Omega-3 polyunsaturated fatty acid supplementation versus placebo on vascular health, glycaemic control, and metabolic parameters in people with type 1 diabetes: a randomised controlled preliminary trial

Background The role of omega-3 polyunsaturated fatty acids (n-3PUFA), and the potential impact of n-3PUFA supplementation, in the treatment and management of type 1 diabetes (T1D) remains unclear and controversial. Therefore, this study aimed to examine the efficacy of daily high-dose-bolus n-3PUFA supplementation on vascular health, glycaemic control, and metabolic parameters in subjects with T1D. Methods Twenty-seven adults with T1D were recruited to a 6-month randomised, double-blind, placebo-controlled trial. Subjects received either 3.3 g/day of encapsulated n-3PUFA or encapsulated 3.0 g/day corn oil placebo (PLA) for 6-months, with follow-up at 9-months after 3-month washout. Erythrocyte fatty acid composition was determined via gas chromatography. Endpoints included inflammation-associated endothelial biomarkers (vascular cell adhesion molecule-1 [VCAM-1], intercellular adhesion molecule-1 [ICAM-1], E-selectin, P-selectin, pentraxin-3, vascular endothelial growth factor [VEGF]), and their mediator tumor necrosis factor alpha [TNFα] analysed via immunoassay, vascular structure (carotid intima-media thickness [CIMT]) and function (brachial artery flow mediated dilation [FMD]) determined via ultrasound technique, blood pressure, glycosylated haemoglobin (HbA1c), fasting plasma glucose (FPG), and postprandial metabolism. Results Twenty subjects completed the trial in full. In the n-3PUFA group, the mean ± SD baseline n-3PUFA index of 4.93 ± 0.94% increased to 7.67 ± 1.86% (P < 0.001) after 3-months, and 8.29 ± 1.45% (P < 0.001) after 6-months. Total exposure to n-3PUFA over the 6-months (area under the curve) was 14.27 ± 3.05% per month under n-3PUFA, and 9.11 ± 2.74% per month under PLA (P < 0.001). VCAM-1, ICAM-1, E-selectin, P-selectin, pentraxin-3, VEGF, TNFα, CIMT, FMD, blood pressure, HbA1c, FPG, and postprandial metabolism did not differ between or within groups after treatment (P > 0.05). Conclusions This study indicates that daily high-dose-bolus of n-3PUFA supplementation for 6-months does not improve vascular health, glucose homeostasis, or metabolic parameters in subjects with T1D. The findings from this preliminary RCT do not support the use of therapeutic n-3PUFA supplementation in the treatment and management of T1D and its associated complications. Trial Registration ISRCTN, ISRCTN40811115. Registered 27 June 2017, http://www.isrctn.com/ISRCTN40811115.


Background
The role of omega-3 polyunsaturated fatty acids (n-3PUFA), and the potential impact of n-3PUFA supplementation, in the treatment and management of diabetes remains unclear and controversial. Cross-sectional epidemiological studies suggest that inadequate n-3PUFA intake is associated with an increased risk of developing both type 2 diabetes (T2D) [1] and type 1 diabetes (T1D) [2]. However, a recent meta-analysis of randomised controlled trials (RCTs) concluded that n-3PUFA supplementation has little effect on the prevention of T2D in humans [3], and evidence for preventing T1D remains preliminary and limited to animal studies [4]. In murine models, research has shown that increased n-3PUFA intake reduces the risk of microvascular complications in vivo [5], and some studies [6,7], although not all [8], have shown n-3PUFA supplementation improves biomarkers of vascular health and metabolic parameters in people with T2D [9,10]. However, RCTs investigating n-3PUFA supplementation in T2D have failed to show reductions in major vascular events [11].
Dietary recommendations for people with and without diabetes currently advocate increased consumption of foods rich in n-3PUFA but do not recommend n-3PUFA supplementation [12]. However, the evidence underpinning these recommendations for people with diabetes is limited exclusively to people with T2D as very few RCTs have examined the impact of n-3PUFA supplementation on vascular or metabolic outcomes in T1D [13][14][15][16][17][18]. Further, most RCTs in T1D are confounded by short duration supplementation, low n-3PUFA dose, and failure to control for pretreatment fatty acid profile status. Therefore, the objective of this study was to investigate the efficacy of high-dose-bolus n-3PUFA supplementation on vascular health, glycaemic control, and metabolic parameters in adults with T1D.

