Biomarker datasets

Micronutrient biomarker data from national and regional surveys were accessed from the BRINDA project (www.BRINDA-nutrition.org). The protocol was reviewed and approved by the London School of Hygiene & Tropical Medicine (LSHTM) ethics review committee. The methods for identifying datasets, inclusion and exclusion criteria and data management for the BRINDA project have been described in detail elsewhere^{(Reference Suchdev, Namaste and Aaron20)}. The surveys were nationally or regionally representative, and the BRINDA inclusion criteria were surveys that (1) were conducted after 2004, (2) had target groups including PSC, women of reproductive age or both, and (3) used a similar laboratory methodology for the measurement of at least one biomarker of iron or vitamin A status and at least one biomarker of inflammation (AGP or CRP). We included only surveys of PSC for which the following were available: (1) the measurement of ferritin and at least one inflammation marker (AGP or CRP) and (2) a measure of malaria infection by a standardised method.

Among the thirty datasets available for PSC, ten had information on current or recent malaria infection. However, one of them (Burkina Faso) used retrospective measurement of malaria antibodies in serum to define infection^{(Reference Martin-Prevel, Allemand and Nikiema21)}. This method is unlikely to detect only recent or current infections; thus, the dataset was not included in our database. The 2016 survey from Nepal did not detect any malaria case and was not included. In total, 7886 PSC from eight surveys were available for inclusion (online Supplementary Table 1). Nationally representative survey data were included from Cote d’Ivoire in 2007^{(Reference Rohner, Tschannen and Northrop-Clewes22)}, Cameroon in 2009^{(Reference Engle-Stone, Nankap and Ndjebayi23,Reference Engle-Stone, Ndjebayi and Nankap24)} , Liberia in 2011⁽²⁵⁾ and Malawi in 2016⁽²⁶⁾. Regional survey data were included from Kenya in 2007⁽²⁷⁾ and 2010^{(Reference Foote, Sullivan and Ruth28)}, Nigeria in 2012^{(Reference Maziya-Dixon, Sanusi and Oguntona29)} and Zambia in 2009^{(Reference Hotz, Palaniappan and Chileshe30)}. Only diagnosed infections with P. falciparum were included in the analysis.

Ferritin, AGP and CRP concentrations were assessed with the use of a sandwich ELISA at the VitMin Laboratory^{(Reference Erhardt, Estes and Pfeiffer31)} in all surveys – apart from Zambia, where the same analytical method was used in the Tropical Diseases Research Centre in Ndola. Current malaria infection was assessed with microscopy in Kenya (both surveys), Cote d’Ivoire, Nigeria and Zambia. Current or recent malaria infection was assessed with the Paracheck Pf rapid-diagnostic test (Orchid Biomedical System) in Liberia, the Malaria Ag CELISA kit (Cellabs Pty, Ltd) in Cameroon and the BIOLINE Malaria Ag P.f/Pan in Malawi. These three kits detect the presence of HRP2, a protein specific to P. falciparum ^{(Reference Mbanefo and Kumar9)}.

Inflammation adjustment

For each dataset individually, ferritin values were adjusted for inflammation using the regression approach with the BRINDA package^{(Reference Luo, Ayoya and Geng32)}. The regression approach has been described in detail elsewhere^{(Reference Namaste, Rohner and Huang5)} and uses linear regression to adjust ferritin concentrations by the CRP and AGP concentrations on a continuous scale. All the ferritin observations that have a corresponding CRP value, and/or AGP value above the first decile of the considered biomarker, were adjusted with linear regression. We decided to use the external deciles^{(Reference Suchdev, Namaste and Aaron20)} instead of individual survey deciles for consistency and because two of the individual surveys (Cote d’Ivoire and Zambia) had a very low first decile of CRP, suggesting a low level of inflammation.

Endemicity profile

When assessing malaria endemicity, parasite rate data constitute most of the global information available^{(Reference Hay and Snow33)} and are preferable to using prevalence data from surveys, which are likely to vary according to multiple factors including the survey timing and the seasonality of transmission. A malaria endemicity profile was therefore assigned to each study, considering the year the study was conducted and the study location (Table 1), using infection prevalence data extracted from the database hosted by the Malaria Atlas Project⁽³⁴⁾. It was not possible to identify subnational levels in our dataset, as the region or district names had been removed from the database. Therefore, subnational variations in endemicity were not considered. The data in the Malaria Atlas database were reported from 2010; therefore, the value for the year 2010 was used for surveys conducted before 2010. This was the case for Cameroon, Kenya, Zambia and Cote d’Ivoire. For these countries, other data sources on malaria prevalence were consulted, such as Demographic and Health Survey reports, to confirm the prevalence data; no discrepancies were noted⁽³⁵⁾. The different categories were defined by the WHO⁽¹¹⁾: very low intensity (PfP < 1 %), low intensity (PfP ≥ 1 % and < 10 %), moderate intensity (PfP ≥ 10 % and < 35 %) and high intensity (PfP ≥ 35 %).

