Acute malnutrition is a prevalent public health problem in many low- and middle-income countries. It contributes significantly to childhood morbidity and mortality and affects more than 70 million children annually(Reference Black, Victora and Walker1,Reference Lapidus, Luquero and Gaboulaud2) . Acute malnutrition is partly caused by insufficient intakes of energy and nutrients for maintaining essential body functions. The food consumption in low- and middle-income countries is often a starch-based diet such as rice, legumes, fruits and vegetables that is low in PUFA(3,Reference Michaelsen, Hoppe and Roos4) .
Dietary linoleic acid (18 : 2n-6; LA) and α-linolenic acid (18 : 3n-3; ALA) are essential fatty acids and can be metabolized to arachidonic acid (20 : 4n-6; AA) and DHA (22 : 6n-3), respectively. These long-chain PUFA (LCPUFA) are critical for healthy growth, immune function, brain development and the skin–water barrier(Reference Lauritzen, Hansen and Jørgensen5–Reference Ratnayake and Galli7). Acutely malnourished children may be particularly vulnerable to essential fatty acid deficiency owing to low food consumption, disturbed lipid metabolism and absorption, and/or diarrhoea caused by intestinal infections(Reference Holman, Johnson and Osvaldo8–Reference Smit, Muskiet and Boersma10).
In children with moderate acute malnutrition (MAM) and/or severe acute malnutrition (SAM), PUFA status has been shown to be altered in different blood pools such as sterols(Reference Koletzko, Abiodun and Laryea11), triacylglycerols(Reference Taylor12), plasma(Reference Naismith13,Reference Franco, Hotta and Jorge14) , erythrocytes(Reference Smit, Dijkstra and Schnater15) and whole blood(Reference Yaméogo, Cichon and Fabiansen16–Reference Babirekere-Iriso, Lauritzen and Mortensen18). Whole-blood samples have logistical advantages for field research collection due to less sample processing immediately post collection, as well as the ability to collect dried blood spots. However, whole blood includes plasma and various types of blood cells that can differentially impact the overall fatty acid composition(Reference Brenna, Plourde and Stark19). Acutely malnourished children living under poor conditions are vulnerable to infections, inflammation, anaemia, and other nutritional and health challenges(Reference Smit, Muskiet and Boersma10,Reference Bachou, Tylleskär and Kaddu-Mulindwa20–Reference Thakur, Chandra and Pemde24) that could affect blood cell counts, such as increased monocytes with infection(Reference Ingersoll, Platt and Potteaux25,Reference Yoshida, Keen, Ansari, Shils, Olson and Shike26) . Changes in cell counts can affect the overall fatty acid composition of whole blood, which could alter interpretations of whole-blood PUFA status. Another health challenge that is prevalent in South-East Asia is genetic Hb disorders (haemoglobinopathies), which may contribute to changes in whole-blood PUFA composition due to increased risk of anaemia and altered erythrocytes caused by these disorders(Reference Weatherall and Clegg27,Reference Fucharoen and Weatherall28) .
The purpose of the present study was to investigate the fatty acid composition, particularly the PUFA content, of whole blood and potential associations with markers of nutritional and health status in acutely malnourished Cambodian children.
Methods
Study design and setting
The present cross-sectional study uses baseline data from an 8-week interventional trial evaluating the effectiveness of a locally produced, fish-based, ready-to-use therapeutic food compared with a standard ready-to-use therapeutic food during outpatient treatment of acute malnutrition in Cambodian children (called the ‘SAM trial’)(Reference Sigh, Roos and Chamnan29,Reference Sigh, Roos and Sok30) . The SAM trial was conducted at the National Pediatric Hospital in Phnom Penh, Cambodia. The sample size in the trial was based on the superiority of one of two ready-to-use therapeutic foods on the main outcome, weight gain (g/kg per d). To detect a 10 % difference with a standard deviation of 0·7 g/kg per d, a sample size of forty-nine in each group was required to achieve 80 % power (α = 0·05, two-sided). To allow for dropouts, a total of 120 children were enrolled(Reference Sigh, Roos and Chamnan29). Initial recruitment was of 0·5–18-year-old children. After recruiting fifty-four children, the recruitment criterion for age was adjusted to enrol only 6–59-month-old children due to limited funding and on request of the funding agency (UNICEF). The final sample was comprised of the fifty-four children aged up to 18 years and 120 children aged 6–59 months.
