BASIC RESEARCH

Low-Dose Growth Hormone is Cardioprotective in Uremia

Ralph Rabkin, Ibrahim Awwad, Yu Chen, Euan A. Ashley, Difei Sun, Sumita Sood, William Clusin, Paul Heidenreich, Grzegorz Piecha and Marie-Luise Gross
JASN September 2008, 19 (9) 1774-1783; DOI: https://doi.org/10.1681/ASN.2007121386

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Abstract

Growth hormone (GH) is required to maintain normal cardiac structure and function and has a positive effect on cardiac remodeling in experimental and possibly human disease. Cardiac resistance to GH develops in the uremic state, perhaps predisposing to the characteristic cardiomyopathy associated with uremia. It was hypothesized that administration of low-dosage GH may have a salutary effect on the cardiac remodeling process in uremia, but because high levels of GH have adverse cardiac effects, administration of high-dosage GH may worsen uremic cardiomyopathy. In rats with chronic renal failure, quantitative cardiac morphology revealed a decrease in total capillary length and capillary length density and an increase in mean intercapillary distance and fibroblast volume density evident. Low-dosage GH prevented these changes. Collagen and TGF-β immunostaining, increased in chronic renal failure, were also reduced by GH, suggesting a mechanism for its salutary action. Low-dosage GH also prevented thickening of the carotid artery but did not affect aortic pathology. In contrast, high-dosage GH worsened several of these variables. These results suggest that low-dosage GH may benefit the heart and possibly the carotid arteries in chronic renal failure.

Cardiovascular disease (CVD) is the most common cause of death in adults with advanced chronic renal failure (CRF)13 and also is of concern in children.4 In ESRD, CVD may present as a cardiomyopathy with left ventricular (LV) hypertrophy or dilation or as ischemic heart disease often culminating in congestive heart failure (CHF). Also of concern is decreased tolerance to myocardial ischemia with reduced long-term survival after a myocardial infarct.5,6 In addition to the usual forms of heart disease, a characteristic cardiomyopathy develops in uremia.79 Features include LV hypertrophy, interstitial expansion with fibrosis, and reduced capillary length density, abnormalities that contribute to the increased susceptibility to ischemic injury. These features are reproduced in uremic rats.10,11 Uremia also seems to alter cardiac function directly, impairing myocyte relaxation and calcium handling.12

Maintenance of cardiac structure and function depends on the interplay of several growth factors and hormones, among which growth hormone (GH) is essential.13,14 In GH deficiency, cardiac size diminishes, there is endothelial dysfunction15 and stiffness of large arteries, and death from CVD increases.16 In contrast, when GH levels are persistently elevated as in acromegaly, the heart enlarges, interstitial fibrosis develops, and cardiac performance falls.13,14 These manifestations of GH deficiency or excess can be reversed with correction of the abnormal GH state.1719 Interestingly, there is evidence that GH may have a favorable effect on cardiac remodeling and cardiac output in pituitary intact animals and possibly humans with cardiac disease.14,20,21

In advanced CRF, resistance to GH develops, and this is a cause of growth retardation in children and muscle wasting in adults.2224 Fortunately treatment with GH can overcome the resistant state. In animals, we established that GH resistance arises, in part, because of a defect in GH-mediated JAK-STAT5 signaling.23,25,26 This pathway is used by GH to increase production of IGF-1 that in turn mediates most but not all of GH's actions.27,28 It is thus difficult to separate the actions of these two hormones on cardiac structure and function, although it seems that the hemodynamic response to GH is largely mediated through IGF1.13,29,30

Because GH is required for maintenance of cardiac structure and function and may positively affect cardiac remodeling, we postulate that the cardiac resistance to GH that develops in CRF (26) may predispose to the remodeling characteristic of uremia, and, hence, that GH in low dosages (LD) will have a salutary effect on the remodeling process. Conversely, because high GH levels have adverse cardiac effects, we postulated that high-dosage (HD) GH therapy may well worsen uremic cardiomyopathy. To test this thesis, we studied the impact of LD, intermediate-dosage (ID), and HD GH treatment on the cardiac changes in chronically uremic rats.

