Targeting myeloperoxidase to stabilize unruptured aneurysm: an imaging-guided approach

To evaluate the inflammatory response in a rabbit model of aneurysm, carotid aneurysms were created in 59 New Zealand White rabbits. Animals were provided by Animal Experimental Center of North Sichuan Medical College, and randomly allocated to one of two groups as ABAH(+) (n = 31), or ABAH(-) (n = 28) using a computer-generated table of random numbers. Two groups were assigned to a study with or without 4-aminobenzoic acid hydrazide (ABAH, an irreversible inhibitor of MPO [30‐33]) respectively. Primary outcomes were defined as aneurysm wall signal intensity and aneurysm growth of 4 consecutive weeks after its creation based on MR imaging findings. Secondary outcomes were aneurysm wall histology, MPO activity and expression, and MMPs activity at week 1 and 4 after intervention.

The 59 male rabbits with a mean weight of 2.5 ± 0.5 kg and mean age of 16 weeks (± 3days) were housed at room temperature of 22–24 °C with a 12-hour light/dark cycle. The rabbits had free access to a hay diet as well as water. All animals received daily care in accordance with the local institutional guidelines. Animals allocated to the ABAH(+) groups were administered intraperitoneally with ABAH (40 mg/kg), twice daily [33] for 28 days, with same dose of saline to the ABAH(-) group. Rabbits with carotid artery embolism (which is detected in the subsequent MR imaging) or who is dead during the 4 follow-up weeks were excluded from the analysis. Figure 2, shown below, summarized the overall process.

Detailed technique of surgical creation of the carotid aneurysm have been described elsewhere [34]. Briefly, for rabbits undergoing surgery, anesthesia was induced with 4% isoflurane gas in a gas chamber, and maintained with 2% isoflurane via a face mask. Carotid aneurysms were created with 30 units of porcine pancreatic elastase (sigma, USA) retaining in the left common carotid artery for 20 min. All animals were given daily clopidogrel (1 mg/kg), heparin (100 U) for anti-coagulation [35], and penicillin (200,000 U) for anti-infection treatment for 7 days.

In this study, the inflammatory response was assessed by contrast-enhanced T1-weighted imaging using the MPO-activatable contrast agent Mn-TyrEDTA, which was prepared using a previously reported protocol [26]. The T1-relaxivity of Mn-TyrEDTA increases with increasing peroxidase activity (at 0.47 T, 32 °C, horseradish peroxidase (HRP) = 0 U, r₁ = 3.3 mmol^[-1s^[-1; HRP = 500 U, r₁ = 8.2 mmol^[-1s^[-1).

All animals were examined on a 3.0 T MR scanner (Discovery MR750, GE Medical System, Milwaukee, WI) with a Knee Coil under respiration-monitored. For rabbits undergoing MRI, anesthesia was induced with 4% isoflurane gas, and maintained at 2% isoflurane. Three-dimensional time of flight (3D TOF) MRA and T2-weighted (T2W) scans were performed to locate and evaluate the overall condition of the aneurysm before injection of the contrast agent. MPO-sensitive molecular MR imaging was performed to evaluate MPO activity within the lesion using Mn-TyrEDTA as the probe at a dosage of 0.1 mmol/kg injected intravenously at the ear margin in both groups of rabbits (n = 5). The duration of the acquisitions is 20 min. T1-weighted imaging (T1WI) was performed before and 0 min, 5 min, 10 min, 15 min, and 20 min post-injection of the probe, respectively. The sequence parameters are as follows: 3D TOF TR / TE = 22 ms / 5.7 ms; matrix = 320 × 256; flip angle (FA) = 20°; section thickness = 0.6 mm; bandwidth = 31.20 kHz; field of view (FOV) = 20 × 20 cm [2]; number of excitations (NEX = 1). T2-weighted FSE Parameters(with fat-suppression)TR / TE = 4241 ms / 72 ms; matrix = 288 × 192; flip angle (FA) = 142°; section thickness = 1 mm; bandwidth = 31.76 kHz; field of view (FOV) = 18 × 18 cm [2]; number of excitations (NEX = 3). T1-weighted FSE Parameters (with fat-suppression) TR / TE = 775 ms / 15 ms; matrix = 320 × 224; flip angle (FA) = 142°; section thickness = 1 mm; bandwidth = 31.65 kHz; field of view (FOV) = 10 × 10 cm [2]; number of excitations (NEX = 3).

