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首页> 外文OA文献 >Molecular Analysis of Voltage-gated ?-Na+ Channel Toxin Binding Site 3 to Determine Key Residues that Confer Resistance to ?-scorpion Toxin
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Molecular Analysis of Voltage-gated ?-Na+ Channel Toxin Binding Site 3 to Determine Key Residues that Confer Resistance to ?-scorpion Toxin

机译:电压门控α-Na +通道毒素结合位点3的分子分析,以确定对β-蝎毒素具有抗性的关键残基

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摘要

Voltage-gated Na+ channels (Nav1.2) which are proteins that posses 4 (I-IV) domains and six transmembrane (S1-S6) helices in each domain display abnormally slowed fast inactivation when an ?-scorpion toxin binds to it. However, voltage gated Na+ channels of the Mesobuthus martensii Karsch (MmK) scorpion that produces a-scorpion toxins are resistant to their toxins. The previously described ?-toxin binding site 3 of the MmK voltage-gated Na+ channels were examined by a comparative method using an alignment of many sodium channel protein sequences (multi-alignment) generated using the rat Nav1.2 ?-toxin sequence of binding site 3 as a template for the alignment. The ?-toxin binding site 3 is comprised of 4 regions or segments and found in domains I and IV of the Na+ channel. An analysis suggested that key residues exist that presumably are essential for the ?-scorpion toxin binding at each of the four segments of the toxin binding site 3. The most significant mutations either altered the charge distribution and or polarity of the binding region or likely introduced changes in secondary structure (introduction of a turn). Mutations observed in the first segment of domain I S5-S6 that correspond to protein sequence positions in the rat and scorpion Na+ channel (rat/Mmk) at K355/S339, A356/N340, -/Y341 (- refers to a missing residue), R358/P343, Y362/H347, and G371- S371/Y356 were the most significant. Significant mutations in the second segment of domain I S5-S6 were evident at K399/P384 and T400/W385. The fourth segment of domain IV S5-S6 had significant mutations at K1687/H1599, E168/R1600, and M1694/N1606. The third segment of domain IV S3-S4 was suspected of having significant mutations at E1616/A1528 and K1617/S1529. Changes in these key resides may introduce resistance to binding and action of ?-scorpion toxins to the Na+ channel. Future experimentation and or analysis will be needed to determine which of these residues are the most important for binding of the toxin to the channel.
机译:电压门控的Na +通道(Nav1.2)是一种蛋白质,具有α-蝎毒素与之结合,在每个域中具有4个(I-IV)域和6个跨膜(S1-S6)螺旋,显示出异常缓慢的快速失活。然而,产生α-蝎毒素的马氏肉食蝎(Mesobuthus martensii Karsch(MmK))蝎的电压门控Na +通道对其毒素具有抗性。 MmK电压门控Na +通道的先前描述的β-毒素结合位点3通过比较方法进行了比较,使用了许多通过大鼠Nav1.2β-毒素结合序列生成的钠通道蛋白序列(多序列)的比对。位点3作为比对的模板。 α-毒素结合位点3由4个区域或区段组成,并且存在于Na +通道的结构域I和IV中。分析表明,关键残基存在于毒素结合位点3的四个区段的每一个处,对于α-蝎子毒素的结合可能是必不可少的。最显着的突变或者改变了电荷分布和/或结合区域的极性,或者可能引入了二级结构的变化(引入转弯)。在结构域I S5-S6的第一段中观察到的突变,与K355 / S339,A356 / N340,-/ Y341处大鼠和蝎子Na +通道(大鼠/ Mmk)中的蛋白质序列位置相对应(-表示缺失的残基) ,R358 / P343,Y362 / H347和G371-S371 / Y356最重要。在K399 / P384和T400 / W385处,结构域I S5-S6的第二部分中的明显突变是明显的。域IV S5-S6的第四段在K1687 / H1599,E168 / R1600和M1694 / N1606处具有明显的突变。域IV S3-S4的第三段被怀疑在E1616 / A1528和K1617 / S1529具有明显的突变。这些关键部位的变化可能会导致对α蝎毒素对Na +通道的结合和作用产生抗性。需要进一步的实验和分析,以确定这些残基中哪些对毒素与通道的结合最重要。

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    Souqiyyeh Anas;

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