Methods
We performed a single-centre, parallel-group, doubleblind, randomised, placebo-controlled trial in subjects with T1D, testing the efficacy of 6-months high-dosebolus n-3PUFA supplementation on vascular health, glycaemic control, and metabolic parameters. Outcome assessments and safety outcomes were recorded at baseline, and after 3-and 6-months, with further assessment at 9-months following a subsequent 3-month washout (Additional file 1: Fig. S1). This trial was prospectively registered at the International Clinical Trials Registry Platform (ID: ISRCTN40811115), and ethical approval was granted by the local National Health Service Research Ethics Committee (17/NE/0244). In June 2018 a substantial ethics amendment was approved to increase the pool of available study participants. The amendment served to modify the inclusion criteria from "Not taking any prescribed medication other than insulin" to "Not taking any medication known to interact with n-3PUFA supplementation". All subjects provided written informed consent before participating in the trial. Recruitment took place from September 2017-January 2019.
Twenty-seven adults aged 18-65 years with a diagnosis of T1D (glycosylated haemoglobin [HbA1c]: < 11% [97 mmol/mol]) > 2 years on enrolment and free from diabetes-related complications were eligible for inclusion. Exclusion criteria included any significant medical conditions including hepatic or haematological abnormalities, compromised glycaemic control (HbA1c > 11% (97 mmol/mol), current or previous pregnancy within the last 12-months or planning to become pregnant within 12-months, and taking any medication known to interact with n-3PUFA. All subjects were treated with a stable basal-bolus insulin regimen using either continuous subcutaneous insulin infusion (n = 9) or multiple daily injection (n = 11) therapy. Subjects following continuous subcutaneous insulin infusion therapy used insulins Aspart (n = 6) or Lispro (n = 3). For multiple daily injection therapy the basal component consisted of insulins Glargine (n = 5), Degludec (n = 2), Detemir (n = 3), or Isophane (n = 1) and the bolus component consisted of rapid-acting insulins Aspart (n = 8), Lispro (n = 2), or Glulisine (n = 1). Subjects were required to maintain their usual dietary habits and existing use of multivitamins throughout the duration of the study.
Following study enrolment, subjects were randomly assigned to treatment with n-3PUFA or placebo (PLA) in a 1:1 allocation ratio. Randomisation was conducted via the Minimization Program for allocating patients to clinical trials [19]; this algorithm ensures a balanced allocation of subjects across both groups for prognostic factors (i.e. age, BMI, diabetes duration). Randomization and safety monitoring as well as study drug labelling and dispensing were completed by staff not involved in recruitment or testing procedures. All subjects, clinical investigators, and outcome assessors were blinded to treatment allocation.
Subjects randomised to n-3PUFA supplementation ingested a daily high-dose-bolus of encapsulated 3.3 g/ day (2.3 g EPA and 0.8 g DHA) (OmegaVia fish oil, OmegaVia, Calabasas, USA) over a 6-month period, whereas the placebo group ingested an encapsulated dose of 3.0 g/day corn oil (Pure corn oil, Mazola, Liverpool, UK). Capsules were aesthetically identical and dispensed in sealed pharmaceutical bottles. Monthly emails were sent individually to ensure compliance and monitor adverse effects. Subjects were instructed to retain packaging and informed that compliance would be objectively assessed through periodic blood analysis. On each laboratory visit, upper gastrointestinal symptoms (reflux, abdominal pain, and indigestion) were assessed via a self-administered validated questionnaire [20].
Subjects attended four separate but identical morningtime laboratory visits at baseline, 3-months, 6-months, and 9-months. Subjects refrained from caffeine, alcohol, and vigorous physical activity in the 48-h prior to each laboratory visit, in addition to adopting an overnight fast. During each visit, resting blood samples were obtained to analyse vascular and metabolic biomarkers. Vascular structure and function were assessed via ultrasound. Anthropometric measures (weight, body mass index, percentage body fat) were obtained via bioelectrical impedance analysis (SC-331S, Tanita, Amsterdam, Netherlands), and blood pressure was assessed via an automated oscillometric device (Intellisense HEM-907XL, Omron, Kyoto, Japan). In addition, subjects completed two subsequent mixed-meal tolerance tests to assess the potential impact of n-3PUFA supplementation on postprandial metabolism (see Additional file 1: Fig. S1 and Table S1).
On arrival to the laboratory, a 22-gauge cannula (Vasofix, B.Braun, Melsungen AG, Germany) was inserted into the antecubital vein of the non-dominant arm which was kept patent for periodic blood draws. Following initial measures (anthropometry and vascular assessment), subjects completed a meal-tolerance test (see Additional file 1: Table S1). At 4-h post-breakfast, subjects completed a second meal-tolerance test (see Additional file 1: Table S1) followed by a 4-h observation window. Subjects were instructed to consume each meal within a 20-min window and were permitted water intake ad libitum, for which quantity was recorded. Blood draws were made throughout the meal tolerance tests at 30-min intervals.
Venous blood samples were collected using 3 mL EDTA vacutainers and 6 mL lithium-heparin vacutainers (BD, New Jersey, USA). Fasting whole blood samples from each visit were analysed for HbA1c and erythrocyte fatty acid composition (Omegametrix GmbH laboratory, Planegg, Germany) via gas chromatography by methods described previously [21]; erythrocyte fatty acid composition was determined to establish baseline fatty acid status and was used as an objective measure of compliance to the intervention. The n-3PUFA index (O3I) was calculated as eicosapentaenoic acid plus docosahexaenoic acid. The remaining blood sample was centrifuged at 2700×g for 10 min at 4 °C and the resultant plasma was subsequently stored at − 80 °C for retrospective analysis of vascular biomarkers and metabolic parameters. A customised 7-plex human fluid-phase magnetic immunoassay (R&D Systems, Minneapolis, USA) was used for the simultaneous detection and quantification of vascular cell adhesion molecule-1 (VCAM-1), intercellular adhesion molecule-1 (ICAM-1), E-selectin, P-selectin, pentraxin-3, vascular endothelial growth factor (VEGF), and tumor necrosis factor alpha (TNFα) as per the manufacturer's instructions. All vascular biomarker data were collected on a Luminex ® 200 ™ cytometer (Luminex, Texas, USA) and analysed using specialised software (Bio-Plex Manager 6.1, Bio-Rad, California, USA). In addition, fasting plasma glucose (FPG), triglycerides, cholesterol, and non-esterified fatty acids (NEFA) were quantified via an enzymatic colorimetric assay using a fully automated random-access analyser (Randox Daytona Plus, Randox Laboratories, UK). Further blood draws were made at 30-min intervals for the duration of the 8-h laboratory stay to capture postprandial glucose (PPGR) and triglyceride (PPTR) responses to each meal tolerance test; the trapezoidal rule was used to calculate individual areas under the plasma concentration curves (AUC); data is presented as sum AUC (0-8 h) for two consecutive mixed-meal tolerance tests. The intra-assay coefficient of variation was < 5% for all biochemical analyses.
Non-invasive high-resolution B-mode ultrasound imaging (GE Healthcare, Vivid I BT 12 EMEA, Illinois, USA) was performed using a GE 9L linear array ultrasound transducer probe (GE Healthcare, 12L-RS Linear Probe, Illinois, USA), to assess carotid-artery intimamedia thickness (CIMT) and brachial artery flow mediated dilation (FMD) via previously described methods [22,23]. Independently validated edge detection software (Vascular Research Tools 6, Medical Imaging Application, LLC, Iowa, USA) was used for offline analysis of all ultrasound images.

