Differences in L-type Ca<sup>2+</sup> channel activity partially underlie the regional dichotomy in pumping behavior by murine peripheral and visceral lymphatic vessels

Zawieja, Scott D.; Castorena‐Gonzalez, Jorge A.; Scallan, Joshua P.; Davis, Michael J.

doi:10.1152/ajpheart.00499.2017

Cited by 67 publications

(136 citation statements)

References 59 publications

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“…This includes the extreme case in most strains of mice, in which phasic contractions are so weak as to appear absent. Notably, the regional differences in the strength of lymphatic contractions in mice is related to differences in the activity of L-type Ca 2+ channels (1202). …”

Section: Lymphangions and The Lymphatic Pump Mechanismmentioning

confidence: 99%

Lymphatic Vessel Network Structure and Physiology

Breslin

Yang

Scallan

et al. 2018

Comprehensive Physiology

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The lymphatic system is comprised of a network of vessels interrelated with lymphoid tissue, which has the holistic function to maintain the local physiologic environment for every cell in all tissues of the body. The lymphatic system maintains extracellular fluid homeostasis favorable for optimal tissue function, removing substances that arise due to metabolism or cell death, and optimizing immunity against bacteria, viruses, parasites, and other antigens. This article provides a comprehensive review of important findings over the past century along with recent advances in the understanding of the anatomy and physiology of lymphatic vessels, including tissue/organ specificity, development, mechanisms of lymph formation and transport, lymphangiogenesis, and the roles of lymphatics in disease.

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Section: Lymphangions and The Lymphatic Pump Mechanismmentioning

confidence: 99%

Lymphatic Vessel Network Structure and Physiology

Breslin

Yang

Scallan

et al. 2018

Comprehensive Physiology

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263

258

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“…A segment of an excised lymphatic vessel containing at least one valve was transferred to a 3-mL chamber where it was cannulated onto two micropipettes and pressurized to 3 cmH 2 O. The bath solution containing Krebs buffer was exchanged at a rate of 0.5 mL/min and equilibrated for 30-60 minutes, at 37 °C, as previously described 52 . The inner diameter was tracked continuously from video images using a digital edge-detection method 54 .…”

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confidence: 99%

T-type, but not L-type, voltage-gated calcium channels are dispensable for lymphatic pacemaking and spontaneous contractions

Gui

et al. 2020

Sci Rep

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the spontaneous contractions of collecting lymphatic vessels provide an essential propulsive force to return lymph centrally. these contractions are driven by an intrinsic electrical pacemaker, working through an unknown underlying ionic mechanism that becomes compromised in some forms of lymphedema. in previous studies, t-type voltage-gated ca 2+ channels (VGccs) were implicated in this pacemaking mechanism, based on the effects of the reputedly selective T-type VGCC inhibitors mibefradil and ni 2+. Our goal was to test this idea in a more definitive way using genetic knock out mice. first, we demonstrated through both pcR and immunostaining that mouse lymphatic muscle cells expressed ca v 3.1 and Ca v 3.2 and produced functional T-type VGCC currents when patch clamped. We then employed genetic deletion strategies to selectively test the roles of each t-type VGcc isoform in the regulation of lymphatic pacemaking. Surprisingly, global deletion of either, or both, isoform(s) was without significant effect on either the frequency, amplitude, or fractional pump flow of lymphatic collectors from two different regions of the mouse, studied ex vivo. further, both Wt and ca v 3.1 −/− ; 3.2 −/− double knockout lymphatic vessels responded similarly to mibefradil and ni 2+ , which substantially reduced contraction amplitudes and slightly increased frequencies at almost all pressures in both strains: a pattern consistent with inhibition of L-type rather than t-type VGccs. Neither T-type VGCC isoform was required for ACh-induced inhibition of contraction, a mechanism by which those channels in smooth muscle are thought to be targets of endothelium-derived nitric oxide. Sharp intracellular electrode measurements in lymphatic smooth muscle revealed only subtle, but not significant, differences in the resting membrane potential and action potential characteristics between vessels from wild-type and ca v 3.1 −/− ; 3.2 −/− double knockout mice. in contrast, smoothmuscle specific deletion of the L-type VGCC, Ca v 1.2, completely abolished all lymphatic spontaneous contractions. collectively our results suggest that, although t-type VGccs are expressed in mouse lymphatic smooth muscle, they do not play a significant role in modulating the frequency of the ionic pacemaker or the amplitude of spontaneous contractions. We conclude that the effects of mibefradil and ni 2+ in other lymphatic preparations are largely or completely explained by off-target effects on L-type VGCCs, which are essential for controlling both the frequency and strength of spontaneous contractions. The spontaneous contractions of collecting lymphatic vessels propel lymph centrally to account for 2/3 of peripheral lymph flow 1,2. These rapid, large-amplitude contractions are analogous to twitch contractions of cardiac and skeletal muscle and are particularly important for moving lymph uphill against the adverse hydrostatic gradients that exist in dependent extremities. Lymphatic contractions are triggered by action potentials (APs) in lymphatic smooth muscle cell...

