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分子链上的配体:活细胞中抗体和底物与钠-葡萄糖协同转运蛋白SGLT1相互作用的单分子原子力显微镜研究

Ligands on the string: single-molecule AFM studies on the interaction of antibodies and substrates with the Na+-glucose co-transporter SGLT1 in living cells.

作者信息

Puntheeranurak Theeraporn, Wildling Linda, Gruber Hermann J, Kinne Rolf K H, Hinterdorfer Peter

机构信息

Institute for Biophysics, Johannes Kepler University of Linz, Altenbergerstrasse 69, A-4040 Linz, Austria.

出版信息

J Cell Sci. 2006 Jul 15;119(Pt 14):2960-7. doi: 10.1242/jcs.03035. Epub 2006 Jun 20.

DOI:10.1242/jcs.03035
PMID:16787940
Abstract

Atomic force microscopy (AFM) was used to probe topology, conformational changes and initial substrate-carrier interactions of Na+-glucose co-transporter (SGLT1) in living cells on a single-molecule level. By scanning SGLT1-transfected Chinese hamster ovary (CHO) cells with AFM tips carrying an epitope-specific antibody directed against the extramembranous C-terminal loop 13, significant recognition events could be detected. Specificity was confirmed by the absence of events in nontransfected CHO cells and by the use of free antigen and free antibody superfusion. Thus, contrary to computer predictions on SGLT1 topology, loop 13 seems to be part of the extracellular surface of the transporter. Binding probability of the antibody decreased upon addition of phlorizin, a specific inhibitor of SGLT1, suggesting a considerable conformational change of loop 13 when the inhibitor occludes the sugar translocation pathway. Using an AFM tip carrying 1-thio-D-glucose, direct evidence could be obtained that in the presence of Na+ a sugar-binding site appears on the transporter surface. The binding site accepts the sugar residue of the glucoside phlorizin, free D-glucose, and D-galactose, but not free L-glucose and probably represents the first of several selectivity filters of the transporter. This work demonstrates the potential of AFM to study the presence and dynamics of plasma membrane transporters in intact cells on the single molecule level.

摘要

原子力显微镜(AFM)用于在单分子水平上探测活细胞中钠-葡萄糖共转运蛋白(SGLT1)的拓扑结构、构象变化以及初始底物-载体相互作用。通过用携带针对膜外C末端环13的表位特异性抗体的AFM探针扫描转染了SGLT1的中国仓鼠卵巢(CHO)细胞,可检测到显著的识别事件。未转染的CHO细胞中无此类事件以及使用游离抗原和游离抗体灌注证实了特异性。因此,与关于SGLT1拓扑结构的计算机预测相反,环13似乎是转运蛋白细胞外表面的一部分。加入SGLT1的特异性抑制剂根皮苷后,抗体的结合概率降低,这表明当抑制剂阻断糖转运途径时,环13发生了相当大的构象变化。使用携带1-硫代-D-葡萄糖的AFM探针,可直接获得证据表明在存在Na+的情况下,转运蛋白表面出现一个糖结合位点。该结合位点可接受糖苷根皮苷的糖残基、游离D-葡萄糖和D-半乳糖,但不接受游离L-葡萄糖,可能代表转运蛋白多个选择性过滤器中的第一个。这项工作证明了AFM在单分子水平上研究完整细胞中质膜转运蛋白的存在和动态的潜力。

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