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首页> 外文期刊>Protein Expression and Purification >Preparation of soluble isotopically labeled NKp30, a human natural cytotoxicity receptor, for structural studies using NMR
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Preparation of soluble isotopically labeled NKp30, a human natural cytotoxicity receptor, for structural studies using NMR

机译:使用NMR制备可溶性同位素标记的NKp30(人类天然细胞毒性受体),用于结构研究

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Using a codon-optimized gene fragment, we report remarkable yields for extracellular domain of human NK cell receptor (NKp30ex) when produced on M9 minimal medium, even with low (2 g/L) glucose concentration. The yields were identical using media containing 15NH 4Cl or 15NH 4Cl in combination with all- 13C-d-glucose allowing to produce homogenous soluble monomeric NKp30 in several formats needed for advanced NMR studies. Our optimized protocol now allows to produce routinely 10 mg batches of these NKp30ex proteins per 1 L of M9 production medium in four working days. The purity and identity of the produced proteins were checked by SDS-PAGE, MALDI MS peptide mapping, and high resolution ion cyclotron resonance MS. Analytical ultracentrifugation confirmed the monomeric status of the produced proteins. Long-term stability of the produced protein proved to be very good allowing its use for NMR studies using elevated temperatures. These studies should reveal further details of the interaction of NKp30 with several of its ligands including target cell surface proteins and heparin-derived oligosaccharides.
机译:使用密码子优化的基因片段,我们报道了在M9基本培养基上产生的人NK细胞受体(NKp30ex)细胞外域的显着产量,即使低(2 g / L)葡萄糖浓度也是如此。使用包含15NH 4Cl或15NH 4Cl的培养基与全13C-d-葡萄糖结合使用,可以产生高级NMR研究所需的几种格式的均质可溶性单体NKp30,产率相同。我们优化的方案现在允许在四个工作日内,每1升M9生产培养基常规生产10毫克批次的NKp30ex蛋白。通过SDS-PAGE,MALDI MS肽图分析和高分辨率离子回旋共振MS检查所产生蛋白质的纯度和身份。分析超离心证实了所产生蛋白质的单体状态。事实证明,所产生蛋白质的长期稳定性非常好,可用于高温下的NMR研究。这些研究应揭示NKp30与包括靶细胞表面蛋白和肝素衍生的寡糖在内的几种配体相互作用的更多细节。

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