- Email: [email protected]
Effects of DASH diet on lipid profiles and biomarkers of oxidative stress in overweight and obese women with polycystic ovary syndrome: A randomized clinical trial
Accepted Manuscript The effects of DASH diet on lipid profiles and biomarkers of oxidative stress in overweight and obese women with polycystic ovary syndrome: a randomised clinical trial Zatollah Asemi, Ph.D Mansooreh Samimi, M.D Zohreh Tabassi, M.D Hossein Shakeri, M.Sc Sima-Sadat Sabihi, B.Sc Ahmad Esmaillzadeh, Ph.D PII:
S0899-9007(14)00142-7
DOI:
10.1016/j.nut.2014.03.008
Reference:
NUT 9255
To appear in:
Nutrition
Received Date: 9 October 2013 Revised Date:
20 November 2013
Accepted Date: 9 March 2014
Please cite this article as: Asemi Z, Samimi M, Tabassi Z, Shakeri H, Sabihi S-S, Esmaillzadeh A, The effects of DASH diet on lipid profiles and biomarkers of oxidative stress in overweight and obese women with polycystic ovary syndrome: a randomised clinical trial, Nutrition (2014), doi: 10.1016/ j.nut.2014.03.008. 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.
ACCEPTED MANUSCRIPT
The effects of DASH diet on lipid profiles and biomarkers of oxidative stress in
2
overweight and obese women with polycystic ovary syndrome: a randomised
3
clinical trial
4
Zatollah Asemi Ph.D. a, Mansooreh Samimi M.D. b, Zohreh Tabassi M.D. b, Hossein Shakeri
5
M.Sc. a, Sima-Sadat Sabihi B.Sc. a, Ahmad Esmaillzadeh Ph.D. c,d,* a
Research Center for Biochemistry and Nutrition in Metabolic Diseases, Kashan University of
SC
6
RI PT
1
Medical Sciences, Kashan, I.R. Iran
7 b
Department of Gynecology and Obstetrics, School of Medicine, Kashan University of Medical
M AN U
8
Sciences, Kashan, I.R. Iran
9 c
10 11
d
Food Security Research Center, Isfahan University of Medical Sciences, Isfahan, Iran
Department of Community Nutrition, School of Nutrition and Food Science, Isfahan University of Medical Sciences, Isfahan, Iran
12
Running title: DASH diet for PCOS
14 15
Z.A. conducted the study, carried out the statistical analyses, wrote the manuscript and
16
contributed in the interpretation of the findings. M.S,Z.T, H.Sh and S-S. S contributed in data
17
collection and assisted in writing the manuscript. A.E. contributed in conception and design and
18
also advised on statistical analyses and assisted in interpretation of the findings. None of the
19
authors had any personal or financial conflict of interest. All authors approved the final version
20
for submission Clinical trial registration number:www.irct.ir:IRCT201304235623N6.
21
* Corresponding author. Tel.: 98-311-7922720; fax: 98-311-6682509.
22
E-mail address: [email protected] (A. Esmaillzadeh).
AC C
EP
TE D
13
23
1
ACCEPTED MANUSCRIPT
Abstract
25
Objective: This study was designed to assess the effects of the Dietary Approaches to Stop
26
Hypertension (DASH) diet on lipid profiles and biomarkers of oxidative stress in overweight and
27
obese women with polycystic ovary syndrome (PCOS).
28
Methods: This randomised controlled clinical trial was done among 48women diagnosed with
29
PCOS. Subjects were randomly assigned to consume either the control (n=24) or the DASH
30
eating pattern (n=24) for 8 weeks. Both diets were designed to be calorie-restricted. The DASH
31
and control diets were consisted of 52% carbohydrates, 18% proteins, 30% total fats. The DASH
32
diet was designed to be rich in fruits, vegetables, whole grains, and low-fat dairy products and
33
low in saturated fats, cholesterol and refined grains. Fasting blood samples were taken at baseline
34
and after 8-wk intervention to measure lipid profiles and biomarkers of oxidative stress including
35
plasma total antioxidant capacity (TAC) and total glutathione (GSH).
36
Results: Adherence to the DASH diet, compared to the control diet, resulted in a significant
37
decrease in weight (-4.4 vs. -1.5 kg; P<0.001) and BMI (-1.7 vs. -0.6 kg/m2; P<0.001), decreased
38
serum triglycerides (-10.0 vs. +19.2 mg/dL; P-interaction=0.005) and VLDL-C levels (-2.0 vs.
39
+3.9 mg/dL; P-interaction=0.005). Increased concentrations of TAC (+98.6 vs. -174.8 mmol/L;
40
P-interaction<0.001) and GSH (+66.4 vs. -155.6 µmol/L; P-interaction=0.005) were also found
41
in the DASH group compared with the control group.
42
Conclusion: Consumption of DASH diet for 8 weeks led to a significant reduction in serum
43
insulin, triglycerides and VLDL-C and a significant increase in TAC and GSH levels.
44
KEYWORDS: DASH, polycystic ovary syndrome, lipids, oxidative stress, women
AC C
EP
TE D
M AN U
SC
RI PT
24
45
2
ACCEPTED MANUSCRIPT
Introduction
47
Polycystic ovary syndrome (PCOS) is the most common endocrinopathy among reproductive-
48
aged women [1] affecting6 to 18% of female adults[2].The estimated prevalence of this condition
49
in Iran has been reported to be7% based on the National Institute of Health (NIH)criteria, 15.2%
50
according to the Rotterdam criteria, and 7.9% according to the Androgen Excess Society
51
(AES)criteria [3].Women with PCOS have androgen excess, insulin resistance, variable amounts
52
of estrogen exposure, all of which can result in increased lipid profiles and biomarkers of
53
oxidative stress [4-5]. In addition, increased visceral fat and the reduction of adiponectin levels in
54
PCOS would result in elevated lipid profiles [6-7]. Decreased expression of peroxisome
55
proliferators activated receptor (PPAR) in PCOS patients can also result in dyslipidimia and
56
increased biomarkers of oxidative stress [8]. PCOS is associated with infertility [9], increased
57
risk of endometrial, breast and ovarian cancers [10] and increased incidence of type 2 diabetes
58
[11].
59
Weight loss and lifestyle modifications including increased physical activity is the first-line
60
treatment in the management of PCOS [12]. It has been reported that losing 5% of body weight in
61
obese women with PCOS can result in improved hyperandrogenic features[13].Furthermore, the
62
use of oral contraceptive pills and metformin may help induce the regular menses [14] and reduce
63
hyperinsulinemia and ovarian androgens production in these women[15].Recently, it has been
64
suggested that low-carbohydrate, low glycemic load and high-protein diets might beneficially
65
influence PCOS than the conventional low-fat, high-carbohydrate diets[16-17].Consumption of a
66
low glycemic load diet in combination with medications has been resulted in symptoms relief in
67
patients with PCOS [18]. However, adherence to a high-protein and low-glycemicload diet for 12
68
weeks did not influence lipid profiles among women with PCOS [19].
AC C
EP
TE D
M AN U
SC
RI PT
46
3
ACCEPTED MANUSCRIPT
The dietary approaches to stop hypertension (DASH) eating plan is a low-glycemic-index low
70
energy-dense diet that has firstly been suggested for lowering blood pressure [20]; however, its
71
beneficial effects have also been reported in type 2 diabetes[21],gestational diabetes[22]and
72
metabolic syndrome [23]. Although the influence of some dietary components of DASH diet like
73
antioxidants[24-25], magnesium[26], dietary fiber, fruit and vegetables[25] in PCOS has been
74
assessed in previous studies, we are aware of no study examining the effects of DASH diet on
75
metabolic profiles and biomarkers of oxidative stress in patients with PCOS. High contents of
76
dietary fiber, antioxidants, phytoestrogens and isoflavones along with its low glycemic index [21,
77
23] might help PCOS patients to control their increased levels of lipid profile and oxidative
78
stress. Furthermore, adherence to the DASH diet has been associated with lower body fat [21],
79
which could in turn result in lower testosterone levels [27], a key component in PCOS. The
80
current study was, therefore, performed to investigate the effects of the DASH eating plan on
81
lipid profiles and biomarkers of oxidative stress in overweight and obese women with PCOS.
82
Materials and Methods
83
Participants
84
This two-arm parallel randomized controlled clinical trial was carried out in Kashan, Iran, from
85
January 2012 to May2012. With the exception of the study dietitian (Z.A.), who provided the
86
dietary education, all the study personnel and participants were blinded to dietary assignment.
87
Overweight or obese (BMI≥25 kg/m2) women aged 18-40 y diagnosed with PCOS based on
88
Rotterdam criteria were recruited in this study. On the basis of sample size formula suggested for
89
randomized clinical trials [19], considering the type I error of 5% (α=0.05), type II error of 20%
90
(β=0.20; Power=80%) and serum LDL-cholesterol levels as a key variable, we reached the
91
sample size of 20 persons for each group. Diagnosis of PCOS was done according to the
92
Rotterdam criteria[28]:those with the two of the following criteria were considered as having
AC C
EP
TE D
M AN U
SC
RI PT
69
4
ACCEPTED MANUSCRIPT
PCOS: oligo- and/or anovulation, excess androgen activity (clinical or biochemical)and
94
polycystic ovaries(by gynecologic ultrasound).We did not include women aged<18 or >40 years,
95
those with BMI<25 kg/m2, individuals with neoplastic, hepatic, renal or cardiovascular disorders,
96
malabsorptive disorders, current or previous (within the last 6 months) use of hormonal,
97
antidiabetic, or anti-obesity medications and intention to adopt a diet and/or a specific physical
98
activity program. A total of 150 women attended gynecology clinics affiliated to Kashan
99
University of Medical Sciences, Kashan, Iran, were screened for PCOS. Females who reported
100
menstrual irregularity and/or had a modified Ferriman Gallwey (mF-G) score of 8 [29] were
101
invited for a clinical examination. Those who did not have these criteria were not further
102
evaluated and were deemed not to have PCOS. Taking a medical history and focusing on
103
symptoms of PCOS, specifically menstrual irregularities, clinical hyperandrogenism and
104
medication use including hormone therapy was done by trained midwifes. Menstrual irregularity
105
was assessed as the presence of chronic amenorrhea or a menstrual cycle length of less than 21
106
days or more than 35 days, or more than four days variation between cycles. Clinical
107
hyperandrogenism was assessed as the self-reported degree of hirsutism using the modified
108
Ferriman Gallwey (mF-G) scoring method based on a chart displaying degree of hair growth in
109
nine regions. Polycystic ovaries were diagnosed by Ultrasonography (US) in participants with
110
menstrual dysfunction and/or hirsutism (12 or more small follicles observed in an ovary on
111
ultrasound examination).Furthermore, hormone profiles including serum prolactin, T3, T4 and
112
TSH levels were assessed for all individuals at study baseline and having abnormal levels of
113
these hormones was considered as a criteria for PCOS rejection based on the Rotterdam criteria.
114
Finally, 54 women met the inclusion criteria and were enrolled in the study (Fig. 1).Subjects
115
were stratified according to BMI (<30 and ≥30 kg/m2) and age (<30 and ≥30 y) and then were
116
randomly assigned to the control (n=27) or the DASH diet (n=27) for 8 weeks. Random
AC C
EP
TE D
M AN U
SC
RI PT
93
5
ACCEPTED MANUSCRIPT
assignment was done by the use of computer-generated random numbers [30].The study was
118
conducted according to the guidelines laid down in the Declaration of Helsinki. The ethical
119
committee of Kashan University of Medical Sciences approved the study (no. P/29/5/1/9213) and
120
informed written consent was obtained from all participants.
121
Study design
122
Participants were randomly assigned to consume the control or the DASH diet for 8 weeks. They
123
were asked not to alter their routine physical activity, and not to receive any lipid-lowering
124
medications as well as medications that might affect their reproductive physiology during the 8-
125
wk intervention. Compliance with the consumption of diets was monitored once a week through
126
phone interviews. The compliance was also double-checked by the use of three-day dietary
127
records completed throughout the study. Dietary intakes of participants were assessed by means
128
of three-day dietary records (two week days at weeks 3 and 6 and one weekend day at week 8 of
129
intervention) completed throughout the study. The dietary records were based on estimated
130
values in household measurements.To obtain nutrient intakes of participants based on these three-
131
day food diaries, we used Nutritionist IV software (First Databank, San Bruno, CA) modified for
132
Iranian foods.
133
Diets
134
Calorie requirements of each subject were estimated based on resting energy expenditure (by the
135
use of Harris-Benedict equation) and physical activity level [31]. As all study participants were
136
overweight or obese, both diets were designed to be calorie-restricted (350-700 kcal less than the
137
computed energy requirement for each participant; 350 kcal for subjects with the BMI in the
138
range of 25-27.5 kg/m2; 500 kcal for those with the BMI in the range of 27.5-31 kg/m2; and 700
139
kcal for those with the BMI >31 kg/m2) to avoid ethical problems. We used two dietary plans: 1)
140
a DASH diet that was consisted of 52% carbohydrates, 18% proteins, 30% total fats. The DASH
AC C
EP
TE D
M AN U
SC
RI PT
117
6
ACCEPTED MANUSCRIPT
diet was designed to be rich in fruits, vegetables, whole grains, and low-fat dairy products and
142
low in saturated fats, cholesterol, refined grains, and sweets. Prescribed sodium in the DASH diet
143
was less than 2,400 mg/day.2) The control diet was also designed to contain52% carbohydrates,
144
18% protein and 30% total fat [23]; however, the two diets were different in terms of food groups
145
contained (Table 1). It must be kept in mind that this study was not a feeding trial; therefore, we
146
did not prepare foods for participants. In this study we just provided 7-day menu cycles to
147
participants. The diets were individually planned using a ‘calorie count’ system. To facilitate the
148
compliance to the diets, subjects were given and instructed an exchange list. To control for
149
dietary intakes of participants throughout the study, the dietitian was calling the participants to
150
resolve their probable problems. Furthermore, to examine the compliance to the diets, we asked
151
participants to record their dietary intakes every two weeks. All participants spent about 45
152
minutes with a dietitian learning the basics of their diets.
