|Extracorporeal shock wave therapy reverses ischemia-related left ventricular dysfunction and remodeling: molecular-cellular and functional assessment.|
|Jump to Full Text|
|PMID: 21915315 Owner: NLM Status: MEDLINE|
|An optimal treatment for patients with diffuse obstructive arterial disease unsuitable for catheter-based or surgical intervention is still pending. This study tested the hypothesis that extracorporeal shock wave (ECSW) therapy may be a therapeutic alternative under such clinical situation. Myocardial ischemia was induced in male mini-pigs through applying an ameroid constrictor over mid-left anterior descending artery (LAD). Twelve mini-pigs were equally randomized into group 1 (Constrictor over LAD only) and group 2 (Constrictor over LAD plus ECSW [800 impulses at 0.09 mJ/mm(2)] once 3 months after the procedure). Results showed that the parameters measured by echocardiography did not differ between two groups on days 0 and 90. However, echocardiography and left ventricular (LV) angiography showed higher LV ejection fraction and lower LV end-systolic dimension and volume in group 2 on day 180 (p<0.035). Besides, mRNA and protein expressions of CXCR4 and SDF-1α were increased in group 2 (p<0.04). Immunofluorescence staining also showed higher number of vWF-, CD31-, SDF-1α-, and CXCR4-positive cells in group 2 (all p<0.04). Moreover, immunohistochemical staining showed notably higher vessel density but lower mean fibrosis area, number of CD40-positive cells and apoptotic nuclei in group 2 (all p<0.045). Mitochondrial protein expression of oxidative stress was lower, whereas cytochrome-C was higher in group 2 (all p<0.03). Furthermore, mRNA expressions of MMP-9, Bax and caspase-3 were lower, whereas Bcl-2, eNOS, VEGF and PGC-1α were higher in group 2 (all p<0.01). In conclusion, ECSW therapy effectively reversed ischemia-elicited LV dysfunction and remodeling through enhancing angiogenesis and attenuating inflammation and oxidative stress.|
|Morgan Fu; Cheuk-Kwan Sun; Yu-Chun Lin; Ching-Jen Wang; Chiung-Jen Wu; Sheung-Fat Ko; Sarah Chua; Jiunn-Jye Sheu; Chiang-Hua Chiang; Pei-Lin Shao; Steve Leu; Hon-Kan Yip|
Related Documents :
|1959965 - Effect of zinc sulphate on infarct size in experimental myocardial infarction in dogs.
2375545 - The effect of parathyroid hormone on the acutely ischemic myocardium.
4062435 - Effect of cinpropazide on ischemic myocardial acidosis in dogs.
8371165 - Cyclocreatine inhibits neutrophil accumulation in the myocardium of a canine model of c...
7446425 - Clinical relevance of exercise-induced s-t segment elevation.
8573555 - Rate-dependent anisotropic conduction property in the epicardial border zone of canine ...
|Type: Journal Article; Research Support, Non-U.S. Gov't Date: 2011-09-06|
|Title: PloS one Volume: 6 ISSN: 1932-6203 ISO Abbreviation: PLoS ONE Publication Date: 2011|
|Created Date: 2011-09-14 Completed Date: 2012-02-14 Revised Date: 2013-06-27|
Medline Journal Info:
|Nlm Unique ID: 101285081 Medline TA: PLoS One Country: United States|
|Languages: eng Pagination: e24342 Citation Subset: IM|
|Division of Cardiology, Department of Internal Medicine, Kaohsiung Chang Gung Memorial Hospital and Chang Gung University College of Medicine, Kaohsiung, Taiwan.|
|APA/MLA Format Download EndNote Download BibTex|
High-Energy Shock Waves / therapeutic use*
Ventricular Dysfunction, Left / radiotherapy*
Ventricular Remodeling / radiation effects*
Journal ID (nlm-ta): PLoS One
Journal ID (publisher-id): plos
Journal ID (pmc): plosone
Publisher: Public Library of Science, San Francisco, USA
This is an open-access article, free of all copyright, and may be freely reproduced, distributed, transmitted, modified, built upon, or otherwise used by anyone for any lawful purpose. The work is made available under the Creative Commons CC0 public domain dedication.
Received Day: 18 Month: 2 Year: 2011
Accepted Day: 9 Month: 8 Year: 2011
collection publication date: Year: 2011
Electronic publication date: Day: 6 Month: 9 Year: 2011
Volume: 6 Issue: 9
E-location ID: e24342
PubMed Id: 21915315
Publisher Id: PONE-D-11-03564
|Extracorporeal Shock Wave Therapy Reverses Ischemia-Related Left Ventricular Dysfunction and Remodeling: Molecular-Cellular and Functional Assessment Alternate Title:Shock Wave Reverses Ischemic Heart Dysfunction|
1Division of Cardiology, Department of Internal Medicine, Kaohsiung Chang Gung Memorial Hospital and Chang Gung University College of Medicine, Kaohsiung, Taiwan
2Department of Emergency Medicine, E-Da Hospital, I-Shou University, Kaohsiung, Taiwan
3Division of General Surgery, Department of Surgery, Kaohsiung Chang Gung Memorial Hospital and Chang Gung University College of Medicine, Kaohsiung, Taiwan
4Center for Translational Research in Biomedical Sciences, Kaohsiung Chang Gung Memorial Hospital and Chang Gung University College of Medicine, Kaohsiung, Taiwan
5Department of Orthopedic Surgery, Kaohsiung Chang Gung Memorial Hospital and Chang Gung University College of Medicine, Kaohsiung, Taiwan
6Department of Radiology, Kaohsiung Chang Gung Memorial Hospital and Chang Gung University College of Medicine, Kaohsiung, Taiwan
7Division of Thoracic and Cardiovascular Surgery, Department of Surgery, Kaohsiung Chang Gung Memorial Hospital and Chang Gung University College of Medicine, Kaohsiung, Taiwan
8Department of Veterinary Medicine, National Pingtung University of Science and Technology, Pingtung, Taiwan
9Graduate Institute of Medicine, College of Medicine, Kaohsiung Medical University, Kaohsiung, Taiwan
|University of Modena and Reggio Emilia, Italy
|Correspondence: * E-mail: email@example.com
Contributed by footnote: Conceived and designed the experiments: MF YCL. Performed the experiments: CKS JJS CHC PLS. Analyzed the data: C.-J. Wang C-J. Wu SFK SC. Wrote the paper: SL HKY.
