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Физиология
DOI: 10.14529/hsm200301
EFFECTS OF ZIZIPHUS JUJUBE SUPPLEMENTATION ON PRO- AND ANTI-APOPTOTIC PROTEIN EXPRESSION IN NEUTROPHILS AFTER RESISTANCE EXERCISE
S.M. Tayebi1, tayebism@atu.ac.ir, tayebism@gmail.com, ORCID: 0000-0003-0459-4443, K. Krüger2, karsten.krueger@sport.uni-giessen.de, ORCID: 0000-0003-1506-8254, M. Safakar3, safakar.m@yahoo.com, ORCID: 0000-0002-6355-2107, P. Bahrami3, bahrami.pouran@yahoo.com, ORCID: 0000-0002-0111-2077, G. Tahmasb3, tahmasb.g@yahoo.com, ORCID: 0000-0002-6663-4319, A.V. Nenasheva4, nenashevaav@susu.ru, ORCID: 0000-0003-0092-2948
1Allameh Tabataba'i University, Tehran, Iran, 2Justus-Liebig-Universität Gießen, Gießen, Germany, 3Kerman Branch, Islamic Azad University, Kerman, Iran, 4South Ural State University, Chelyabinsk, Russian Federation
Introduction. It is suggested that jujube might have beneficial effects on exercise-induced immune perturbations, specifically on neutrophils apoptosis regulation, but its cellular mechanism is unclear. Aim. The aim of this study was to investigate the acute effect of Ziziphus jujuba administration on pro- and anti-apoptotic protein levels in human neutrophils in response to a session of circuit resistance exercise (Ex). Material and Methods. Participants completed an Ex (75 % 1RM, 9 exercises, 3 sets). While one group received a placebo, the other group (Zj) was supplemented daily with jujube (0.5 gr/kg body weight suspended in 2.5cc distilled water) one hour before Ex. Results. Ex increased the neutrophil level of [Ca2+]b calpain-1 and caspase-3 (p < 0.05) while a reduction of calpastatin and XIAP were observed (p < 0.05). Zj either suppressed the [Ca2+]j or reversed the calpastatin, calpain-1, XIAP, and caspase-3 responses (p < 0.01). Conclusions. The data indicate that a single session of intensive Ex induced apoptotic signaling in human neutrophils with the involvement of [Ca^-calpastatin-calpain axis upstream caspase-3. Acute administration of jujube solution before exercise attenuated these effects probably by providing energy sources for neutrophils or by functioning as antioxidants.
Keywords: jujube supplementation, resistance exercise, neutrophil apoptosis, calpastatin-calpain axis, caspase-3, XIAP.
INTRODUCTION
Neutrophils are cells which represent a first line defense against pathogens. Besides, they are known to be key regulators of inflammatory responses which die through spontaneous apoptosis at inflamed tissues [16, 17, 31].
A single bout of high intensity exercise is known to mobilize neutrophils from the marginal pool into the circulation [17]. After intensive exercise, several neutrophils function like oxida-tive burst or migration are temporarily inhibited which is speculated to clinically affect risk of infection. Recently, it was shown that intense exercise affects neutrophils lifespan by modifying their susceptibility to apoptosis [16]. There are conflicting data regarding exercise-induced
neutrophil apoptosis. It is demonstrated that acute severe exercise induced an oxidative state in neu-trophils which resulted in acceleration of spontaneous neutrophil apoptosis [31]. Besides, it is found that moderate exercise did not affect neu-trophil apoptosis, but intensive resistance and endurance exercise delayed neutrophil apoptosis during recovery period [23]. So, what is the explanation to these conflicting results? Maybe focus on cellular and molecular mechanisms.
