Study design, setting and participants

A cross-sectional, prospective study of children aged between 12 and 60 months, diagnosed with undernutrition, admitted to the Kalembe-Lembe Pediatric Hospital of Kinshasa was carried out between 10 July 2017 and 10 January 2018. Ethical approval was obtained from the Ministry of Health of DR. Congo and the ethical committee of China Tongji Medical College. Kalembe-Lembe is a Red Cross (Croix Rouge) hospital situated in Lingwala Municipality, Kinshasa City. It is the only referral hospital for the Kinshasa Metropolis in that it admits children with undernutrition aged between 12 months and 15 years. All children admitted to the hospital with HIV and with or without undernutrition, marasmus, kwashiorkor or undernutrition like defined according to weight-for-height Z-score (WHZ) <−3s.d. of the median WHO reference values (WHO, 2009) or with symmetrical oedema attributable to undernutrition (WHO, 1999) and as per the management protocol of the WHO (2011) were included in the study. Additionally, the included undernutrition participants' were diagnosed by calculation of the body mass index (BMI) combined with evaluation of brachial perimeter (PB). The children with undernutrition was classified as marasmus, kwashiorkor or oedematous undernutrition and classified as a marasmic-kwashiorkor (combination of both). The exclusion criterion in this study was the participants with a congenital haemoglobinopathies (sickle cell anaemia) and the refusal of parental consent or of the children consent. A sample size of 225 was calculated based on a prevalence of 17.4% reported by Fergusson et al. (Reference Fergusson, Chinkhumba and Grijalva-Eternod2009) and a response rate of 90%. Recruitment was done prospectively until the sample size was reached. The recruitment process started with the agreement of the admission office staff; and after the attending medical team had completed their initial assessment and managed life-threatening complications. For all eligible children, the study was explained to the parent or guardian, and written informed consent was obtained. Parents/guardians of the patients were referred to the Voluntary Counselling and Testing centre to undergo pre- and post-test counselling.

Measurements and definitions

Blood was obtained by finger prick for thick smear malaria parasite test, and, HIV, while venous blood was collected into well-labelled ethylenediamine tetra acetate tubes for haemoglobin and haematocrit analyses. For those children who tested positive, their parents were also offered HIV testing. Testing for HIV was done by trained counsellors at the counselling unit of the hospital and consisted of two rapid HIV antibody tests (First Response and Ora Quick). Discordant results were retested with enzyme-linked immunosorbent assay (ELISA) and polymerase chain reaction (PCR).

The diagnosis of HIV disease was determined as follows: for HIV-1 DNA quantification, total HIV-1 DNA was extracted from 200 µL peripheral blood using Qiagen QIA symphony DNA Mini Kits (QIAGEN, Valencia, CA). The extraction of HIV-1 DNA and PCR for HIV-1 DNA was carried out using frozen samples. HIV-1 DNA in the peripheral blood [mainly white blood cells (WBCs)] was amplified and quantified for long terminal repeats gene using a fluorescence-based, real-time SUPBIO HIV Quantitative Detection Kit (SUPBIO, Guangzhou, China). The reaction system was as follows: reaction mixture 44.2 µL, enzyme 0.8 µL and DNA 5 µL. The housekeeping genes were amplified at the same time to quantify the cell amount. HIV-1 DNA were measured in duplicate and the quantification range of this assay was 20–5 × 10⁶ of 8 copies per 10⁶ WBCs. The amount of HIV-1 DNA per 10⁶ peripheral blood mononuclear cells was calculated. All patients' with positives results underwent confirmatory tests by ELISA and PCR before being admitted in the hospital, according to the National Protocol of Management of HIV in DR. Congo. Four trained nutritionists and laboratory technicians assisted with the analysis and the anthropometric measurements. The relevant laboratory analyses, socio-demographic, anthropometric and clinical data were then recorded into a case report form. Data were collected specifically for the purposes of this study throughout admission until discharge by the principal investigator. The diagnosis of urinary tract infection was made only if it was culture proven. Severe anaemia was diagnosed if the haemoglobin level was ⩽5 g dL⁻¹. Malaria diagnosis was determined in concordance with WHO (2008, 2009). Uncomplicated (mild) malaria was defined by the seeking of treatment for symptoms consistent with malaria (i.e. fever, headache), axillary temperature >37.5 °C and parasite density <500 000 µL⁻¹. Severe (life threatening) malaria was defined as hyperparasitaemia (⩾500 000 µL⁻¹) or the presence of any parasite density associated with one or more of the following clinical criteria: cerebral malaria (Blantyre coma score ⩽2, witnessed convulsions), severe anaemia (haematocrit level <15.0% or haemoglobin level <5 g L⁻¹), respiratory distress or prostration (inability to sit unassisted in a child usually able to do so) (Guindo et al., Reference Guindo, Fairhurst and Doumbo2007). The diagnosis of undernutrition was calculated by the BMI combined with evaluation of PB by the measured arm circumference, otherwise known as mid upper arm circumference (MUAC). Undernutrition was defined as BMI (kg m⁻²) between 16.0 and 18.4, whereas when the BMI varied between 18.5 and 24.0 it was considered to be well-nourished (good nutritional status). Good nutritional status by MUAC was defined when the PB was ⩾125 mm in children under 5 years of age, otherwise the child was considered to have undernutrition. In contrast, a PB ⩾ 145 mm was a good nutritional status in children aged 5–9 years, while <145 mm of PB was estimated as undernutrition status. HIV seropositive children were referred to the Kalembe-Lembe Hospital HIV clinic for comprehensive management and follow-up. A confirmatory HIV antibody test was performed at 18 months in HIV exposed children and the results were documented. Anthropometric index variable was assessed by three different computational models: percentages from the median, percentile or Z-score.

Statistical analysis

Data were transported to Stata Intercool version 11.2 (StataCorp LP, 4905 Lakeway Drive, College Station, TX, USA) for analysis. Any variable with the substantial level of missing data was excluded from the analysis. Categorical variables such as sex and some clinical variables were analysed and presented as percentages with their 95% confidence intervals (CIs). Continuous variables were analysed and presented as means with standard deviation (s.d.) for normally distributed variables, and median with inter-quartile ranges (IQR) for skewed variables. Associations between various clinical variables of malaria and HIV status were determined and reported as risk ratios (RR), with the corresponding 95% CIs and P values, using Fisher's exact test. A stepwise logistic regression (Wald χ ² statistic) was used to identify the most significant independent clinical predictors of malaria and HIV seropositivity. The diagnostic parameters (sensitivities, specificities, negative and positive predictive values) of the identified clinical predictors of malaria and HIV seropositivity were then determined. The clinical predictors were then combined in an algorithm to determine the likelihood of having malaria and HIV seropositivity based on the number of predictive clinical variables a child presents with. For all analysis, a two-sided P value ⩽0.05 was considered statistically significant.