[other] ¶ These authors also contributed equally to this work.
Coronary artery disease (CAD), which develops initially from endothelial dysfunction followed by plaque formation and propagation before the development of obstructive syndrome, remains one of the most notorious killers in industrial counties , , . Despite the advance in pharmacological therapy , , mature technique of coronary artery bypass grafting (CABG) , , newly developed instrument-supported percutaneous coronary intervention (PCI) ,  for restoring myocardial perfusion, and current guideline focused on management strategy , restenosis due to preexisting systemic endothelial dysfunction and diffused vascular obstruction remain the Achilles' heel that limits therapeutic success and long-term prognostic outcome , , . Of importance is that quite a lot of patients suffering from diffuse obstructive CAD, for whom pharmacological treatment is of limited help, are not suitable candidates for interventional therapy through either PCI or CABG. The majority of these patients, therefore, are still in a helpless clinical situation. Hence, finding a safe and effective therapeutic regimen for patients who have diffuse obstructive CAD, especially those unsuitable for coronary intervention, is of utmost importance for cardiologists and cardiovascular surgeons.
Shock wave (SW) therapy can deliver a sequence of transient pressure disturbances characterized by high peak pressure (100 MPa), fast pressure rise (<10 ns), rapid propagation, and short lifecycle (10 µs) produced by an appropriate generator and directed to a specific target area with an energy density in the range of 0.003–0.890 mJ/mm2, , , . A number of studies have revealed that not only does SW provide mechanical means of treatment such as in lithotripsy for kidney and ureteral stones, but its low-energy form (0.03 to 0.11 mJ/mm2) also produces a series of subtle biological changes in the musculoskeletal ,  and cardiovascular system , , . Additionally, in vitro studies have demonstrated that extracorporeal (EC) SW therapy can enhance vascular endothelial growth factor (VEGF) mRNA expression in cultured human umbilical vein endothelial cells  and in rat bone marrow cells (BMCs)  as well as promote BMCs differentiation into cells with endothelial phenotype . Hence, by applying appropriate energy to ischemic organs  or tissues , , ECSW therapy can attenuate inflammatory response and induce angiogenesis/vasculognesis , , . Thus, ESCW therapy may provide promising therapeutic benefits in relieving the ischemic syndrome for patients with diffuse obstructive CAD who are not suitable candidates for interventional therapies. However, prior to utilization of ECSW for daily clinical practice, a pre-clinical experimental model for verifying its safety and efficacy is mandatory. This study utilized a mini-pig ischemic heart model to test the hypothesis that ECSW therapy may improve ischemia-related left ventricular (LV) dysfunction and attenuate LV remodeling.
All experimental animal procedures were approved by the Institute of Animal Care and Use Committee at Chang Gung Memorial Hospital – Kaohsiung Medical Center (Affidavit of Approval of Animal Use Protocol No. 2006121501) and performed in accordance with the Guide for the Care and Use of Laboratory Animals (NIH publication No. 85–23, National Academy Press, Washington, DC, USA, revised 1996).
Male mini-pig (Taitung Animal Propagation Station, Livestock Research Institute, Taiwan), weighting 16–18 kg, was anesthetized by intramuscular injections of ketamine (15 mg/kg) and maintained with an inhalation of 1.5% isoflurane during the procedures. After being shaved on the chest, the mini-pig was placed in supine position on a warming pad at 37°C followed by endotracheal intubation with positive-pressure ventilation (180 ml/min) with room air using a ventilator (Sn: Q422ZO, SIMS PneuPAC, Ltd.). Electrocardiographic (ECG) monitor and defibrillator were then connected to the chest wall.
Under sterile conditions, the heart was exposed through mid-thoracotomy. After gentle removal of the pericardium, an ameroid constrictor (Research Instruments NW, Inc. Lebanon, OR, USA) was applied to the mid-left anterior descending artery (LAD) just distal to the first diagonal branch. The constrictor constitutes an outer layer of stainless steel and an inner layer of fluid-absorbing casein that swells as it slowly absorbs body fluid to produce an inward concentric expansion. It usually required several weeks to create a significant stenosis over the mid-portion of LAD.
Neither regional ischemia nor wall motion abnormality was noted over LV anterior wall after the procedure. The absence of cardiac ischemia was further confirmed by complete ECG following the procedure. Ameroid constrictors were applied to mid-LAD in twelve mini-pigs which were equally divided into group 1 (Constrictor over LAD only) and group 2 [Constrictor over LAD plus ECSW (800 impulses at 0.09 mJ/mm2) after the procedure]. The muscle and skin were then closed in layers. The animals were allowed to remain on the warming pad and recover under care. A flowchart of the experimental procedure is shown in Figure 1.
