Quantifying Muscle Fiber Damage

PM injury following LC-induced injury was assessed as before (Vila et al., 2017 (link)) using PO dye, which is excluded from myofibers with intact sarcolemma. Immediately after the LC assay, muscles were trimmed of tendons, blotted, weighed, and then incubated while held at L_o in a 0.2% PO solution at room temperature for 30 min, washed in Ringer solution, and quickly frozen in isopentane prechilled with liquid nitrogen. Frozen cross sections of 10-µm thickness were cut, mounted with fluorescent mounting medium (DAKO), and viewed under a fluorescent microscope to identify the presence of PO. Fields, containing the majority of the muscle cross sections were photographed and scaled under identical conditions at ×10 magnification using Olympus BX61 widefield microscope. By thresholding for unstained muscle, we identified fibers that showed no uptake of PO from fibers that showed PO uptake. From each muscle cross section, the area occupied by PO-labeled fibers ranging from minimal to maximal dye uptake was measured and expressed as a percentage of the complete muscle section area. PO-labeled fibers at the edges of the sections were considered as artifact and were excluded from analysis.

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Chandra G., Sreetama S.C., Mázala D.A., Charton K., VanderMeulen J.H., Richard I, & Jaiswal J.K. (2021). Endoplasmic reticulum maintains ion homeostasis required for plasma membrane repair. The Journal of Cell Biology, 220(5), e202006035.

Publication 2021

fluorescent mounting medium BX61 widefield microscope

Assay Frozen Frozen sections Held Injury Isopentane Microscope Muscle Nitrogen Ringer solution Sarcolemma Tendons

Corresponding Organization :

Other organizations : Children's National, Genethon (France), Inserm, Georgetown University, George Washington University

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Variable analysis

independent variables

Injury condition: LC-induced injury

dependent variables

PM injury following LC-induced injury
Area occupied by PO-labeled fibers ranging from minimal to maximal dye uptake as a percentage of the complete muscle section area

control variables

L_o condition: Muscles were held at L_o during incubation in PO solution
PO solution concentration: 0.2%
Incubation time: 30 minutes
Temperature: Room temperature
Muscle trimming: Tendons were trimmed off
Muscle sectioning: Frozen cross sections of 10-µm thickness were cut
Imaging conditions: Fields containing the majority of the muscle cross sections were photographed under identical conditions at ×10 magnification using Olympus BX61 widefield microscope

controls

Positive control: Not explicitly mentioned
Negative control: Not explicitly mentioned

Annotations

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