Introduction

Diabetes mellitus (DM) is a complex metabolic syndrome characterized by hyperglycemia, that increases the risk of microvascular and macrovascular diseases [1]. It is one of the major causes of morbidity and mortality with its complications affecting many people through out the world.

Epidemiological studies have shown that diabetes mellitus is an independent risk factor for cardiovascular diseases. The risk of death due to coronary artery disease is high in diabetic patients compared with non-diabetic patients. Furthermore, the risk of mortality in patients with known diabetes mellitus and who are not clinically diagnosed with coronary artery disease is similar to non-diabetic patients who previously experienced myocardial infarction [2]. Hyperglycemia directly causes endothelial dysfunction and is frequently associated with cardiovascular diseases [3, 4]. The development of atherosclerosis occurs at an earlier age in diabetic patients and rapidly progresses [5].

It is known that myocardial cells lack the ability to regenerate or have very little regeneration capacity. However, regenerative cells have been detected in the myocardium and have given rise to the idea that these cells may be manipulated. Stem cells, which are the building blocks of all living subjects, rest in different regions of the tissues. They are programmed to increase tissue regeneration, especially in the case of tissue loss or damage [6].

Although studies have shown that stem cells reduce cardiac damage caused by ischemia [68], the most important limiting factor in these studies is that a determined methodology has not been established. It has been shown that angiographic methods or intraoperative injected stem cells after myocardial infarction reduced ischemic cardiac damage and affect myocardial functions positively [9, 10]. Erythropoietin is a glycoprotein molecule which is synthesized in the case of hypoxia. In preclinical studies, it has been reported that the erythropoietin molecule has significant tissue protective effects with mechanisms such as apoptosis inhibition, vascular restoration, reduction of inflammatory response and increased tissue function in cardiac, neuronal, retinal and renal ischemic injury models [11, 12]. Recent studies have shown that erythropoietin (EPO) has tissue-protecting effects in the heart by increasing vascular endothelial growth factor (VEGF) expression and alleviating myocardial fibrosis in ischemia models [13].

Many studies using stem cells have ignored diabetic patients and usually the effects of diabetes mellitus on endothelial and coronary arteries have been mostly emphasized [14, 15]. In this study, we aimed to evaluate the effects of erythropoietin on stem cell synthesis and tissue regeneration in the context of damaged tissues.

Material and methods

Research plan

The study was carried out at the Istanbul University Experimental Medicine and Research Institute. Histopathological examinations were performed at Istanbul University Cerrahpasa Veterinary Faculty, Department of Pathology and biochemical investigations were performed at Istanbul University Medical Faculty. The necessary approval was obtained from the Experimental Medicine Ethics Committee of the Experimental Medicine and Research Institute of Istanbul University (Ethics Committee no: 27/2018).

In the study 25 adult Sprague Dawley rats (approximately 3 months) fed with normal food at a suitable weight of 350-400 g were used. The rats were divided into three groups as the control group (group 1), diabetic group (group 2) and erythropoietin-induced diabetic group (group 3).

Measurement methods

In all rats, blood glucose levels were measured in a drop blood taken from the tail vein after 6 h of fasting before the experiment and rats with a blood glucose level ≥ 110 mg/dl were not included in the study. Additionally, mean basal blood glucose level was determined. A MediSense Precision Q.I.D glucometer and MediSense Sensor Electrodes (Abbott Laboratories Warszawa, Poland) were used for blood glucose measurement. In group 2 and group 3 rats, following the anesthesia achieved by 40 mg/kg sodium pentothal, intraperitoneal 50 mg/kg streptozocin (STZ) was given and irreversible pancreatic damage was induced. Following the second day of streptozocin administration, blood drops taken from the tail vein after 6 h of fasting were measured, and blood glucose levels were higher than 300 mg/dl in all rats.

The rats were kept alive for 1 month in order to observe the possible cardiovascular complications of diabetes. Blood glucose re-measurements were not required, and clinical findings of diabetes such as polyuria and polydipsia were monitored. During the follow-up period, 2 rats died in the diabetes group probably due to the side effects of diabetes mellitus.

