Molecular Imaging of the Initial Inflammatory Response in AtherosclerosisImplications for Early Detection of DiseaseFrom the Division of Cardiovascular Medicine (B.A.K., C.L.C., J.T.B., A.X., Q.Y., S.C., E.S.C., J.K., J.R.L.), Oregon Health & Science University Portland; and the Department of Tumor Biology and Angiogenesis (S. Bullens, S. Bunting), Genentech Inc, South San Francisco, Calif.
Correspondence to Jonathan R. Lindner, MD, Cardiovascular Division, UHN-62, Oregon Health & Science University, 3181 SW Sam Jackson Park Rd, Portland, OR 97239. E-mail lindnerj@ohsu.edu
Background—We hypothesized that molecular imaging of endothelial cell adhesion molecule expression could noninvasively evaluate prelesion atherogenic phenotype. Methods and Results—Mice deficient for the LDL-receptor and the Apobec-1 editing peptide (DKO mice) were studied as an age-dependent model of atherosclerosis. At 10, 20, and 40 weeks of age, ultrasound molecular imaging of the proximal thoracic aorta was performed with contrast agents targeted to P-selectin and VCAM-1. Atherosclerotic lesion severity and content were assessed by ultrahigh frequency ultrasound, histology, and immunohistochemistry. In wild-type mice at all ages, there was neither aortic thickening nor targeted tracer signal enhancement. In DKO mice, lesions progressed from sparse mild intimal thickening at 10 weeks to widespread severe lesions with luminal encroachment at 40 weeks. Molecular imaging for P-selectin and VCAM-1 demonstrated selective signal enhancement (P<0.01 versus nontargeted agent) at all ages for DKO mice. P-selectin and VCAM-1 signal in DKO mice were greater by 3-fold at 10 weeks, 4- to 6-fold at 20 weeks, and 9- to 10-fold at 40 weeks compared to wild-type mice. En face microscopy demonstrated preferential attachment of targeted microbubbles to regions of lesion formation. Conclusions—Noninvasive ultrasound molecular imaging of endothelial activation can detect lesion-prone vascular phenotype before the appearance of obstructive atherosclerotic lesions. Contrast ultrasound molecular imaging of was used to determine whether prelesion proatherogenic phenotype could be imaged noninvasively by targeting VCAM-1 and P-selectin expression in a mouse model of atherosclerosis. Adhesion molecule expression was detected by molecular imaging at the earliest stages of plaque development, indicating that molecular imaging could be used to detect initial atherosclerotic events.
The inflammatory response plays an important role in the initiation and progression of atherosclerosis and the susceptibility to acute ischemic syndromes. Novel methods for detecting vascular inflammation are being developed to better ascertain risk for adverse events. One strategy is to directly visualize the molecular or cellular components of the immune response with targeted imaging probes. This approach could also potentially be used for early identification of individuals predisposed to severe atherosclerosis by detecting phenotypic changes that occur decades before clinical manifestations arise.1 The aim of this study was to test whether the early and inciting events of atherosclerosis can be detected in vivo by molecular imaging. The targets for this study, VCAM-1 and P-selectin, are key endothelial cell adhesion molecules that regulate leukocyte trafficking in atherosclerosis.2–5 Surface expression of both of these molecules occurs in response to oxidized LDL cholesterol and are present early at lesion-prone sites.2–10 Most targeted imaging technologies have been tested in models where plaque formation and inflammatory cell influx are advanced. However, ex vivo microscopy studies have demonstrated that imaging probes targeted to VCAM-1 or P-selectin accumulate in early atherosclerotic lesions.11,12 In this study, we hypothesized that molecular imaging in vivo could detect upregulation of adhesion molecules before the development of advanced atherosclerotic lesions. To test our hypothesis, targeted imaging and histomorphometric analysis were performed at various ages in mice with a genetic deletion of both the LDL receptor and the apolipoprotein (Apo) mRNA editing protein Apobec-1 that is responsible for preferential transcription of ApoB-48 over ApoB-100 in mice.13,14 These double knockout (DKO) mice have high circulating LDL cholesterol with full-length ApoB-100 and develop a predictable age-dependent course of atherosclerosis in the proximal aorta and all branch points while on a chow diet.14
Study Design The study was approved by the Animal Care and Use Committee of the Oregon Health & Science University. Control wild-type C57Bl/6 mice and DKO mice with gene-targeted deletion of the LDL receptor and Apobec-1 on a C57Bl/6 background underwent imaging studies at 10, 20, or 40 weeks of age (n=7 to 10 for each strain at each age) (Genentech, San Francisco, Calif.). Approximately half of the mice were euthanized after either the 10 or 20 weeks imaging study for aortic histomorphometry and immunohistochemistry for adhesion molecule expression. Total lesion area from en face oil red O staining of aortic whole mounts was performed in an additional 15 DKO mice (n=5 for each age). Spatial characterization of adhesion for fluorescently-labeled targeted microbubbles was assessed from ex vivo microscopy of the aortic arch in DKO mice. Microbubble Preparation Targeted Imaging of VCAM-1 and P-Selectin Plaque Morphometry by Ultrasound Ex Vivo Imaging of Microbubble Adhesion Histology Statistical Analysis
Cardiac Performance and Aortic Flow Velocities On echocardiography left ventricular fractional shortening, aortic internal diameter, and aortic peak systolic flow velocities were similar for DKO and wild-type mice at each age (Table). These data indicate that hemodynamic and shear rates that can influence microbubble adhesion in the aorta were similar between groups.
