Abstract
Cardiac stem cells (CSCs) play a vital role in cardiac remodeling. Uncontrolled hypertension leads to cardiac hypertrophy, followed by cardiac failure. Pathological remodeling is associated with enhanced oxidative stress. Decreased cardiac stem cell efficiency is speculated in heart diseases. Maintaining a healthy stem cell population is essential for preventing progressive cardiac remodeling. Some anti-hypertensive drugs are cardioprotective. However, the effect of these drugs on CSCs has not been investigated. Metoprolol is a cardioprotective anti-hypertensive agent. To examine whether metoprolol can prevent the deterioration of CSC efficiency, spontaneously hypertensive rats (SHRs) were treated with this drug, and the effects on stem cell function were evaluated. Six-month-old male SHRs were treated with metoprolol (50 mg × kg−1per day) for 2 months. The effectiveness of the treatment at reducing blood pressure and reducing hypertrophy was ensured, and the animals were killed. Cardiac stem cells were isolated from the atrial tissue, and the effect of metoprolol on stem cell migration, proliferation, differentiation, and survival was evaluated by comparing the treated SHRs with untreated SHRs and normotensive Wistar rats. Compared to the Wistar rats, the SHR rats presented with a decrease in stem cell migration and proliferation and an increase in intracellular oxidative stress and senescence. Treating SHRs with metoprolol increased CSC migration and proliferation potential and stemness retention. Cellular senescence and oxidative stress were reduced. The attributes of stem cells from the metoprolol-treated SHRs were comparable to those of the Wistar rats. The restoration of stem cell efficiency is expected to prevent hypertension-induced progressive cardiac remodeling.
Similar content being viewed by others
Introduction
Cardiac hypertrophy and failure are common cardiac sequelae of hypertension. Stem cells have a mediatory role in progressive cardiac remodeling. Compromised stem cell function has been implicated in different cardiac ailments [1], but the efficiency of stem cells in hypertensive heart disease has not been evaluated. Protecting the resident cardiac stem cell population as a prelude to preventing cardiac failure has not received much attention. Cycling stem cells for the replenishment of lost myocytes and the unfavorable microenvironment of the pathological heart can lead to stem cell aging. A decrease in the proportion of healthy stem cells can affect the reparative capacity. The role of stem cells in tissue regeneration is further highlighted by the observation of the positive effect of stem cell transplantation on myocardial regeneration [2]. The efficiency of c-kit+ cardiac stem cells was found to be impaired in disease models, implying the role of stem cells in maladaptive cardiac remodeling [1]. Only one report on a surgical model of hypertrophy exists in which the β-adrenergic blocker metoprolol induced the attenuation of LV remodeling in rat and was associated with an increased number of c-kit+ cells [3]. Metoprolol was more effective than an angiotensin receptor blocker, losartan [3]. However, functional changes in stem cells were not evaluated.
Beta-adrenergic blockers are beneficial for patients with symptomatic heart failure. Oxidative stress has been implicated in the pathogenesis of cardiovascular diseases [4, 5], including heart failure [6, 7]. Beta-blockers have antioxidant potential. Carvedilol decreased the serum levels of 8-OHdG by 19% [8] and of myocardial HNE-modified proteins by 40%, in addition to ameliorating the cardiac function of patients with heart failure [9]. Antioxidant β-blockers such as carvedilol and nebivolol attenuated oxidation and improved Prdx2 expression as well as increased the number of endothelial progenitor cells (EPCs) in the cardiovascular system of SHRs; in contrast, compared with carvedilol and nebivolol, short-term treatment with the angiotensin-II receptor blocker telmisartan had more beneficial effects on cardiovascular protection, EPC number, and Prdx2 expression [10]. Chronic β-receptor inhibition prevented cardiac remodeling in Dahl salt-sensitive hypertensive rats as effectively as renal denervation, despite maintaining blood pressure, thereby delinking blood pressure from cardiac remodeling [11]. Metoprolol is a cardioselective β1-adrenergic blocking agent. Cardiac hypertrophy regression and an increased life span have been reported in hypertensive individuals treated with metoprolol [12]. Experimental studies have shown that the continuous administration of β-receptor antagonists prevented the development of hypertension in growing SHRs [13]. Chronic metoprolol treatment markedly attenuated both cardiac and vascular remodeling in aging SHRs, thus preventing the onset of heart failure and improving survival, independent of blood pressure reduction [14]. The cause for the transition from adaptive remodeling to cardiac decompensation is enigmatic. Stem cell attribute deterioration is one of the causative factors of progressive cardiac remodeling. Based on the premise that stem cell function is compromised in hypertensive heart disease, this study was carried out to evaluate the efficiency of metoprolol in restoring stem cell attributes in SHRs.
