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Cardiorespiratory responses, nitric oxide production and inflammatory factors in patients with myocardial infarction after rehabilitation
Accepted Manuscript Cardiorespiratory responses, nitric oxide production and inflammatory factors in patients with myocardial infarction after rehabilitation José V. Subiela, Sonia H. Torres, Juan B. De Sanctis, Noelina Hernández PII:
S1089-8603(17)30258-6
DOI:
10.1016/j.niox.2018.03.006
Reference:
YNIOX 1759
To appear in:
Nitric Oxide
Received Date: 25 September 2017 Revised Date:
3 March 2018
Accepted Date: 5 March 2018
Please cite this article as: José.V. Subiela, S.H. Torres, J.B. De Sanctis, N. Hernández, Cardiorespiratory responses, nitric oxide production and inflammatory factors in patients with myocardial infarction after rehabilitation, Nitric Oxide (2018), doi: 10.1016/j.niox.2018.03.006. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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CARDIORESPIRATORY RESPONSES, NITRIC OXIDE PRODUCTION AND INFLAMMATORY
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FACTORS IN PATIENTS WITH MYOCARDIAL INFARCTION AFTER REHABILITATION.
Running title: Skeletal muscle inflammation in rehabilitated myocardial infarction patients. José V Subiela, MD, PhDa, Sonia H Torres, MD, PhDa, Juan B De Sanctis, PhDb, Noelina Hernández,
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PhDa.
a. Institute of Experimental Medicine, Section of Muscle Adaptation (SEAM), Medical Faculty, Central University of Venezuela, Caracas, Venezuela.
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b. Institute of Immunology, Medical Faculty, Central University of Venezuela, Caracas, Venezuela
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Corresponding author: Dr. Sonia H. Torres. Instituto de Medicina Experimental. Sección para el Estudio de la Adaptabilidad Muscular (SEAM). Facultad de Medicina. Universidad Central de Venezuela. Ciudad Universitaria. Caracas. Venezuela. Postal Code: 1050 E.mail: [email protected] Work telephone: 58- 212- 6053395 Home telephone: 58-212.-7307503 Cell phone: 58 04143116551. WhatsApp +58 4143116551
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Emails of authors José V Subiela: [email protected] Juan B De Sanctis: [email protected] Noelina Hernández: [email protected]
FUNDING This work was funded by “Consejo de Desarrollo Científico y Humanístico”. Universidad Central de Venezuela. 09-00-6717 CONFLICTS OF INTEREST: none.
CONTRIBUTORS: All authors have materially participated in the research and article preparation and have approved the final article. 1
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ABSTRACT
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There is evidence that myocardial infarction (MI) patients have an inflammatory process that includes skeletal muscles, and exercise has been reported to reduce some inflammatory markers. The aim of this work was to study NO and some inflammatory markers in quadriceps muscle of MI patients before and after cardiac rehabilitation. Muscle biopsy was obtained in17 MI patients before and after CR and only once in 11 healthy subjects. Several cardiorespiratory and metabolic parameters were evaluated and skeletal muscle levels of nitric oxide synthases, nitrate, nitrite, nitrotyrosine, tumor necrosis factor alpha (TNF-α), transforming growth factor beta (TGF-β), interleukin- 6 (IL-6) and CD154. After CR there was an increase in maximal oxygen consumption (21.2±1.4 vs 25.7±2.5 mL/kg/min, P<0.0001); work load (116.2±14.9 vs 140±17 W, P<0.0001); pulmonary ventilation (59.8±7,5 vs 73.8±11.6 L/min, P<0.0001); anaerobic threshold (53.8%±3.5% vs 60.2%±3.3% of maximal VO2, P<0.0001), maximal lactatemia (8.1±1.4 vs 9.3±1.5 mmol/L, P<0.0001), and oxygen pulse (11.7±1.6 vs 14.0±1.9 mL/pulse, P<0.0001). CSA of type I fibers increased (4380±1868 vs 5237±1530 µm2, P=0.02), and nitrate (18.6±3.04 vs 20.7±2.0 ng/mg, P<0.001). There was a negative correlation between BMI, fat%, waist and hip circumferences and NO synthase, nitrite and nitrate after CR. The inflammatory mediators were higher in patients than in control subjects and did not change with CR. TGF-β correlated directly with nitrite and nitrate and inversely to other inflammatory factors. In conclusion, there is an increase of nitrate post CR, indicating a more effective NO production. TGF-β was related to anti-inflammatory processes even before CR.
Key Words: Cardiac rehabilitation, cardiorespiratory indices, nitric oxide, inflammation factors Abbreviations:
Highlights:
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AT = aerobic threshold BMI= body mass index CAD= coronary artery disease CD154 = CD40 ligand. Protein in macrophage membrane, CD4 + activated T cell, endothelial and other cells. CVD=cardiovascular disease CR = cardiac rehabilitation CSA = cross sectional area eNOS = constitutive endothelial nitric oxide synthase iNOS = inducible nitric oxide synthase nNOS = constitutive neuronal nitric oxide synthase TNF-α = Tumor necrosis factor alfa TGF-β = Transforming growth factor beta IL-6 = interleukin 6
After cardiac rehabilitation nitrate levels increased in skeletal muscle. Body fat correlated inversely with higher NO production in rehabilitated patients. Transforming growth factor β was related with decreased inflammation and higher NO.
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ACCEPTED MANUSCRIPT 1.INTRODUCTION. Cardiovascular diseases (CVD) are the leading cause of death in the world. According to WHO in 2012, 17.5 million people died from CVD, of which 7.5 million deaths were from coronary artery disease and 6.7 million from cerebrovascular accidents [1]. Exercise based CR programs were developed for patients after
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acute myocardial infarction (MI) to help them regain their previous exercise capacity and facilitate reintegration into working life. It has been demonstrated that CR is a highly efficient, innocuous and economic therapeutic intervention [2]. There is ample evidence that diet and medical treatment of risk
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factors play a role in prevention and control of CVD [3]; moreover, CR including its 6 fundamental aspects (patient education, psychological aid, occupational therapy, dietetic orientation, medical treatment and
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exercise) is crucial in secondary prevention of the disease. Some studies indicate that the modification of risk factors have a very positive impact on morbidity due to cardiac events, both recent and recurrent. After an acute coronary syndrome, the effects seem to be even more pronounced leading to a 40% decline in 6month mortality. [3, 4]. Physical training improves exercise capacity more than conventional medical
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therapy alone [5]. A year program of regular physical exercise in selected patients with stable coronary artery disease (CAD) resulted in higher event-free survival and exercise capacity compared with standard percutaneous coronary intervention [6]. Since 1995, CR participation after acute coronary syndrome and
treatment [7].
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coronary artery bypass grafting is associated with reduced mortality even in the modern era of CAD
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Training induces in both healthy subjects and CAD patients an increase in maximal oxygen consumption, which is the product of the capacity of the cardiovascular system to supply oxygen (i.e. cardiac output) and the capacity of skeletal muscles to use oxygen (i.e. arterial-venous oxygen difference).
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individuals this increase is aproximately produced in equal proportion by central and peripheral adaptations while in CAD subjects impaired cardiac function would place a higher contribution on adaptive changes in the periphery, and consequently demand less effort on cardiac function [8]. Regular physical exercise as part of a multifactorial intervention improves symptom free exercise tolerance and myocardial perfusion. Because no net regression of epicardial coronary stenosis was observed in the majority of patients, and many 4
studies of collateralization in CAD patients have reported that exercise did not improve angiographically
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detectable collateralization, the current evidence does not firmly support the hypothesis that these beneficial effects of exercise result from a blunted progression and/or an increased regression of coronary lesions, instead it indicates that exercise increases endothelium dependent dilation in the conduit arteries and larger resistance arteries [9], as a result of increased nitric oxide (NO) production and bioavailability [10].
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Exercise also produces higher myogenic control, increased metabolic vasodilatation in small resistance arteries, and direct cardiac effects as improved calcium handling, increased P13K activity, reduction of fibrosis and cardiomyocyte apoptosis [4].
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Adaptive changes to endurance training in peripheral muscle are: increased oxygen extraction by correcting endothelial dysfunction and increasing basal NO formation [11]; improvement of oxidative metabolism,
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showed by increase in activity of oxidative enzymes [12]; increased levels of phosphocreatine/inorganic phosphates [13]; changes in mitochondrial ultrastructure [14]; increase of radical scavenger enzyme activity [15]; increase of COX-activity inversely correlated with iNOS expression /iNOS protein content [16]. In addition, there is a reduction of sarcopenia related to attenuation of MuRF-1 expression, a component of the
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ubiquitin-proteasome system involved in muscle proteolysis [17].
There are several reports of muscle inflammation in general diseases as type II diabetes mellitus [18] and chronic obstructive pulmonary disease (COPD) [19]. Patients with acute coronary syndrome, stable CAD, or
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chronic heart failure (CHF) showed elevated levels of inflammatory markers in peripheral blood mononuclear cells [20], plasma [21, 22] or skeletal muscle [23].
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Exercise has been reported to reduce some inflammatory markers in skeletal muscle of CHF patients [23], but not in plasma [22]. Generation of NO is related to inflammatory markers, as demonstrated by the induction of iNOS expression in skeletal muscle by IL-1b and NFkB activation [24]. Most of the work on peripheral effects of exercise on skeletal muscle in patients with CVD has been done ln patients with CHF, however, there is scarce information in MI patients. The hypothesis of the present work is that the improvement in oxygen consumption that is obtained with the rehabilitation program currently used in our University Hospital may be related to an increase in skeletal muscle NO production and to reduction in the muscle inflammatory state. For that purpose, nitric oxide synthases (NOS), nitrate, nitrite, 5
nitrotyrosine, tumor necrosis factor alpha (TNF-α), transforming growth factor beta (TGF-β), interleukin-6
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(IL-6) and CD154 were determined, along with several cardiorespiratory and metabolic parameters.
2. METHODS 2.1. Study subjects
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Seventeen male patients (54±8 years old) who entered a 12 weeks program of CR in the Unit of Cardiac Rehabilitation of the “Hospital Clínico Universitario” in Caracas (Venezuela), 8 weeks after been released from hospitalization due to a myocardial infarction (MI) of low or medium risk profile [25]. Each patient
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was examined before and after the CR program to be his own control. Eleven healthy male subjects (56±1 years old) were also examined to compare with them the results of the MI patients before and after CR
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(Table 1). All patients were treated with β-blockers, 16 had anti-aggregation therapy, 9 received ARAII, 4 received calcium antagonists, 3 were taking IECA and one, anticoagulant therapy; treatment was maintained during rehabilitation and for the performance of the ergometric tests. The Bioethical Committee of the hospital approved the study and patients and healthy subjects signed the informed consent.