The acquired images are transferred to a workstation (Advantage Workstation 4.4; GE Healthcare) and analyzed by an investigator who was blinded to the experimental groups. Regions of interest (ROIs) were then drawn manually on the slice showed the most enlarged arterial lumen for quantitative analysis. Signal intensity (SI) of the left carotid artery, the right carotid artery and adjacent muscle was measured before and after injection of contrast agents, and the noise was defined as the standard deviation (SD) of the signal in the air. Using the adjacent muscle as control, contrast-to-noise ratio (CNR) of the left aneurysmal lesion or right normal artery was calculated using the following formula: CNR = (SI_{left or right} - SI muscle)/SD_air; the enhancement attributable to MPO was then assessed by calculating the ΔCNR = CNR_{post-contrast} - CNR_pre-contrast. Vascular expansion rate = vascular diameter (largest on the ipsilateral) - vascular diameter (contralateral) / vascular diameter (contralateral position) × 100%.

Histology tests were performed by an investigator who was blinded to the experimental groups on two cohorts of ABAH (-) (n = 6; receiving saline vehicle) and ABAH (-) (n = 6) rabbits on days 7 and 28 after surgical creation of the carotid aneurysm. Rabbits were euthanized by an intraperitoneal overdose ( > = 100 mg/kg) of sodium pentobarbital. Carotid aneurysms were identified optically, isolated and dissected (with the contralateral artery as control). The tissue was fixed with 4% paraformaldehyde, embedded in paraffin (2–3 μm) and stained with Hematoxylin and eosin (HE) staining for overall histology. Neutrophils and macrophages were counted by professional pathologists. Masson staining and Elastin Van Gieson (EVG) staining were used to evaluate the content and integrity of collagen and elastic fibers of carotid aneurysms, respectively.

The MPO activity assay is based on the previously described method [36]. The carotid aneurysm was weighed, ground and homogenized in 0.5% sodium cetyl sulfate buffer, and then the homogenate was frozen/thawed four times, followed by centrifugation at 13,000 g at 4 °C for 20 min to obtain its supernatant. 10ul of supernatant was added to 3.0 ml of a solution which prepared by the following solution containing: 26.9 ml of water, 3.0 ml of sodium phosphate buffer solution (0.1 M, pH 7.0), 0.1 ml of H₂O₂ (0.1 M), and 0.048 ml of guaiacol. The optical density change(ΔOD) per minute is calculated from the second minute absorbance rate. The peroxidase activity was calculated according to the following equation: Activity = (OD × Vt × 4) / (E × t × Vs), E = 26.6 mM^[-1 cm^[-1 at 470 nm; OD = change in absorbance; Vt = total volume; Vs = sample volume and t = change in time. After measuring the total protein content in each sample, the results were expressed as U of MPO activity per gram of tissue. Horseradish peroxidase was used as a positive control.

The rabbit carotid aneurysm tissue, prepared as described earlier, were de-paraffinized, rehydrated and subjected to antigen retrieval. The sections were then incubated with rabbit anti-MPO (1:100, Bioss antibody, bs-4943R) overnight at 4 °C, FITC-labeled goat anti-rabbit secondary antibody (1:100, Servicebio, GB22303)was added and incubated at room temperature for 30 min. DAPI (ZSGB-BIO, ZLI-9557) was added at room temperature for 10 min to delineate nucleus. The sections were imaged using a microscopic camera system (3DHISTECH, CaseViewer 2.4).

One week postoperatively, the rabbits were euthanized. The carotid aneurysms were identified visually, isolated, dissected, and prepared as frozen sections as previous study demonstrated [37]. The contralateral artery incubated with ROS detecting kit build-in Rosup was used as a positive control. ROS production in aneurysms was detected by treating frozen section of arterial tissue with 10 µM of 2’,7’-dichlorodihydrofluorescein diacetate (DCFH-DA; Beyotime Biotechnology) and observing the fluorescence of DCFH (Ex: 488 nm, Em: 525 nm).

The activities of MMP-2 and MMP-9 in rabbit carotid aneurysms were detected by a MMP Zymography Assay Kit (Applygen). The protein sample obtained from arteries were loaded on to a gelatin-coated pre-casted polyacrylamide gel (Bio Rad). Electrophoresis was carried out under sodium dodecyl sulfate (SDS) at constant voltage. Gel was incubated with 2.5% Triton X-100 at room temperature for 2 h to remove SDS. Then the gel was washed 3 times to remove Triton X-100 and incubated at 37 ℃ in a developing buffer (Tris-HCl, pH 7.4) containing 10mM CaCl₂. 24 h later, the gel was stained with Coomassie Brilliant Blue R250. The metalloprotease activity was visualized after de-staining and then photographed. The intensity of the bands was quantitated by densitometry. Rabbit whole blood was used as a positive control.

All statistical analyses were calculated using the unpaired student’s t-test after F-test and S-W test were conducted and met. A p value of < 0.05 was considered significant. The data were statistically analyzed by SPSS 26 statistical analysis software. ImageJ (version 1.45s, National Institutes of Health, MD, USA) was used for image analysis. All values are expressed as mean ± SD.