Sample size and statistical analysis
Sample size for this study was estimated on the basis of prior work in T1D with shared similarities as well as published meal tolerance data [24][25][26]. Priori power calculations estimated a sample size of n = 16 in each arm would provide 80% power with α set at 0.05 to detect a small effect (d = 0.25) in the change variables for primary and secondary outcomes, namely: VCAM-1, E selectin, P-selectin, TNFα, pentraxin-3, ICAM-1, VEGF, HbA1c, triglycerides, PPGR, and PPGT [27]. On completion of the study, we used the realised sample size (20 subjects rather than 32) and standard error to calculate post hoc power for the observed estimates. Post-hoc power analysis on the attained sample size calculated the estimated power to be: > 99% for VCAM-1, E selectin, P-selectin, TNFα, pentraxin-3, FMD, CIMT, HbA1c, and triglycerides; 98% and 94% for PPTR and PPGR, respectively; 89% for ICAM-1; and 64% for VEGF.
Statistical analysis was performed using SPSS (Version 26, IBM, Illinois, USA). Primary analysis was per protocol and performed using a general linear mixed model repeated-measures analysis of variance. Secondary analysis was performed as intention to treat with last observation carried forward. The within-groups factor was time with treatment allocation as the between-groups factor. Pairwise comparisons were used to investigate significant interactions adjusted using a Bonferroni correction. Statistical models were further adjusted to include pretreatment fatty-acid exposure, and age, gender, age of diagnosis, duration of disease, and mode of insulin therapy as prognostic markers. Total exposure to n-3PUFA during the study period was calculated as the individual areas under the plasma concentration curves derived from the measurements at baseline and after 3-months, 6-months, and 9-months by using the trapezoidal rule. Statistical significance was set at P ≤ 0.05. Data are presented mean ± SD.

