Sarver Ronald W, Gao Hua, Tian Fang
Discovery Technologies, Pfizer Global Research and Development, Ann Arbor, MI 48105, USA.
Anal Biochem. 2005 Dec 15;347(2):297-302. doi: 10.1016/j.ab.2005.09.039. Epub 2005 Oct 21.
An NMR method was developed for determining binding sites of small molecules on human serum albumin (HSA) by competitive displacement of (13)C-labeled oleic acid. This method is based on the observation that in the crystal structure of HSA complexed with oleic acid, two principal drug-binding sites, Sudlow's sites I (warfarin) and II (ibuprofen), are also occupied by fatty acids. In two-dimensional [(1)H,(13)C]heteronuclear single quantum coherence NMR spectra, seven distinct resonances were observed for the (13)C-methyl-labeled oleic acid as a result of its binding to HSA. Resonances corresponding to the major drug-binding sites were identified through competitive displacement of molecules that bind specifically to each site. Thus, binding of molecules to these sites can be followed by their displacement of oleic acids. Furthermore, the amount of bound ligand at each site can be determined from changes in resonance intensities. For molecules containing fluorine, binding results were further validated by direct observations of the bound ligands using (19)F NMR. Identifying the binding sites for drug molecules on HSA can aid in determining the structure-activity relationship of albumin binding and assist in the design of molecules with altered albumin binding.
开发了一种核磁共振(NMR)方法,通过(13)C标记油酸的竞争性置换来确定小分子在人血清白蛋白(HSA)上的结合位点。该方法基于以下观察结果:在与油酸复合的HSA晶体结构中,两个主要的药物结合位点,即Sudlow位点I(华法林)和位点II(布洛芬),也被脂肪酸占据。在二维[(1)H,(13)C]异核单量子相干NMR光谱中,由于(13)C-甲基标记的油酸与HSA结合,观察到七个不同的共振峰。通过特异性结合每个位点的分子的竞争性置换,确定了与主要药物结合位点相对应的共振峰。因此,分子与这些位点的结合可以通过它们对油酸的置换来跟踪。此外,每个位点结合配体的量可以根据共振强度的变化来确定。对于含氟分子,使用(19)F NMR直接观察结合的配体,进一步验证了结合结果。确定药物分子在HSA上的结合位点有助于确定白蛋白结合的构效关系,并有助于设计具有改变的白蛋白结合特性的分子。