Syntaxin-16, a putative Golgi t-SNARE

被引:102
作者
Simonsen, A
Bremnes, B
Ronning, E
Aasland, R
Stenmark, H
机构
[1] Norwegian Radium Hosp, Dept Biochem, N-0310 Oslo, Norway
[2] Univ Bergen, HiB, Dept Mol Biol, Bergen, Norway
关键词
Golgi apparatus; membrane traffic; SNARE; syntaxin;
D O I
10.1016/S0171-9335(98)80116-7
中图分类号
Q2 [细胞生物学];
学科分类号
071009 ; 090102 ;
摘要
Members of the syntaxin family of integral membrane proteins have recently been implicated as vesicle receptors on target membranes, coresponsible for the specificity of intracellular membrane traffic. So far, only a small number of different mammalian syntaxins have been identified. Here we report the cloning of three new human syntaxin cDNAs, presumably originating from alternative splicing of the same transcript. Syntaxin-16A and syntaxin-16B are identical, except that the latter contains an insertion of 21 amino acid residues. Syntaxin-16C is a truncated version of syntaxin-16A, lacking the C-terminal coiled-coil and hydrophobic regions characteristic for syntaxins. Database searches identified putative yeast, plant and nematode homologues of syntaxin-16, indicating that this protein is conserved through evolution, and syntaxin-16 belongs to a new subgroup of syntaxins. Epitope-tagged syntaxin-16A and syntaxin-16B were found to colocalize with the Golgi marker beta-COP, while syntaxin-16C was found in the cytosol. Syntaxin-16A associates posttranslationally with microsomes, and appears to be transported to the Golgi via the endoplasmic reticulum. The three syntaxin-16 forms may have differential roles in intracellular trafficking.
引用
收藏
页码:223 / 231
页数:9
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