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Microinjection of Ca2+ Store-Enriched Microsome Fractions to Dividing Newt Eggs Induces Extra-Cleavage Furrows via Inositol 1,4,5- Trisphosphate-Induced Ca2+ Release

โœ Scribed by Fuyuki Mitsuyama; Tsuyoshi Sawai; Ernesto Carafoli; Teiichi Furuichi; Katsuhiko Mikoshiba


Book ID
115598198
Publisher
Elsevier Science
Year
1999
Tongue
English
Weight
435 KB
Volume
214
Category
Article
ISSN
0012-1606

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โœฆ Synopsis


The cleavage signal transferred to the future cleavage cortex during anaphase has been proposed as "cleavage stimulus," but no signal has proved to induce cleavage furrows. The local Ca 2ุ‰ transient along the cleavage furrow has been reported, but the Ca 2ุ‰ source has remained unknown. To address these questions, we studied functions of Ca 2ุ‰ stores in dividing newt eggs and found that microinjection of the Ca 2ุ‰ store-enriched microsome fraction to the dividing newt egg induced a local extra-cleavage furrow at the injection site in 64 -67% of the injected newt eggs while coinjection with inositol 1,4,5-trisphosphate receptor (IP 3 R) antagonists heparin or anti-type 1-IP 3 R antibody clearly suppressed this induction (5 and 11% in induction rates, respectively). Injection of cerebellar microsomes from the type 1-IP 3 R-deficient mice induced extracleavage furrows albeit at a low rate (19%). Our observations strongly suggest that Ca 2ุ‰ stores with IP 3 R induce and position a cleavage furrow via IP 3 -induced Ca 2ุ‰ release (IICR) as Ca 2ุ‰ -releasing machinery and putative cleavage stimulus itself.


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