RESULTS

Study 1: Cardiac Morphometrics

Body Weight and Serum Biochemistry.

Serum creatinine and urea nitrogen levels were elevated in the five-sixths-nephrectomized rats and were not altered significantly by GH treatment. Although body weight was similar before nephrectomy (approximately 245 g), after 10 wk, CRF vehicle (V)-treated rats weighed less than the sham-operated (SO)-V controls (409 ± 21 versus 508 ± 35g; P < 0.05); however, after 6 weeks of GH, body weight increased in the CRF groups, and net weight gained was comparable to control SO-V group gain (66 ± 15 g) and greater than the gain in the CRF-V group (15 ± 7 g; P < 0.05), confirming the bioefficacy of the administered GH. On average, the HD group gained most weight, but this did not reach statistical significance. Serum C-reactive protein (CRP) levels were similar in the SO-V–and CRF-V–treated rats but increased significantly in all of the GH-treated CRF groups, likely reflecting the immunoregulatory properties of GH (Table 1).31

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Table 1.

Body weight and serum biochemistry in study 1a

BP and Heart Weight.

Systolic BP was elevated in CRF rats versus SO-V controls (149 ± 16 versus 120 ± 5 mmHg; P < 0.05) and was unaltered by GH. Heart and LV weight corrected for body weight increased significantly in CRF rats, and these parameters were not altered by GH (Table 2).

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Table 2.

BP and heart weight in study 1a

Quantitative Cardiac Morphology.

Capillary length density was reduced significantly in CRF. Of note, GH at an LD, 1.5 mg/kg, prevented this decrease. In contrast, when given at an ID or HD, 4 or 10 mg/kg, GH had no protective effect. Mean intercapillary distance increased significantly in CRF, and, again, LD had a salutary effect preventing this increase. ID GH had no protective effect, whereas HD GH increased the intercapillary distance significantly. Total capillary length was reduced in CRF, and this decline was prevented by LD and ID GH (P < 0.05). Capillary volume density, nonvascular interstitial tissue volume density, and myocyte volume density were not altered in CRF and did not change with GH therapy. In contrast, fibroblast volume density (FVv) increased significantly in CRF: LD GH prevented this but when given in greater dosages had no effect. These findings (Figure 1) indicate that LD GH has a salutary effect on cardiac disease in CRF. LD GH prevented the decrease in capillary length density and total capillary length and blocked the increase in mean capillary distance and fibroblast volume density. In contrast, HD GH seemed to be ineffective and may even have an adverse effect, because it caused an increase in intercapillary distance (Table 3).

Figure 1.
Figure 1.

Summary of key morphologic changes in the uremic heart and response to GH treatment. After 10 wk of chronic uremia, rats were treated with V (group 2) or GH, 1.5 (group 3), 4 (group 4), and 10 mg/kg per d (group 5) for 6 wk; SO rats served as controls (group 1). The numbers above each bar refer to groups with values that differ significantly from the group value below (P < 0.05). Results are expressed as a percentage of the control group values (mean ± SD). CLv, capillary length density; MID, mean intercapillary distance; TCL, total capillary length; FVv, fibroblast volume density.

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Table 3.

Cardiac capillary morphometrics in study 1a

Quantitative Morphology of the Arteries.

Ascending aorta wall thickness was increased significantly in CRF rats, whereas lumenal diameter was unchanged (Table 4). Accordingly wall thickness/lumen diameter ratio was increased in CRF; all of these parameters were unaffected by GH. Similar results were obtained for wall area/lumen area ratio. Carotid artery wall thickness and wall lumen ratio were significantly increased in CRF and reduced to control values with LD GH (Table 5). Intramyocardial artery wall thickness increased on average in CRF but did not reach statistical significance (Table 6). Of note, wall thickness increased significantly in the HD GH group (P < 0.05).

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Table 4.

Aorta morphometrics in study 1a

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Table 5.

Carotid artery morphometrics in study 1a

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Table 6.