In group 3, stem cell synthesis was induced by administering 3000 U/kg erythropoietin 2 times intraperitoneally on the 24th and 27th days before rats were sacrificed.

At the end of 1 month, rats in all groups were euthanized with high dose anesthesia (90 mg/kg pentothal) and blood was drawn. In order to evaluate the stem cell levels, blood samples were obtained from the rats and the heart was removed en bloc for adequate sampling of the right atrium, right ventricle, left atrium and left ventricular tissues (Figure 1).

Figure 1

En bloc cardiac tissue

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Tissue fibrosis, CD34 and VEGF level measurement

Heart tissues were fixed in 10% formalin. Right atrium, right ventricle, left atrium and left ventricular biopsies were taken from each heart tissue after fixation. In the pathology laboratory, the specimen block was prepared following alcohol, xylene and paraffin applications on the tissues. By using an automatic microtome, 4 micron thick sections were taken from each of the paraffin-embedded tissues; and hematoxylin-eosin, mason trichrome staining and immunohistochemical studies were performed with appropriate methods and suitable antigens according to the manufacturers’ protocols, which were previously explained in detail in many studies in the literature.

The results were evaluated for each category from 0 to 3: 0 – no staining, 1 – poor staining (10% staining), 2 – moderate staining (10–50% staining), 3 – severe staining (more than 50% staining).

Statistical analysis

Statistical analysis was performed using the SPSS (SPSS for Windows, SPSS Inc, Chicago, IL, US) 15.0 program package. Variables were expressed as mean ± standard deviation. Non-parametric methods were used in the statistical evaluation of the data. Kruskal-Wallis variance analysis was used to evaluate the difference between the groups. The Mann-Whitney U test with Bonferroni correction was used for determination of the difference between groups. Correlation analysis of the data was performed by Spearman rank correlation analysis. A p-value of less than 0.05 was considered statistically significant.

Results

The mean blood glucose level was measured before the experiment in all rats and found to be 72.80 ±11.516 mg/dl. After the administration of streptozocin, mean blood glucose level was 358.70 ±44.749 mg/dl on the 2nd day and 382.80 ±34.941 mg/dl at the end of the 1st week. According to the Spearman rank correlation analysis, the rho values were evaluated as follows: 0.00–0.24: poor correlation, 0.25–0.49: moderate correlation, 0.50–0.74: strong correlation, 0.75–1.00: very strong correlation.

The increase in blood sugar resulted in a statistically significant decrease in reticulocyte levels in group 2 and a statistically significant increase in tissue levels of CD34 and VEGF in group 2 and group 3. There was a strong positive and statistically significant correlation only between right atrium CD34 levels and serum reticulocyte levels (rho = 0.701, p = 0.024); however, such a correlation was not observed for the left atrium, left ventricle and right ventricle, unexpectedly.

In the control group, diabetic group and erythropoietin-induced diabetic group, the difference in right atrium, right ventricle, left atrium and left ventricular fibrosis was found to be strongly significant when comparing the groups with each other. According to the results of the analysis, the differences between the fibrosis levels of the 3 groups in the right atrial tissue were significant (χ2K-W = 8.858, SD = 2, p = 0.012). No significant difference was found between group 1 and group 3, and group 2 and group 3. There was a significant difference between group 1 and group 2 (Table I). This significant difference was proved to be due to less fibrosis in group 1.

Table I

Statistical analysis of fibrosis, CD34 and VEGF levels in right atrium of control, diabetic and diabetic rats induced with erythropoietin. A – Descriptive statistics, B – Kruskal-Wallis test, test statistics, C – Mann-Whitney 1&2 test, D – Mann-Whitney 2&3 test, E – Mann-Whitney 1&3 test

A
GroupParameterNMinimumMaximumMeanStd. deviation
ControlReticulocyte%51.201.491.33000.11790
Glucose57710090.0010.700
CD345121.200.447
VEGF5121.200.447
Fibrosis5121.200.447
Valid N (listwise)5
DiabeticReticulocyte%81.302.801.92500.53918
Glucose8270494397.5071.841
CD348131.620.744
VEGF8131.880.641
Fibrosis8132.500.756
Valid N (listwise)8
ErythropoietinReticulocyte%1012.0028.0020.90005.70477
Glucose10350450410.7031.609
CD3410232.800.422
VEGF10232.700.483
Fibrosis10132.100.568
Valid N (listwise)10
B
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
χ218.31911.26713.89212.7278.858
df22222
Asymp. sig.0.0000.0040.0010.0020.012

[i] Kruskal-Wallis test, grouping variable: group.