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2.2. Body composition
Body fat percentage was estimated by skinfold thickness measurements using a caliper in four body regions; and equations to calculate body density and fat % [26]. Waist and hips circumference [27], and body mass
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index were assessed by standard procedures. 2.3. Ergometric test
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An exercise test was performed before and after the CR program, in an electrically braked cycle ergometer (Lode Excalibur Sport, USA), frequency of 60 cycles per min. After 3 min of unloaded pedaling, 25 watts´ resistance increases were added every 3 min until exhaustion, or when blood pressure or heart rate increased or decreased disproportionally, or ECG changes showed signs of complex arrhythmias or myocardial ischemia. ECG was monitored during the whole test, and the 15 final seconds (s) of each stage were recorded. Blood pressure (BP) was measured in the final 30 s of each stage and at 1, 2, 3, 5, 7 and 10 min post-test. Physiological variables were registered in an automatic equipment (ULTIMA 20 MedGraphics,
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USA), with a metabolic and respiratory analyzer, following the established protocol. All patients finished
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the test despite of minor ECG and cardiac rhythm changes in some subjects,
2.4. Physical training The CR program used is that currently practiced in the University Hospital of Caracas. Training program
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consisted in three weekly sessions of approximately 60 min of exercise, during 12 weeks for a total of 36 sessions during the study period. Sessions consisted of three parts: 1) warming and neuromuscular conditioning including loosening, stretching, articular mobility and flexibility, during 15 min. 2) aerobic
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exercise during 20 min the first two weeks and then 30 min the rest of the sessions, bicycling or walking on a thread-mill in the firsts sessions, that allowed a better control of HR and BP, and walking on a track
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in the lasts sessions. The intensity was tailored for each patient according to the result of the prerehabilitation ergometric test (60-80% of VO2 max). 3) final recovery and relaxation exercises for 10-15 min. First week started with 60% of maximum heart rate obtained in the previous effort test, if well tolerated, it was increased to 70% in the second week, to 80% in the third week and kept at this level until
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the end of the 12 weeks. Walk speed/pedaling rate were adjusted accordingly to maintain the intensity at 80%. Al training sessions were supervised by physiotherapists and one cardiologist.
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2.5. Lactatemia
Blood lactate was measured in the ear lobe, before the test and 3 min after the end. Blood was analysed with
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a mini-photometric equipment (Miniphotometer Dr Lange Plus 20, Berlin, Germany). 2.6. Echocardiogram
A trans-thoracic echocardiogram (TTE) was performed with a Philips Sonos 4500 equipment, before and after CR. The axes determined were; long left parasternal, short left parasternal, sub-costal, and 4 chambers, with a transducer of 2.5 MHz. The inter-ventricular septum width, the diameters of the posterior wall of the left ventricle and the left atrium, and the ejection fraction were measured. 2.7. Skeletal muscle determinations
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Patients underwent needle muscle biopsies [28] before and after CR. Healthy subjects were biopsied only
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once. The sample of approximately 50 mg was immediately blotted and divided in three parts; the first part was embedded in OCT compound (Tissue TEK; Sakura Finetek Torrance, CA) and dipped in isopentane frozen in liquid nitrogen; the two other parts were directly frozen in isopentane, all samples were wrapped in identified aluminum paper and placed in liquid nitrogen to transport them to a freezer to be stored at -80ο
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until processing. The procedure from taking the sample to be frozen lasted less than 1 min. 2.7.1. Histochemical Procedures
Fiber type classification and capillary measurements were done in 10 µm transverse serial sections cut in a
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cryostat at – 20°C, with the adenosine triphosphatase reaction after alkaline (pH 10.3) and acid (pH 4.37 and pH 4.6) preincubation [29]. Capillaries were visualized by the α-amylase periodic acid Schiff reaction [30].
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Photomicrographs at a final magnification X 200 were made, and fibers were identified by comparison with the adenosine triphosphatase sections. An area of the photograph was delimited, measured with a planimeter, and fibers and capillaries were counted to calculate the mean fiber CSA, capillaries per square millimeter, and capillaries per fiber ratio. Capillaries around each fiber type were counted and all the fibers
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of one type were drawn together to measure area by planimetry to calculate the mean area of each fiber type. 2.7.2. Determinations of muscle metabolism enzymes. Muscle samples for enzymes activities were weighted at -20οC, homogenized in ice cooled potassium
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phosphate buffer. The activities of citrate synthase (CS) 3-31hydroxy-acyl-CoA-dehydrogenase (HAD) and lactate dehydrogenase (LDH) were assayed using fluorometric techniques [31].
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2.7.3. Assessment of nitrate, nitrite, eNos, iNOs, nNOs and nitrotyrosine levels. The muscle sample was weighed and homogenized with a glass pestle in 1 mL of Tris-HCl buffer, 10 mmol/L, pH 7.5; NaCl, 150 mmol/L; ethylene-diamine tetra-acetic acid, 5 mmol/L; triton x-100, 1% (volume/volume); leupeptin, 10 µg/mL; aprotinin,10 g/mL; and pepstatin, 2.5 g/mL. The homogenate was centrifuged at 90g for 5 min. Supernatant was used for the assays. Protein concentration was assessed by the BCA protein assay kit (Pierce Biochemicals; Rockfort IL). NO levels were determined indirectly by quantification of their oxidized products of degradation, using nitrate reductase and the Griess reagent. A standard curve was obtained with sodium nitrate dissolved in water or in a pool of normal sera. Nitrite 8
concentration was determined at 540 nm using enzyme-linked immunosorbent assay (ELISA) plate reader
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(Multiscan MCC/340; Labsystems; Helsinki, Finland). All three NO synthases were assessed using sandwich ELISA assays. Constitutive eNOS was detected using a commercial kit (R&D Systems; Minneapolis, MN). Monoclonal and polyclonal antibodies for nNOS were from BD Biosciences (San Diego CA), and the recombinant enzyme for the standard curve was from Calbiochem (San Diego, CA).
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iNOS was assessed using a pair of antibodies (Serotec Corporation; Kidlington, Oxford, UK). The sensitivity of all assays was 25 pg/mL. Total amount of nitrotyrosine was determined by ELISA. The mouse immunoglobulin (Ig)-G monoclonal antibody, the polyclonal antibody against nitrotyrosine and the
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polyclonal goat anti-rabbit IgG-peroxidase antibody were purchased from Upstate Biotechnology (LakePlacid, NY, USA). The quantification of nitrotyrosine was performed using a standard curve with
the assay was 50 pg/mL [19]. 2.7.4. Assessment of inflammatory markers.
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known concentrations of nitrotyrosine from chemically modified bovine serum albumin. The sensitivity of
CD154 levels were detected by a commercial sandwich immunoenzymatic assay purchased from Chemicon
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Corporation (Temécula, CA, USA). The ELISA plates were already coated with the capturing monoclonal. The samples were diluted as specified by the manufacturer in the assay buffer, and the only modification was that samples were incubated for 18 h at 4º C. Quantitative analysis was performed with a standard
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curve. The detection limit was 1 ng CD154 per mg of protein. TGF-β and IL-6 were measured with ELISA sandwich in solid phase following the protocol recommended by the manufacturers of the reactive (R&D
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Systems, Minneapolis, USA).
TNF-a was assessed by a third generation TNF-a quantikine assay (R & D systems) following the manufacturer’s instructions, except that samples were diluted as suggested for serum samples and incubated for 18 h instead of 3 h. The sensitivity of the assay was 0.5–3 pg/mL. 2.8. Statistical Analysis Data in tables is expressed as mean ± SD. The results of each variable were evaluated in patients before and after CR with Student paired “t” test. The comparison of control subjects with patients before and after CR was done with non-paired “t” test. The Pearson product-moment correlation coefficient for grouped data and 9
Spearman for ungrouped data were used to establish correlations between the different variables of the
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study. The statistical program StatSoft Statistica was used for the analysis. A “P” value of less than 0.05 was considered statistically significant.
3. RESULTS
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3.1. Anthropometric characteristics Table 2 shows the bio-anthropometric characteristics of the patients. Although there was not a significant difference in weight and BMI, fat percentage was reduced after rehabilitation, indicating an increase in fat
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free mass and body density. The anthropometric characteristics measured in the healthy subjects group were not different compared to those of the patients before rehabilitation: weight (71.9±14.8 vs 75.5± 10.2 kg),
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height (167±8 vs165±17 cm), and BMI (26.43±3.0 vs 26.27±17.0), all P>0.05.
3.2. Exercise capacity
After CR, a highly significant increase in maximal oxygen consumption was found (P< 0.001), all patients
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passed the first category of Weber and Janicki [32]. Work load and work time increased; pulmonary ventilation, anaerobic threshold, maximal lactatemia and oxygen pulse also showed significant increments (p<0.001), (Table 3).
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3.3. Skeletal muscle characteristics
3.3.1. Cross sectional area and capillary indexes
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Patients showed an increase in the CSA of type I fibres after CR, P< 0.02 (Table 1). Before CR the patients, compared to healthy subjects, had a lower mean CSA of fibers (P<0.02), however, after CR there were no differences between the CSA of muscle fibers of patients and the healthy subjects (Table 1). Capillary density did not change after CR and did not differ between the healthy subject and the patient groups. (Table 1). 3.3.2. Muscle metabolism enzymes There were no changes after CR in muscle oxidative enzymes: (Table 1). CS activity was found higher in patients than in healthy subjects, both before and after rehabilitation (P<0.05). HAD activity was similar in 10
healthy subjects and patients; LDH was lower in patients before CR than in healthy subjects (P<0.05);
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however, significance of the difference disappeared after CR (Table 1). 3.3.3. NO production in muscle After CR, nitrate level was found highly significantly increased (P<0.001) (Table 1). No modification in the activity of NOS isoforms was seen after CR. Nitrate and nitrite concentrations were lower in patients as
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compared to healthy subjects (p<0.0001 and p<0.005 respectively); on the contrary, nitrotyrosine was higher (p<0.001) (Table 1). Although the value of nitrate increased after CR, it did not reach that of the healthy subjects. The constitutive isoforms of NOS, nNOS and eNOS, were lower in patients compared to healthy
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subjects (p<0.0001 and 0.05 respectively), and the inducible isoform iNOS was higher (p<0.005) (Table 1). 3.3.4. Inflammatory markers in muscle
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In Table 1 it is shown that there were not significant differences in the levels of the inflammatory markers post CR in comparison with those before rehabilitation. The measured inflammatory markers were significantly higher in patients as compared to healthy subjects, both before and after CR (TNF-α P<0.05, TGF-β and IL-6 P<0.005, and CD154 P<0.002). In all the healthy subjects, the levels of TNF-α were under
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the sensitivity of the method (Table 1).