153
Assessment of anthropometric measures
154
Weight was assessed at baseline and after 8 weeks of intervention in gynecology clinics by
155
trained midwifes. Body weight was measured in an overnight fasting status without shoes in a
156
minimal clothing state by the use of a digital scale (Seca, Hamburg, Germany) to the nearest 0.1
157
kg. Height was measured using a non-stretched tape measure (Seca, Hamburg, Germany) to the
158
nearest 0.1 cm. BMI was calculates as weight in kg divided by height in meters squared.
159
Biochemical assessment
160
Fasting blood samples (10 mL) were taken at baseline and after 8-wk intervention at Kashan
161
reference laboratory in an early morning after an overnight fasting. Serum total cholesterol and
162
triglycerides concentrations were assayed using commercial kits (Parsazmun, Tehran, Iran) by
163
enzymatic colorimetric tests with cholesterol oxidase p-aminophenazone and glycerol phosphate
164
oxidase, respectively. Serum HDL-cholesterol was measured after precipitation of the
AC C
EP
TE D
M AN U
SC
RI PT
141
7
ACCEPTED MANUSCRIPT
apolipoprotein B containing lipoproteins with phosphotungistic acid. Serum VLDL- and LDL-
166
cholesterol levels were also measured using available kits. Plasma total antioxidant capacity
167
(TAC) was assessed by means of the FRAP method developed by Benzie and Strain [32]. Plasma
168
GSH levels were measured using the method of Beutler et al [33].
169
Statistical analysis
170
We used Kolmogrov-Smirnov test to examine the normal distribution of variables. Log
171
transformation was applied for non-normally distributed variables. The analyses were done based
172
on intention-to-treat analysis. Missing values were treated based on Last-Observation-Carried-
173
Forward method. Independent samples Student’s t test was used to detect differences in general
174
characteristics and dietary intakes between the two groups. Energy-adjusted dietary intakes of
175
nutrients were computed using residual method and compared using analysis of covariance. To
176
determine the effects of DASH diet on lipid profiles and biomarkers of oxidative stress, we used
177
one-way repeated measures analysis of variance. In this analysis, the treatment (DASH vs.
178
control diet) was regarded as between-subject factor and time with two time-points (baseline and
179
week 8 of intervention) was considered as within-subject factor. An additional model was
180
constructed to control for the effect of age. We further adjusted for weight changes to determine
181
of if the effect of DASH diet is independent of weight change. P<0.05 was considered as
182
statistically significant. All statistical analyses were done using the Statistical Package for Social
183
Science version 17 (SPSS Inc., Chicago, Illinois, USA).
184
Results
185
Among individuals in the control diet, 3 women [IVF treatment (n=1), became pregnant (n=1) or
186
the use of medications (n=1)] were excluded. The exclusions in the DASH diet were 3 persons
187
[IVF treatment (n=1), health problems (n=1) and the use of medications (n=1)]. Finally, 48
188
participants [control diet (n=24) and the DASH diet (n=24) completed the trial (Fig. 1).
AC C
EP
TE D
M AN U
SC
RI PT
165
8
ACCEPTED MANUSCRIPT
Mean age of study participants was not statistically different between the DASH and control
190
groups. Comparison of weight and BMI both at baseline and end of trial did not reveal a
191
significant difference between the two groups (Table 2). When we compared the changes in
192
weight and BMI between the two groups, we found greater reductions in both weight (-4.4±2.7
193
vs. -1.5±2.6 kg, P<0.001) and BMI (-1.7±1.1 vs. -0.6±0.9 kg/m2, P<0.001) in DASH group than
194
those in the control group.
195
Based on the three-day dietary records that participants provided throughout the study, no
196
statistically significant difference was seen between the two groups in terms of dietary intakes of
197
energy, carbohydrates, protein and fat; however, significant differences were found in dietary
198
intakes of saturated fatty acids (SFA), polyunsaturated fatty acids (PUFA), cholesterol, dietary
199
fiber, simple sugar, sodium, potassium, magnesium and calcium between the two groups (Table
200
3).
201
Compared to the control diet, consumption of DASH eating pattern led to decreased serum
202
triglycerides (-10.0 vs. +19.2 mg/dL; P-interaction=0.005) and VLDL-C levels (-2.0 vs. +3.9
203
mg/dL; P-interaction=0.005) (Table 4). Further control for age did not alter the findings. After
204
additional adjustments for weight change, we found that those in the DASH group tended to have
205
reduced levels of serum triglycerides (-5.9±7.5 vs. +15.2±7.5 mg/dL, P-interaction=0.07) and
206
VLDL-C levels (-1.2±1.5 vs. +3.0±1.5 mg/dL, P-interaction=0.07) compared with individuals in
207
control group. Increased concentrations of plasma TAC (+98.6 vs. -174.8 mmol/L; P-
208
interaction<0.001) and total GSH (+66.4 vs. -155.6 µmol/L; P-interaction=0.005) were also
209
found in the DASH group compared with the control group. When age and weight changes were
210
taken into account, we observed that individuals in the DASH diet tended to have lower levels of
211
plasma GSH levels than those in the control group (+34.1±57.6 vs. -123.3±57.6µmol/L, P-
212
interaction=0.07).Adherence to the DASH eating pattern, compared to the control diet, resulted in
AC C
EP
TE D
M AN U
SC
RI PT
189
9
ACCEPTED MANUSCRIPT
a significant reduction in serum insulin levels (-1.88 vs. +2.89 µIU/mL, P-interaction=0.03), but
214
did not significantly affect fasting plasma glucose levels (-0.5 vs. +5.7 mg/dL; P-
215
interaction=0.20).We failed to find significant differences in mean changes of serum total
216
cholesterol, HDL- and LDL-C levels between the two diets. Within-group changes revealed a
217
significant decrease of serum triglycerides levels (P=0.04) and a significant increase of plasma
218
TAC levels (P= 0.03) in the DASH diet, but a significant elevation of serum triglyceride levels
219
(P=0.03) and a significant reduction of plasma TAC levels (P=0.001) was seen in the control diet.
220
Furthermore, a significant within-group reduction in plasma total GSH levels was also seen in the
221
control group (P=0.005).
222
Discussion
223
We found that adherence of the DASH eating pattern for 8 weeks among overweight and obese
224
women with PCOS had beneficial effects on weight, BMI, serum triglycerides, VLDL-C, insulin,
225
plasma TAC and total GSH levels compared with the control diet. However, the effects of DASH
226
eating pattern on serum total cholesterol, HDL- and LDL-C were not significantly different
227
compared with the control diet.
228
Few studies evaluated the beneficial effects of diet therapy on metabolic status in women PCOS.
229
According to our knowledge, no information is available indicating the effect of DASH diet on
230
metabolic profiles of PCOS patients. Although the efficacy of DASH diet has been examined in
231
metabolic syndrome [23], childhood obesity [34] and patients with stroke [35], we are aware of
232
no study examining the effect of DASH diet on metabolic profiles of PCOS patients.
233
Furthermore, there is still no definite dietary recommendation for these patients. In a previous
234
study, Mehrabani et al [19] reported the beneficial effects of a high-protein, low-glycemic-load
235
hypocaloric diet (30% of daily energy from protein plus low-glycemic-load foods) in overweight
236
and obese women with PCOS after 12 weeks. Mehrabani et al have examined the effect of a high
AC C
EP
TE D
M AN U
SC
RI PT
213
10
ACCEPTED MANUSCRIPT
protein diet, while in the current study we assessed the effect of DASH diet. The high protein
238
diets are totally different from the DASH diet. Furthermore while both diets in our study were
239
designed to be calorie-restricted (350-700 kcal less than the computed energy requirement for
240
each participant), Mehrabani et al [19] prescribed a fixed range of dietary energy (1200-1700
241
kcal/d) for all participants. Finally, Mehrabani et al did not examine the effect of their dietary
242
intervention on biomarkers of oxidative stress, while we assessed the effect of DASH diet on
243
these biomarkers as well.
244
The current study showed that consumption of the DASH diet compared with the control diet led
245
to a significant reduction in weight, BMI and serum insulin levels. In line with our study, weight
246
loss and improved insulin sensitivity was also seen following energy restriction for 12 weeks in
247
overweight women with PCOS [17].Even short-term energy restrictions for 4 weeks in PCOS
248
patients resulted in a lower fasting insulin [36-37]. It is possible that the family of insulin-like
249
growth factors (IGFs) and their binding proteins get involved, as they have been shown to be
250
differentially influenced by energy restriction [37] and weight loss [36]. Specifically, decreased
251
insulin levels would result in increased IGF-binding protein-1 during short-term energy
252
restriction [17].
253
It has been shown that PCOS is associated with decreased levels of adiponectine concentrations,
254
which in turn is associated with disturbances of the mitogen-activated protein kinases (MAPK)
255
and nuclear factor kappa-light-chain-enhancer of activated B cells (NF-kB) signaling pathway.
256
These conditions would lead to increased inflammatory markers and biomarkers of oxidative
257
stress [7]. Increased lipid profiles and biomarkers of oxidative stress would result in several
258
aberrations [38-39].Our study demonstrated that consumption of the DASH eating plan
259
significantly reduced serum triglycerides and VLDL-C levels, but could not affect serum total-,
260
HDL- and LDL-C levels among women with PCOS. Previous studies have shown the beneficial
AC C
EP
TE D
M AN U
SC
RI PT
237
11
ACCEPTED MANUSCRIPT
effects of DASH diet on serum lipid profiles of patients with hypertension, cardiovascular
262
disease, metabolic syndrome and type 2 diabetes [21, 23, 40-41]. Our previous study among
263
pregnant women with gestational diabetes mellitus (GDM) has also indicated a significant
264
reduction of serum triglycerides, total cholesterol and LDL-C concentrations following
265
consumption of the DASH eating patternfor4 weeks [22]. Azadbakht et al [21] have shown a
266
significant decrease of serum LDL-C and an increase of HDL-C levels after intervention with the
267
DASH diet intype 2 diabetic patients.Similar findings were also seen with the administration of
268
DASH dietfor8 weeks in patients with the metabolic syndrome [23], for 30 days in subjects with
269
elevated blood pressure [42]and for 8 weeks in hypercholestrolemic patients[43].Several
270
mechanisms can explain the beneficial effects of DASH diet on lipid profiles in PCOS women. In
271
this study, dietary intake of simple sugar in the DASH diet was about half that of the control diet.
272
Furthermore, its fiber content was 1.5-2.0 times higher than that of the control diet. Earlier
273
studies have shown that high-sugar diets might induce mitochondrial dysfunction in adipose
274
tissue, which can in turn lead to metabolic impairment and elevated serum triglycerides levels
275
[44].The DASH diet contain high amounts of arginine-rich foods including fish, soy, beans,
276
lentils, whole grains, and nuts, parsley and fresh basil. The high arginine content of DASH diet
277
might also explain its beneficial effects on insulin resistance and serum triglycerides levels.
278
Decreased serum triglycerides levels following arginine intake have been attributed to shifting
279
nutrient partitioning to promote muscle over fat gain and may in turn provide a useful treatment
280
for improving the metabolic profile [45]. The DASH diet is also a rich source of dietary calcium
281
and magnesium, through which it can affect triglyceride levels. Increased intracellular calcium in
282
liver may stimulate microsomal triglyceride transfer protein (MTP) which is implicated in the
283
formation and secretion of VLDL, and then result in decreased serum triglycerides levels
284
[46].Furthermore, magnesium intake has been associated with lower levels of serum lipids due to
AC C
EP
TE D
M AN U
SC
RI PT
261
12
ACCEPTED MANUSCRIPT
suppressing endothelial injury, reducing the peroxidation of lipids and increasing the antioxidant
286
capacity in serum and tissues [47].
287
The current study revealed that consumption of the DASH diet resulted in a significant increase
288
in plasma TAC and total GSH levels among overweight and obese women with PCOS. Our
289
previous study has indicated that consumption of DASH diet increased plasma TAC and total
290
GSH levels in pregnant women with GDM after 4 weeks[48].Similar findings has also been
291
reported following consumption of the DASH eating pattern in free-living obese hypertensive’s
292
after 4 weeks [49].Adherence to the low-sodium DASH diet in salt-sensitive (SS) subjects has
293
also been resulted in decreased urine F2-isoprostanes, a biomarker of oxidative stress, than a
294
standardized usual low fruit and vegetables diet (ULFV) [50].However, consumption of the
295
DASH eating plan after 3 months led to a non-significant increase in plasma TAC in healthy
296
individuals [51]. Overall, as PCOS is associated with increased oxidative stress [52],
297
consumption of the DASH diet in patients with PCOS could help them control the complications
298
these conditions might led to. The favorable effects of DASH diet on biomarkers of oxidative
299
stress could be attributed to its high content of antioxidant-rich fruit and vegetables [49, 53-54].
300
Individuals in the DASH group received vitamin C nearly 2 times greater than that in the control
301
group. Vitamin C, a major component of TAC, can decrease the NADPH oxidase activity, which
302
is a major superoxide-generating enzyme and increased oxidative stress [55]. High intakes of
303
calcium and magnesium in the DASH diet might also help explain it effects on decreased
304
oxidative stress. Calcium can act as a DNA damage reducing agent [56], which in turn results in
305
the free radical scavenging and increased plasma TAC and total GSH levels. In addition,
306
restoring the activity of anti-oxidative enzymes [57] and scavenging oxygen radicals [58] that
307
results from magnesium intake can provide some reasons for our findings. Finally, the arginine
308
content of DASH diet might also explain its beneficial effects on decreased oxidative stress.
AC C
EP
TE D
M AN U
SC
RI PT
285
13
ACCEPTED MANUSCRIPT
Arginine intake has been shown to reduce serum levels of angiotensin II and measures of
310
oxidative stress [59].
311
Our findings must be interpreted in the context of some limitations. The first limitation is the
312
relatively short duration of intervention. Long-term interventions might result in greater changes
313
in lipid profiles. Second, we could not assess the effects of DASH eating plan on other
314
biochemical indicators of oxidative stress and factors of peroxidation. Further studies are required
315
to examine the effects of DASH diet on other measures of oxidative stress.
