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Original Articles |
From the Cardiovascular and Urogenital Center of Excellence for Drug Discovery (G.H.T., A.R.O., R.E.B., K.A., H.W.K., R.N.W., P.J.G., B.M.J.), and Safety Assessment (R.C.M.), GlaxoSmithKline, King of Prussia, Pa.
Correspondence to Beat M. Jucker, PhD, GlaxoSmithKline, 709 Swedeland Rd, King of Prussia, PA 19406. E-mail beat.m.jucker{at}gsk.com
Received April 22, 2008; accepted September 5, 2008.
| Abstract |
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Methods and Results— Suprarenal aortic aneurysms were generated in apolipoprotein E–deficient mice administered angiotensin II (1000 ng/kg per min) for up to 28 days. In vivo MRI was performed serially (once weekly) to assess AAA development and rupture. Comparison of AAA size as measured by in vivo and ex vivo MRI resulted in excellent agreement (r=0.96, P<0.0001). In addition, MRI correlated with histology-derived AAA area assessment (in vivo versus histology: r=0.84, P<0.0001; ex vivo versus histology: r=0.89, P<0.0001). In a separate study, angiotensin II–administered apolipoprotein E–deficient mice were treated with doxycycline (broad-based matrix metalloproteinase inhibitor; 30 mg/kg per day for 28 days). MRI was able to noninvasively assess a reduced rate of AAA development (46% versus 71%, P<0.05), a decreased AAA area (2.56 versus 4.02 mm2, P<0.01), and decreased incidence of rupture (43% versus 100%) in treated versus control animals. Inhibition of aorta matrix metalloproteinase 2/9 activity was observed in the treated animals.
Conclusions— These results demonstrate the use of MRI to noninvasively and temporally assess AAA development on pharmacological intervention in this preclinical cardiovascular disease model.
Key Words: abdominal aortic aneurysms imaging MRI doxycycline MMP
| Introduction |
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1 cm and has a gross morphology consistent with a pseudoaneurysm, with 2 distinct regions: a remodeled adventitia that results in compression of the aortic lumen and a rupture of the medial vascular wall, which allows blood to flow into the remodeled adventitial space.8 The characterization of aneurysms in preclinical mouse models has been performed mostly through gross morphometry of the harvested aorta8,16 or histological evaluation of sectioned aortas.1,3,8 Although these methods provide morphological and immunohistochemical information, they are terminal measurements and, therefore, limit their use for studying the development and progression of AAAs. For this reason, ultrasound imaging has been used to assess AAA morphometry in mouse in vivo,17,18 but detailed morphological changes are difficult to determine because of limited sensitivity and/or poor signal to noise. MRI has been used to monitor aortic wall dimensions for studying atherosclerosis19,20 and the progression of aortic dilation at the sinus level in Marfan syndrome mice.21 Spontaneous aortic aneurysms in aged apolipoprotein E–deficient (apoE–/–) mice have been visualized via MRI.22 However, this earlier aneurysm study was performed at low magnetic field (2 T), did not use an intervention to drive AAA development (such as Ang II), and did not use bright-blood contrast to visualize blood flowing into the aneurysms. To date, there have been no reports of imaging studies examining pharmacological intervention on AAA development in mice.
In the current work, we use high magnetic field (9.4 T) MRI to follow the temporal development of AAAs in vivo. High-field MRI provides the means to track the progression of aneurysm development at greater contrast sensitivity and signal to noise than ultrasound. In addition, the imaging was optimized to visualize blood flow for the detection of aortic medial wall rupture, an additional measure of aneurysm severity. Following validation of the MRI technique, a pharmacological intervention study was performed using doxycycline, a broad spectrum matrix metalloproteinase (MMP) inhibitor, which was previously demonstrated to inhibit AAA development.4 The current study, to the authors knowledge, is the first use of bright-blood MRI to study in vivo AAA temporal development and pharmacological intervention on this development in an Ang II–infused mouse model.
| Methods |
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Study 1
To validate the in vivo MRI assessment of AAA development, a group of apoE–/– mice (n=20) were administered Ang II as stated above. Baseline MRI scanning followed by weekly scanning up to 28 days was performed. Animals with AAAs (n=10) as detected by MRI were euthanized and their aortas were formalin fixed in situ under fixed (110 mm Hg) pressure immediately after final scanning. At the end of study, necropsy was performed on the remaining animals to confirm that no AAAs were present.
Study 2
To evaluate the effect of pharmacological intervention on AAA development, apoE–/– mice were randomized into 2 groups (n=15 each) and dosed with either vehicle or doxycycline (broad spectrum MMP inhibitor,23 Sigma-Aldrich; 30 mg/kg per day) as a tool compound. Vehicle and doxycycline dosing were started on the same date. Doxycycline was prepared every other day and administered via drinking water and was used to profile the effects of a known inhibitor of AAA formation.4 MRI scanning was performed at baseline, then weekly for up to 28 days.
