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      Mechanisms of calcium elevation in the micromeres of sea urchin embryos.

      1 , , ,
      Biology of the cell

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          Abstract

          The micromeres, the first cells to be specified in sea urchin embryos, are generated by unequal cleavage at the fourth cell division. The micromeres differentiate autonomously to form spicules and dispatch signals to induce endomesoderm in the neighbouring macromeres cells in the embryo. Using a calcium indicator Fura-2/AM and a mixture of dextran conjugated Oregon green-BAPTA 488 and Rhodamine red, the intracellular calcium ion concentration ([Ca2+]i) was studied in embryos at the 16-cell stage. [Ca2+]i was characteristically elevated in the micromeres during furrowing at the 4th cleavage. Subsequently, Ca2+ oscillated for about 10 min in the micromeres, resulting in episodic high levels of [Ca2+]i. High [Ca2+]i regions were associated with regional localizations of the endoplasmic reticulum (ER), though not with ER accumulated at the vegetal pole of the micromeres during the 4th division. Pharmacological studies, using a blocker of IP3-mediated Ca2+ release (Xestospongin), a store-operated Ca2+ entry inhibitor (2 aminoethoxydiphenyl borate (2-APB)) and an inhibitor of stretch-dependent ion channels (gadolinium), suggest that the high [Ca2+]i and oscillations in the micromeres are triggered by calcium influx caused by the activation of stretch-dependent calcium channels, followed by the release of calcium ions from the endoplasmic reticulum. On the basis of these new findings, a possible mechanism for autonomous formation of the micromeres is discussed.

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          Author and article information

          Journal
          Biol. Cell
          Biology of the cell
          0248-4900
          0248-4900
          Mar 2004
          : 96
          : 2
          Affiliations
          [1 ] Department of Biology, Tokyo Metropolitan University, Minamiohsawa 1-1, Hachiohji, Tokyo 192-0397, Japan. ikuko@comp.metro-u.ac.jp
          Article
          S0248490004000085
          10.1016/j.biolcel.2003.11.009
          15050370
          26c1c983-320b-4200-962f-fd394d544060
          History

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