Variability of in vivo Sarcomere Length Measures in the Upper Limb Obtained With Second Harmonic Generation Microendoscopy

Adkins, Amy N.; Fong, Ryan M.; Dewald, Julius P. A.; Murray, Wendy M.

doi:10.3389/fphys.2021.817334

Cited by 6 publications

(2 citation statements)

References 24 publications

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“…Optical imaging is the only available tool for characterizing the sarcomeric striation pattern and the corresponding average SL, which is highly informative for understanding the functional relationships between actual SL and the contractile state of the cell ( Bub et al, 2010 ; Botcherby et al, 2013 ; Aguirre et al, 2014 ; Guo and Song, 2014 ; Pasqualin et al, 2016 ; Kobirumaki-Shimozawa et al, 2018 ; Varga et al, 2020 ; Dowrick et al, 2021 ). Recent studies have also focused on the existence of intracellular SL heterogeneity in striated muscle ( Rassier, 2017 ; Haeger et al, 2020 ; Adkins et al, 2022 ) and, importantly, its alteration upon the transition of myofilaments from the inactivated to the activated state ( Johnston et al, 2016 ; de Souza Leite et al, 2017 ; Moo et al, 2017 ; Haeger and Rassier, 2020 ; Lookin et al, 2022 ). Therefore, special care is needed to choose a proper method for SL measurements.…”

Section: Introductionmentioning

confidence: 99%

Cardiomyocyte sarcomere length variability: Membrane fluorescence versus second harmonic generation myosin imaging

Lookin

Tombe

Boulali

et al. 2023

Journal of General Physiology

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Sarcomere length (SL) and its variation along the myofibril strongly regulate integrated coordinated myocyte contraction. It is therefore important to obtain individual SL properties. Optical imaging by confocal fluorescence (for example, using ANEPPS) or transmitted light microscopy is often used for this purpose. However, this allows for the visualization of structures related to Z-disks only. In contrast, second-harmonic generation (SHG) microscopy visualizes A-band sarcomeric structures directly. Here, we compared averaged SL and its variability in isolated relaxed rat cardiomyocytes by imaging with ANEPPS and SHG. We found that SL variability, evaluated by several absolute and relative measures, is two times smaller using SHG vs. ANEPPS, while both optical methods give the same average (median) SL. We conclude that optical methods with similar optical spatial resolution provide valid estimations of average SL, but the use of SHG microscopy for visualization of sarcomeric A-bands may be the “gold standard” for evaluation of SL variability due to the absence of optical interference between the sarcomere center and non-sarcomeric structures. This contrasts with sarcomere edges where t-tubules may not consistently colocalize to Z-disks. The use of SHG microscopy instead of fluorescent imaging can be a prospective tool to map sarcomere variability both in vitro and in vivo conditions and to reveal its role in the functional behavior of living myocardium.

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Section: Introductionmentioning

confidence: 99%

Cardiomyocyte sarcomere length variability: Membrane fluorescence versus second harmonic generation myosin imaging

Lookin

Tombe

Boulali

et al. 2023

Journal of General Physiology

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“…In addition, we are aware that additional evidence from more direct characterization methods is needed to confirm the predictions of the present work regarding the contractile dynamics at the sarcomere level. We believe the microendoscopy could be helpful in this regard 75 – 77 . Beyond these considerations, the data and methods described here could be the basis to continue delving into the implications of the ligand-binding behaviors in skeletal muscle biomechanics.…”

Section: Discussionmentioning

confidence: 98%

Load sharing between synergistic muscles characterized by a ligand-binding approach and elastography

Grinspan,

Fernandes de Oliveira,

Brandao

et al. 2023

Sci Rep

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The skeletal muscle contraction is determined by cross-bridge formation between the myosin heads and the actin active sites. When the muscle contracts, it shortens, increasing its longitudinal shear elastic modulus ($${\mu }_{L}$$ μ L ). Structurally, skeletal muscle can be considered analogous to the molecular receptors that form receptor–ligand complexes and exhibit specific ligand-binding dynamics. In this context, this work aims to apply elastography and the ligand-binding framework to approach the possible intrinsic mechanisms behind muscle synergism. Based on the short-range stiffness principle and the acoustic–elasticity theory, we define the coefficient $$C$$ C , which is directly related to the fraction saturation of molecular receptors and links the relative longitudinal deformation of the muscle to its $${\mu }_{L}$$ μ L . We show that such a coefficient can be obtained directly from $${\mu }_{L}$$ μ L estimates, thus calculating it for the biceps brachii, brachioradialis, and brachialis muscles during isometric elbow flexion torque (τ) ramps. The resulting $$C\left(\tau \right)$$ C τ curves were analyzed by conventional characterization methods of receptor–ligand systems to study the dynamical behavior of each muscle. The results showed that, depending on muscle, $$C\left(\tau \right)$$ C τ exhibits typical ligand-binding dynamics during joint torque production. Therefore, the above indicates that these different behaviors describe the longitudinal shortening pattern of each muscle during load sharing. As a plausible interpretation, we suggested that this could be related to the binding kinetics of the cross-bridges during their synergistic action as torque increases. Likewise, it shows that elastography could be useful to assess contractile processes at different scales related to the change in the mechanical properties of skeletal muscle.

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Impact of stretch on sarcomere length variability in isolated fully relaxed rat cardiac myocytes

Lookin,

Boulali,

Cazorla

et al. 2023

Pflugers Arch - Eur J Physiol

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The contractility of cardiac muscle is greatly affected by preload via the Frank-Starling Mechanism (FSM). It is based on the preload-dependent activation of sarcomeres -the elementary contractile units in muscle cells. Recent ndings show a natural variability in sarcomere length (SL) in resting cardiomyocytes that, moreover, is altered in an actively contracting myocyte. SL variability may contribute to the FSM but it remains unresolved whether the change in the SL variability is regulated by activation process per se or simply by changes in cell stretch, i.e. average SL.To separate the roles of activation and SL, we characterized SL variability in isolated fully relaxed rat ventricular cardiomyocytes (n = 12) subjected to a longitudinal stretch with the carbon ber (CF) technique. Each cell was tested in three states: without CF attachment (control, no preload), with CF attachment without stretch, and with CF attachment and ~ 10% stretch of initial SL. The cells were imaged by transmitted light microscopy to retrieve and analyze individual SL and SL variability off-line by multiple quantitative measures like coe cient of variation or median absolute deviation.We found that CF attachment without stretch did not affect the extent of SL variability and averaged SL.In stretched myocytes, the averaged SL signi cantly increased while the SL variability remained unchanged. This result clearly indicates that the non-uniformity of individual SL is not sensitive to the average SL itself in fully relaxed myocytes. We conclude that SL variability per se does not contribute to the FSM in the heart.

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Variability of in vivo Sarcomere Length Measures in the Upper Limb Obtained With Second Harmonic Generation Microendoscopy

Cited by 6 publications

References 24 publications

Cardiomyocyte sarcomere length variability: Membrane fluorescence versus second harmonic generation myosin imaging

Cardiomyocyte sarcomere length variability: Membrane fluorescence versus second harmonic generation myosin imaging

Load sharing between synergistic muscles characterized by a ligand-binding approach and elastography

Impact of stretch on sarcomere length variability in isolated fully relaxed rat cardiac myocytes

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