3.4. Correlations between the studied variables
Positive and negative correlations between anthropometric characteristics versus NO products, enzymes and
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inflammatory markers are shown in Table 4. In Table 5 are reported the correlations between aerobic (CS and HAD) and anaerobic (LDH) metabolism enzymes; NO production enzymes (NOS), NO products
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(nitrite, nitrate and nitrotyrosine) and the inflammatory mediators (TNF-α, TGF-β, IL-6 and CD154). There was a negative correlation (see Table 4 for P values) between weight, BMI, fat%, waist and hip circumferences and eNOS, nitrite or nitrate after CR (Table 4). TGF-β correlated directly with nitrite and nitrate before CR, with all NOS after CR, and inversely to other inflammatory factors (see Table 5 for P values.). Correlation between the differences of the values after and before CE were significant for nitrite and maximal oxygen consumption expressed as VO2 mL/Kg.min (P<0.0001), and between nitrite and nitrate (P<0.002).
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4. DISCUSSION
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4.1. Main findings. There is ample information on the effects of regularly practiced exercise in skeletal muscle of healthy subjects. However, the morphological and functional changes in skeletal muscles in disease, and their modification by CR, is less known. The present study was done in patients with MI. In agreement with our
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hypothesis it was found a significant increase of nitrate levels in muscle after CR (P<0.001); the increase of nitrate and/or nitrite is considered a physiological increase of NO production. In addition, the differences of nitrite levels and maximal oxygen consumption (VO2 mL/Kg.min) after and before CE showed a direct
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correlation (P<0.0001). Also, a direct correlation was found between the differences pre- and postrehabilitation values of nitrite and nitrate (P<0.002). Another relevant finding was the inverse correlation
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between weight, BMI, percentage of body fat and circumference of waist and hip, and muscle eNOS values and, except percentage of body fat, also to nitrite; moreover, percentage of body fat was inversely related to nitrate levels (Fig. 1). The decrease of body fat percentage was not accompanied by weight change or by decrease of body mass index, which means an increase of lean body mass and body density. These results
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could be interpreted as a higher capacity of subjects with less fat to produce NO. On the other hand, the second part of our hypothesis, the decrease in the levels of inflammatory markers after CR, could not be demonstrated (Table 1). An important finding regarding inflammatory markers was the positive correlation
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of TGF-β with nitrites and nitrates before CR, and post CR with nitrite and all the three NOS (Table 4, Fig. 2). Fig. 3 illustrates the negative relationship of TGF-β with nitrotyrosine (post CR), with TNF-α (pre- and
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post- CR) and also with IL-6 (before CR). These results are in favor to a role of TGF-β as an antiinflammatory factor in patients with MI. 4.2. Cardiorespiratory effects The results obtained in cardiorespitatory functions with the present program of CR are likethose found by others:19.1% and 21.2 % for absolute and relative maximal oxygen consumption [33,34]. The changes in work load (watts) and exercise time were 12.6% and 20.3%, without change in mechanical efficiency. Maximal pulmonary ventilation increased 23.4%. There was a highly significant increase in oxygen pulse, which is a better indicator than VO2 for the appreciation of changes in maximal cardiac output [35]. In the 12
present study the increment of AT after CR was 11.8% and that of lactatemia was 13.6% [36]. Accordingly,
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AT, work load and pulmonary ventilation correlated directly to VO2 max. 4.3. Muscular changes 4.3.1. Fiber types and CSA In the present work no differences was found in the distribution of fiber type after CR, although Hambrecht
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et al [37] have reported a marginal increase in type I fibres proportion. This difference may be due to the longer duration of their program (6 months compared to 3 months). CSA of type I fibers augmented, and this caused that the differences in mean CSA disappeared after CR between patients and healthy subjects; this
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result differs from that of only 4 weeks training study [17]. 4.3.2. Muscle metabolism enzymes
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A group of MI patients has been studied in a previous work of the same laboratory (12); that group showed low levels of CS, 9.0 ± 2.9 µmol/gr.min before CR that increased to 16.0 ± 4.8, P<0.01 after only 6 weeks of a similar program of CR, they also showed an increase in HAD and a decrease in LDH after rehabilitation in contrast with the group of the present study that did not show any change in the enzyme levels with
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rehabilitation. In the present work the level of CS was higher in patients before CR than in healthy subjects and the difference was maintained after CR. These results may be explained because our healthy subjects were sedentary and the present group of patients was heterogeneous in their activity level. It is to be noticed
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that patients joined the CR program 8 weeks after leaving hospital with a recommendation to initiate a program of moderate exercise before joining formal CR; most of the patients confirmed to have done it.
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However, it was observed that the three patients that showed the higher increment in in max VO2 (25%, 26% and 27%) did have an increase in CS and HAD levels. 4.3.3. NO generation
The patients studied showed endothelial dysfunction, with low levels of nitrite and nitrate, eNOS and nNOS, and increased nitrotyrosine and iNOS in skeletal muscle. This indicates a low production of “physiological” NO with high production of “pathological” NO that reacted with superoxide to form peroxynitrite [15, 38] as shown by the increase of nitrotyrosine, the end-product of the nitrosylation of tyrosine by peroxynitrite. In addition, iNOS showed a negative correlation with both constitutive isozymes nNOS and eNOS levels. 13
Other authors have found increased iNOS expression and nitrotyrosine levels in skeletal muscle of patients
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with chronic heart failure [39]. It is well known that regular physical exercise, personally tailored and controlled, has important effects on cardiovascular health and survival [40,41], attenuates disease progression [9], reduces hypertension [42] and produces changes in the lipoprotein subclass profile [43]. Reactive oxygen species (ROS), inflammatory
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factors and NO are involved in the development of these responses [15,4,10]. Unexpectedly eNOS was not increased in muscle after CR in the current work. However, the direct correlation between nNOS and nitrite present before CE reached a higher signification post-rehabilitation; moreover, a high significance direct
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correlation appeared between eNOS and nitrite. This may be interpreted as an improvement in vasodilator
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capacity in muscle after CR.
4.3.4. Inflammatory markers
There is evidence of the role of inflammatory processes in cardiovascular diseases: it has been demonstrated in the development of atherosclerosis [21]; expression of TNF-α and IL-6, together with other interleukins
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(IL-10, IL-23A, IL-27 and IL-37), was significantly higher in peripheral blood mononuclear cells of patients with acute coronary syndrome [20]; patients with cardiac hearth failure showed increased serum levels of TNF-alpha, IL-6, and IL-1-beta [22]. In skeletal muscle of patients with cardiac heart failure it has been
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found increased levels of TNF-α, IL-1-beta, IL-6 with normal values in serum, [23]. In the present work
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patients showed increased levels of TNF-α, TGF-β and IL-6, and CD154 in skeletal muscle. It has been demonstrated that training for 6 months significantly reduced the local expression of TNF-α, IL1-beta, IL-6 and iNOS in skeletal muscle of patients with cardiac hearth failure [23]. Other authors did not find reduction of inflammatory markers in blood after 4 months of high intensity training in patients with cardiac heart failure and arterial hypertension, but they did in patients with idiopathic dilated cardiomyopathy [22]. Differences in results may be related to duration of training and to the cardiovascular status of patients. It is to note that the standard deviation of the values of inflammatory markers in our patients was high, and some of them showed reduction after CR. It also may be possible that these 14
inflammatory markers have a modulatory effect in different moments of the rehabilitation process and in a
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different metabolic milieu.For example TGF-β is a pleiotropic peptide released by many cell types and involved in the regulation of tissue growth and homeostasis in many processes including inflammation and its resolution [44]. It represses skeletal muscle specific gene expression and has also been reported to modulate proliferation in satellite cells [45]. The relations between different inflammatory markers may also
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change during the rehabilitation process; for instance, in the present study TGF-β levels showed an inverse correlation with TNF-α both before and after CR; with IL-6 only before, and with nitrotyrosine after CR. Some markers have been demonstrated to modify NO production, TGF-β suppressed IL-1-induced iNOS
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expression and NO production in chondrocytes [46]. In our results, after CR, TGF-β correlated directly with all the tree isoforms of NOS, but also post CR iNOS negatively correlated to nitrotyrosine, suggesting that
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NO produced by iNOS was not reacting with ROS, but joining the vasodilator pool of NO. All this suggests that in our patients TGF-β was acting as an anti-inflammatory factor and this effect was more important after CR. Other change in relationship between the different inflammatory markers was seen with CD154, before CR CD154 levels directly correlated with IL-6 and TNF-α and the two last mentioned cytokines were also
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directly related between them. However, after rehabilitation the significance of the direct correlation between CD154 and IL-6 was reduced, and the direct correlation between TNF-α and CD154 disappeared.
exercise. 4.4. Limitations
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These results suggest that the modulation effect between pro-inflammatory markers may be affected by
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Due to the invasive nature of procedure used to obtain the skeletal muscle samples, a relatively small number of subjects was included in the study; this probably limits the direct extrapolation of the present findings to the entire population of patients with myocardial infarction. The diversity of the level of physical activity in the patients provided a heterogeneous group that made difficult to obtain significant statistical results in some of the variables studied. The method applied to measure % body fat may be not sufficiently accurate, however it was performed by personnel that evaluates athletes and the results are coherent with the data of BMI and waist and hip circumferences. Greiss method is not the most sensitive assay to measure
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nitrite, but the results obtained with nitrate were highly significant, and we could not find other references of
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direct NO measurements in skeletal muscle in MI patients to compare.
5. CONCLUSION The present work reinforces the knowledge of the positive effects of CR in MI patients on oxygen
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consumption, physical work capacity, cardiac function, lactate production, anaerobic threshold and anthropometric characteristics. Skeletal muscle showed increase in NO production, as shown by the increase in the level of nitrate. The change in nitrite levels in muscle after rehabilitation was directly correlated with
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the increase in maximal oxygen consumption. CSA of the muscle fibers increased. The enhancement of the correlations of NOS isoforms with nitrite and nitrate suggests a more efficient production of NO. There was
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found an inverse relationship between NO production and BMI, body fat percentage, and waist and hip circumferences, indicating a better NO production in subjects with less body fat. The direct association of TGF-β with NO, nitrite, nitrate and NOS, and inverse relationship with inflammatory markers TNF-α and IL-6 in skeletal muscle strongly suggest an anti-inflammatory role. The direct correlation between pro-
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inflammatory markers was less significant or disappeared after CR. All these results may be interpreted as a change of the modulatory effects of inflammatory markers after the rehabilitation treatment, concurrent with
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the improvement on exercise capacity of the patients.
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6. ACKNOWLEDGEMENTS.
Our special thanks to Professor Stephen Tillett for correction of the English language and to
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Assistant Professor Luis Vázquez (Public Health Department) for his help with statistics.