Morphometrics of small intramyocardial arteries in study 1a

Study 2: Hemodynamics and Gene and Protein Expression

Body Weight, Biochemistry, and Hematocrit.

As in study 1, net weight gain was reduced in the CRF-V compared with SO-V group (30 ± 20 versus 48 ± 18 g/6 wk; P < 0.05). GH treatment, 1.5 mg/kg per d, stimulated a similar increase in weight in CRF and SO groups (84 ± 18 versus 96 ± 20 g). Serum creatinine and urea nitrogen were elevated in CRF rats, and the creatinine level was considerably higher than in study 1. Urinary albumin excretion (albumin/creatinine ratio) was increased, whereas hematocrit levels were reduced in CRF. None of these parameters were affected by GH (Table 7).

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Table 7.

Body weight, serum biochemistry, and BP in study 2a

Cardiac Gene Expression.

There was a small but NS increase in IGF-1 mRNA level in the GH-treated rats. Atrial natriuretic factor mRNA levels increased two-fold in CRF-V rats (P < 0.05) and rose further with GH, although not statistically significantly. Collagen type I and collagen type III mRNA were unaffected by CRF but increased in the SO and CRF GH-treated groups. α-Smooth muscle actin (α-SMA), TGF-β, and GH receptor mRNA levels did not differ between groups (Table 8).

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Table 8.

Relative mRNA levels (specific mRNA/18s RNA) in study 2a

Immunohistochemistry.

Immunohistochemistry revealed a significant increase in collagen type I in CRF-V rats; GH attenuated (P < 0.05) but did not normalize the overexpressed protein in CRF-GH rats (Figure 2). Collagen type IV expression increased significantly in CRF-V rats, and GH reduced the levels to a value that did not differ from the SO-GH rats. TGF-β protein was barely detectable in the SO-V or SO-GH groups but increased significantly in the CRF-V group (Figure 3). GH significantly reduced TGF-β protein expression, which fell to values that did not differ from SO values. Vascular endothelial growth factor expression increased significantly in CRF-V and was not reduced significantly by GH.

Figure 2.
Figure 2.

Immunohistochemistry score. Semiquantitative analysis of the effect of uremia and GH treatment on proteins involved in cardiac remodeling. After 10 wk of chronic uremia, rats were treated with V (group 3) or LD GH (group 4), 1.5 mg/kg, for 6 wk; SO rats treated in the same manner with V (group 1) or GH (group 2) served as controls. Results are expressed as a percentage of the control group values (mean ± SD). The numbers above each bar refer to groups with values that differ significantly from the group value below (P < 0.05, ANOVA or Kruskal-Wallis test).

Figure 3.
Figure 3.

Representative figure shows TGF-β immunohistochemistry. TGF-β immunostaining was markedly increased in CRF heart (CRF-V) compared with control (SHAM-V). GH treatment reduced TGF-β overexpression significantly in CRF (CRF-GH).

Hemodynamics.

Echocardiography findings are shown in Table 9. There was a significant increase in LV mass in CRF that did not change with GH. Values for interventricular septal thickness and posterior wall thickness revealed a concentric hypertrophy consistent with a response to the hypertension in these animals. CRF animals also demonstrated a smaller LV cavity and increased fractional shortening and ejection fraction. Although GH did not change fractional shortening in the SO group, it did increase fractional shortening in CRF animals. In addition, cavity size was modestly increased with GH, although this did not reach statistical significance.

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Table 9.

Echocardiography parameters in study 2a

DISCUSSION

The pathogenesis of uremic cardiomyopathy is poorly understood and is under intense investigation. An important area of focus has been the impact of increased levels of circulating factors, including vasoactive hormones, inflammatory cytokines, and cardiac glycosides.1,4,32 Less well studied is the impact of uremia-induced resistance to hormones essential for normal cardiac structure and function, such as GH and IGF-1.26,33 Accordingly, we tested the hypothesis that GH resistance in uremia predisposes to the development of a cardiomyopathy and that administration of GH in low dosages is sufficient to overcome the resistance will have a salutary effect on the remodeling process. Conversely, because high GH levels adversely affect the heart,13,14 we proposed that HD GH may worsen the cardiomyopathy.