Table 1. Endemicity profile of the survey settings from eight datasets from the BRINDA database in malaria endemic countries in Africa

PfP, Plasmodium falciparum infection prevalence.

Data were extracted from the Malaria Atlas Project database⁽³⁴⁾.

* Zambia was considered moderate as one province was in the moderate category and the other province was in the upper end of the low endemicity category.

In three of these datasets (Cote d’Ivoire, Kenya 2007 and Kenya 2010), additional information on the number of P. falciparum parasites was available. This was then converted into a parasitaemia level, which is the number of parasites per microlitre of blood, on the basis of 8000 leucocytes in one microlitre of blood. A low level of parasitaemia was defined as < 1000 parasites per microlitre of blood, based on previous publications^{(Reference Stoltzfus, Chwaya and Montresor36)}.

Statistical analysis

The outcome variable, inflammation-adjusted serum ferritin, was continuous. The exposure variable, malaria infection, was a binary variable (infected, uninfected). We examined the data to check for missing data, errors and inconsistencies and to gain an understanding of the distributions and patterns among the variables. We included only children who had a result for a malaria test and ferritin values. In the data, we examined the associations between the exposure and each potential confounder and potential effect modifier (age, sex, rurality, malaria endemicity profile and malaria diagnostic method), and between the outcome and each of these potential confounders and effect modifiers. Complex survey weights were accounted for when analysing individual data. Weights were not applied for pooled estimates, as the pooled dataset is used to assess a biological association and is not meant to be representative at any regional level; therefore, weights were also not used for the linear models which draw on the pooled dataset.

Linear model

A pooled multivariable linear regression analysis was conducted to estimate the association between malaria and inflammation-adjusted ferritin. To account for the clustering effect by country in the pooled database, we included the survey identifier in the model as a fixed effect. The dependent variable serum ferritin was transformed (natural log) to improve the original skewed distribution. Consequently, the regression model was built on the logarithmic scale. If the estimated coefficient for malaria is β̂, then a malaria infection was associated with a 100 × (e ^β̂ − 1) = x percent change in ferritin. The crude association between malaria and inflammation-adjusted ferritin was assessed. The model was then adjusted for each potential confounder, as follows: (1) individual characteristics such as age (categorical, in age group: < 2 years and > 2 years), sex, rural or urban location, and (2) variables likely to modify the relation between ferritin and malaria (malaria endemicity profile, malaria diagnostic method, age, sex and residence). A new model was created after adding each of these confounders and effect modifiers, and all the results of the different models are presented in online Supplementary Table 2. The confounders were selected based on plausible biological mechanisms and previously observed associations. Decisions about whether to include potential confounders in the final model were made according to whether their inclusion changed the effect estimate for the main exposure. Therefore, model A was chosen as the model for the analysis of the main effect of malaria on inflammation-adjusted ferritin, while model M was chosen as the final model with interactions. We limited the list of potential cofounders or effect modifiers to those available for all countries. For example, the presence of fever in the last 24 h, an important variable to define the stage of malaria infection, was available in only three datasets. Maternal education was not available for two of the datasets. Similarly, information regarding iron supplement consumption was available for only three datasets. Two-factor interaction of each predictor variable with malaria infection was tested. Interactions with P > 0·1 were removed from the model. Collinearity was examined with the variable inflation factor (VIF), which determines the strength of the correlation between independent variables. A VIF > 5 indicated high collinearity. The coefficients from the linear model M were used to calculate the malaria-adjusted biomarker concentrations and to estimate the prevalence of malaria-adjusted deficiency with the equation:

log(malaria-adjusted biomarker) = inflammation-adjusted biomarker + β̂(malaria) + β̂ _i (interactions) + survey identifier

When adding an interaction in the model, the main effect of each variable included in the interaction is also included in the model. Model checking was based on residual and normal probability plots. In the models presented in these analyses, the residual plots showed no fitted pattern, and linear relationship between the predictors and the outcome variables was assumed. The residuals were spread equally along the ranges of predictors, suggesting no heteroscedasticity. The normality assumption was checked with the QQ plot of residuals. All analyses were performed using R Statistical Software (v4.1.2; R Core Team 2022)^{(Reference Team37)}. Individual survey analyses, accounting for the complex survey design, were performed with the use of the ‘survey’ package in R 4.2.1 software^{(Reference Lumley38)}. Collinearity was assessed with the package ‘car’^{(Reference Fox and Weisberg39)}. The tables and graphs were made with the packages ‘kableExtra’, ‘interactions’ and ‘sjPlot’^{(Reference Long40–Reference Hao42)}. The protocol was reviewed and approved by the LSHTM observation research ethics committee (study reference 28219).