Methods
Experimental design
Spontaneously hypertensive rats, a genetic model of hypertension and cardiac hypertrophy, were used for the experimental model and were compared with normotensive Wistar (WST) rats. Six-month-old male SHR and WST rats were housed at 22 °C, maintained on a 12 h light–dark cycle, fed with regular rat chow and given free access to drinking water. All animal procedures were approved by the Institutional Animal Ethics Committee, according to the Committee for the Purpose of Control and Supervision of Experiments on Animals (CPCSEA) guidelines.
Twelve male SHRs were randomly assigned to two groups of six rats each. Untreated SHRs served as the hypertensive control, and the other group received a daily oral dose of 50 mg × kg−1 per day of metoprolol tartrate for 2 months. Sex- and age-matched WST rat served as normotensive controls. To ensure treatment effectiveness, blood pressure and cardiac hypertrophy were assessed by echocardiography. Myocardial oxidative stress was assessed by lipid peroxidation assays. After establishing the cardioprotective and antioxidant effects of the metoprolol treatment, the cardiac stem cell response was evaluated.
Isolation and characterization of cardiac stem cells
c-kit+ cardiac stem cells (CSCs) were isolated following a previously reported protocol, with minor modifications [15, 16]. The atria were washed in phosphate-buffered saline (PBS), minced into small pieces (1 mm3) and plated onto 2% gelatin-coated culture plates. The explants were grown in Iscove’s modified Dulbecco’s medium (IMDM) supplemented with 10% fetal bovine serum (FBS) and antibiotics. The phase-bright cells that migrated out of the explants were dissociated by mild trypsinization, and c-kit+ CSCs were sorted by immunomagnetic isolation using an Easy Sep magnet and FITC-positive selection kit (Stem Cell Technologies, Canada). The sorted cells were cultured with IMDM containing 10% FBS, 10 ng/mL bFGF, and insulin–selenium–transferrin mixture at 37 °C in a humidified atmosphere with 5% CO2. Cells from passage 3 were used for further experiments.
Immunostaining for the identification of c-kit+ stem cells was performed by incubating the cells with a rat-specific rabbit anti-c-kit (diluted 1:100, Santa Cruz Biotechnology, USA) at 4 °C overnight. The cells were then incubated with FITC-conjugated rat anti-rabbit IgG (diluted 1:250) at 25 °C for 1 h. The nuclei were stained with DAPI. The immunoreactions were observed using a fluorescence microscope.
Flow cytometric analysis for cell surface markers
Immunomagnetically isolated c-kit+ cells were fixed in 4% paraformaldehyde for 15 min at room temperature and were analyzed for the expression of cell surface markers. The collected cells were stained with FITC-conjugated antibodies against c-kit, CD34, and CD45 (Invitrogen, Carlsbad, CA), indicative of cardiac stem cells and endothelial and hematopoietic markers. IgG was used as the isotype control.
Clonogenic assay
Single-cell CSC suspensions were serially diluted to 50 cells in 10 mL of complete medium and seeded onto a 96-well plate at a density of 0.5 cells per well to generate single-cell clones. After 4 h, each well containing a single cell was identified under a light microscope and was examined for growing colonies twice weekly. After 2 weeks, the number of wells with clones derived from a single cell was counted. Clonogenicity was determined using the following formula:
Growth kinetics, growth rate, and population-doubling time
To determine the growth kinetics, 10,000 cells were seeded in 35 mm culture plates. Cells were dissociated by trypsinization, and the cell density was determined using a Neubauer improved hemocytometer from a minimum of three culture plates at 48 h intervals for 10 days. The growth kinetics were plotted. Population-doubling time (PDT) and growth rate (GR) were calculated. GR was determined with the following equation: GR = ln(Nt/N0)/T, where T is the incubation time, N0 is the cell number at the beginning of the incubation time, and Nt is the cell number at the end of the incubation time. Population-doubling time was calculated using the formula PDT = ln(2)/GR.
Colony-forming unit assay
CSCs were seeded onto 60 mm cell culture plates in triplicate at a density of 500 cells per plate. Culture medium was changed every 3–4 days. After 9 days, the cultures were washed with PBS and stained with 3% crystal violet in methanol for 30 min at room temperature. The number of colonies per plate was counted.
Cell migration assay
For trans-well migration assays, 1 × 104 cells were suspended in 300 µl of serum-free IMDM and seeded onto the upper chamber of transwells with an 8 µm pore size. Cells were allowed to migrate toward the IMDM containing 10% serum for 18 h; then, the cells on the upper surface of the membrane were wiped away, and the migrated cells on the lower surface of the membrane were fixed and stained. Cells were counted from six random fields, and the mean was calculated. Experiments were repeated three times.