Vessel Morphometry and Histology
Vessel wall thickness measured by ultrahigh frequency ultrasound of was 60 μm in wild-type mice and did not change with age (Figure 2, supplemental Video I). In DKO mice, wall thickness at 10 weeks of age was similar to wild-type mice. At 20 weeks, there was a small increase in arterial wall thickness in DKO mice that did not reach statistical significance, indicating that the small lesions seen on histology could not be reliably detected by high-frequency ultrasound. At 40 weeks of age, ultrasound detected marked arterial thickening of the lesser curvature of the aorta and focal plaque formation at the proximal brachiocephalic artery (Figure 2, supplemental Video II).
On immunohistochemistry for VCAM-1, there was minimal staining in wild-type mice at all ages. In DKO mice, VCAM-1 was present on the intimal surface at 10, 20, and 40 weeks of age (Figure 3A through 3D). At 40 weeks of age, VCAM-1 was particularly intense on the endothelium at shoulder regions and within the complex lesions containing immune cells. Aortic whole mounts with in vivo labeling with P-selectin-targeted Q-dots demonstrated endothelial surface expression of P-selectin only in DKO mice, particularly at sites of lesion formation (supplemental Figure B).
Targeted Imaging of Adhesion Molecule Expression CEU molecular imaging signal in the ascending aorta and arch of wild-type mice was similar between control microbubbles and targeted microbubbles (Figure 4A). In DKO mice there was selective signal enhancement for P-selectin and VCAM-1-targeted microbubbles compared to control microbubbles at 10, 20, and 40 weeks of age. Signal from stationary targeted microbubbles occurred at both the specular edges of the vessel and "within the lumen" due to volume averaging of the entire mouse aorta within the elevational profile of the beam.16 P-selectin and VCAM-1 signal in DKO mice was greater than wild-type controls at all time points. The ratio of targeted signal in DKO mice versus control mice increased with age (approximately 3-fold greater at 10 weeks, 4- to 6-fold greater at 20 weeks, and 9- to 10-fold at 40 weeks). A diffuse pattern of enhancement throughout the aortic arch was seen in 40 weeks DKO mice (illustrated in Figure 4). Signal enhancement at the early time intervals (10 and 20 weeks) was often focal, illustrated in Figure 5, which also demonstrates how spatial localization was performed. A linear relation between the microbubble concentration and CEU intensity was found from in vitro water bath experiments (Figure 6).