C
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U3.0000.00013.5008.5004.000
Wilcoxon W18.00015.00028.50023.50019.000
Z–2.492–2.928–1.105–1.873–2.498
Asymp. sig. (2-tailed)0.0130.0030.2690.0610.012
ExactSig. [2*(1-tailed sig.)]0.011a0.002a0.354a0.093a0.019a

a Not corrected for ties.

D
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U0.00038.5009.00014.00025.500
Wilcoxon W36.00074.50045.00050.00080.500
Z–3.560–.133–2.996–2.542–1.425
Asymp. sig. (2-tailed)0.0000.8940.0030.0110.154
ExactSig. [2*(1-tailed Sig.)]0.000a0.897a0.004a0.021a0.203a

a Not corrected for ties.

E
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U0.00038.5009.00014.00025.500
Wilcoxon W36.00074.50045.00050.00080.500
Z–3.560–.133–2.996–2.542–1.425
Asymp. sig. (2-tailed)0.0000.8940.0030.0110.154
ExactSig. [2*(1-tailed Sig.)]0.000a0.897a0.004a0.021a0.203a

a Not corrected for ties.

The difference between the fibrosis levels of the 3 groups in the right ventricular tissue (χ2K-W = 13.200, SD = 2, p = 0.001), left atrial tissues(χ2K-W = 14.883, SD = 2, p = 0.001) and left ventricular tissues (χ2K-W = 13.520, SD = 2, p = 0.001) were statistically significant. The differences between group 1 and group 2, and group 2 and group 3 were significant while the difference between group 1 and group 3 was not significant (Tables IIIV). This difference was attributed to increased fibrosis in group 2 (Figure 2) and minimal fibrosis in group 1 and attenuated fibrosis in group 3 with erythropoietin injection.

Table II

Statistical analysis of fibrosis, CD34 and VEGF levels in right ventricle of control, diabetic and diabetic rats induced with erythropoietin. A – Descriptive statistics, B – Kruskal-Wallis test, test statistics, C – Mann-Whitney 1&2 test, D – Mann-Whitney 1&3 test, E – Mann-Whitney 2&3 test

A
GroupParameterNMinimumMaximumMeanStd. deviation
ControlReticulocyte%51.201.491.33000.11790
Glucose57710090.0010.700
CD345121.400.548
VEGF5121.200.447
Fibrosis5111.000.000
Valid N (listwise)5
DiabeticReticulocyte%81.302.801.92500.53918
Glucose8270494397.5071.841
CD348131.880.835
VEGF8132.000.756
Fibrosis8232.750.463
Valid N (listwise)8
ErythropoietinReticulocyte%1012.0028.0020.90005.70477
Glucose10350450410.7031.609
CD3410132.600.699
VEGF10232.600.516
Fibrosis10131.900.738
Valid N (listwise)10
B
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
χ218.31911.2677.57310.29413.200
df22222
Asymp. sig.0.0000.0040.0230.0060.001
C
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U3.0000.00013.5008.0000.000
Wilcoxon W18.00015.00028.50023.00015.000
Z–2.492–2.928–1.034–1.910–3.183
Asymp. sig. (2-tailed)0.0130.0030.3010.0560.001
ExactSig. [2*(1-tailed sig.)]0.011a0.002a0.354a0.093a0.002a

a Not corrected for ties.

D
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U0.0000.0005.5002.0007.500
Wilcoxon W15.00015.00020.50017.00022.500
Z–3.067–3.062–2.569–2.996–2.378
Asymp. sig. (2-tailed)0.0020.0020.0100.0030.017
ExactSig. [2*(1-tailed sig.)]0.001a0.001a0.013a0.003a0.028a

a Not corrected for ties.