To test this thesis, we studied the impact of 6 wk of LD, ID, or HD recombinant bovine GH on the cardiac changes that develop during 4 mo of CRF in rats. GH increased body weight of the growth-retarded CRF rats, indicating that the dosages administered were sufficient to overcome resistance to the hormone and any antibodies that might have formed in response to the exogenous GH.34 Serum CRP levels were not elevated in the V-treated CRF rats but rose significantly with GH treatment. This was unanticipated, because GH is without effect on CRP levels in patients with ESRD,35 and GH replacement in GH-deficient humans lowers CRP levels.36 Conversely, GH does stimulate cytokine production in human monocytes37 and in liver of endotoxin-treated rat.38; therefore, further study in humans with ESRD is indicated. Whereas GH had no impact on serum creatinine, urea nitrogen, albuminuria, or elevated BP levels in the CRF rats, it had a notable impact on cardiac morphology. At an LD, GH prevented the decrease in capillary length density evident in the untreated CRF rats, whereas at higher dosages GH had no protective effect. LD GH also had a beneficial effect on mean intercapillary distance, preventing the CRF-induced increase, whereas HD GH caused an even greater increase in intercapillary distance. Total capillary length was reduced in CRF, and this was prevented by LD and ID GH treatment and is consistent with the reported ability of GH to stimulate cardiac capillary growth.39 Capillary volume density, nonvascular interstitial tissue volume density, and myocyte volume density were not altered in CRF and did not change with GH. In contrast, fibroblast volume density increased significantly in CRF, and LD GH prevented this increase. When given in higher dosages GH had no protective effect. The development of CRF was associated with a significant increase in aorta and carotid artery wall thickness. Although LD GH had no impact on aortic pathology, it did prevent carotid artery thickening. There was a modest but not statistically significant increase in intramyocardial artery wall thickness in CRF, and this was worsened by administration of GH in high dosages. Together, these results indicate that treatment with an LD GH regimen has a salutary effect on the course of the cardiac and possibly carotid artery disease of CRF, whereas HD treatment may have an adverse effect. Extrapolating these findings, it is conceivable that the protection against uremia-induced cardiac microcirculatory disease afforded by LD GH therapy may reduce the susceptibility to ischemic events in CRF.

Immunohistochemistry revealed a significant increase in cardiac collagen types I and IV in CRF. GH reduced but did not normalize the overexpressed type I collagen, whereas there was a tendency for type IV collagen expression to be reduced. Consistent with our findings, Grimm et al.40 noted that GH reduced the accumulation of type I collagen that followed a myocardial infarct in rats. We found that cardiac TGF-β protein was barely detectable in the SO-V or SO-GH groups but increased significantly in CRF. LD GH reduced TGF-β protein expression to values similar to normal control values. This suggests that the beneficial effect of GH may be mediated partly by suppression of TGF-β protein levels. In this regard, Imanishi et al.41 reported that GH may also suppress TGF-β–mediated cardiac fibrosis by inhibiting signal transduction. In contrast to the changes in protein expression, collagen type I and type III mRNA expression were unaffected by CRF but increased after GH treatment in the SO and CRF groups. This dissociation between protein and mRNA expression likely reflects a translational event,42 but, taken together, these changes in gene expression indicate that attention be paid to the long-term effects of GH treatment. Note that in all of these experiments, normal pair-fed control animals were not included for logistical reasons and additional experiments to dissect out any impact of reduced food intake will be required.