Senescence-associated β-galactosidase staining
Senescence-associated β-galactosidase staining (β-Gal staining) was used as a biomarker of senescence. Β-Gal activity was assessed cytochemically using a staining kit (Abcam), and the percentage of senescent cells, as represented by positive staining, was calculated. The expression levels of senescence-associated proteins, p16ink4a, and p21, were detected by western blot analysis.
Cell differentiation assay
CSCs were seeded onto six-well plates. Cell differentiation was induced in semiconfluent cultures using azacytidine (IMDM, 10% FCS and 10 µM 5-azacytidine) for 2 weeks. The differentiation potential was determined by analyzing the expression of cell-specific markers (cardiac troponin I and smooth muscle a×ctin).
Western blotting analysis
Protein concentrations were determined by the Bradford assay. Equal amounts of protein were electrophoresed on 10% polyacrylamide SDS gels. Proteins were transferred onto nitrocellulose membranes and blocked for 1 h with 5% skimmed milk in Tris-buffered saline containing 0.1% Tween 20. Proteins were incubated with primary antibodies, followed by appropriate secondary antibodies. Protein bands were visualized by chemiluminescence, and images were quantified using ImageJ software. The expression of target proteins was normalized to the respective beta actin level.
Statistical analysis
Values are presented as the means ± SD. For comparisons between groups, ANOVA was followed by Student’s t test (two-tailed). Results were considered statistically significant when p values were <0.05.
Results
Cardiovascular response to treatment with metoprolol
Both the systolic and diastolic blood pressure of SHRs were significantly reduced in response to the metoprolol treatment (Table 1). Hypertrophy regression was apparent from the decreased relative wall thickness and lateral wall thickness. The reduced isovolumic relaxation time indicates functional improvement (Table 2). The decreased myocardial lipid peroxidation indicated a reduction in oxidative stress (Table 3). The values of treated SHRs were comparable to those of WST rats.
CSC isolation, culture, and characterization
After metoprolol treatment for 60 days, animals were killed, and the hearts were dissected under aseptic conditions. For isolating cardiac stem cells, the atria were separated from the ventricular tissue and were cultured as explants. Within 14 days, small, phase-bright cells that migrated from the explants were seen loosely attached over a layer of fibroblast-like cells. These cells were trypsinized and subjected to immunomagnetic isolation to sort the c-kit+ CSCs. Sorted cells were cultured in IMDM containing supplements and antibiotics. The purity of the cultured CSCs was confirmed in passage 3 by flow cytometry and immunocytochemistry. The analysis revealed that >90% of the cells were positive for c-kit and negative for the hematopoietic and endothelial markers CD45 and CD34 (Fig. 1). Culture stemness was further confirmed by clonogenicity assays, where 94 ± 4% of the cells formed single-cell colonies. Cultured CSCs from the third passage were used for further experiments.
Effect of metoprolol on CSC self-renewal capacity
Colony formation was significantly lower in CSCs from SHRs than in WST rat CSCs (Fig. 2a). However, after treatment with metoprolol, the ability of SHR CSCs to form colonies was significantly increased (p < 0.01 compared to the untreated control) and was comparable with that of WST rat CSCs (p = 0.2).
Effect of metoprolol on CSC growth kinetics, population-doubling time, and growth rate
Following 10 days in culture, the CSC yield from WST rats (126 ± 13 × 104 cells) was significantly greater than that obtained from SHRs (72 ± 5.5 × 104 cells). Treatment with metoprolol stimulated CSC proliferation, and the cell yield was comparable with that of WST rats (Fig. 2b). Growth rate and PDT, both of which were negatively affected in SHRs, were restored by the beta-blocker treatment (Fig. 2c, d).
Effect of metoprolol on CSC migration potential
The migratory capacity of CSCs from SHRs was 62% lower than that of WST rats, as evidenced by the trans-well migration assays (Fig. 3). Metoprolol enhanced the ability of CSCs to migrate by 72% and was comparable with the ability of WST rat CSCs.
Effect of metoprolol on intracellular Reactive oxygen species (ROS) levels in CSCs
Oxidative stress is implicated in hypertrophy. CSCs are also influenced by the oxidative stress in the surrounding milieu, which was apparent in the H2DCFDA fluorescence assay. CSCs from SHRs had significantly higher levels of ROS than CSCs from WST rats (Fig. 4). Metoprolol treatment decreased the ROS levels, comparable to that of normotensive rats.