Previous studies demonstrated that a single session of acute exercise induced DNA fragmentation, mitochondrial membrane depolarization, and increased expression of pro-apoptotic genes (bax and bcl-xS), while expression of anti-apoptotic genes (bcl-xL) in rat neutrophils were
suppressed [15, 18]. Furthermore, exercise was accompanied by an increase of p53 and caspase-3 expression, whilep38 MAPK and JNK where phosphorylated [16]. An important anti-apoptotic modulator in neutrophils is represented by cal-pastatin. A decrease in calpastatin expression may release the constitutively active calpains to cleave Bax into an active fragment and deactivate XIAP [9]. Both calpastatin and calpain-1 represent critical proximal elements in a cascade of pro-apoptotic events leading to Bax, mitochondria, and caspase-3 activation, and their altered expression appears to affect life span of neutrophils under pathologic conditions [3]. However, the expression of these calcium-dependent proteins after exercise has not been investigated yet. Recently, exercise induced an increase of intracel-lular calcium ([Ca2+]i) transients [23], suggesting the involvement of calpastatin-calpain-calcium axis in neutrophils apoptosis regulation during exercise.
In athletes, an increasing prevalence of supplementation is reported [30]. An important reason for taking supplements is to prevent exercise induced immunodepression and to decrease likelihood of illness [24]. Although supplementation of hydrolyzed whey protein enriched with gluta-mine dipeptide had no effect on immune cells [7], glutamine supplementation affected exercise induced immune perturbations by reducing neutro-phils apoptosis [15, 16, 18]. However, long-term consumption of chemical supplements can be harmful [39]. Accordingly, it is recommended to use natural or herbal supplements [32, 37].
Jujube (Ziziphus) is a native plant from southern Europe and Specially Asia [28]. It is known as Chinese date and red date [27]. It also grows in east, southeast and central of Iran, and is called "annab" [12]. Jujube has been traditionally used fresh or processed (dried) as food, food additive and flavoring agent for thousands of years, due to its high nutritional values [19]. Previous studies have revealed that jujube contains various constituents, including triterpenic acids [11] fla-vonoids [25], cerebrosides [11], amino acids [5], phenolic acids [8], mineral constituents [19], and polysaccharides [13]. Recent studies showed that jujube fruits have multiple bioactivities, such as anticancer [26], hepatoprotective [29], gastrointestinal protective [13], neuroprotective effects [40], antioxidant [4], anti-insomnia, immunos-timulating [20], and anti-inflammatory [41]. Accordingly, it is suggested that jujube might have
beneficial effects on exercise induced immune perturbations, specifically on neutrophils apoptosis regulation. In this regard, we previously demonstrated that solution supplementation one hour before exercise [34] and one week jujube solution supplementation [35] affected number of Annexin V positive neutrophils after exercise. However, up to now there are no data about the underlying cellular and molecular mechanisms which might affect balance of pro-and anti-apoptotic signals.
MATERIALS AND METHODS
Participants. The present study was approved by the Research Ethics Committee of the Tarbiat Modares University of Medical Science and was conducted in accordance with the policy statement of the Declaration of Iranian Ministry of Health. Written informed consent was obtained from participants. All subjects were asked to complete a medical examination and fill a medical questionnaire to ensure that during the past month they had not taken any regular medication, smoked, consumed alcohol or taken any regular exercise in the past 2 months, and were free of cardiovascular or metabolic diseases or recent symptoms of upper respiratory tract infection in the month prior to the start of these tests. Volunteers were randomly assigned to 2 groups (n = 7) including a Circuit Resistance Exercise (Ex) group with placebo (age: 25 ± 3 years, height: 171 ± 2 cm, weight: 67.5 ± 4.9 kg) and Ex group (n = 7) with Ziziphus jujube (Zj)/ solution (age: 25 ± 1 years, height: 180 ± 4 cm, weight: 74.1 ± ± 5.8 kg).
One repeat maximum (1-RM) test. 1-RM
value was determined by trial in three separate sessions, by adding or removing weights after each attempt, as required. Subjects were allowed to take as much time as they felt necessary to recover from each attempt. This was confirmed by visual and verbal feedback from participants.
Jujube preparation. The semi-dried fruits of Zj were washed, and seeds were separated and the soft red parts were removed. The samples were dried at 50 °C and ground to a powder using a mortar [37].
