Lipidic Vacuoles in Plasmodium knowlesi Erythrocytic Schizonts

ABSTRACT. Electron microscopy of schizont development in erythrocytic Plasmodium knowlesi has revealed that spheroidal vacuoles 250 nm in diameter with semi-dense contents appear at the periphery of the parasite prior to the budding of merozoites. When treated with non-polar solvents, their contents are completely extracted, and after fixation in tannic-glutaraldehyde they contain regular lamellae with a periodicity of 5.5 nm. Both of these reactions are typical of lipids. Some of these structures are associated with phagosomal vacuoles which may contribute to their lamellae. They disappear at the onset of merozoite formation, but membranous whorls of various sizes continue to be associated with the schizont surface during budding of merozoites. It is suggested that the lipidic vacuoles are a source of preformed lipid which can be utilized rapidly during the generation of merozoites.     

Etude Ultrastructurale des Mérozoites et de la Schizogonie des Coccidies (Eimeriina): Eimeria magna (Perard 1925) de I'Intestin des Lapins et E. tenella (Railliet et Lucet, 1891) des Coecums des Poulets

SYNOPSIS. An electron microscopic study is made of merozoites and schizogony of Eimeria magna and Eimeria tenella from rabbits and chickens infected 5 days before fixation.
The merozoite outer layer is formed by a unit membrane lined by a dense osmiophilic layer. A micropyle is present. The apical complex of the cell is constituted by a conoid surmounted by 2 rings and surrounded by another from which about 26 subpellicular, tubular fibrils start. Two "rhoptries" (= toxonemes) go thru the conoid to the apex of cell. Rare sarconemes (= convoluted tubes) are disseminated in the anterior part of merozoites. A nucleus with nucleolus, Golgi apparatus, mitochondria, endoplasmic reticulum, lipid globules and glucidic grains were observed.
Schizogony starts by the formation of a multinucleated schizont which has a centriolar structure. The new merozoites appear as evaginations of the schizont's membrane. Cellular organelles (conoid, rhoptries, micropyle, sarconemes) differentiate and the nuclei enter the diverticula of the schizont. Then the development of merozoites proceeds by "external budding".
The ultrastructural similarities between the merozoites of Eimeria and the endodyocytes of Toxoplasmea, appear to us to be extremely interesting and indicate a close relationship between the Toxoplasmea and the Coccidia.     

Monoclonal antibody characterization of Plasmodium falciparum antigens in immune complexes formed when schizonts rupture in the presence of immune serum

When Plasmodium falciparum parasites are cultured with some immune sera, merozoites are agglutinated by antibodies to form immune clusters of merozoites and prevent their invasion into erythrocytes. Within these immune clusters of merozoites, several antigens that are normally found in the soluble fraction after detergent extraction accumulate in relatively insoluble immune complexes. From mice immunized with these immune complexes, we obtained hybridomas secreting monoclonal antibodies (mAb) that react with various immune clusters of merozoites antigens, including mAb 3D5, which recognizes a 101-kDa antigen (p101) and mAb, 5E3, which recognizes a 113-kDa antigen (p113). Both mAb reacted with antigens at the surface of schizonts, in the vacuolar space, and at the surface of merozoites before their release from schizont-infected cells. Both p101 and p113 were synthesized by mature trophozoites and young schizonts. In pulse-chase experiments, p113 was processed to 100-, 70-, 55-, and 50-kDa products. Both p101 and p113 appeared in the culture medium when schizont rupture occurred in normal culture medium but were found in immune complexes when schizont rupture occurred in the presence of immune serum. Antibodies in immune complexes, when dissociated with acid and used to probe immunoblots, reacted with affinity-purified p101 and p113. Antigens such as these, which are accessible at the parasite surface and react with antibodies present in immune serum that inhibits parasite invasion, are logical candidates to study in the search for a vaccine against the erythrocytic stages of malaria.     

