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钠/碘同向转运体活性在395位需要一个小的不带电荷的氨基酸残基。

Na(+)/I(-) symporter activity requires a small and uncharged amino acid residue at position 395.

作者信息

Dohán Orsolya, Gavrielides M Verónica, Ginter Christopher, Amzel L Mario, Carrasco Nancy

机构信息

Department of Molecular Pharmacology, Albert Einstein College of Medicine, Bronx, New York 10461, USA.

出版信息

Mol Endocrinol. 2002 Aug;16(8):1893-902. doi: 10.1210/me.2002-0071.

Abstract

Active iodide uptake in the thyroid is mediated by the Na(+)/I(-) symporter (NIS), a key plasma membrane glycoprotein. Several NIS mutations have been shown to cause I(-) transport defect, a condition that, if untreated, can lead to congenital hypothyroidism and, ultimately, cretinism. The study of I(-) transport defect-causing NIS mutations provides valuable insights into the structure-function and mechanistic properties of NIS. Here we report the thorough analysis of the G395R NIS mutation. We observed no I(-) uptake activity at saturating or even supersaturating external I(-) concentrations in COS-7 cells transiently transfected with G395R NIS cDNA, even though we demonstrated normal expression of G395R NIS and proper targeting to the plasma membrane. Several amino acid substitutions at position 395 showed that the presence of an uncharged amino acid residue with a small side chain at position 395 is required for NIS function, suggesting that glycine 395 is located in a tightly packed region of NIS. Substitutions of large amino acid residues at position 395 resulted in lower V(max) without affecting K(m) values for I(-) and Na(+), suggesting that these residues hamper the Na(+)/I(-) coupling reaction.

摘要

甲状腺中碘的主动摄取由钠碘同向转运体(NIS)介导,NIS是一种关键的质膜糖蛋白。已证实几种NIS突变会导致碘转运缺陷,这种情况若不治疗,可导致先天性甲状腺功能减退,并最终发展为呆小症。对导致碘转运缺陷的NIS突变的研究为NIS的结构功能和机制特性提供了有价值的见解。在此,我们报告对G395R NIS突变的深入分析。在用G395R NIS cDNA瞬时转染的COS-7细胞中,即使在饱和甚至超饱和的细胞外碘浓度下,我们也未观察到碘摄取活性,尽管我们证实了G395R NIS的正常表达以及其向质膜的正确靶向。395位的几个氨基酸替换表明,395位存在一个带有小侧链的不带电荷的氨基酸残基是NIS功能所必需的,这表明甘氨酸395位于NIS的紧密堆积区域。395位大氨基酸残基的替换导致最大转运速率(Vmax)降低,而不影响碘和钠的米氏常数(Km)值,这表明这些残基阻碍了钠碘偶联反应。

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