通过DNA免疫产生一组针对非典型趋化因子受体CCX-CKR的单克隆抗体。
Generation of a panel of monoclonal antibodies against atypical chemokine receptor CCX-CKR by DNA immunization.
作者信息
Takatsuka Shogo, Sekiguchi Aya, Tokunaga Masayuki, Fujimoto Akira, Chiba Joe
机构信息
Department of Biological Science and Technology, Tokyo University of Science, 2641 Yamazaki, Noda-shi, Chiba 278-8510, Japan.
出版信息
J Pharmacol Toxicol Methods. 2011 May-Jun;63(3):250-7. doi: 10.1016/j.vascn.2010.12.003. Epub 2010 Dec 22.
INTRODUCTION
Chemokines are regulated by a family of 'atypical' chemokine receptors, D6, DARC and CCX-CKR, each of which efficiently internalizes its cognate chemokine ligands. Development of monoclonal antibodies (MAbs) that would recognize CCX-CKR on the cell surface will be helpful to identify primary CCX-CKR-expressing cell types and analyze the fate of CCX-CKR after ligand binding to the receptor.
METHODS
We generated IgG MAbs recognizing the cell-surface CCX-CKR by DNA immunization using a molecular adjuvant, and analyzed the epitope recognized by the MAbs. Then, the reactivities of the MAbs with CCX-CKR-transfected cells, and also hepatocytes and hepatic tumor lines were evaluated. Finally, we also tested the ligand-like activities of the MAbs, namely, induction of internalization of CCX-CKR by the MAbs.
RESULTS
A panel of MAbs reacting with CCX-CKR expressed on the cell surface was prepared. The panel was a small one, consisting of only ten MAbs, but was rich in terms of diversity of the Ig isotypes and of the epitopes. Epitope analyses revealed that all the 10 MAbs recognized at least three different, although very close, peptide structures of the N-terminal domain. Three MAbs, namely, 2F11, 13E11 and 14F10, were selected to represent the panel. All of the MAbs were applicable for flow cytometry and immunoflurescent assays and immunoprecipitation. The reactivity of the 2F11 MAb was also confirmed by western blotting. Endogenous expression of CCX-CKR on human hepatocytes and hepatic tumor cell lines was demonstrated using the 13E11 MAb. Interestingly, binding of the 13E11 MAb with B300-19 cells expressing CCX-CKR resulted in induction of CCX-CKR internalization.
DISCUSSION
This panel of MAbs may be expected to prove valuable for further study of the functions of this silent chemokine receptor, including those related to the homeostasis of lymphoid cells, and to the growth and metastasis of hepatic cancer.
引言
趋化因子受一类“非典型”趋化因子受体(D6、DARC和CCX-CKR)调控,其中每种受体都能有效地内化其同源趋化因子配体。开发能够识别细胞表面CCX-CKR的单克隆抗体(MAb)将有助于鉴定主要表达CCX-CKR的细胞类型,并分析配体与受体结合后CCX-CKR的命运。
方法
我们使用分子佐剂通过DNA免疫产生了识别细胞表面CCX-CKR的IgG单克隆抗体,并分析了单克隆抗体识别的表位。然后,评估了单克隆抗体与CCX-CKR转染细胞、肝细胞和肝肿瘤细胞系的反应性。最后,我们还测试了单克隆抗体类似配体的活性,即单克隆抗体诱导CCX-CKR内化的能力。
结果
制备了一组与细胞表面表达的CCX-CKR反应的单克隆抗体。该组数量较少,仅由十种单克隆抗体组成,但在Ig同种型和表位的多样性方面较为丰富。表位分析表明,所有10种单克隆抗体至少识别N端结构域的三种不同但非常接近的肽结构。选择了三种单克隆抗体,即2F11、13E11和14F10来代表该组。所有单克隆抗体都适用于流式细胞术、免疫荧光分析和免疫沉淀。2F11单克隆抗体的反应性也通过蛋白质印迹得到证实。使用13E11单克隆抗体证实了人肝细胞和肝肿瘤细胞系上CCX-CKR的内源性表达。有趣的是,13E11单克隆抗体与表达CCX-CKR的B300-19细胞结合导致CCX-CKR内化。
讨论
这组单克隆抗体有望在进一步研究这种沉默趋化因子受体的功能方面证明是有价值的,这些功能包括与淋巴细胞稳态以及肝癌生长和转移相关的功能。
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