Abstract
AbstractMembrane Contact Sites (MCS) between the plasma membrane (PM) and endoplasmic reticulum (ER) have been shown to regulate Ca2+influx into animal cells. However, the mechanisms by which cells modulate ER-PM MCS density is not understood and the role of Ca2+, if any, in regulating this process is not known. We report that inDrosophilaphotoreceptors, MCS density is dependent on the activity of the Ca2+permeable channels-TRP and TRPL. This regulation of MCS density by Ca2+is mediated by extended synaptotagmin (dEsyt), a protein localised to ER-PM MCS in photoreceptors and previously shown to regulate MCS density. We find that the Ca2+binding activity of dEsyt is required for its functional activityin vivo. dEsytCaBM, a Ca2+non-binding mutant of dEsyt is unable to modulate MCS structure in a manner equivalent to its wild type counterpart. Further, when reconstituted in dEsyt null photoreceptors, in contrast to wild type dEsyt, dEsytCaBMis unable to rescue ER-PM MCS density and other key phenotypes. Finally, when expressed in wild type photoreceptors, dEsytCaBMphenocopies loss of dEsyt function. Taken together, our data supports a role for the Ca2+binding activity of dEsyt in regulating the ER-PM MCS density in photoreceptors thus tuning signal transduction in response to Ca2+influx triggered by ambient illumination.Abstract Figure
Publisher
Cold Spring Harbor Laboratory