To compare the findings at cellular-molecular level between normal and disease animals (i.e. groups 1 and 2), standard control samples were obtained from six healthy mini-pigs with similar age and body weight that served as normal controls.
By day 90 after the procedure, each mini-pig in group 2 was anesthetized again without intubation. ECSW therapy was applied to group 2 animals on day 90 after the procedure using the shock wave generator system (Cardiospec, Medispec, Israel). A cardiac ultrasound imaging system was used to locate the treatment areas of left ventricle. Under transthoracic sonographic guidance, shock waves were then delivered via a special applicator through the anatomical acoustic window to the treatment area under ECG R-wave gating. Briefly, after echocardiographic localization of the four ischemic zones of LV (i.e. middle anterior, middle anteroseptal, middle inferior, and middle inferolateral segments) using parasternal axis approach, ECSW was applied once to each of the four ischemic zones at an intensity of 200 impulses at 0.09 mJ/mm2/zone which was a dosage modified according to a previous report  so that the total energy applied to LV myocardium was 800 impulses at 0.09 mJ/mm2.
Transthoracic echocardiography was performed preoperatively and on days 90 and 180 after the procedure under general anesthesia as described previously  using an ultrasound system (Hewlett Packard SONOS 7500) equipped with 2.5 to 3.5 MHz linear probes. With the animals in a supine position, left ventricular internal dimensions [i.e. end-systolic diameter (ESD) and end-diastolic diameter (EDD)] were measured according to the American Society of Echocardiography leading-edge method using at least 3 consecutive cardiac cycles .
The LV ejection fraction (LVEF) was calculated as: LVEF (%) = [(LVEDD3−LVEDS3)/LVEDD3] x 100. All measurements were performed by a cardiologist blinded to treatment and non-treatment groups.
By six months following the procedure, cardiac catheterization was performed via right common carotid artery. A 6-French pigtail was used for measuring the arterial blood pressure in ascending aorta, LV systolic and end-diastolic pressure as well as for performing left ventriculography. Coronary angiographic study was achieved using a 6-French Kimny guiding catheter (Boston Scientific, Scimed, Inc. Maple Grove, MN).
Left ventriculography, which was immediately performed after the insertion of arterial sheath into right common carotid artery, was recorded at 30° right anterior oblique and 60° left anterior oblique views. The blood pressures of ascending aorta and LV chambers as well as LVEF were then determined.
The mini-pigs were sacrificed by intra-coronary injection of potassium chloride in catheterization room after the procedure. The heart was carefully removed for further studies.
Paraffin sections (3 µm thick) were obtained from LV myocardium of each mini-pig. To block the action of endogenous peroxidase, the sections were initially incubated with 3% hydrogen peroxide, and then further processed using Beat Blocker Kit (Zymed Company, #50–300) with immersion in solutions A and B for 30 minutes and 10 minutes, respectively, at room temperature. Polyclonal rabbit antibodies against CD40 (dilution 1/100; Spring Bioscience) were then used, followed by application of SuperPicTureTM Polymer Detection Kit (Zymed) for 10 minutes at room temperature. Finally, the sections were counterstained with hematoxylin. For negative control experiments, primary antibodies were omitted.
Immunohistofluorescence (IHF) staining for vWF-positive cells, an index of endothelial cells in capillaries, was performed with anti-vWF antibody (Chemicon).
The Oxyblot Oxidized Protein Detection Kit was purchased from Chemicon (S7150). The procedure was performed according to our recent study . The 2,4-Dinitrophenylhydrazine (DNPH) derivatization was carried out on 6 μg of protein for 15 minutes according to manufacturer's instructions. One-dimensional electrophoresis was carried out on 12% SDS/polyacrylamide gel after DNPH derivatization. Proteins were transferred to nitrocellulose membranes which were then incubated in the primary antibody solution (anti-DNP 1:150) for 2 hours, followed by incubation with second antibody solution (1:300) for one hour at room temperature. The washing procedure was repeated eight times within 40 minutes. Immunoreactive bands were visualized by enhanced chemiluminescence (ECL) which was then exposed to Biomax L film (Kodak). For quantification, ECL signals were digitized using Labwork software (UVP). On each gel, a standard control sample was loaded.
The LV myocardium was excised and then washed with buffer A (100 mM Tris-HCl, 70 mM sucrose, 10 mM EDTA and 210 mM mannitol, pH 7.4). Samples were minced finely in cold buffer A and then incubated for 10 min. All samples were homogenized in an additional 3 mL of buffer A using a motor-driven grinder. The homogenate was centrifuged twice at 700 g for 10 min at 4°C. The supernatant was centrifuged again at 8,500 g for 15 min, and the pellets were washed with buffer B (10 mM Tris-HCl, 70 mM sucrose, 1 mM EDTA, and 230 mM mannitol, pH 7.4). The mitochondria-rich pellets were collected and stored at −70°C.