Combination assessment of jujube extraction by gas chromatography-mass spectrome-try (GC-MS). Compounds of Zj extraction were detected by GC-MS by semi-quantitative method. The contents of Zj extraction compounds were quantified using an internal standard (3-octanol, 99 %, Sigma-Aldrich). Wine volatile compounds
were analyzed using an Agilent 5975 Mass Spectrometer coupled to an Agilent 7890A Gas Chromatograph (Agilent, Santa Clara, USA). A DB-WAX column (60 m x 0.25 mm ID and 0.25 pm film thickness) was used for separation. The working parameters were as follows: injector temperature of 210 °C, EI source of 230 °C, MS Quad of 150 °C and transfer line of 210 °C. The initial temperature was 30 °C for 8 min, which was increased to 150 °C at a rate of 3 °C/min. Injector port temperature was 290 °C and helium used as carrier gas at a flow rate 1.5 ml/min. A total of 15 compounds were positively or tentatively identified by GC-MS that contain 92.27% the area under the peak totally (Table 1).
Exercise protocol. All participants performed a session of Ex in two cycles, simultaneously. Each cycle contained 9 exercises (seat up, back extension, biceps curl, triceps press, knee extension, knee curl, standing calf raise, chest press, seated row, machines were used in all exercises). The test included three non-stop circuits with a 3-minute active rest period between circuits. Each exercise was performed for 30 s (about 10-14 repeats) with 1RM of 75 % [33, 36].
Supplement protocol and blood collection.
The groups had a standard diet program during
3 days before test for unification and nutritional control. They received three meals/day: breakfast (10 kcalkg-1 BW, 70 carbohydrates, 18 % protein, 12 % fat), lunch (10 kcalkg-1 BW, 70 % carbohydrates, 18 % protein, 12 % fat) and, dinner (18 kcalkg-1 BW, 70 % carbohydrates, 15 % protein, 15 % fat). Subjects arrived at the test location, after 12 hours overnight fast, at 08:00 where they rested for about 30 minutes. Then subjects received placebo (2.5 cc/kg of body weight in distilled water sweetened with sugar without calories and colored by food dye) and Zj solution (0.5 gr/kg body weight in 2.5 cc distilled water) at 08:30 in double-blind manner and rested for about 60 min, at 09:30 all subjects performed the Ex in two cycles, simultaneously. The first peripheral venous blood samples were drawn at 08:30 before supplements of placebo and Zj solution, second blood samples were taken immediately after exercise at 10:00, then subjects remained seated for 120 min, and the third set of blood samples were taken at 12:00. The research design and blood collection is shown in Fig. 1.
Neutrophil isolation. Neutrophils were purified from venous blood treated with ACD from healthy volunteers by 3-steps: Dextran sedimentation, hypotonic lysis, and Ficoll sedimentation, as described previously [35].
Table 1
Combination assessment of jujube extraction by gas chromatography-mass spectrometry (GC-MS)
Combination The area under the Peak (%) Retention time (min)
Furfural 51.33 20.21
4-Pyrone 9.51 17.07
Oleic acid 6.31 39.00
Palmic acid 4.15 35.70
Imidazole 3.03 23.59
Cyclononasiloxane 2.03 42.05
Cyclodecasiloxane 1.75 35.63
Oxantin 1.61 10.65
Guanine 1.58 27.20
Gamma.-Sitosterol 1.17 44.56
Niphimycin 1.16 26.89
Iron 1.10 45.65
Butanediol 1.07 27.00
Phthalic acid 1.02 45.48
Pentasiloxane 1.01 48.34
Dodecanoic acid 0.97 27.616
Octadecamethyl 0.95 32.604
Methyl 2-furoate 0.92 14.28
1,4-dicarbonic acid 0.86 51.997
Tetradecanoic acid 0.74 31.840
Total 92.27
Fig. 1. Research Design and Blood Collection
Neutrophil's proteins and [Ca2+]i assessments. Determination of caspase-3 (E20120710034, 0.05-10 ng/ml), calpain-1 (E20120710031, 13-800 IU/L), calpastatin (E20120710032, 16-1000 IU/L), Bax (E20120710035, 0.3-90 ng/ml), and XIAP (E20120710036, 0.05-20 ng/ml) was analyzed by ELISA (Glory Science Co., Ltd, China). [Ca2+]iassessed by Atomic Absorption/ Flame Emission method and SPECTROPHOTOMETER system (Shimadzu, AA-670).