Effect of metoprolol on CSC differentiation potential
The differentiation potential, as detected by the expression levels of cardiac troponin I and smooth muscle actin, were not significantly different among the three groups. CSCs from both SHRs and WSTs had comparable expression levels of both the proteins, and these levels remained unaffected by the metoprolol treatment (Fig. 5).
Effect of metoprolol on CSC senescence
The proportion of senescent CSCs was about threefold higher in SHRs than in WSTs, as identified by beta-galactosidase staining (Fig. 6a). The proportion of senescent cells was decreased in response to the treatment and was comparable with that in WSTs. Immunoblot analysis of p16ink4a and p21 also exhibited the same trend (Fig. 6b, c). The levels of both proteins were significantly higher in SHR CSCs than in WST CSCs. Metoprolol reduced the expression of these proteins, indicating the prevention of stem cell aging.
Discussion
Cardiac stem cells play a critical role in pathological remodeling [1]. It is now recognized that reactive oxygen species are involved in the pathophysiology of myocardial hypertrophy and failure [17]. There is evidence for increased oxidative stress in patients with heart failure and in animal models of pressure overload [18]. The adverse microenvironment that prevails in this disease condition can have a significant role in modulating stem cell characteristics. Hypertension and hypertrophy are assumed to affect the behavior of CSCs. c-kit+ CSCs were isolated from atrial explants by immunomagnetic isolation and were further expanded in culture to obtain a sufficient number of CSCs for experiments. Cell purity and stemness were assessed by immunostaining, clonogenic assays, and flow cytometric analysis (Fig. 1). CSCs from the third passage were used for assessing stem cell characteristics and efficiency. Previous studies have shown that even after long-term culture, up to 40 passages, c-kit+ CSCs maintain their characteristics in vitro [19]. Supporting this observation, epigenetic modifications characteristic of the somatic tissue of origin are retained in cultured, induced pluripotent stem cells [20]. Even after long-term culture, DNA methylation reflects the tissue of origin. DNA methylation patterns are maintained throughout the long-term culture of human MSCs [21]. These studies reiterate the contention that in vitro cultures of CSCs maintain their characteristics. Studies have shown that metoprolol’s anti-hypertensive response is mediated by downregulating the DNA methylation status [22].
Reduced hypertension was accompanied by hypertrophy regression and decreased oxidative stress (Tables 1, 2, and 3). Although the effect of oxidative stress on differentiated cells is well known, little is known regarding how stem cells respond to oxidative stress. Reactive oxygen species can alter gene expression profiles, leading to a decline in factors that promote stem cell self-renewal and maintenance.
Compared with WST rats, SHRs presented with a significant decrease in GR (Fig. 2b, c, d), colony formation (Fig. 2a), and migration potential (Fig. 3) and an increase in senescence (Fig. 6a, b, c). Oxidative stress was also significantly higher in SHR CSCs (Fig. 4). Since CSC efficiency is compromised in SHRs, decreased cardiac regeneration potential is anticipated, which, in turn, can lead to cardiac failure. A therapeutic intervention that restores the efficiency of stem cells is therefore anticipated to maintain the myocardium in a healthy state and prevent progressive remodeling. Some of the anti-hypertensive drugs prevent cardiac remodeling and reduce oxidative stress. However, the impact of these drugs on stem cell characteristics remains unexplored. Hence, we investigated the effect of a commonly used cardioprotective beta-blocker, metoprolol, on CSCs. To our knowledge, the effect of metoprolol on CSC properties in chronic pressure overload has not been studied. Our study demonstrates that in addition to reduced blood pressure and cardioprotection, metoprolol increased the CSC efficiency, which was compromised in the untreated SHRs.
Spontaneously hypertensive rats, in the stable phase of hypertrophy, were treated with metoprolol tartrate for 2 months. In response to the treatment, reduced blood pressure, cardiac hypertrophy, and oxidative stress were confirmed (Tables 1, 2, and 3). Beta-adrenergic signaling plays an important role in cardiac adaptation following physiological demands or pathological stress [23]. Khan et al. [24] observed that selective β1-AR inhibition augmented cardiac progenitor cell survival and proliferation in the failing myocardium. However, the compromised efficiency of CSCs in hypertensive heart disease and restoration with metoprolol treatment have not been reported. Impaired growth kinetics, GRs, and PDTs were observed in SHRs (Fig. 2). After treatment with metoprolol, CSCs regained their growth potential and proliferation capacity, comparable to that of the normotensive control (Fig. 2a, b, c, d). An increase in CSC number after treatment with metoprolol has been reported in a surgical model of hypertrophy [3], which may be the consequence of increased proliferation as observed in this study. The colony-forming unit assay is a measure of the self-renewal capacity of stem cells. Colony formation was decreased 59% in the CSCs of SHRs compared to those of WST rats (Fig. 2a). Beta-blocker treatment enhanced the efficiency of CSCs to form colonies by 19%. Beta-blockers lower blood pressure and reduce oxygen consumption in the surrounding myocardium, which may help maintain the stemness/quiescent state of CSCs [25]. Hence, modifying the surrounding milieu in response to the treatment may account for the increased efficiency of stem cells.