316
In conclusion, consumption of DASH eating pattern for 8 weeks among overweight and obese
317
women with PCOS resulted in a significant decrease in weight, BMI, serum insulin, triglycerides
318
and VLDL-C levels as well as a significant increase in plasma TAC and total GSH levels. Given
319
the high prevalence of PCOS and based on the findings of the current study, we believe that the
320
DASH diet could be recommended as a suitable diet for these patients to control abnormal
321
metabolic profiles.
TE D
M AN U
SC
RI PT
309
AC C
EP
322
14
ACCEPTED MANUSCRIPT
Acknowledgment
324
The present study was supported by a grant (no. 9213) from the Vice-chancellor for Research,
325
KUMS, Kashan, Iran. The authors would like to thank the staff of Naghavi and Shaheed Beheshti
326
gynecology Clinics (Kashan, Iran) for their assistance in this project.
327
Clinical trial registration number: www.irct.ir:IRCT201304235623N6.
328
Name of trial registry: Effects of the hypocaloric DASH diet on metabolic parameters,
329
inflammatory factor and biomarkers of oxidative stress in overweight and obese women with
330
polycystic ovary syndrome.
331
Accessed protocol: www.irct.ir:IRCT201304235623N6.
SC
M AN U
AC C
EP
TE D
332
15
RI PT
323
ACCEPTED MANUSCRIPT
333
References
334
[1]
335
with metformin and clomiphene citrate for ovulation induction in women with PCOS. Cochrane
336
Database Syst Rev 2012;10:CD006226.
RI PT
Sinawat S, Buppasiri P, Lumbiganon P, Pattanittum P. Long versus short course treatment
337 338
[2]
Teede HJ, Joham AE, Paul E, Moran LJ, Loxton D, Jolley D, et al. Longitudinal weight
339
gain in women identified With polycystic ovary syndrome: Results of an observational study in
340
young women. Obesity (Silver Spring) 2013; 21:1526-32.
SC
341
[3]
Mehrabian F, Khani B, Kelishadi R, Ghanbari E. The prevalence of polycystic ovary
343
syndrome in Iranian women based on different diagnostic criteria. Endokrynol Pol 2011;62:238-
344
42.
M AN U
342
345
[4]
Wild RA. Dyslipidemia in PCOS. Steroids 2012;77:295-9.
348
[5]
Gonzalez F. Inflammation in Polycystic Ovary Syndrome: underpinning of insulin
349
resistance and ovarian dysfunction. Steroids 2012;77:300-5.
346
TE D
347
350
[6]
352
Front Horm Res 2013;40:40-50.
353
Carmina E. Obesity, adipokines and metabolic syndrome in polycystic ovary syndrome.
EP
351
[7]
355
modulates oxidative stress-induced autophagy in cardiomyocytes. PLoS One 2013;8:e68697.
356
Essick EE, Wilson RM, Pimentel DR, Shimano M, Baid S, Ouchi N, et al. Adiponectin
AC C
354
357
[8]
San Millan JL, Corton M, Villuendas G, Sancho J, Peral B, Escobar-Morreale HF.
358
Association of the polycystic ovary syndrome with genomic variants related to insulin resistance,
359
type 2 diabetes mellitus, and obesity. J Clin Endocrinol Metab 2004;89:2640-6.
360 361
[9]
McGowan MP. Polycystic ovary syndrome: a common endocrine disorder and risk factor
362
for vascular disease. Curr Treat Options Cardiovasc Med 2011;13:289-301.
363
16
ACCEPTED MANUSCRIPT
364
[10]
Fanta M. Is polycystic ovary syndrome, a state of relative estrogen excess, a real risk
365
factor for estrogen-dependant malignancies? Gynecol Endocrinol 2013;29:145-7.
366
[11]
Hudecova M, Jan H, Christian B, Poromaa Inger S. Long-term reproductive and
368
metabolic consequences of PCOS. Curr Diabetes Rev 2012;8:444-51.
369
RI PT
367
[12]
Costello MF, Misso ML, Wong J, Hart R, Rombauts L, Melder A, et al. The treatment of
371
infertility in polycystic ovary syndrome: a brief update. Aust N Z J Obstet Gynaecol
372
2012;52:400-3.
SC
370
373
[13]
Motta AB. The role of obesity in the development of polycystic ovary syndrome. Curr
375
Pharm Des 2012;18:2482-91.
M AN U
374
376 377
[14]
Harwood K, Vuguin P, DiMartino-Nardi J. Current approaches to the diagnosis and
378
treatment of polycystic ovarian syndrome in youth. Horm Res 2007;68:209-17.
379
[15]
Costello MF, Ledger WL. Evidence-based lifestyle and pharmacological management of
381
infertility in women with polycystic ovary syndrome. Womens Health (Lond Engl) 2012;8:277-
382
90.
TE D
380
383
[16]
Galletly C, Moran L, Noakes M, Clifton P, Tomlinson L, Norman R. Psychological
385
benefits of a high-protein, low-carbohydrate diet in obese women with polycystic ovary
386
syndrome--a pilot study. Appetite 2007;49:590-3.
387
AC C
EP
384
388
[17]
Moran LJ, Noakes M, Clifton PM, Tomlinson L, Galletly C, Norman RJ. Dietary
389
composition in restoring reproductive and metabolic physiology in overweight women with
390
polycystic ovary syndrome. J Clin Endocrinol Metab 2003;88:812-9.
391 392
[18]
Herriot AM, Whitcroft S, Jeanes Y. An retrospective audit of patients with polycystic
393
ovary syndrome: the effects of a reduced glycaemic load diet. J Hum Nutr Diet 2008;21:337-45.
394
17
ACCEPTED MANUSCRIPT
395
[19]
Mehrabani HH, Salehpour S, Amiri Z, Farahani SJ, Meyer BJ, Tahbaz F. Beneficial
396
effects of a high-protein, low-glycemic-load hypocaloric diet in overweight and obese women
397
with polycystic ovary syndrome: a randomized controlled intervention study. J Am Coll Nutr
398
2012;31:117-25.
RI PT
399 400
[20]
Vollmer WM, Sacks FM, Ard J, Appel LJ, Bray GA, Simons-Morton DG, et al. Effects of
401
diet and sodium intake on blood pressure: subgroup analysis of the DASH-sodium trial. Ann
402
Intern Med 2001;135:1019-28.
SC
403
[21]
Azadbakht L, Fard NR, Karimi M, Baghaei MH, Surkan PJ, Rahimi M, et al. Effects of
405
the Dietary Approaches to Stop Hypertension (DASH) eating plan on cardiovascular risks among
406
type 2 diabetic patients: a randomized crossover clinical trial. Diabetes Care 2011;34:55-7.
M AN U
404
407 408
[22]
Asemi Z, Tabassi Z, Samimi M, Fahiminejad T, Esmaillzadeh A. Favourable effects of
409
the Dietary Approaches to Stop Hypertension diet on glucose tolerance and lipid profiles in
410
gestational diabetes: a randomised clinical trial. Br J Nutr 2013; 109:2024-30.
TE D
411 412
[23]
Azadbakht L, Mirmiran P, Esmaillzadeh A, Azizi T, Azizi F. Beneficial effects of a
413
Dietary Approaches to Stop Hypertension eating plan on features of the metabolic syndrome.
414
Diabetes Care 2005;28:2823-31.
EP
415
[24]
417
intakes of fat and antioxidant vitamins are predictors of subclinical inflammation in overweight
418
Swiss children. Am J Clin Nutr 2006;84:748-55.
419
Aeberli I, Molinari L, Spinas G, Lehmann R, l'Allemand D, Zimmermann MB. Dietary
AC C
416
420
[25]
Holt EM, Steffen LM, Moran A, Basu S, Steinberger J, Ross JA, et al. Fruit and vegetable
421
consumption and its relation to markers of inflammation and oxidative stress in adolescents. J
422
Am Diet Assoc 2009;109:414-21.
423 424
[26]
King DE, Mainous AG, 3rd, Geesey ME, Ellis T. Magnesium intake and serum C-
425
reactive protein levels in children. Magnes Res 2007;20:32-6. 18
ACCEPTED MANUSCRIPT
426 427
[27]
Luo X, Xu L. [Association of fat distribution with metabolic syndrome in patients with
428
polycystic ovary syndrome]. Nan Fang Yi Ke Da Xue Xue Bao 2012;32:1325-7.
429
[28]
Revised 2003 consensus on diagnostic criteria and long-term health risks related to
431
polycystic ovary syndrome. Fertil Steril 2004;81:19-25.
RI PT
430
432
[29]
Liang SJ, Hsu CS, Tzeng CR, Chen CH, Hsu MI. Clinical and biochemical presentation
434
of polycystic ovary syndrome in women between the ages of 20 and 40. Hum Reprod
435
2011;26:3443-9.
SC
433
437
[30]
438
Care J 2010;1:7-9.
M AN U
436
Dettori J. The random allocation process: two things you need to know. Evid Based Spine
439 440
[31]
American Dietetic Association, Pediatric Weight Management Guideline. The 2005 US
441
Institutes of Medicine "Dietary Reference Intakes for Energy, Carbohydrate, Fiber, Fat, Fatty
442
Acids,
443
http://wwwadaevidencelibrarycom/topiccfm?format_tables=0&cat=3060&auth=1.
Protein,
and
Amino
Acids
(Macronutrients)".
444
[32]
446
"antioxidant power": the FRAP assay. Anal Biochem 1996;239:70-6.
Benzie IF, Strain JJ. The ferric reducing ability of plasma (FRAP) as a measure of
[33]
Beutler E, Gelbart T. Plasma glutathione in health and in patients with malignant disease.
449
J Lab Clin Med 1985;105:581-4.
AC C
448
450
at:
EP
445
447
Available
TE D
Cholesterol,
451
[34]
Saneei P, Hashemipour M, Kelishadi R, Rajaei S, Esmaillzadeh A. Effects of
452
recommendations to follow the Dietary Approaches to Stop Hypertension (DASH) diet v. usual
453
dietary advice on childhood metabolic syndrome: a randomised cross-over clinical trial. Br J Nutr
454
2013. Epub ahead of print; DOI: 10.1017/S0007114513001724.
455
19
ACCEPTED MANUSCRIPT
456
[35]
Lin PH, Yeh WT, Svetkey LP, Chuang SY, Chang YC, Wang C, et al. Dietary intakes
457
consistent with the DASH dietary pattern reduce blood pressure increase with age and risk for
458
stroke in a Chinese population. Asia Pac J Clin Nutr 2013;22:482-91.
459
[36]
Kiddy DS, Hamilton-Fairley D, Seppala M, Koistinen R, James VH, Reed MJ, et al. Diet-
461
induced changes in sex hormone binding globulin and free testosterone in women with normal or
462
polycystic ovaries: correlation with serum insulin and insulin-like growth factor-I. Clin
463
Endocrinol (Oxf) 1989;31:757-63.
RI PT
460
SC
464
[37]
Hamilton-Fairley D, Kiddy D, Anyaoku V, Koistinen R, Seppala M, Franks S. Response
466
of sex hormone binding globulin and insulin-like growth factor binding protein-1 to an oral
467
glucose tolerance test in obese women with polycystic ovary syndrome before and after calorie
468
restriction. Clin Endocrinol (Oxf) 1993;39:363-7.
M AN U
465
469 470
[38]
Atiomo W, Daykin CA. Metabolomic biomarkers in women with polycystic ovary
471
syndrome: a pilot study. Mol Hum Reprod 2012;18:546-53.
TE D
472 473
[39]
Murri M, Luque-Ramirez M, Insenser M, Ojeda-Ojeda M, Escobar-Morreale HF.
474
Circulating markers of oxidative stress and polycystic ovary syndrome (PCOS): a systematic
475
review and meta-analysis. Hum Reprod Update 2013; 19:268-88.
EP
476
[40]
478
syndrome, and other conditions: a review. Nutr Clin Pract 2008;23:142-51.
479
Champagne CM. Magnesium in hypertension, cardiovascular disease, metabolic
AC C
477
480
[41]
Doyle L, Cashman KD. The effect of nutrient profiles of the Dietary Approaches to Stop
481
Hypertension (DASH) diets on blood pressure and bone metabolism and composition in
482
normotensive and hypertensive rats. Br J Nutr 2003;89:713-24.
483 484
[42]
Harsha DW, Sacks FM, Obarzanek E, Svetkey LP, Lin PH, Bray GA, et al. Effect of
485
dietary sodium intake on blood lipids: results from the DASH-sodium trial. Hypertension
486
2004;43:393-8. 20
ACCEPTED MANUSCRIPT
487 488
[43]
Obarzanek E, Sacks FM, Vollmer WM, Bray GA, Miller ER, 3rd, Lin PH, et al. Effects
489
on blood lipids of a blood pressure-lowering diet: the Dietary Approaches to Stop Hypertension
490
(DASH) Trial. Am J Clin Nutr 2001;74:80-9.
RI PT
491 492
[44]
Lomba A, Milagro FI, Garcia-Diaz DF, Campion J, Marzo F, Martinez JA. A high-
493
sucrose isocaloric pair-fed model induces obesity and impairs NDUFB6 gene function in rat
494
adipose tissue. J Nutrigenet Nutrigenomics 2009;2:267-72.
SC
495
[45]
Jobgen W, Meininger CJ, Jobgen SC, Li P, Lee MJ, Smith SB, et al. Dietary L-arginine
497
supplementation reduces white fat gain and enhances skeletal muscle and brown fat masses in
498
diet-induced obese rats. J Nutr 2009;139:230-7.
M AN U
496
499 500
[46]
Cho HJ, Kang HC, Choi SA, Ju YC, Lee HS, Park HJ. The possible role of Ca2+ on the
501
activation of microsomal triglyceride transfer protein in rat hepatocytes. Biol Pharm Bull
502
2005;28:1418-23.
TE D
503 504
[47]
King JL, Miller RJ, Blue JP, Jr., O'Brien WD, Jr., Erdman JW, Jr. Inadequate dietary
505
magnesium intake increases atherosclerotic plaque development in rabbits. Nutr Res
506
2009;29:343-9.