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•
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cardiac rehabilitation participation and health status outcomes after acute myocardial infarction. JAMA Cardiol. 2016 JAMA Cardiol. 2016; 1:980-8. [42] Neves VJ, Fernandes T, Roque FR, Soci UP, Melo SF, de Oliveira EM. Exercise training in hypertension: Role of microRNAs. World J Cardiol. 2014; 6: 713-27.
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meta-analysis. Open Access Journal of Sports Medicine. 2018;9: 1–17.
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ACCEPTED MANUSCRIPT TEXTS OF FIGURES FIGURE 1 Correlations between body mass index (BMI) and body fat percentage (% fat) after cardiac rehabilitation.
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eNOS: endothelial nitric oxide synthase. A: p<0.005. B: p<0.005. C: p<0.05. D: p<0.02.
FIGURE 2
Correlations between transforming growth factor beta (TGF-β) and products and enzymes of nitric oxide.
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eNOS: endothelial nitric oxide synthase, nNOS: neuronal nitric oxide synthase. A: Before cardiac rehabilitation p<0.0005. B: After cardiac rehabilitation p<0.05, before cardiac rehabilitation the correlation
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between these variables was present with similar characteristics (not shown). C: After cardiac rehabilitation, p<0.01. D: After cardiac rehabilitation, p<0.005.
FIGURE 3
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Correlations between transforming growth factor beta (TGF-β) and inflammatory factors. TNFα: tumor necrosis factor alfa, IL-6: interleukin 6. A: Before cardiac rehabilitation p<0.05. B: After cardiac
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rehabilitation p<0.05. C: Before cardiac rehabilitation p<0.01. D: After cardiac rehabilitation p<0.005.
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ACCEPTED MANUSCRIPT TABLE 1. Comparison between healthy subjects and patients before (BCR) and after (ACR) cardiac rehabilitation, and comparison between patient values BCR and ACR. VARIABLES
Healthy
PBCR
subjects
H vs PBCR
PACR
P
H vs. PACR
PBCR vs.
P
PACR p
45±12
43±13
NS
42±9
NS
NS
% type IIA fibers
39±13
40±9
NS
43±10
NS
NS
% type IIX fibers
16±9
16±8
NS
16±9
NS
NS
Mean CSA (µm2)
5618±1273
3789±1104
<0.001
4399±1534
NS
NS
CSA type I fib(µm2)
6447±1441
4380±1868
<0.02
5237±1530
NS
<0.02
CSA type II fib(µm2)
5568±1331
4193±945
<0.05
5523±1830
NS
NS
CSA type IIX fib (µm2)
5166±1514
4218±1490
NS
5237±2452
NS
NS
Cap Adj. I (n)
4.6±0.8
4.8±0.8
NS
4.7±0.5
NS
Ns
Cap Adj. IIA (n)
4.2±0.8
4.2±0.3
Cap Adj. IIX (n)
3.6±1.0
3.0±0.8
DC (cap x mm2)
308±83
410±98
C x F (n)
1.65±0.29
1.57±0.34
CS (ng/mg-prot)
11.14±2.10
14.32±3.0
HAD (ng/mg-prot)
10.04±1.90
LDH (ng/mg-prot)
196±53.00
Nitrite (ng/mg)
17.44±4.47
Nitrate (ng/mg)
24.04±3.85
NO2- + NO3- (ng/mg)
4 1.83±6.49
Nitrotyrosine(ng/mg)
7.93±3.86
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NS
NS
NS
3.7±0.9
NS
NS
<0.05
411±128
<0.05
NS
NS
1.63±1.59
NS
NS
<0.05
15.90±5.08
<0.05
NS
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NS
10.15±2.6
NS
10.86±3.69
NS
NS
151.1±45.92
<0.05
150.8±58.20
NS
NS
5.64±0.56
<0.000000
5.79±0.70
<0.000000
NS
18.59±3.04
<0.005
20.71±2.00
<0.005
<0.001
24.23±3.21
<0.000000
26.61±2.29
<0.000000
NS
13.70±3.95
<0.001
14.90±5.04
<0.001
NS
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% type I fibers
nNOS (ng/mg-prot)
120.00±31.36
12.19±3.99
<0.000000
13.33±3.52
<0.000000
NS
iNOS (ng/mg-prot)
8.05±4.21
14.05±3.60
<0.005
14.31±3.72
<0.005
NS
eNOS (ng/mg-prot)
43.65±31.35
21.92±5.27
<0.05
23.79±6.22
<0.05
NS
TNF-α (pg/mL)
< 5.00
63.67±59.50
<0.05
53.50±46.81
<0.05
NS
TGF-β (pg/mL)
19.66±4.64
162.67±97.61
<0.005
172.20±102.0
<0.005
NS
IL-6(pg/mL)
18.64±4.79
182.17±108.25
<0.005
165.9±106.70
<0.005
NS
CD 154 (pg/mL)
24.32±6.47
130.50±79.09
<0.002
108.4±50.14
<0.002
NS
H: Healthy. PBCR: patients before cardiac rehabilitation. PACR: patients after cardiac rehabilitation.CSA: Cross sectional area. Cap adj..I: Mean number of capillaries around type one fiber. C x F: Capillary per fiber index. DC: Capillary density. NS: no significant.
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ACCEPTED MANUSCRIPT TABLE 2. Bio-anthropometric data and body composition. Before RC
After RC
P
Age (years)
53.9±8.03
-
-
Weight (kg)
75.6±10.24
74.4±8.62
NS
Height (cm)
168.4±5
-
BMI (kg/m2)
26.3±3.02
26.0±2.58
Fat %
16.8±4.60
15.0±2.58
Waist (cm)
93.3±6.58
92.3±6.30
Hip (cm)
96.9±5.09
95.7±4.73
<0.05
Waist/Hip
0.96±0.06
0.96±0.05
NS
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Variables
NS
<0.001 <0.01
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BMI: Body mass index.
-
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TABLE 3. Cardio-circulatory and respiratory variables in exercise test before and after
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After RC
P
Watts
116±15
140±17
<0.001
Exercise time (sec)
836±107
1006±125
<0.001
VE (L/min)
59.8±7.5
73.8±11.6
<0.001
VO2 max (mL/min)
1596±216
1901±223
<0.001
VO2 max(mL/kg/min)
21.2±1.4
25.7±2.5
<0.001
VE/VO2
37.2±5.1
VE/VCO2
31.9±4.5
La max (mM/L)
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Variables
NS
33.2±3.8
NS
8.1±1.4
9.3±1.5
<0.001
AT (% VO2 max)
53.8±3.5
60.2±3.3
<0.001
Oxymetry (SpO2%)
96.1±1.3
96.0±1.1
NS
HR max (bpm)
135±13
136±15
NS
183±11
186±12
NS
92±5
91±4
NS
DP (SBP x HR)
24673±3085
25286±3708
NS
VO2/HR (mL/beat)
11.7±1.6
14.0±1.9
<0.001
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DBP max (mmHg)
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SBP max (mmHg)
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38.7±4.0
AT: anaerobic threshold. DP: double product. La max: maximal lactate.
VP: pulmonary ventilation. Max HR: maximal heart rate. VP: pulmonary ventilation. VO2/HR (mL/beat): Oxygen pulse
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TABLE 4.- CORRELATIONS BETWEEN ANTHROPOMETRIC CHARACTERISTICS vs. NO PRODUCTS, ENZYMES AND INFLAMMATORY MARKERS. PRE-REHABILITATION eNOS
NO2-
nNOS
NO3-
NO2-+NO3-
IL-6
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Weight 0.65*e
0.58*e
NO3-
NO2-+NO3-
-0.58*f
-0.61*f
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Height BMI FFMII % fat Waist Hip Waist/hip
POST-REHABILITATION nNOS
-0.63*f -0.76**f -0.70*f
IL-6
-0.66*f
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-0.74**f
NO2-0.57**f
-0.56*f
-0.56*f -0.71**f -0.74**f
-0.55*f
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Weight Height BMI FFMI % fat Waist Hip Waist/hip
eNOS -0.59*f
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p < 0.05; ** p< 0.01; *** p < 0.001. Negative correlations are preceded by a negative sign. Letters are used to point that signification was: a= similar before and after CR, b= higher after CR, c=lower after CR, d= changed from + to – after CR, e=present only before CR, f= present only after CR
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TABLE 5 CORRELATIONS BETWEEN OXIDATIVE AND GLYCOLITIC ENZYMES, ISOFORMS OF NOS, NO PRODUCTS AND INFLAMMATORY MARKERS PRE-REHABILITATION AND POST-REHABILITATION
NO2-
NO2-+NO3-
PRE-REHABILITATION nNOS iNOS
NITROT.
0.58*d 0.62*b
NO2-+NO3-
TGF-β -0.62*e
IL-6
-0.75**a
0.64*a 0.87**e 0.89***e
-0.76**e
-0.60*a
0.79**e -0.72**e
CD 154
0.52*f -0.57*d 0.59*f 0.96***a
0.58*f -0.70**f
-0.56*a 0.56*b
-0.59*a
0.56*e 0.77**c
eNOS
TNF-α
TGF-β
IL-6
CD 154 0.62*
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0.78***b
NO2-
POST-REHABILITATION NITROT. nNOS iNOS
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CS HAD LDH NO2NO3NO2-+NO3NITROT. nNOS iNOS eNOS TNF-α TGF-β IL-6
LDH
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-0.56*b
HAD
TNF-α
0.64*e
0.99***a
POST.R
eNOS
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LDH
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HAD 0.55*b
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PRE-R CS HAD LDH NO2NO3NO2-+NO3NITROT. nNOS iNOS eNOS TNF-α TGF-β IL-6
0.83***b
0.87***b
0.68**f -0.74**a
-0.84***b
0.65* -0.58*a 0.71**b
0.63*f -0.62*a
-0.56*f
-0.65*
0.65*a
-0.75**f 0.75**f 0.57*f 0.77*f -0.65*a 0.59*c
p < 0.05; ** p< 0.01; *** p < 0.001. Negative correlations are preceded by a negative sign. Letters are used to point that signification was: a= similar before and after CR, b= higher after CR, c=lower after CR, d= changed from + to – after CR, e=present only before CR, f= present only after CR 28
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Highlights:
After cardiac rehabilitation nitrate levels increased in skeletal muscle. Body fat correlated inversely with higher NO production in rehabilitated patients.
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Transforming growth factor β was related with decreased inflammation and higher NO.