Statistical analysis. Repeated measure (two-way) ANOVA was used to determine the effects of TIME and Group by SPSS software at significance level of p < 0.05.
RESULTS
Muchly's sphericity assumption was meet for [Ca2+]i (W = 0.794; p = 0.281), calpastatin (W = 0.904; p = 0.573), calpain-1 (W = 0.849; p = 0.406), Bax (W = 0.712; p = 0.154), XIAP (W = 0.712; p = 0.154), and caspase-3 (W = 0.884; p = 0.508).
[Ca2+]i. The interaction effect ofTIMExGROUP was significant (F2,24 = 6.875; p = 0.005; n2 = 0.361). Accordingly, it increased linearly in placebo group during Ex and recovery period (Pre.Ex = = 0.88 ± 0.06, Po.Ex = 1.28 ± 0.02, 2hEx = 1.40 ± 0.04 mg/L). In contrast, in Zj group [Ca2+]i. levels remained unchanged over time (Pre.Ex = 1.47 ± 0.01, Po.Ex = 1.53 ± 0.01, 2hEx = 1.68 ± 0.08 mg/L) (Fig. 2a).
Calpastatin. The interaction effect of TIMExGROUP was significant (F2,24 = 4.802; p = 0.018; n2 = 0.286). Accordingly, it decreased linearly during exercise and recovery in placebo group (Pre.Ex = = 28 ± 0.8, Po.Ex = 26 ± 0.6, 2hEx = 23 ± 0.8 IU/L). But in Zj group, it is increased and decreased during exercise and recovery periods (Pre.Ex = 26 ± 1.2, Po.Ex = 30 ± 0.5, 2hEx = 25 ± 0.7 IU/L), respectively (Fig. 2b).
Calpain-1. The interaction effect of TIMExGROUP was significant (F2,24 = 14.799; p < 0.001; n2 = 0.552). Although it remained unchanged immediately after exercise in both placebo (Pre.Ex = 257 ± ± 7.3, Po.Ex = 256 ± 5.7 IU/L) and Zj (Pre.Ex = 280 ± 7.5, Po.Ex = 276 ± 6.7 IU/L) group, a significant elevation and placebo (2hEx = 276 ± 6.2 IU/L) and decline in Zj (2hEx = 259 ± 5.2 IU/L) group was found at 120 after exercise (Fig. 2c).
Bax. The interaction effect of TIMExGROUP was insignificant (F2,24 = 1.154; p = 0.332; n2 = 0.088) (Fig. 2d). Accordingly, it remained unchanged in both placebo (Pre.Ex = 37.5 ± 5.4, Po.Ex = = 29.3 ± 0.9, 2hEx = 30.1 ± 1.0 ng/ml) and Zj (Pre.Ex = 30.1 ± 0.8, Po.Ex = 29.3 ± 0.5, 2hEx = 29.8 ± ± 3.1 ng/ml) groups over time (Fig. 2d).
XIAP. The interaction effect of TIMExGROUP was significant (F2,24 = 6.727; p = 0.005; n2 = 0.359). Accordingly, it unchanged in both placebo (Pre.Ex = 4.21 ± 0.26, Po.Ex = 4.33 ± ± 0.17 ng/ml) and Zj (Pre.Ex = 4.21 ± 0.14, Po.Ex = 4.47 ± 0.12 ng/ml) group during exercise, but during recovery it had reduction in placebo group (2hEx = 3.89 ± 0.22 ng/ml) and elevation in Zj group (2hEx = 4.83 ± 0.18 ng/ml) (Fig. 2e).
Caspase-3. The interaction effect of TIMExGROUP was significant (F2,24 = 24.231; p < 0.001; n2 = 0.669). Accordingly, levels increased linearly during both exercise and recovery in placebo group (Pre.Ex = 5.5 ± 0.1, Po.Ex = 6.0 ± 0.1, 2hEx = 6.9 ± 0.2 ng/ml); and in Zj group, it unchanged during exercise and decreased during 120m recovery period (Pre.Ex = 6.3 ± 0.1, Po.Ex = 6.0 ± 0.2, 2hEx = = 5.4 ± 0.1 ng/ml) (Fig. 2f).