Upregulation and surface expression of vascular endothelial cell adhesion molecules are early events in atherogenesis. Results from this study performed in a reproducible age-dependent murine model of aortic atherosclerosis indicate that molecular imaging of pathogenic endothelial cell adhesion molecules such as VCAM-1 and p-selectin can detect atheresclerotic vascular phenotype before the development of advanced lesions. Over the past decade, there has been increasing interest in the development of molecular imaging methods to assess the inflammatory response in atherosclerotic disease. Probe design has been governed by the intended clinical use. For example, the differentiation of high-risk "vulnerable" disease from more stable disease requires a technique that can detect the tempestuous late-stage events that contribute to plaque rupture or erosion. These events include macrophage infiltration, endothelial cell activation, protease activity, chemokine production, thinned fibrous cap, and increased metabolic activity. The aim of this study was to determine whether a molecular imaging approach could unmask early pathophysiologic changes and reveal risk for future development of severe disease. The scope of potential targets that can identify very early atherosclerosis is narrower than those for high-risk late-stage disease. One strategy has been to image the accumulation of oxidized lipoproteins in the vessel wall.17,18 In this study, our approach was to image the secondary inflammatory responses that occur in response to oxidized lipids by targeting microbubbles to adhesion molecules that are preferentially expressed at disease-prone regions.2–10 Interactions between P-selectin on the endothelial cell surface and modified glycoprotein counterligands on leukocytes mediates rolling and activation of leukocytes in postcapillary venules.19,20 These events are requisite for firm arrest and transmigration. Slow rolling and firm adhesion are, in part, mediated by interaction between leukocyte VLA-4 (4β1) and VCAM-1 on the endothelial surface. The selection of P-selectin and VCAM-1 as endothelial markers of early disease was based not solely on their importance in the inflammatory response. These molecules play a critical role in leukocyte arrest in high-shear stress vessels such as the mouse aorta,21 and participate in the early stages of atherogenesis.4,5 It has been previously shown that expression of endothelial cell adhesion molecules such as VCAM-1 and P-selectin in advanced atherosclerotic disease can be imaged in vivo with ultrasound or MRI targeted imaging probes.11,12,16,22,23 VCAM-1 signal intensity on CEU has been shown to correlate with the severity of diet-modulated vascular inflammation in late stage ApoE–/– mice.16 Feasibility for detecting disease at an early stage has been suggested by ex vivo optical imaging of aortas from ApoE–/– mice where accumulation of VCAM-1-targeted optical probes can be observed at the site nonobstructive atherosclerotic lesions.11,12 In the present study we show for the first time that it is possible to noninvasively image vascular inflammation in atherosclerosis at the onset of inflammatory cell entry into the vessel wall before the development of intimal xanthomas (fatty streaks). It was interesting to note that targeted signal enhancement in DKO mice was relatively consistent between ages, which could reflect a constant pattern of endothelial expression, despite and increase in intraplaque VCAM-1 signal exemplified in Figure 3. However, signal enhancement for microbubbles targeted to P-selectin and VCAM-1 in DKO relative to wild-type mice did increase with age, possibly reflecting a limitation in using a fixed dose of contrast agent rather than indexed to weight. The age-related increase in en face plaque area and cross-sectional plaque area on Movat staining outpaced the age-related increase in targeted signal for DKO versus wild type animals. Based on the spatial pattern of microbubble attachment, we believe that minimal increase in signal despite increasing plaque area could also reflect the preferential expression of adhesion molecules such as VCAM-1 that occurs at the margins rather than the central "dome" of plaques.6,7 We believe that the detection of very early immune responses is an ideal application for molecular imaging with a CEU approach. Because early identification of proatherogenic vascular phenotype is likely to be used as a screening tool, the brevity of CEU molecular imaging protocols and availability of ultrasound in the outpatient setting are practical advantages. Transition to humans will be contingent on development of probes suitable for human use in terms of conjugation chemistry and ligand composition such as peptides that have been discovered through phage-display screening.23 There are several limitations of this study that deserve attention. We cannot yet draw any conclusions regarding whether disease management can be improved by molecular imaging of the early inflammatory response. Although ultrahigh-frequency imaging was able to evaluate focal aortic thickening, the lower-frequency contrast-specific imaging method did not provide adequate spatial resolution to colocalize signal enhancement with degree of thickening. This issue is related to the small scale of the animal model used and the phenomenon of volume averaging that occurs when the full dimension of the mouse aorta fits within the beam elevation.16 It is likely that high-frequency ultrasound measurements overestimated the relative degree of aortic thickening in 40-week DKO mice compared to controls, largely because the axial resolution (approximately 50 to 70 μm) precluded true representation of normal wall dimensions. The data do, however, support the notion that molecular imaging can detect the molecular signature of disease before even the most sensitive of techniques for evaluating morphology. We also did not evaluate the relative contribution of platelets to p-selectin signal enhancement,24 although histology studies did not show evidence of significant platelet thrombi. In conclusion, we show that CEU molecular imaging can be used to noninvasively detect the expression of cell adhesion molecules that are involved in the early pathogenesis of atherosclerosis. These inflammatory changes can be imaged noninvasively before the development of advanced lesions. This method could in the future be useful for early risk stratification in atherosclerosis.
