K Goda, H Nagy, L Bene, M Balázs, R Arceci, E Mechetner, G Szabó
{"title":"Conformational heterogeneity of P-glycoprotein.","authors":"K Goda, H Nagy, L Bene, M Balázs, R Arceci, E Mechetner, G Szabó","doi":"","DOIUrl":null,"url":null,"abstract":"<p><p>P-glycoprotein (P-gp) acts as an active efflux mechanism for a large number of cytostatics and seems to be involved in the frequent failure of cancer chemotherapy. The molecular events of substrate recognition and transport still are not understood completely. We show here that the percentage of P-gp epitopes available for labeling with UIC2 monoclonal antibody is increased significantly after methanol permeabilization/fixation of cells. At the same time, binding of the MRK16 and 4E3 anti-P-gp antibodies is changed only moderately. Confocal microscopical images of UIC2-PE-labeled cells show that the epitopes becoming available after fixation are situated mainly in the plasma membrane. Thus, only a minority of P-gp molecules are accessible for UIC2 in the cell membrane of live cells, and methanol treatment can expose a large pool of previously plasma membrane-embedded, cryptic UIC2 epitopes. The UIC2-reactive P-gp molecules do not appear to be sequestered spatially, as suggested by the high fluorescence resonance energy transfer efficiency measured between the fluorescently labeled competing UIC2 and MRK16 antibodies, suggestive of P-gp dimerization and oligomerization on live cells.</p>","PeriodicalId":9499,"journal":{"name":"Cancer detection and prevention","volume":"24 5","pages":"415-21"},"PeriodicalIF":0.0000,"publicationDate":"2000-01-01","publicationTypes":"Journal Article","fieldsOfStudy":null,"isOpenAccess":false,"openAccessPdf":"","citationCount":"0","resultStr":null,"platform":"Semanticscholar","paperid":null,"PeriodicalName":"Cancer detection and prevention","FirstCategoryId":"1085","ListUrlMain":"","RegionNum":0,"RegionCategory":null,"ArticlePicture":[],"TitleCN":null,"AbstractTextCN":null,"PMCID":null,"EPubDate":"","PubModel":"","JCR":"","JCRName":"","Score":null,"Total":0}
引用次数: 0
Abstract
P-glycoprotein (P-gp) acts as an active efflux mechanism for a large number of cytostatics and seems to be involved in the frequent failure of cancer chemotherapy. The molecular events of substrate recognition and transport still are not understood completely. We show here that the percentage of P-gp epitopes available for labeling with UIC2 monoclonal antibody is increased significantly after methanol permeabilization/fixation of cells. At the same time, binding of the MRK16 and 4E3 anti-P-gp antibodies is changed only moderately. Confocal microscopical images of UIC2-PE-labeled cells show that the epitopes becoming available after fixation are situated mainly in the plasma membrane. Thus, only a minority of P-gp molecules are accessible for UIC2 in the cell membrane of live cells, and methanol treatment can expose a large pool of previously plasma membrane-embedded, cryptic UIC2 epitopes. The UIC2-reactive P-gp molecules do not appear to be sequestered spatially, as suggested by the high fluorescence resonance energy transfer efficiency measured between the fluorescently labeled competing UIC2 and MRK16 antibodies, suggestive of P-gp dimerization and oligomerization on live cells.
p -糖蛋白(P-gp)作为大量细胞抑制剂的主动外排机制,似乎与癌症化疗的频繁失败有关。底物识别和运输的分子事件仍未完全了解。我们在这里表明,在甲醇渗透/固定细胞后,可用UIC2单克隆抗体标记的P-gp表位的百分比显着增加。同时,MRK16和4E3抗p -gp抗体的结合仅发生适度变化。uic2 - pe标记细胞的共聚焦显微镜图像显示,固定后可用的表位主要位于质膜上。因此,只有一小部分P-gp分子可以被活细胞细胞膜上的UIC2所利用,而甲醇处理可以暴露出大量先前嵌入质膜的隐性UIC2表位。UIC2反应性P-gp分子在空间上并没有被隔离,正如在荧光标记的竞争型UIC2和MRK16抗体之间测量的高荧光共振能量转移效率所表明的那样,这提示了P-gp在活细胞上的二聚化和寡聚化。