Between 2017 and 2021, blood samples were collected from 29 patients with imported severe malaria with hyperparasitemia (>4% parasitemia) in France. Severe cases were defined by a positive blood smear with asexual forms of P. falciparum associated with at least one of the WHO’s severity criteria. All the patients included were involved in the national surveillance program of the French National Reference Center for Malaria and were treated by first-line treatment with intravenous artesunate (2.4 mg/kg, Guilin Pharmaceutical), or other artemisinin derivatives (Eurartesim 320 mg/40 mg, ≥ 35 kg: four tablets; or artemether Lumefantrine 20 mg/120 mg, ≥ 75 kg: 4 tablets).

RBC from patients before or after treatment and RBC control from blood bank were washed 4 times in RPMI 1640 GlutaMAX containing HEPES (Life Technologies) and cryopreserved in 50% PBS1X in liquid nitrogen until lipidomic analysis by HPLC and MS/MS. Lipid extraction was performed according to a modified chloroform/methanol (2:1, v/v) procedure (Petkovic et al., 2005). Briefly, frozen samples were transferred into a 15 ml tube and 2 ml of chloroform/methanol (2:1, v/v) was added; chloroform (Sigma 288,,306-1 L), methanol (Fisher 10675112). The suspension was vortexed and incubated at room temperature with agitation for 20 min. After the incubation, 400 µL of 0.9% NaCl was added to the mixture and was then vortexed and centrifuged at 500 x g for 10 min to separate the organic phase from the aqueous phase. The chloroform (lower) layer was transferred into a new 1.5 ml tube and was centrifuged at 500 x g for 10 min. Finally, the supernatant was collected without touching the pellet and was transferred into a new 1.5 ml tube. Internal standards (Cer d18:1/15:0, 16 ng; PE 12:0/12:0, 180 ng; PC 13:0/13:0, 16 ng; SM d18:1/12:0, 16 ng; PI 16:0/17:0, 30 ng; PS 12:0/12:0, 156.25 ng; all from Avanti Polar Lipids) were added to 45 µL of lipid extract. Sample solutions were analyzed using an Agilent 1290 UPLC system coupled to a G6460 triple quadripole spectrometer (Agilent Technologies). MassHunter software was used for data acquisition and analysis. A Kinetex HILIC column (Phenomenex, 50 × 4.6 mm, 2.6 μm) was used for LC separations. The column temperature was maintained at 40°C. Mobile phase A was acetonitrile and B was 10 mM ammonium formate in water at pH 3.2. The gradient was as follows: from 10 to 30% B in 10 min, 100% B from 10 to 12 min, and then back to 10% B at 13 min for 1 min to re-equilibrate prior to the next injection. The flow rate of the mobile phase was 0.3 ml/min, and the injection volume was 5 μL. An electrospray source was employed in positive (for Cer, PE, PC, and SM analysis) or negative ion mode (for PI and PS analysis). The collision gas was nitrogen. Needle voltage was set at +4,000 V. Several scan modes were used. First, to obtain the naturally different masses of different species, we analyzed cell lipid extracts with a precursor ion scan at 184 m/z, 241 m/z, and 264 m/z for PC/SM, PI, and Cer, respectively. We performed a neutral loss scan at 141 and 87 m/z for PE and PS, respectively. The collision energy optimums for Cer, PE, PC, SM, PI, and PS were 25 eV, 20 eV, 30 eV, 25 eV, 45 eV, and 22 eV, respectively. The corresponding SRM transitions were used to quantify different phospholipid species for each class. Two MRM acquisitions were necessary, due to important differences between phospholipid classes. Data were treated with QqQ Quantitative (vB.05.00) and Qualitative analysis software (vB.04.00).

RBC from patients before or after treatment and RBC control were washed 4 times in RPMI 1640 GlutaMAX containing HEPES (Life Technologies) and fixed with 1% glutaraldehyde diluted in PBS 1X. After two washes in PBS1X, samples were incubated with a human polyclonal hyper immune serum (Buffet et al., 2006) at 1:10 in PBS with 1% Albumax II (Life Technologies) and 0.1% Triton X100 (Sigma Aldrich) for membrane permeabilization. After 25 min of incubation under agitation, samples were washed two times in PBS1X and incubated with a secondary antibody goat anti-human IgG coupled with either Alexa Fluor 488 or 568 at 1:500 (Life technologies) or Dylight755 (Invitrogen) at 1:100. Based on the color of the secondary antibody already used, DNA was labeled with either Hoechst 34,580 at 1:1000 or SybrGreen at 1:5000 (Life Technologies) for 25 min. Parasitemia and pittemia were finally measured by the cytometer BD FACSCanto^TMII, BD Biosciences and analyses were performed using FlowJo software.

After blood collection, elongation indexes of each sample diluted at 1:100 in Polyvinylpyrrolidone polymers buffer (RR mechatronics) were measured by ektacytometry with shear stress from 0.3 to 30Pa. All the samples were processed within 48 h after blood collection. A laser-assisted optical rotational cell analyzer (LORRCA, RR Mechatronics) was used to calculate the elongation index, which is defined as the ratio of the difference between two axes of the ellipsoidal diffraction pattern and the sum of these two axes. An elongation index at 1.69 Pa shear stress reflects deformability due to membrane rigidity and 30 Pa shear stress reflects deformability due to intern viscosity (Baskurt OK et al. Clin Hemorheol Microcirc. 2009). A one-way Anova parametric unpaired t-test with Bonferroni’s correction was performed for statistical analysis.