S1089-8603(17)30258-6
DOI:
10.1016/j.niox.2018.03.006
Reference:
YNIOX 1759
To appear in:
Nitric Oxide
Received Date: 25 September 2017 Revised Date:
3 March 2018
Accepted Date: 5 March 2018
Please cite this article as: José.V. Subiela, S.H. Torres, J.B. De Sanctis, N. Hernández, Cardiorespiratory responses, nitric oxide production and inflammatory factors in patients with myocardial infarction after rehabilitation, Nitric Oxide (2018), doi: 10.1016/j.niox.2018.03.006. This is a PDF file of an unedited manuscript that has been accepted for publication. As a service to our customers we are providing this early version of the manuscript. The manuscript will undergo copyediting, typesetting, and review of the resulting proof before it is published in its final form. Please note that during the production process errors may be discovered which could affect the content, and all legal disclaimers that apply to the journal pertain.
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CARDIORESPIRATORY RESPONSES, NITRIC OXIDE PRODUCTION AND INFLAMMATORY
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FACTORS IN PATIENTS WITH MYOCARDIAL INFARCTION AFTER REHABILITATION.
Running title: Skeletal muscle inflammation in rehabilitated myocardial infarction patients. José V Subiela, MD, PhDa, Sonia H Torres, MD, PhDa, Juan B De Sanctis, PhDb, Noelina Hernández,
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PhDa.
a. Institute of Experimental Medicine, Section of Muscle Adaptation (SEAM), Medical Faculty, Central University of Venezuela, Caracas, Venezuela.
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b. Institute of Immunology, Medical Faculty, Central University of Venezuela, Caracas, Venezuela
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Corresponding author: Dr. Sonia H. Torres. Instituto de Medicina Experimental. Sección para el Estudio de la Adaptabilidad Muscular (SEAM). Facultad de Medicina. Universidad Central de Venezuela. Ciudad Universitaria. Caracas. Venezuela. Postal Code: 1050 E.mail: [email protected] Work telephone: 58- 212- 6053395 Home telephone: 58-212.-7307503 Cell phone: 58 04143116551. WhatsApp +58 4143116551
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Emails of authors José V Subiela: [email protected] Juan B De Sanctis: [email protected] Noelina Hernández: [email protected]
FUNDING This work was funded by “Consejo de Desarrollo Científico y Humanístico”. Universidad Central de Venezuela. 09-00-6717 CONFLICTS OF INTEREST: none.
CONTRIBUTORS: All authors have materially participated in the research and article preparation and have approved the final article. 1
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ABSTRACT
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There is evidence that myocardial infarction (MI) patients have an inflammatory process that includes skeletal muscles, and exercise has been reported to reduce some inflammatory markers. The aim of this work was to study NO and some inflammatory markers in quadriceps muscle of MI patients before and after cardiac rehabilitation. Muscle biopsy was obtained in17 MI patients before and after CR and only once in 11 healthy subjects. Several cardiorespiratory and metabolic parameters were evaluated and skeletal muscle levels of nitric oxide synthases, nitrate, nitrite, nitrotyrosine, tumor necrosis factor alpha (TNF-α), transforming growth factor beta (TGF-β), interleukin- 6 (IL-6) and CD154. After CR there was an increase in maximal oxygen consumption (21.2±1.4 vs 25.7±2.5 mL/kg/min, P<0.0001); work load (116.2±14.9 vs 140±17 W, P<0.0001); pulmonary ventilation (59.8±7,5 vs 73.8±11.6 L/min, P<0.0001); anaerobic threshold (53.8%±3.5% vs 60.2%±3.3% of maximal VO2, P<0.0001), maximal lactatemia (8.1±1.4 vs 9.3±1.5 mmol/L, P<0.0001), and oxygen pulse (11.7±1.6 vs 14.0±1.9 mL/pulse, P<0.0001). CSA of type I fibers increased (4380±1868 vs 5237±1530 µm2, P=0.02), and nitrate (18.6±3.04 vs 20.7±2.0 ng/mg, P<0.001). There was a negative correlation between BMI, fat%, waist and hip circumferences and NO synthase, nitrite and nitrate after CR. The inflammatory mediators were higher in patients than in control subjects and did not change with CR. TGF-β correlated directly with nitrite and nitrate and inversely to other inflammatory factors. In conclusion, there is an increase of nitrate post CR, indicating a more effective NO production. TGF-β was related to anti-inflammatory processes even before CR.
Key Words: Cardiac rehabilitation, cardiorespiratory indices, nitric oxide, inflammation factors Abbreviations:
Highlights:
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AT = aerobic threshold BMI= body mass index CAD= coronary artery disease CD154 = CD40 ligand. Protein in macrophage membrane, CD4 + activated T cell, endothelial and other cells. CVD=cardiovascular disease CR = cardiac rehabilitation CSA = cross sectional area eNOS = constitutive endothelial nitric oxide synthase iNOS = inducible nitric oxide synthase nNOS = constitutive neuronal nitric oxide synthase TNF-α = Tumor necrosis factor alfa TGF-β = Transforming growth factor beta IL-6 = interleukin 6
After cardiac rehabilitation nitrate levels increased in skeletal muscle. Body fat correlated inversely with higher NO production in rehabilitated patients. Transforming growth factor β was related with decreased inflammation and higher NO.
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ACCEPTED MANUSCRIPT 1.INTRODUCTION. Cardiovascular diseases (CVD) are the leading cause of death in the world. According to WHO in 2012, 17.5 million people died from CVD, of which 7.5 million deaths were from coronary artery disease and 6.7 million from cerebrovascular accidents [1]. Exercise based CR programs were developed for patients after
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acute myocardial infarction (MI) to help them regain their previous exercise capacity and facilitate reintegration into working life. It has been demonstrated that CR is a highly efficient, innocuous and economic therapeutic intervention [2]. There is ample evidence that diet and medical treatment of risk
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factors play a role in prevention and control of CVD [3]; moreover, CR including its 6 fundamental aspects (patient education, psychological aid, occupational therapy, dietetic orientation, medical treatment and
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exercise) is crucial in secondary prevention of the disease. Some studies indicate that the modification of risk factors have a very positive impact on morbidity due to cardiac events, both recent and recurrent. After an acute coronary syndrome, the effects seem to be even more pronounced leading to a 40% decline in 6month mortality. [3, 4]. Physical training improves exercise capacity more than conventional medical
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therapy alone [5]. A year program of regular physical exercise in selected patients with stable coronary artery disease (CAD) resulted in higher event-free survival and exercise capacity compared with standard percutaneous coronary intervention [6]. Since 1995, CR participation after acute coronary syndrome and
treatment [7].
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coronary artery bypass grafting is associated with reduced mortality even in the modern era of CAD
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Training induces in both healthy subjects and CAD patients an increase in maximal oxygen consumption, which is the product of the capacity of the cardiovascular system to supply oxygen (i.e. cardiac output) and the capacity of skeletal muscles to use oxygen (i.e. arterial-venous oxygen difference).
In healthy
individuals this increase is aproximately produced in equal proportion by central and peripheral adaptations while in CAD subjects impaired cardiac function would place a higher contribution on adaptive changes in the periphery, and consequently demand less effort on cardiac function [8]. Regular physical exercise as part of a multifactorial intervention improves symptom free exercise tolerance and myocardial perfusion. Because no net regression of epicardial coronary stenosis was observed in the majority of patients, and many 4
studies of collateralization in CAD patients have reported that exercise did not improve angiographically
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detectable collateralization, the current evidence does not firmly support the hypothesis that these beneficial effects of exercise result from a blunted progression and/or an increased regression of coronary lesions, instead it indicates that exercise increases endothelium dependent dilation in the conduit arteries and larger resistance arteries [9], as a result of increased nitric oxide (NO) production and bioavailability [10].
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Exercise also produces higher myogenic control, increased metabolic vasodilatation in small resistance arteries, and direct cardiac effects as improved calcium handling, increased P13K activity, reduction of fibrosis and cardiomyocyte apoptosis [4].
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Adaptive changes to endurance training in peripheral muscle are: increased oxygen extraction by correcting endothelial dysfunction and increasing basal NO formation [11]; improvement of oxidative metabolism,
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showed by increase in activity of oxidative enzymes [12]; increased levels of phosphocreatine/inorganic phosphates [13]; changes in mitochondrial ultrastructure [14]; increase of radical scavenger enzyme activity [15]; increase of COX-activity inversely correlated with iNOS expression /iNOS protein content [16]. In addition, there is a reduction of sarcopenia related to attenuation of MuRF-1 expression, a component of the
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ubiquitin-proteasome system involved in muscle proteolysis [17].
There are several reports of muscle inflammation in general diseases as type II diabetes mellitus [18] and chronic obstructive pulmonary disease (COPD) [19]. Patients with acute coronary syndrome, stable CAD, or
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chronic heart failure (CHF) showed elevated levels of inflammatory markers in peripheral blood mononuclear cells [20], plasma [21, 22] or skeletal muscle [23].
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Exercise has been reported to reduce some inflammatory markers in skeletal muscle of CHF patients [23], but not in plasma [22]. Generation of NO is related to inflammatory markers, as demonstrated by the induction of iNOS expression in skeletal muscle by IL-1b and NFkB activation [24]. Most of the work on peripheral effects of exercise on skeletal muscle in patients with CVD has been done ln patients with CHF, however, there is scarce information in MI patients. The hypothesis of the present work is that the improvement in oxygen consumption that is obtained with the rehabilitation program currently used in our University Hospital may be related to an increase in skeletal muscle NO production and to reduction in the muscle inflammatory state. For that purpose, nitric oxide synthases (NOS), nitrate, nitrite, 5
nitrotyrosine, tumor necrosis factor alpha (TNF-α), transforming growth factor beta (TGF-β), interleukin-6
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(IL-6) and CD154 were determined, along with several cardiorespiratory and metabolic parameters.
2. METHODS 2.1. Study subjects
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Seventeen male patients (54±8 years old) who entered a 12 weeks program of CR in the Unit of Cardiac Rehabilitation of the “Hospital Clínico Universitario” in Caracas (Venezuela), 8 weeks after been released from hospitalization due to a myocardial infarction (MI) of low or medium risk profile [25]. Each patient
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was examined before and after the CR program to be his own control. Eleven healthy male subjects (56±1 years old) were also examined to compare with them the results of the MI patients before and after CR
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(Table 1). All patients were treated with β-blockers, 16 had anti-aggregation therapy, 9 received ARAII, 4 received calcium antagonists, 3 were taking IECA and one, anticoagulant therapy; treatment was maintained during rehabilitation and for the performance of the ergometric tests. The Bioethical Committee of the hospital approved the study and patients and healthy subjects signed the informed consent.
