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Myofibrillar degeneration with diphtheria toxin
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Abstract
Objectives
Cardiac damage in patient with diphtheritic myocarditis is reported as the leading cause of mortality. Diphtheria toxin (DTx) is a well-known bacterial toxin inducing various cytotoxic effects. Mainly, catalytic fragment inhibits protein synthesis, induces cytotoxicity, and depolymerizes actin filaments. In this study, we aimed to demonstrate the extent of myofibrillar damage under DTx treatment to porcine cardiac tissue samples.
Methods
Tissue samples were incubated with DTx for 1–3 h in culture conditions. To analyze whole toxin (both fragments) distribution, conjugation of DTx with FITC was performed. Measurements were carried out with fluorescence spectrophotometer before and after dialysis. Immunofluorescence microscopy was used to show localization of DTx-FITC (15 nM) on cardiac tissue incubated for 2 h. Ultrastructural characterization of cardiac tissue samples treated with DTx (15 or 150 nM) was performed with transmission electron microscopy.
Results
DTx exerts myofibrillar disorganization. Myofilament degeneration, mitochondrial damage, vacuolization, and abundant lipid droplets were determined with 150 nM of DTx treatment.
Conclusions
This finding is an addition to depolymerization of actin filaments as a result of the DTx-actin interactions in
in vitro
conditions, indicating that myofilament damage can occur with DTx directly besides protein synthesis inhibition. Ultrastructural results support the importance of filamentous actin degeneration at diphtheritic myocarditis.
Walter de Gruyter GmbH
Title: Myofibrillar degeneration with diphtheria toxin
Description:
Abstract
Objectives
Cardiac damage in patient with diphtheritic myocarditis is reported as the leading cause of mortality.
Diphtheria toxin (DTx) is a well-known bacterial toxin inducing various cytotoxic effects.
Mainly, catalytic fragment inhibits protein synthesis, induces cytotoxicity, and depolymerizes actin filaments.
In this study, we aimed to demonstrate the extent of myofibrillar damage under DTx treatment to porcine cardiac tissue samples.
Methods
Tissue samples were incubated with DTx for 1–3 h in culture conditions.
To analyze whole toxin (both fragments) distribution, conjugation of DTx with FITC was performed.
Measurements were carried out with fluorescence spectrophotometer before and after dialysis.
Immunofluorescence microscopy was used to show localization of DTx-FITC (15 nM) on cardiac tissue incubated for 2 h.
Ultrastructural characterization of cardiac tissue samples treated with DTx (15 or 150 nM) was performed with transmission electron microscopy.
Results
DTx exerts myofibrillar disorganization.
Myofilament degeneration, mitochondrial damage, vacuolization, and abundant lipid droplets were determined with 150 nM of DTx treatment.
Conclusions
This finding is an addition to depolymerization of actin filaments as a result of the DTx-actin interactions in
in vitro
conditions, indicating that myofilament damage can occur with DTx directly besides protein synthesis inhibition.
Ultrastructural results support the importance of filamentous actin degeneration at diphtheritic myocarditis.
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