Equal amounts (10–30 µg) of protein extracts from remote viable LV myocardium were loaded and separated by SDS-PAGE using 8–10% acrylamide gradients. Following electrophoresis, the separated proteins were transferred electrophoretically to a polyvinylidene difluoride (PVDF) membrane (Amersham Biosciences). Nonspecific proteins were blocked by incubating the membrane in blocking buffer (5% nonfat dry milk in T-TBS containing 0.05% Tween 20) overnight. The membranes were incubated with the indicated primary antibodies (Cx43, 1:1000, Chemicon; CXCR4, 1:1000, Abcam; SDF-1, 1:1000, Cell Signaling; cytochrome C, 1: 1000, BD Biosciences; Actin, 1:10000, Chemicon) for 1 h at room temperature for Cx43, cytochrome C and CXCR4 and overnight at 4°C for SDF-1α, respectively. Horseradish peroxidase-conjugated anti-mouse immunoglobulin IgG (1:2000, Amersham Biosciences) was applied as the second antibody for Cx43 for 1 h at room temperature; Horseradish peroxidase-conjugated anti-rabbit immunoglobulin IgG (1:2000, Cell Signaling) was applied as the secondary antibody for one hour for Cx43, cytochrome C and CXCR4 and 45 minutes for SDF-1α at room temperature. The washing procedure was repeated eight times within 1 h.
Real-time polymerase chain reaction (PCR) was conducted using LighCycler TaqMan Master (Roche, Germany) in a single capillary tube according to the manufacturer's guidelines for individual component concentrations. Forward and reverse primers were each designed based on individual exon of the target gene sequence to avoid amplifying genomic DNA.
During PCR, the probe was hybridized to its complementary single-strand DNA sequence within the PCR target. As amplification occurred, the probe was degraded due to the exonuclease activity of Taq DNA polymerase, thereby separating the quencher from reporter dye during extension. During the entire amplification cycle, light emission increased exponentially. A positive result was determined by identifying the threshold cycle value at which reporter dye emission appeared above background.
Immunohistochemical (IHC) staining of arterioles was performed with α-SMA (1:400) as primary antibody at room temperature for 1 h, followed by washing with phosphate buffered saline (PBS) thrice. The anti-mouse-horseradish peroxidase-conjugated (HRP) conjugated secondary antibody was then added for 10 min, followed by washing with PBS thrice. The 3, 3’ diaminobenzidine (DAB) (0.7 gm/tablet) (Sigma) was added for 1 minute, followed by washing with PBS thrice. Finally, hematoxylin was added for 1 minute as a counter stain for nuclei, followed by washing twice. Three coronal sections of the heart were analyzed in each mini-pig. For quantification, three randomly selected high-power fields (HPFs) (x200) were analyzed in each slide. The mean number per HPF for each animal was then determined by summation of all numbers divided by 9.
Masson's trichrome staining was used for studying fibrosis of LV myocardium. Three serial sections of LV myocardium were prepared at 4 µm thickness by Cryostat (Leica CM3050S). The integrated area (µm2) of fibrosis in the slides was calculated using Image Tool 3 (IT3) image analysis software (University of Texas, Health Science Center, San Antonio, UTHSCSA; Image Tool for Windows, Version 3.0, USA). Three selected sections were quantified for each animal. Three randomly selected HPFs (400 x) were analyzed in each section. After determining the number of pixels in each fibrotic area per HPF, the numbers of pixels obtained from the three HPFs were summed. The procedure was repeated in two other slides for each animal. The mean pixel number per HPF for each animal was then determined by summating all pixel numbers and dividing by 9. The mean the integrated area (µm2) of fibrosis in LV myocardium per HPF was obtained using a conversion factor of 19.24 (1 µm2 represented 19.24 pixels).
For each animal, 6 sections (3 longitudinal and 3 transverse sections of LV myocardium) were analyzed by an in situ Cell Death Detection Kit, AP (Roche) according to the manufacture's guidelines. The TUNEL-positive cells was examined in 3 randomly chosen HPF (×400) and normalized to the total number of cells divided by 18.
Data were expressed as mean values (mean ± SD). The significance of differences between two groups was evaluated with t-test. The significance of differences among the groups was evaluated using analysis of variance followed by Bonferroni multiple-comparison post hoc test. Statistical analyses were performed using SAS statistical software for Windows version 8.2 (SAS institute, Cary, NC). A probability value <0.05 was considered statistically significant.
There were no significant differences in initial and day 90 LVEDD, LVESD, left ventricular end-diastolic volume (LVEDV), left ventricular end-systolic volume (LVESV), LVEF and FS between group 1 (without ECSW therapy) and group 2 (with ECSW therapy) (Table 1). Moreover, LVEDD and LVEDV were similar between group 1 and group 2 on day 180 after the procedure. However, LVESD (2.97±0.58 vs. 2.24±0.31, p = 0.021) and LVESV (36.0±17.4 vs. 17.2±6.3, p = 0.032) were significantly higher, whereas LVEF (43.7±10.1 vs. 63.9±9.9, p = 0.006) and FS (20.9±5.5 vs. 36.1±7.3, p = 0.002) were significantly lower in group 1 than in group 2 on day 180 after the procedure. Furthermore, using paired two-tailed t-test for LVEDD between 90 day and 180 day in the same group, this parameter was found to be significantly reduced in group 2 (4.02±0.46 vs. 3.52±0.48, p = 0.043), but it showed no difference in group 1 (3.70±0.45 vs. 3.73±0.49, p = 0.897). These findings imply that ECSW therapy attenuated ischemia-related LV remodeling and improved ischemia-related LV dysfunction. Of importance is the fact that no ECSW therapy-related side effect was observed.
