Cantón Irene, Sarwar Umran, Kemp E Helen, Ryan Anthony J, MacNeil Sheila, Haycock John W
Department of Engineering Materials, Kroto Research Institute, University of Sheffield, and Northern General Hospital, Sheffield, United Kingdom.
Tissue Eng. 2007 May;13(5):1013-24. doi: 10.1089/ten.2006.0357.
The main objective of this study was to develop a nondestructive reporter system for assessing the response of human cells contained within a three-dimensional (3D) tissue-engineered construct to exogenous stress. Dermal fibroblasts were transiently transfected with a reporter construct linked to nuclear factor kappaB (NF-kappaB) activation which led to expression of a nonstable form of enhanced green fluorescent protein (d2EGFP) after stimulation. This led to a temporary production of fluorescence, which could be readily detected but was not intrinsically toxic, as cells were able to metabolize the initial cycle of d2EGFP produced. This permitted the model to be used for restimulation post recovery. To investigate the performance and predictive ability of this method for assessing cellular response to stress in 3D, we used a range of compounds known to have pro-inflammatory or oxidative properties. Tumor necrosis factor-alpha (TNF-alpha) and interleukin-1-beta (IL-1beta) were selected for having a direct cytokine action; lipopolysaccharide (LPS) was selected for modeling bacterial-mediated inflammation; and hydrogen peroxide was selected as a crude method for delivering an oxidative stress. Transfected cells were stimulated with the above compounds in 3D and the synthesis of d2EGFP was detected as a measure of NF-kappaB activation. The resultant fluorescence was scored using a series of photomicrographs taken by epifluorescence microscopy. All agents activated NF-kappaB when cells were grown in 3D scaffolds but did not cause any significant reduction in cell viability as measured by a standard MTT-ESTA viability test. Parallel NF-kappaB activation and MTT measurements was also conducted in two-dimension (2D) and confirmed findings in 3D. The 3D model described using a fluorescent reporter gene is a highly sensitive and reliable method for detecting cellular stress and represents a key step in developing tissue engineering models with the potential for screening pharmaceutical and cosmetic compounds, as an alternative to existing in vitro and in vivo methods.
本研究的主要目的是开发一种非破坏性报告系统,用于评估三维(3D)组织工程构建物中所含人类细胞对外源应激的反应。将真皮成纤维细胞用与核因子κB(NF-κB)激活相关的报告构建体进行瞬时转染,刺激后导致不稳定形式的增强型绿色荧光蛋白(d2EGFP)表达。这导致了荧光的暂时产生,其易于检测且本质上无毒,因为细胞能够代谢产生的d2EGFP的初始循环。这使得该模型可用于恢复后的再刺激。为了研究该方法在评估3D中细胞对应激反应的性能和预测能力,我们使用了一系列已知具有促炎或氧化特性的化合物。选择肿瘤坏死因子-α(TNF-α)和白细胞介素-1-β(IL-1β)是因为它们具有直接的细胞因子作用;选择脂多糖(LPS)来模拟细菌介导的炎症;选择过氧化氢作为施加氧化应激的粗略方法。在3D中用上述化合物刺激转染的细胞,并检测d2EGFP的合成作为NF-κB激活的指标。使用落射荧光显微镜拍摄的一系列显微照片对产生的荧光进行评分。当细胞在3D支架中生长时,所有试剂均激活了NF-κB,但通过标准MTT-ESTA活力测试测量,未导致细胞活力有任何显著降低。还在二维(2D)中进行了平行的NF-κB激活和MTT测量,并证实了3D中的结果。使用荧光报告基因描述的3D模型是检测细胞应激的高度敏感和可靠的方法,并且代表了开发具有筛选药物和化妆品化合物潜力的组织工程模型的关键步骤,作为现有体外和体内方法的替代方法。
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