Assessment of methods and analysis of outcomes for comprehensive optimization of nucleofection.

Christopher Bradburne, Kelly Robertson, Dzung Thach
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引用次数: 10

Abstract

Background: Nucleofection is an emerging technology for delivery of nucleic acids into both the cytoplasm and nucleus of eukaryotic cells with high efficiency. This makes it an ideal technology for gene delivery and siRNA applications. A 96-well format has recently been made available for high-throughput nucleofection, however conditions must be optimized for delivery into each specific cell type. Screening each 96-well plate can be expensive, and descriptions of methods and outcomes to determine the best conditions are lacking in the literature. Here we employ simple methods, including cell counting, microscopy, viability and cytotoxicity assays to describe the minimal experimental methods required to optimize nucleofection conditions for a given cell line.

Methods: We comprehensively measured and analyzed the outcomes of the 96-well nucleofection of pmaxGFP plasmids encoding green fluorescent protein (GFP) into the A-549 human lung epithelial cell line. Fluorescent microscopy and a plate reader were used to respectively observe and quantify green fluorescence in both whole and lysed cells. Cell viability was determined by direct counting/permeability assays, and by both absorbance and fluorescence-based plate reader cytotoxicity assays. Finally, an optimal nucleofection condition was used to deliver siRNA and gene specific knock-down was demonstrated.

Results: GFP fluorescence among conditions ranged from non-existent to bright, based upon the fluorescent microscopy and plate reader results. Correlation between direct counting of cells and plate-based cytotoxicity assays were from R = .81 to R = .88, depending on the assay. Correlation between the GFP fluorescence of lysed and unlysed cells was high, ranging from R = .91 to R = .97. Finally, delivery of a pooled sample of siRNAs targeting the gene relA using an optimized nucleofection condition resulted in a 70-95% knock down of the gene over 48 h with 90-97% cell viability.

Conclusion: Our results show the optimal 96-well nucleofection conditions for the widely-used human cell line, A-549. We describe simple, effective methods for determining optimal conditions with high confidence, providing a useful road map for other laboratories planning optimization of specific cell lines or primary cells. Our analysis of outcomes suggests the need to only measure unlysed, whole-cell fluorescence and cell metabolic activity using a plate reader cytotoxicity assay to determine the best conditions for 96-well nucleofection.

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核酸综合优化方法评价及结果分析。
背景:核酸转染是一种新兴的将核酸高效率地传递到真核细胞的细胞质和细胞核中的技术。这使其成为基因传递和siRNA应用的理想技术。最近,高通量核转染的96孔格式已经可用,然而,必须优化条件才能将其输送到每种特定的细胞类型。筛选每个96孔板可能会很昂贵,并且文献中缺乏确定最佳条件的方法和结果的描述。在这里,我们采用简单的方法,包括细胞计数,显微镜,活力和细胞毒性测定来描述优化给定细胞系的核感染条件所需的最小实验方法。方法:对编码绿色荧光蛋白(GFP)的pmaxGFP质粒转染A-549人肺上皮细胞系96孔的结果进行综合测定和分析。用荧光显微镜和平板阅读器分别观察和定量整个细胞和裂解细胞的绿色荧光。细胞活力通过直接计数/通透性测定,以及吸光度和荧光板细胞毒性测定测定。最后,采用最佳的转染条件来传递siRNA,并演示了基因特异性敲除。结果:根据荧光显微镜和平板阅读器的结果,GFP荧光在不同的条件下从不存在到明亮。直接细胞计数和基于平板的细胞毒性测定之间的相关性从R = 0.81到R = 0.88,取决于测定方法。裂解细胞与未裂解细胞的GFP荧光相关性高,R = 0.91 ~ 0.97。最后,使用优化的核感染条件递送针对relA基因的sirna混合样本,在48小时内导致70-95%的基因敲低,90-97%的细胞存活率。结论:我们的研究结果为广泛应用的人A-549细胞株提供了96孔的最佳核转染条件。我们描述了一种简单、有效的方法来确定高可信度的最佳条件,为其他实验室规划特定细胞系或原代细胞的优化提供了有用的路线图。我们对结果的分析表明,只需要使用平板阅读器细胞毒性试验来测量未裂解的全细胞荧光和细胞代谢活性,以确定96孔细胞核感染的最佳条件。
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