EP
507
[48]
509
clinical trial investigating the effect of DASH diet on insulin resistance, inflammation, and
510
oxidative stress in gestational diabetes. Nutrition 2013;29:619-24.
511
Asemi Z, Samimi M, Tabassi Z, Sabihi SS, Esmaillzadeh A. A randomized controlled
AC C
508
512
[49]
Lopes HF, Martin KL, Nashar K, Morrow JD, Goodfriend TL, Egan BM. DASH diet
513
lowers blood pressure and lipid-induced oxidative stress in obesity. Hypertension 2003;41:422-
514
30.
515
21
ACCEPTED MANUSCRIPT
516
[50]
Al-Solaiman Y, Jesri A, Zhao Y, Morrow JD, Egan BM. Low-Sodium DASH reduces
517
oxidative stress and improves vascular function in salt-sensitive humans. J Hum Hypertens
518
2009;23:826-35.
519
[51]
Miller ER, 3rd, Erlinger TP, Sacks FM, Svetkey LP, Charleston J, Lin PH, et al. A dietary
521
pattern that lowers oxidative stress increases antibodies to oxidized LDL: results from a
522
randomized controlled feeding study. Atherosclerosis 2005;183:175-82.
RI PT
520
523
[52]
De Leo V, La Marca A, Cappelli V, Stendardi A, Focarelli R, Musacchio MC, et al.
525
[Evaluation of the treatment with D-chiroi-nositol on levels of oxidative stress in pcos patients.].
526
Minerva Ginecol 2012;64:531-8.
M AN U
SC
524
527 528
[53]
Avignon A, Hokayem M, Bisbal C, Lambert K. Dietary antioxidants: Do they have a role
529
to play in the ongoing fight against abnormal glucose metabolism? Nutrition 2012;28:715-21.
530
[54]
Puchau B, Zulet MA, de Echavarri AG, Hermsdorff HH, Martinez JA. Dietary total
532
antioxidant capacity is negatively associated with some metabolic syndrome features in healthy
533
young adults. Nutrition 2010;26:534-41.
TE D
531
534
[55]
Chen X, Touyz RM, Park JB, Schiffrin EL. Antioxidant effects of vitamins C and E are
536
associated with altered activation of vascular NADPH oxidase and superoxide dismutase in
537
stroke-prone SHR. Hypertension 2001;38:606-11.
EP
535
538
[56]
Fedirko V, Bostick RM, Long Q, Flanders WD, McCullough ML, Sidelnikov E, et al.
540
Effects of supplemental vitamin D and calcium on oxidative DNA damage marker in normal
541
colorectal mucosa: a randomized clinical trial. Cancer Epidemiol Biomarkers Prev 2010;19:280-
542
91.
AC C
539
543 544
[57]
Yang Y, Gao M, Nie W, Yuan J, Zhang B, Wang Z, et al. Dietary magnesium sulfate
545
supplementation protects heat stress-induced oxidative damage by restoring the activities of anti-
546
oxidative enzymes in broilers. Biol Trace Elem Res 2012;146:53-8. 22
ACCEPTED MANUSCRIPT
547 548
[58]
Hans CP, Chaudhary DP, Bansal DD. Effect of magnesium supplementation on oxidative
549
stress in alloxanic diabetic rats. Magnes Res 2003;16:13-9.
550
[59]
Vasdev S, Gill V. The antihypertensive effect of arginine. Int J Angiol 2008;17:7-22.
RI PT
551 552
AC C
EP
TE D
M AN U
SC
553
23
ACCEPTED MANUSCRIPT
554
Table 1
555
Constituents of the DASH and control diets used in the study٭ DASH diet
Grains †
9
6
Simple sugar
5
Vegetables
2
Fruits
2
Dairy ††
2
Meats, poultry and fish†††
4
Nuts, seeds and legumes
1
Fats and oils
3
556
DASH, Dietary Approaches to Stop Hypertension
557
٭
558
†
559
††
560
†††
SC
3
4 2
3
4 servings from lean meat in the DASH diet and 2 servings in the control diet
TE D EP AC C
567
5
Low-fat (<2%) in the DASH diet
563
566
4
At least 3 servings from whole grains in the DASH diet
562
565
2
Data are presented for a calorie intake of 1700 kcal/day
561
564
RI PT
Control diet
M AN U
Food group
568 569 570
24
ACCEPTED MANUSCRIPT
571
Table 2
572
General characteristics of the study participants٭ DASH diet (n=24) 22.1±3.2
P value†
Height (cm)
161.3±6.0
160.5±4.9
0.60
Weight at study baseline (kg)
74.6±16.2
78.0±12.0
0.41
Weight at end-of-trial (kg)
73.1±15.5
73.6±12.1
0.90
-4.4±2.7
<0.001
30.3±4.5
0.27
BMI at study baseline (kg/m2)
28.6±5.8
BMI at end-of-trial (kg/m2)
28.0±5.7
28.6±4.4
0.74
BMI change (kg/m2)
-0.6±0.9
-1.7±1.1
<0.001
* Data are means ± SD.
575
† Obtained from independent t test.
TE D
574
576
582 583
AC C
581
EP
577
580
M AN U
-1.5±2.6
BMI, Body mass index
579
0.07
Weight change (kg)
573
578
SC
Age (y)
RI PT
Control diet (n=24) 24.7±6.0
584 585 586
25
ACCEPTED MANUSCRIPT
587
Table 3
588
Dietary intakes of study participants throughout the study٭ P value†
DASH diet
(n=24)
(n=24)
Energy (kcal/d)
1887±138
1839±122
0.20
Fat (g/d)
62.9±4.6
61.3±4.0
0.20
Protein (g/d)
84.9±6.2
82.8±5.5
0.20
245.3±17.9
239.1±15.8
0.20
Crude
13.8±1.0
<0.001
Model 1
13.6±0.1
8.8±0.1
<0.001
Crude
11.3±0.8
18.6±1.2
<0.001
Model 1
11.1±0.1
18.8±0.1
<0.001
Crude
185.5±14.6
141.6±20.7
0.001
Model 1
182.3±1.0
144.8±1.0
0.001
Crude
12.1±1.5
17.2±1.3
<0.001
Model 1
11.9±0.2
17.4±0.2
<0.001
Crude
3.5±0.4
4.8±0.4
<0.001
Model 1
3.5±0.1
4.9±0.1
<0.001
Crude
2815.5 ±460.4
1729.8±103.5
<0.001
Model 1
2785.5 ±41.2
1699.1±15.4
<0.001
Crude
3190.4±278.3
4864.4±329.3
<0.001
Model 1
3140.3±29.0
4914.3±29.0
<0.001
PUFA (g/d)
TE D
Cholesterol (mg/d)
Dietary fiber (g/d)
AC C
Insoluble fiber (g/d)
M AN U
8.7±0.6
EP
SFA (g/d)
SC
Carbohydrate (g/d)
RI PT
Control diet
Sodium (mg/d)
Potassium (mg/d)
Magnesium (mg/d)
26
ACCEPTED MANUSCRIPT
Crude
233.1±17.9
411.5±15.2
<0.001
Model 1
230.9±2.3
413.7±2.3
<0.001
Crude
1038.6±42.2
1717.2±36.2
<0.001
Model 1
1032.3±1.7
1724.3±1.7
<0.001
Fruit (servings/day)
2.8±0.4
5.2±0.4
<0.001
Vegetables (servings/day)
2.6±0.5
4.3±0.4
<0.001
Nuts (servings/day)
1.0±0.2
2.5±0.4
<0.001
Fats and oils (servings/day)
3.5±0.5
3.6±0.5
0.40
SC
RI PT
Calcium (mg/d)
DASH, Dietary Approaches to Stop Hypertension; PUFA, Polyunsaturated fats; SFA, Saturated fatty
590
acids
591
* Data are means ± SD.
592
† Obtained from independent t test.
593
Model 1: Adjusted for energy intake (data are means± standard error)
594 595
M AN U
589
.
AC C
EP
TE D
596
27
ACCEPTED MANUSCRIPT
Table 4
P value†
DASH diet (n=24) Wk8
Change
Time
Group
Time x Group
162.8±33.6
-4.2±24.7
0.95
0.33
0.29
166.4±6.2
-3.2±6.2
0.34
0.10
0.45
165.9±6.7
1.2±6.5
0.72
0.33
0.84
109.2±49.7
99.2±45.2٭
-10.0±22.3
0.35
0.93
0.005
112.5±9.9
104.6±11.3
-7.9±7.0
0.18
0.48
0.01
113.5±10.7
107.6±12.1
-5.9±7.5
0.30
0.39
0.07
21.8±9.9
19.8±9.0٭
-2.0±4.5
0.35
0.93
0.005
22.5±2.0
20.9±2.3
-1.6±1.4
0.18
0.48
0.01
3.0±1.5
22.7±2.1
21.5±2.4
-1.2±1.5
0.30
0.39
0.07
46.7±7.9
-0.2±9.9
48.4±9.9
48.2±12.8
-0.2±9.3
0.89
0.59
0.95
46.5±2.3
46.9±2.2
0.4±2.0
48.8±2.3
48.0±2.2
-0.8±2.0
0.20
0.68
0.54
Model 2
46.6±2.5
46.6±2.4
EP
Control diet (n=24)
RI PT
Means (±standard deviation) of serum lipid profiles and biomarkers of oxidative stress at baseline and after the intervention
Wk0
Wk8
Change
Wk0
Crude
153.5±42.0
158.3±31.5
4.8±34.4
167.0±33.7
Model 1
151.0±7.8
154.6±6.2
3.6±6.2
169.6±7.8
Model 2
155.8±8.1
155.1±6.7
-0.7±6.5
164.7±8.1
Crude
93.3±47.9
112.5±67.3٭
19.2±42.8
Model 1
89.9±9.9
107.1±11.3
17.2±7.0
Model 2
88.9±10.7
104.1±12.1
15.2±7.5
Crude
18.6±9.6
22.5±13.5٭
3.9±8.6
Model 1
18.0±2.0
21.4±2.3
3.4±1.4
Model 2
17.8±2.1
20.8±2.4
Crude
46.9±11.8
Model 1
0.0±2.1
48.7±2.5
48.3±2.4
-0.4±2.1
0.18
0.57
0.89
Crude
88.0±30.0
89.0±23.2
1.0±25.9
96.8±30.6
94.8±29.5
-2.0±22.7
0.89
0.65
0.65
Model 1
86.5±6.3
86.3±5.2
-0.2±5.0
98.3±6.3
97.5±5.2
-0.8±5.0
0.19
0.13
0.93
Model 2
91.4±6.4
87.7±5.5
-3.7±5.2
93.3±6.4
96.1±5.5
2.8±5.2
0.48
0.53
0.40
3.4±0.8
3.4±0.7
0.0±0.48
3.6±1.0
3.6±1.1
0.0±0.7
0.67
0.43
0.54
TE D
VLDL-C(mg/dL)
AC C
HDL-C (mg/dL)
LDL-C(mg/dL)
M AN U
Triglycerides (mg/dL)
SC
Total cholesterol(mg/dL)
Total: HDL-C ratio Crude
28
ACCEPTED MANUSCRIPT
Model 1
3.3±0.2
3.4±0.2
0.1±0.1
3.6±0.2
3.7±0.2
0.1±0.1
0.03
0.24
0.99
Model 2
3.4±0.2
3.4±0.2
0.0±0.1
3.6±0.2
3.7±0.2
0.1±0.1
0.14
0.50
0.27
Crude
968.5±233.1
793.7±103.4٭
-174.8±218.0
921.7±226.7
1020.3±301.9٭
98.6±213.7
0.22
0.12
<0.001
Model 1
978.0±47.7
795.7±47.4
-182.3±45.0
912.2±47.7
1018.0±47.4
105.8±45.0
0.27
0.20
<0.001
Model 2
983.7±51.1
795.8±51.2
-187.9±48.5
906.5±51.5
1018.0±51.2
111.5±48.5
0.34
0.29
<0.001
Crude
601.8±267.9
446.2±131.9٭
-155.6±242.8
478.3±195.9
544.7±220.2
66.4±279.0
0.24
0.79
0.005
Model 1
586.8±47.9
445.0±38.1
-141.8±53.9
493.4±47.8
545.9±38.1
52.5±53.9
0.27
0.93
0.01
Model 2
566.0±50.9
442.7±41.2
-123.3±57.6
514.1±50.9
548.2±41.2
34.1±57.6
0.44
0.63
0.07
RI PT
TAC (mmol/L)
M AN U
SC
GSH (µmol/L)
DASH, Dietary Approaches to Stop Hypertension; FPG, Fasting plasma glucose; GSH, Total glutathione; HOMA-IR, Homeostasis Model of Assessment-Insulin Resistance; HDL-C, High density lipoprotein-cholesterol; hs-CRP, High-sensitivity C-reactive protein; LDL-C, Low density lipoprotein-cholesterol; TAC, total antioxidant capacity; VLDL-C, Very low density lipoprotein-cholesterol ٭Different from wk 0, P < 0.05with paired samples t test. Model 1: Adjusted for age (data are means± standard error)
TE D
†Obtained from repeated measures ANOVA test.
