Malnutrition impairs mitochondrial function and leukocyte activation

The participants in this cross-sectional study consisted of outpatients attending the Endocrinology and Nutrition Service of the University Hospital Dr. Peset in Valencia (Spain) between January 2015 and December 2017.

Subjects aged 18 or older were eligible for inclusion in the study. Exclusion criteria were pregnancy or lactation, severe renal (chronic kidney disease in stage ≥4 and glomerular filtration rate < 30 mL/min) or severe hepatic disease (Child-pugh B or C), and previous monitoring by the Nutrition Unit. Patients were categorized based on the recent diagnostic consensus of malnutrition, employing the following etiology- based terminology: malnutrition without inflammation or DRM-I (starvation-related malnutrition); patients with anorexia; mechanic or neurologic dysphagia, in which inflammation was not the main cause of malnutrition; malnutrition with inflammation or DRM + I; and patients with chronic disease-related malnutrition and acute disease or injury-related malnutrition, specifically neoplasm, inflammatory bowel disease or chronic obstructive pulmonary disease (COPD), in which the disease and the chronic underlying inflammation played an active role in their nutritional status [18].

The study was conducted according to the ethical principles stated in the Declaration of Helsinki, and all procedures were approved by our hospital’s Ethics Committee. Written informed consent was obtained from all subjects.

A complete nutritional assessment was performed to evaluate the nutritional status of the subjects according to ASPEN criteria [4]. DRM was diagnosed when at least two of the following characteristics were confirmed: insufficient energy intake; weight loss; loss of muscle mass (wasting of the temples, clavicles, shoulders, interosseous muscles, scapula, thigh and calf); loss of subcutaneous fat (orbital, triceps, fat overlying the ribs); localized or generalized fluid retention; and decrease in functional status measured by gripping force (dynamometry).

For anthropometric determination, actual body weight and height without shoes were determined to the nearest 0.1 kg using an electronic scale and to the nearest 0.1 cm using a stadiometer, respectively. BMI was calculated from these results (BMI = weight in kg / (height in m) ²). To calculate the percentage of lost weight the following equation was applied: % PP = ((habitual weight - actual weight) / habitual weight) × 100.

Triceps skinfold thickness (TST) and mid-upper arm circumference (MUAC) were measured on the non-dominant arm and the mean of three measurements was calculated. TST was assessed using a skinfold calliper (Holtain LTD, Crymych, UK) and MUAC was determined at the middle point between the olecranon and acromion using a non-elastic tape measure. Arm muscle perimeter (AMP) was calculated using the formula AMP (Cm) = MUAC (cm) - (TST (mm) × 0.314). To prevent inter-observer and intra-observer variability, anthropometric parameters were collected by the same person.

Venous blood samples were obtained from the three groups of patients, after 12 h fasting. Centrifugation (1500 g, 10 min, 4 °C) of the samples was carried out for isolating serum and plasma in order to determine biochemical parameters. The leftover aliquots were stored at − 80 °C for other measurements.

All biochemical determinations were carried out in our hospital’s Clinical Analysis Service.

Albumin was determined by the Bromcresol green method (Abbott Laboratories, Abbott Park, IL 60064 USA) with a coefficient of variation (CV) ≤ 3.3% and a sensitivity of 0.3 g/dL. Prealbumin, transferrin, retinol-binding protein (RBP), and complement C3 fraction were determined by kinetic nephelometry with a Beckman LX-20 autoanalyzer (Beckman Coulter La Brea, CA, USA) with a CV of 4%. Triglycerides and total cholesterol were measured by enzymatic assays with a Beckman LX-20 autoanalyzer (Beckman Coulter, La Brea, CA, USA). The intraserial variation coefficient was < 3.5% for all determinations. Absolute lymphocytes were determined by flow cytometry (Coulter-Beckman) and high-sensitive C-reactive protein (hsCRP) by an immunonephelometric assay. The intraserial CV was < 3.5% for all determinations.