A necropsy was performed on animals that died or became moribund over the course of the study to determine whether an AAA was present. After the final week of scanning, animals were euthanized and tissues and blood were collected. Hearts and aortas were excised and washed with cold PBS, snap frozen in liquid nitrogen and stored at –80°C.
MRI
All scanning was performed using a 9.4-T small animal, vertical-bore magnet and BioSpec spectrometer (Bruker, Billerica, Mass) with an 89-mm imaging gradient set (100 gauss/cm) and a 30-mm whole-body mouse transmit/receive coil. Each animal was induced and maintained under isoflurane anesthesia (1% to 2%) in medical-grade air while respiration was continually monitored via a pillow sensor positioned under the abdomen (SA Instruments, Stoney Brook, NY). No physiological triggering was used for image acquisition.
Fast gradient-echo scout images were acquired in 3 orthogonal planes covering the abdominal aorta (repetition time/echo time [TR/TE], 137/2.7 ms transverse/coronal and 50/4.2 ms sagittal; matrix, 128x128; field of view, 3.0 cm; voxel resolution, 0.234x0.234x1 mm;
=30°; 4 excitations). Scout images were followed by a heavily flow-weighted angiographic true-coronal scout image in a plane containing the aorta and renal branches for use as landmarks to obtain true-transverse images through the abdominal aorta (TR/TE, 15/2.7 ms; matrix, 256x256; field of view, 3.0 cm; voxel resolution, 0.117x0.117x1 mm;
=60°; 16 excitations). Gradient echo scans were performed through the transverse plane of the abdominal aorta, encompassing 10 mm immediately superior to the right renal branch (TR/TE, 15/2.7 ms; matrix, 256x256; field of view, 3.0 cm; voxel resolution, 0.117x0.117x1 mm;
=30°; 10 slices; 8 excitations). The imaging parameters were chosen to provide bright-blood weighting, where flowing blood in the lumen appears brighter than the surrounding tissue. Flow compensation gradients were applied to remove motion artifacts from flowing blood within the lumen. The total imaging time per animal was
20 minutes.
For ex vivo imaging, vessels were removed from formalin fixative and rinsed with 0.2% Gd-DTPA (Magnavist, Berlex Labs, Wayne NJ) and transferred to a 5-mm glass nuclear magnetic resonance tube filled with 0.2% Gd-DTPA. Spin-echo images were acquired over the same region as the in vivo images (TR/TE, 300/10 ms; matrix, 256x256; field of view, 1 cm; voxel resolution, 0.039x0.039x1 mm; 10 slices; 4 excitations). After imaging, vessels were transferred to a solution of 70% ethanol in preparation for histology.
Histology
Histological staining was performed in the same region of abdominal aorta that was imaged to obtain morphometric data to correlate with both in vivo and ex vivo MRI data (n=8). AAA tissue was segmented into 3 (2.5-mm spacing) 5-µm-thick serial sections immediately proximal to the right renal branch. After sections were deparaffinized, rehydrated, and placed in 0.05 mol/L Tris buffer (pH=7.6), they were stained on a DAKO autostainer (DAKO Corporation, Carpenteria, Calif) using reagents from the catalyzed signal amplification system provided by DAKO. Serial sections were stained using a Masson trichrome (Santa Cruz Biotechnology Inc, Santa Cruz, Calif). A total of 19 sections contained a measurable aneurysm.
MMP Activity
The thoracic aorta was used to assess MMP activity as this region of aorta is activated by Ang II but did not contain aneurysms and therefore could be controlled for variability associated with AAA sections.24 Aortas were extracted for MMP quantitation by grinding in liquid nitrogen and followed by incubation for 18 hours at 4°C in 0.5% Triton X-100 (Sigma-Aldrich) in PBS containing 0.01% sodium azide (1:3 wt/vol) on a bench shaker. After extraction was complete, the samples were centrifuged at 14 000 rpm (10 minutes, 4°C) and the supernatants were collected. Protein concentration for each sample was determined with the BioRad DC protein assay kit (BioRad Laboratories, Hercules, Calif).
MMP enzyme activity was analyzed by sodium dodecyl sulfate polyacrylamide gel electrophoresis (SDS-PAGE) zymography as described previously.25 Enzyme activity of MMP-9 and MMP-2 was visualized as clear bands in a blue background and compared with human recombinant MMP-9 and MMP-2 standards (3 ng) (Chemicon, Temecula, Calif) that were run on the gels. The activity was determined in terms of inverse optical density units using Kodak Image Station 440C (Carestream, Rochester, NY).