In a previous report,43 we described the impact of GH on bone and remnant kidneys of the same rats described in this study. GH had a positive effect on bone turnover and increased bone volume that was reduced in the untreated CRF rats. In contrast, GH had a negative impact on the remnant kidney: Tubulointerstitial damage worsened, and glomerular volume increased. A deleterious effect of GH on the rodent kidney has been noted by several investigators.44,45 Fortunately, this noxious effect seems to be limited to rodents, because prolonged treatment of children with uremia has not been associated with adverse renal effects.46

Because of its physiologic role in regulating cardiac structure and function, there has been interest in evaluating whether GH might be beneficial in cardiac disease treatment. Several studies suggested that GH may have a salutary effect on cardiac disease, although this is not a uniform finding. For example, when rats with myocardial infarcts are treated with GH, most21,47 but not all reported studies48 showed that LV remodeling and adoptive fibrosis may be attenuated and cardiac function may increase. GH also improves cardiac function in rodents with CHF49 and reverses age-related cardiac myofilament dysfunction50 while improving regional coronary blood flow and capillary density.51 GH has been studied in relatively small clinical trials of patients with ischemic and nonischemic cardiomyopathy and CHF.52,53 The results have been mixed and thus inconclusive, although a recent meta-analysis suggested that GH does improve several cardiovascular parameters in chronic CHF, suggesting the need for large-scale studies.20

In this study with uremic rats in which LV hypertrophy, a decrease in cavity size, and an increase in fractional LV shortening were present, GH treatment induced a substantial increase in fractional shortening and also tended to cause an increase in cavity size. Although diastolic dysfunction was not directly measured, the increase in fractional shortening and decrease in cavity size seen in uremic rats is highly suggestive of this widely recognized phenomenon. Physiologic effects of a therapy, namely GH, known to cause vasodilation and positive inotropy is less clear in this “compensated” setting. Although peripheral vasodilation would be expected to lead to lower BP and perhaps less hypertrophy, the lack of change in BP is likely explained by a concomitant increase in systolic function. In fact, this is what we observed. The increased cavity size in the GH group (P = 0.055) is an additional indication of improved filling that may be a reflection of this overall more favorable hemodynamic milieu, which exists despite the hyperdynamic overall function. Finally, it is conceivable that more prolonged treatment and/or more frequent administration of GH might affect a more prominent hemodynamic response.

We have shown that when GH is administered in an LD sufficient to overcome the acquired resistance of uremia, significant cardiac protection against the development of microvascular disease and possibly interstitial fibrosis is achieved. In contrast, at HD, this response to GH tends to be lost and cardiac disease may even be worsened. Although caution must be exhibited when extrapolating animal data, this study suggests that the lowest effective dosage of GH should be used when treating children with CRF to promote body growth or adults to correct protein-energy wasting,54 especially because GH may induce cardiac enlargement in patients with ESRD.55 Finally, it will be of great interest to determine whether prolonged LD GH therapy has a sustained benefit on the cardiomyopathy of uremia and whether this leads to a reduction in susceptibility to ischemic injury.

CONCISE METHODS

Experimental Animals and Protocols

Male Sprague-Dawley rats weighing approximately 245 g were entered into the study. CRF was created by a two-step five-sixths nephrectomy procedure with ketamine (80 mg/kg) and xylazine (10 mg/kg) anesthesia as described previously.25 Sham nephrectomy operations were performed on other animals. Free access to food and water was allowed. In the first series of experiments carried out over 4 mo, the CRF rats were divided into four groups 10 wk after the partial nephrectomy and treated with V or bovine GH for 6 wk and then killed, at which time the heart was perfusion-fixed for histology. Recombinant bovine GH (gift of Monsanta Corp., St Louis, MO) was used because it does not cross-react with the prolactin receptor and has low immunogenicity in the rat.34 The SO control group was treated with V alone for 6 wk. Thus, five groups of rats were studied: Group 1, SO control V treated; group 2, CRF V treated; group 3, CRF GH treated, LD (1.5 mg/kg per d); group 4, CRF GH treated, ID (4 mg/kg per d); and group 5, CRF GH treated, HD (10 mg/kg per d). Dietary protein content was increased from the standard 20 to 40% for the last 4 wk of the study.

In the second set of experiments, four groups were studied for 4 mo and were treated with V or GH, 1.5 mg/kg per d for the last 6 wk of the experiment. Group 1, SO control V treated; group 2, SO control GH treated; group 3, CRF V treated; and group 4, CRF GH treated. Echocardiography was performed on these rats. At killing, the heart was saline-perfused and collected as described next. Animals were provided a standard diet throughout.