Eligibility and nutritional markers
The eligibility criteria for enrolment in the present study were children aged 0·5–18 years with non-complicated acute malnutrition, defined as weight-for-height Z-score (WHZ) or BMI-for-age Z-score (BAZ) of ≤−2·8. Children younger than 60 months were also re-enrolled based on mid-upper-arm circumference (MUAC) of ≤115 mm and/or presence of nutritional oedema(Reference Sigh, Roos and Chamnan29). Children with complications affecting food intake or participating in other clinical trials were not eligible. Personal and sociodemographic information was obtained from caregivers using questionnaires. Age was obtained from birth growth monitoring cards, or by asking the caregiver if the card was not available. Current breast-feeding status was reported by interviewing caregivers using a structured questionnaire.
Nutritional markers were assessed by anthropometric measures (weight, length/height, MUAC, skinfolds) using standard equipment as described in Sigh et al.(Reference Sigh, Roos and Chamnan29). Anthropometric Z-scores, namely WHZ or BAZ (wasting), weight-for-age Z-score (WAZ; underweight) and height-for-age Z-score (HAZ; stunting), were calculated from the WHO Growth Standards 2006 for children aged 6–59 months(31) and the WHO Growth References 2007 for children aged 5–19 years(Reference de Onis, Onyango and Borghi32). The mid-upper-arm fat percentage and muscle area were calculated according to Rolland-Cachera et al.(Reference Rolland-Cachera, Brambilla and Manzoni33) using MUAC and triceps skinfold measures, which were measured to nearest 0·1 mm using a Holtain skinfold calliper.
Blood sampling
Four millilitres of venous whole blood from the cubital vein were drawn using a sterile 23G/25G × ¾″ scalp vein set (Vinahankook Medical Supplies Co., Hanoi, Vietnam) or a sterile 24G IV cannula needle with catheter and injection valve (HarsoriaTM, Gurgaon, India) by trained health staff. Two millilitres of whole blood were collected in 2 × 2 ml EDTA-coated vacutainers and 2 ml of whole blood were collected in a 6 ml trace-element Sodium NH Heparin vacutainer (VACUETTE®; Greiner Bio-One International GmbH, Frickenhausen, Germany). One EDTA vacutainer was used to perform dried blood spots to measure PUFA and blood cell count analysis. Haemoglobinopathies were analysed using the second EDTA vacutainer and inflammation status was analysed using the sodium heparin vacutainer.
Dried blood spots and fatty acid analysis
Dried blood spots were performed using the laboratory facilities at the National Pediatric Hospital, following validated procedures(Reference Metherel, Aristizabal Henao and Stark34). Dried blood spots were made by applying 40 µl of EDTA whole blood on pre-treated chromatography paper (Grade 3MM, Whatman Ltd; Danish supplier: Frederiksen Scientific A/S, Ølgod, Denmark). The samples were dried at room temperature and stored in a polypropylene ‘Ziplock’ bag at 4°C for a maximum of 2 months prior to shipment to the University of Waterloo in Canada for fatty acid analysis(Reference Metherel, Aristizabal Henao and Stark34,Reference Metherel and Stark35) . The samples were analysed on a Varian 3900 gas chromatograph equipped with a DB-FFA 15 m × 0·10 mm capillary column coated with a 0·10 μm film of nitroterephthalic-acid-modified polyethylene glycol (J&W Scientific; Agilent Technologies, Mississauga, ON, Canada) using hydrogen as the carrier gas(Reference Metherel and Stark35–Reference Metherel, Buzikievich and Charkhzarin38). The eluted fatty acid methyl ester peaks were identified by comparing retention times with an external standard (GLC-246; Nu Chek Prep Inc., Elysian, MN, USA)(Reference Armstrong, Metherel and Stark39). Fatty acid data are expressed as relative percentage of all fatty acids (% FA) and as fatty acid concentration (µg per 100 µg whole blood).
The inter- and intra-assay CV for the dried blood spot fatty acid analyses were similar to values previously reported for wet whole-blood analyses(Reference Lauritzen, Sørensen and Harsløf40). For the fatty acids reported, all the inter-assay CV were below 7 % and all the intra-assay CV were below 3 %, with higher CV being associated with the fatty acids with relatively low abundance (i.e. docosapentaenoic acid (22 : 5n-6; DPA) and mead acid (20 : 3n-9; MA)).