Six-month angiographic results showed that the systolic or diastolic blood pressure of ascending aorta and LV systolic pressure were similar between group 1 and group 2. However, LV end-diastolic pressure was remarkably higher (18.6±4.8 vs. 8.4±2.7, p<0.001), whereas LVEF (43.8±9.6 vs. 62.5±8.4, p = 0.004) was substantially lower in group 1 than in group 2 (all p<0.005). These findings further support the effect of ECSW therapy on inhibiting LV remodeling and improving LV function in the setting of myocardial ischemia.
Compared with normal controls, Western blotting revealed notably enhanced mitochondrial oxidative stress (Fig. 2A) in groups 1 and 2 (all p<0.001). Moreover, the protein expression of oxidative stress in mitochondria was remarkably increased in group 1 than in group 2 (p<0.05). The total cytochrome C protein expression in both mitochondria (Fig. 2B) and cytosol (Fig. 2C) did not differ between normal controls and group 2, whereas its expression in mitochondria was significantly reduced in group 1 as compared with normal controls and group 2 (all p<0.04). In contrast, its cytosolic expression was significantly enhanced in group 1 compared to normal controls and group 2 (all p<0.04). These findings indicate that the expression of cytochrome C, an index of energy supply and storage in mitochondria, was relatively well-preserved in group 2 compared with that in group 1. The increase in cytosolic cytochrome C content also suggests significant mitochondrial damage with cytochrome C release into the cytosol in the myocardium of group 1 animals. These findings highlight the fact that ECSW therapy significantly alleviated the intensity of oxidative stress resulting from free radical production due to a change in permeability of the mitochondrial transition pore after myocardial ischemia.
The protein expressions of CXCR4 (Fig. 2D), an index of endothelial progenitor cells (EPCs), and SDF-1α (Fig. 2E), a chemokine for EPCs homing in ischemic tissue, were remarkably higher in group 2 as compared with those in normal controls and in group 1, and notably higher in group 1 than in normal controls (all p<0.05). Moreover, VEGF (Fig. 2F), an index of chemokine for angiogenesis, was notably higher in group 2 than in both normal controls and group 1, and significantly higher in group 1 than in normal controls (all p<0.03). These findings indicate that EPCs, SDF-1α and VEGF were increased in response to ischemic stimuli and ECSW therapy enhanced these cellular and chemokine expressions for angiogenesis which, in turn, leaded to an increase in the number of endothelial cells in ischemic tissue.
The protein expression of Cx43 (Fig. 2G), an indicator of the integrity of signal transduction and communication between cardiomyocytes, was significantly lower in group 1 than in both normal controls and group 2, and was notably lower in group 2 than in normal controls (all p<0.005).
TUNEL assay (Fig. 3, A–D) identified notably higher number of apoptotic nuclei in group 1 than that in both normal controls and group 2, and remarkably higher in group 2 than in normal controls (all p<0.001). Furthermore, Masson's trichrome staining (Fig. 3, E–H) showed markedly increased fibrotic area in group 1 compared with that in normal controls and group 2, and significantly higher in group 2 than in normal controls (all p<0.0001). These findings may suggest that ECSW therapy attenuated cardiomyocyte death and myocardial fibrosis.
The results of IHF staining demonstrated that the numbers of CXCR4-, SDF-1α-, vWF-, and CD31-positive cells (Fig. 4 and 5) were remarkably higher in group 2 than in both normal controls and group 1 in LV myocardium (all p<0.001). Besides, the numbers of vWF- and CD31-positive cells (Fig. 4) were significantly higher in normal controls than in group 1 (all p<0.01). In contrast, the numbers of both CXCR4- and SDF-1α-positive cells (Fig. 5) were notably higher in group 1 than in normal controls (all p<0.01). IHC staining revealed that the number of small vessel (≤25 µm in diameter) (Fig. 6, A–D) was notably higher in group 2 than in both normal controls and group 1, and was significantly higher in normal controls than in group 1 (all p<0.002). On the other hand, IHC staining demonstrated that the number of CD40-positive cells (Fig. 6, E–H), an index of inflammation, was notably higher in group 1 than that in normal controls and group 2, and was significantly higher in group 2 than normal controls (all p<0.001). These findings indicate that ECSW therapy, in addition to enhancing angiogenesis, was effective in attenuating inflammatory response.
The mRNA expressions of vWF, SDF-1α, and CXCR4 (Fig.7, A–C) were notably higher in group 2 than in controls and group 1, and significantly higher in group 1 than in normal controls (all p<0.01). In addition, mRNA expression of IL-8/Gro (Fig. 7D), an EPC-homing chemokine, was notably elevated in group 2 than in normal controls and group 1, and notably higher in group 1 than in normal controls (all p<0.01).
NO is the molecule related to angiogenesis and anti-inflammation. The mRNA expression of eNOS (Fig. 7E), an index of NO production, was remarkably suppressed in group 1 compared with that in normal controls and group 2, and was notably lower in group 2 than that in normal controls (all p<0.03). Moreover, the mRNA expression of MMP-9 (Fig. 7F), a pro-inflammatory index, was significantly elevated in group 1 than that in normal controls and group 2, and notably higher in group 2 than in normal controls (all p<0.04). On the other hand, the mRNA expression of IL-10 (Fig. 7G), an anti-inflammatory index, was notably lower in group 1 than in normal controls and group 2, and significantly lower in group 2 than normal controls (all p<0.03). These findings suggest that ECSW therapy exerted an anti-inflammatory effect.