Plasmodium falciparum antigens synthesized by schizonts and stabilized at the merozoite surface by antibodies when schizonts mature in the presence of growth inhibitory immune serum

Some immune sera that inhibit erythrocyte invasion by merozoites also agglutinate the merozoites as they emerge from rupturing schizonts. These immune clusters of merozoites (ICM) possess a surface coat that is cross-linked by antibody and is thicker than the surface coat associated with normal merozoites (NM) obtained from cultures containing preimmune serum. Analysis of metabolically labeled ICM and NM performed by using sodium dodecyl sulfate-polyacrylamide gel electrophoresis showed that washed ICM possessed immune complexes containing antigens representative of schizonts and merozoites. Characteristics of the immune complexes included: a) they were not soluble in pH 8 Triton X-100, b) they were soluble at an acid pH, and c) after pH neutralization they were precipitated by using staphylococcal protein A. Merozoite antigens having Mr of 83, 73, and 45 kDa were associated with immune complexes in ICM. The 83 and 73 kDa antigens were recovered in considerably larger quantities from ICM than from NM. Schizont antigens having Mr of 230, 173 (triplet), 152 (doublet), and 31 kDa were associated with immune complexes in ICM, and a 195 kDa antigen(s) from schizonts and merozoites was also present in the immune complexes. In addition, other antigens of Mr 113, 101, 65, and 51 kDa may have been immune complexed. These 15 antigens accounted for less than 30% of the schizont and merozoite antigens recognized by the immune serum. Immune complexes probably formed between antibodies and a) surface antigens of schizont-infected erythrocytes exposed to antibody before schizont rupture, b) surface antigens of merozoites and schizonts exposed during schizont rupture, and c) soluble antigens normally released during schizont rupture. The antibody components of the immune complexes may have prevented rapid degradation or shedding of some antigens from the merozoite surface. Allowing schizonts to rupture in the presence of inhibitory antibodies (to form ICM) is a useful approach to identifying exposed targets of protective immunity against malaria.     

Fine structure of the erythrocytic stages of Plasmodium knowlesi

Summary The fine structure of erythrocytic stages of Plasmodium knowlesi was compared with that of the same parasite isolated from its host cell by a saponin technique. Rhesus monkeys experimentally infected with Plasmodium knowlesi were the source of parasitized red cells. The erythrocytic stages of this Plasmodium showed all the organelles described in other mammalian forms; the nucleus lacked a typical nucleolus but contained a cluster of granules. P. knowlesi did not have protozoan-type mitochondria as do the avian and reptilian forms, but had double-membrane-bounded bodies as observed in other mammalian malarial parasites.The isolation procedure caused a slight swelling of the parasite, but in general, the structure and structural relationships of the parasite were preserved. However, the isolation technique gave a new insight into the connection of the host cell cytoplasm with the large, so-called food vacuoles of the parasite. The parasite freed from its host cell showed clear spaces where the large vacuoles had been. The content of these vacuoles had been removed together with the red cell cytoplasm. As the nature of the isolation procedure precluded any disruption of the parasite itself, these findings support our view that the vacuoles are not true food vacuoles. If these were true food vacuoles, they would be completely enclosed by a parasite membrane within the parasite cytoplasm. However, we have demonstrated that they represent extensions of host cell cytoplasm in direct communication with the rest of the red cell. The outer membrane surrounding the intra-erythrocytic parasites disappeared after isolation of the parasite from the host cell. This strongly suggested that the outer membrane is of host cell origin. The budding process of the merozoites from a schizont was also described and discussed.This paper is contribution No. 558 from the Army Research Program on Malaria and was supported in part by Research Grant AI 08970-01 from the United States Public Health Service.     

Investigations into the fire structure of the asexual developmental stages of Frenkelia in the liver of the bank vole (author's transl)]