Sources of Funding These studies were supported by grants R01-HL-074443, R01-HL-078610, and R01-DK-063508 to Dr Lindner from the National Institutes of Health, and from a grant from Genentech Inc. Dr Kaufmann is supported by grant SNF 32323B_123919/1 from the Swiss National Science Foundation and a grant from the Lichtenstein Foundation. Dr Carr is supported by a Postdoctoral Fellowship Grant from the Pacific Mountain Affiliate of the American Heart Association. Dr Chadderdon is supported by a Fellow to Faculty Transition Award from the American Heart Association. Disclosures Dr Lindner serves on the Scientific Advisory Board for VisualSonics Inc.
Received May 7, 2009; accepted October 6, 2009.
1. Strong JP, Malcom GT, McMahan CA, Tracy RE, Newman WP, Herderick EE, Cornhill JF. Prevalence and extent of atherosclerosis in adolescents and young adults: implications for prevention from the Pathobiological Determinants of Atherosclerosis in Youth Study. JAMA. 1999; 281: 727–735. 2. Cybulsky MI, Iiyama K, Li H, Zhu S, Chen M, Iiyama M, Davis V, Gutierrez-Ramos JC, Connelly PW, Milstone DS. A major role for VCAM-1, but not ICAM-1, in early atherosclerosis. J Clin Invest. 2001; 107: 1255–1262.[Medline] [Order article via Infotrieve] 3. Dansky HM, Barlow CB, Lominska C, Sikes JL, Kao C, Weinsaft J, Cybulsky MI, Smith JD. Adhesion of monocytes to arterial endothelium and initiation of atherosclerosis are critically dependent on vascular cell adhesion molecule-1 gene dosage. Arterioscler Thromb Vasc Biol. 2001; 21: 1662–1667. 4. Johnson RC, Chapman SM, Dong ZM, Ordovas JM, Mayadas TN, Herz J, Hynes RO, Schaefer EJ, Wagner DD. Absence of P-selectin delays fatty streak formation in mice. J Clin Invest. 1997; 99: 1037–1043.[Medline] [Order article via Infotrieve] 5. Dong ZM, Chapman SM, Brown AA, Frenette PS, Hynes RO, Wagner DD. The combined role of P- and E-selectins in atherosclerosis. J Clin Invest. 1998; 102: 145–152.[Medline] [Order article via Infotrieve] 6. Iiyama K, Hajra L, Iiyama M, Li H, DiChiara M, Medoff BD, Cybulsky MI. Patterns of vascular cell adhesion molecule-1 and intercellular adhesion molecule-1 expression in rabbit and mouse atherosclerotic lesions and at sites predisposed to lesion formation. Circ Res. 1999; 85: 199–207. 7. Nakashima Y, Raines EW, Plump AS, Breslow JL, Ross R. Upregulation of VCAM-1 and ICAM-1 at atherosclerosis-prone sites on the endothelium in the ApoE-deficient mouse. Arterioscler Thromb Vasc Biol. 1998; 18: 842–851. 8. Khan BV, Parthasarathy SS, Alexander RW, Medford RM. Modified low density lipoprotein and its constituents augment cytokine-activated vascular cell adhesion molecule-1 gene expression in human vascular endothelial cells. J Clin Invest. 1995; 95: 1262–1270.[Medline] [Order article via Infotrieve] 9. Ramos CL, Huo Y, Jung U, Ghosh S, Manka DR, Sarembock IJ, Ley K. Direct demonstration of P-selectin- and VCAM-1-dependent mononuclear cell rolling in early atherosclerotic lesions of apolipoprotein E-deficient mice. Circ Res. 1999; 84: 1237–1244. 10. Mehta A, Yang B, Khan S, Hendricks JB, Stephen C, Mehta JL. Oxidized low-density lipoproteins facilitate leukocyte adhesion to aortic intima without affecting endothelium-dependent relaxation. Role of P-selectin. Arterioscler Thromb Vasc Biol. 1995; 15: 2076–2083. 