E
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U0.00038.50020.50022.00015.000
Wilcoxon W36.00074.50056.50058.00070.000
Z–3.560–0.133–1.885–1.760–2.407
Asymp. sig. (2-tailed)0.0000.8940.0590.0780.016
ExactSig. [2*(1-tailed sig.)]0.000a0.897a0.083a0.122a0.027a

a Not corrected for ties.

Table III

Statistical analysis of fibrosis, CD34 and VEGF levels in left atrium of control, diabetic and diabetic rats induced with erythropoietin. A – Descriptive statistics, B – Kruskal-Wallis test, test statistics, C – Mann-Whitney 1&2 test, D – Mann-Whitney 1&3 test, E – Mann-Whitney 2&3 test

A
GroupParameterNMinimumMaximumMeanStd. deviation
ControlReticulocyte%51.201.491.33000.11790
Glucose57710090.0010.700
CD345121.400.548
VEGF5121.200.447
Fibrosis5121.200.447
Valid N (listwise)5
DiabeticReticulocyte%81.302.801.92500.53918
Glucose8270494397.5071.841
CD348131.880.835
VEGF8121.750.463
Fibrosis8232.870.354
Valid N (listwise)8
ErythropoietinReticulocyte%1012.0028.0020.90005.70477
Glucose10350450410.7031.609
CD3410232.800.422
VEGF10232.800.422
Fibrosis10131.900.568
Valid N (listwise)10
B
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
χ218.31911.26711.13015.96114.883
df22222
Asymp. sig.0.0000.0040.0040.0000.001
C
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U3.0000.00013.5009.0000.500
Wilcoxon W18.00015.00028.50024.00015.500
Z–2.492–2.928–1.034–1.859–3.160
Asymp. sig. (2-tailed)0.0130.0030.3010.0630.002
ExactSig. [2*(1-tailed sig.)]0.011a0.002a0.354a0.127a0.002a

a Not corrected for ties.

D
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U0.0000.0002.0001.0009.500
Wilcoxon W15.00015.00017.00016.00024.500
Z–3.067–3.062–3.101–3.236–2.139
Asymp. sig. (2-tailed)0.0020.0020.0020.0010.032
ExactSig. [2*(1-tailed sig.)]0.001a0.001a0.003a0.001a0.055a

a Not corrected for ties.

E
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U0.00038.50015.0006.0008.000
Wilcoxon W36.00074.50051.00042.00063.000
Z–3.560–0.133–2.476–3.325–3.129
Asymp. sig. (2-tailed)0.0000.8940.0130.0010.002
ExactSig. [2*(1-tailed sig.)]0.000a0.897a0.027a0.001a0.003a

a Not corrected for ties.

Table IV

Statistical analysis of fibrosis, CD34 and VEGF levels in left ventricle of control, diabetic and diabetic rats induced with erythropoietin. A – Descriptive statistics, B – Kruskal-Wallis test, test statistics, C – Mann-Whitney 1&2 test, D – Mann-Whitney 1&3 test, E – Mann-Whitney 2&3 test

A
GroupParameterNMinimumMaximumMeanStd. deviation
ControlReticulocyte%51.201.491.33000.11790
Glucose57710090.0010.700
CD345121.400.548
VEGF5121.200.447
Fibrosis5121.200.447
Valid N (listwise)5
DiabeticReticulocyte%81.302.801.92500.53918
Glucose8270494397.5071.841
CD348132.000.756
VEGF8121.750.463
Fibrosis8232.870.354
Valid N (listwise)8
ErythropoietinReticulocyte%1012.0028.0020.90005.70477
Glucose10350450410.7031.609
CD3410232.700.483
VEGF10232.700.483
Fibrosis10132.000.667
Valid N (listwise)10
B
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
χ218.31911.2679.85514.56113.520
df22222
Asymp. sig.0.0000.0040.0070.0010.001
C
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U3.0000.00011.0009.0000.500
Wilcoxon W18.00015.00026.00024.00015.500
Z–2.492–2.928–1.432–1.859–3.160
Asymp. sig. (2-tailed)0.0130.0030.1520.0630.002
ExactSig. [2*(1-tailed sig.)]0.011a0.002a0.222a0.127a0.002a

a Not corrected for ties.