AC C
EP
Model 2: Adjusted for Model 1+ weight change (data are means± standard error)
29
ACCEPTED MANUSCRIPT
Assessed for screening (n=150)
Lost to follow-up (n=3)
M AN U
Allocated to control (n=27)
Allocated to intervention (n=27)
Lost to follow-up (n=3)
♦ IVF treatment (n=1) ♦ Health problems (n=1) ♦ The use of medications (n=1)
Analyzed (n=24)
Analyzed (n=24)
EP
TE D
♦ IVF treatment (n=1) ♦ Became pregnant (n=1) ♦ The use of medications (n=1)
AC C
Analysis
Follow-up
Allocation
Randomized (n=54)
SC
RI PT
Enrollment
Excluded (n=96) ♦ Not living in Kashan (n=24) ♦ Taking excluded medications (n=17) ♦ Within normal weight range (n=15) ♦ Outside the age range required (n=14) ♦ Unable to commit to study (n=12) ♦ Excluded health condition (n=6) ♦ Not diagnosed with PCOS (n=4) ♦ Recent weight loss (n=4)
Fig. 1.Summary of patient flow
IVF, In vitro fertilisation; PCOS, Polycystic ovary syndrome
30
S0899-9007(14)00142-7
DOI:
10.1016/j.nut.2014.03.008
Reference:
NUT 9255
To appear in:
Nutrition
Received Date: 9 October 2013 Revised Date:
20 November 2013
Accepted Date: 9 March 2014
Please cite this article as: Asemi Z, Samimi M, Tabassi Z, Shakeri H, Sabihi S-S, Esmaillzadeh A, The effects of DASH diet on lipid profiles and biomarkers of oxidative stress in overweight and obese women with polycystic ovary syndrome: a randomised clinical trial, Nutrition (2014), doi: 10.1016/ j.nut.2014.03.008. 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.
ACCEPTED MANUSCRIPT
The effects of DASH diet on lipid profiles and biomarkers of oxidative stress in
2
overweight and obese women with polycystic ovary syndrome: a randomised
3
clinical trial
4
Zatollah Asemi Ph.D. a, Mansooreh Samimi M.D. b, Zohreh Tabassi M.D. b, Hossein Shakeri
5
M.Sc. a, Sima-Sadat Sabihi B.Sc. a, Ahmad Esmaillzadeh Ph.D. c,d,* a
Research Center for Biochemistry and Nutrition in Metabolic Diseases, Kashan University of
SC
6
RI PT
1
Medical Sciences, Kashan, I.R. Iran
7 b
Department of Gynecology and Obstetrics, School of Medicine, Kashan University of Medical
M AN U
8
Sciences, Kashan, I.R. Iran
9 c
10 11
d
Food Security Research Center, Isfahan University of Medical Sciences, Isfahan, Iran
Department of Community Nutrition, School of Nutrition and Food Science, Isfahan University of Medical Sciences, Isfahan, Iran
12
Running title: DASH diet for PCOS
14 15
Z.A. conducted the study, carried out the statistical analyses, wrote the manuscript and
16
contributed in the interpretation of the findings. M.S,Z.T, H.Sh and S-S. S contributed in data
17
collection and assisted in writing the manuscript. A.E. contributed in conception and design and
18
also advised on statistical analyses and assisted in interpretation of the findings. None of the
19
authors had any personal or financial conflict of interest. All authors approved the final version
20
for submission Clinical trial registration number:www.irct.ir:IRCT201304235623N6.
21
* Corresponding author. Tel.: 98-311-7922720; fax: 98-311-6682509.
22
E-mail address: [email protected] (A. Esmaillzadeh).
AC C
EP
TE D
13
23
1
ACCEPTED MANUSCRIPT
Abstract
25
Objective: This study was designed to assess the effects of the Dietary Approaches to Stop
26
Hypertension (DASH) diet on lipid profiles and biomarkers of oxidative stress in overweight and
27
obese women with polycystic ovary syndrome (PCOS).
28
Methods: This randomised controlled clinical trial was done among 48women diagnosed with
29
PCOS. Subjects were randomly assigned to consume either the control (n=24) or the DASH
30
eating pattern (n=24) for 8 weeks. Both diets were designed to be calorie-restricted. The DASH
31
and control diets were consisted of 52% carbohydrates, 18% proteins, 30% total fats. The DASH
32
diet was designed to be rich in fruits, vegetables, whole grains, and low-fat dairy products and
33
low in saturated fats, cholesterol and refined grains. Fasting blood samples were taken at baseline
34
and after 8-wk intervention to measure lipid profiles and biomarkers of oxidative stress including
35
plasma total antioxidant capacity (TAC) and total glutathione (GSH).
36
Results: Adherence to the DASH diet, compared to the control diet, resulted in a significant
37
decrease in weight (-4.4 vs. -1.5 kg; P<0.001) and BMI (-1.7 vs. -0.6 kg/m2; P<0.001), decreased
38
serum triglycerides (-10.0 vs. +19.2 mg/dL; P-interaction=0.005) and VLDL-C levels (-2.0 vs.
39
+3.9 mg/dL; P-interaction=0.005). Increased concentrations of TAC (+98.6 vs. -174.8 mmol/L;
40
P-interaction<0.001) and GSH (+66.4 vs. -155.6 µmol/L; P-interaction=0.005) were also found
41
in the DASH group compared with the control group.
42
Conclusion: Consumption of DASH diet for 8 weeks led to a significant reduction in serum
43
insulin, triglycerides and VLDL-C and a significant increase in TAC and GSH levels.
44
KEYWORDS: DASH, polycystic ovary syndrome, lipids, oxidative stress, women
AC C
EP
TE D
M AN U
SC
RI PT
24
45
2
ACCEPTED MANUSCRIPT
Introduction
47
Polycystic ovary syndrome (PCOS) is the most common endocrinopathy among reproductive-
48
aged women [1] affecting6 to 18% of female adults[2].The estimated prevalence of this condition
49
in Iran has been reported to be7% based on the National Institute of Health (NIH)criteria, 15.2%
50
according to the Rotterdam criteria, and 7.9% according to the Androgen Excess Society
51
(AES)criteria [3].Women with PCOS have androgen excess, insulin resistance, variable amounts
52
of estrogen exposure, all of which can result in increased lipid profiles and biomarkers of
53
oxidative stress [4-5]. In addition, increased visceral fat and the reduction of adiponectin levels in
54
PCOS would result in elevated lipid profiles [6-7]. Decreased expression of peroxisome
55
proliferators activated receptor (PPAR) in PCOS patients can also result in dyslipidimia and
56
increased biomarkers of oxidative stress [8]. PCOS is associated with infertility [9], increased
57
risk of endometrial, breast and ovarian cancers [10] and increased incidence of type 2 diabetes
58
[11].
59
Weight loss and lifestyle modifications including increased physical activity is the first-line
60
treatment in the management of PCOS [12]. It has been reported that losing 5% of body weight in
61
obese women with PCOS can result in improved hyperandrogenic features[13].Furthermore, the
62
use of oral contraceptive pills and metformin may help induce the regular menses [14] and reduce
63
hyperinsulinemia and ovarian androgens production in these women[15].Recently, it has been
64
suggested that low-carbohydrate, low glycemic load and high-protein diets might beneficially
65
influence PCOS than the conventional low-fat, high-carbohydrate diets[16-17].Consumption of a
66
low glycemic load diet in combination with medications has been resulted in symptoms relief in
67
patients with PCOS [18]. However, adherence to a high-protein and low-glycemicload diet for 12
68
weeks did not influence lipid profiles among women with PCOS [19].
AC C
EP
TE D
M AN U
SC
RI PT
46
3
ACCEPTED MANUSCRIPT
The dietary approaches to stop hypertension (DASH) eating plan is a low-glycemic-index low
70
energy-dense diet that has firstly been suggested for lowering blood pressure [20]; however, its
71
beneficial effects have also been reported in type 2 diabetes[21],gestational diabetes[22]and
72
metabolic syndrome [23]. Although the influence of some dietary components of DASH diet like
73
antioxidants[24-25], magnesium[26], dietary fiber, fruit and vegetables[25] in PCOS has been
74
assessed in previous studies, we are aware of no study examining the effects of DASH diet on
75
metabolic profiles and biomarkers of oxidative stress in patients with PCOS. High contents of
76
dietary fiber, antioxidants, phytoestrogens and isoflavones along with its low glycemic index [21,
77
23] might help PCOS patients to control their increased levels of lipid profile and oxidative
78
stress. Furthermore, adherence to the DASH diet has been associated with lower body fat [21],
79
which could in turn result in lower testosterone levels [27], a key component in PCOS. The
80
current study was, therefore, performed to investigate the effects of the DASH eating plan on
81
lipid profiles and biomarkers of oxidative stress in overweight and obese women with PCOS.
82
Materials and Methods
83
Participants
84
This two-arm parallel randomized controlled clinical trial was carried out in Kashan, Iran, from
85
January 2012 to May2012. With the exception of the study dietitian (Z.A.), who provided the
86
dietary education, all the study personnel and participants were blinded to dietary assignment.
87
Overweight or obese (BMI≥25 kg/m2) women aged 18-40 y diagnosed with PCOS based on
88
Rotterdam criteria were recruited in this study. On the basis of sample size formula suggested for
89
randomized clinical trials [19], considering the type I error of 5% (α=0.05), type II error of 20%
90
(β=0.20; Power=80%) and serum LDL-cholesterol levels as a key variable, we reached the
91
sample size of 20 persons for each group. Diagnosis of PCOS was done according to the
92
Rotterdam criteria[28]:those with the two of the following criteria were considered as having
AC C
EP
TE D
M AN U
SC
RI PT
69
4
ACCEPTED MANUSCRIPT
PCOS: oligo- and/or anovulation, excess androgen activity (clinical or biochemical)and
94
polycystic ovaries(by gynecologic ultrasound).We did not include women aged<18 or >40 years,
95
those with BMI<25 kg/m2, individuals with neoplastic, hepatic, renal or cardiovascular disorders,
96
malabsorptive disorders, current or previous (within the last 6 months) use of hormonal,
97
antidiabetic, or anti-obesity medications and intention to adopt a diet and/or a specific physical
98
activity program. A total of 150 women attended gynecology clinics affiliated to Kashan
99
University of Medical Sciences, Kashan, Iran, were screened for PCOS. Females who reported
100
menstrual irregularity and/or had a modified Ferriman Gallwey (mF-G) score of 8 [29] were
101
invited for a clinical examination. Those who did not have these criteria were not further
102
evaluated and were deemed not to have PCOS. Taking a medical history and focusing on
103
symptoms of PCOS, specifically menstrual irregularities, clinical hyperandrogenism and
104
medication use including hormone therapy was done by trained midwifes. Menstrual irregularity
105
was assessed as the presence of chronic amenorrhea or a menstrual cycle length of less than 21
106
days or more than 35 days, or more than four days variation between cycles. Clinical
107
hyperandrogenism was assessed as the self-reported degree of hirsutism using the modified
108
Ferriman Gallwey (mF-G) scoring method based on a chart displaying degree of hair growth in
109
nine regions. Polycystic ovaries were diagnosed by Ultrasonography (US) in participants with
110
menstrual dysfunction and/or hirsutism (12 or more small follicles observed in an ovary on
111
ultrasound examination).Furthermore, hormone profiles including serum prolactin, T3, T4 and
112
TSH levels were assessed for all individuals at study baseline and having abnormal levels of
113
these hormones was considered as a criteria for PCOS rejection based on the Rotterdam criteria.
114
Finally, 54 women met the inclusion criteria and were enrolled in the study (Fig. 1).Subjects
115
were stratified according to BMI (<30 and ≥30 kg/m2) and age (<30 and ≥30 y) and then were
116
randomly assigned to the control (n=27) or the DASH diet (n=27) for 8 weeks. Random
AC C
EP
TE D
M AN U
SC
RI PT
93
5
ACCEPTED MANUSCRIPT
assignment was done by the use of computer-generated random numbers [30].The study was
118
conducted according to the guidelines laid down in the Declaration of Helsinki. The ethical
119
committee of Kashan University of Medical Sciences approved the study (no. P/29/5/1/9213) and
120
informed written consent was obtained from all participants.
121
Study design
122
Participants were randomly assigned to consume the control or the DASH diet for 8 weeks. They
123
were asked not to alter their routine physical activity, and not to receive any lipid-lowering
124
medications as well as medications that might affect their reproductive physiology during the 8-
125
wk intervention. Compliance with the consumption of diets was monitored once a week through
126
phone interviews. The compliance was also double-checked by the use of three-day dietary
127
records completed throughout the study. Dietary intakes of participants were assessed by means
128
of three-day dietary records (two week days at weeks 3 and 6 and one weekend day at week 8 of
129
intervention) completed throughout the study. The dietary records were based on estimated
130
values in household measurements.To obtain nutrient intakes of participants based on these three-
131
day food diaries, we used Nutritionist IV software (First Databank, San Bruno, CA) modified for
132
Iranian foods.
133
Diets
134
Calorie requirements of each subject were estimated based on resting energy expenditure (by the
135
use of Harris-Benedict equation) and physical activity level [31]. As all study participants were
136
overweight or obese, both diets were designed to be calorie-restricted (350-700 kcal less than the
137
computed energy requirement for each participant; 350 kcal for subjects with the BMI in the
138
range of 25-27.5 kg/m2; 500 kcal for those with the BMI in the range of 27.5-31 kg/m2; and 700
139
kcal for those with the BMI >31 kg/m2) to avoid ethical problems. We used two dietary plans: 1)
140
a DASH diet that was consisted of 52% carbohydrates, 18% proteins, 30% total fats. The DASH
AC C
EP
TE D
M AN U
SC
RI PT
117
6
ACCEPTED MANUSCRIPT
diet was designed to be rich in fruits, vegetables, whole grains, and low-fat dairy products and
142
low in saturated fats, cholesterol, refined grains, and sweets. Prescribed sodium in the DASH diet
143
was less than 2,400 mg/day.2) The control diet was also designed to contain52% carbohydrates,
144
18% protein and 30% total fat [23]; however, the two diets were different in terms of food groups
145
contained (Table 1). It must be kept in mind that this study was not a feeding trial; therefore, we
146
did not prepare foods for participants. In this study we just provided 7-day menu cycles to
147
participants. The diets were individually planned using a ‘calorie count’ system. To facilitate the
148
compliance to the diets, subjects were given and instructed an exchange list. To control for
149
dietary intakes of participants throughout the study, the dietitian was calling the participants to
150
resolve their probable problems. Furthermore, to examine the compliance to the diets, we asked
151
participants to record their dietary intakes every two weeks. All participants spent about 45
152
minutes with a dietitian learning the basics of their diets.
153
Assessment of anthropometric measures
154
Weight was assessed at baseline and after 8 weeks of intervention in gynecology clinics by
155
trained midwifes. Body weight was measured in an overnight fasting status without shoes in a
156
minimal clothing state by the use of a digital scale (Seca, Hamburg, Germany) to the nearest 0.1
157
kg. Height was measured using a non-stretched tape measure (Seca, Hamburg, Germany) to the
158
nearest 0.1 cm. BMI was calculates as weight in kg divided by height in meters squared.