Bank voles (Clethrionomys glareolus) were infected by stomach tube with Frenkelia sporocysts from the faeces of buzzards (Buteo buteo). The voles were sacrificed at regular intervals and their livers examined electronmicroscopically. Seven days p.i. developmental stages of Frenkelia could be detected in liver parenchymal cells. The youngest schizonts detected are enveloped by a pellicle consisting of two membranes. This pellicle, which is in direct contact with the host cell mitochondria, shows marked invaginations which increase with the development of the schizont. A parasitophorous vacuole is not detectable. In developing schizonts numerous sections through nuclei with nucleic spindles and merozoite anlagen (dome-shaped) structures) are visible. It is not clear whether there are several nuclei or a section through one large and lobed nucleus. Within the merozoite anlagen the conoid and the subpellicular microtubules are formed first. By the prolongation of the dome-shaped structures towards the posterior pole, the nucleus and the other newly formed cell organelles are incorporated into the forming merozoite. The posterior pole of the merozoite still remains open at this stage of development. With increasing differentiation the merozoites become lancet-shaped, their apical poles bing always directed towards the periphery of the schizont. The outer membrane of the pellicle of the schizont forms the outer part of the pellicle of the merozoites by invaginating around them. At this stage of development the inner membrane of the pellicle of the schizont is no longer detectable. Thus the typical pellicle of the motile stages of sporozoaonsisting of three membranes is formed. In the centre of the merozoites which lie freely in the liver cell a residual body is present. The host cell reacts against the parasites by forming a thick border of mitochondria and distinct endoplasmic reticulum.     

The Fine Structure of Some Developmental Stages of Mattesia grandis McLaughlin (Sporozoa, Neogregarinida), a Parasite of the Boll Weevil Anthonomus grandis Boheman

SYNOPSIS Sporozoites, macronuclear schizonts, merozoites and gamonts of Mattesia grandis were examined by electron microscopy. A conoidal complex, consisting of conoid, polar rings and subpellicular microtubules was present in all of these stages. The conoidal complex was similar in structure to the same organelle of other Sporozoa. The conoidal complex in mono- to quadrinucleate macronuclear schizonts is transformed into an organelle similar to the mucron of some eugregarines.
This mucron consists of a specialized area of the cell membrane from which fine fibers extend into a large vacuole situated directly beneath the cell membrane. The top part of the vacuole is encircled by 2 ring-like structures formed by the dilatation of the original apical rings. The vacuole of the mucron contains many anastomosing protrusions of the cytoplasm, suggesting a nutritional role. The mucron disappears when the schizont reaches the multinucleate state. Later the merozoites bud from the surface of the schizont as in the coccidia. Each merozoite again has a conoidal complex, which persists thru the gamont stage and usually serves as the point of contact between 2 gamonts during their pairing.
The presence of a conoidal complex thru a major portion of the life cycle, its transformation into a mucron and the mode of formation of merozoites indicate that the Neogregarinida combine the fine structure characters of both the Eugregarinida and the Eucoccida, thereby suggesting a phylogenetic relationship between these sporozoans, with the neogregarines as a link between eugregarines and coccidia.     

The Fine Structure of Differentiating Merozoites of Haemoproteus columbae Kruse*

SYNOPSIS. The first sign of merozoite formation in schizonts of Haemoproteus columbae is the accumulation of dense material at intervals beneath the plasma membrane of the schizont. The schizont's membrane then invaginates in deep furrows cleaving the parasite into pseudo-cytomeres. thereby increasing the area of membrane available for differentiation. Signs of differentiation appear under this membrane as soon as it is formed. Rhoptries and polar rings develop in the region of the dense accumulations, the cytoplasm containing these structures begins to elevate, and each evagination differentiates into a merozoite. When the merozoite is half-formed, the cytostome appears, then dense bodies at the apex of the organism, and finally a spherical body intimately associated with a mitochondrion. These merozoites of Haemoproteus are assumed to be the forms that penetrate erythrocytes and become gametocytes. They contain the same organelles as merozoites of Plasmodium. However, the merozoites of Haemoproteus are oval like the erythrocytic merozoites of Plasmodium rather than elongate like the exoerythrocytic merozoites. This body shape may be a generic characteristic or it may indicate a structural difference between exoerythrocytic merozoites and merozoites that infect erythrocytes. When the merozoites of Plasmodium, Haemoproteus and Leucocytozoon are compared, the first 2 genera appear closely related, but Leucocytozoon seems very different. Perhaps it should not be included within the Haemoproteidae.     

