Enhanced Ex Vivo Plasmodium vivax Intraerythrocytic Enrichment and Maturation for Rapid and Sensitive Parasite Growth Assays

Rangel, Gabriel W.; Clark, Martha A.; Kanjee, Usheer; Lim, Caeul; Shaw-Saliba, Kathryn; Menezes, Marcelo Bezerra de; Mascarenhas, Anjali; Chéry, Lisly; Gomes, Edwin; Rathod, Pradipsinh K.; Ferreira, Marcelo U.; Duraisingh, Manoj T.

doi:10.1128/aac.02519-17

Cited by 45 publications

(100 citation statements)

References 31 publications

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“…Cryopreserved infected RBCs were thawed and cultured in IMDM medium (Gibco) supplemented with 0.5% Albumax II (Gibco), 2.5% heat-inactivated human serum, 25 mM HEPES (Gibco), 20 μg ml −1 gentamicin (Sigma) and 0.2 mM hypoxanthine (C-C Pro) for~24 or~48 h until a majority of schizont stage parasites were observed. The schizont-infected erythrocytes were enriched using KCl-Percoll density gradient 38 , then mixed at a ratio of 1 erythrocyte to 1 reticulocyte enriched from cord blood and labeled with CellTrace Far Red dye following manufacturer's instructions. The cultures were incubated for~8 h in a final volume of 50 μL in 96 well plates or 20 μL in 384 well plates, in presence of the human monoclonal antibodies.…”

Section: Methodsmentioning

confidence: 99%

Amplification of Duffy binding protein-encoding gene allows Plasmodium vivax to evade host anti-DBP humoral immunity

et al. 2020

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Antigenic variation, the capacity to produce a range of variable antigens, is a well-described strategy of Plasmodium and other parasites to evade host immunity. Here, we show that gene amplification is an additional evasion mechanism used by Plasmodium vivax to escape humoral immunity targeting PvDBP, the key ligand involved in reticulocyte invasion. PvDBP gene amplification leads to increased mRNA levels and protects P. vivax in vitro against invasion inhibitory human monoclonal antibodies targeting a conserved binding domain of DBP. Patient samples suggest that parasites with increased pvdbp copy number are able to infect individuals with naturally acquired antibodies highly blocking the binding of PvDBP to the Duffy receptor. These results show that gene copy number variation affect the parasite's ability to evade anti-PvDBP humoral immunity.

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Section: Methodsmentioning

confidence: 99%

Amplification of Duffy binding protein-encoding gene allows Plasmodium vivax to evade host anti-DBP humoral immunity

et al. 2020

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“…increasing drug concentrations, but the use of these assays has been limited until recently by the lack of practical and standardized protocols (4,5). Moreover, results may be affected by previous or concomitant antimalarial use, patterns of parasite synchronicity in clinical samples, and time delays in processing field-collected samples (6).…”

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confidence: 99%

Monitoring the Efficacy of Chloroquine-Primaquine Therapy for Uncomplicated Plasmodium vivax Malaria in the Main Transmission Hot Spot of Brazil

Ladeia‐Andrade

et al. 2019

Antimicrob Agents Chemother

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Emerging Plasmodium vivax resistance to chloroquine (CQ) may undermine malaria elimination efforts in South America. CQ-resistant P. vivax has been found in the major port city of Manaus but not in the main malaria hot spots across the Amazon Basin of Brazil, where CQ is routinely coadministered with primaquine (PQ) for radical cure of vivax malaria. Here we randomly assigned 204 uncomplicated vivax malaria patients from Juruá Valley, northwestern Brazil, to receive either sequential (arm 1) or concomitant (arm 2) CQ-PQ treatment. Because PQ may synergize the blood schizontocidal effect of CQ and mask low-level CQ resistance, we monitored CQ-only efficacy in arm 1 subjects, who had PQ administered only at the end of the 28-day follow-up. We found adequate clinical and parasitological responses in all subjects assigned to arm 2. However, 2.2% of arm 1 patients had microscopy-detected parasite recrudescences at day 28. When PCR-detected parasitemias at day 28 were considered, response rates decreased to 92.1% and 98.8% in arms 1 and 2, respectively. Therapeutic CQ levels were documented in 6 of 8 recurrences, consistent with true CQ resistance in vivo. In contrast, ex vivo assays provided no evidence of CQ resistance in 49 local P. vivax isolates analyzed. CQ-PQ coadministration was not found to potentiate the antirelapse efficacy of PQ over 180 days of surveillance; however, we suggest that larger studies are needed to examine whether and how CQ-PQ interactions, e.g., CQ-mediated inhibition of PQ metabolism, modulate radical cure efficacy in different P. vivax-infected populations. (This study has been registered at ClinicalTrials.gov under identifier NCT02691910.)

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“…Having established that the youngest CD71 + reticulocytes that are preferred by P. vivax for invasion 13,14 are the most osmotically stable of all enucleated RBCs, we next assessed the impact of P. vivax infection on reticulocyte osmotic stability. In the absence of continuous P. vivax in vitro culture, cryopreserved clinical P. vivax samples are an invaluable resource for investigating P. vivax biology [40][41][42][43] . Cognizant of the decreased stability of cryopreserved RBCs, however ( Fig.…”

Section: Resultsmentioning

confidence: 99%

“…Indian and Brazilian clinical P. vivax samples and P. falciparum 3D7 P2G12 were cultured at 100 × 10 6 cells per mL in IMDM (Gibco) containing 10% AB + heat-inactivated sera and 50 µg/mL gentamicin at 37 o C in 5% CO 2, 1% O 2 , and 94% N 2 as previously described 40 . Hemacolor-stained cytospins were prepared and 200 cells per slide (1000x magni cation) were called as either asexual stage (I-V) or gametocyte 60 .…”

Section: P Vivax and P Falciparum In Vitro Culturementioning

confidence: 99%

Plasmodium vivax infection compromises reticulocyte stability.

Clark

Kanjee

Rangel

et al. 2020

Preprint

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The structural integrity of the host red blood cell (RBC) must be maintained for propagation of Plasmodium spp. during the disease causing blood-stage of malaria infection. Plasmodium vivax infection is restricted to reticulocytes. To assess the impact of P. vivax infection on reticulocyte stability, we developed a flow cytometry-based assay capable of measuring osmotic stability within heterogeneous RBC populations. We found that P. vivax preferred young reticulocytes are more osmotically stable than older reticulocytes and normocytes, and P. vivax infection decreased reticulocyte stability to levels observed for RBC disorders that cause hemolytic anemia. Moreover, P. vivax reticulocyte destabilization was more significant than P. falciparum normocyte destabilization. Finally, we found that P. vivax new permeability pathways contribute to the decreased osmotic stability of infected-reticulocytes. These results reveal a key vulnerability of P. vivax that could be manipulated to yield both in vitro culture and novel therapeutics.

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Enhanced Ex Vivo Plasmodium vivax Intraerythrocytic Enrichment and Maturation for Rapid and Sensitive Parasite Growth Assays

Cited by 45 publications

References 31 publications

Amplification of Duffy binding protein-encoding gene allows Plasmodium vivax to evade host anti-DBP humoral immunity

Amplification of Duffy binding protein-encoding gene allows Plasmodium vivax to evade host anti-DBP humoral immunity

Monitoring the Efficacy of Chloroquine-Primaquine Therapy for Uncomplicated Plasmodium vivax Malaria in the Main Transmission Hot Spot of Brazil

Plasmodium vivax infection compromises reticulocyte stability.

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