159
Biochemical assessment
160
Fasting blood samples (10 mL) were taken at baseline and after 8-wk intervention at Kashan
161
reference laboratory in an early morning after an overnight fasting. Serum total cholesterol and
162
triglycerides concentrations were assayed using commercial kits (Parsazmun, Tehran, Iran) by
163
enzymatic colorimetric tests with cholesterol oxidase p-aminophenazone and glycerol phosphate
164
oxidase, respectively. Serum HDL-cholesterol was measured after precipitation of the
AC C
EP
TE D
M AN U
SC
RI PT
141
7
ACCEPTED MANUSCRIPT
apolipoprotein B containing lipoproteins with phosphotungistic acid. Serum VLDL- and LDL-
166
cholesterol levels were also measured using available kits. Plasma total antioxidant capacity
167
(TAC) was assessed by means of the FRAP method developed by Benzie and Strain [32]. Plasma
168
GSH levels were measured using the method of Beutler et al [33].
169
Statistical analysis
170
We used Kolmogrov-Smirnov test to examine the normal distribution of variables. Log
171
transformation was applied for non-normally distributed variables. The analyses were done based
172
on intention-to-treat analysis. Missing values were treated based on Last-Observation-Carried-
173
Forward method. Independent samples Student’s t test was used to detect differences in general
174
characteristics and dietary intakes between the two groups. Energy-adjusted dietary intakes of
175
nutrients were computed using residual method and compared using analysis of covariance. To
176
determine the effects of DASH diet on lipid profiles and biomarkers of oxidative stress, we used
177
one-way repeated measures analysis of variance. In this analysis, the treatment (DASH vs.
178
control diet) was regarded as between-subject factor and time with two time-points (baseline and
179
week 8 of intervention) was considered as within-subject factor. An additional model was
180
constructed to control for the effect of age. We further adjusted for weight changes to determine
181
of if the effect of DASH diet is independent of weight change. P<0.05 was considered as
182
statistically significant. All statistical analyses were done using the Statistical Package for Social
183
Science version 17 (SPSS Inc., Chicago, Illinois, USA).
184
Results
185
Among individuals in the control diet, 3 women [IVF treatment (n=1), became pregnant (n=1) or
186
the use of medications (n=1)] were excluded. The exclusions in the DASH diet were 3 persons
187
[IVF treatment (n=1), health problems (n=1) and the use of medications (n=1)]. Finally, 48
188
participants [control diet (n=24) and the DASH diet (n=24) completed the trial (Fig. 1).
AC C
EP
TE D
M AN U
SC
RI PT
165
8
ACCEPTED MANUSCRIPT
Mean age of study participants was not statistically different between the DASH and control
190
groups. Comparison of weight and BMI both at baseline and end of trial did not reveal a
191
significant difference between the two groups (Table 2). When we compared the changes in
192
weight and BMI between the two groups, we found greater reductions in both weight (-4.4±2.7
193
vs. -1.5±2.6 kg, P<0.001) and BMI (-1.7±1.1 vs. -0.6±0.9 kg/m2, P<0.001) in DASH group than
194
those in the control group.
195
Based on the three-day dietary records that participants provided throughout the study, no
196
statistically significant difference was seen between the two groups in terms of dietary intakes of
197
energy, carbohydrates, protein and fat; however, significant differences were found in dietary
198
intakes of saturated fatty acids (SFA), polyunsaturated fatty acids (PUFA), cholesterol, dietary
199
fiber, simple sugar, sodium, potassium, magnesium and calcium between the two groups (Table
200
3).
201
Compared to the control diet, consumption of DASH eating pattern led to decreased serum
202
triglycerides (-10.0 vs. +19.2 mg/dL; P-interaction=0.005) and VLDL-C levels (-2.0 vs. +3.9
203
mg/dL; P-interaction=0.005) (Table 4). Further control for age did not alter the findings. After
204
additional adjustments for weight change, we found that those in the DASH group tended to have
205
reduced levels of serum triglycerides (-5.9±7.5 vs. +15.2±7.5 mg/dL, P-interaction=0.07) and
206
VLDL-C levels (-1.2±1.5 vs. +3.0±1.5 mg/dL, P-interaction=0.07) compared with individuals in
207
control group. Increased concentrations of plasma TAC (+98.6 vs. -174.8 mmol/L; P-
208
interaction<0.001) and total GSH (+66.4 vs. -155.6 µmol/L; P-interaction=0.005) were also
209
found in the DASH group compared with the control group. When age and weight changes were
210
taken into account, we observed that individuals in the DASH diet tended to have lower levels of
211
plasma GSH levels than those in the control group (+34.1±57.6 vs. -123.3±57.6µmol/L, P-
212
interaction=0.07).Adherence to the DASH eating pattern, compared to the control diet, resulted in
AC C
EP
TE D
M AN U
SC
RI PT
189
9
ACCEPTED MANUSCRIPT
a significant reduction in serum insulin levels (-1.88 vs. +2.89 µIU/mL, P-interaction=0.03), but
214
did not significantly affect fasting plasma glucose levels (-0.5 vs. +5.7 mg/dL; P-
215
interaction=0.20).We failed to find significant differences in mean changes of serum total
216
cholesterol, HDL- and LDL-C levels between the two diets. Within-group changes revealed a
217
significant decrease of serum triglycerides levels (P=0.04) and a significant increase of plasma
218
TAC levels (P= 0.03) in the DASH diet, but a significant elevation of serum triglyceride levels
219
(P=0.03) and a significant reduction of plasma TAC levels (P=0.001) was seen in the control diet.
220
Furthermore, a significant within-group reduction in plasma total GSH levels was also seen in the
221
control group (P=0.005).
222
Discussion
223
We found that adherence of the DASH eating pattern for 8 weeks among overweight and obese
224
women with PCOS had beneficial effects on weight, BMI, serum triglycerides, VLDL-C, insulin,
225
plasma TAC and total GSH levels compared with the control diet. However, the effects of DASH
226
eating pattern on serum total cholesterol, HDL- and LDL-C were not significantly different
227
compared with the control diet.
228
Few studies evaluated the beneficial effects of diet therapy on metabolic status in women PCOS.
229
According to our knowledge, no information is available indicating the effect of DASH diet on
230
metabolic profiles of PCOS patients. Although the efficacy of DASH diet has been examined in
231
metabolic syndrome [23], childhood obesity [34] and patients with stroke [35], we are aware of
232
no study examining the effect of DASH diet on metabolic profiles of PCOS patients.
233
Furthermore, there is still no definite dietary recommendation for these patients. In a previous
234
study, Mehrabani et al [19] reported the beneficial effects of a high-protein, low-glycemic-load
235
hypocaloric diet (30% of daily energy from protein plus low-glycemic-load foods) in overweight
236
and obese women with PCOS after 12 weeks. Mehrabani et al have examined the effect of a high
AC C
EP
TE D
M AN U
SC
RI PT
213
10
ACCEPTED MANUSCRIPT
protein diet, while in the current study we assessed the effect of DASH diet. The high protein
238
diets are totally different from the DASH diet. Furthermore while both diets in our study were
239
designed to be calorie-restricted (350-700 kcal less than the computed energy requirement for
240
each participant), Mehrabani et al [19] prescribed a fixed range of dietary energy (1200-1700
241
kcal/d) for all participants. Finally, Mehrabani et al did not examine the effect of their dietary
242
intervention on biomarkers of oxidative stress, while we assessed the effect of DASH diet on
243
these biomarkers as well.
244
The current study showed that consumption of the DASH diet compared with the control diet led
245
to a significant reduction in weight, BMI and serum insulin levels. In line with our study, weight
246
loss and improved insulin sensitivity was also seen following energy restriction for 12 weeks in
247
overweight women with PCOS [17].Even short-term energy restrictions for 4 weeks in PCOS
248
patients resulted in a lower fasting insulin [36-37]. It is possible that the family of insulin-like
249
growth factors (IGFs) and their binding proteins get involved, as they have been shown to be
250
differentially influenced by energy restriction [37] and weight loss [36]. Specifically, decreased
251
insulin levels would result in increased IGF-binding protein-1 during short-term energy
252
restriction [17].
253
It has been shown that PCOS is associated with decreased levels of adiponectine concentrations,
254
which in turn is associated with disturbances of the mitogen-activated protein kinases (MAPK)
255
and nuclear factor kappa-light-chain-enhancer of activated B cells (NF-kB) signaling pathway.
256
These conditions would lead to increased inflammatory markers and biomarkers of oxidative
257
stress [7]. Increased lipid profiles and biomarkers of oxidative stress would result in several
258
aberrations [38-39].Our study demonstrated that consumption of the DASH eating plan
259
significantly reduced serum triglycerides and VLDL-C levels, but could not affect serum total-,
260
HDL- and LDL-C levels among women with PCOS. Previous studies have shown the beneficial
AC C
EP
TE D
M AN U
SC
RI PT
237
11
ACCEPTED MANUSCRIPT
effects of DASH diet on serum lipid profiles of patients with hypertension, cardiovascular
262
disease, metabolic syndrome and type 2 diabetes [21, 23, 40-41]. Our previous study among
263
pregnant women with gestational diabetes mellitus (GDM) has also indicated a significant
264
reduction of serum triglycerides, total cholesterol and LDL-C concentrations following
265
consumption of the DASH eating patternfor4 weeks [22]. Azadbakht et al [21] have shown a
266
significant decrease of serum LDL-C and an increase of HDL-C levels after intervention with the
267
DASH diet intype 2 diabetic patients.Similar findings were also seen with the administration of
268
DASH dietfor8 weeks in patients with the metabolic syndrome [23], for 30 days in subjects with
269
elevated blood pressure [42]and for 8 weeks in hypercholestrolemic patients[43].Several
270
mechanisms can explain the beneficial effects of DASH diet on lipid profiles in PCOS women. In
271
this study, dietary intake of simple sugar in the DASH diet was about half that of the control diet.
272
Furthermore, its fiber content was 1.5-2.0 times higher than that of the control diet. Earlier
273
studies have shown that high-sugar diets might induce mitochondrial dysfunction in adipose
274
tissue, which can in turn lead to metabolic impairment and elevated serum triglycerides levels
275
[44].The DASH diet contain high amounts of arginine-rich foods including fish, soy, beans,
276
lentils, whole grains, and nuts, parsley and fresh basil. The high arginine content of DASH diet
277
might also explain its beneficial effects on insulin resistance and serum triglycerides levels.
278
Decreased serum triglycerides levels following arginine intake have been attributed to shifting
279
nutrient partitioning to promote muscle over fat gain and may in turn provide a useful treatment
280
for improving the metabolic profile [45]. The DASH diet is also a rich source of dietary calcium
281
and magnesium, through which it can affect triglyceride levels. Increased intracellular calcium in
282
liver may stimulate microsomal triglyceride transfer protein (MTP) which is implicated in the
283
formation and secretion of VLDL, and then result in decreased serum triglycerides levels
284
[46].Furthermore, magnesium intake has been associated with lower levels of serum lipids due to
AC C
EP
TE D
M AN U
SC
RI PT
261
12
ACCEPTED MANUSCRIPT
suppressing endothelial injury, reducing the peroxidation of lipids and increasing the antioxidant
286
capacity in serum and tissues [47].
287
The current study revealed that consumption of the DASH diet resulted in a significant increase
288
in plasma TAC and total GSH levels among overweight and obese women with PCOS. Our
289
previous study has indicated that consumption of DASH diet increased plasma TAC and total
290
GSH levels in pregnant women with GDM after 4 weeks[48].Similar findings has also been
291
reported following consumption of the DASH eating pattern in free-living obese hypertensive’s
292
after 4 weeks [49].Adherence to the low-sodium DASH diet in salt-sensitive (SS) subjects has
293
also been resulted in decreased urine F2-isoprostanes, a biomarker of oxidative stress, than a
294
standardized usual low fruit and vegetables diet (ULFV) [50].However, consumption of the
295
DASH eating plan after 3 months led to a non-significant increase in plasma TAC in healthy
296
individuals [51]. Overall, as PCOS is associated with increased oxidative stress [52],
297
consumption of the DASH diet in patients with PCOS could help them control the complications
298
these conditions might led to. The favorable effects of DASH diet on biomarkers of oxidative
299
stress could be attributed to its high content of antioxidant-rich fruit and vegetables [49, 53-54].
300
Individuals in the DASH group received vitamin C nearly 2 times greater than that in the control
301
group. Vitamin C, a major component of TAC, can decrease the NADPH oxidase activity, which
302
is a major superoxide-generating enzyme and increased oxidative stress [55]. High intakes of
303
calcium and magnesium in the DASH diet might also help explain it effects on decreased
304
oxidative stress. Calcium can act as a DNA damage reducing agent [56], which in turn results in
305
the free radical scavenging and increased plasma TAC and total GSH levels. In addition,
306
restoring the activity of anti-oxidative enzymes [57] and scavenging oxygen radicals [58] that
307
results from magnesium intake can provide some reasons for our findings. Finally, the arginine
308
content of DASH diet might also explain its beneficial effects on decreased oxidative stress.
AC C
EP
TE D
M AN U
SC
RI PT
285
13
ACCEPTED MANUSCRIPT
Arginine intake has been shown to reduce serum levels of angiotensin II and measures of
310
oxidative stress [59].
311
Our findings must be interpreted in the context of some limitations. The first limitation is the
312
relatively short duration of intervention. Long-term interventions might result in greater changes
313
in lipid profiles. Second, we could not assess the effects of DASH eating plan on other
314
biochemical indicators of oxidative stress and factors of peroxidation. Further studies are required
315
to examine the effects of DASH diet on other measures of oxidative stress.
316
In conclusion, consumption of DASH eating pattern for 8 weeks among overweight and obese
317
women with PCOS resulted in a significant decrease in weight, BMI, serum insulin, triglycerides
318
and VLDL-C levels as well as a significant increase in plasma TAC and total GSH levels. Given
319
the high prevalence of PCOS and based on the findings of the current study, we believe that the
320
DASH diet could be recommended as a suitable diet for these patients to control abnormal
321
metabolic profiles.