The Malarial Serine Protease SUB1 Plays an Essential Role in Parasite Liver Stage Development

Transmission of the malaria parasite to its vertebrate host involves an obligatory exoerythrocytic stage in which extensive asexual replication of the parasite takes place in infected hepatocytes. The resulting liver schizont undergoes segmentation to produce thousands of daughter merozoites. These are released to initiate the blood stage life cycle, which causes all the pathology associated with the disease. Whilst elements of liver stage merozoite biology are similar to those in the much better-studied blood stage merozoites, little is known of the molecular players involved in liver stage merozoite production. To facilitate the study of liver stage biology we developed a strategy for the rapid production of complex conditional alleles by recombinase mediated engineering in Escherichia coli, which we used in combination with existing Plasmodium berghei deleter lines expressing Flp recombinase to study subtilisin-like protease 1 (SUB1), a conserved Plasmodium serine protease previously implicated in blood stage merozoite maturation and egress. We demonstrate that SUB1 is not required for the early stages of intrahepatic growth, but is essential for complete development of the liver stage schizont and for production of hepatic merozoites. Our results indicate that inhibitors of SUB1 could be used in prophylactic approaches to control or block the clinically silent pre-erythrocytic stage of the malaria parasite life cycle.     

Endogenous development of Eimeria intestinalis in rabbits (Oryctolagus cuniculus).

The endogenous life cycle of a pure strain of Eimeria intestinalis was studied by light and electron microscopy in coccidia-free rabbits. Four schizont generations could be observed: the first one, not previously described, was seen between 36 and 144 hr postinoculation (PI), the second one between 64 and 168 hr PI, the third one between 96 and 192 hr PI, and the fourth one between 168 and 240 hr PI. Gamogony apparently started as early as 144 hr PI. Thus, it was possible for oocysts to develop from third generation merozoites, later oocysts developing after the fourth schizont generation. Electron microscopic observation suggested that oocysts were derived mainly from merozoites of the fourth schizont generation. During the first stage of the life cycle, sporozoites were seen in intraepithelial lymphocytes. All asexual generations, except the fourth, were characterized by 2 schizont types: the first, regarded as female, contained mononuclear merozoites and the second, regarded as male, contained polynuclear merozoites.     

Secretion of multilamellar whorls by Eimeria tenella zoites.

Multilamellar whorls were demonstrated by transmission electron microscopy to be associated with sporozoites and all generations of merozoites of Eimeria tenella, in chicken cecal tissue fixed without tannic acid or ruthenium red at room temperature. Whorls were found within the parasitophorous vacuoles of recently invaded cells at all stages of development, suggesting a role in the formation of the host parasite interface. Whorls were also associated with intraluminal third-generation merozoites prior to host cell invasion and appeared to be secreted directly through the pellicle. Membranous sheaths, shown by serial sectioning to be derived from intracellular whorl material, were observed enveloping some intraluminal merozoites. In many third-generation merozoites, whorl material was located within discrete novel organelles (here termed lamellosomes) located in the apical region. These densely staining spherical organelles were morphologically distinct from micronemes and rhoptries and were one-third the size of dense granules. These findings confirm that whorls are nonartifactual secretions whose lamellar organization is lost during normal fixation on ice without tannic acid. It is hypothesized that whorls secreted prior to invasion are involved in protection of the motile zoite, immune evasion, or some aspect of gliding motility.     

Structure and development of the surface coat of erythrocytic merozoites of Plasmodium knowlesi

Summary The surface of extracellular merozoites of P. knowlesi is covered with a coat 15–20 nm thick, made up of clusters of filaments standing erect on the plasma membrane. Filaments have stems 2 nm thick, the peripheral ends of which are complex, branching or ending in long trailing threads. Coat filaments occur on the surface of the parasite in regular rows at an early schizont stage, and persist until well after merozoite release. They are sensitive to trypsin and papain, and bind ethanolic phosphotungstate, indicating a proteinaceous nature. They are also removed by exposure to phosphate-buffered saline. Filaments bear negative charges, binding cationised ferritin throughout the depth of the coat and staining with ruthenium red. They cover the whole merozoite surface and mediate intercellular adhesion at distances of 15–150 nm, membrane to membrane. It is suggested that these filaments correspond to a major merozoite surface protein, and are important in the initial capture of red cells.     