The ability of cardiac stem cells to migrate in response to myocardial injury is a critical determinant of their efficiency. Stem cells respond to various injury-associated stimuli, such as Stromal-derived factor (SDF) release that promotes stem cell homing [26]. It is apparent that CSCs from SHRs exhibit a decreased ability to migrate as early as 6 months of age (Fig. 3). Treatment with metoprolol enhanced the migratory capacity of stem cells. A study on mouse cardiac fibroblasts reported an association between histone deacetyltransferase levels and cell migration, supporting the possibility for CSC epigenetic modification via metoprolol treatment [27]. The protective effect of metoprolol on the myocardium can therefore be attributed to the efficient availability of CSCs for repair. Directed cardiovascular lineage differentiation was unaffected in SHRs, and metoprolol also did not influence the differentiation potential (Fig. 5). Redox-based mechanisms underlie stem cell differentiation into cardiogenic lineages [28]. An increased proportion of beating cells was observed after embryonic stem cells were exposed to agents that increased the intracellular ROS levels [29]. In contrast, agents that reduce intracellular ROS levels impair cardiomyocyte formation in embryoid bodies [30, 31]. This effect possibly accounts for the relative decrease in the proportion of differentiated cells, though the difference was not statistically significant (Fig. 5). Stem cell maintenance in the undifferentiated state helps to preserve the stem cell pool. The lack of distinction between the differentiation potential of SHRs and WST rats and the insignificant response to the treatment possibly signifies that the variation in ROS levels was not beyond the limits that modulate differentiation. Embryonic stem cell exposure to H2O2 revealed that the enhancement and impairment of cardiomyogenic differentiation was dose- and time-dependent [30, 32]. Oxidative stress is implicated as early as 2 months of age in SHRs and can trigger left ventricular remodeling [33, 34]. Comparably, CSCs from untreated SHRs exhibited increased intracellular ROS levels (Fig. 4). Despite the known antioxidant potential of beta-blockers, there are no reports on the impact of these drugs on the oxidative stress of CSCs. In addition to being an anti-hypertensive drug, metoprolol effectively quenches the ROS level and helps maintain a suitable atmosphere for stem cells [35]. The reduced oxidative stress in CSCs after metoprolol treatment is an interesting observation (Fig. 4). Studies using angiotensin II receptor blockers revealed that EPC dysfunction was improved through antioxidative mechanisms [36]. Studies have also shown that preconditioning human cardiac stem cells (hCSCs) with a nitric oxide adduct promotes cell survival and resistance to oxidative stress by activating cell survival pathways [37]. However, studies on the effect of antioxidants on CSCs are limited. Oxidative stress can induce cell cycle arrest or senescence in stem cells [38]. Over time, the senescent cells undergo apoptosis, thereby reducing the stem cell pool. The increased expression of senescent markers in SHR CSCs (Fig. 6) is possibly a consequence of the compromised efficiency of stem cells in the pathological setting. However, compared to the untreated animals, metoprolol-treated rats presented with an improved stem cell phenotype by retaining stemness. Receptor inhibition by metoprolol stimulates downstream pathways, thereby downregulating the expression of genes involved in senescence and apoptosis [39].
This study has demonstrated that stem cell efficiency is affected during hypertensive heart disease. In addition to being a potent anti-hypertensive drug, metoprolol modulates stem cell characteristics. Hence, the beneficial role of metoprolol in preventing progressive pathological remodeling can also be attributed to improved cardiac stem cell efficiency. These observations encourage further studies in clinical settings that validate the claim that modulating stem cell attributes prevent progressive cardiac remodeling.
References
Cesselli D, Beltrami AP, D’Aurizio F, Marcon P, Bergamin N, Toffoletto B, Pandolfi M, Puppato E, Marino L, Signore S, Livi U, Verardo R, Piazza S, Marchionni L, Fiorini C, Schneider C, Hosoda T, Rota M, Kajstura J, Anversa P, Beltrami CA, Leri A. Effects of age and heart failure on human cardiac stem cell function. Am J Pathol. 2011;179:349–66.
Smits AM, van Vliet P, Hassink RJ, Goumans M-J, Doevendans PA. The role of stem cells in cardiac regeneration. J Cell Mol Med. 2005;9:25–36.