The mRNA expressions of Bax (Fig. 7H) and caspase 3 (Fig. 7I), two indicators of apoptosis, were substantially higher in group 1 than in normal controls and group 2, and significantly higher in group 2 than in normal controls (all p<0.02). Conversely, the mRNA expression of Bcl-2 (Fig. 7J), an index of anti-apoptosis, was notably lower in group 1 than in normal controls and group 2, and significantly lower in group 2 than in normal controls (all p<0.02). These findings imply that ECSW therapy was anti-apoptotic.
The mRNA expression of PGC-1α (Fig. 7K), a transcriptional coactivator for upstream regulator of lipid catabolism, oxidative metabolism, mitochondrial metabolism and biogenesis, was notably lower in group 1 than in both normal controls and group 2, and significantly lower in group 2 than in normal controls (all p<0.02). This finding implicates ECSW therapy reversed the downregulation in PGC-1α gene expression in ischemia heart disease.
This study, which investigated the impact of ECSW on ischemia-related LV dysfunction, provided several striking implications. First, ECSW therapy markedly increased EPCs and EPC homing-related chemokines in LV ischemic area, thereby enhancing angiogenesis. Second, ECSW therapy remarkably reduced inflammatory response, oxidative stress, cellular apoptosis, and fibrotic change in ischemic LV myocardium. Third, of importance is the fact that ECSW substantially reversed ischemia-related LV dysfunction and significantly attenuated ischemia-induced LV remodeling without any side effect.
Interestingly, while both clinical and experimental studies have clearly shown that ECSW therapy improved recovery of chronic hind limb ischemia and accelerated the healing process of ischemic skin ulceration , , , the effect of ECSW therapy on ischemia-related LV dysfunction has seldom been reported , . The most important finding in the current study is that ECSW treatment significantly reversed LV dysfunction and LV remodeling. Besides, it is a non-invasive procedure with absolute safety as demonstrated in the presented study. Practically, the treatment for patients with severe diffuse CAD , , so-called “end-stage coronary artery disease”, remains a vexing problem for interventional cardiologists and surgeons over several decades because the majority of these patients are not suitable candidates for either PCI or CABG. The results of our study, in addition to supporting those from recent clinical observational studies , , also highlight the therapeutic potential of ECSW for patients with severe diffuse-obstructive CAD unsuitable for PCI and CABG.
One previous animal study has revealed that application of ECSW in ischemic heart disease induced by restricting blood flow over left circumflex artery improved ischemia-related LV dysfunction through enhancing angiogenesis . Besides, another recent study using a myocardial ischemia-reperfusion injury model in pigs has demonstrated that ECSW therapy enhanced protein expressions of eNOS and VEGF in ischemic myocardium . However, evidence of angiogenesis after ECSW therapy was only supported by observation of an increased eNOS and VEGF in myocardium and angiographic findings of increased capillary density in that study , . Therefore, the precise mechanism underlying ECSW-induced angiogenesis is still unclear . One important finding in the present study is that the mRNA expressions of vWF, CXCR4, SDF-1α, eNOS, and IL-8/Gro were remarkably higher in group 2 (Constrictor over LAD plus ECSW) as compared with group 1 (Constrictor over LAD only). In addition, the protein expressions of VEGF, SDF-1α and CXCR4 were also notably higher in group 2 than in group 1. Moreover, IHF staining showed that the number of SDF-1α-, vWF-, CXCR4-, and CD31-positive cells were substantially higher in group 2 than in group 1. Furthermore, IHC staining for α-SMA demonstrated that the number of small vessel in LV myocardium was significantly higher in group 2 than in group 1. Our findings, in addition to reinforcing and extending the findings of the previous studies , , also support that angiogenesis may contribute to improved LV function after ECSW treatment.
The association among inflammation, reactive oxygen species, and cellular apoptosis/death has been fully investigated in the setting of myocardial ischemia , , . An important finding in the present study is the notably lower mRNA expression of MMP-9 and the remarkably elevated mRNA expression of IL-10 in LV myocardium after ECSW treatment on day 180 after the procedure. Furthermore, the significantly reduced oxidative stress and the suppression of CD40-positive cells in LV myocardium after ECSW administration imply significant roles of ECSW in attenuating inflammation and oxidative stress in ischemic myocardium.
Importantly, ECSW therapy also remarkably reduced the mRNA expressions of Bax and caspase 3 and significantly increased the mRNA expression of Bcl-2. The anti-apoptotic action of ECSW was further confirmed by TUNEL staining of LV myocardium. Furthermore, ECSW treatment also significantly reduced fibrosis of LV myocardium. Of importance is that ECSW therapy significantly preserved the level of PGC-1α gene expression and mitochondrial cytochrome C and maintained the protein expression of Cx43 in LV myocardium which have been shown to be depressed in the setting of dilated cardiomyopathy . These findings further strengthen the therapeutic potential of ECSW in reversing ischemia-related LV dysfunction and remodeling through inhibiting cellular apoptosis/death and myocardial fibrosis as well as preserving the integrities of Cx43 and energy biogenesis and metabolism which plays a key role in electrical coupling between cardiomyocytes , .
In conclusion, ECSW therapy significantly reversed ischemia-related LV remodeling and preserved LV function through enhancing angiogenesis, attenuating inflammation, and suppressing oxidative stress. The proposed mechanisms of potential impacts of ECSW therapy on preserving heart function in the porcine model have been summarized in Figure 8.