Definition of essential fatty acid deficiency
Low LA and ALA are reflected in a ratio between their long-chain metabolites. The ratios MA:AA and n-6 DPA:DHA are commonly used biomarkers of essential fatty acid deficiencies(Reference Holman and Holman41,Reference Bourre, Francois and Youyou42) . For whole blood, deficiency levels for these markers have not been defined. However, it has been proposed that in whole blood, MA:AA > 0·02 indicates very low n-6 PUFA status and n-6 DPA:DHA > 0·2 and total n-6:n-3 PUFA > 10·5 indicate very low n-3 PUFA status(Reference Yaméogo, Cichon and Fabiansen16). We applied these cut-off values to define low PUFA.
Assessment of health markers
The markers assessed for health status were Hb concentration (for anaemia), blood cell counts (overall health status), Hb variations (for haemoglobinopathies), the presence of HIV (for HIV status), C-reactive protein (CRP; acute inflammation marker) and α1-acid glycoprotein (AGP; progressed inflammation marker). Approximately 300 µl EDTA whole blood was used to assess blood cell counts, including Hb concentration, using a haematology analyser (Sysmex Kx-21, ID no. NP021 and NP023; Sysmex Corporation, Kobe, Japan) at the National Pediatric Hospital. Anaemia status was diagnosed based on Hb concentration using cut-off values recommended by WHO(43). The presence of haemoglobinopathies (only in the 6–59-month-old children) was analysed using electrophoreses (Minicap; SEBIA, Lisses, France). Samples were analysed at the National Pediatric Hospital. Following a disruption of the capacity for analysing at the hospital, five samples were analysed at the Pasture Institute, Phnom Penh, using the same method and analysis protocol. Normal Hb was classified for 0–23-month-old children as HbA > 70 %, HbF ≤ 30 %, HbA2 < 2 %; and for 24–59-month-old children as HbA > 95·5 %, HbA2 = 2·0–3·5 %, HbF < 5 %. All other Hb variations were classified as haemoglobinopathies, except HbE/heterozygote, which was classified as HbE ~ 20–30 %(Reference Wieringa, Dahl and Chamnan44). Complete blood counts and haemoglobinopathies were analysed one sample at a time and no certified standard was available. Therefore, no inter- and intra-assay CV were available.
HIV status was self-reported via a questionnaire asking if the child had been tested and, if so, the result of the test. All HIV-positive children in the study received treatment at the National Pediatric Hospital. CRP and AGP were measured in a combined sandwich ELISA method in duplicate(Reference Erhardt, Estes and Pfeiffer45). The control samples’ (n 40) inter-assay CV were 5·8 % (CRP) and 8·1 % (AGP). Inflammation was indicated by CRP > 5 mg/l and/or AGP > 1 g/l(Reference Thurnham, McCabe and Haldar46).
Statistical analysis
All data, except blood analyses, were entered directly into tablets and uploaded to an online software system (Kobotoolbox) or double entered into EpiData version 3.1 (The EpiData Association, Odense, Denmark). Statistical analyses were conducted using the software R studio (version 3.4.0 for Windows). Models were assessed by visual residuals and normal probability plots inspection. Non-normal distributed models were log10 transformed. Descriptive statistics are presented as percentages and frequencies, means and standard deviations, or medians and interquartile ranges. All analyses, not pre-including age, are age-adjusted owing to large age variations in the study. To analyse correlations between PUFA and nutritional and health status markers, a simple or multiple linear regression was applied adjusted for age, sex and breast-feeding due to the well-known effects of breast-feeding on PUFA(Reference Yaméogo, Cichon and Fabiansen16,Reference Dalmeijer, Wijga and Gehring47–Reference Barbarich, Willows and Wang50) . The analyses are reported as regression coefficients (β) with 95 % confidence intervals and P values. Comparisons in cell counts between health markers were assessed using ANCOVA adjusted for age and sex with the Emmeans R package, which takes multiple comparisons into consideration. Statistical significance was defined as P < 0·05. P values were not adjusted for false discovery rates, as the correlation between PUFA and markers of nutrition status was consistent across variables, meaning the P values would be overcorrected if adjusted using the traditional Bonferroni method, resulting in a lower correlation factor and hence increased risk of type 2 errors.
Results
Participants
Out of 609 children screened, 174 (28·6 %) were eligible for enrolment (Table 1). Their mean age was 4·1 years and their mean wasting Z-score was −3·0. The anaemia prevalence was 52 %, ~35 % of the children had haemoglobinopathies and 20 % (n 35) were HIV positive. Median levels of inflammation markers were 0·6 mg/l (CRP) and 0·7 g/l (AGP), reflecting an inflammation prevalence of 16 and 35 % according to CRP and AGP, respectively.