Perfusion Fixation, Tissue Collection, and Processing

The abdominal aorta was catheterized under ketamine/xylazine anesthesia, and blood was collected. In the first set of experiments, perfusion at a pressure of approximately 100 mmHg was initiated with a 10% dextran solution containing 0.5 g/L procaine-hydrochloride, and the vena cava was incised to allow drainage of the blood containing perfusate. After 2 min, the perfusate was changed to 0.2 mol/L phosphate solution containing 3% glutaraldehyde and continued for 12 min. The heart and aorta were collected and processed according to the orientator method.56 Uniformly random sampling of the myocardium was achieved by preparing a set of equidistant slices of the LV and the interventricular septum with a random start. Two slices were selected by area weighted sampling and processed accordingly. Eight pieces of LV muscle, including the septum, were prepared and afterward embedded in Epon-Araldite. Semithin sections (0.8 μm) were stained with methylene blue and basic fuchsin and examined by light microscopy with oil immersion and phase contrast at a magnification of 1000:1. A 1-mm-thick section of the descending aorta was cut perpendicular to the vessel axis and embedded and sectioned as described already.

In the second series of experiments, tissues were perfused as already described, with PBS containing 0.5 g/L procaine hydrochloride for 2 min at room temperature followed by 2 min of perfusion with ice-cold saline. The heart was excised, the apex was frozen in liquid nitrogen for gene analysis, and the remainder was bisected and fixed in 10% formal saline before embedding in paraffin or placed in OCT and frozen at −70°C. The following antibodies were used using the avidin biotin method: TGF-β1 (sc-146, polyclonal rabbit; Santa Cruz Biotechnology, Santa Cruz, CA; 1:50), vascular endothelial growth factor (BP2990, polyclonal rabbit; ID Labs, London, ON, Canada; 1:25), collagen I (BT2150-0160, polyclonal rabbit; Bio Trend, Cologne, Germany; 1:200), collagen IV (BT2150-1470, rabbit polyclonal; Bio Trend; 1:100), collagen III (AM167-5M, mouse monoclonal; Bio Genex, San Ramon, CA; 1:100), IGF-I (sc-1422, goat polyclonal; Santa Cruz Biotechnology; 1:100).

Morphologic Analysis

All investigations were performed in a blinded manner (i.e., the observer was unaware of the animal's study group). Stereologic analysis was performed on eight random samples of differently oriented sections of the LV myocardium per animal according to the orientator method.56 Length density (LV) of capillaries (i.e., the length of capillaries per unit tissue volume) and the volume density (VV) of cardiac capillaries, defined as the volume of capillaries per unit of myocardial tissue volume, were measured in eight systematically subsampled areas per section using a Zeiss eyepiece with 100 points for point counting. The length density of myocardial capillaries (LV) was determined using the equation LV = 2 QA, where QA is area density, for example, the number of capillary transects per area of myocardial reference tissue. Total capillary length per heart was calculated using the volume of the left ventricle (V) according to the formula L = LV× V. Intercapillary distance (i.e., the distance between the centers of two adjacent intramyocardial capillaries) was calculated according to a modification of the formula of Henquell and Honig.57 Volume density (VV) of the capillaries, interstitial tissue, fibroblasts, and myocytes was obtained using the point-counting method according to the equation PP = VV, where PP is point density. Reference volume was the total myocardial tissue (exclusive of noncapillary vessels, i.e., arterioles and veins). Vascular geometry of intramyocardial arteries and of the aorta (i.e., wall thickness, lumen diameter, media, and lumen area) was analyzed using a semiautomatic image analysis system (Videoplan; Kontron Co., Eching, Germany) as described previously.58

Immunohistochemical Evaluation

Immunohistochemical evaluation was performed using a semiquantitative immunoreactive score: Two investigators, blinded with respect to the animal group, used a semiquantitative scoring system for the analysis (light microscopy; magnification ×200). The intensity of staining was ranked on an arbitrary scale: Grade 0, no staining; grade 1, faintly positive staining; grade 2, positive staining involving up to 50% of the field of view; grade 3, positive staining involving >50%; grade 4, positive staining of all structures within the field of view.