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2.2. Body composition
Body fat percentage was estimated by skinfold thickness measurements using a caliper in four body regions; and equations to calculate body density and fat % [26]. Waist and hips circumference [27], and body mass
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index were assessed by standard procedures. 2.3. Ergometric test
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An exercise test was performed before and after the CR program, in an electrically braked cycle ergometer (Lode Excalibur Sport, USA), frequency of 60 cycles per min. After 3 min of unloaded pedaling, 25 watts´ resistance increases were added every 3 min until exhaustion, or when blood pressure or heart rate increased or decreased disproportionally, or ECG changes showed signs of complex arrhythmias or myocardial ischemia. ECG was monitored during the whole test, and the 15 final seconds (s) of each stage were recorded. Blood pressure (BP) was measured in the final 30 s of each stage and at 1, 2, 3, 5, 7 and 10 min post-test. Physiological variables were registered in an automatic equipment (ULTIMA 20 MedGraphics,
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USA), with a metabolic and respiratory analyzer, following the established protocol. All patients finished
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the test despite of minor ECG and cardiac rhythm changes in some subjects,
2.4. Physical training The CR program used is that currently practiced in the University Hospital of Caracas. Training program
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consisted in three weekly sessions of approximately 60 min of exercise, during 12 weeks for a total of 36 sessions during the study period. Sessions consisted of three parts: 1) warming and neuromuscular conditioning including loosening, stretching, articular mobility and flexibility, during 15 min. 2) aerobic
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exercise during 20 min the first two weeks and then 30 min the rest of the sessions, bicycling or walking on a thread-mill in the firsts sessions, that allowed a better control of HR and BP, and walking on a track
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in the lasts sessions. The intensity was tailored for each patient according to the result of the prerehabilitation ergometric test (60-80% of VO2 max). 3) final recovery and relaxation exercises for 10-15 min. First week started with 60% of maximum heart rate obtained in the previous effort test, if well tolerated, it was increased to 70% in the second week, to 80% in the third week and kept at this level until
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the end of the 12 weeks. Walk speed/pedaling rate were adjusted accordingly to maintain the intensity at 80%. Al training sessions were supervised by physiotherapists and one cardiologist.
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2.5. Lactatemia
Blood lactate was measured in the ear lobe, before the test and 3 min after the end. Blood was analysed with
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a mini-photometric equipment (Miniphotometer Dr Lange Plus 20, Berlin, Germany). 2.6. Echocardiogram
A trans-thoracic echocardiogram (TTE) was performed with a Philips Sonos 4500 equipment, before and after CR. The axes determined were; long left parasternal, short left parasternal, sub-costal, and 4 chambers, with a transducer of 2.5 MHz. The inter-ventricular septum width, the diameters of the posterior wall of the left ventricle and the left atrium, and the ejection fraction were measured. 2.7. Skeletal muscle determinations
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Patients underwent needle muscle biopsies [28] before and after CR. Healthy subjects were biopsied only
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once. The sample of approximately 50 mg was immediately blotted and divided in three parts; the first part was embedded in OCT compound (Tissue TEK; Sakura Finetek Torrance, CA) and dipped in isopentane frozen in liquid nitrogen; the two other parts were directly frozen in isopentane, all samples were wrapped in identified aluminum paper and placed in liquid nitrogen to transport them to a freezer to be stored at -80ο
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until processing. The procedure from taking the sample to be frozen lasted less than 1 min. 2.7.1. Histochemical Procedures
Fiber type classification and capillary measurements were done in 10 µm transverse serial sections cut in a
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cryostat at – 20°C, with the adenosine triphosphatase reaction after alkaline (pH 10.3) and acid (pH 4.37 and pH 4.6) preincubation [29]. Capillaries were visualized by the α-amylase periodic acid Schiff reaction [30].
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Photomicrographs at a final magnification X 200 were made, and fibers were identified by comparison with the adenosine triphosphatase sections. An area of the photograph was delimited, measured with a planimeter, and fibers and capillaries were counted to calculate the mean fiber CSA, capillaries per square millimeter, and capillaries per fiber ratio. Capillaries around each fiber type were counted and all the fibers
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of one type were drawn together to measure area by planimetry to calculate the mean area of each fiber type. 2.7.2. Determinations of muscle metabolism enzymes. Muscle samples for enzymes activities were weighted at -20οC, homogenized in ice cooled potassium
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phosphate buffer. The activities of citrate synthase (CS) 3-31hydroxy-acyl-CoA-dehydrogenase (HAD) and lactate dehydrogenase (LDH) were assayed using fluorometric techniques [31].
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2.7.3. Assessment of nitrate, nitrite, eNos, iNOs, nNOs and nitrotyrosine levels. The muscle sample was weighed and homogenized with a glass pestle in 1 mL of Tris-HCl buffer, 10 mmol/L, pH 7.5; NaCl, 150 mmol/L; ethylene-diamine tetra-acetic acid, 5 mmol/L; triton x-100, 1% (volume/volume); leupeptin, 10 µg/mL; aprotinin,10 g/mL; and pepstatin, 2.5 g/mL. The homogenate was centrifuged at 90g for 5 min. Supernatant was used for the assays. Protein concentration was assessed by the BCA protein assay kit (Pierce Biochemicals; Rockfort IL). NO levels were determined indirectly by quantification of their oxidized products of degradation, using nitrate reductase and the Griess reagent. A standard curve was obtained with sodium nitrate dissolved in water or in a pool of normal sera. Nitrite 8
concentration was determined at 540 nm using enzyme-linked immunosorbent assay (ELISA) plate reader
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(Multiscan MCC/340; Labsystems; Helsinki, Finland). All three NO synthases were assessed using sandwich ELISA assays. Constitutive eNOS was detected using a commercial kit (R&D Systems; Minneapolis, MN). Monoclonal and polyclonal antibodies for nNOS were from BD Biosciences (San Diego CA), and the recombinant enzyme for the standard curve was from Calbiochem (San Diego, CA).
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iNOS was assessed using a pair of antibodies (Serotec Corporation; Kidlington, Oxford, UK). The sensitivity of all assays was 25 pg/mL. Total amount of nitrotyrosine was determined by ELISA. The mouse immunoglobulin (Ig)-G monoclonal antibody, the polyclonal antibody against nitrotyrosine and the
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polyclonal goat anti-rabbit IgG-peroxidase antibody were purchased from Upstate Biotechnology (LakePlacid, NY, USA). The quantification of nitrotyrosine was performed using a standard curve with
the assay was 50 pg/mL [19]. 2.7.4. Assessment of inflammatory markers.
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known concentrations of nitrotyrosine from chemically modified bovine serum albumin. The sensitivity of
CD154 levels were detected by a commercial sandwich immunoenzymatic assay purchased from Chemicon
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Corporation (Temécula, CA, USA). The ELISA plates were already coated with the capturing monoclonal. The samples were diluted as specified by the manufacturer in the assay buffer, and the only modification was that samples were incubated for 18 h at 4º C. Quantitative analysis was performed with a standard
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curve. The detection limit was 1 ng CD154 per mg of protein. TGF-β and IL-6 were measured with ELISA sandwich in solid phase following the protocol recommended by the manufacturers of the reactive (R&D
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Systems, Minneapolis, USA).
TNF-a was assessed by a third generation TNF-a quantikine assay (R & D systems) following the manufacturer’s instructions, except that samples were diluted as suggested for serum samples and incubated for 18 h instead of 3 h. The sensitivity of the assay was 0.5–3 pg/mL. 2.8. Statistical Analysis Data in tables is expressed as mean ± SD. The results of each variable were evaluated in patients before and after CR with Student paired “t” test. The comparison of control subjects with patients before and after CR was done with non-paired “t” test. The Pearson product-moment correlation coefficient for grouped data and 9
Spearman for ungrouped data were used to establish correlations between the different variables of the
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study. The statistical program StatSoft Statistica was used for the analysis. A “P” value of less than 0.05 was considered statistically significant.
3. RESULTS
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3.1. Anthropometric characteristics Table 2 shows the bio-anthropometric characteristics of the patients. Although there was not a significant difference in weight and BMI, fat percentage was reduced after rehabilitation, indicating an increase in fat
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free mass and body density. The anthropometric characteristics measured in the healthy subjects group were not different compared to those of the patients before rehabilitation: weight (71.9±14.8 vs 75.5± 10.2 kg),
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height (167±8 vs165±17 cm), and BMI (26.43±3.0 vs 26.27±17.0), all P>0.05.
3.2. Exercise capacity
After CR, a highly significant increase in maximal oxygen consumption was found (P< 0.001), all patients
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passed the first category of Weber and Janicki [32]. Work load and work time increased; pulmonary ventilation, anaerobic threshold, maximal lactatemia and oxygen pulse also showed significant increments (p<0.001), (Table 3).
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3.3. Skeletal muscle characteristics
3.3.1. Cross sectional area and capillary indexes
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Patients showed an increase in the CSA of type I fibres after CR, P< 0.02 (Table 1). Before CR the patients, compared to healthy subjects, had a lower mean CSA of fibers (P<0.02), however, after CR there were no differences between the CSA of muscle fibers of patients and the healthy subjects (Table 1). Capillary density did not change after CR and did not differ between the healthy subject and the patient groups. (Table 1). 3.3.2. Muscle metabolism enzymes There were no changes after CR in muscle oxidative enzymes: (Table 1). CS activity was found higher in patients than in healthy subjects, both before and after rehabilitation (P<0.05). HAD activity was similar in 10
healthy subjects and patients; LDH was lower in patients before CR than in healthy subjects (P<0.05);
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however, significance of the difference disappeared after CR (Table 1). 3.3.3. NO production in muscle After CR, nitrate level was found highly significantly increased (P<0.001) (Table 1). No modification in the activity of NOS isoforms was seen after CR. Nitrate and nitrite concentrations were lower in patients as
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compared to healthy subjects (p<0.0001 and p<0.005 respectively); on the contrary, nitrotyrosine was higher (p<0.001) (Table 1). Although the value of nitrate increased after CR, it did not reach that of the healthy subjects. The constitutive isoforms of NOS, nNOS and eNOS, were lower in patients compared to healthy
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subjects (p<0.0001 and 0.05 respectively), and the inducible isoform iNOS was higher (p<0.005) (Table 1). 3.3.4. Inflammatory markers in muscle
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In Table 1 it is shown that there were not significant differences in the levels of the inflammatory markers post CR in comparison with those before rehabilitation. The measured inflammatory markers were significantly higher in patients as compared to healthy subjects, both before and after CR (TNF-α P<0.05, TGF-β and IL-6 P<0.005, and CD154 P<0.002). In all the healthy subjects, the levels of TNF-α were under
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the sensitivity of the method (Table 1).
