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ReO4(-)与工程化 MoO4(2-)-结合蛋白的结合:迈向放射性药物应用的新方法。

Binding of ReO4(-) with an engineered MoO4(2-)-binding protein: towards a new approach in radiopharmaceutical applications.

机构信息

Department of Chemistry, Institute for Biophysical Dynamics, The University of Chicago, 929 East 57th Street, Chicago, IL 60637, USA.

出版信息

J Biol Inorg Chem. 2012 Jan;17(1):97-106. doi: 10.1007/s00775-011-0833-4. Epub 2011 Aug 23.

DOI:10.1007/s00775-011-0833-4
PMID:21861186
Abstract

Radiolabeled biomolecules are routinely used for clinical diagnostics. (99m)Tc is the most commonly used radioactive tracer in radiopharmaceuticals. (188)Re and (186)Re are also commonly used as radioactive tracers in medicine. However, currently available methods for radiolabeling are lengthy and involve several steps in bioconjugation processes. In this work we present a strategy to engineer proteins that may selectively recognize the perrhenate (ReO(4)(-)) ion as a new way to label proteins. We found that a molybdate (MoO(4)(2-))-binding protein (ModA) from Escherichia coli can bind perrhenate with high affinity. Using fluorescence and isothermal titration calorimetry measurements, we determined the dissociation constant of ModA for ReO(4)(-) to be 541 nM and we solved a crystal structure of ModA with a bound ReO(4)(-). On the basis of the structure we created a mutant protein containing a disulfide linkage, which exhibited increased affinity for perrhenate (K(d) = 104 nM). High-resolution crystal structures of ModA (1.7 Å) and A11C/R153C mutant (2.0 Å) were solved with bound perrhenate. Both structures show that a perrhenate ion occupies the molybdate binding site using the same amino acid residues that are involved in molybdate binding. The overall structure of the perrhenate-bound ModA is unchanged compared with that of the molybdate-bound form. In the mutant protein, the bound perrhenate is further stabilized by the engineered disulfide bond.

摘要

放射性标记的生物分子通常用于临床诊断。(99m)Tc 是放射性药物中最常用的放射性示踪剂。(188)Re 和 (186)Re 也常用于医学作为放射性示踪剂。然而,目前用于放射性标记的方法冗长且涉及生物缀合过程中的多个步骤。在这项工作中,我们提出了一种工程蛋白的策略,该蛋白可能选择性地识别高铼酸盐 (ReO(4)(-)) 离子作为标记蛋白的新方法。我们发现来自大肠杆菌的钼酸盐 (MoO(4)(2-)) 结合蛋白 (ModA) 可以与高铼酸盐高亲和力结合。使用荧光和等温滴定量热法测量,我们确定 ModA 与 ReO(4)(-) 的解离常数为 541 nM,并且我们解决了具有结合的 ReO(4)(-) 的 ModA 的晶体结构。基于该结构,我们创建了一个包含二硫键的突变蛋白,其对高铼酸盐表现出增加的亲和力 (K(d) = 104 nM)。用结合的高铼酸盐解决了 ModA(1.7 Å)和 A11C/R153C 突变体(2.0 Å)的高分辨率晶体结构。两种结构都表明,高铼酸盐离子使用参与钼酸盐结合的相同氨基酸残基占据钼酸盐结合位点。与钼酸盐结合形式相比,结合高铼酸盐的 ModA 的整体结构保持不变。在突变体蛋白中,结合的高铼酸盐进一步通过工程化的二硫键稳定。

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