Echocardiography

Echocardiography was carried out using the GE Vivid 7 (GE Medical Systems, Milwaukee, WI) and the small animal probe (13 MHz). Rats were anesthetized with ketamine/xylazine, then placed supine and warmed using a heating pad. Using a gel buffer, parasternal long- and short-axis views were recorded in each animal to allow estimation of structure and function. Indices of structure included LV internal diameter at end diastole (LVIDd), LV internal diameter at end systole (LVIDs), interventricular septum at end diastole (IVSd), posterior wall thickness at end diastole (PWd), and LV mass [1.05 * (IVSd + LVIDd + PWd)3 − LVIDd3). LV mass was also corrected for body size. Indices of contractility included fractional shortening [(LVIDd − LVIDs)/LVIDd] and ejection fraction [(LVIDd3 − LVIDs3)/LVIDd3]. All measurements were made by one operator, who was blinded to group.

Biochemistry

Serum creatinine and urea nitrogen (mg/dl) were measured with a Beckman LX 20 Analyzer (Beckman Coulter, Fullerton, CA). Serum IGF-1 levels (ng/ml) were measured by using the OCTEIA Rat/Mouse IGF-1 Kit (IDS, Fountain Hills, AZ). Serum CRP levels were measured with a highly sensitive rat CRP ELISA Kit (Alpha Diagnostic International, San Antonio, TX).

Real-Time Quantitative RT-PCR Assay

Real-time quantitative RT-PCR with SYBR green dye was performed as described previously59 using the ABI Prism 7900 Sequence Detection System (Applied Biosystems, Foster City, CA) and protocols from the manufacturer. Primers for quantification of IGF-1, atrial natriuretic factor, collagen I, collagen III, α-SMA, TGF-β, and GH receptor and the internal control gene ribosomal 18S (Table 10) were designed with the primer design software Primer Express (Applied Biosystems) and synthesized by Operon Biotechnology (Huntsville, AL). Total RNA was extracted from the heart and used for cDNA synthesis by reverse transcription (Applied Biosystems), and the cDNA samples were subjected to PCR analysis. Results were quantified using the relative standard curve method. An internal control gene standard curve was also generated, and the target gene was normalized for this endogenous control. Each sample was analyzed in triplicate in individual assays performed on two or more occasions. Specific mRNA were normalized for the internal control gene 18S and are expressed as transcript/housekeeping gene ratios. The control SO-V group mean was given a value of 100, and individual values are expressed relative to this value.

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Table 10.

Primer sequences for quantitative real-time PCR analysis

Statistical Analysis

All data are means ± SD. Comparisons between more than two normally distributed groups were made by one-way ANOVA followed by pair-wise multiple comparison with the Duncan test.60 For more than two non-normally distributed groups, the Kruskal-Wallis statistic was applied followed by the Dunn test to distinguish between groups. P < 0.05 was considered statistically significant.

DISCLOSURES

None.

Acknowledgments

This study was supported by a Grant-in-Aid from the American Heart Association (R.R.) and a Merit Review Grant from the Research Service of the Department Veterans Affairs (R.R.) and National Institutes of Health grant RO1 DK 068517 (R.R.).

This work was presented in part in abstract form at the annual meeting of the American Society of Nephrology; San Francisco, CA; November 3, 2007.

Footnotes

  • Published online ahead of print. Publication date available at www.jasn.org.

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Low-Dose Growth Hormone is Cardioprotective in Uremia
Ralph Rabkin, Ibrahim Awwad, Yu Chen, Euan A. Ashley, Difei Sun, Sumita Sood, William Clusin, Paul Heidenreich, Grzegorz Piecha, Marie-Luise Gross
JASN Sep 2008, 19 (9) 1774-1783; DOI: 10.1681/ASN.2007121386
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