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Expression and purification of a functional heteromeric GABAA receptor for structural studies

机译:表达和纯化功能性异源GABAA受体用于结构研究

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摘要

The GABA-gated chloride channels of the Cys-loop receptor family, known as GABAA receptors, function as the primary gatekeepers of fast inhibitory neurotransmission in the central nervous system. Formed by the pentameric arrangement of five identical or homologous subunits, GABAA receptor subtypes are defined by the subunit composition that shape ion channel properties. An understanding of the structural basis of distinct receptor properties has been hindered by the absence of high resolution structural information for heteromeric assemblies. Robust heterologous expression and purification protocols of high expressing receptor constructs are vital for structural studies. Here, we describe a unique approach to screen for well-behaving and functional GABAA receptor subunit assemblies by using the Xenopus oocyte as an expression host in combination with fluorescence detection size exclusion chromatography (FSEC). To detect receptor expression, GFP fusions were introduced into the α1 subunit isoform. In contrast to expression of α1 alone, co-expression with the β subunit promoted formation of monodisperse assemblies. Mutagenesis experiments suggest that the α and β subunits can tolerate large truncations in the non-conserved M3/M4 cytoplasmic loop without compromising oligomeric assembly or GABA-gated channel activity, although removal of N-linked glycosylation sites is negatively correlated with expression level. Additionally, we report methods to improve GABAA receptor expression in mammalian cell culture that employ recombinant baculovirus transduction. From these methods we have identified a well-behaving minimal functional construct for the α1/β1 GABAA receptor subtype that can be purified in milligram quantities while retaining high affinity agonist binding activity.
机译:半胱氨酸环受体家族的GABA门控氯离子通道,称为GABAA受体,在中枢神经系统中起着快速抑制神经传递的主要守门员的作用。由五个相同或同源亚基的五聚体排列形成,GABAA受体亚型由塑造离子通道特性的亚基组成定义。缺乏对异聚体组装的高分辨率结构信息阻碍了对独特受体特性的结构基础的理解。高表达受体构建体的稳健异源表达和纯化方案对于结构研究至关重要。在这里,我们描述了一种独特的方法,通过使用爪蟾卵母细胞作为表达宿主与荧光检测尺寸排阻色谱法(FSEC)结合,筛选行为良好且功能正常的GABAA受体亚基装配体。为了检测受体表达,将GFP融合物引入α1亚基同工型。与单独表达α1相比,与β亚基的共表达促进了单分散组装的形成。诱变实验表明,尽管N联糖基化位点的去除与表达水平呈负相关,但α和β亚基可以耐受非保守的M3 / M4细胞质环中的大截短而不损害寡聚组装或GABA门控的通道活性。此外,我们报告了采用重组杆状病毒转导来提高哺乳动物细胞培养物中GABAA受体表达的方法。从这些方法中,我们已经为α1/β1GABAA受体亚型确定了行为良好的最小功能构建体,可以以毫克量进行纯化,同时保留高亲和力激动剂结合活性。

著录项

  • 期刊名称 other
  • 作者

    Derek P. Claxton; Eric Gouaux;

  • 作者单位
  • 年(卷),期 -1(13),7
  • 年度 -1
  • 页码 e0201210
  • 总页数 25
  • 原文格式 PDF
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