This study has limitations. First, since serial studies on the cause-and-effect relationship using different dosages of ECSW have not been performed, the optimal dosage for maximal therapeutic effects within safety margin is still unknown. Additionally, the sample size of the current study was relatively small. However, the impact of our results, on the other hand, is impressive. Second, this study did not investigate in details the mechanistic basis of ECSW therapy underlying the observed pro-angiogenic, anti-inflammatory, and anti-oxidant effects at molecular-cellular level. Further studies, therefore, may be warranted to clarify a cause-and-effect relationship when it comes to mechanistic findings of ESCW treatment against ischemic cardiac dysfunction and remodeling. Third, this study did not examine the effect of ECSW therapy on normal mini-pig myocardium. Thus, we did not provide information on the possibility of enhancement of angiogenesis through ECSW on normal mini-pig myocardium.
Competing Interests: The authors have declared that no competing interests exist.
Funding: This study was supported by a program grant from Chang Gung Memorial Hospital, Chang Gung University (grant no. CMRPG 870341). The funders had no role in study design, data collection and analysis, decision to publish, or preparation of the manuscript.
|1.||van der Wal AC,Becker AE,van der Loos CM,Das PK. Year: 1994Site of intimal rupture or erosion of thrombosed coronary atherosclerotic plaques is characterized by an inflammatory process irrespective of the dominant plaque morphology.Circulation8936448281670|
|2.||Epstein FH,Ross R. Year: 1999Atherosclerosis, Äî An Inflammatory Disease.New England Journal of Medicine3401151269887164|
|3.||Corti R,Fuster V,Badimon JJ. Year: 2003Pathogenetic concepts of acute coronary syndromes.J Am Coll Cardiol417S14S12644335|
|4.||Desai NR,Bhatt DL. Year: 2010The state of periprocedural antiplatelet therapy after recent trials.JACC Cardiovasc Interv357158320630450|
|5.||Boden WE,O'Rourke RA,Teo KK,Hartigan PM,Maron DJ,et al. Year: 2007Optimal medical therapy with or without PCI for stable coronary disease.N Engl J Med3561503151617387127|
|6.||Yusuf S,Zucker D,Peduzzi P,Fisher LD,Takaro T,et al. Year: 1994Effect of coronary artery bypass graft surgery on survival: overview of 10-year results from randomised trials by the Coronary Artery Bypass Graft Surgery Trialists Collaboration.Lancet3445635707914958|
|7.||Year: 1982Long-term results of prospective randomised study of coronary artery bypass surgery in stable angina pectoris. European Coronary Surgery Study Group.Lancet2117311806128492|
|8.||Yip HK,Wu CJ,Chang HW,Fang CY,Yang CH,et al. Year: 2003Effect of the PercuSurge GuardWire device on the integrity of microvasculature and clinical outcomes during primary transradial coronary intervention in acute myocardial infarction.Am J Cardiol921331133514636915|
|9.||Turco MA,Ormiston JA,Popma JJ,Mandinov L,O'Shaughnessy CD,et al. Year: 2007Polymer-based, paclitaxel-eluting TAXUS Liberte stent in de novo lesions: the pivotal TAXUS ATLAS trial.J Am Coll Cardiol491676168317448368|
|10.||Fraker TD Jr,Fihn SD,Gibbons RJ,Abrams J,Chatterjee K,et al. Year: 20072007 chronic angina focused update of the ACC/AHA 2002 Guidelines for the management of patients with chronic stable angina: a report of the American College of Cardiology/American Heart Association Task Force on Practice Guidelines Writing Group to develop the focused update of the 2002 Guidelines for the management of patients with chronic stable angina.Circulation1162762277217998462|
|11.||Manske CL,Wang Y,Rector T,Wilson RF,White CW. Year: 1992Coronary revascularisation in insulin-dependent diabetic patients with chronic renal failure.Lancet34099810021357450|
|12.||Detre KM,Guo P,Holubkov R,Califf RM,Sopko G,et al. Year: 1999Coronary revascularization in diabetic patients: a comparison of the randomized and observational components of the Aypass Angioplasty Revascularization Investigation (BARI).Circulation996336409950660|
|13.||Azar RR,Prpic R,Ho KK,Kiernan FJ,Shubrooks SJ Jr,et al. Year: 2000Impact of end-stage renal disease on clinical and angiographic outcomes after coronary stenting.Am J Cardiol8648548911009262|
|14.||Ogden JA,Toth-Kischkat A,Schultheiss R. Year: 2001Principles of shock wave therapy.Clin Orthop Relat Res81711400898|
|15.||Nishida T,Shimokawa H,Oi K,Tatewaki H,Uwatoku T,et al. Year: 2004Extracorporeal cardiac shock wave therapy markedly ameliorates ischemia-induced myocardial dysfunction in pigs in vivo.Circulation1103055306115520304|
|16.||Oi K,Fukumoto Y,Ito K,Uwatoku T,Abe K,et al. Year: 2008Extracorporeal shock wave therapy ameliorates hindlimb ischemia in rabbits.Tohoku J Exp Med21415115818285673|
|17.||Zimpfer D,Aharinejad S,Holfeld J,Thomas A,Dumfarth J,et al. Year: 2009Direct epicardial shock wave therapy improves ventricular function and induces angiogenesis in ischemic heart failure.J Thorac Cardiovasc Surg13796397019327525|
