Rab27A and its effector MyRIP link secretory granules to F-actin and control their motion towards release sites

被引:127
作者
Desnos, C
Schonn, JS
Huet, S
Tran, VS
El-Amraoui, A
Raposo, GA
Fanget, I
Chapuis, C
Ménasché, G
de saint Basile, G
Petit, C
Cribier, S
Henry, JP
Darchen, F
机构
[1] Inst Biol Physicochim, CNRS, UPR 1929, F-75005 Paris, France
[2] Inst Biol Physicochim, CNRS, UMR 7099, F-75005 Paris, France
[3] Inst Pasteur, CNRS, URA 1968, F-75724 Paris, France
[4] Inst Curie, CNRS, UMR 144 Curie, F-75248 Paris 05, France
[5] Hop Necker Enfants Malad, INSERM, U429, F-75743 Paris 15, France
关键词
Rab27A; MyRIP; exocytosis; actin; neuroendocrine cell;
D O I
10.1083/jcb.200302157
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
The GTPase Rab27A interacts with myosin-VIIa and myosin-Va via MyRIP or melanophilin and mediates melanosome binding to actin. Here we show that Rab27A and MyRIP are associated with secretory granules (SGs) in adrenal chromaffin cells and PC12 cells. Overexpression of Rab27A, GTPase-deficient Rab27A-Q78L, or MyRIP reduced secretory responses of PC12 cells. Amperometric recordings of single adrenal chromaffin cells revealed that Rab27A-Q78L and MyRIP reduced the sustained component of release. Moreover, these effects on secretion were partly suppressed by the actin-depolymerizing drug latrunculin but strengthened by jasplakinolide, which stabilizes the actin cortex. Finally, MyRIP and Rab27A-Q78L restricted the motion of SGs in the subplasmalemmal region of PC12 cells, as measured by evanescent-wave fluorescence microscopy. In contrast, the Rab27A-binding domain of MyRIP and a MyRIP construct that interacts with myosin-Va but not with actin increased the mobility of SGs. We propose that Rab27A and MyRIP link SGs to F-actin and control their motion toward release sites through the actin cortex.
引用
收藏
页码:559 / 570
页数:12
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