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An efficient method for introducing macromolecules into living cells

机译:一种将大分子引入活细胞的有效方法

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摘要

The hemagglutinin (HA) of influenza virus was used to obtain efficient and rapid bulk delivery of antibodies and horseradish peroxidase (HRP) into the cytoplasm of living tissue culture cells. By exploiting HA's efficient cell surface expression, its high affinity for erythrocytes, and its acid-dependent membrane fusion activity, a novel delivery method was developed. The approach is unique in that the mediator of both binding and fusion (the HA) is present on the surfaces of the target cells. A recently developed 3T3 cell line which permanently expresses HA, Madin-Darby canine kidney cells infected with influenza virus, and CV-1 cells infected with a simian virus 40 vector carrying the HA gene were used as recipient cells. Protein-loaded erythrocytes were bound to the HA on the cell surface and a brief drop in pH to 5.0 was used to trigger HA's fusion activity and hence delivery. About 3 to 8 erythrocytes fused per 3T3 and CV-1 cell, respectively, and 75-95% of the cells received IgG or HRP. Quantitative analysis showed that 1.8 X 10(8) molecules of HRP and 1.4 X 10(7) IgG molecules were delivered per CV-1 cell and 6.2 X 10(7) HRP molecules per 3T3 cell. Cell viability, as judged by methionine incorporation into protein and cell growth and division, was not impaired. Electron and fluorescence microscopy showed that the fused erythrocyte membranes remained as discrete domains in the cell's plasma membrane. The method is simple, reliable, and nonlytic. The ability to simultaneously and rapidly deliver impermeable substances into large numbers of cells will permit biochemical analysis of the fate and effect of a variety of delivered molecules.
机译:流感病毒的血凝素(HA)用于将抗体和辣根过氧化物酶(HRP)快速有效地大量递送到活组织培养细胞的细胞质中。通过利用HA的有效细胞表面表达,其对红细胞的高亲和力以及其酸依赖性膜融合活性,开发了一种新颖的递送方法。该方法的独特之处在于,靶细胞表面上同时存在结合和融合的介体(HA)。使用最近开发的永久表达HA的3T3细胞系,感染流感病毒的Madin-Darby犬肾细胞和感染携带HA基因的猿猴病毒40载体的CV-1细胞作为受体细胞。载有蛋白质的红细胞与细胞表面的HA结合,pH值短暂降至5.0即可触发HA的融合活性,从而触发其转运。每个3T3和CV-1细胞分别融合约3至8个红细胞,其中75-95%的细胞接受IgG或HRP。定量分析表明,每个CV-1细胞可递送1.8 X 10(8)HRP分子和1.4 X 10(7)IgG分子,每个3T3细胞可递送6.2 X 10(7)HRP分子。通过将蛋氨酸掺入蛋白质以及细胞生长和分裂来判断细胞活力并没有受到损害。电子和荧光显微镜检查显示,融合的红细胞膜在细胞质膜中保留为离散域。该方法简单,可靠且不易分解。同时快速将不可渗透物质输送到大量细胞中的能力将允许对各种输送分子的命运和作用进行生化分析。

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