Single-molecule displacement mapping unveils nanoscale heterogeneities in intracellular diffusivity

Xiang, Limin; Chen, Kun; Yan, Rui; Li, Wan; Xu, Ke

doi:10.1038/s41592-020-0793-0

Cited by 90 publications

(196 citation statements)

References 48 publications

(57 reference statements)

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“…Our results, presented in Figure 2 , were compared to measurements reported by other groups. 10 , 13 , 30 , 38 − 40 The results of the comparison are shown in SI5 ( Figure SI5 ). In general, our results are in good agreement with scattered data reported by other groups, with mismatches that could be attributed to different methods of measurements.…”

Section: Length-scale Dependent Viscosity Of Cytoplasmmentioning

confidence: 99%

Nanoscale Viscosity of Cytoplasm Is Conserved in Human Cell Lines

Kwapiszewska

Szczepański

Kalwarczyk

et al. 2020

J. Phys. Chem. Lett.

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Metabolic reactions in living cells are limited by diffusion of reagents in the cytoplasm. Any attempt to quantify the kinetics of biochemical reactions in the cytosol should be preceded by careful measurements of the physical properties of the cellular interior. The cytoplasm is a complex, crowded fluid characterized by effective viscosity dependent on its structure at a nanoscopic length scale. In this work, we present and validate the model describing the cytoplasmic nanoviscosity, based on measurements in seven human cell lines, for nanoprobes ranging in diameters from 1 to 150 nm. Irrespective of cell line origin (epithelial–mesenchymal, cancerous–noncancerous, male–female, young–adult), we obtained a similar dependence of the viscosity on the size of the nanoprobes, with characteristic length-scales of 20 ± 11 nm (hydrodynamic radii of major crowders in the cytoplasm) and 4.6 ± 0.7 nm (radii of intercrowder gaps). Moreover, we revealed that the cytoplasm behaves as a liquid for length scales smaller than 100 nm and as a physical gel for larger length scales.

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Section: Length-scale Dependent Viscosity Of Cytoplasmmentioning

confidence: 99%

Nanoscale Viscosity of Cytoplasm Is Conserved in Human Cell Lines

Kwapiszewska

Szczepański

Kalwarczyk

et al. 2020

J. Phys. Chem. Lett.

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“…The heterogeneous molecular transport velocities inside cells should be modulated by the local viscosity and diffusivity related to intracellular structures and microenvironments [36] . Because the distribution of actin cytoskeleton bundles largely determines the local viscosity and diffusivity at different parts of a single cell, [36] we used confocal fluorescence microscopy to image actin bundles by an FITC‐tagged phalloidin stain (Figure S19) [36, 37] . The fluorescence image shows that the actin cytoskeleton networks bridge the cell nucleus to the plasma membrane across the cytoplasm, and finally converge on the nucleus.…”

Section: Resultsmentioning

confidence: 99%

Bio‐Coreactant‐Enhanced Electrochemiluminescence Microscopy of Intracellular Structure and Transport

Zhou

et al. 2021

Angewandte Chemie

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A bio‐coreactant‐enhanced electrochemiluminescence (ECL) microscopy realizes the ECL imaging of intracellular structure and dynamic transport. This microscopy uses Ru(bpy)32+ as the electrochemical molecular antenna connecting extracellular and intracellular environments, and uses intracellular biomolecules as the coreactants of ECL reactions via a “catalytic route”. Accordingly, intracellular structures are identified without using multiple labels, and autophagy involving DNA oxidative damage is detected using nuclear ECL signals. A time‐resolved image sequence discloses the universal edge effect of cellular electroporation due to the influence of the geometric properties of cell membranes on the induced transmembrane voltage. The dynamic transport of Ru(bpy)33+ in the different cellular compartments unveils the heterogeneous intracellular diffusivity correlating with the actin cytoskeleton. In addition to single‐cell studies, the bio‐coreactant‐enhanced ECL microscopy is used to image a slice of a mouse liver and a colony of Shewanella oneidensis MR‐1.

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“…), or a large aggregate (> 500 a.u.). A similar approach has been previously used to quantify membrane receptors via calibrated QD intensities (41). Fig.…”

Section: Resultsmentioning

confidence: 99%

Visualizing the cytosolic delivery of bioconjugated QDs into T cell lymphocytes

Jing

Pálmai

Saed

et al. 2020

Preprint

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The aggregation state and endosomal trapping of engineered nanocarriers once internalized into cells remain poorly characterized. Here, we visualized the membrane penetrating dynamics of semiconductor quantum dots (QDs) into the cytosol of T cells on a single-cell and single-nanoparticle basis. We water solubilized CdSe/CdZnS QDs with polymer encapsulants functionalized with a cell-penetrating peptide composed of an Asp-Ser-Ser (DSS) repeat sequence. T cells tolerated the 24-h incubation with QDs at concentrations of 5 nM or lower. Single-particle imaging demonstrated that the number of internalized nanoparticles was dependent upon the concentration of the probes for both control (peptide-free) and DSS-QDs. DSS-QDs were mostly distributed as monomers, whereas the control QDs were aggregated into clusters. Single-particle tracking using total internal reflection and highly inclined illumination showed that DSS-QDs were stationary near the activating surface and mobile within the cytosol of the T cell. A correlation exhibited between the mobility and aggregation state of individual QD clusters, with monomeric DSS-QDs showing the highest mobility. In addition, monomeric DSS-QDs displayed much faster diffusion than the endosomes. A small-molecule endosome marker confirmed the absence of colocalization between endosomes and DSS-QDs, indicating their endosomal escape. The ability to deliver and track individual QDs in the cytosol of live T cells creates inroads for the optimization of drug delivery and gene therapy through the use of nanoparticles.

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Single-molecule displacement mapping unveils nanoscale heterogeneities in intracellular diffusivity

Cited by 90 publications

References 48 publications

Nanoscale Viscosity of Cytoplasm Is Conserved in Human Cell Lines

Nanoscale Viscosity of Cytoplasm Is Conserved in Human Cell Lines

Bio‐Coreactant‐Enhanced Electrochemiluminescence Microscopy of Intracellular Structure and Transport

Visualizing the cytosolic delivery of bioconjugated QDs into T cell lymphocytes

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