Myosin Light Chain-activating Phosphorylation Sites Are Required for Oogenesis in Drosophila

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© The Rockefeller University Press, 0021-9525/1997//1805 $5.00
The Journal of Cell Biology, Volume 139, Number 7, , 1997 1805-1819

Article

Myosin Light Chain–activating Phosphorylation Sites Are Required for Oogenesis in Drosophila

Pascale Jordan and Roger Karess

Centre de Génétique Moleculaire, 91198 Gif-sur-Yvette, France

The Drosophila spaghetti squash (sqh) gene encodes the regulatorymyosin light chain (RMLC) of nonmuscle myosin II. Biochemicalanalysis of vertebrate nonmuscle and smooth muscle myosin IIhas established that phosphorylation of certain amino acids of the RMLC greatly increases the actin-dependent myosin ATPaseand motor activity of myosin in vitro. We have assessed thein vivo importance of these sites, which in Drosophila correspondto serine-21 and threonine-20, by creating a series of transgenesin which these specific amino acids were altered. The phenotypesof the transgenes were examined in an otherwise null mutantbackground during oocyte development in Drosophila females.

Germ line cystoblasts entirely lacking a functional sqh geneshow severe defects in proliferation and cytokinesis. The ringcanals, cytoplasmic bridges linking the oocyte to the nursecells in the egg chamber, are abnormal, suggesting a role ofmyosin II in their establishment or maintenance. In addition,numerous aggregates of myosin heavy chain accumulate in thesqh null cells. Mutant sqh transgene sqh-A20, A21 in which both serine-21 and threonine-20 have been replaced by alaninesbehaves in most respects identically to the null allele inthis system, with the exception that no heavy chain aggregatesare found. In contrast, expression of sqh-A21, in which onlythe primary phosphorylation target serine-21 site is altered,partially restores functionality to germ line myosin II, allowingcystoblast division and oocyte development, albeit with somecytokinesis failure, defects in the rapid cytoplasmic transportfrom nurse cells to cytoplasm characteristic of late stageoogenesis, and some damaged ring canals. Substituting a glutamatefor the serine-21 (mutant sqh-E21) allows oogenesis to be completedwith minimal defects, producing eggs that can develop normallyto produce fertile adults. Flies expressing sqh-A20, in whichonly the secondary phosphorylation site is absent, appear tobe entirely wild type. Taken together, this genetic evidenceargues that phosphorylation at serine-21 is critical to RMLCfunction in activating myosin II in vivo, but that the functioncan be partially provided by phosphorylation at threonine-20.

Abbreviations used in this paper: hts, huli-tai-shau; MHC, myosin heavy chain; MLCK, myosin light chain kinase; RMLC, regulatory myosin light chain.

Address all correspondence to Dr. Roger Karess, Centre de Génétique Moleculaire, Ave de la Terrasse, 91198 Gif-sur-Yvette, France.Tel.: (33-1) 69-82-32-25; Fax: (33-1) 69-82-31-50. E-mail:karess{at}cgm.cnrs-gif.fr

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