D
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U0.0000.0003.0001.5009.000
Wilcoxon W15.00015.00018.00016.50024.000
Z–3.067–3.062–2.910–3.096–2.144
Asymp. sig. (2-tailed)0.0020.0020.0040.0020.032
ExactSig. [2*(1-tailed sig.)]0.001a0.001a0.005a0.001a0.055a

a Not corrected for ties.

E
ParameterReticulocyte%GlucoseCD34VEGFFibrosis
Mann-Whitney U0.00038.50019.0009.00012.000
Wilcoxon W36.00074.50055.00045.00067.000
Z–3.560–0.133–2.064–3.047–2.752
Asymp. sig. (2-tailed)0.0000.8940.0390.0020.006
ExactSig. [2*(1-tailed sig.)]0.000a0.897a0.068a0.004a0.012a

a Not corrected for ties.

Figure 2

Thin fibrillary connective tissue formation in necrotic tissue by Masson trichrome staining in diabetic group

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When the right atrial, right ventricular, left atrial and left ventricular CD34 were compared between the control group, diabetic group and erythropoietin-induced diabetic group, the difference was found to be highly significant. According to the results of the analysis, the differences between the CD34 levels of the 3 groups in the right atrial tissue (χ2K-W = 13.892, SD = 2, p = 0.001) and left atrial tissue (χ2K-W = 11.130, SD = 2, p = 0.004) were statistically significant. There was a significant difference between group 1 and group 3, and group 2 and group 3. No significant difference was found between group 1 and group 2 (Tables I, III). The differences between the CD34 levels of the 3 groups in the right ventricular tissue (χ2K-W = 7.573, SD = 2, p = 0.023) and left ventricular tissue (χ2K-W = 9.855, SD = 2, p = 0.007) were statistically significant. A significant difference was found between group 1 and group 3, and no significant difference was found between group 1 and group 2, and group 2 and group 3 (Tables II, IV). The significant differences between the CD34 levels of different tissues were proven to be due to the high amount of CD34 in group 3 (Figure 3).

Figure 3

Increased tissue stain with CD34

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When the right atrium, right ventricle, left atrium and left ventricular VEGF levels were compared in the control group, diabetic group and erythropoietin induced diabetic group, the difference was found to be highly significant. According to the results of the analysis, the difference between the VEGF levels of the 3 groups in the right atrial tissue (χ2K-W = 12.727, SD = 2, p = 0.002), and left atrial tissue (χ2K-W = 15.961, SD = 2, p < 0.001) was statistically significant. There was significant difference between group 1 and group 3 and group 2 and group 3, and no significant difference was found between group 1 and group 2 (Tables I, III, IV). The differences between the VEGF levels of the 3 groups in the right ventricular tissue (χ2K-W = 10.294, SD = 2, p = 0.006) and left ventricular tissue (χ2K-W = 14.561, SD = 2, p = 0.001) were statistically significant. There was a statistically significant difference between group 1 and group 3, and no significant difference was found between group 1 and group 2, and group 2 and group 3 (Table II). This significant difference was proved to be due to the high amount of VEGF in group 3 (Figure 4).

Figure 4

Increased tissue stain with VEGF

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Discussion

In developed western countries, at least half of all deaths are due to cardiovascular diseases and 3/4 of them are related to atherosclerotic coronary artery disease (CAD). It is one of the leading causes of morbidity and mortality [16]. Diabetes mellitus is defined as a complex metabolic syndrome characterized by hyperglycemia, which increases the risk of microvascular and macrovascular disease [1]. Diabetes was closely associated with other risk factors and due to high mortality (4–6 times) rates in the case of myocardial infarction, it was accepted as a risk equivalent of CAD [4].

Studies on stem cells also attract attention in the field of cardiac surgery. In order to help tissue regeneration in stress conditions such as ischemia, hyperthermia and hypothermia, these cells, which increase in number, may also serve in the defense mechanisms when needed in various stress situations [17, 18]. Studies have shown that stem cells may reduce cardiac damage caused by ischemia [7, 8].

