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Image Search Results
Journal: bioRxiv
Article Title: Phase Separation-based Antiviral Decoy Particles as Basis for Programmable Broad-spectrum Therapeutics
doi: 10.1101/2024.08.28.610020
Figure Lengend Snippet: (A) Scheme of assay: ACE2 labelled with an mCherry fluorescent protein and fused to tdPCP is incubated with a slncRNA cassette, encoding for multiple PCP-binding hairpins. 1h post incubation, an sfGFP-labelled RBD is added, facilitating FRET with the mCherry-labelled ACE2 proteins bound to the slncRNA granules. (B) (Left) Representative image of ACE2 granules in a typical field of view. Scalebar: 5µm. (Right) Enlarged images highlighted by white squares on the left. (Right-top) protein only condensate. (Right-bottom) An sRNP granule of protein co-localized with slncRNA. Scalebar for enlarged images 1µm and 2µm for top and bottom, respectively. (C) Correlation between mCherry and AF405 signals intensities of 339 mCherry-positive events. Representative events – see 1 and 2 from panel B and Supplementary Figure 2A. (D) (Left) Representative image of ACE granules together with RBD (green label). Scalebar: 5µm. (Right) Enlarged images highlighted by white squares on the left showing typical triple labelled structures. Scalebar: 5µm. (E-F) FRET intensity signal (E) and FRET efficiency (F) measured for the highlighted granule structures shown in . ( G) Putative green-red FRET excitation events obtained for various RBD concentrations. (H-I) (Left) Images of triple-labelled granules, FRET intensity and FET efficiency, and (right) putative intensity of FRET excitation events obtained for the non-dimerizing ACE2 (Δ616-726) (h) and the non-RBD-binding missense ACE2 mutant (D355A) (I).
Article Snippet: The enzyme was then heat-inactivated by incubating the restriction reaction at 65 °C for 20 min. For fluorescently labeled RNA, 1µg of the restriction product was used as template for in vitro transcription using
Techniques: Incubation, Binding Assay, Mutagenesis
Journal: bioRxiv
Article Title: Phase Separation-based Antiviral Decoy Particles as Basis for Programmable Broad-spectrum Therapeutics
doi: 10.1101/2024.08.28.610020
Figure Lengend Snippet: (A) Predicted AlphaFold structure for LAMP1-mCherry-tdPCP. Black, red, and green are LAMP1, mCherry, and tdPCP, respectively. Putative sialylation sites are marked by light-blue shading (asparagine residues in an N-X-S/T motif), yellow (serine residue), and magenta (threonine residue). (B) Typical field-of-view of SNA-LAMP1 granule biocondensate divided into the individual channels. (Top-left) protein (mCherry). (Top-right) SNA (AF488). (Bottom-left) slncRNA (AF405). (Bottom-right) Merged panel with all three images overlayed. (Top-set) No SNA added (scalebar: 5µm FoV, 1µm enlargement). (Bottom-set) High SNA concentration (scalebar: 5µm). (C) Box-plot distributions for D RNA for each candidate sialoprotein. The mean of each distribution is marked by red circle. Low and high SNA concentrations were set at below 1µg/ml (molar ratio of ∼1 SNA : 50 sialoproteins) and above 50µg/ml (molar ratio of ∼3 SNA : 2 sialoproteins), respectively. (D) Plot showing ΔD avg as a function of putative sialylated sited. ΔD avg is defined as the difference between the high and low mean D RNA values obtained for each protein in panel C. Color and size of dot correspond to the student t-test p-value computed for each panel in .
Article Snippet: The enzyme was then heat-inactivated by incubating the restriction reaction at 65 °C for 20 min. For fluorescently labeled RNA, 1µg of the restriction product was used as template for in vitro transcription using
Techniques: Residue, Concentration Assay
Journal: bioRxiv
Article Title: Phase Separation-based Antiviral Decoy Particles as Basis for Programmable Broad-spectrum Therapeutics
doi: 10.1101/2024.08.28.610020
Figure Lengend Snippet: (A) Typical field-of-view of SNA-LAMP1 granule biocondensate divided into individual channels. (Top-left) protein (mCherry). (Top-right) SNA (AF488). (Bottom-left) slncRNA (AF405). (Bottom-right) Merged panel with all three images overlayed. Scalebar: 5µm. (B) Close-up on the two features highlighted in panel a displayed via the same three separated channels and merged image. Scalebar: 5μm. (C) LAMP1 dose-response curves for RNA-displacement (blue), SNA binding to protein (green), and triple colocalized biocondensate structures (purple). (Left) decision tree used to classify the different structures. (D) Dose responses (see Supplementary Figure S7B) displayed as a normalized heatmap for SNA binding (top) and RNA displacement (bottom). Each row was normalized by its maximum value. (E) Plot of the combined agglutination score for each candidate sialoprotein as a function of the number of putative sialylation site showing a strong linear dependence. Each score is the summation of three separate values: ΔD RNA, ΔΔG SNA binding , and ΔΔG RNA displacement (see methods and text for definitions).
Article Snippet: The enzyme was then heat-inactivated by incubating the restriction reaction at 65 °C for 20 min. For fluorescently labeled RNA, 1µg of the restriction product was used as template for in vitro transcription using
Techniques: Binding Assay, Agglutination
Journal: Frontiers in Immunology
Article Title: An RNA vaccine against adrenomedullin reduces angiogenesis and tumor burden in a syngeneic metastatic melanoma mouse model
doi: 10.3389/fimmu.2025.1604156
Figure Lengend Snippet: Representative confocal images of LNPs containing unlabeled mRNA (control) or Cy5-labeled mRNA that were added to a culture of RAW 264.7 macrophages. A cytoplasmic red staining can be seen in some macrophages exposed to the labeled LNPs. Scale bar = 20 µm.
Article Snippet: The KLH-AM mRNA was labeled with the
Techniques: Control, Labeling, Staining
Journal: bioRxiv
Article Title: Evaluation of dsRNA delivery methods for targeting macrophage migration inhibitory factor MIF in RNAi-based aphid control
doi: 10.1101/2021.02.24.432707
Figure Lengend Snippet: Confocal images of detached barley leaves having absorbed fluorescence-labeled SaMIF1 -dsRNA A488 through cut basal ends. The leaf base was submerged in 1 mL of 200 mM sucrose solution containing 20 µg dsRNA. Surface views of a , leaf base; b , leaf segment 2 cm away from the base at 24 h after onset of soaking. c , leaf segment 5 cm from the base 48 h after onset of soaking. d-g , leaf cross-section (3 cm from the cutting), photographs taken at three days after onset of the SaMIF1 -dsRNA A488 treatment. The green color represents the fluorescence (λ exc 494, λ em 515 nm) of the Alexa Flour 488 (AF488) dye. xy, xylem; ph, phloem; bs, bundle sheath.
Article Snippet: Fluorescence labeling of SaMIF1 -dsRNA was performed using the
Techniques: Fluorescence, Labeling