Subjects

Patients with type 2 diabetes were recruited primarily by local advertisements. Ninety-six subjects participated in the study (Fig. 1). Inclusion criteria were type 2 diabetes, age 30–65 years, diabetes duration of ≤15 years, HbA₁c ≤ 8 %, BMI ≥22 and <35 kg/m², not taking insulin or α-glucosidase inhibitors, stable weight (±3 kg) during the past 3 months and not being on weight-loss or vegan diet. Subjects with hepatic, cardiac, renal, thyroid, respiratory, gastrointestinal and eating disorders were not included. Exclusion criteria were poor compliance to the prescribed diet or change in medications use throughout the study.

Fig. 1. Flow chart of the study participants. HC, high-carbohydrate evening meal; ST, standard evening meal; HP, high-protein evening meal; ITT, intention-to-treat; PP, per-protocol.

Study design and procedure

This is a 10-week single-blinded, parallel, randomised controlled trial with dietary intervention. The primary outcome of the current study was glycated Hb (HbA₁c), while the secondary outcomes were fasting blood glucose (FBG), insulin resistance, lipid profile, anthropometric measurements and blood pressure. The study procedure was described to all volunteers. However, the participants were not aware of the type of diet they were assigned to and the differences between them (single-blinded). A questionnaire with demographic questions was completed. The participants’ dietary habits and their medical history were also recorded. This study was conducted according to the guidelines laid down in the Declaration of Helsinki, and all procedures involving human subjects were approved by the Ethics Committee of Shiraz University of Medical Sciences (no. IR.SUMS.REC.1396.7) and registered in the Iranian Registry of Clinical Trials (no. IRCT2017042733666N1). Written informed consent was obtained from all participants.

There was a 2-week run-in period at the beginning of the study (weeks –2 to 0). Throughout this period, the participants were advised to maintain their usual diet and physical activity and refrain from unusual physical activity or diet such as fasting. They were also asked to keep a 3-d food record (two weekdays and one weekend day). After the run-in period, applying block randomisation, the participants were randomly assigned to either of the following three groups: standard evening meal (ST), high-carbohydrate evening meal (HC) and high-protein evening meal (HP). The participants were followed for 10 weeks, during which they visited the specially designated clinic at weeks 2, 5 and 10. Anthropometric indices and blood pressure were monitored at weeks 0, 5 and 10, except for body weight that was measured at all sessions. Blood tests were performed at the beginning and the end of the study, except for FBG which was also measured at weeks 2 (optional) and 5. Physical activity was measured using a validated International Physical Activity Questionnaire^{(Reference Criniere, Lhommet and Caille17,Reference Moghaddam, Aghdam and Jafarabadi18)} . Patients were advised not to change their physical activity level and smoking habits throughout the study and were not advised to keep on smoking throughout this period.

Diets

All participants received a balanced diet including 15–20 % protein, 50–55 % carbohydrate and 25–30 % fat. Total energy expenditure of each subject was calculated using the Institute of Medicine equations⁽¹⁹⁾. Exchange lists for Meal Planning⁽²⁰⁾ were provided for all subjects, and they were instructed how to substitute foods in their diets according to the exchange lists. Furthermore, they received dietary recommendations according to the American Diabetes Association guidelines (online Supplementary material)^{(Reference Evert, Boucher and Cypress21)}. The only difference between the three prescribed diets was the distribution of protein and carbohydrate among meals. In the ST group, protein and carbohydrate were rather evenly distributed among the meals. In the HC group, 40–45 % of the total carbohydrate intake was provided at dinner and evening snack. In the HP group, 40–45 % of the total protein intake was at dinner and evening snack (online Supplementary material). It is worth noticing that in Iranian dietary culture, lunch is the main meal of the day and dinner is predominantly light. One of our major concerns about experimenting carbohydrate–protein redistribution diet was the rate of compliance and durability of the diet. In other words, more extreme changes in the proportions of carbohydrate or protein in the evening would probably reduce the participants’ compliance dramatically. Therefore, we designed diets with a practical proportion of macronutrients which could be willingly followed by the patients during the study and in the long-term if it turns out to be beneficial. In order to prevent high energy intake in the evening, we reduced the protein and fat intake in the HC dinner. For the same reason, carbohydrate and fat intake in the HP dinner was decreased.

