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小鼠自然杀伤细胞受体NKR-P1C(B6)可溶性形式在大肠杆菌中的高水平表达。

High-level expression of soluble form of mouse natural killer cell receptor NKR-P1C(B6) in Escherichia coli.

作者信息

Rozbeský Daniel, Kavan Daniel, Chmelík Josef, Novák Petr, Vaněk Ondřej, Bezouška Karel

机构信息

Department of Biochemistry, Charles University in Prague, CZ-12840 Prague 2, Czech Republic.

出版信息

Protein Expr Purif. 2011 Jun;77(2):178-84. doi: 10.1016/j.pep.2011.01.013. Epub 2011 Feb 1.

DOI:10.1016/j.pep.2011.01.013
PMID:21284957
Abstract

Mouse NKR-P1C(B6) receptor corresponding to NK1.1 alloantigen is one of the most widespread surface markers of mouse NK and NKT cells in C57BL/6 mice detected by monoclonal antibody PK136. Although functional studies revealed the ability of this receptor to activate both natural killing and production of cytokines upon antibody crosslinking, the ligand for NKR-P1C(B6) remains unknown. In order to initiate ligand identification, structural studies, and epitope mapping experiments, we developed a simple and efficient expression and purification protocol allowing to produce large amounts of pure soluble monomeric mouse NKR-P1C(B6). Our protein encompassed approximately half of the stalk region and the entire C-terminal globular ligand binding domain. The identity of protein that was devoid of N-terminal initiation methionine and had all three expected disulfides closed was confirmed using high resolution ion cyclotron resonance mass spectrometry. Protein produced into inclusion bodies in Escherichia coli was efficiently refolded into a unique three dimensional structure as confirmed by NMR using (1)H-(15)N-HSQC spectra of uniformly labeled protein. The exceptional purity of the protein should allow its crystallization and detailed structural investigations, and is a prerequisite for its use as a probe in ligand identification and antibody epitope mapping experiments.

摘要

与NK1.1同种抗原相对应的小鼠NKR-P1C(B6)受体,是通过单克隆抗体PK136在C57BL/6小鼠中检测到的小鼠NK细胞和NKT细胞中分布最广泛的表面标志物之一。尽管功能研究表明该受体在抗体交联后具有激活自然杀伤和细胞因子产生的能力,但NKR-P1C(B6)的配体仍然未知。为了启动配体鉴定、结构研究和表位作图实验,我们开发了一种简单有效的表达和纯化方案,能够大量生产纯的可溶性单体小鼠NKR-P1C(B6)。我们的蛋白质包含大约一半的柄区和整个C端球状配体结合结构域。使用高分辨率离子回旋共振质谱法确认了该蛋白质的身份,其不含N端起始甲硫氨酸,且所有三个预期的二硫键均已形成。通过对均匀标记蛋白质的(1)H-(15)N-HSQC谱进行核磁共振分析,证实了在大肠杆菌中产生于包涵体的蛋白质能够有效地重折叠成独特的三维结构。该蛋白质的超高纯度应有助于其结晶和详细的结构研究,并且是将其用作配体鉴定和抗体表位作图实验探针的先决条件。

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