3.4. Correlations between the studied variables
Positive and negative correlations between anthropometric characteristics versus NO products, enzymes and
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inflammatory markers are shown in Table 4. In Table 5 are reported the correlations between aerobic (CS and HAD) and anaerobic (LDH) metabolism enzymes; NO production enzymes (NOS), NO products
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(nitrite, nitrate and nitrotyrosine) and the inflammatory mediators (TNF-α, TGF-β, IL-6 and CD154). There was a negative correlation (see Table 4 for P values) between weight, BMI, fat%, waist and hip circumferences and eNOS, nitrite or nitrate after CR (Table 4). TGF-β correlated directly with nitrite and nitrate before CR, with all NOS after CR, and inversely to other inflammatory factors (see Table 5 for P values.). Correlation between the differences of the values after and before CE were significant for nitrite and maximal oxygen consumption expressed as VO2 mL/Kg.min (P<0.0001), and between nitrite and nitrate (P<0.002).
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4. DISCUSSION
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4.1. Main findings. There is ample information on the effects of regularly practiced exercise in skeletal muscle of healthy subjects. However, the morphological and functional changes in skeletal muscles in disease, and their modification by CR, is less known. The present study was done in patients with MI. In agreement with our
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hypothesis it was found a significant increase of nitrate levels in muscle after CR (P<0.001); the increase of nitrate and/or nitrite is considered a physiological increase of NO production. In addition, the differences of nitrite levels and maximal oxygen consumption (VO2 mL/Kg.min) after and before CE showed a direct
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correlation (P<0.0001). Also, a direct correlation was found between the differences pre- and postrehabilitation values of nitrite and nitrate (P<0.002). Another relevant finding was the inverse correlation
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between weight, BMI, percentage of body fat and circumference of waist and hip, and muscle eNOS values and, except percentage of body fat, also to nitrite; moreover, percentage of body fat was inversely related to nitrate levels (Fig. 1). The decrease of body fat percentage was not accompanied by weight change or by decrease of body mass index, which means an increase of lean body mass and body density. These results
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could be interpreted as a higher capacity of subjects with less fat to produce NO. On the other hand, the second part of our hypothesis, the decrease in the levels of inflammatory markers after CR, could not be demonstrated (Table 1). An important finding regarding inflammatory markers was the positive correlation
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of TGF-β with nitrites and nitrates before CR, and post CR with nitrite and all the three NOS (Table 4, Fig. 2). Fig. 3 illustrates the negative relationship of TGF-β with nitrotyrosine (post CR), with TNF-α (pre- and
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post- CR) and also with IL-6 (before CR). These results are in favor to a role of TGF-β as an antiinflammatory factor in patients with MI. 4.2. Cardiorespiratory effects The results obtained in cardiorespitatory functions with the present program of CR are likethose found by others:19.1% and 21.2 % for absolute and relative maximal oxygen consumption [33,34]. The changes in work load (watts) and exercise time were 12.6% and 20.3%, without change in mechanical efficiency. Maximal pulmonary ventilation increased 23.4%. There was a highly significant increase in oxygen pulse, which is a better indicator than VO2 for the appreciation of changes in maximal cardiac output [35]. In the 12
present study the increment of AT after CR was 11.8% and that of lactatemia was 13.6% [36]. Accordingly,
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AT, work load and pulmonary ventilation correlated directly to VO2 max. 4.3. Muscular changes 4.3.1. Fiber types and CSA In the present work no differences was found in the distribution of fiber type after CR, although Hambrecht
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et al [37] have reported a marginal increase in type I fibres proportion. This difference may be due to the longer duration of their program (6 months compared to 3 months). CSA of type I fibers augmented, and this caused that the differences in mean CSA disappeared after CR between patients and healthy subjects; this
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result differs from that of only 4 weeks training study [17]. 4.3.2. Muscle metabolism enzymes
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A group of MI patients has been studied in a previous work of the same laboratory (12); that group showed low levels of CS, 9.0 ± 2.9 µmol/gr.min before CR that increased to 16.0 ± 4.8, P<0.01 after only 6 weeks of a similar program of CR, they also showed an increase in HAD and a decrease in LDH after rehabilitation in contrast with the group of the present study that did not show any change in the enzyme levels with
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rehabilitation. In the present work the level of CS was higher in patients before CR than in healthy subjects and the difference was maintained after CR. These results may be explained because our healthy subjects were sedentary and the present group of patients was heterogeneous in their activity level. It is to be noticed
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that patients joined the CR program 8 weeks after leaving hospital with a recommendation to initiate a program of moderate exercise before joining formal CR; most of the patients confirmed to have done it.
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However, it was observed that the three patients that showed the higher increment in in max VO2 (25%, 26% and 27%) did have an increase in CS and HAD levels. 4.3.3. NO generation
The patients studied showed endothelial dysfunction, with low levels of nitrite and nitrate, eNOS and nNOS, and increased nitrotyrosine and iNOS in skeletal muscle. This indicates a low production of “physiological” NO with high production of “pathological” NO that reacted with superoxide to form peroxynitrite [15, 38] as shown by the increase of nitrotyrosine, the end-product of the nitrosylation of tyrosine by peroxynitrite. In addition, iNOS showed a negative correlation with both constitutive isozymes nNOS and eNOS levels. 13
Other authors have found increased iNOS expression and nitrotyrosine levels in skeletal muscle of patients
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with chronic heart failure [39]. It is well known that regular physical exercise, personally tailored and controlled, has important effects on cardiovascular health and survival [40,41], attenuates disease progression [9], reduces hypertension [42] and produces changes in the lipoprotein subclass profile [43]. Reactive oxygen species (ROS), inflammatory
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factors and NO are involved in the development of these responses [15,4,10]. Unexpectedly eNOS was not increased in muscle after CR in the current work. However, the direct correlation between nNOS and nitrite present before CE reached a higher signification post-rehabilitation; moreover, a high significance direct
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correlation appeared between eNOS and nitrite. This may be interpreted as an improvement in vasodilator
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capacity in muscle after CR.
4.3.4. Inflammatory markers
There is evidence of the role of inflammatory processes in cardiovascular diseases: it has been demonstrated in the development of atherosclerosis [21]; expression of TNF-α and IL-6, together with other interleukins
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(IL-10, IL-23A, IL-27 and IL-37), was significantly higher in peripheral blood mononuclear cells of patients with acute coronary syndrome [20]; patients with cardiac hearth failure showed increased serum levels of TNF-alpha, IL-6, and IL-1-beta [22]. In skeletal muscle of patients with cardiac heart failure it has been
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found increased levels of TNF-α, IL-1-beta, IL-6 with normal values in serum, [23]. In the present work
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patients showed increased levels of TNF-α, TGF-β and IL-6, and CD154 in skeletal muscle. It has been demonstrated that training for 6 months significantly reduced the local expression of TNF-α, IL1-beta, IL-6 and iNOS in skeletal muscle of patients with cardiac hearth failure [23]. Other authors did not find reduction of inflammatory markers in blood after 4 months of high intensity training in patients with cardiac heart failure and arterial hypertension, but they did in patients with idiopathic dilated cardiomyopathy [22]. Differences in results may be related to duration of training and to the cardiovascular status of patients. It is to note that the standard deviation of the values of inflammatory markers in our patients was high, and some of them showed reduction after CR. It also may be possible that these 14
inflammatory markers have a modulatory effect in different moments of the rehabilitation process and in a
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different metabolic milieu.For example TGF-β is a pleiotropic peptide released by many cell types and involved in the regulation of tissue growth and homeostasis in many processes including inflammation and its resolution [44]. It represses skeletal muscle specific gene expression and has also been reported to modulate proliferation in satellite cells [45]. The relations between different inflammatory markers may also
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change during the rehabilitation process; for instance, in the present study TGF-β levels showed an inverse correlation with TNF-α both before and after CR; with IL-6 only before, and with nitrotyrosine after CR. Some markers have been demonstrated to modify NO production, TGF-β suppressed IL-1-induced iNOS
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expression and NO production in chondrocytes [46]. In our results, after CR, TGF-β correlated directly with all the tree isoforms of NOS, but also post CR iNOS negatively correlated to nitrotyrosine, suggesting that
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NO produced by iNOS was not reacting with ROS, but joining the vasodilator pool of NO. All this suggests that in our patients TGF-β was acting as an anti-inflammatory factor and this effect was more important after CR. Other change in relationship between the different inflammatory markers was seen with CD154, before CR CD154 levels directly correlated with IL-6 and TNF-α and the two last mentioned cytokines were also
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directly related between them. However, after rehabilitation the significance of the direct correlation between CD154 and IL-6 was reduced, and the direct correlation between TNF-α and CD154 disappeared.
exercise. 4.4. Limitations
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These results suggest that the modulation effect between pro-inflammatory markers may be affected by
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Due to the invasive nature of procedure used to obtain the skeletal muscle samples, a relatively small number of subjects was included in the study; this probably limits the direct extrapolation of the present findings to the entire population of patients with myocardial infarction. The diversity of the level of physical activity in the patients provided a heterogeneous group that made difficult to obtain significant statistical results in some of the variables studied. The method applied to measure % body fat may be not sufficiently accurate, however it was performed by personnel that evaluates athletes and the results are coherent with the data of BMI and waist and hip circumferences. Greiss method is not the most sensitive assay to measure
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nitrite, but the results obtained with nitrate were highly significant, and we could not find other references of
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direct NO measurements in skeletal muscle in MI patients to compare.
5. CONCLUSION The present work reinforces the knowledge of the positive effects of CR in MI patients on oxygen
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consumption, physical work capacity, cardiac function, lactate production, anaerobic threshold and anthropometric characteristics. Skeletal muscle showed increase in NO production, as shown by the increase in the level of nitrate. The change in nitrite levels in muscle after rehabilitation was directly correlated with
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the increase in maximal oxygen consumption. CSA of the muscle fibers increased. The enhancement of the correlations of NOS isoforms with nitrite and nitrate suggests a more efficient production of NO. There was
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found an inverse relationship between NO production and BMI, body fat percentage, and waist and hip circumferences, indicating a better NO production in subjects with less body fat. The direct association of TGF-β with NO, nitrite, nitrate and NOS, and inverse relationship with inflammatory markers TNF-α and IL-6 in skeletal muscle strongly suggest an anti-inflammatory role. The direct correlation between pro-
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inflammatory markers was less significant or disappeared after CR. All these results may be interpreted as a change of the modulatory effects of inflammatory markers after the rehabilitation treatment, concurrent with
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the improvement on exercise capacity of the patients.
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6. ACKNOWLEDGEMENTS.
Our special thanks to Professor Stephen Tillett for correction of the English language and to
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Assistant Professor Luis Vázquez (Public Health Department) for his help with statistics.
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ACCEPTED MANUSCRIPT 7. REFERENCES [1] World Health Organization. (2013, March) Cardiovascular diseases (CVDs) fact sheet No. 317. Retrieved from http://www.who.int/mediacentre/factsheets/ fs317/en/index.html.
