Calcium-vesicles perform active diffusion in the sea urchin embryo during larval biomineralization.

Calcium-vesicles perform active diffusion in the sea urchin embryo during larval biomineralization.

Biomineralization is the process by which organisms use minerals to harden their tissues and provide them with physical support. Biomineralizing cells concentrate the mineral in vesicles that they secret into a dedicated compartment where crystallization occurs. The dynamics of vesicle motion and th...

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Main Authors: Mark R Winter, Miri Morgulis, Tsvia Gildor, Andrew R Cohen, Smadar Ben-Tabou de-Leon
Format: Article
Language:English
Published: Public Library of Science (PLoS) 2021-02-01
Series:PLoS Computational Biology
Online Access:https://doi.org/10.1371/journal.pcbi.1008780
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spelling doaj-ea482918279748aeb723f305b6c2e1892021-07-09T04:31:59ZengPublic Library of Science (PLoS)PLoS Computational Biology1553-734X1553-73582021-02-01172e100878010.1371/journal.pcbi.1008780Calcium-vesicles perform active diffusion in the sea urchin embryo during larval biomineralization.Mark R WinterMiri MorgulisTsvia GildorAndrew R CohenSmadar Ben-Tabou de-LeonBiomineralization is the process by which organisms use minerals to harden their tissues and provide them with physical support. Biomineralizing cells concentrate the mineral in vesicles that they secret into a dedicated compartment where crystallization occurs. The dynamics of vesicle motion and the molecular mechanisms that control it, are not well understood. Sea urchin larval skeletogenesis provides an excellent platform for investigating the kinetics of mineral-bearing vesicles. Here we used lattice light-sheet microscopy to study the three-dimensional (3D) dynamics of calcium-bearing vesicles in the cells of normal sea urchin embryos and of embryos where skeletogenesis is blocked through the inhibition of Vascular Endothelial Growth Factor Receptor (VEGFR). We developed computational tools for displaying 3D-volumetric movies and for automatically quantifying vesicle dynamics. Our findings imply that calcium vesicles perform an active diffusion motion in both, calcifying (skeletogenic) and non-calcifying (ectodermal) cells of the embryo. The diffusion coefficient and vesicle speed are larger in the mesenchymal skeletogenic cells compared to the epithelial ectodermal cells. These differences are possibly due to the distinct mechanical properties of the two tissues, demonstrated by the enhanced f-actin accumulation and myosinII activity in the ectodermal cells compared to the skeletogenic cells. Vesicle motion is not directed toward the biomineralization compartment, but the vesicles slow down when they approach it, and probably bind for mineral deposition. VEGFR inhibition leads to an increase of vesicle volume but hardly changes vesicle kinetics and doesn't affect f-actin accumulation and myosinII activity. Thus, calcium vesicles perform an active diffusion motion in the cells of the sea urchin embryo, with diffusion length and speed that inversely correlate with the strength of the actomyosin network. Overall, our studies provide an unprecedented view of calcium vesicle 3D-dynamics and point toward cytoskeleton remodeling as an important effector of the motion of mineral-bearing vesicles.https://doi.org/10.1371/journal.pcbi.1008780
collection DOAJ
language English
format Article
sources DOAJ
author Mark R Winter
Miri Morgulis
Tsvia Gildor
Andrew R Cohen
Smadar Ben-Tabou de-Leon
spellingShingle Mark R Winter
Miri Morgulis
Tsvia Gildor
Andrew R Cohen
Smadar Ben-Tabou de-Leon
Calcium-vesicles perform active diffusion in the sea urchin embryo during larval biomineralization.
PLoS Computational Biology
author_facet Mark R Winter
Miri Morgulis
Tsvia Gildor
Andrew R Cohen
Smadar Ben-Tabou de-Leon
author_sort Mark R Winter
title Calcium-vesicles perform active diffusion in the sea urchin embryo during larval biomineralization.
title_short Calcium-vesicles perform active diffusion in the sea urchin embryo during larval biomineralization.
title_full Calcium-vesicles perform active diffusion in the sea urchin embryo during larval biomineralization.
title_fullStr Calcium-vesicles perform active diffusion in the sea urchin embryo during larval biomineralization.
title_full_unstemmed Calcium-vesicles perform active diffusion in the sea urchin embryo during larval biomineralization.
title_sort calcium-vesicles perform active diffusion in the sea urchin embryo during larval biomineralization.
publisher Public Library of Science (PLoS)
series PLoS Computational Biology
issn 1553-734X
1553-7358
publishDate 2021-02-01
description Biomineralization is the process by which organisms use minerals to harden their tissues and provide them with physical support. Biomineralizing cells concentrate the mineral in vesicles that they secret into a dedicated compartment where crystallization occurs. The dynamics of vesicle motion and the molecular mechanisms that control it, are not well understood. Sea urchin larval skeletogenesis provides an excellent platform for investigating the kinetics of mineral-bearing vesicles. Here we used lattice light-sheet microscopy to study the three-dimensional (3D) dynamics of calcium-bearing vesicles in the cells of normal sea urchin embryos and of embryos where skeletogenesis is blocked through the inhibition of Vascular Endothelial Growth Factor Receptor (VEGFR). We developed computational tools for displaying 3D-volumetric movies and for automatically quantifying vesicle dynamics. Our findings imply that calcium vesicles perform an active diffusion motion in both, calcifying (skeletogenic) and non-calcifying (ectodermal) cells of the embryo. The diffusion coefficient and vesicle speed are larger in the mesenchymal skeletogenic cells compared to the epithelial ectodermal cells. These differences are possibly due to the distinct mechanical properties of the two tissues, demonstrated by the enhanced f-actin accumulation and myosinII activity in the ectodermal cells compared to the skeletogenic cells. Vesicle motion is not directed toward the biomineralization compartment, but the vesicles slow down when they approach it, and probably bind for mineral deposition. VEGFR inhibition leads to an increase of vesicle volume but hardly changes vesicle kinetics and doesn't affect f-actin accumulation and myosinII activity. Thus, calcium vesicles perform an active diffusion motion in the cells of the sea urchin embryo, with diffusion length and speed that inversely correlate with the strength of the actomyosin network. Overall, our studies provide an unprecedented view of calcium vesicle 3D-dynamics and point toward cytoskeleton remodeling as an important effector of the motion of mineral-bearing vesicles.
url https://doi.org/10.1371/journal.pcbi.1008780
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AT tsviagildor calciumvesiclesperformactivediffusionintheseaurchinembryoduringlarvalbiomineralization
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