Placebo —•—Jujube (а) --•- Placebo —•—Jujube
J-
200 -T-1- 5 -I-
Pre.CRE Im.Po.CRE 120tti.Pii.CRE Pre.CRE Im.Po.CRE 120m.Po.CRE
Blood Sampling Time Blood Sampling Time
Fig. 2. The Acute Effect of Ziziphus jujuba Supplementation on some Pro- and Anti-Apoptotic Protein Levels of Human Neutrophils in Response to a Session of Intensive Circuit Resistance Exercise: a - effect on intracellular calcium levels; b - effect on calpastatin expression; c - effect on Calpain-1 expression; d - effect on Bax expression; e -effects on XIAP levels; f - effects on Caspase-3 levels. Pre: previous. CRE: circuit resistance exercise. Im.po: Immediately Post. 120 m: 120 minutes. x - interaction effect of GROUPxTIME is significant at p < 0.05; + - significant diference with Pre.CRE in Placebo at p < 0.05; ± - significant diference with Im.Po.CRE in Placebo at p < 0.05; * - significant diference with Pre.CRE in Jujube at p < 0.05; ** - significant diference with Im.Po.CRE in Jujube at p < 0.05. Error Bars peresent as SE
DISCUSSION
Current data implicate that acute resistance exercise induced an increase of [Ca2+]j, calpain-1, and caspase-3, while XIAP and calpastatin levels decreased. Accordingly, pro-apoptotic molecular signals with involvement of [Ca2+]i-calpastatin-calpain-caspase-3 axis were up-regulated in response to exercise. In contrast, supplementation with Zj attenuated the exercise induced increase of pro-apoptotic signals and increased the levels of anti-apoptotic signals such as XIAP.
In neutrophils the critical balance between cell life and cell death is regulated by the balance between levels of anti-apoptotic andpro-apoptotic proteins levels [14]. Although the neutrophils [Ca2+]j-calpastatin-calpain axis was not investi-
gated during exercise conditions before, it is supposed that the calcium-dependent cysteine pro-teasis calpain is an important mediator of neutrophil apoptosis. During the apoptosis process, cal-pastatin is broken down and calpains cleave the Bax, and deactivate XIAP, thus causing neu-trophil apoptosis [9].
In placebo group, [Ca2+]i levels increased during exercise and recovery. In parallel, anti-apoptotic calpastatin decreased. While calpain-1 and XIAP remained unchanged during exercise, they increased or decreased during recovery, respectively. Caspase-3 increased linearly during exercise and recovery suggesting that intensive Ex affects the balance between pro- and anti-apoptotic proteins in neutrophils to pro-apoptosis.
An increase of neutrophil apoptosis after intensive exercise was found previously after acute exercise; Here, it a change in the oxidative state in neutrophils was documented which resulted in apoptosis [31]. Similarly, our own group found an increase of Annexin-positive neutrophils after intensive resistance exercise [35]. The involvement of ([Ca2+]i) in apoptosis regulation during exercise was previously demonstrated in lymphocytes [22] and neutrophils [23]. Here it was found that exercise affect neutrophils calcium transients followed by a modulation of neutrophils life span. A study showed that incubation with Gra-nulocyte Colony-Stimulating Factor (G-CSF) delayed in vitro neutrophils apoptosis for 12 h and prevented the activation of caspase-3 and -9. Besides it strongly prevented activation of cal-pains (upstream of caspase-3) through control of calcium permeation. Accordingly, it is strongly suggested that [Ca2+]i modulation is involved in apoptosis during exercise with the involvement of calpains. In addition, prevention of Calpain caused stability of XIAP and so activity inhibition of caspase-3 and -9 [38].
