Optimization of the viability of stem cells derived from umbilical cord blood after maternal supplementation with DHA during the second or third trimester of pregnancy: study protocol for a randomized controlled trial

The trial is designed to target pregnant women within the 20th or 28th week of gestation. At the time of recruitment, the participants will sign an informed consent form, and complete a questionnaire authorizing third parties to obtain demographic, anamnestic and nutritional data. The information thus obtained will be entered into a case report form for each pregnant woman.

Detailed information on benefits and risks of DHA will be provided to study candidates. Participants that meet pre-specified eligibility criteria (Table 1) and provide written informed consent will be enrolled in the study.

The Ethics Committee of the San Giovanni Calibita Fatebenefratelli Hospital (Rome, Italy), in compliance with the Helsinki Declaration, approved the study protocol (9 July 2009, reference: 35/2009; and 9 December 2010, reference: 67/2010). The trial is registered at the International Standard Randomised Controlled Trial Number Register (ISRCTN58396079).

Participants included in the trial will be divided into two groups: one group will be given the placebo; and the other group will be given DHA (Figure 2). The placebo or DHA will be assigned in a double-blind, randomized manner, created by a computer program producing a sequence of codes attributed to one of the two groups. An identifying code, assigning the woman to one of the two study groups, guarantees, from that moment on, anonymity in treating sensitive data.

Each participant will receive a complete set of capsules of either placebo or DHA, to take one a day from the 20th or 28th week up to the 40th week of estimated gestational age. The placebo pills (placebo batch) will contain 250 mg of olive oil. This choice is conditioned by the need to use a product of proven safety with a consistency and flavour as similar as possible to fish oil.

The DHA capsules (active batch) will contain 250 mg of DHA (Incromega™ DHA 250TG SR, Croda, Goole, UK) + 10 mg natural vitamin E (Avantgarde sigma-tau, Rome, Italy). The DHA in the capsule is extracted from fish oil by PureMax™ technology (Croda) that enables lipids to be purified and concentrated to maximum standards. This ensures that the DHA used for this study is free of contaminants, including: heavy metals, such as mercury, arsenic, cadmium and lead; oxidant impurities; dioxins and furans; dioxin-type polychlorinated biphenyls; and polycyclic aromatic hydrocarbons.

The packaging of the capsules in the two groups will be identical (see Table 2).

To evaluate the effectiveness of the diet supplement, a venous blood sample will be taken from half of the study participants with the purpose of finding the DHA concentration in the erythrocyte membranes. Two samples of 2 cc of venous blood will be taken from all participants before taking placebo or DHA, at the 20th or 28th week after recruitment, and at the 37th to 38th week of pregnancy. The blood samples will be taken with a specific kit provided by Lipinutragen-CNR (Bologna, Italy) and shipped to the Lipinutragen-CNR laboratory for testing. The DHA concentration, with respect to the total erythrocyte membrane phospholipids, will be determined by treating a 0.5 ml portion of the maternal blood sample or cord blood samples to separate the erythrocytes and isolate the erythrocyte membranes [24]. The fraction of total phospholipids will be treated with 0.5 M KOH/MeOH for 10 minutes at room temperature in order to obtain the chemical derivation of the phospholipids and compare them with the corresponding chemical fatty acid methyl esters (FAME). FAMEs will be evaluated by gas chromatography (GC) with a flame ionization detector (Agilent 6850; Agilent Technologies, Santa Clara, CA, USA) and a DB-23 column (90% biscyanopropyl/10% phenylcyanopropyl polysiloxane capillary column; 60 m, 0.25 mm ID, 0.25 μm film thickness) or similar, with hydrogen as carrier gas at a constant flow of 1 ml/min; the oven programme will be fixed for the efficient separation of the FAMEs, including the cis and trans isomers. FAMEs can be recognized by comparing them with commercially available references. Trans geometric isomers will be recognized by comparison with a library of trans isomers obtained by radical isomerization as described in previous publications [25]. The FAMEs will be identified by a randomized analysis of the samples by GC coupled with mass spectrometry. The values of the fatty acids will be given as a percentage of all the most important peaks resulting from the GC analysis, representing 98 to 99% of the total chromatographic peaks. The analyses will be repeated so that the value of the DHA can be checked at zero time and compared with the known normal range in healthy subjects.

The statistical assessment of the treatment effectiveness will be obtained by comparison with the DHA values obtained after therapy.