Study recruitment and follow-up
We screened 218 subjects randomly allocating a total of 27 to treatment with n-3PUFA (n = 14) or PLA (n = 13) (Fig. 1). The main exclusion criteria were either significant medical conditions (42%) or pre-existing selfadministration of n-3PUFA supplementation (25%). One subject was removed from the study shortly following baseline laboratory analysis due to elevated pretreatment HbA1c. Six subjects were lost to follow-up, and therefore 20 subjects completed the study in full (n-3PUFA, n = 10; PLA, n = 10). Subject demographic and pretreatment clinical characteristics are shown in Table 1.

Outcomes
No significant differences were found between n-3PUFA and PLA groups in vascular, glycaemic, or metabolic endpoints ( Table 2). The change in inflammatory-associated vascular endothelial proteins (VCAM-1, ICAM-1, VEGF, E-selectin, P-selectin, pentraxin-3) and TNFα measured as the difference between baseline and 6-months showed no significant differences between n-3PUFA and PLA (Table 2). Similarly, CIMT and FMD, as well as blood pressure remained unchanged in both n-3PUFA and PLA groups (P > 0.05; Table 2). The change in glycaemic control, measured as HbA1c, FPG, and PPGR, did not differ between groups; no within-group changes during treatment were found (P > 0.05; Table 2). Fasting cholesterol, NEFA, and triglyceride levels, as well as PPTR, remained unchanged and were not different within or between groups (P > 0.05; Table 2). Likewise, body weight, body mass index, and percentage body fat remained similar between the two treatment groups throughout the study (P > 0.05; Table 2). No changes in insulin requirements were observed with basal and bolus insulin doses remaining unchanged within each group. Bolus insulin administration was maintained for all mixed-meal tolerance tests across all four visits (n-3PUFA: 9.27 ± 3.00 IU; PLA: 8.04 ± 4.19 IU).
Adjustment for pretreatment fatty acid composition, age, gender, age of T1D diagnosis, duration of diabetes, or mode of insulin therapy did not impact outcomes (Additional file 1: Table S3). Intention-to-treat analyses on the basis of last observation carried forward did not significantly alter outcomes (Additional file 1: Table S5).

Safety
Overall, no important safety issues occurred during n-3PUFA supplementation. The mean severity of gastrointestinal side effects assessed did not significantly differ over time for either treatment condition. The reported severity of gastrointestinal symptoms changed from no symptoms to mild during the 6-month supplementation period in seven subjects (n-3PUFA: n = 2; PLA: n = 5), whereas symptoms changed from mild to moderate in five subjects (n-3PUFA: n = 3; PLA: n = 2).

Discussion
In this RCT of n-3PUFA versus placebo in subjects with T1D, daily high-dose-bolus n-3PUFA supplementation for 6-months did not improve vascular health, glycaemic control, or metabolic parameters in subjects with T1D. These findings have important clinical implications concerning dietary recommendations and nutritional guidance for people with T1D. Specifically, our findings question the efficacy of n-3PUFA supplementation for the treatment and management of T1D and its associated complications. Our data support previous studies conducted in T2D patients [28][29][30][31][32] and provide new insight within the context of T1D [13][14][15][16][17][18]. This is the first study to comprehensively assess the impact of n-3PUFA supplementation on vascular health in subjects with T1D. We have previously shown that inflammation and vascular markers are raised in people with T1D, even in those with good metabolic control [26,33]. The pretreatment inflammatory cytokine and endothelial cell adhesion molecule concentrations of patients in the present study, appear elevated compared to previously published data in T1D [26,34]. Such differences may be due to differences in clinical characteristics (i.e. age, BMI, and diabetes duration) between study populations and indicates increased endothelial activation our patients. It is widely recognised that vascular adhesion molecules play an important pathophysiological role in atherosclerosis [35], and are upregulated early into the progression of microvascular complications in subjects with T1D [36]. n-3PUFAs have previous been shown to attenuate the expression of adhesion molecules and vascular inflammation in human endothelial cells in vitro [9,10,37]. Additionally, the metabolism of n-3PUFA: (i) modulates macrophage functions [38], (ii) produces bioactive metabolites which possess anti-inflammatory properties [39], and (iii) reduces atherogenesis and platelet aggregation [40]. A high n-6PUFA:n-3PUFA ratio has also been associated with increased systemic inflammation in T2D [41]. Therefore, it is plausible to speculate that similar improvements in vascular inflammation would be observed in people with T1D following n-3PUFA supplementation. Notably, however, no significant improvements were detected in vascular adhesion molecules or their mediator TNFα in the present study. In addition, we found no effect of n-3PUFA supplementation on CIMT, FMD, or blood pressure. Previous research investigating n-3PUFA supplementation in T2D has reported conflicting results regarding CIMT [32,42] and blood pressure responses [6,43].
Further, we report for the first time, the impact of n-3PUFA supplementation on postprandial metabolism. Postprandial metabolic handling is a strong and independent predictor of cardiovascular disease [44,45] and a critical component of T1D self-management. We show that a daily high-dose-bolus of n-3PUFAs does not modulate postprandial glycemia or lipemia. Additionally, it was found n-3PUFA supplementation does not improve long-term glycaemic control or metabolic parameters. Prior research investigating the utility of n-3PUFAs in T1D has shown both improvements [18] and no change on glucose homeostasis [13,14,17]. The beneficial effects of n-3PUFAs on fasting triglycerides are well documented in T2D [46]. Although not statistically significant, we observed a numerical reduction in fasting triglyceride levels in the n-3PUFA arm at 3-months and 6-months that was restored following washout. In our study, changes in fasting triglycerides from 3 to 9 months in the PLA group may have masked a statistically significant effect in the n-3PUFA group. Although speculative, one potential mechanism for triglyceride reduction is decreased secretion of inflammatory cytokines, which reduces hepatic very low-density lipoprotein synthesis and accelerates chylomicron clearance [47,48]. Considering our chosen inflammatory biomarkers, particularly TNFα, remained unchanged, this could, in part, explain why triglyceride levels in our participants remained statistically unchanged. Although, reductions in fasting triglyceride levels have been shown in response to n-3PUFAs independent of baseline triglyceride values, higher reductions in triglycerides are observed when baseline triglycerides are elevated [49][50][51]. Further, the

