首页> 外文期刊>Biochimica et biophysica acta. Biomembranes >Use of peptide antibodies to probe for the mitoxantrone resistance-associated protein MXR/BCRP/ABCP/ABCG2
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Use of peptide antibodies to probe for the mitoxantrone resistance-associated protein MXR/BCRP/ABCP/ABCG2

机译:使用肽抗体探测抗米托蒽醌相关蛋白MXR / BCRP / ABCP / ABCG2

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摘要

Recent studies have characterized the ABC half-transporter associated with mitoxantrone resistance in human cancer cell lines. Encoded by the ABCG2 gene, overexpression confers resistance to camptothecins, as well as to mitoxantrone. We developed four polyclonal antibodies against peptides corresponding to four different epitopes on the mitoxantrone resistance-associated protein, ABCG2. Three epitopes localized on the cytoplasmic region of ABCG2 gave rise to high-affinity antibodies, which were demonstrated to be specific for ABCG2. Western blot analysis of cells with high levels of ABCG2 showed a single major band of the expected 72-kDa molecular size of ABCG2 under denaturing conditions. Immunoblot analysis performed under non-reducing conditions and after treatment with cross-linking reagents demonstrated a molecular weight shift from 72 kDa to several bands of 180 kDa and higher molecular weight, suggesting detection of dimerization products of ABCG2. Evidence of N-linked glycosylation was also obtained using tunicamycin and N-glycosidase F. Finally, both by light, fluorescence and electron microscopic immunohistochemical staining, we demonstrate cytoplasmic and predominantly plasma membrane localization f ABCG2 in cell lines with high levels of expression. Plasma membrane staining was observed on the surface of the chorionic villi in placenta. These results support the hypothesis that ABCG2 is an ABC half-transporter that forms dimers in the plasma membrane, functioning as an ATP-dependent outward pump for substrate transport.
机译:最近的研究已经表征了与人类癌细胞系中的米托蒽醌抗性有关的ABC半转运蛋白。由ABCG2基因编码,过表达赋予喜树碱和米托蒽醌抗性。我们开发了针对与米托蒽醌抗性相关蛋白ABCG2上四个不同表位相对应的肽的四种多克隆抗体。位于ABCG2细胞质区域的三个表位产生了高亲和力抗体,这些抗体被证明对ABCG2具有特异性。对具有高水平ABCG2的细胞进行的蛋白质印迹分析显示,在变性条件下,ABCG2的预期分子量为72 kDa的一条主带。在非还原条件下和用交联剂处理后进行的免疫印迹分析表明,分子量从72 kDa移至180 kDa的多个条带和更高的分子量,这表明检测到ABCG2的二聚化产物。也使用衣霉素和N-糖苷酶F获得了N-连接的糖基化的证据。最后,通过光,荧光和电子显微镜免疫组织化学染色,我们证明了在高表达水平的细胞系中细胞质和主要是质膜定位f ABCG2。在胎盘绒毛膜表面观察到质膜染色。这些结果支持以下假设:ABCG2是在质膜中形成二聚体的ABC半转运蛋白,起底物转运的ATP依赖性向外泵的作用。

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