Figure 3.
Figure 3. MyD88L265P transferred by the EVs forms aggregates with endogenous MyD88 in the recipient cells. (A) EVL265P-CFP (cyan) were isolated and added (5 μg/mL) to the HEK293 cells for 16 hours. Cell membranes were dyed with CT-B Alexa 647 (magenta). (B,D) HEK293 and HEK293 MyD88KO cells were transfected with MyD88wt-YFP (magenta) or (C) left untreated. After 4 hours, EVL265P-CFP (cyan) or EVL265P-YFP (magenta) (both 5 μg/mL) were added for 16 hours. Confocal imaging was performed. Bar for all images, 10 μm. (E) HEK293 and HEK293 MyD88KO cells expressing luciferase under NF-κB promotor and Renilla luciferase for normalization were stimulated with EVL265P (12 μg/mL) for 24 hours. Negative controls are transfected but unstimulated cells. Dual luciferase test for NF-κB activity was performed.

MyD88L265Ptransferred by the EVs forms aggregates with endogenous MyD88 in the recipient cells. (A) EVL265P-CFP (cyan) were isolated and added (5 μg/mL) to the HEK293 cells for 16 hours. Cell membranes were dyed with CT-B Alexa 647 (magenta). (B,D) HEK293 and HEK293 MyD88KO cells were transfected with MyD88wt-YFP (magenta) or (C) left untreated. After 4 hours, EVL265P-CFP (cyan) or EVL265P-YFP (magenta) (both 5 μg/mL) were added for 16 hours. Confocal imaging was performed. Bar for all images, 10 μm. (E) HEK293 and HEK293 MyD88KO cells expressing luciferase under NF-κB promotor and Renilla luciferase for normalization were stimulated with EVL265P (12 μg/mL) for 24 hours. Negative controls are transfected but unstimulated cells. Dual luciferase test for NF-κB activity was performed.

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