首页> 美国卫生研究院文献>The Journal of Biological Chemistry >Comprehensive Cysteine-scanning Mutagenesis Reveals Claudin-2 Pore-lining Residues with Different Intrapore Locations
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Comprehensive Cysteine-scanning Mutagenesis Reveals Claudin-2 Pore-lining Residues with Different Intrapore Locations

机译:全面的半胱氨酸扫描诱变揭示了Claudin-2孔内残基具有不同的孔内位置。

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摘要

The first extracellular loop (ECL1) of claudins forms paracellular pores in the tight junction that determine ion permselectivity. We aimed to map the pore-lining residues of claudin-2 by comprehensive cysteine-scanning mutagenesis of ECL1. We screened 45 cysteine mutations within the ECL1 by expression in polyclonal Madin-Darby canine kidney II Tet-Off cells and found nine mutants that displayed a significant decrease of conductance after treatment with the thiol-reactive reagent 2-(trimethylammonium)ethyl methanethiosulfonate, indicating the location of candidate pore-lining residues. Next, we stably expressed these candidates in monoclonal Madin-Darby canine kidney I Tet-Off cells and exposed them to thiol-reactive reagents. The maximum degree of inhibition of conductance, size selectivity of degree of inhibition, and size dependence of the kinetics of reaction were used to deduce the location of residues within the pore. Our data support the following sequence of pore-lining residues located from the narrowest to the widest part of the pore: Ser68, Ser47, Thr62/Ile66, Thr56, Thr32/Gly45, and Met52. The paracellular pore appears to primarily be lined by polar side chains, as expected for a predominantly aqueous environment. Furthermore, our results strongly suggest the existence of a continuous sequence of residues in the ECL1 centered around Asp65–Ser68 that form a major part of the lining of the pore.
机译:claudins的第一个细胞外环(ECL1)在紧密连接中形成决定离子渗透选择性的细胞旁孔。我们旨在通过全面的半胱氨酸扫描诱变ECL1来绘制claudin-2的孔衬残基图。我们通过在多克隆Madin-Darby犬肾II Tet-Off细胞中的表达筛选了ECL1中的45个半胱氨酸突变,发现9个突变体在用硫醇反应试剂2-(三甲基铵)甲硫代磺酸盐处理后显示出电导率的显着降低,这表明候选孔衬残留物的位置。接下来,我们在单克隆Madin-Darby犬肾I Tet-Off细胞中稳定表达这些候选物,并将其暴露于硫醇反应试剂中。电导的最大抑制程度,抑制程度的大小选择性以及反应动力学的大小依赖性被用来推断孔内残基的位置。我们的数据支持以下从毛孔最窄到最宽的部分的衬里残余物序列:Ser 68 ,Ser 47 ,Thr 62 / Ile 66 ,Thr 56 ,Thr 32 / Gly 45 和Met 52 < / sup>。如主要在水性环境中所预期的,细胞旁孔似乎主要被极性侧链所衬。此外,我们的结果强烈表明,在ECL1中存在以Asp 65 -Ser 68 为中心的残基连续序列,这些残基构成了孔壁的主要部分。

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