The importance of the [Ca2+]i-calpastatin-calpain axis for induction of apoptosis is supported by the contrary effects of Zj supplementation on neutrophils protein expression after exercise. Accordingly, in Zj solution group, increase of [Ca2+]i was inhibited compared to placebo group. In accordance, calpastatin and XIAP increased while a decrease of calpain-1 was found the resulting decrease of caspase-3 in Zj group suggested that supplementation one hour before exercise is able to reverse the exercise induced changes of pro- and anti- apoptotic proteins in human neutrophil. Similarly, glutamine feeding resulted in reduction neutrophils apoptosis induced by exercise; in which assumed that supplementation might have protective effects on mitochondrial integrity [18]. In other study, one session of exercise increased neutrophils' cas-pase-3 gene expression in rats, which was attenuated by supplementation with glutamine [16]. Zj fruit contains high carbohydrates, fat, protein, various amino acids such as three precursor of glutamine and several others [10]. Accordingly, it is suggested that glucose and glutamine are important energy sources of neutrophils during exercise [17], which might be more important than glucose [6]. Thus, Zj supplementation (0.5 gr/kg body weight in 2.5 cc distilled water) might be an important provider of energy for neutrophils which is specifically important
during energy demanding activities like circuit training. In accordance with our data, 30 days of Zj extraction supplementation reduced Bax expression and increased Bcl-2 expression in rats' heart muscle in response to two swimming bouts (15-min) on two days [21].
Besides, Zj contains various minerals and vitamins which have anti-oxidative we properties such as vitamins C, and A. It also contains glyco-side complexes, including phenols (Querectin and Kaemferol) as well as flavonoids and triter-penes [4, 5, 8], which also have anti-oxidative properties. We know that acute exercise with high intensity elevates oxidative stress and tissue damage [31], and intensive resistance training also have a profound effect on in lipid peroxida-tion and production of free radicals through blood ischemia-reperfusion and mechanical loads exerted on the involved soft tissues [1]. The involvement of oxidative mechanisms is likely because it was shown that exercise induced neutro-phil apoptosis is related to an altered oxidative status [31, 35]. In contrast, 3 weeks Zj administration (0.4 gr/kg body weight) improved negative effect of a bout of resistance exercise (5 exercise with 90 % 1RM) on suppression of total antioxidant capacity [2] and glutathione pero-xidase (GPX) [1]. It is found 30 days supplementation with Zj extraction reduced Bax expression and increased Bcl-2 expression in rats' heart muscle accompanied by reduced levels of lipid peroxidation and increase antioxidant enzymes activities [21].
CONCLUSION
In summary, intensive Ex turned protein balance in neutrophils to pro-apoptotic signals. In contrast supplementation with Zj solution an hour before exercise suppressed these responses suggesting that supplementation inhibits cell death. Mechanistically, it is suggested that the [Ca2+]i-Calpastatin-Calpain axis upstream cas-pase-3 is involved in exercise induced apoptosis modulation of neutrophils. The modifying effects of Zj on this pathway might be due the supply of energy or its anti-oxidative capacity. Any clinical effects of Zj on the immune system after exercise remain to be shown in future studies.
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Received 20 June 2020
УДК 796.011.1 й01: 10.14529/Ивт200301
ВЛИЯНИЕ УПОТРЕБЛЕНИЯ ЗИЗИФУСА НАСТОЯЩЕГО НА ПРО- И АНТИАПОПТОТИЧЕСКУЮ ЭКСПРЕССИЮ БЕЛКА В НЕЙТРОФИЛАХ ПОСЛЕ СИЛОВЫХ УПРАЖНЕНИЙ
С.М. Тайеби1, К. Крюгер2, М. Сафакар3, П. Бахрами3, Г. Тахмасб3, А.В. Ненашева4