Table 1 Pretreatment demographic and clinical characteristics of study subjects included in final analysis
Data presented as mean ± SD. n-3PUFA compared to placebo. Independent samples t tests were performed on metric variables a ; Fisher exact tests performed on categorical variables b . n-3PUFA, omega-3 polyunsaturated fatty acid. Omega-3 index calculated as eicosapentaenoic acid plus docosahexaenoic acid. A, Aspart; D, Detemir; DG, Degludec; G, Glargine; GL, Glulisine; I, Isophane; L, Lispro  with triglyceride levels < 1.0 mmol/L at study entry. Thus, we cannot exclude the possibility that n-3PUFA supplementation over a longer duration or in less well-controlled subjects (± comorbidities) may have nongenomic effects on glycaemic control, metabolic health or vascular health, that were not detectable in our cohort or by our study design. Whilst we administered n-3PUFA at a dose above the 2 g/day minimum suggested necessary to elicit beneficial cardiovascular effects [52], the current study focused on the additive effects of n-3PUFA to habitual dietary habits given the known poor adherence to chronic dietary changes [53]. However, research suggests that n-3PUFA supplementation alone is insufficient and needs to replace saturated fatty acid intake in order to modify CVD risk [54]. While increased n-3PUFA intake may reduce the risk of developing T1D [55], the current study questions the therapeutic utility and disease modifying potential of n-3PUFA in adults with T1D.

Strengths and limitations
Although the strengths of this study include its doubleblind randomised placebo-controlled design; long supplementation duration and daily high dose of n-3PUFA; assessment of legacy effects and follow-up after washout; objective assessment of compliance via erythrocyte gas chromatography; the inclusion of a broad and comprehensive assessment of outcomes using gold-standard measures; and control of pretreatment fatty acid composition and subject characteristics it is not without limitations. Firstly, the broad selection of subjects with different treatment regimens, duration of disease, and sex may have caused heterogeneity in the study sample and may have masked a positive effect. However, controlling for these potentially confounding factors in our statistical analysis did not change the outcome of study findings and increases generalizability. The obtained sample size was relatively small and the number of subjects lost to follow up was proportionately high. However, our sample size was deemed sufficient to yield adequate statistical power across outcomes, and is comparable to previously published RCTs assessing the effectiveness of n-3PUFA supplementation in adults with T1D [14,18].

Conclusions
This study indicates that daily high-dose-bolus n-3PUFA supplementation for 6-months does not improve vascular health, glucose homeostasis, or metabolic parameters in well controlled subjects with T1D without existing microvascular complications. Despite the lack of evidence to support clinical benefit, n-3PUFA supplementation is common in people living with T1D. However, the findings from this preliminary RCT do not support the use of therapeutic n-3PUFA supplementation in the treatment and management of T1D and its associated complications. Future research is needed to assess the effectiveness of other potential adjunct therapies that may act to modify the markedly elevated CVD risk amongst adults with T1D.