R Blostein, S E Daly, N Boxenbaum, L K Lane, J M Arguello, J B Lingrel, S J Karlish, M J Caplan, L Dunbar
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The first two mutations, either separately or in combination (alpha 1M32E233K), shift the equilibrium between the major conformational states of the enzyme, E1 and E2, in favor of E1 as manifested by increased apparent affinity for ATP, lower catalytic turnover, and decreased sensitivity to inhibition by vanadate. The striking changes observed with alpha 1M32E233K suggests interactions between the N-terminus, the beta-strand in the M2-M3 loop and the catalytic phosphorylation site. The behavior of these mutants contrasts with that of least one mutant involving substitution of a residue in the putative cation binding pocket, namely S775A in the fifth transmembrane segment (Arguello, J.M., & Lingrel, J. B. J. Biol. Chem. 270: 22764-22771, 1995). Although its K+/ATP antagonism resembles that of the foregoing cytoplasmic mutants, its vanadate sensitivity is unaltered suggesting that changes in apparent affinity for ATP are secondary to changes in K+ ligation. The question of cation selectivity, in particular that of Na+ versus protons, has been addressed in structure/function analysis of a cytoplasmic chimera involving the M4-M5 loop. Transport studies performed in the presence or absence of Na+ and at low versus high pH indicate a marked alteration in cation affinity and/or selectivity. This results suggests coupling of an alteration in the large M4-M5 cytoplasmic domain to cation binding in, presumably, the juxtapositioned transmembrane domain.</p>","PeriodicalId":75414,"journal":{"name":"Acta physiologica Scandinavica. 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引用次数: 0
摘要
本文总结了有关Na - k - atp酶α 1亚基细胞质区域突变的功能后果的实验,特别是氨基端,跨膜段M2和M3之间的第一个细胞质环,以及M4和M5之间的主要细胞质环。在第一个突变(α 1M32)中,从n端去除32个残基。第二个突变(E233K)发生在M2-M3环的β链上,第三个突变包括Na, k - atp酶环M4-M5的氨基末端被胃H, k - atp酶的同源片段(残基356-519)取代。前两个突变,无论是单独的还是联合的(α 1M32E233K),都改变了酶E1和E2的主要构象状态之间的平衡,有利于E1,表现为对ATP的明显亲和力增加,催化转化率降低,对钒酸盐抑制的敏感性降低。在α 1M32E233K中观察到的显著变化表明,n端、M2-M3环中的β链和催化磷酸化位点之间存在相互作用。这些突变体的行为与至少一种涉及在假定的阳离子结合袋中置换残基的突变体相反,即第五跨膜段的S775A (Arguello, j.m., & Lingrel, J. B. J. Biol)。化学。270:22764-22771,1995)。虽然其对K+/ATP的拮抗作用类似于上述细胞质突变体,但其对钒酸盐的敏感性没有改变,这表明对ATP的表观亲和力的变化是继发于K+连接的变化。在涉及M4-M5环的细胞质嵌合体的结构/功能分析中,已经解决了阳离子选择性问题,特别是Na+对质子的选择性问题。在存在或不存在Na+以及低pH值和高pH值下进行的转运研究表明,阳离子亲和力和/或选择性有显著变化。这一结果表明,在大的M4-M5细胞质结构域的改变耦合到阳离子结合,推测,并置跨膜结构域。
Conformational alterations resulting from mutations in cytoplasmic domains of the alpha subunit of the Na,K-ATPase.
This paper summarizes experiments concerned with the functional consequences of mutations in cytoplasmic regions of the alpha 1 subunit of the Na,K-ATPase, in particular the amino terminus, the first cytoplasmic loop between transmembrane segments M2 and M3, and the major cytoplasmic loop between M4 and M5. In the first mutation (alpha 1M32), 32 residues were removed from the N-terminus. The second mutation (E233K) was in the putative beta strand of M2-M3 loop and the third, comprised the replacement of the amino terminal half of loop M4-M5 of the Na,K-ATPase with the homologous segment (residues 356-519) of the gastric H,K-ATPase. The first two mutations, either separately or in combination (alpha 1M32E233K), shift the equilibrium between the major conformational states of the enzyme, E1 and E2, in favor of E1 as manifested by increased apparent affinity for ATP, lower catalytic turnover, and decreased sensitivity to inhibition by vanadate. The striking changes observed with alpha 1M32E233K suggests interactions between the N-terminus, the beta-strand in the M2-M3 loop and the catalytic phosphorylation site. The behavior of these mutants contrasts with that of least one mutant involving substitution of a residue in the putative cation binding pocket, namely S775A in the fifth transmembrane segment (Arguello, J.M., & Lingrel, J. B. J. Biol. Chem. 270: 22764-22771, 1995). Although its K+/ATP antagonism resembles that of the foregoing cytoplasmic mutants, its vanadate sensitivity is unaltered suggesting that changes in apparent affinity for ATP are secondary to changes in K+ ligation. The question of cation selectivity, in particular that of Na+ versus protons, has been addressed in structure/function analysis of a cytoplasmic chimera involving the M4-M5 loop. Transport studies performed in the presence or absence of Na+ and at low versus high pH indicate a marked alteration in cation affinity and/or selectivity. This results suggests coupling of an alteration in the large M4-M5 cytoplasmic domain to cation binding in, presumably, the juxtapositioned transmembrane domain.
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