Erythropoietin is a glycoprotein hormone that is induced by hypoxia that stimulates the proliferation and differentiation of erythroid precursor cells to eliminate the reduced levels of oxygen caused by anemia and hypoxia. Several studies have shown that EPO can induce proliferation cascades in the myocardium [12]. Thus, the idea that EPO may be used as a cytoprotective agent in the cardiovascular system has been born [19, 20]. EPO may also trigger neovascularization, reduce infarct size and provide effective cardiac protection against ischemia-reperfusion injury and chronic heart failure. Erythropoietin protects the myocardium from ischemic injury and promotes re-modeling [11].

Diabetic cardiomyopathy (DCM) is characterized by microvascular pathology and interstitial fibrosis leading to progressive heart failure. Diabetic microvascular complications are thought to be affected by angiogenic factors, including VEGF, in response to both ischemia and hyperglycemia. Hyperglycemia also causes interstitial fibrosis and progressive cardiac dysfunction along with apoptosis and necrosis of cardiomyocytes [18, 20]. In a study with EPO in DCM-induced rats, it was found that EPO administration can reverse the reshaping of the heart by increasing angiogenesis and weakening interstitial fibrosis without affecting blood sugar [18]. Erythropoietin has been shown to have tissue-protective effects in the heart by increasing VEGF expression and alleviating myocardial fibrosis in ischemia models [19].

Many studies using stem cells have ignored diabetic patients. However, we know that diabetes is a risk factor for many postoperative morbidities which are thought to be caused by differences in stem cell level [14, 15]. Streptozocin is a pancreatic beta cell toxin that disrupts the ability to produce insulin in animals and has led to the development of the model of diabetic atherosclerosis. This model was first described by Park and resulted in a 5.3-fold plaque increase in the aortic sinus compared to the control group after 6-week follow-up in mice with diabetes induced by streptozocin [21]. Thus, diabetic atherosclerosis, which develops plaque morphology in a similar way to human beings, was created in the animal model and it allowed animal experiments in diabetic models.

In this study, we aimed to investigate the effects of diabetes on the direct cardiovascular system tissues and the effect of erythropoietin, which is known to increase stem cells in diabetic rats. In the literature, it is seen that VEGF levels are investigated most frequently and safely in order to evaluate the neovascularization histopathologically [19]. In addition, CD34 is a marker that is bound to the surface of stem cells. In the literature, CD34 is frequently and safely evaluated in identifying stem cells [11]. VEGF and CD34 antibodies were used as markers in this study where tissue regeneration was investigated in the diabetic population using erythropoietin. Thus, the role of erythropoietin in stem cell synthesis and tissue regeneration in the context of damaged tissues was evaluated. In our study, reticulocytes and serum levels of CD34 and VEGF in different tissues of the cardiovascular system were evaluated in the diabetic model of rats for the first time in the literature.

In diabetic rats, CD34 and VEGF levels were higher in cardiovascular system tissues compared to healthy rats. The administration of erythropoietin, which is known to increase the amount of stem cells and endothelial growth factor, led to a larger increase in tissue levels of CD34 and VEGF in diabetic rats. Another remarkable finding is that although there was an increase in CD34 and VEGF levels and larger fibrosis reduction in the presence of erythropoietin in diabetics, it did not significantly correlate with reticulocyte levels, fibrosis, CD34 and VEGF levels except right atrial tissue. The current situation was thought to be related to the low number of subjects in the groups. A significant correlation was observed only in serum reticulocyte level and right atrium CD34 level.

The major limitation of our study is the low number of subjects. Also, we failed to detect a correlation between reticulocyte levels, CD34 and VEGF levels in different tissues of the heart other than the right atrium. Although the results indicated higher levels of CD34 and VEGF in erythropoietin induced diabetic rats, the provocative mechanism of erythropoietin to induce stem cells other than reticulocytes could not be clearly identified in this study.

In conclusion, the amount of CD34 and VEGF for tissue regeneration increases in the case of fibrotic insult in the cardiovascular system in rats. Tissue levels of CD34 and VEGF molecules that are involved in cellular protection and regeneration may be further enhanced by the safe use of erythropoietin in the diabetic rat population.