Filtration of RBCs was performed using a mix of calibrated metal microbeads (Industrie des Poudres Sphériques, France), composed of 70% of 5–15 µm diameter and 30% of 15–25 µm diameter and supported by a layer of 25–45 µm diameter microbeads. The beads were distributed in a special 96-well plate adapted for microsphiltration as described in Deplaine et al. Blood 2011. RBCs were prepared at 2% hematocrit (or 1% if parasitemia exceeded 10%) in PBS 1X/1% Albumax II. For each well, 200 µL of RBC suspension were loaded and filtered by aspiration. Wells were flushed with 1.6 ml of PBS/1% Albumax II and downstream suspension was collected. Healthy RBC fixed with 1% glutaraldehyde or not were used as controls. Retention rate was calculated as following [(% Downstream - % Upstream)/% Upstream] x100. Positive values represented enrichments and negative values retentions.

Statistical analyses were performed using GraphPad PRISM six software. For Hb comparison before and after therapy, only patients with available data in both periods were analyzed by a paired t-test with a normal distribution (D'Agostino and Pearson test). Differences at p < 0.05 were considered significant. For populational analysis, deformability index and retention rate in microsphiltration, RBC parameters were compared before and after therapy and with healthy RBC from blood bank. Anova test was used when appropriate with a Bonferroni correction. One asterisk (*) identifies adjusted p values between 0.01 and 0.05, two asterisks (**) identify adjusted p values between 0.01 and 0.001.

Hemoglobin (Hb) decline was 1.93G/dl with a mean Hb level of BT of 12.86 G/dl vs. 11.01 G/dl AT (n = 13, p = 0.0003, Figure 1). RBC loss was thus of 15.9% (or less since a small part of the hemoglobin drop was due to hemodilution AT (Levin et al., 2001; Drevon et al., 2021). During the same period, the loss of iRBC was 5.9%, and the gain of pitted RBC was 5.1% of all RBC, corresponding to a net loss of 0.8% of total RBC. Altogether, the net loss of the subpopulation of RBC directly modified by invasion of RBC by parasites accounted for minor part of the total loss of RBC during this period. The bulk of Hb loss was therefore related to the elimination of RBC that had never been infected (niRBC).

We measured the composition of lipids (de novo biosynthesis or uptake by P. falciparum) in RBC samples BT and at complete clearance of parasites AT. A lipidomic analysis including cholesterol (Chol), four phospholipids (phosphatidylethanolamine: PE, phosphatidylinositol: PI, phosphatidylcholine: PC and phosphatidylserine: PS), and two sphingolipids (ceramide and sphingomyelin) was performed by HPLC and MS/MS on membrane extracts from RBC collected in infected patients BT and AT. RBC from healthy donors were used as controls. Regarding ceramide, PC, PS and sphingomyelin, no significant variations were observed between RBC from healthy donors and RBC from infected patients either BT or AT. Conversely, compared to healthy controls (400.5 arbitrary units (AU), n = 12, Figure 2), total Chol amounts were slightly higher than controls BT (433.6, p = 0.491) and significantly higher than controls AT (479.5 AU, p = 0.020). Compared to healthy controls, PE and PI contents were higher BT (2,111 vs. 2665 AU, n = 10, p = 0.021 for PE and 883 vs. 1192 AU, n = 10, p = 0.095 for PI, Figure 2A); and then decreased significantly AT to control levels (2082 AU, n = 12, p = 0.009 for PE and 850 AU, n = 12, p = 0.0462 for PI, Figure 2A). When we analyzed Chol/PE or Chol/PI ratio that are associated with membrane deformability and stability, both the Chol/PI and Chol/PE ratio increased significantly AT compared to BT (0.24 vs. 0.17, p < 0.001 for Chol/PE and 0.67 vs. 0.36 for Chol/PI, p = 0.001, Figure 2B). These results suggest that infection, treatment, and pitting altered the lipid composition of RBC plasma membranes.

Changes in the lipid contents of RBCs have been shown to be associated to altered deformability and may contribute to their elimination by the spleen (Sarkar et al., 2018; Martinez-Vieyra et al., 2019). The deformability of RBC collected either BT (parasitemia ranging from 1 to 10.7%, n = 12) or AT (concentrations of pitted RBC ranging from 0.4 to 12%, n = 16), was quantified by ektacytometry and compared to RBC from healthy donors (CTL, n = 27). RBC deformability was significantly lower than controls both BT and AT with and elongation Index (EI) at 1.69 Pa of 0.24 BT and 0.23 AT vs. 0.28 in healthy donors (n = 28, p < 0.0001). At 30 Pa EI was 0.56 BT and 0.56 AT vs. 0.60 in healthy donors (n = 27, p < 0.001 (Figures 3A, B). This suggests that their decreased deformability is related to infection-related increase in membrane rigidity or internal viscosity, or both. These results also show that alterations in circulating RBC are not immediately restored after treatment with AD. Finally, the ability of RBC subpopulations (iRBC BT and pitted RBC AT) to cross splenic inter-endothelial slits was assessed using a spleen-mimetic method where microsphere-based filters quantify the retention rates (rr) of RBC subpopulations (Deplaine et al., 2011; Ndour et al., 2015; Depond et al., 2019) (Figure 3B). Both iRBC (n = 6) and pitted RBC (n = 7) were more retained in microsphere layers than healthy controls (n = 8), at strikingly similar levels (mean rr iRBC: 20% and rr pitted RBC: 19%, Figure 3C).