Image Analysis
MRI image analysis was performed using Analyze AVW software (AnalyzeDirect, Leneka, Kans) and histological image analysis was performed using Image-Pro-Plus software (Media Cybernetics, Bethesda, Md). In the MRI images, the lumen and remodeled vessel wall of the AAA were traced separately for area measurements. In histological sections, the AAA was traced using the medial wall of the aorta and the collagen capsule separating the aneurysm from the adventitia as boundaries. Cross-sectional area measurement of all image slices through the aneurysm (defined as remodeling of vessel wall area >50% of lumen area) was performed to obtain the section with the largest aneurysm area. This single section of aneurysm was then analyzed serially throughout the study. For comparison between in vivo and ex vivo MRI images, area measurements (using the same procedure as the in vivo measurements) were made in both sets of data on 3 slices per aneurysm. MRI and histology sections were coregistered based on anatomic landmarks and distance from the right renal branch.
Analytic Analysis
End-of-study plasma doxycycline concentration was measured using a standard protein precipitation, and API-4000 LC/MS/MS (Applied Biosystems, Calif) and plasma lipid were measured using an Olympus AU640 chemical analyzer (Olympus America Inc, Melville, NY).
Statistical Analysis
All statistics (log-rank for survival and AAA development, Student t test for area measurement, correlations for AAA area and lumen comparisons) were performed using either the Prism (GraphPad, San Diego, Calif) software package for MRI or Microsoft Excel (Microsoft, Redmond, Wash) for zymography. P<0.05 was used for significance.
The authors had full access to the data and take responsibility for its integrity. All authors have read and agree to the manuscript as written.
| Results |
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In vivo and ex vivo cross-sectional areas of AAA and aortic lumen as determined by image analysis strongly correlated (r=0.96, P<0.0001, Figure 3A, and r=0.86, P<0.0001, Figure 3B, respectively). Statistically significant cross-sectional area correlations between histology and both in vivo MRI (r=0.83, P<0.0001, Figure 3C) and ex vivo MRI (r=0.88, P<0.0001, Figure 3D) were observed. These measures validate the accuracy of using MRI for quantitating in vivo aneurysm formation and progression in the mouse. In addition, the mean AAA area measured by ex vivo MRI was not different from that measured by in vivo MRI or histology (2.99±0.22 versus 2.87±0.22 versus 2.16±0.23 mm2, respectively).
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1 week of Ang II administration, study animals began to die or become moribund (Figure 4A). The percentage of animals that died or became moribund over the course of the study was 47% versus 33% (vehicle versus doxycycline, P=NS). Plasma cholesterol, low-density lipoprotein, and triglycerides were higher in the doxycycline versus vehicle group (P<0.05), with no difference in high-density lipoprotein. Plasma concentration of doxycycline at the end of the study was 282±33 ng/mL.
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Cross-sectional area of AAA measured from transverse image slices obtained at the same location were analyzed throughout the duration of the study. Weekly AAA areas of aneurysms detected in the end of study survivors for both groups are shown in Figure 5A. Aneurysm development was rapid on onset, but also exhibited continuous growth throughout the duration of the experiment. Doxycycline treatment resulted in a reduction of aneurysm size (P<0.05 at 2- and 4-week time points). The aorta lumen area changes due to remodeling of the vessel wall were also measured throughout the study. The doxycycline group had reduced lumen stenosis during the first 3 weeks of the study, after which the lumen size was reduced to a level similar to vehicle (Figure 5B).
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Effect of Doxycycline on MMP Inhibition
To confirm treatment with doxycycline resulted in reduced MMP activity, gel zymography was performed on thoracic aortas from both groups at end of study. Thoracic aorta was chosen to eliminate any bias because of the presence of macrophage-rich AAA tissue. After 4 weeks of treatment, the doxycycline group had lower levels of MMP2 (
38%, P<0.05), pro-MMP2 (
31%, P<0.05), and pro-MMP9 (
21%, P<0.05) activity, consistent with the reduced development of AAAs detected by MRI in this group.
| Discussion |
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In addition to visualization of adventitial remodeling, in vivo MRI reveals some degree of functional information about the aortic lumen. By using short MR pulse repetition times, excitation of fresh nuclear spins brought in by flowing blood results in higher MRI signal than in surrounding tissue. This bright-blood contrast allows for the effects of AAA development on the aortic lumen to be examined in vivo. Dilation of the lumen due to aorta medial rupture is a characteristic of AAAs in this model.8 Although the exact location of medial wall rupture is difficult to define by in vivo MRI given the 1-mm slice thickness in the present study, the technique provides for the visualization of blood flow into the dilated lumen. Although bright-blood contrast was implemented this study, the use of black-blood contrast where the vessel lumen appears dark compared with the surrounding tissue, would be of particular interest for examining the vessel wall as this technique would provide superior contrast in comparison with bright-blood imaging.26 However, in the present study, the interest was in luminal visualization and the effect of blood flow through medial breaks into the adventitial space rather than obtaining a detailed visualization of the remodeled aortic wall. In addition, black-blood imaging typically requires longer scanning times to produce optimal contrast, especially if physiological triggering is used.26 Because of the throughput required for preclinical serial imaging pharmacology studies, rapid scan times are beneficial. Full appreciation of the advantages and disadvantages of these 2 imaging methods in this animal model requires further investigation.
