Barrán-Berdón Ana L, Yélamos Belén, Malfois Marc, Aicart Emilio, Junquera Elena
Grupo de Química Coloidal y Supramolecular, Departamento de Química Física I, and ∥Departamento de Bioquímica y Biología Molecular I, Facultad de Ciencias Químicas, Universidad Complutense de Madrid , 28040 Madrid, Spain.
Langmuir. 2014 Oct 7;30(39):11704-13. doi: 10.1021/la502823z. Epub 2014 Sep 25.
Several experimental methods, such as zeta potential, gel electrophoresis, small-angle X-ray scattering, gene transfection, fluorescence microscopy, flow cytometry, and cell viability/cytotoxicity assays, have been used to analyze the potential of anionic lipids (AL) as effective nontoxic and nonviral DNA vectors, assisted by divalent cations. The lipoplexes studied are those comprised of the green fluorescent protein-encoding plasmid DNA pEGFP-C3, an anionic lipid as 1,2-dioleoyl-sn-glycero-3-phospho-(1'-rac-glycerol) (DOPG) or 1,2-dioleoyl-sn-glycero-3-phospho-L-serine (DOPS), and a zwitterionic lipid, the 1,2-dioleoyl-sn -glycero-3-phosphatidylethanolamine (DOPE, not charged at physiological pH). The studies have been carried on at different liposome and lipoplex compositions and in the presence of a variety of [Ca2+]. Electrochemical experiments reveal that DOPG/DOPE and DOPS/DOPE anionic liposomes may compact more effectively pDNA at low molar fractions (with an excess of DOPE) and at AL/pDNA ratios ≈20. Calcium concentrations around 15-20 mM are needed to yield lipoplexes neutral or slightly positive. From a structural standpoint, DOPG/DOPE-Ca2+-pDNA lipoplexes are self-assembled into a HIIc phase (inverted cylindrical micelles in hexagonal ordering with plasmid supercoils inside the cylinders), while DOPS/DOPE-Ca2+-pDNA lipoplexes show two phases in coexistence: one classical HIIc phase which contains pDNA supercoils and one Lα phase without pDNA among the lamellae, i.e., a lamellar stack of lipidic bilayers held together by Ca2+ bridges. Transfection and cell viability studies were done with HEK293T and HeLa cells in the presence of serum. Lipoplexes herein studied show moderate-to-low transfection levels combined with moderate-to-high cell viability, comparable to those yield by Lipofectamine2000*, which is a cationic lipid (CL) standard formulation, but none of them improve the output of typical CL gen vectors, mostly if they are gemini or dendritic. This fact would be indicating that, nowadays, lipofection via anionic lipids and divalent cations as mediators still needs to enhance transfection levels in order to be considered as a real and plausible alternative to lipofection through improved CLs-based lipoplexes.
已经使用了几种实验方法,如zeta电位、凝胶电泳、小角X射线散射、基因转染、荧光显微镜、流式细胞术和细胞活力/细胞毒性测定,来分析阴离子脂质(AL)作为有效的无毒非病毒DNA载体在二价阳离子辅助下的潜力。所研究的脂质体复合物由编码绿色荧光蛋白的质粒DNA pEGFP-C3、作为1,2-二油酰基-sn-甘油-3-磷酸-(1'-rac-甘油)(DOPG)或1,2-二油酰基-sn-甘油-3-磷酸-L-丝氨酸(DOPS)的阴离子脂质以及两性离子脂质1,2-二油酰基-sn-甘油-3-磷脂酰乙醇胺(DOPE,在生理pH下不带电荷)组成。研究在不同的脂质体和脂质体复合物组成以及各种[Ca2+]存在的情况下进行。电化学实验表明,DOPG/DOPE和DOPS/DOPE阴离子脂质体在低摩尔分数(DOPE过量)和AL/pDNA比率≈20时可能更有效地压缩pDNA。需要约15-20 mM的钙浓度才能产生中性或略带正电的脂质体复合物。从结构角度来看,DOPG/DOPE-Ca2+-pDNA脂质体复合物自组装成HIIc相(六边形排列的反圆柱胶束,圆柱内有质粒超螺旋),而DOPS/DOPE-Ca2+-pDNA脂质体复合物显示出两相共存:一个经典的HIIc相,其中包含pDNA超螺旋,另一个Lα相,在片层中没有pDNA,即由Ca2+桥连接在一起的脂质双层的层状堆叠。在有血清存在的情况下,用HEK293T和HeLa细胞进行了转染和细胞活力研究。本文研究的脂质体复合物显示出中低转染水平与中高细胞活力相结合,与阳离子脂质(CL)标准制剂Lipofectamine2000*产生的水平相当,但它们都没有提高典型CL基因载体的输出,尤其是如果它们是双子型或树枝状的。这一事实表明,如今,以阴离子脂质和二价阳离子作为介质的脂质转染仍需要提高转染水平,以便被视为通过改进的基于CL的脂质体复合物进行脂质转染的真正可行替代方案。