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“…Mesenteric lymphatic vessels were isolated as previously described Scallan et al 2016;Zawieja et al 2017;Castorena-Gonzalez et al 2018a,b;Zawieja et al 2018). Each vessel was pinned down with short segments of 40 µm stainless steel wire onto the Sylgard-coated surface of a dissection chamber filled with BSA containing Krebs buffer at room temperature.…”

Section: Vessel Isolation Pressure Myography and Data Acquisitionmentioning

confidence: 99%

Simplified method to quantify valve back‐leak uncovers severe mesenteric lymphatic valve dysfunction in mice deficient in connexins 43 and 37

Castorena‐Gonzalez

Srinivasan

King

et al. 2020

The Journal of Physiology

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Key points Lymphatic valve defects are one of the major causes of lymph transport dysfunction; however, there are no accessible methods for quantitatively assessing valve function. This report describes a novel technique for quantifying lymphatic valve back‐leak. Postnatal endothelial‐specific deletion of connexin 43 (Cx43) in connexin 37 null (Cx37−/−) mice results in rapid regression of valve leaflets and severe valve dysfunction. This method can also be used for assessing the function of venous and lymphatic valves from various species, including humans. Abstract The lymphatic system relies on robust, spontaneous contractions of collecting lymphatic vessels and one‐way secondary lymphatic valves to efficiently move lymph forward. Secondary valves prevent reflux and allow for the generation of propulsive pressure during each contraction cycle. Lymphatic valve defects are one of the major causes of lymph transport dysfunction. Genetic mutations in multiple genes have been associated with the development of primary lymphoedema in humans; and many of the same mutations in mice result in valve defects that subsequently lead to chylous ascites or chylothorax. At present the only experimental technique for the quantitative assessment of lymphatic valve function utilizes the servo‐null micropressure system, which is highly accurate and precise, but relatively inaccessible and difficult to use. We developed a novel, simplified alternative method for quantifying valve function and determining the degree of pressure back‐leak through an intact valve in pressurized, single‐valve segments of isolated lymphatic vessels. With this diameter‐based method, the competence of each lymphatic valve is challenged over a physiological range of pressures (e.g. 0.5–10cmH2O) and pressure back‐leak is extrapolated from calibrated, pressure‐driven changes in diameter upstream from the valve. Using mesenteric lymphatic vessels from C57BL/6J, Ub‐CreERT2;Rasa1fx/fx, Foxc2Cre/+, Lyve1‐Cre;Cx43fx/fx, and Prox1‐CreERT2;Cx43fx/fx;Cx37−/− mice, we tested our method on lymphatic valves displaying a wide range of dysfunction, from fully competent to completely incompetent. Our results were validated by simultaneous direct measurement of pressure back‐leak using a servo‐null micropressure system. Our diameter‐based technique can be used to quantify valve function in isolated lymphatic valves from a variety of species. This method also revealed that haplodeficiency in Foxc2 (Foxc2Cre/+) is not sufficient to cause significant valve dysfunction; however, postnatal endothelial‐specific deletion of Cx43 in Cx37−/− mice results in rapid regression of valve leaflets and severe valve dysfunction.

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Differences in L-type Ca²⁺ channel activity partially underlie the regional dichotomy in pumping behavior by murine peripheral and visceral lymphatic vessels

Cited by 67 publications

References 59 publications

Lymphatic Vessel Network Structure and Physiology

Lymphatic Vessel Network Structure and Physiology

T-type, but not L-type, voltage-gated calcium channels are dispensable for lymphatic pacemaking and spontaneous contractions

Simplified method to quantify valve back‐leak uncovers severe mesenteric lymphatic valve dysfunction in mice deficient in connexins 43 and 37

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Differences in L-type Ca2+ channel activity partially underlie the regional dichotomy in pumping behavior by murine peripheral and visceral lymphatic vessels

Cited by 67 publications

References 59 publications

Lymphatic Vessel Network Structure and Physiology

Lymphatic Vessel Network Structure and Physiology

T-type, but not L-type, voltage-gated calcium channels are dispensable for lymphatic pacemaking and spontaneous contractions

Simplified method to quantify valve back‐leak uncovers severe mesenteric lymphatic valve dysfunction in mice deficient in connexins 43 and 37

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Differences in L-type Ca²⁺ channel activity partially underlie the regional dichotomy in pumping behavior by murine peripheral and visceral lymphatic vessels