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Quantification of nanoscale forces in lectin-mediated bacterial attachment and uptake into giant liposomes

机译:量化的纳米级部队lectin-mediated细菌吸附和吸收成巨大的脂质体

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摘要

Interactions of the bacterial lectin LecA with the host cells glycosphingolipid Gb3 have been shown to be crucial for the cellular uptake of the bacterium Pseudomonas aeruginosa. LecA-induced Gb3 clustering, referred to as lipid zipper mechanism, leads to full membrane engulfment of the bacterium. Here, we aim for a nanoscale force characterization of this mechanism using two complementary force probing techniques, atomic force microscopy (AFM) and optical tweezers (OT). The LecA-Gb3 interactions are reconstituted using giant unilamellar vesicles (GUVs), a well-controlled minimal system mimicking the plasma membrane and nanoscale forces between either bacteria (PAO1 wild-type and LecA-deletion mutant strains) or LecA-coated probes (as minimal, synthetic bacterial model) and vesicles are measured. Lec-AGb3 interactions strengthen the bacterial attachment to the membrane (1.5-8-fold) depending on the membrane tension and the applied technique. Moreover, significantly less energy (reduction up to 80%) is required for the full uptake of LecA-coated beads into Gb3-functionalized vesicles. This quantitative approach highlights that lectin-glycolipid interactions provide adequate forces and energies to drive bacterial attachment and uptake.
机译:的细菌凝集素LecA的交互宿主细胞鞘糖脂Gb3已被证明为细胞的吸收至关重要细菌铜绿假单胞菌。Gb3集群,称为脂质拉链机制,导致膜吞没这种细菌。使用两个特征的机制互补力探测技术,原子力显微镜(AFM)和光学镊子(OT)。重组使用的LecA-Gb3交互巨大的单膜囊泡(爸爸),严格的最小系统模仿质膜和纳米级部队之间细菌(PAO1野生型和LecA-deletion突变株)或LecA-coated探测器(如最小的,合成细菌模型)和囊泡测量。细菌附着膜(1.5 8番)根据膜张力和应用技术。大大减少能源(减少80%)需要的全部吸收LecA-coated吗珠子Gb3-functionalized囊泡。定量方法强调lectin-glycolipid交互提供足够的力量和能量来驱动细菌附件和吸收。

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