IQR, interquartile range; WAZ, weight-for-age Z-score; HAZ, height-for-age Z-score; MUAC, mid-upper-arm circumference; SAM, severe acute malnutrition; MAM, moderate acute malnutrition; CRP, C-reactive protein; AGP, α1-acid glycoprotein.
† n 173, missing exact age and sex from one child.
‡ Measured using weight-for-height Z-score (WHZ) or BMI-for-age Z-score (BAZ) as an indication of wasting.
§ n 146, missing specific birthdate for twenty-eight children.
‖ Among children aged ≤59 months: SAM defined as either WHZ < –3 or MUAC < 115 mm; MAM defined as either WHZ between –2 and –3 or MUAC = 115–125 mm. Among children aged ≥60 months: SAM defined as either BAZ < –3 or MUAC < 129 mm (children aged 5–9 years), MUAC < 160 mm (children aged 10–14 years), MUAC < 190 mm (children aged 15–18 years); MAM defined as either BAZ between –2 and –3 or MUAC = 129–154 mm (children aged 5–9 years), MUAC = 160–185 mm (children aged 10–14 years), MUAC = 190–215 mm (children aged 15–18 years).
¶ Anaemia cut-off is age- and sex-dependent.
†† Haemoglobinopathies were only assessed in the 6–59-month-old children, n 106 out of the total 174; thus the percentage is calculated based on the n of the actual sampling.
‡‡ Defined as CRP > 5 mg/l and AGP > 1 g/l.
§§ n 163, data on blood cell counts were missing for ten children.
‖‖ Erythrocytes, leucocytes and platelets combined.
Whole-blood PUFA and very low PUFA status
The relative contribution in whole blood was 13·2 % FA for LA and was 0·2 % FA for ALA (Table 2). The mean relative contribution for MA was 0·1 % FA and this was reflected in a high MA:AA ratio, indicating very low n-6 PUFA status in the children according to the predefined cut-off (MA:AA > 0·02). Based on the predefined cut-offs (n-6 DPA:DHA > 0·2 and total n-6:n-3 PUFA > 10·5), 68 % of the children appeared to have very low n-3 PUFA status. We estimated that 14 % of the children may actually be both n-6 and n-3 deficient (MA:AA > 0·02, n-6 DPA:DHA > 0·2 and total n-6:n-3 PUFA > 10·5) based on these cut-offs.
% FA, percentage of total fatty acids.
† Total fatty acid concentration is expressed as µg/100 µl whole blood.
Associations between whole-blood PUFA and markers of nutritional status
HAZ was significantly and positively correlated with total PUFA (β = 0·57 % FA; 95 % CI 0·14, 1·00 % FA), LA (β = 0·33 % FA; 95 % CI 0·02, 0·64 % FA), AA (β = 0·16 % FA; 95 % CI 0·01, 0·31 % FA) and total n-6 LCPUFA (β = 0·20 % FA; 95 % CI 0·02, 0·38 % FA; Table 3). The estimates indicated that an increase in HAZ of 1 was correlated with a ~0·6 % FA-point increase in total PUFA. A similar association was found for absolute age-adjusted height. Height was also significantly positively associated with whole-blood DHA and n-3 LCPUFA (Table 4). A 6 cm increase in height was correlated with a ~0·7 % FA-point increase in DHA (Table 4). A 50 cm increase in height was associated with a –0·01 % FA-point decrease in MA:AA and hence with a decreased risk of n-6 essential fatty acid deficiencies.
LA, linoleic acid; AA, arachidonic acid; LCPUFA, long-chain PUFA; MA, mead acid; HAZ, height-for-age Z-score; CRP, C-reactive protein; AGP, α1-acid glycoprotein.
* P < 0·05.
† For blood counts only, results are given as ×10–4 for total PUFA, ×103 for LA and AA, ×102 for n-6 LCPUFA and ×10–2 for MA:AA to present meaningful results.
‡ For nutritional status and health status markers, results (except blood counts) are given as ×103 to present meaningful results.
§ Wasting Z-score is weight-for-height Z-score for children aged <5 years and BMI-for-age Z-score BAZ for children aged ≥5 years.
‖ Adjusted only for breast-feeding.
¶ Erythrocytes, leucocytes and platelets combined.
LCPUFA, long-chain PUFA; DPA, docosapentanoic acid; CRP, C-reactive protein; AGP, α1-acid glycoprotein.
* P < 0·05.
† For blood counts only, results are total given as ×10−2 for EPA, ×102 for n-3 LCPUFA and ×10−3 for n-6 DPA:DHA to present meaningful results.