Serpi R, Tolonen A-M, Tenhunen O, Pieviläinen O, Kubin A-M, Vaskivuo T, Soini Y, Kerkelä R, Leskinen H, Ruskoaho H. Divergent effects of losartan and metoprolol on cardiac remodeling, c-kit+ cells, proliferation and apoptosis in the left ventricle after myocardial infarction. Clin Transl Sci. 2009;2:422–30.
Griendling KK, Sorescu D, Ushio-Fukai M. NAD(P)H oxidase: role in cardiovascular biology and disease. Circ Res. 2000;86:494–501.
Fukai T, Folz RJ, Landmesser U, Harrison DG. Extracellular superoxide dismutase and cardiovascular disease. Cardiovasc Res. 2002;55:239–49.
Belch JJ, Bridges AB, Scott N, Chopra M. Oxygen free radicals and congestive heart failure. Br Heart J. 1991;65:245–8.
McMurray J, Chopra M, Abdullah I, Smith WE, Dargie HJ. Evidence of oxidative stress in chronic heart failure in humans. Eur Heart J. 1993;14:1493–8.
Kono Y, Nakamura K, Kimura H, Nishii N, Watanabe A, Banba K, Nishii N, Watanabe A, Banba K, Miura A, Nagase S, Sakuragi S, Kusano KF, Matsubara H, Ohe T. Elevated levels of oxidative DNA damage in serum and myocardium of patients with heart failure. Circ J Off J Jpn Circ Soc. 2006;70:1001–5.
Nakamura K, Kusano K, Nakamura Y, Kakishita M, Ohta K, Nagase S, Yamamoto M, Miyaji K, Saito H, Morita H, Emori T, Matsubara H, Toyokuni S, Ohe T. Carvedilol decreases elevated oxidative stress in human failing myocardium. Circulation. 2002;105:2867–71.
Yoo SM, Choi SH, Jung MDY, Lim SC, Baek SH. Short-term use of telmisartan attenuates oxidation and improves Prdx2 expression more than antioxidant β-blockers in the cardiovascular systems of spontaneously hypertensive rats. Hypertens Res Off J Jpn Soc Hypertens. 2015;38:106–15.
Watanabe H, Iwanaga Y, Miyaji Y, Yamamoto H, Miyazaki S. Renal denervation mitigates cardiac remodeling and renal damage in Dahl rats: a comparison with β-receptor blockade. Hypertens Res Off J Jpn Soc Hypertens. 2016;39:217–26.
Corea L, Bentivoglio M, Verdecchia P, Provvidenza M, Motolese M. Left ventricular hypertrophy regression in hypertensive patients treated with metoprolol. Int J Clin Pharmacol. 1984;22:365–70.
Weiss L, Lundgren Y, Folkow B. Effects of prolonged treatment with adrenergic β-receptor antagonists on blood pressure, cardiovascular design and reactivity in spontaneously hypertensive rats (SHR). Acta Physiol Scand. 1974;91:447–57.
Chan V, Fenning A, Hoey A, Brown L. Chronic β-adrenoceptor antagonist treatment controls cardiovascular remodeling in heart failure in the aging spontaneously hypertensive rat. J Cardiovasc Pharmacol. 2011;58:424–31.
Messina E, Angelis LD, Frati G, Morrone S, Chimenti S, Fiordaliso F, Salio M, Battaglia M, Latronico MV, Coletta M, Vivarelli E, Frati L, Cossu G, Giacomello A. Isolation and expansion of adult cardiac stem cells from human and murine heart. Circ Res. 2004;95:911–21.
Linke A, Müller P, Nurzynska D, Casarsa C, Torella D, Nascimbene A, Castaldo C, Cascapera S, Böhm M, Quaini F, Urbanek K, Leri A, Hintze TH, Kajstura J, Anversa P. Stem cells in the dog heart are self-renewing, clonogenic, and multipotent and regenerate infarcted myocardium, improving cardiac function. Proc Natl Acad Sci USA. 2005;102:8966–71.
Mallat Z, Philip I, Lebret M, Chatel D, Maclouf J, Tedgui A. Elevated levels of 8-iso-prostaglandin F2alpha in pericardial fluid of patients with heart failure: a potential role for in vivo oxidant stress in ventricular dilatation and progression to heart failure. Circulation. 1998;97:1536–9.
Dhalla AK, Hill MF, Singal PK. Role of oxidative stress in transition of hypertrophy to heart failure. J Am Coll Cardiol. 1996;28:506–14.
Miyamoto S, Kawaguchi N, Ellison GM, Matsuoka R, Shin’oka T, Kurosawa H. Characterization of long-term cultured c-kit+ cardiac stem cells derived from adult rat hearts. Stem Cells Dev. 2010;19:105–16.