TE D
M AN U
SC
RI PT
309
AC C
EP
322
14
ACCEPTED MANUSCRIPT
Acknowledgment
324
The present study was supported by a grant (no. 9213) from the Vice-chancellor for Research,
325
KUMS, Kashan, Iran. The authors would like to thank the staff of Naghavi and Shaheed Beheshti
326
gynecology Clinics (Kashan, Iran) for their assistance in this project.
327
Clinical trial registration number: www.irct.ir:IRCT201304235623N6.
328
Name of trial registry: Effects of the hypocaloric DASH diet on metabolic parameters,
329
inflammatory factor and biomarkers of oxidative stress in overweight and obese women with
330
polycystic ovary syndrome.
331
Accessed protocol: www.irct.ir:IRCT201304235623N6.
SC
M AN U
AC C
EP
TE D
332
15
RI PT
323
ACCEPTED MANUSCRIPT
333
References
334
[1]
335
with metformin and clomiphene citrate for ovulation induction in women with PCOS. Cochrane
336
Database Syst Rev 2012;10:CD006226.
RI PT
Sinawat S, Buppasiri P, Lumbiganon P, Pattanittum P. Long versus short course treatment
337 338
[2]
Teede HJ, Joham AE, Paul E, Moran LJ, Loxton D, Jolley D, et al. Longitudinal weight
339
gain in women identified With polycystic ovary syndrome: Results of an observational study in
340
young women. Obesity (Silver Spring) 2013; 21:1526-32.
SC
341
[3]
Mehrabian F, Khani B, Kelishadi R, Ghanbari E. The prevalence of polycystic ovary
343
syndrome in Iranian women based on different diagnostic criteria. Endokrynol Pol 2011;62:238-
344
42.
M AN U
342
345
[4]
Wild RA. Dyslipidemia in PCOS. Steroids 2012;77:295-9.
348
[5]
Gonzalez F. Inflammation in Polycystic Ovary Syndrome: underpinning of insulin
349
resistance and ovarian dysfunction. Steroids 2012;77:300-5.
346
TE D
347
350
[6]
352
Front Horm Res 2013;40:40-50.
353
Carmina E. Obesity, adipokines and metabolic syndrome in polycystic ovary syndrome.
EP
351
[7]
355
modulates oxidative stress-induced autophagy in cardiomyocytes. PLoS One 2013;8:e68697.
356
Essick EE, Wilson RM, Pimentel DR, Shimano M, Baid S, Ouchi N, et al. Adiponectin
AC C
354
357
[8]
San Millan JL, Corton M, Villuendas G, Sancho J, Peral B, Escobar-Morreale HF.
358
Association of the polycystic ovary syndrome with genomic variants related to insulin resistance,
359
type 2 diabetes mellitus, and obesity. J Clin Endocrinol Metab 2004;89:2640-6.
360 361
[9]
McGowan MP. Polycystic ovary syndrome: a common endocrine disorder and risk factor
362
for vascular disease. Curr Treat Options Cardiovasc Med 2011;13:289-301.
363
16
ACCEPTED MANUSCRIPT
364
[10]
Fanta M. Is polycystic ovary syndrome, a state of relative estrogen excess, a real risk
365
factor for estrogen-dependant malignancies? Gynecol Endocrinol 2013;29:145-7.
366
[11]
Hudecova M, Jan H, Christian B, Poromaa Inger S. Long-term reproductive and
368
metabolic consequences of PCOS. Curr Diabetes Rev 2012;8:444-51.
369
RI PT
367
[12]
Costello MF, Misso ML, Wong J, Hart R, Rombauts L, Melder A, et al. The treatment of
371
infertility in polycystic ovary syndrome: a brief update. Aust N Z J Obstet Gynaecol
372
2012;52:400-3.
SC
370
373
[13]
Motta AB. The role of obesity in the development of polycystic ovary syndrome. Curr
375
Pharm Des 2012;18:2482-91.
M AN U
374
376 377
[14]
Harwood K, Vuguin P, DiMartino-Nardi J. Current approaches to the diagnosis and
378
treatment of polycystic ovarian syndrome in youth. Horm Res 2007;68:209-17.
379
[15]
Costello MF, Ledger WL. Evidence-based lifestyle and pharmacological management of
381
infertility in women with polycystic ovary syndrome. Womens Health (Lond Engl) 2012;8:277-
382
90.
TE D
380
383
[16]
Galletly C, Moran L, Noakes M, Clifton P, Tomlinson L, Norman R. Psychological
385
benefits of a high-protein, low-carbohydrate diet in obese women with polycystic ovary
386
syndrome--a pilot study. Appetite 2007;49:590-3.
387
AC C
EP
384
388
[17]
Moran LJ, Noakes M, Clifton PM, Tomlinson L, Galletly C, Norman RJ. Dietary
389
composition in restoring reproductive and metabolic physiology in overweight women with
390
polycystic ovary syndrome. J Clin Endocrinol Metab 2003;88:812-9.
391 392
[18]
Herriot AM, Whitcroft S, Jeanes Y. An retrospective audit of patients with polycystic
393
ovary syndrome: the effects of a reduced glycaemic load diet. J Hum Nutr Diet 2008;21:337-45.
394
17
ACCEPTED MANUSCRIPT
395
[19]
Mehrabani HH, Salehpour S, Amiri Z, Farahani SJ, Meyer BJ, Tahbaz F. Beneficial
396
effects of a high-protein, low-glycemic-load hypocaloric diet in overweight and obese women
397
with polycystic ovary syndrome: a randomized controlled intervention study. J Am Coll Nutr
398
2012;31:117-25.
RI PT
399 400
[20]
Vollmer WM, Sacks FM, Ard J, Appel LJ, Bray GA, Simons-Morton DG, et al. Effects of
401
diet and sodium intake on blood pressure: subgroup analysis of the DASH-sodium trial. Ann
402
Intern Med 2001;135:1019-28.
SC
403
[21]
Azadbakht L, Fard NR, Karimi M, Baghaei MH, Surkan PJ, Rahimi M, et al. Effects of
405
the Dietary Approaches to Stop Hypertension (DASH) eating plan on cardiovascular risks among
406
type 2 diabetic patients: a randomized crossover clinical trial. Diabetes Care 2011;34:55-7.
M AN U
404
407 408
[22]
Asemi Z, Tabassi Z, Samimi M, Fahiminejad T, Esmaillzadeh A. Favourable effects of
409
the Dietary Approaches to Stop Hypertension diet on glucose tolerance and lipid profiles in
410
gestational diabetes: a randomised clinical trial. Br J Nutr 2013; 109:2024-30.
TE D
411 412
[23]
Azadbakht L, Mirmiran P, Esmaillzadeh A, Azizi T, Azizi F. Beneficial effects of a
413
Dietary Approaches to Stop Hypertension eating plan on features of the metabolic syndrome.
414
Diabetes Care 2005;28:2823-31.
EP
415
[24]
417
intakes of fat and antioxidant vitamins are predictors of subclinical inflammation in overweight
418
Swiss children. Am J Clin Nutr 2006;84:748-55.
419
Aeberli I, Molinari L, Spinas G, Lehmann R, l'Allemand D, Zimmermann MB. Dietary
AC C
416
420
[25]
Holt EM, Steffen LM, Moran A, Basu S, Steinberger J, Ross JA, et al. Fruit and vegetable
421
consumption and its relation to markers of inflammation and oxidative stress in adolescents. J
422
Am Diet Assoc 2009;109:414-21.
423 424
[26]
King DE, Mainous AG, 3rd, Geesey ME, Ellis T. Magnesium intake and serum C-
425
reactive protein levels in children. Magnes Res 2007;20:32-6. 18
ACCEPTED MANUSCRIPT
426 427
[27]
Luo X, Xu L. [Association of fat distribution with metabolic syndrome in patients with
428
polycystic ovary syndrome]. Nan Fang Yi Ke Da Xue Xue Bao 2012;32:1325-7.
429
[28]
Revised 2003 consensus on diagnostic criteria and long-term health risks related to
431
polycystic ovary syndrome. Fertil Steril 2004;81:19-25.
RI PT
430
432
[29]
Liang SJ, Hsu CS, Tzeng CR, Chen CH, Hsu MI. Clinical and biochemical presentation
434
of polycystic ovary syndrome in women between the ages of 20 and 40. Hum Reprod
435
2011;26:3443-9.
SC
433
437
[30]
438
Care J 2010;1:7-9.
M AN U
436
Dettori J. The random allocation process: two things you need to know. Evid Based Spine
439 440
[31]
American Dietetic Association, Pediatric Weight Management Guideline. The 2005 US
441
Institutes of Medicine "Dietary Reference Intakes for Energy, Carbohydrate, Fiber, Fat, Fatty
442
Acids,
443
http://wwwadaevidencelibrarycom/topiccfm?format_tables=0&cat=3060&auth=1.
Protein,
and
Amino
Acids
(Macronutrients)".
444
[32]
446
"antioxidant power": the FRAP assay. Anal Biochem 1996;239:70-6.
Benzie IF, Strain JJ. The ferric reducing ability of plasma (FRAP) as a measure of
[33]
Beutler E, Gelbart T. Plasma glutathione in health and in patients with malignant disease.
449
J Lab Clin Med 1985;105:581-4.
AC C
448
450
at:
EP
445
447
Available
TE D
Cholesterol,
451
[34]
Saneei P, Hashemipour M, Kelishadi R, Rajaei S, Esmaillzadeh A. Effects of
452
recommendations to follow the Dietary Approaches to Stop Hypertension (DASH) diet v. usual
453
dietary advice on childhood metabolic syndrome: a randomised cross-over clinical trial. Br J Nutr
454
2013. Epub ahead of print; DOI: 10.1017/S0007114513001724.
455
19
ACCEPTED MANUSCRIPT
456
[35]
Lin PH, Yeh WT, Svetkey LP, Chuang SY, Chang YC, Wang C, et al. Dietary intakes
457
consistent with the DASH dietary pattern reduce blood pressure increase with age and risk for
458
stroke in a Chinese population. Asia Pac J Clin Nutr 2013;22:482-91.
459
[36]
Kiddy DS, Hamilton-Fairley D, Seppala M, Koistinen R, James VH, Reed MJ, et al. Diet-
461
induced changes in sex hormone binding globulin and free testosterone in women with normal or
462
polycystic ovaries: correlation with serum insulin and insulin-like growth factor-I. Clin
463
Endocrinol (Oxf) 1989;31:757-63.
RI PT
460
SC
464
[37]
Hamilton-Fairley D, Kiddy D, Anyaoku V, Koistinen R, Seppala M, Franks S. Response
466
of sex hormone binding globulin and insulin-like growth factor binding protein-1 to an oral
467
glucose tolerance test in obese women with polycystic ovary syndrome before and after calorie
468
restriction. Clin Endocrinol (Oxf) 1993;39:363-7.
M AN U
465
469 470
[38]
Atiomo W, Daykin CA. Metabolomic biomarkers in women with polycystic ovary
471
syndrome: a pilot study. Mol Hum Reprod 2012;18:546-53.
TE D
472 473
[39]
Murri M, Luque-Ramirez M, Insenser M, Ojeda-Ojeda M, Escobar-Morreale HF.
474
Circulating markers of oxidative stress and polycystic ovary syndrome (PCOS): a systematic
475
review and meta-analysis. Hum Reprod Update 2013; 19:268-88.
EP
476
[40]
478
syndrome, and other conditions: a review. Nutr Clin Pract 2008;23:142-51.
479
Champagne CM. Magnesium in hypertension, cardiovascular disease, metabolic
AC C
477
480
[41]
Doyle L, Cashman KD. The effect of nutrient profiles of the Dietary Approaches to Stop
481
Hypertension (DASH) diets on blood pressure and bone metabolism and composition in
482
normotensive and hypertensive rats. Br J Nutr 2003;89:713-24.
483 484
[42]
Harsha DW, Sacks FM, Obarzanek E, Svetkey LP, Lin PH, Bray GA, et al. Effect of
485
dietary sodium intake on blood lipids: results from the DASH-sodium trial. Hypertension
486
2004;43:393-8. 20
ACCEPTED MANUSCRIPT
487 488
[43]
Obarzanek E, Sacks FM, Vollmer WM, Bray GA, Miller ER, 3rd, Lin PH, et al. Effects
489
on blood lipids of a blood pressure-lowering diet: the Dietary Approaches to Stop Hypertension
490
(DASH) Trial. Am J Clin Nutr 2001;74:80-9.
RI PT
491 492
[44]
Lomba A, Milagro FI, Garcia-Diaz DF, Campion J, Marzo F, Martinez JA. A high-
493
sucrose isocaloric pair-fed model induces obesity and impairs NDUFB6 gene function in rat
494
adipose tissue. J Nutrigenet Nutrigenomics 2009;2:267-72.
SC
495
[45]
Jobgen W, Meininger CJ, Jobgen SC, Li P, Lee MJ, Smith SB, et al. Dietary L-arginine
497
supplementation reduces white fat gain and enhances skeletal muscle and brown fat masses in
498
diet-induced obese rats. J Nutr 2009;139:230-7.
M AN U
496
499 500
[46]
Cho HJ, Kang HC, Choi SA, Ju YC, Lee HS, Park HJ. The possible role of Ca2+ on the
501
activation of microsomal triglyceride transfer protein in rat hepatocytes. Biol Pharm Bull
502
2005;28:1418-23.
TE D
503 504
[47]
King JL, Miller RJ, Blue JP, Jr., O'Brien WD, Jr., Erdman JW, Jr. Inadequate dietary
505
magnesium intake increases atherosclerotic plaque development in rabbits. Nutr Res
506
2009;29:343-9.
EP
507
[48]
509
clinical trial investigating the effect of DASH diet on insulin resistance, inflammation, and
510
oxidative stress in gestational diabetes. Nutrition 2013;29:619-24.