Serum levels of proinflammatory cytokines, interleukin-6 (IL6) and TNFα, and intercellular adhesion molecule 1 (ICAM-1) and vascular cell adhesion molecule 1 (VCAM-1) were analysed using a Luminex 200 flow analyser system (Austin, TX, USA). Milliplex® MAP human high sensitivity T Cell and Human Cardiovascular Disease Magnetic Bead Panel were purchased from Millipore Corporation (Billerica, MA, USA). The intraserial and interserial variation coefficients were < 5.0 and < 15.0%, respectively, for all determinations.

Citrated blood samples were mixed with dextran (3%) and left for 45 min in order to obtain human leukocytes. The supernatant was collected and poured over Ficoll-Hypaque (GE Healthcare, Uppsala, Sweden) and centrifuged at 1200 rpm for 25 min. The supernatant was discarded and the pellet was lysed for 5 min at room temperature using Lysis Buffer. The sample was then centrifuged (1200 rpm, 5 min) and the pellet washed in Hank’s Balance Salt Solution (HBSS) and resuspended in complete RPMI media (RPMI supplemented with 10% FBS).

Total ROS production, GSH content and membrane potential were determined using the fluorescent probes 2′, 7′-dichlorodihydrofluorescein diacetate (DCFH-DA, 5 μM) 5-chloromethylfluorescein diacetate (CMFDA, 2.5 μM) and tetramethylrhodamine methylester (TMRM, 5 μM), respectively. The leukocytes were seeded in 48-well plates and incubated with the probes for 30 min. Next, the wells were washed with HBSS and data was acquired with an IX81 Olympus fluorescence microscope (Olympus, Hamburg, Germany) and static cytometry software ‘ScanR’ version 2.03.2 (Olympus). Single cell fluorescence was measured and quantified. All probes were purchased from Invitrogen (Life Technologies, Barcelona, Spain). In order to assess Oxygen consumption, leukocytes were resuspended at a density of 5 × 10⁶ cells/mL in HBSS and placed in a gastight chamber coupled to a Clark-Type O₂ electrode (Rank Brothers). In order to check whether O₂ consumption was mainly mitochondrial, Sodium cyanide (10^− 3 M) was employed.

Umbilical cord samples obtained from normal deliveries were employed to harvest Human Umbilical Vein Endothelial Cells (HUVEC). In short, the procedure was as follows: the vein was washed with PBS and incubated in a solution of collagenase (1 mg/mL) for 17 min at 37 °C; after which the collagenase was collected in a 50 mL tube and neutralised with complete RPMI medium. The endothelial cells were then collected by centrifugation (1200 rpm, 10 min) and resuspended in Endothelial Growth Medium (EGM-2). The cells were seeded in T25 flasks and cultured until confluence. After confluence, cells were detached using trypsin and transferred to 6-well plates. The cells were cultured until confluence in 25 mm diameter plastic coverslips covered with fibronectin (5 mg/mL). In the flow chamber in vitro study, leukocytes (1·10⁶ cells/mL) were resuspended in Dulbecco’s PBS containing 20 × 10^− 3 mol/L HEPES and 0.1% human serum albumin. The coverslip with confluent HUVEC monolayer was placed in the flow chamber and leukocytes were drawn across the monolayer at a flow rate of 0.36 mL/min (approximately shear stress of 0.7 dyne/cm²) under a microscope (Nikon Eclipse TE 2000-S; Amstleveen, The Netherlands) connected to a video camera (Sony Exware HAD; Koeln, Germany). Rolling and adhesion parameters in a single field were recorded for 5 min. Rolling velocity was evaluated by measuring the time in which a cell crossed a distance of 100 μm. Leukocyte rolling flux was determined by counting the number of leukocytes rolling over a surface of 100 μm² of the endothelial monolayer during a 1-min period.

Adhesion was measured by counting the number of cells that maintained stable contact with the HUVEC monolayer for 30 s. The positive controls Platelet-activating factor (PAF, 1 μmol/L, 1 h) and TNFα, (10 ng/mL, 4 h) were used for leukocytes and HUVEC respectively.

Based on our preliminary data [9, 12], the study was designed to detect 5 and 20% differences in variation of the serum cytokines (IL6 and TNFα) between and within groups, respectively, with a power of 80% and an α risk of 0.05. Under these premises, at least 20 subjects per group were considered.