Kim K, Doi A, Wen B, Ng K, Zhao R, Cahan P, Kim J, Aryee MJ, Ji H, Ehrlich LI, Yabuuchi A, Takeuchi A, Cunniff KC, Hongguang H, McKinney-Freeman S, Naveiras O, Yoon TJ, Irizarry RA, Jung N, Seita J, Hanna J, Murakami P, Jaenisch R, Weissleder R, Orkin SH, Weissman IL, Feinberg AP, Daley GQ. Epigenetic memory in induced pluripotent stem cells. Nature. 2010;467:285–90.
Reinisch A, Etchart N, Thomas D, Hofmann NA, Fruehwirth M, Sinha S, Chan CK, Senarath-Yapa K, Seo EY, Wearda T, Hartwig UF, Beham-Schmid C, Trajanoski S, Lin Q, Wagner W, Dullin C, Alves F, Andreeff M, Weissman IL, Longaker MT, Schallmoser K, Majeti R, Strunk D. Epigenetic and in vivo comparison of diverse MSC sources reveals an endochondral signature for human hematopoietic niche formation. Blood. 2015;125:249–60.
Ganesh SK, Tragante V, Guo W, Guo Y, Lanktree MB, Smith EN, Johnson T, Castillo BA, Barnard J, Baumert J, Chang YP, Elbers CC, Farrall M, Fischer ME, Franceschini N, Gaunt TR, Gho JM, Gieger C, Gong Y, Isaacs A, Kleber ME, Mateo Leach I, McDonough CW, Meijs MF, Mellander O, Molony CM, Nolte IM, Padmanabhan S, Price TS, Rajagopalan R, Shaffer J, Shah S, Shen H, Soranzo N, van der Most PJ, Van Iperen EP, Van Setten J, Vonk JM, Zhang L, Beitelshees AL, Berenson GS, Bhatt DL, Boer JM, Boerwinkle E, Burkley B, Burt A, Chakravarti A, Chen W, Cooper-Dehoff RM, Curtis SP, Dreisbach A, Duggan D, Ehret GB, Fabsitz RR, Fornage M, Fox E, Furlong CE, Gansevoort RT, Hofker MH, Hovingh GK, Kirkland SA, Kottke-Marchant K, Kutlar A, Lacroix AZ, Langaee TY, Li YR, Lin H, Liu K, Maiwald S, Malik R, Murugesan G, Newton-Cheh C, O’Connell JR, Onland-Moret NC, Ouwehand WH, Palmas W, Penninx BW, Pepine CJ, Pettinger M, Polak JF, Ramachandran VS, Ranchalis J, Redline S, Ridker PM, Rose LM, Scharnag H, Schork NJ, Shimbo D, Shuldiner AR, Srinivasan SR, Stolk RP, Taylor HA, Thorand B, Trip MD, van Duijn CM, Verschuren WM, Wijmenga C, Winkelmann BR, Wyatt S, Young JH, Boehm BO, Caulfield MJ, Chasman DI, Davidson KW, Doevendans PA, Fitzgerald GA, Gums JG, Hakonarson H, Hillege HL, Illig T, Jarvik GP, Johnson JA, Kastelein JJ, Koenig W, LifeLines Cohort Study, März W, Mitchell BD, Murray SS, Oldehinkel AJ, Rader DJ, Reilly MP, Reiner AP, Schadt EE, Silverstein RL, Snieder H, Stanton AV, Uitterlinden AG, van der Harst P, van der Schouw YT, Samani NJ, Johnson AD, Munroe PB, de Bakker PI, Zhu X, Levy D, Keating BJ, Asselbergs FW. Loci influencing blood pressure identified using a cardiovascular gene-centric array. Hum Mol Genet. 2013;22:1663–78.
Collis LP, Srivastava S, Coetzee WA, Artman M. beta2-Adrenergic receptor agonists stimulate L-type calcium current independent of PKA in newborn rabbit ventricular myocytes. Am J Physiol Heart Circ Physiol. 2007;293:H2826–35.
Khan M, Mohsin S, Avitabile D, Siddiqi S, Nguyen J, Wallach K, Quijada P, McGregor M, Gude N, Alvarez R, Tilley DG, Koch WJ, Sussman MA. β-Adrenergic regulation of cardiac progenitor cell death versus survival and proliferation. Circ Res. 2013;112:476–86.
Cruickshank JM. The beta 1 hyperselectivity in beta-blocker treatment. J Cardiovasc Pharmacol. 1995;25:S35–46.
Askari AT, Unzek S, Popovic ZB, Goldman CK, Forudi F, Kiedrowski M, Rovner A, Ellis SG, Thomas JD, DiCorleto PE, Topol EJ, Penn MS. Effect of stromal-cell-derived factor 1 on stem-cell homing and tissue regeneration in ischaemic cardiomyopathy. Lancet Lond Engl. 2003;362:697–703.