‡ For nutritional status and health status markers, results (except blood counts) are given as ×103 to present meaningful results.
§ Wasting Z-score is weight-for-height Z-score for children aged <5 years and BMI-for-age Z-score BAZ for children aged ≥5 years.
‖ Adjusted only for breast-feeding.
¶ Erythrocytes, leucocytes and platelets combined.
MUAC was not significantly correlated with any of the PUFA measures (see online supplementary material, Supplemental Tables S1 and S2). However, separating MUAC into fat percentage and muscle area showed that a low mid-upper-arm fat percentage was associated with high AA, n-6 LCPUFA and n-3 LCPUFA (Tables 3 and 4), and a high mid-upper-arm muscle area was positively associated with AA and n-6 LCPUFA (Table 3).
Wasting Z-score and WAZ were not associated with any PUFA, but high body weight was associated with high EPA (20 : 5n-3; see online supplementary material, Supplemental Tables S1 and S2).
Associations between markers of health challenges and whole-blood PUFA
Hb concentration was not correlated with overall PUFA, n-6 PUFA, n-3 PUFA or either of the markers of low PUFA, MA:AA or n-6 DPA:DHA (Tables 3 and 4). Also, no associations were observed for anaemia (see online supplementary material, Supplemental Tables S1 and S2). However, the presence of haemoglobinopathies was associated with high MA:AA and a non-statistically significant tendency for low total PUFA (β = −1·34 % FA-points; 95 % CI −2·72, 0·04 % FA-points; Table 3). An age-stratified analysis showed a 1·39 % FA-point (95 % CI −2·78, −0·00 % FA-point, n 103) lower total PUFA in 6–59-month-old children with haemoglobinopathies than in the children without haemoglobinopathies.
HIV infection and high AGP concentration were associated with high MA:AA (Table 3). No associations were observed between CRP and any of the PUFA (Tables 3 and 4).
Unexpectedly, total whole-blood cell count was not associated with any of the PUFA measures. Furthermore, no correlations were observed for total count of leucocytes or erythrocytes. However, high platelet count was associated with high total PUFA and LA (Table 3), and high monocyte count was associated with high total PUFA, AA, n-6 LCPUFA, DHA and n-3 LCPUFA (Tables 3 and 4).
Comparing blood cell counts in children with and without health challenges
There was no significant difference observed in blood cell counts between children with SAM and MAM (see online supplementary material, Supplemental Table S3). Children with anaemia appeared to have a higher mean platelet count than those without anaemia (×109/l: 434 v. 371, P = 0·010; Table 5). Furthermore, an association analysis adjusted for age and sex showed a non-significant tendency towards a negative correlation between Hb concentration and platelet count (×109/l: −16·8; 95 % CI −33·8, 0·2), but not for monocyte count (×109/l: −0·00; 95 % CI −0·05, 0·05). Presence of inflammation v. no inflammation resulted in a significantly higher mean platelet count (×109/l: 462 v. 386, P = 0·002) and a strong tendency for a higher mean monocyte count (×109/l: 0·9 v. 0·8, P = 0·052; Table 5). Children with inflammation defined as CRP > 5 mg/l (72 counts; 95 % CI 9, 135 counts) or AGP > 1 g/l (74 counts; 95 % CI 25, 123 counts) had higher mean platelets (×109/l) compared with children with no signs of infection. Monocyte counts were elevated in children with CRP > 5 mg/l (estimated difference, ×109/l: 0·20 counts; 95 % CI 0·01, 0·39 counts) compared with children with normal CRP, but not in children with AGP above the cut-off of >1 g/l (estimated difference, ×109/l: 0·09 counts; 95 % CI −0·06, 0·25 counts). Hence, the association was dependent on the stage of inflammation.
† Analyses were not adjusted for age and sex, as this is included in the diagnostic criteria.
‡ Only including children who had been tested for HIV.
§ Inflammation was defined as C-reactive protein >5 mg/l or α1-acid glycoprotein >1 g/l.
Children with HIV had lower counts of erythrocytes, leucocytes and neutrophils (Table 5). The presence of haemoglobinopathies was significantly associated with a higher mean eosinophil count (×109/l: 0·5 v. 0·3, P = 0·021) and a tendency towards a lower mean platelet count (×109/l: 481 v. 436, P = 0·179).
