Figure 1
Figure 1. An overview of the assay methodology. Thin smears stained with new methylene blue (A-B) or Giemsa (D-G) illustrating the key methodologic steps of the ex vivo P vivax invasion assay. (A) Cord blood at collection contains a mixture of normocytes, reticulocytes, and leukocytes. (B) After 2 rounds of leukocyte depletion on a CF-11 cellulose column, reticulocytes form the majority of the cells present in the band (seen at the 5.5-mL mark on the tube pictured in panel C) obtained by enrichment on a 70% Percoll cushion. (D) Thin smear showing mature trophozoites (black arrows) and leukocytes typically observed from P vivax isolates collected from patients. (E) Typical yield of concentrated mature P vivax parasites obtained on a 45% Percoll cushion (from a band similar to the one depicted in panel C after a single round of leukocyte depletion on CF-11 and 20 hours ex vivo maturation). (F) The concentrated reticulocyte target cells (B) and mature P vivax schizonts (E) are mixed at a ratio of 6:1 for the invasion assay. (G) After culturing for ∼ 24 hours, the invasion assay mixture shows remnants of ruptured schizonts (*), and RBCs newly invaded by one (black arrow) or multiple merozoites (orange arrowhead). Black scale bar on the micrographs corresponds to 10 μm.

An overview of the assay methodology. Thin smears stained with new methylene blue (A-B) or Giemsa (D-G) illustrating the key methodologic steps of the ex vivo P vivax invasion assay. (A) Cord blood at collection contains a mixture of normocytes, reticulocytes, and leukocytes. (B) After 2 rounds of leukocyte depletion on a CF-11 cellulose column, reticulocytes form the majority of the cells present in the band (seen at the 5.5-mL mark on the tube pictured in panel C) obtained by enrichment on a 70% Percoll cushion. (D) Thin smear showing mature trophozoites (black arrows) and leukocytes typically observed from P vivax isolates collected from patients. (E) Typical yield of concentrated mature P vivax parasites obtained on a 45% Percoll cushion (from a band similar to the one depicted in panel C after a single round of leukocyte depletion on CF-11 and 20 hours ex vivo maturation). (F) The concentrated reticulocyte target cells (B) and mature P vivax schizonts (E) are mixed at a ratio of 6:1 for the invasion assay. (G) After culturing for ∼ 24 hours, the invasion assay mixture shows remnants of ruptured schizonts (*), and RBCs newly invaded by one (black arrow) or multiple merozoites (orange arrowhead). Black scale bar on the micrographs corresponds to 10 μm.

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