Somanna NK, Valente AJ, Krenz M, McDonald KS, Higashi Y, Noda M, Chandrasekar B. Histone deacetyltransferase inhibitors trichostatin A and mocetinostat differentially regulate MMP9, IL-18 and RECK expression, and attenuate angiotensin II-induced cardiac fibroblast migration and proliferation. Hypertens Res Off J Jpn Soc Hypertens. 2016;39:709–16.
Murray TVA, Smyrnias I, Shah AM, Brewer AC. NADPH oxidase 4 regulates cardiomyocyte differentiation via redox activation of c-Jun protein and the cis-regulation of GATA-4 gene transcription. J Biol Chem. 2013;288:15745–59.
Schmelter M, Ateghang B, Helmig S, Wartenberg M, Sauer H. Embryonic stem cells utilize reactive oxygen species as transducers of mechanical strain-induced cardiovascular differentiation. FASEB J Off Publ Fed Am Soc Exp Biol. 2006;20:1182–4.
Li J, Stouffs M, Serrander L, Banfi B, Bettiol E, Charnay Y, Steger K, Krause KH, Jaconi ME. The NADPH oxidase NOX4 drives cardiac differentiation: role in regulating cardiac transcription factors and MAP kinase activation. Mol Biol Cell. 2006;17:3978–88.
Sauer H, Rahimi G, Hescheler J, Wartenberg M. Role of reactive oxygen species and phosphatidylinositol 3-kinase in cardiomyocyte differentiation of embryonic stem cells. FEBS Lett. 2000;476:218–23.
Puceat M. Role of Rac-GTPase and reactive oxygen species in cardiac differentiation of stem cells. Antioxid Redox Signal. 2005;7:1435–9.
Takimoto E, Kass DA. Role of oxidative stress in cardiac hypertrophy and remodeling. Hypertension. 2007;49:241–8.
Purushothaman S, Renuka Nair R, Harikrishnan VS, Fernandez AC. Temporal relation of cardiac hypertrophy, oxidative stress, and fatty acid metabolism in spontaneously hypertensive rat. Mol Cell Biochem. 2011;351:59–64.
Nakamura K, Murakami M, Miura D, Yunoki K, Enko K, Tanaka M, Saito Y, Nishii N, Miyoshi T, Yoshida M, Oe H, Toh N, Nagase S, Kohno K, Morita H, Matsubara H, Kusano KF, Ohe T, Ito H. Beta-blockers and oxidative stress in patients with heart failure. Pharmaceuticals. 2011;4:1088–100.
Yao EH, Yu Y, Fukuda N. Oxidative stress on progenitor and stem cells in cardiovascular diseases. 2017. http://www.eurekaselect.com/55726/article.
Teng L, Bennett E, Cai C. Preconditioning c-Kit positive human cardiac stem cells with a nitric oxide donor enhances cell survival through activation of survival signaling pathways. J Biol Chem. 2016;291:9733–47.
Chen J-H, Ozanne SE, Hales CN. Methods of cellular senescence induction using oxidative stress. Methods Mol Biol. 2007;371:179–89.
Su Q, Li L, Liu Y-C, Zhou Y, Lu Y-G, Wen W-M. Effect of metoprolol on myocardial apoptosis and caspase-9 activation after coronary microembolization in rats. Exp Clin Cardiol. 2013;18:161–5.
Acknowledgements
The study was supported by the Board of Research in Nuclear Sciences, Govt. of India. Ms. Sherin Saheera received an INSPIRE Fellowship from the Department of Science and Technology, Govt. of India. We are grateful to the director of the Sree Chitra Tirunal Institute for Medical Sciences and Technology, Trivandrum, for the facilities and permission to publish the findings.
Author contributions
Sherin Saheera: designed the study, performed the experiments, analyzed the data, and prepared the manuscript; Ajay Godwin Potnuri: designed and performed the animal experiments; Renuka Nair: conceived the study and edited the manuscript.
Author information
Authors and Affiliations
Corresponding author
Ethics declarations
Conflict of interest
The authors declare that they have no conflict of interest.
Rights and permissions
About this article
Cite this article
Saheera, S., Potnuri, A.G. & Nair, R.R. Modulation of cardiac stem cell characteristics by metoprolol in hypertensive heart disease. Hypertens Res 41, 253–262 (2018). https://doi.org/10.1038/s41440-018-0015-7
Received:
Revised:
Accepted:
Published:
Issue Date:
DOI: https://doi.org/10.1038/s41440-018-0015-7