Quantification of Macrophage-Driven Inflammation During Myocardial Infarction with 18F-LW223, a Novel TSPO Radiotracer with Binding Independent of the rs6971 Human Polymorphism

被引:45
|
作者
MacAskill, Mark G. [1 ,2 ]
Stadulyte, Agne [1 ,2 ]
Williams, Lewis [3 ]
Morgan, Timaeus E. F. [3 ]
Sloan, Nikki L. [3 ]
Alcaide-Corral, Carlos J. [1 ,2 ]
Walton, Tashfeen [1 ,2 ]
Wimberley, Catriona [2 ,4 ]
Mckenzie, Chris-Anne [5 ]
Spath, Nick [1 ]
Mungall, William [6 ]
BouHaidar, Ralph [7 ]
Dweck, Marc R. [1 ]
Gray, Gillian A. [1 ]
Newby, David E. [1 ]
Lucatelli, Christophe [2 ]
Sutherland, Andrew [3 ]
Pimlott, Sally L. [8 ,9 ]
Tavares, Adriana A. S. [1 ,2 ]
机构
[1] Univ Edinburgh, Univ BHP Ctr Cardiovasc Sci, Edinburgh, Midlothian, Scotland
[2] Univ Edinburgh, Edinburgh Imaging, Edinburgh, Midlothian, Scotland
[3] Univ Glasgow, WestCHEM, Sch Chem, Glasgow, Lanark, Scotland
[4] Univ Edinburgh, Ctr Clin Brain Sci, Edinburgh, Midlothian, Scotland
[5] Univ Edinburgh, MRC Edinburgh Brain Tissue Bank, Edinburgh, Midlothian, Scotland
[6] Univ Edinburgh, Biores & Vet Serv, Edinburgh, Midlothian, Scotland
[7] Univ Edinburgh, Forens Pathol, Edinburgh, Midlothian, Scotland
[8] Univ Glasgow, Sch Med, Glasgow, Lanark, Scotland
[9] NHS Greater Glasgow & Clyde, Glasgow, Lanark, Scotland
基金
英国工程与自然科学研究理事会;
关键词
TSPO; PET; macrophage; inflammation; myocardial infarction; POSITRON-EMISSION-TOMOGRAPHY; 18-KDA TRANSLOCATOR PROTEIN; BENZODIAZEPINE-RECEPTOR; RAT MODEL; 18; KDA; PET; NEUROINFLAMMATION; AFFINITY; MOUSE; MARKER;
D O I
10.2967/jnumed.120.243600
中图分类号
R8 [特种医学]; R445 [影像诊断学];
学科分类号
1002 ; 100207 ; 1009 ;
摘要
Myocardial infarction (MI) is one of the leading causes of death worldwide, and inflammation is central to tissue response and patient outcomes. The 18-kDa translocator protein (TSPO) has been used in PET as an inflammatory biomarker. The aims of this study were to screen novel, fluorinated, TSPO radiotracers for susceptibility to the rs6971 genetic polymorphism using in vitro competition binding assays in human brain and heart; assess whether the in vivo characteristics of our lead radiotracer, F-18-LW223, are suitable for clinical translation; and validate whether F-18-LW223 can detect macrophage-driven inflammation in a rat MI model. Methods: Fifty-one human brain and 29 human heart tissue samples were screened for the rs6971 polymorphism. Competition binding assays were conducted with H-3-PK11195 and the following ligands: PK11195, PBR28, and our novel compounds (AB5186 and LW223). Naive rats and mice were used for in vivo PET kinetic studies, radiometabolite studies, and dosimetry experiments. Rats underwent permanent coronary artery ligation and were scanned using PET/CT with an invasive input function at 7 d after MI. For quantification of PET signal in the hypoperfused myocardium, K-1 (rate constant for transfer from arterial plasma to tissues) was used as a surrogate marker of perfusion to correct the binding potential for impaired radiotracer transfer from plasma to tissue (BPTC). Results: LW223 binding to TSPO was not susceptible to the rs6971 genetic polymorphism in human brain and heart samples. In rodents, F-18-LW223 displayed a specific uptake consistent with TSPO expression, a slow metabolism in blood (69% of parent at 120 min), a high plasma free fraction of 38.5%, and a suitable dosimetry profile (effective dose of 20.5-24.5 mu Sv/MBq). F-18-LW223 BPTC was significantly higher in the MI cohort within the infarct territory of the anterior wall relative to the anterior wall of naive animals (32.7 +/- 5.0 vs. 10.0 +/- 2.4 cm(3)/mL/min, P <= 0.001). Ex vivo immunofluorescent staining for TSPO and CD68 (macrophage marker) resulted in the same pattern seen with in vivo BPFc analysis. Conclusion: F-18-LW223 is not susceptible to the rs6971 genetic polymorphism in in vitro assays, has favorable in vivo characteristics, and is able to accurately map macrophage-driven inflammation after MI.
引用
收藏
页码:536 / 544
页数:9
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