A second characteristic of the AAA described by Daugherty was remodeling of the media-adventitia interface. MRI provided adequate contrast to distinguish between the blood-filled luminal dilation and remodeled adventitia. The formation of a thrombus and degraded collagen within the adventitial space resulted in varying degrees of stenosis in the aorta immediately adjacent to the remodeled adventitia that could be monitored by MRI. Barisione et al17 reported luminal dilation in aortas with AAAs detected by ultrasound; however, ultrasound lacks the contrast sensitivity of MRI and may not be able to distinguish between the compressed lumen and the remodeled wall. We also detected an absence of extravasation of blood into the adventitial space in some animals. Similar aneurysms have been reported previously in apoE–/– mice fed a high fat diet.9 In these AAAs evidence of the medial rupture typically reported in this model was absent at the time of the initial detection of the aneurysm and throughout the subsequent weekly scans.
The in vivo images often yielded distinct structures within the remodeled adventitia. These structures were also found in the ex vivo images in the same segment of the aorta. Trichrome staining revealed differences in ex vivo MR contrast, which corresponded to either collagen (dark in the MR images) or thrombus (light in the MR images). The composition of aneurysms determined by histology was similar to that found in previous studies.8 Variations in MR contrast within the aneurysm could yield valuable information on AAA development beyond changes in gross morphology and blood flow. Changes in composition of the remodeled adventitia and the presence and size of thrombus in relation to the presence or absence of an aorta medial rupture reflects pathological changes in the early development of AAAs that could potentially be followed by repeated scanning during the early stage of aneurysm development. Further, the parameters used in this study were optimized to emphasize blood flow. Variations in the weighting of image contrast and the use of black-blood imaging techniques could be further refined to allow greater emphasis on specific features of AAAs.
The use of this technique for pharmacological studies was clearly demonstrated by treating mice with the broad spectrum MMP inhibitor, doxycycline. Protection from doxycycline occurs most likely as a result of MMP-2 and MMP-9 inhibition both of which have been closely linked to AAA development.23,27,28 Over the 4 weeks of Ang II infusion, treatment effects of AAA development (P<0.05) and size could be detected (P<0.05). However, there were significant differences in time-to-aneurysm formation (P<0.01) and aneurysm size (P<0.05) after only 2 weeks. Because of the increased risk for mortality in this disease model, the longer animals are administered Ang II, the greater the chance group size differences could confound results. In our study, there was slight decrease in mortality, albeit nonsignificant, in the treatment versus vehicle group (33% versus 47%, respectively). In previous studies published by Daugherty et al,17 a range of mortality has been reported from as low as 10% up to 40%. One inherent limitation in this model is that not every animal given Ang II will develop an AAA during the 28-day dosing period. In an earlier study by Manning et al4 using a similar protocol, after 4 weeks of Ang II infusion, 86% of the vehicle mice versus 35% of the doxycycline treated mice generated AAAs. In the current study, 71% of the vehicle and 46% of the treated mice produced AAAs. A potential explanation for the differences between the 2 studies may be in the age (28 weeks in the present study versus 8 weeks) and/or strain (apoE–/– in the present study versus low-density lipoprotein–/–) of the mouse model used. A detailed comparison of AAA development between the 2 strains of mice has not been performed.
In summary, MRIs potential for noninvasively and temporally assessing AAA development and drug efficacy in this preclinical cardiovascular disease model was presented. MR images yielded multiple end points including morphometry and composition, whereas bright-blood contrast allowed the visualization of blood flow into the remodeled adventitia as a consequence of a rupture of the media. The ability to evaluate AAAs in vivo provides a mechanism for refining drug studies in this model. By obtaining serial data on AAA progression, future optimization of study design with proper statistical power while adjusting for incidence of mortality may be performed. In addition, AAA development may be tracked serially in the same animals resulting in the use of fewer animals to assess AAA modulation. The use of MRI to refine drug studies in the preclinical discovery phase may provide valuable input for clinical advancement decision making using a technology that is clinically translatable.
| Acknowledgments |
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Sources of Funding
All funding for this research was provided by GlaxoSmithKline.
Disclosures
All authors are employed by GlaxoSmithKline.
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