Two isoforms of Drosophila dynamin in wild-type and shibire(ts) neural tissue: Different subcellular localization and association mechanisms

被引:6
作者
Gass, GV
Lin, JJC
Scaife, R
Wu, CF
机构
[1] UNIV IOWA,DEPT BIOL SCI,IOWA CITY,IA 52242
[2] INST BIOL STRUCT,F-38027 GRENOBLE,FRANCE
关键词
dynamin isoforms; endocytosis; shibire(ts) mutants; Drosophila; cultured neurons; liposomes; membrane association; pH; temperature; GTPase;
D O I
10.3109/01677069509083462
中图分类号
Q3 [遗传学];
学科分类号
071007 ; 090102 ;
摘要
The temperature-sensitive mutations of the shibire (shi) gene in Drosophila cause endocytic arrest, resulting in neurotransmission block and paralysis at high temperatures. However, underlying mechanism for the defects is not yet known. We examined the subcellular distribution of dynamin, a product of the shi gene, by immunoblotting and immunocytochemical assays. Two isoforms of dynamin with apparent M(r) of 92 kD and 94 kD have been detected in wild-type and shi(ts) adult neural tissue. The two isoforms were reproducibly associated with different subcellular fractions of head homogenates. The 94 kD isoform is fractionated in the low speed (2,000 x g) pellet containing plasma membrane fragments, and the 92 kD isoform in the high speed (130,000 x g) pellet. In this procedure, very little dynamin remained in the high speed supernatant fraction. The 94 kD isoform represents the majority (65-75%) of total dynamin and appears to be a peripheral membrane protein. It can be extracted from the low speed membrane pellet by high salt, Na2CO3 (pH 11) or Triton X-100 treatments. Extracted 94 kD dynamin from both wild-type and mutant homogenates is able to reassociate with artificial phospholipid vesicles at both permissive and restrictive temperatures. Binding of the 94 kD dynamin to liposomes appears to be pH-dependent, varying most significantly within the physiological pH range, which may be functionally important. The 92 kD isoform cannot be released by high salt or Na2CO3 treatments and only a small fraction is released by Triton X-100, suggesting a different mechanism of association with cell structures. The distribution of the two isoforms is not altered by the presence of stabilized microtubules in homogenates. No apparent degradation or subcellular redistribution of mutant dynamin was detected in two shi(ts) alleles after heat shock or block of the dynamin GTPase activity, suggesting that intracellular redistribution or degradation of mutant dynamin are not involved in the endocytosis arrest in these mutants. These observations resemble the effect of endocytosis' arrest by GTP-gamma-S in rat brain synaptosomes (Takei el al., 1995), in which dynamin is trapped at the neck of invaginated pits but is absent in the clathrin-coated distal end undergoing internalization. Our finding that endocytosis arrest by shi(ts) mutations and GTP-gamma-S do not lead to cumulation of dynamin in the low speed pellet fraction further suggests that the 94 kD isoform remains associated with the plasma membrane during coated vesicle pinch-off and that the two isoforms do not appear to correspond to different functional states of dynamin but are likely to be involved in separate cellular compartments within the membrane cycling pathway (e.g., the plasma membrane, endosomes, and endoplasmic reticulum).
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页码:169 / 191
页数:23
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