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A human monocytic NF-κB fluorescent reporter cell line for detection of microbial contaminants in biological samples

机译:用于检测生物样品中微生物污染物的人类单核细胞NF-κB荧光报告细胞系

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摘要

Sensing of pathogens by innate immune cells is essential for the initiation of appropriate immune responses. Toll-like receptors (TLRs), which are highly sensitive for various structurally and evolutionary conserved molecules derived from microbes have a prominent role in this process. TLR engagement results in the activation of the transcription factor NF-κB, which induces the expression of cytokines and other inflammatory mediators. The exquisite sensitivity of TLR signalling can be exploited for the detection of bacteria and microbial contaminants in tissue cultures and in protein preparations. Here we describe a cellular reporter system for the detection of TLR ligands in biological samples. The well-characterized human monocytic THP-1 cell line was chosen as host for an NF-ᴋB-inducible enhanced green fluorescent protein reporter gene. We studied the sensitivity of the resultant reporter cells for a variety of microbial components and observed a strong reactivity towards TLR1/2 and TLR2/6 ligands. Mycoplasma lipoproteins are potent TLR2/6 agonists and we demonstrate that our reporter cells can be used as reliable and robust detection system for mycoplasma contaminations in cell cultures. In addition, a TLR4-sensitive subline of our reporters was engineered, and probed with recombinant proteins expressed in different host systems. Bacterially expressed but not mammalian expressed proteins induced strong reporter activity. We also tested proteins expressed in an E. coli strain engineered to lack TLR4 agonists. Such preparations also induced reporter activation in THP-1 cells highlighting the importance of testing recombinant protein preparations for microbial contaminations beyond endotoxins. Our results demonstrate the usefulness of monocytic reporter cells for high-throughput screening for microbial contaminations in diverse biological samples, including tissue culture supernatants and recombinant protein preparations. Fluorescent reporter assays can be measured on standard flow cytometers and in contrast to established detection methods, like luciferase-based systems or Limulus Amebocyte Lysate tests, they do not require costly reagents.
机译:先天性免疫细胞对病原体的感应对于启动适当的免疫反应至关重要。对微生物衍生的各种结构和进化保守分子高度敏感的Toll样受体(TLR)在此过程中起着重要作用。 TLR参与导致转录因子NF-κB的激活,从而诱导细胞因子和其他炎症介质的表达。 TLR信号的灵敏性可用于检测组织培养物中和蛋白制品中的细菌和微生物污染物。在这里,我们描述了用于检测生物样品中TLR配体的细胞报告系统。选择特征明确的人单核THP-1细胞系作为NF-ᴋB诱导的增强型绿色荧光蛋白报道基因的宿主。我们研究了所得报告细胞对多种微生物成分的敏感性,并观察到了对TLR1 / 2和TLR2 / 6配体的强反应性。支原体脂蛋白是有效的TLR2 / 6激动剂,我们证明了我们的报告细胞可以用作细胞培养中支原体污染的可靠而强大的检测系统。此外,我们对我们的报道分子的TLR4敏感亚系进行了工程改造,并用在不同宿主系统中表达的重组蛋白进行了探测。细菌表达而不是哺乳动物表达的蛋白诱导强烈的报道分子活性。我们还测试了在缺乏TLR4激动剂的大肠杆菌菌株中表达的蛋白质。此类制剂还诱导THP-1细胞中的报告基因激活,突出了测试重组蛋白制剂对内毒素以外的微生物污染的重要性。我们的结果证明了单核细胞报告细胞对于高通量筛选各种生物样品(包括组织培养上清液和重组蛋白制品)中微生物污染的有用性。荧光报告基因检测可以在标准的流式细胞仪上进行测量,与已建立的检测方法(例如基于荧光素酶的系统或Li变形细胞溶解试验)相比,它们不需要昂贵的试剂。

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