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Clathrin assembly protein AP180: primary structure domain organization and identification of a clathrin binding site.

机译:网格蛋白装配蛋白AP180:网格蛋白结合位点的一级结构结构域和鉴定。

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摘要

Binding of AP180 to clathrin triskelia induces their assembly into 60-70 nm coats. The largest rat brain cDNA clone isolated predicts a molecular weight of 91,430 for AP180. Two cDNA clones have an additional small 57 bp insert. The deduced molecular weight agrees with gel filtration results provided the more chaotropic denaturant 6 M guanidinium thiocyanate is substituted for the weaker guanidinium chloride. The sequence and the proteolytic cleavage pattern suggest a three domain structure. The N-terminal 300 residues (pI 8.7) harbour a clathrin binding site. An acidic middle domain (pI 3.6, 450 residues), interrupted by an uncharged alanine rich segment of 59 residues, appears to be responsible for the anomalous physical properties of AP180. The C-terminal domain (166 residues) has a pI of 10.4. AP180 mRNA is restricted to neuronal sources. AP180 shows no significant homology to known clathrin binding proteins, but is nearly identical to a mouse phosphoprotein (F1-20). This protein, localized to synaptic termini, has so far been of unknown function.
机译:AP180与网格蛋白triskelia的结合诱导其组装成60-70 nm涂层。分离出的最大的大鼠脑cDNA克隆预测AP180的分子量为91,430。两个cDNA克隆还有一个额外的57 bp小插入片段。推导的分子量与凝胶过滤结果一致,条件是用离液性更高的变性剂6 M硫氰酸胍代替较弱的氯化胍。序列和蛋白水解切割模式提示三结构域结构。 N末端300个残基(pI 8.7)具有网格蛋白结合位点。酸性中间结构域(pI 3.6,450个残基)被不带电荷的富含59个残基的丙氨酸片段中断,似乎是AP180异常物理特性的原因。 C端结构域(166个残基)的pI为10.4。 AP180 mRNA仅限于神经元来源。 AP180与已知的网格蛋白结合蛋白无明显同源性,但与小鼠磷蛋白(F1-20)几乎相同。迄今为止,定位于突触末端的这种蛋白质的功能尚不清楚。

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