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AE2跨膜结构域的非保守带电残基在pH调节阴离子交换中的作用

Role of nonconserved charged residues of the AE2 transmembrane domain in regulation of anion exchange by pH.

作者信息

Stewart A K, Kurschat C E, Alper S L

机构信息

Molecular and Vascular Medicine Unit and Renal Unit, Department of Medicine, Harvard Medical School, Beth Israel Deaconess Medical Center, Boston, MA 02215, USA.

出版信息

Pflugers Arch. 2007 Jun;454(3):373-84. doi: 10.1007/s00424-007-0220-8. Epub 2007 Feb 16.

Abstract

The ubiquitous AE2/SLC4A2 anion exchanger is acutely and independently regulated by intracellular (pH(i)) and extracellular pH (pH(o)), whereas the closely related AE1/SLC4A1 of the red cell and renal intercalated cell is relatively pH-insensitive. We have investigated the contribution of nonconserved charged residues within the C-terminal transmembrane domain (TMD) of AE2 to regulation by pH through mutation to the corresponding AE1 residues. AE2-mediated Cl(-)/Cl(-) exchange was measured as 4,4'-di-isothiocyanatostilbene-2,2'-disulfonic acid-sensitive (36)Cl(-) efflux from Xenopus oocytes by varying pH(i) at constant pH(o), and by varying pH(o) at near-constant pH(i). All mutations of nonconserved charged residues of the AE2 TMD yielded functional protein, but mutations of some conserved charged residues (R789E, R1056A, R1134C) reduced or abolished function. Individual mutation of AE2 TMD residues R921, F922, P1077, and R1107 exhibited reduced pH(i) sensitivity compared to wt AE2, whereas TMD mutants K1153R, R1155K, R1202L displayed enhanced sensitivity to acidic pH(i). In addition, pH(o) sensitivity was significantly acid- shifted when nonconserved AE2 TMD residues E981, K982, and D1075 were individually converted to the corresponding AE1 residues. These results demonstrate that multiple conserved charged residues are important for basal transport function of AE2 and that certain nonconserved charged residues of the AE2 TMD are essential for wild-type regulation of anion exchange by pH(i) and pH(o).

摘要

普遍存在的AE2/SLC4A2阴离子交换蛋白受细胞内pH值(pH(i))和细胞外pH值(pH(o))的急性且独立调节,而红细胞和肾闰细胞中密切相关的AE1/SLC4A1对pH相对不敏感。我们通过将AE2 C末端跨膜结构域(TMD)中的非保守带电残基突变为相应的AE1残基,研究了AE2的这些残基对pH调节的作用。通过在恒定pH(o)下改变pH(i)以及在接近恒定pH(i)下改变pH(o),将AE2介导的Cl(-)/Cl(-)交换测定为非洲爪蟾卵母细胞中4,4'-二异硫氰酸根合芪-2,2'-二磺酸敏感的(36)Cl(-)流出。AE2 TMD的非保守带电残基的所有突变都产生了功能性蛋白,但一些保守带电残基(R789E、R1056A、R1134C)的突变降低或消除了功能。与野生型AE2相比,AE2 TMD残基R921、F922、P1077和R1107的单个突变表现出降低的pH(i)敏感性,而TMD突变体K1153R、R1155K、R1202L对酸性pH(i)表现出增强的敏感性。此外,当非保守的AE2 TMD残基E981、K982和D1075分别转变为相应的AE1残基时,pH(o)敏感性明显向酸性偏移。这些结果表明,多个保守带电残基对AE2的基础转运功能很重要,并且AE2 TMD的某些非保守带电残基对于pH(i)和pH(o)对阴离子交换的野生型调节至关重要。

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