Discussion
We found low relative contributions of total whole-blood PUFA in children admitted to outpatient treatment of acute malnutrition. Stunting and low height were associated with low total PUFA, LA, AA and n-6 LCPUFA. Low mid-upper-arm muscle area and high mid-upper-arm fat percentage were also associated with low AA and n-6 LCPUFA, but no associations were observed for wasting or any other measures of weight except for EPA and total weight. No associations were observed between Hb, CRP or AGP, and total PUFA, sub-classes of PUFA or any of the individual PUFA. The presence of HIV infection, progressed inflammation (defined by AGP) and haemoglobinopathies were associated with high MA:AA, and hence a risk of very low n-6 PUFA status. The presence of haemoglobinopathies was also associated with low total PUFA, especially in the young children. High platelet and monocyte counts appeared to be linked with inflammation and anaemia. High platelet and monocyte counts were also associated with high total PUFA and LA and with n-6 and n-3 LCPUFA, respectively.
Whole-blood PUFA levels
The acutely malnourished children in the current study had considerably lower total PUFA, n-6 and n-3 PUFA, and AA and DHA compared with a population of rural Cambodian infants(Reference Nurhasan, Roos and Skau49) living in an environment with limited dietary resources(Reference Skau, Bunthang and Chamnan51) and vulnerable to stunting and wasting(Reference Skau, Touch and Chhoun52), respectively. The whole-blood ALA assessed in the present study children diagnosed with acute malnutrition was similar to what was reported in children with MAM from Burkina Faso (0·2 % FA)(Reference Yaméogo, Cichon and Fabiansen16), while a study in Ugandan children with a more severe stage of SAM found even lower ALA (0·15 % FA) as well as lower LA (10·5 v. 13·2 % FA in the present study)(Reference Babirekere-Iriso, Lauritzen and Mortensen18). We found relatively low MA (0·08 % FA) compared with well-nourished Ugandan children (0·10 % FA), which was unexpected, since the Ugandan children with SAM had higher whole-blood MA (0·12 % FA)(Reference Babirekere-Iriso, Lauritzen and Mortensen18). Our results are in line with the MAM study in Burkina Faso with regard to the essential fatty acid deficiency markers of MA:AA, n-6 DPA:DHA and n-6:n-3 PUFA(Reference Yaméogo, Cichon and Fabiansen16).
Low PUFA in acutely malnourished children could be due to infection and metabolic disturbances associated with malnutrition(Reference Smit, Dijkstra and Schnater15). These disturbances could directly impair lipid digestion and uptake(Reference Smit, Dijkstra and Schnater15) and also indirectly be affected by other nutritional imbalances such as Fe deficiency, which, in combination with acute malnutrition, could impact on PUFA metabolism through reduced Δ-6-desaturase enzyme activity(Reference Smuts, Tichelaar and Jaarsveld53) and consequently reduced capacity for the conversion of LA and ALA to their long-chain metabolites.
Whole-blood PUFA is highly influenced by diet, rather than by malnutrition per se (Reference Smit, Muskiet and Boersma10). Cambodian children generally consume a diet based on rice, with limited amounts of vegetables, legumes and fruits, and little or no animal-source foods(3,Reference Michaelsen, Hoppe and Roos4) . This diet is at risk of being low in PUFA. Also, the cooking oils typically used are low in n-3 fatty acids(Reference Michaelsen, Hoppe and Roos4). Fish and fish products are the main animal-source food in the typical Cambodian diet(54) and, overall, fish is a highly important and valuable PUFA source in diets. The fish in the Cambodian diet are primarily freshwater fish available from the rich aquatic environment of the Mekong river basin. Tropical freshwater fish are generally lower in DHA and EPA compared with cold-water marine fish species(Reference Karapanagiotidis, Yakupitiyage and Little55–Reference Li, Sinclair and Li57). Furthermore, despite fish being consumed very frequently in Cambodia (even daily in the peak fishing season) the portion size can be very small, especially for children, resulting in low overall fish intake(Reference Skau, Bunthang and Chamnan51) and a diet low in n-3 PUFA. The low PUFA status of the children in our study could therefore also be the result of a low dietary intake, further enforced by the suffering from acute malnutrition.