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[2] Al Quait A, Doherty P. Does cardiac rehabilitation favor the young over the old? Open Heart, 2016; 3: doi: 10.1136/openhrt-2016- 000450.
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Circulation. 2010; 122:1221-38.
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Coronary Angioplasty Compared With Exercise Training in Patients With Stable Coronary Artery Disease. A Randomized Trial. Circulation. 2004; 109:1371-78.
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cardiac rehabilitation participation and health status outcomes after acute myocardial infarction. JAMA Cardiol. 2016 JAMA Cardiol. 2016; 1:980-8. [42] Neves VJ, Fernandes T, Roque FR, Soci UP, Melo SF, de Oliveira EM. Exercise training in hypertension: Role of microRNAs. World J Cardiol. 2014; 6: 713-27.
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meta-analysis. Open Access Journal of Sports Medicine. 2018;9: 1–17.
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ACCEPTED MANUSCRIPT TEXTS OF FIGURES FIGURE 1 Correlations between body mass index (BMI) and body fat percentage (% fat) after cardiac rehabilitation.
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eNOS: endothelial nitric oxide synthase. A: p<0.005. B: p<0.005. C: p<0.05. D: p<0.02.
FIGURE 2
Correlations between transforming growth factor beta (TGF-β) and products and enzymes of nitric oxide.
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eNOS: endothelial nitric oxide synthase, nNOS: neuronal nitric oxide synthase. A: Before cardiac rehabilitation p<0.0005. B: After cardiac rehabilitation p<0.05, before cardiac rehabilitation the correlation
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between these variables was present with similar characteristics (not shown). C: After cardiac rehabilitation, p<0.01. D: After cardiac rehabilitation, p<0.005.
FIGURE 3
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Correlations between transforming growth factor beta (TGF-β) and inflammatory factors. TNFα: tumor necrosis factor alfa, IL-6: interleukin 6. A: Before cardiac rehabilitation p<0.05. B: After cardiac
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rehabilitation p<0.05. C: Before cardiac rehabilitation p<0.01. D: After cardiac rehabilitation p<0.005.
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ACCEPTED MANUSCRIPT TABLE 1. Comparison between healthy subjects and patients before (BCR) and after (ACR) cardiac rehabilitation, and comparison between patient values BCR and ACR. VARIABLES
Healthy
PBCR
subjects
H vs PBCR
PACR
P
H vs. PACR
PBCR vs.
P
PACR p
45±12
43±13
NS
42±9
NS
NS
% type IIA fibers
39±13
40±9
NS
43±10
NS
NS
% type IIX fibers
16±9
16±8
NS
16±9
NS
NS
Mean CSA (µm2)
5618±1273
3789±1104
<0.001
4399±1534
NS
NS
CSA type I fib(µm2)
6447±1441
4380±1868
<0.02
5237±1530
NS
<0.02
CSA type II fib(µm2)
5568±1331
4193±945
<0.05
5523±1830
NS
NS
CSA type IIX fib (µm2)
5166±1514
4218±1490
NS
5237±2452
NS
NS
Cap Adj. I (n)
4.6±0.8
4.8±0.8
NS
4.7±0.5
NS
Ns
Cap Adj. IIA (n)
4.2±0.8
4.2±0.3
Cap Adj. IIX (n)
3.6±1.0
3.0±0.8
DC (cap x mm2)
308±83
410±98
C x F (n)
1.65±0.29
1.57±0.34
CS (ng/mg-prot)
11.14±2.10
14.32±3.0
HAD (ng/mg-prot)
10.04±1.90
LDH (ng/mg-prot)
196±53.00
Nitrite (ng/mg)
17.44±4.47
Nitrate (ng/mg)
24.04±3.85
NO2- + NO3- (ng/mg)
4 1.83±6.49
Nitrotyrosine(ng/mg)
7.93±3.86
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NS
NS
NS
3.7±0.9
NS
NS
<0.05
411±128
<0.05
NS
NS
1.63±1.59
NS
NS
<0.05
15.90±5.08
<0.05
NS
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NS
10.15±2.6
NS
10.86±3.69
NS
NS
151.1±45.92
<0.05
150.8±58.20
NS
NS
5.64±0.56
<0.000000
5.79±0.70
<0.000000
NS
18.59±3.04
<0.005
20.71±2.00
<0.005
<0.001
24.23±3.21
<0.000000
26.61±2.29
<0.000000
NS
13.70±3.95
<0.001
14.90±5.04
<0.001
NS
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% type I fibers
nNOS (ng/mg-prot)
120.00±31.36
12.19±3.99
<0.000000
13.33±3.52
<0.000000
NS
iNOS (ng/mg-prot)
8.05±4.21
14.05±3.60
<0.005
14.31±3.72
<0.005
NS
eNOS (ng/mg-prot)
43.65±31.35
21.92±5.27
<0.05
23.79±6.22
<0.05
NS
TNF-α (pg/mL)
< 5.00
63.67±59.50
<0.05
53.50±46.81
<0.05
NS
TGF-β (pg/mL)
19.66±4.64
162.67±97.61
<0.005
172.20±102.0
<0.005
NS
IL-6(pg/mL)
18.64±4.79
182.17±108.25
<0.005
165.9±106.70
<0.005
NS
CD 154 (pg/mL)
24.32±6.47
130.50±79.09
<0.002
108.4±50.14
<0.002
NS
H: Healthy. PBCR: patients before cardiac rehabilitation. PACR: patients after cardiac rehabilitation.CSA: Cross sectional area. Cap adj..I: Mean number of capillaries around type one fiber. C x F: Capillary per fiber index. DC: Capillary density. NS: no significant.
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ACCEPTED MANUSCRIPT TABLE 2. Bio-anthropometric data and body composition. Before RC
After RC
P
Age (years)
53.9±8.03
-
-
Weight (kg)
75.6±10.24
74.4±8.62
NS
Height (cm)
168.4±5
-
BMI (kg/m2)
26.3±3.02
26.0±2.58
Fat %
16.8±4.60
15.0±2.58
Waist (cm)
93.3±6.58
92.3±6.30
Hip (cm)
96.9±5.09
95.7±4.73
<0.05
Waist/Hip
0.96±0.06
0.96±0.05
NS
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Variables
NS
<0.001 <0.01
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BMI: Body mass index.
-
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TABLE 3. Cardio-circulatory and respiratory variables in exercise test before and after
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After RC
P
Watts
116±15
140±17
<0.001
Exercise time (sec)
836±107
1006±125
<0.001
VE (L/min)
59.8±7.5
73.8±11.6
<0.001
VO2 max (mL/min)
1596±216
1901±223
<0.001
VO2 max(mL/kg/min)
21.2±1.4
25.7±2.5
<0.001
VE/VO2
37.2±5.1
VE/VCO2
31.9±4.5
La max (mM/L)
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Variables
NS
33.2±3.8
NS
8.1±1.4
9.3±1.5
<0.001
AT (% VO2 max)
53.8±3.5
60.2±3.3
<0.001
Oxymetry (SpO2%)
96.1±1.3
96.0±1.1
NS
HR max (bpm)
135±13
136±15
NS
183±11
186±12
NS
92±5
91±4
NS
DP (SBP x HR)
24673±3085
25286±3708
NS
VO2/HR (mL/beat)
11.7±1.6
14.0±1.9
<0.001
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DBP max (mmHg)
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SBP max (mmHg)
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38.7±4.0
AT: anaerobic threshold. DP: double product. La max: maximal lactate.
VP: pulmonary ventilation. Max HR: maximal heart rate. VP: pulmonary ventilation. VO2/HR (mL/beat): Oxygen pulse
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TABLE 4.- CORRELATIONS BETWEEN ANTHROPOMETRIC CHARACTERISTICS vs. NO PRODUCTS, ENZYMES AND INFLAMMATORY MARKERS. PRE-REHABILITATION eNOS
NO2-
nNOS
NO3-
NO2-+NO3-
IL-6
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Weight 0.65*e
0.58*e
NO3-
NO2-+NO3-
-0.58*f
-0.61*f
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Height BMI FFMII % fat Waist Hip Waist/hip
POST-REHABILITATION nNOS
-0.63*f -0.76**f -0.70*f
IL-6
-0.66*f
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-0.74**f
NO2-0.57**f
-0.56*f
-0.56*f -0.71**f -0.74**f
-0.55*f
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Weight Height BMI FFMI % fat Waist Hip Waist/hip
eNOS -0.59*f
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p < 0.05; ** p< 0.01; *** p < 0.001. Negative correlations are preceded by a negative sign. Letters are used to point that signification was: a= similar before and after CR, b= higher after CR, c=lower after CR, d= changed from + to – after CR, e=present only before CR, f= present only after CR
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TABLE 5 CORRELATIONS BETWEEN OXIDATIVE AND GLYCOLITIC ENZYMES, ISOFORMS OF NOS, NO PRODUCTS AND INFLAMMATORY MARKERS PRE-REHABILITATION AND POST-REHABILITATION
NO2-
NO2-+NO3-
PRE-REHABILITATION nNOS iNOS
NITROT.
0.58*d 0.62*b
NO2-+NO3-
TGF-β -0.62*e
IL-6
-0.75**a
0.64*a 0.87**e 0.89***e
-0.76**e
-0.60*a
0.79**e -0.72**e
CD 154
0.52*f -0.57*d 0.59*f 0.96***a
0.58*f -0.70**f
-0.56*a 0.56*b
-0.59*a
0.56*e 0.77**c
eNOS
TNF-α
TGF-β
IL-6
CD 154 0.62*
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0.78***b
NO2-
POST-REHABILITATION NITROT. nNOS iNOS
EP
CS HAD LDH NO2NO3NO2-+NO3NITROT. nNOS iNOS eNOS TNF-α TGF-β IL-6
LDH
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-0.56*b
HAD
TNF-α
0.64*e
0.99***a
POST.R
eNOS
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LDH
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HAD 0.55*b
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PRE-R CS HAD LDH NO2NO3NO2-+NO3NITROT. nNOS iNOS eNOS TNF-α TGF-β IL-6
0.83***b
0.87***b
0.68**f -0.74**a
-0.84***b
0.65* -0.58*a 0.71**b
0.63*f -0.62*a
-0.56*f
-0.65*
0.65*a
-0.75**f 0.75**f 0.57*f 0.77*f -0.65*a 0.59*c
p < 0.05; ** p< 0.01; *** p < 0.001. Negative correlations are preceded by a negative sign. Letters are used to point that signification was: a= similar before and after CR, b= higher after CR, c=lower after CR, d= changed from + to – after CR, e=present only before CR, f= present only after CR 28
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Highlights:
After cardiac rehabilitation nitrate levels increased in skeletal muscle. Body fat correlated inversely with higher NO production in rehabilitated patients.
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Transforming growth factor β was related with decreased inflammation and higher NO.