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Single-Molecule Detection of Protein Efflux from Microorganisms using Fluorescent Single Walled Carbon Nanotube Sensor Arrays

机译:使用荧光单壁碳纳米管传感器阵列从微生物中单分子检测蛋白质流出。

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摘要

A distinct advantage of nanosensor arrays is their ability to achieve ultra-low detection limits in solution by proximity placement to an analyte. Here, we demonstrate label-free detection of individual proteins from Escherichia coli (bacteria) and Pichia pastoris (yeast) immobilized in a microfluidic chamber, measuring protein efflux from single organisms in real time. The array is fabricated using non-covalent conjugation of an aptamer-anchor polynucleotide sequence to near-infrared emissive single-walled carbon nanotubes, using a variable chemical spacer shown to optimize sensor response. Unlabeled RAP1 GTPase and HIV integrase proteins were selectively detected from various cell lines, via large near-infrared fluorescent turn-on responses. We show the process of E. coli induction, protein synthesis, and protein export is highly stochastic, yielding variability in protein secretion, with E. coli cells undergoing division under starved conditions producing 66% fewer secreted protein products than their non-dividing counterparts. We further demonstrate the detection of a unique protein product resulting from T7 bacteriophage infection of E. coli, illustrating that nanosensor arrays can enable real-time, single-cell analysis of a broad range of protein products from various cell types.
机译:纳米传感器阵列的显着优势是它们能够通过与分析物接近放置而在溶液中实现超低检测限。在这里,我们展示了来自固定在微流控室中的大肠杆菌(细菌)和巴斯德毕赤酵母(酵母)的单个蛋白质的无标签检测,可实时测量单个生物体的蛋白质流出。使用适配体-锚定多核苷酸序列与近红外发射单壁碳纳米管的非共价缀合来制造阵列,并使用所示的可变化学间隔基来优化传感器响应。通过大的近红外荧光开启响应,从各种细胞系中选择性地检测到未标记的RAP1 GTPase和HIV整合酶蛋白。我们表明,大肠杆菌的诱导,蛋白质合成和蛋白质输出过程是高度随机的,在蛋白质分泌方面产生差异,大肠杆菌细胞在饥饿条件下进行分裂产生的分泌蛋白质产物比未分裂的同类细胞少66%。我们进一步证明了对大肠杆菌T7噬菌体感染产生的独特蛋白质产物的检测,表明纳米传感器阵列可以实现对来自各种细胞类型的多种蛋白质产物的实时单细胞分析。

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