Nutritional markers associated with whole-blood PUFA
The associations between stunting, height and low n-6 PUFA support the idea that sufficient dietary PUFA intake may be important in preventing stunting. Height gain was found to be correlated with higher DHA in young children in treatment for SAM in Uganda(Reference Babirekere-Iriso, Mortensen and Mupere17). A study of 2–6-year-old children from Tanzania found associations between risk of stunting and low whole-blood LA and total n-6 PUFA(Reference Jumbe, Comstock and Hahn58), while mixed findings between stunting and PUFA were reported in Ghanaian children(Reference Adjepong, Yakah and Harris59,Reference Adjepong, Pickens and Jain60) . The indication of a biological link between linear growth and PUFA status could be mediated by eicosanoids such as AA-derived prostaglandin E2, which can affect proteolysis in skeletal muscle and thereby have an impact on linear growth(Reference Rodemanns and Goldberg61). Another pathway could go through prostaglandin E2 stimulation of insulin-like growth factor-1 expression, which again meditates bone Ca accretion(Reference Smit, Muskiet and Boersma10,Reference Jumbe, Comstock and Hahn58,Reference Harada, Balena and Rodan62) . A few studies have found increased insulin-like growth factor-1 after fish-oil supplementation in children(Reference Damsgaard, Harslof and Andersen63,Reference Damsgaard, Mølgaard and Matthiessen64) .
We observed an association between high PUFA and muscle mass. Low mid-upper-arm fat percentage and high mid-upper-arm muscle area were associated with high AA and n-6 LCPUFA, meaning that high fat percentage or a reduced muscle mass was associated with less PUFA in the blood. Acute malnutrition causes muscle atrophy, which could be linked to increased stress metabolism and hypercortisolaemia(Reference Manary, Muglia and Vogt65). Although beyond the conclusions of the present study, we speculate that hypercortisolaemia may promote muscle proteolysis and increase energy expenditure and fat oxidation(Reference Brillion, Zheng and Campbell66), which could result in a combined effect of lower PUFA and muscle mass. Cortisol and muscle proteolysis as well as low PUFA could also be caused by the combination of low dietary intake and malnutrition.
Compromised health is associated with very low PUFA status
Hb concentration and anaemia were not associated with any PUFA or the cut-off used to define very low PUFA status. This is inconsistent with studies of children with either MAM or SAM that show a correlation between Hb concentration and AA and DHA and low PUFA status (n-6 DPA:DHA and MA:AA)(Reference Yaméogo, Cichon and Fabiansen16,Reference Babirekere-Iriso, Lauritzen and Mortensen18) .
Other studies observed an association between acute inflammation (CRP > 5 mg/l) and PUFA (LA, EPA and n-3 DPA) in children with SAM(Reference Babirekere-Iriso, Lauritzen and Mortensen18) and between progressed inflammation (AGP ≥ 1 g/l) and PUFA (AA, n-6 DPA, ALA and DHA) in children with MAM(Reference Yaméogo, Cichon and Fabiansen16). The present study’s finding that the inflammation markers were not associated with PUFA could probably be because the prevalence of inflammation was low compared with the two other studies(Reference Yaméogo, Cichon and Fabiansen16,Reference Babirekere-Iriso, Lauritzen and Mortensen18) . Studies in various populations have shown reduced CRP following fish-oil supplementation(Reference Bowden, Wilson and Deike67–Reference Ciubotaru, Lee and Wander69), which could support the suggestion that high PUFA may have a protective effect against inflammation.
Haemoglobinopathies were associated with low total PUFA in an age-stratified analysis in the young children. We speculate that haemoglobinopathies could cause a higher erythrocyte turnover, and thereby a higher phospholipid turnover. In the presence of haemoglobinopathies, a higher repair of blood cells, required due to oxidant stress and lipid damage of the erythrocyte membrane, is also speculated. Furthermore, because of lipid oxidation, the phospholipid repair system is insufficient in maintaining a proper molecular fatty acid composition in erythrocytes.
All blood cells are exposed to the same pool of fatty acid substrate from plasma, and the difference in PUFA measured in the whole-blood samples could be caused by the activity of enzymes using the fatty acid pool for phospholipid repair. Oxidant stress in erythrocytes may challenge the incorporation of PUFA, which affects the fatty acid composition of the membrane(Reference Kuypers, Cappellini and Vichinsky70). This may lead to low PUFA in cells and thereby to lower PUFA in children with haemoglobinopathies than in children without haemoglobinopathies.
Health markers’ influence on blood counts may indirectly implicate incorrect assessment of whole-blood PUFA status
Unexpectedly, the inflammation markers were not associated with any PUFA but were found to be associated with counts of platelets and monocytes, also formed as a response to infection. A sub-analysis showed an association between the markers of inflammation and platelets and monocytes, which confirms the expected biological response of CRP and AGP at the onset of infection and inflammation. The pattern of associations between the different markers used to define inflammation indicated differences in the biological response to acute and progressed inflammation.