1 Университет им. Алламе Табатабаи, г. Тегеран, Иран, 2Гисенский Университет им. Юстуса Либиха, г. Гиссен, Германия, 3Исламский Университет Азад в г. Керман, г. Керман, Иран, 4Южно-Уральский государственный университет, г. Челябинск, Россия
Считается, что зизифус способен оказывать положительное воздействие на иммунные расстройства, вызванные физической нагрузкой, в частности, речь идет о регуляции апоп-тоза нейтрофилов, однако ее внутриклеточный механизм все еще остается неизученным. Цель. Цель данного исследования - изучить мгновенный эффект от употребления зизифу-са настоящего на про- и антиапоптотический уровни белка в нейтрофилах человека в ответ на сеанс круговой тренировки. Материалы и методы. Участники завершили круговую тренировку (75 %, 1ПМ, 9 упражнений, 3 подхода). Пока одна группа получала плацебо, другая группа ежедневно употребляла зизифус (0,5 г/кг веса тела в 2,5 см3 дистиллированной воды) за час до тренировки. Результаты. У участников группы, получавшей плацебо, повысился уровень нейтрофилов [Са2+]ъ кальпаина-1 и каспазы-3 (р < 0,05) при одновременном снижении уровня кальпастатина и Х-связанного ингибитора белка апоптоза (р < 0,05). В свою очередь зизифус либо подавлял [Са2+]ъ либо реверсировал ответы на кальпастатин, кальпаин-1, Х-связанный ингибитор белка апоптоза и каспазу-3 (р < 0,01). Заключение. Данные показывают, что один сеанс интенсивной круговой тренировки индуцировал апоптотическую передачу сигналов в нейтрофилах человека с участием оси [Са2+]гкальпастатин-кальпаин, расположенной выше каспазы-3. Однократный прием раствора зизифуса перед тренировкой ослабил эти эффекты, вероятно, за счет обеспечения источников энергии для нейтрофилов или за счет функционирования в качестве антиокси-дантов.
Ключевые слова: добавка зизифуса, силовые упражнения, апоптоз нейтрофилов, ось [Са2+] -кальпастатин-кальпаин, каспаза-3, Х-связанный ингибитор белка апоптоза.
Тайеби Сейед Мортеза, кафедра физиологии упражнений, факультет спортивных наук, Университет им. Алламе Табатабаи, г. Тегеран, Иран. E-mail: tayebism@atu.ac.ir, tayebism@ gmail.com, ORCID: 0000-0003-0459-4443.
Крюгер Карстен, кафедра физиологии упражнений и спортивной терапии, Гисенский Университет им. Юстуса Либиха, г. Гиссен, Германия. E-mail: karsten.krueger@sport.uni-giessen.de, ORCID: 0000-0003-1506-8254.
Сафакар Мехрнуш, кафедра физиологии упражнений, гуманитарный факультет, Исламский университет Азад в г. Керман, г. Керман, Иран. E-mail: safakar.m@yahoo.com. ORCID: 0000-0002-6355-2107.
Бахрами Поуран, кафедра физиологии упражнений, гуманитарный факультет, Исламский университет Азад в г. Керман, г. Керман, Иран. E-mail: bahrami.pouran@yahoo.com. ORCID: 0000-0002-0111-2077.
Тахмасб Гасем, кафедра физиологии упражнений, гуманитарный факультет, Исламский университет Азад в г. Керман, г. Керман, Иран. E-mail: tahmasb.g@yahoo.com. ORCID: 0000-0002-6663-4319.
Ненашева Анна Валерьевна, кафедра теории и методики физической культуры и спорта, кафедра спортивного совершенствования, Институт спорта, туризма и сервиса, Южно-Уральский государственный университет (национальный исследовательский университет). 454080, г. Челябинск, проспект Ленина, 76. E-mail: nenashevaav@susu.ru, ORCID: 0000-0003-0092-2948.
Поступила в редакцию 20 июня 2020 г.
ОБРАЗЕЦ ЦИТИРОВАНИЯ
FOR CITATION
Effects of Ziziphus Jujube Supplementation on Pro-and Anti-Apoptotic Protein Expression in Neutrophils after Resistance Exercise / S.M. Tayebi, K. Krüger, M. Safakar et al. // Человек. Спорт. Медицина. - 2020. - Т. 20, № 3. - С. 5-14. DOI: 10.14529/hsm200301
Tayebi S.M., Krüger K., Safakar M., Bahrami P., Tahmasb G., Nenasheva A.V. Effects of Ziziphus Jujube Supplementation on Pro- and Anti-Apoptotic Protein Expression in Neutrophils after Resistance Exercise. Human. Sport. Medicine, 2020, vol. 20, no. 3, pp. 5-14. DOI: 10.14529/hsm200301