|18.||Ma HZ,Zeng BF,Li XL. Year: 2007Upregulation of VEGF in subchondral bone of necrotic femoral heads in rabbits with use of extracorporeal shock waves.Calcif Tissue Int8112413117629736|
|19.||Wang CJ,Wang FS,Yang KD,Weng LH,Hsu CC,et al. Year: 2003Shock wave therapy induces neovascularization at the tendon-bone junction. A study in rabbits.J Orthop Res2198498914554209|
|20.||Yip HK,Chang LT,Sun CK,Youssef AA,Sheu JJ,et al. Year: 2008Shock wave therapy applied to rat bone marrow-derived mononuclear cells enhances formation of cells stained positive for CD31 and vascular endothelial growth factor.Circ J7215015618159117|
|21.||Wang CJ,Huang HY,Pai CH. Year: 2002Shock wave-enhanced neovascularization at the tendon-bone junction: an experiment in dogs.J Foot Ankle Surg41162211858601|
|22.||Sahn DJ,DeMaria A,Kisslo J,Weyman A. Year: 1978Recommendations regarding quantitation in M-mode echocardiography: results of a survey of echocardiographic measurements.Circulation5810721083709763|
|23.||Sun CK,Chang LT,Sheu JJ,Chiang CH,Lee FY,et al. Year: 2009Bone marrow-derived mononuclear cell therapy alleviates left ventricular remodeling and improves heart function in rat-dilated cardiomyopathy.Crit Care Med371197120519242323|
|24.||Aicher A,Heeschen C,Sasaki K,Urbich C,Zeiher AM,et al. Year: 2006Low-energy shock wave for enhancing recruitment of endothelial progenitor cells: a new modality to increase efficacy of cell therapy in chronic hind limb ischemia.Circulation1142823283017145991|
|25.||Larking AM,Duport S,Clinton M,Hardy M,Andrews K. Year: 2010Randomized control of extracorporeal shock wave therapy versus placebo for chronic decubitus ulceration.Clin Rehabil2422222920156981|
|26.||Saggini R,Figus A,Troccola A,Cocco V,Saggini A,et al. Year: 2008Extracorporeal shock wave therapy for management of chronic ulcers in the lower extremities.Ultrasound Med Biol341261127118394777|
|27.||Ito Y,Ito K,Shiroto T,Tsuburaya R,Yi GJ,et al. Year: 2010Cardiac shock wave therapy ameliorates left ventricular remodeling after myocardial ischemia-reperfusion injury in pigs in vivo.Coron Artery Dis2130431120617568|
|28.||Wang Y,Guo T,Cai HY,Ma TK,Tao SM,et al. Year: 2010Cardiac shock wave therapy reduces angina and improves myocardial function in patients with refractory coronary artery disease.Clin Cardiol3369369921089114|
|29.||Kikuchi Y,Ito K,Ito Y,Shiroto T,Tsuburaya R,et al. Year: 2010Double-blind and placebo-controlled study of the effectiveness and safety of extracorporeal cardiac shock wave therapy for severe angina pectoris.Circ J7458959120134096|
|30.||Zeller M,Korandji C,Guilland JC,Sicard P,Vergely C,et al. Year: 2008Impact of asymmetric dimethylarginine on mortality after acute myocardial infarction.Arterioscler Thromb Vasc Biol2895496018276906|
|31.||Yip HK,Chang LT,Wu CJ,Sheu JJ,Youssef AA,et al. Year: 2008Autologous bone marrow-derived mononuclear cell therapy prevents the damage of viable myocardium and improves rat heart function following acute anterior myocardial infarction.Circ J721336134518654023|
|32.||Garrido AM,Griendling KK. Year: 2009NADPH oxidases and angiotensin II receptor signaling.Mol Cell Endocrinol30214815819059306|
|33.||Chua S,Sun CK,Yen CH,Ko SF,Chang LT,et al. Year: 2009Autologous transplantation of shock wave-treated bone marrow-derived mononuclear cells enhances vascularization and connexin43 expression in rat dilated cardiomyopathy.Acta Cardiol Sin256475|
|34.||Jalife J,Morley GE,Vaidya D. Year: 1999Connexins and impulse propagation in the mouse heart.J Cardiovasc Electrophysiol101649166310636196|
|35.||Vozzi C,Dupont E,Coppen SR,Yeh HI,Severs NJ. Year: 1999Chamber-related differences in connexin expression in the human heart.J Mol Cell Cardiol31991100310336839|
Table 1 Serial Echocardiography Findings and Six-Month Angiographic results of the Animals.
|Variables||Group 1*(n = 6)||Group 2*(n = 6)||p-value|
|Angiographic Results (Day-180)|
|SBP of AsAo (mmHg)||154.2±9.9||141.1±27.0||0.327|
|DBP of AsAo (mmHg)||123.6±6.20||101.9±22.3||0.06|
|180-day mortality||0% (0)||0% (0)||—|
|Malignant dysrhythmia||0% (0)||0% (0)||—|
Data are expressed as mean ±SD or %.
LVEDD = left ventricular end-diastolic dimension; LVESD = left ventricular end-systolic dimension; LVEDV = left ventricular end-diastolic volume; LVESV = left ventricular end-systolic volume; FS = fraction shortening; LVEF = left ventricular ejection fraction; SBP of AsAo = systolic blood pressure of ascending aorta; DBP = diastolic blood pressure; LVEDP = left ventricular end-diastolic pressure.
*group 1 = ischemia without extracorporeal shock wave (ECSW) treatment; group 2 = ischemia plus ECSW-treated.
Previous Document: Insecticide resistance and the future of malaria control in Zambia.
Next Document: Public availability of published research data in high-impact journals.