UCB cells will be stained with fluorescein isothiocyanate (FITC)-conjugated monoclonal antibody against CD45+ and phycoerythrin (PE)-conjugated monoclonal antibody against CD34+. These will be used to identify leukocytes and HSCs, respectively. For analysis of the viability of the cells, they will also be stained with 7-aminoactinomycin D (7-AAD), which will bind to the DNA of cells that are undergoing or have undergone apoptosis (Stem Kit™ Beckman Coulter, Brea, CA, USA). The stained cells will then be lysed (1:10 dilution of ammonium chloride 10x concentrated and deionized water) and analyzed by flow cytometer with a FC 500 cytometer (Beckman Coulter) using CXP software under a single ISHAGE gating strategy.

Before extracting the cord blood, the recruited pregnant women must carry out serological tests to prove the absence of the following infectious diseases: hepatitis B virus; hepatitis C virus; HIV; cytomegalovirus; human T-cell lymphotropic virus; and syphilis. The report will then be presented to the hospital to obtain the licence.

All the participants will receive a free cord blood collection kit provided by SmartBank (SmartBank, Rome, Italy). Hospital staff assisting the birth will immediately extract and collect the cord blood with the kit. Samples will be shipped to the Biovault technical laboratory (Plymouth, UK) for specific analysis of: volume (ml); pH; cell viability (%); number of CD34+ cells; number of leukocytes; and bacterial and viral tests. In order to determine the DHA percentage in the cord blood erythrocyte membranes, 2 cc of the extracted cord blood will be sent to the Lipinutragen-CNR laboratory in Bologna.

The cord blood processing procedures will be carried out in the Biovault laboratory in the UK, possessing medical and healthcare products, and regulatory agency registration, operating according to the World Health Organization (WHO) international good manufacturing practices protocol, and the International Organization for Standardization (ISO) ISO 9001:2008 and ISO 13485:2012 standards, and aseptic treatment, grade A certificate, will be performed in a Biosafety Level 3 (BSL-3) clean room. Biovault is accredited by the American National Standards Institute (ANSI) regulatory accrediting body, Advancing Transfusion and Cellular Therapies Worldwide, and the Joint Accreditation Committee of the International Society for Cellular Therapy (ISCT) and the European Group for Blood and Marrow Transplantation (EBMT) (JACIE), and has a Human Tissue Authority licence.

The sample will enter the BSL-3 clean room through a hermetically sealed window with positive outlet atmospheric pressure. Inside the BSL-3 clean room the sample will be weighed, centrifuged, measured volumetrically, and subjected to microbiological tests, flow cytometry analysis and phase separation with subsequent selection of mononuclear cells. The sample containing the cells will be inserted into the final Pall container (Pall Corporation, Port Washington, NY, USA) and mixed at 4°C with 10% dimethyl sulfoxide (DMSO). The bag or Pall, with a unique, indelible identification code, will be inserted into a computerized temperature reduction system. After the temperature is reduced, the Pall will be inserted in a sealed metal container and preserved in liquid nitrogen vapour at -196°C.

The flow cytometry analysis will be carried out within 48 hours of the UCB sample collection with a FC 500 flow cytometer (Beckman Coulter) on ISHAGE software platform. The analysis method uses double fluorescence (FITC-PE) with rat monoclonal antibody. For a simultaneous identification and count of the CD45+ and CD45+ CD34+ cells, a double antibody marking will be carried out, evaluating the percentage of the positive population with regards to the absolute count. The CD34+ receptor will be used as an indicator of the total number of progenitor stem cells of the haematopoietic lineage. The cell viability will be evaluated by flow cytometry using 7-AAD (Invitrogen Life Technologies, Carlsbad, CA, USA). Apoptotic, necrotic and metabolically inactive cells will be stained and thus considered non-viable while viable cells remain unstained. Total cells will be counted by flow cytometry discriminating between non-viable (7-AAD positive cells) and viable cells (7-AAD negative cells). The flow cytometer will be calibrated every 24 hours and quality controls performed according to the UK National External Quality Assessment Service (NEQAS) protocol.

The statistical analysis of the data obtained will be carried out with the aid of the Statistical Package for the Social Sciences (SPSS) program (IBM Corporation, Armonk, NY, USA) in cooperation with the Fatebenefratelli Association for Research (AFaR) of the San Giovanni Calibita Fatebenefratelli Hospital (Rome, Italy). Each experimental group will be compared versus the respective placebo group. The effectiveness of the DHA supplementation at different stages of gestation will also be evaluated by comparing the two experimental groups. The differences between the quantitative variables of the two groups will be analyzed with the Student’s t-test and analysis of variance (ANOVA); results of P <0.05 will be considered statistically significant. The Spearman test will also be used to compare the parameters of interest, and other quantitative and non-quantitative variables presented by the groups studied.

Patient recruitment is currently being undertaken.