11. Nahrendorf M, Jaffer FA, Kelly KA, Sosnovik DE, Aikawa E, Libby P, Weissleder R. Noninvasive vascular cell adhesion molecule-1 imaging identifies inflammatory activation of cells in atherosclerosis. Circulation. 2006; 114: 1504–1511. 12. McAteer MA, Schneider JE, Ali ZA, Warrick N, Bursill CA, von zur Muhlen C, Greaves DR, Neubauer S, Channon KM, Choudhury RP. Magnetic resonance imaging of endothelial adhesion molecules in mouse atherosclerosis using dual-targeted microparticles of iron oxide. Aterioscler Thromb Vasc Biol. 2008; 28: 77–83. 13. Farese RV, Véniant MM, Cham CM, Flynn LM, Pierotti V, Loring JF, Traber M, Ruland S, Stokowski RS, Huszar D, Young SG. Phenotypic analysis of mice expressing exclusively apolipoprotein B48 or apolipoprotein B100. Proc Natl Acad Sci U S A. 1996; 93: 6396–6398. 14. Powell-Braxton L, Veniant M, Latvala RD, Hirano KI, Won WB, Ross J, Dybdal N, Zlot CH, Young SG, Davidson NO. A mouse model of human familial hypercholesterolemia: markedly elevated low density lipoprotein cholesterol levels and severe atherosclerosis on a low-fat chow diet. Nat Med. 1998; 4: 934–938.[CrossRef][Medline] [Order article via Infotrieve] 15. Lindner JR, Song J, Christiansen J, Klibanov AL, Xu F, Ley K. Ultrasound assessment of inflammation and renal tissue injury with microbubbles targeted to P-selectin. Circulation. 2001; 104: 2107–2112. 16. Kaufmann BA, Sanders JM, Davis C, Xie A, Aldred P, Sarembock IJ, Lindner JR. Molecular imaging of inflammation in atherosclerosis with targeted ultrasound detection of vascular cell adhesion molecule-1. Circulation. 2007; 116: 276–284. 17. Tsimikas S, Palinski W, Halpern SE, Yeung DW, Curtiss LK, Witztum JL. Radiolabeled MDA2, an oxidation-specific, monoclonal antibody, identifies native atherosclerotic lesions in vivo. J Nucl Cardiol. 1999; 6: 41–53.[CrossRef][Medline] [Order article via Infotrieve] 18. Briley-Saebo KC, Shaw PX, Mulder WJ, Choi SH, Vucic E, Aguinaldo JG, Witztum JL, Fuster V, Tsimikas S, Fayad ZA. Targeted molecular probes for imaging atherosclerotic lesions with magnetic resonance using antibodies that recognize oxidation-specific epitopes. Circulation. 2008; 117: 3206–3215. 19. Ley K, Bullard DC, Arbones ML, Bosse R, Vestweber D, Tedder TF, Beaudet AL. Sequential contribution of L- and P-selectin to leukocyte rolling in vivo. J Exp Med. 1995; 181: 669–675. 20. Chigaev A, Waller A, Zwartz GJ, Buranda T, Sklar LA. Regulation of cell adhesion by affinity and conformational unbending of alpha4beta1 integrin. J Immunol. 2007; 178: 6828–6839. 21. Eriksson EE, Werr J, Guo Y, Thoren P, Lindbom L. Direct observations in vivo on the role of endothelial selectins and alpha(4) integrin in cytokine-induced leukocyte-endothelium interactions in the mouse aorta. Circ Res. 2000; 86: 526–533. 22. Hamilton AJ, Huang SL, Warnick D, Rabbat M, Kane B, Nagaraj A, Klegerman M, McPherson DD. Intravascular ultrasound molecular imaging of atheroma components in vivo. J Am Coll Cardiol. 2004; 43: 453–460. 23. Kelly KA, Allport JR, Tsourkas A, Shinde-Patil VR, Josephson L, Weissleder R. Detection of vascular adhesion molecule-1 expression using a novel multimodal nanoparticle. Circ Res. 2005; 96: 327–336. 24. Burger PC, Wagner DD. Platelet P-selectin facilitates atherosclerotic lesion development. Blood. 2003; 101: 2661–2666. |
|