Different blood fractions and cell types contribute different PUFA levels, so changes in the number of a specific cell could shift levels of PUFA in whole blood. This is likely to explain the increased PUFA we observed with increased monocyte and platelet counts, as monocytes consist of ~20 % AA and AA increases with increased monocyte count(Reference Calder71). Also, a decrease in erythrocytes, which is likely to be associated with anaemia, could result in reduced measurement of PUFA in whole-blood samples. These contra-acting mechanisms could explain the lack of associations of health markers for anaemia, inflammation and haemoglobinopathies with PUFA in the present study. The combined effects of anaemia with elevated platelets and monocytes caused by inflammation may have masked changes in PUFA.
The fatty acid composition of immune cells (e.g. lymphocytes and monocytes) is also expected to alter in accordance with dietary intake, which impacts the capacity of the immune cells to produce eicosanoids, which are involved in immune system regulation(Reference Calder, Yaqoob and Thies72). Thus, there is a two-way association between the immune system and PUFA. Inflammation is suggested to cause elevated cell counts in the present study, which may lead to misinterpretation of PUFA in whole blood. Inflammation markers were observed to influence platelets and monocytes differently, and platelets and monocytes were not associated with the same fatty acids. The complexity of these associations would make it difficult to adjust for inflammation markers and cell counts when assessing PUFA in whole blood in populations with severe health challenges such as acute malnutrition.
Limitations
The present study shares the limitation of other observational studies in that it identifies associations but does not identify causality. Another limitation is that we did not include data on total food consumption covering all dietary sources of PUFA such as quantity of fish and breast milk consumed. Also, the predefined cut-offs used to estimate essential fatty acid deficiencies were derived from infants and were applied to older children in the present study. The stage of deficiencies in children above infancy could be different. Finally, all the health markers used in the present study are to some degree related through cell counts, and it could be argued that all health markers should be adjusted for each other (anaemia, inflammation, HIV infection and haemoglobinopathies). Our study used secondary data and unfortunately it did not have insufficient power to adjust all health challenges for each of the others.
Conclusion
Overall, children with acute malnutrition in Cambodia had low total whole-blood PUFA and indicated to have a high prevalence of a very low PUFA. HAZ (stunting) and absolute height were both positively associated with PUFA, whereas no associations were found for wasting and other weight measures. Elevated platelets and monocytes, likely due to inflammation, were positively associated with PUFA, thus indicating that blood cell counts influence whole-blood PUFA levels. Therefore, in acutely malnourished Cambodian children, inflammation that elevates blood cell counts could result in increased blood levels of PUFA that do not reflect dietary intake and nutritional status. These findings indicate the need for further studies on the relationship between stunting and PUFA in acutely malnourished children through randomized controlled trials with dietary PUFA supplementation. Furthermore, future field studies using whole blood and dried blood spots to assess PUFA status should consider co-morbidities associated with severe health challenges, such as malnourishment, that can change the cellular composition of blood.
Acknowledgements
Acknowledgements: The authors would like to thank the National Pediatric Hospital for its collaboration and support in conducting the study. Deep thanks are extended to all caregivers, the participating children and the data collection team. Financial support: The study was financially supported by UNICEF’s national committees (Australia, Republic of Korea, Hong Kong), Institute de Recherché pour le Développment, University of Copenhagen and Neys-van Hoogstraten Foundation (grant number CA271). The funding bodies had no influence on data collection, data analysis or publication of the results. Conflict of interest: The authors have no conflicts of interest to declare. The views expressed are those of the authors and do not reflect the official policies or opinions of the organizations to which they belong. Authorship: S.S., F.T.W., A.L., C.C. and N.R. designed the study and formulated the research questions; S.S., N.A. and D.M. collected the data; S.S drafted the initial manuscript and analysed the data; L.L., F.T.W., K.D.S. and N.R. contributed to the interpretation of the data and the manuscripts; all authors reviewed and approved the final manuscript. Ethics of human subject participation: This study was conducted according to the guidelines laid down in the Declaration of Helsinki and all procedures involving research study participants were approved by the National Ethical Committee for Health Research of the Ministry of Health, Kingdom of Cambodia (April 2015 Version No. 2). Both written and verbal informed consent were obtained from all participants. The trial was registered at ClinicalTrials.gov (name: Comparison of a Locally Produced RUTF With a Commercial RUTF in the Treatment of SAM (FLNS_SAM); trial registration: NCT02907424; URL: https://clinicaltrials.gov/ct2/show/NCT02907424).
Supplementary material
To view supplementary material for this article, please visit https://doi.org/10.1017/S1368980019003744