All dietary interventions were made by the nutritionist. At each visit, dietary consultation was made and the subjects were persuaded to follow their prescribed diet. In addition, phone calls were made if necessary. Participants were asked to fill 3-d food records (two weekdays and one weekend day) at weeks 2, 5 and 10. Nutritionist IV software (version 3.5.2 1994; N-Squared Computing) was used to assess dietary intake and compliance. At each visit, the participants were asked to rate their compliance to the diet in the preceding weeks from 1 to 5, with one meaning non-compliance to the diet and five meaning complete compliance to the diet. At the final visit, the participants were asked to rate their satisfaction with their prescribed diet from 1 to 5, with one meaning completely unsatisfied and five meaning completely satisfied.

Anthropometric and blood pressure measurements

Height was measured without shoes by means of a wall-mounted stadiometer to the nearest 0·5 cm. Body weight and body composition (percentage body fat mass, soft lean mass) were measured by a body composition analyzer (Easy Body 205, Jawon Medical). Weight was measured in light clothing without shoes to the nearest 100 g. BMI was calculated dividing weight (kg) by height (m) squared. Body composition was assessed using the bioelectrical impedance analysis technique. Since dehydration affects the accuracy of body composition analysis, participants were asked to drink enough water and avoid high-caffeine foods or beverages the days before the measurement. In addition, they were asked to refrain from physical activity 12 h and food consumption 2 h before the analysis. Measurement was performed with minimal clothes without socks, jewellery, belt and watch and after emptying the bladder. Waist circumference was measured by a non-stretch fibre glass tape measure to the nearest 0·1 cm at the top of the iliac crest. Blood pressure was obtained in the right arm after at least 5 min of rest using a mercury sphygmomanometer (ALPK2) in a sitting position. Blood pressure was measured twice with at least 1 min interval, and the average of the two measurements was used for analysis.

Laboratory measurements

Blood samples were drawn after 12-h fasting. HbA₁c was measured by the boronate affinity HPLC method. Blood samples were centrifuged. FBG, TAG, total cholesterol (TC), HDL-cholesterol and LDL-cholesterol were measured by the enzymatic colorimetric method using assay kits (Pars Azmun) on autoanalyzer BT 1500 (Biotecnica Instruments S.p.A.). VLDL-cholesterol was calculated using Friedewald equation. Non-HDL-cholesterol and non-HDL-cholesterol:HDL-cholesterol were also computed. Insulin was measured by ELISA kit (Monobind Inc.). Homoeostasis model assessment of insulin resistance (HOMA-IR) and β-cell function (HOMA-β) were calculated by Matthews et al.’s formula as follows:

$${\rm{HOMA \hbox- IR}} = {\rm{fasting\ glucose}}\left( {{\rm{mg/dl}}} \right) \times {\rm{fasting\,insulin}}\ \left( {{\rm{\mu U/ml}}} \right){\rm{/405}}$$

$${\rm{HOMA \hbox- }}\beta = {\rm{360}} \times {\rm{fasting\ insulin/}}\left( {{\rm{fasting \ glucose }}\,\left( {{\rm{mg/dl}}} \right) - {\rm{63}}} \right)$$

Statistical analysis

With regard to the distribution of the primary outcome (HbA₁c) in the study population which was determined by reading routine test results of diabetic patients at the time of registration (mean 6·50, sd 0·79), and the Clinically Meaningful Effect Size of 0·60 unit reduction in the level of HbA₁c determined by a consultant endocrinologist and setting α value at 0·05 and statistical power at 80 %, a sample size of twenty-eight in each group was estimated to be adequate (calculated using G*Power software). More participants were allocated to the reference category (the group with standard diet, n 36) to increase the power of statistical tests. In addition, thirty-one participants were allocated to each of the HC and HP groups. In the HP group, two participants withdrew before starting the diet (n 29). Results were expressed as mean and standard deviation or number (percentages). Baseline characteristics of the study participants were compared using either a one-way ANOVA for quantitative variables or χ ² for qualitative variables. Paired t test was used for testing within-group changes. Due to a marginally significant difference in age between the study groups, generalised linear (GLM repeated measures) models were fitted using age and change in energy intake due to the interventions, and the study groups as independent variables and the values of outcome variables as the dependent variable. In case of significant difference among the intervention groups, Tukey’s multiple comparison test was used to define the effects of which diets are different. A test with P value <0·05 was considered statistically significant. SPSS version 19 (SPSS Inc.) was used for analysis. The analysis was conducted using the intention-to-treat (ITT) approach. In that regard, the latest values of the outcome variables of the dropout participants were used for analysis. We also performed the per-protocol (PP) analysis to see what potential differences are between these two approaches of analysis.