub 2013 Apr 24.

Abstract

Lipoplexes and polyplexes are widely applied as nonviral gene delivery carriers. Although their efficiencies of transfection are comparable, their mechanisms of delivery, specifically at the level of nucleic acid release from endosomes, are different. Thus, lipoplex-mediated release is proposed to rely on lipid mixing, as occurs between lipoplex and endosomal target membrane, the ensuing membrane destabilization leading to nucleic acid delivery into the cytosol. By contrast, the mechanism by which polyplexes, particularly those displaying a high proton buffering capacity, release their nucleic acid cargo from the endosome, is thought to rely on a so-called "proton sponge effect", in essence an osmotically induced rupturing of the endosomal membrane. However, although a wealth of indirect insight supports both these mechanisms, direct evidence is still lacking. Therefore, to further clarify these mechanisms, we have investigated the interaction of lipo- and polyplexes with HeLa cells by live cell imaging. As monitored over an incubation period of 2 h, our data reveal that in contrast to the involvement of numerous nanocarriers in case of lipoplex-mediated delivery, only a very limited number of polyplexes, that is, as few as one up to four/five nanocarriers per cell, with an average of one/two per cell, contribute to the release of nucleic acids from endosomes and their subsequent accumulation into the nucleus. Notably, in neither case complete rupture of endosomes nor release of intact polyplexes or lipoplexes into the cytosol was observed. Rather, at the time of endosomal escape both the polymer and its genetic payload are separately squirted into the cytoplasm, presumably via (a) local pore(s) within the endosomal membrane. Specifically, an almost instantaneous and complete discharge of nucleic acids and carrier (remnants) from the endosomes is observed. In case of lipoplexes, the data suggest the formation of multiple transient pores over time within the same endosomal membrane, via which the cargo is more gradually transferred into the cytosol.

摘要

脂质体和多聚物被广泛应用于非病毒基因传递载体。尽管它们的转染效率相当,但它们的传递机制,特别是在从内涵体释放核酸的水平上,是不同的。因此,脂质体介导的释放被认为依赖于脂质混合,就像脂质体与内涵体靶膜之间发生的那样,随后的膜不稳定导致核酸递送到细胞质中。相比之下,多聚物,特别是那些具有高质子缓冲能力的多聚物,从内涵体中释放其核酸货物的机制被认为依赖于所谓的“质子海绵效应”,本质上是内涵体膜的渗透压诱导破裂。然而,尽管有大量间接的证据支持这两种机制,但仍缺乏直接证据。因此,为了进一步阐明这些机制,我们通过活细胞成像研究了脂质体和多聚物与 HeLa 细胞的相互作用。在 2 小时的孵育期间进行监测,我们的数据表明,与脂质体介导的传递中涉及大量纳米载体相反,只有非常有限数量的多聚物,即每个细胞多达一到四个/五个纳米载体,平均每个细胞一个/两个,有助于从内涵体中释放核酸,并随后将其积累到细胞核中。值得注意的是,在这两种情况下,都没有观察到内涵体完全破裂,也没有观察到完整的多聚物或脂质体释放到细胞质中。相反,在内涵体逃逸时,聚合物及其遗传载荷都分别被喷射到细胞质中,推测是通过内涵体膜内的(一个)局部孔。具体地说,观察到核酸和载体(残留物)几乎瞬间和完全从内涵体中排出。在脂质体的情况下,数据表明随着时间的推移,同一内涵体膜内形成了多个瞬时孔,通过这些孔,货物逐渐转移到细胞质中。

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