511
Asemi Z, Samimi M, Tabassi Z, Sabihi SS, Esmaillzadeh A. A randomized controlled
AC C
508
512
[49]
Lopes HF, Martin KL, Nashar K, Morrow JD, Goodfriend TL, Egan BM. DASH diet
513
lowers blood pressure and lipid-induced oxidative stress in obesity. Hypertension 2003;41:422-
514
30.
515
21
ACCEPTED MANUSCRIPT
516
[50]
Al-Solaiman Y, Jesri A, Zhao Y, Morrow JD, Egan BM. Low-Sodium DASH reduces
517
oxidative stress and improves vascular function in salt-sensitive humans. J Hum Hypertens
518
2009;23:826-35.
519
[51]
Miller ER, 3rd, Erlinger TP, Sacks FM, Svetkey LP, Charleston J, Lin PH, et al. A dietary
521
pattern that lowers oxidative stress increases antibodies to oxidized LDL: results from a
522
randomized controlled feeding study. Atherosclerosis 2005;183:175-82.
RI PT
520
523
[52]
De Leo V, La Marca A, Cappelli V, Stendardi A, Focarelli R, Musacchio MC, et al.
525
[Evaluation of the treatment with D-chiroi-nositol on levels of oxidative stress in pcos patients.].
526
Minerva Ginecol 2012;64:531-8.
M AN U
SC
524
527 528
[53]
Avignon A, Hokayem M, Bisbal C, Lambert K. Dietary antioxidants: Do they have a role
529
to play in the ongoing fight against abnormal glucose metabolism? Nutrition 2012;28:715-21.
530
[54]
Puchau B, Zulet MA, de Echavarri AG, Hermsdorff HH, Martinez JA. Dietary total
532
antioxidant capacity is negatively associated with some metabolic syndrome features in healthy
533
young adults. Nutrition 2010;26:534-41.
TE D
531
534
[55]
Chen X, Touyz RM, Park JB, Schiffrin EL. Antioxidant effects of vitamins C and E are
536
associated with altered activation of vascular NADPH oxidase and superoxide dismutase in
537
stroke-prone SHR. Hypertension 2001;38:606-11.
EP
535
538
[56]
Fedirko V, Bostick RM, Long Q, Flanders WD, McCullough ML, Sidelnikov E, et al.
540
Effects of supplemental vitamin D and calcium on oxidative DNA damage marker in normal
541
colorectal mucosa: a randomized clinical trial. Cancer Epidemiol Biomarkers Prev 2010;19:280-
542
91.
AC C
539
543 544
[57]
Yang Y, Gao M, Nie W, Yuan J, Zhang B, Wang Z, et al. Dietary magnesium sulfate
545
supplementation protects heat stress-induced oxidative damage by restoring the activities of anti-
546
oxidative enzymes in broilers. Biol Trace Elem Res 2012;146:53-8. 22
ACCEPTED MANUSCRIPT
547 548
[58]
Hans CP, Chaudhary DP, Bansal DD. Effect of magnesium supplementation on oxidative
549
stress in alloxanic diabetic rats. Magnes Res 2003;16:13-9.
550
[59]
Vasdev S, Gill V. The antihypertensive effect of arginine. Int J Angiol 2008;17:7-22.
RI PT
551 552
AC C
EP
TE D
M AN U
SC
553
23
ACCEPTED MANUSCRIPT
554
Table 1
555
Constituents of the DASH and control diets used in the study٭ DASH diet
Grains †
9
6
Simple sugar
5
Vegetables
2
Fruits
2
Dairy ††
2
Meats, poultry and fish†††
4
Nuts, seeds and legumes
1
Fats and oils
3
556
DASH, Dietary Approaches to Stop Hypertension
557
٭
558
†
559
††
560
†††
SC
3
4 2
3
4 servings from lean meat in the DASH diet and 2 servings in the control diet
TE D EP AC C
567
5
Low-fat (<2%) in the DASH diet
563
566
4
At least 3 servings from whole grains in the DASH diet
562
565
2
Data are presented for a calorie intake of 1700 kcal/day
561
564
RI PT
Control diet
M AN U
Food group
568 569 570
24
ACCEPTED MANUSCRIPT
571
Table 2
572
General characteristics of the study participants٭ DASH diet (n=24) 22.1±3.2
P value†
Height (cm)
161.3±6.0
160.5±4.9
0.60
Weight at study baseline (kg)
74.6±16.2
78.0±12.0
0.41
Weight at end-of-trial (kg)
73.1±15.5
73.6±12.1
0.90
-4.4±2.7
<0.001
30.3±4.5
0.27
BMI at study baseline (kg/m2)
28.6±5.8
BMI at end-of-trial (kg/m2)
28.0±5.7
28.6±4.4
0.74
BMI change (kg/m2)
-0.6±0.9
-1.7±1.1
<0.001
* Data are means ± SD.
575
† Obtained from independent t test.
TE D
574
576
582 583
AC C
581
EP
577
580
M AN U
-1.5±2.6
BMI, Body mass index
579
0.07
Weight change (kg)
573
578
SC
Age (y)
RI PT
Control diet (n=24) 24.7±6.0
584 585 586
25
ACCEPTED MANUSCRIPT
587
Table 3
588
Dietary intakes of study participants throughout the study٭ P value†
DASH diet
(n=24)
(n=24)
Energy (kcal/d)
1887±138
1839±122
0.20
Fat (g/d)
62.9±4.6
61.3±4.0
0.20
Protein (g/d)
84.9±6.2
82.8±5.5
0.20
245.3±17.9
239.1±15.8
0.20
Crude
13.8±1.0
<0.001
Model 1
13.6±0.1
8.8±0.1
<0.001
Crude
11.3±0.8
18.6±1.2
<0.001
Model 1
11.1±0.1
18.8±0.1
<0.001
Crude
185.5±14.6
141.6±20.7
0.001
Model 1
182.3±1.0
144.8±1.0
0.001
Crude
12.1±1.5
17.2±1.3
<0.001
Model 1
11.9±0.2
17.4±0.2
<0.001
Crude
3.5±0.4
4.8±0.4
<0.001
Model 1
3.5±0.1
4.9±0.1
<0.001
Crude
2815.5 ±460.4
1729.8±103.5
<0.001
Model 1
2785.5 ±41.2
1699.1±15.4
<0.001
Crude
3190.4±278.3
4864.4±329.3
<0.001
Model 1
3140.3±29.0
4914.3±29.0
<0.001
PUFA (g/d)
TE D
Cholesterol (mg/d)
Dietary fiber (g/d)
AC C
Insoluble fiber (g/d)
M AN U
8.7±0.6
EP
SFA (g/d)
SC
Carbohydrate (g/d)
RI PT
Control diet
Sodium (mg/d)
Potassium (mg/d)
Magnesium (mg/d)
26
ACCEPTED MANUSCRIPT
Crude
233.1±17.9
411.5±15.2
<0.001
Model 1
230.9±2.3
413.7±2.3
<0.001
Crude
1038.6±42.2
1717.2±36.2
<0.001
Model 1
1032.3±1.7
1724.3±1.7
<0.001
Fruit (servings/day)
2.8±0.4
5.2±0.4
<0.001
Vegetables (servings/day)
2.6±0.5
4.3±0.4
<0.001
Nuts (servings/day)
1.0±0.2
2.5±0.4
<0.001
Fats and oils (servings/day)
3.5±0.5
3.6±0.5
0.40
SC
RI PT
Calcium (mg/d)
DASH, Dietary Approaches to Stop Hypertension; PUFA, Polyunsaturated fats; SFA, Saturated fatty
590
acids
591
* Data are means ± SD.
592
† Obtained from independent t test.
593
Model 1: Adjusted for energy intake (data are means± standard error)
594 595
M AN U
589
.
AC C
EP
TE D
596
27
ACCEPTED MANUSCRIPT
Table 4
P value†
DASH diet (n=24) Wk8
Change
Time
Group
Time x Group
162.8±33.6
-4.2±24.7
0.95
0.33
0.29
166.4±6.2
-3.2±6.2
0.34
0.10
0.45
165.9±6.7
1.2±6.5
0.72
0.33
0.84
109.2±49.7
99.2±45.2٭
-10.0±22.3
0.35
0.93
0.005
112.5±9.9
104.6±11.3
-7.9±7.0
0.18
0.48
0.01
113.5±10.7
107.6±12.1
-5.9±7.5
0.30
0.39
0.07
21.8±9.9
19.8±9.0٭
-2.0±4.5
0.35
0.93
0.005
22.5±2.0
20.9±2.3
-1.6±1.4
0.18
0.48
0.01
3.0±1.5
22.7±2.1
21.5±2.4
-1.2±1.5
0.30
0.39
0.07
46.7±7.9
-0.2±9.9
48.4±9.9
48.2±12.8
-0.2±9.3
0.89
0.59
0.95
46.5±2.3
46.9±2.2
0.4±2.0
48.8±2.3
48.0±2.2
-0.8±2.0
0.20
0.68
0.54
Model 2
46.6±2.5
46.6±2.4
EP
Control diet (n=24)
RI PT
Means (±standard deviation) of serum lipid profiles and biomarkers of oxidative stress at baseline and after the intervention
Wk0
Wk8
Change
Wk0
Crude
153.5±42.0
158.3±31.5
4.8±34.4
167.0±33.7
Model 1
151.0±7.8
154.6±6.2
3.6±6.2
169.6±7.8
Model 2
155.8±8.1
155.1±6.7
-0.7±6.5
164.7±8.1
Crude
93.3±47.9
112.5±67.3٭
19.2±42.8
Model 1
89.9±9.9
107.1±11.3
17.2±7.0
Model 2
88.9±10.7
104.1±12.1
15.2±7.5
Crude
18.6±9.6
22.5±13.5٭
3.9±8.6
Model 1
18.0±2.0
21.4±2.3
3.4±1.4
Model 2
17.8±2.1
20.8±2.4
Crude
46.9±11.8
Model 1
0.0±2.1
48.7±2.5
48.3±2.4
-0.4±2.1
0.18
0.57
0.89
Crude
88.0±30.0
89.0±23.2
1.0±25.9
96.8±30.6
94.8±29.5
-2.0±22.7
0.89
0.65
0.65
Model 1
86.5±6.3
86.3±5.2
-0.2±5.0
98.3±6.3
97.5±5.2
-0.8±5.0
0.19
0.13
0.93
Model 2
91.4±6.4
87.7±5.5
-3.7±5.2
93.3±6.4
96.1±5.5
2.8±5.2
0.48
0.53
0.40
3.4±0.8
3.4±0.7
0.0±0.48
3.6±1.0
3.6±1.1
0.0±0.7
0.67
0.43
0.54
TE D
VLDL-C(mg/dL)
AC C
HDL-C (mg/dL)
LDL-C(mg/dL)
M AN U
Triglycerides (mg/dL)
SC
Total cholesterol(mg/dL)
Total: HDL-C ratio Crude
28
ACCEPTED MANUSCRIPT
Model 1
3.3±0.2
3.4±0.2
0.1±0.1
3.6±0.2
3.7±0.2
0.1±0.1
0.03
0.24
0.99
Model 2
3.4±0.2
3.4±0.2
0.0±0.1
3.6±0.2
3.7±0.2
0.1±0.1
0.14
0.50
0.27
Crude
968.5±233.1
793.7±103.4٭
-174.8±218.0
921.7±226.7
1020.3±301.9٭
98.6±213.7
0.22
0.12
<0.001
Model 1
978.0±47.7
795.7±47.4
-182.3±45.0
912.2±47.7
1018.0±47.4
105.8±45.0
0.27
0.20
<0.001
Model 2
983.7±51.1
795.8±51.2
-187.9±48.5
906.5±51.5
1018.0±51.2
111.5±48.5
0.34
0.29
<0.001
Crude
601.8±267.9
446.2±131.9٭
-155.6±242.8
478.3±195.9
544.7±220.2
66.4±279.0
0.24
0.79
0.005
Model 1
586.8±47.9
445.0±38.1
-141.8±53.9
493.4±47.8
545.9±38.1
52.5±53.9
0.27
0.93
0.01
Model 2
566.0±50.9
442.7±41.2
-123.3±57.6
514.1±50.9
548.2±41.2
34.1±57.6
0.44
0.63
0.07
RI PT
TAC (mmol/L)
M AN U
SC
GSH (µmol/L)
DASH, Dietary Approaches to Stop Hypertension; FPG, Fasting plasma glucose; GSH, Total glutathione; HOMA-IR, Homeostasis Model of Assessment-Insulin Resistance; HDL-C, High density lipoprotein-cholesterol; hs-CRP, High-sensitivity C-reactive protein; LDL-C, Low density lipoprotein-cholesterol; TAC, total antioxidant capacity; VLDL-C, Very low density lipoprotein-cholesterol ٭Different from wk 0, P < 0.05with paired samples t test. Model 1: Adjusted for age (data are means± standard error)
TE D
†Obtained from repeated measures ANOVA test.
AC C
EP
Model 2: Adjusted for Model 1+ weight change (data are means± standard error)
29
ACCEPTED MANUSCRIPT
Assessed for screening (n=150)
Lost to follow-up (n=3)
M AN U
Allocated to control (n=27)
Allocated to intervention (n=27)
Lost to follow-up (n=3)
♦ IVF treatment (n=1) ♦ Health problems (n=1) ♦ The use of medications (n=1)
Analyzed (n=24)
Analyzed (n=24)
EP
TE D
♦ IVF treatment (n=1) ♦ Became pregnant (n=1) ♦ The use of medications (n=1)
AC C
Analysis
Follow-up
Allocation
Randomized (n=54)
SC
RI PT
Enrollment
Excluded (n=96) ♦ Not living in Kashan (n=24) ♦ Taking excluded medications (n=17) ♦ Within normal weight range (n=15) ♦ Outside the age range required (n=14) ♦ Unable to commit to study (n=12) ♦ Excluded health condition (n=6) ♦ Not diagnosed with PCOS (n=4) ♦ Recent weight loss (n=4)
Fig. 1.Summary of patient flow
IVF, In vitro fertilisation; PCOS, Polycystic ovary syndrome
30