鸡沙氏住白虫的生活史研究

本文报告了鸡沙氏住白虫生活史及其全程发育。经人工实验和流行区调查证明,后宽绳蚋是该虫的自然传播媒介。孢子增殖在后宽绳蚋体内、经3—4天完成发育。无性裂殖体增殖在鸡的肝、肾、心、肺、脾、脑和肠等内脏器官组织细胞内进行,经4—9天完成发育,该裂殖体有二型,即肝裂殖体和巨噬细胞裂殖体。感染9—13天后,血细胞内的配子体发育成熟。感染后第15—25天末稍血液中出现虫体的高峰期。     

毁灭泰泽球虫(Tyzzeria perniciosa)内生发育的超微结构研究——Ⅰ.裂殖生殖(Schizogony)

利用透射电镜对寄生于北京鸭小肠的毁灭泰泽球虫的裂殖生殖过程进行了观察。滋养体内未见多糖颗粒、脂肪体和致密体,在细胞质的被膜空泡内发现退化的微线和棒状体。在裂殖体核分裂过程中,出现典型的球虫型有丝分裂装置(如中心粒、中心锥、纺锤体)。裂殖子的发生是外瓣生方式,裂殖子在裂殖体的表面形成,并以母细胞的限制膜为外膜。     

Fine Structure of Schizonts and Merozoites of Eimeria nieschulzi*

SYNOPSIS. Schizonts of E. nieschulzi lie in a vacuole within the host cell. After nuclear division the cell membrane invaginates forming merozoites. Differentiation of the pellicle and other organelles occurs while merozoites are still attached to the schizont cytoplasm. Merozoites have a pellicle thickened at the anterior end to form a polar ring. Radiating posteriorly from the ring, directly beneath the pellicle, are about 25 microtubules. Within the polar ring is a dense conoid. Extending posteriorly from within the conoid is a paired organelle. The paired organelle varies in size and shape in each generation of merozoites. Numerous toxonemes occupy the anterior half of the merozoites. Two paranuclear bodies are present in 1st generation merozoites. One or 2 granular bodies were seen in the anterior end of 2nd generation merozoites. In 3rd generation merozoites 6 or more granular bodies were seen anterior to the nucleus. Each merozoite has a single nucleus containing diffuse chromatin material. Elongate mitochondria and glycogen granules are present. The vacuole surrounding mature merozoites contains residual cytoplasm of the schizont and some granular material. Microvilli project into the vacuole from the host cell membrane.     

La Genèse des Mérozoïtes chez la Coccidie Eimeria necatrix. Etude Ultrastructurale*

RESUME. Les schizontes de 2 ème génération d'Eimeria necatrix ont étéétudiés au microscope électronique. La différenciation des mérozoïtes est associée à la dernière mitose, qui ne semble pas différer essentiellement des précédentes. Les mérozoïtes se développent à la périphérie du schizonte. Le conoide et 22 microtubules sous pelliculaires, probablement induits par les centrioles, et le complexe membranaire interne ainsi que les précurseurs des rhoptries, qui semblent issus de l'appareil de Golgi, apparaissent auprès de chaque pôle nucléaire, sous la membrane du schizonte. Ces organites sont les premiers inclus dans les ébauches de mérozoïtes. Puis, le noyau, le dictyosome et les vésicules multimembranaires pénètrent dans les futurs mérozoïtes. Les micronèmes, probablement formés par l'appareil de Golgi, et les grains d'amylopectine sont produits plus tard, quand les mérozoïtes se séparent du reliquat cytoplasmique. Le mode de genèse de ces divers organites et les relations entre le dernière mitose et la différenciation sont discutés. SYNOPSIS. Second generation schizonts of Eimeria necatrix were studied with the aid of the electron microscope. Differentiation of daughter merozoites is associated with the last mitosis, which is not significantly different from the earlier ones. The merozoites develop at the periphery of the schizont. The conoid and 22 subpellicular microtubules, probably induced by centrioles, and the inner membranes complex and the rhoptry anlagen which seem to be produced by the Golgi apparatus, appear close to each nuclear pole, just near the schizont membrane. These organelles are the first to appear in the merozoite anlagen. Then, nucleus, dictyosome and multimembranous vesicles enter the budding merozoites. Micronemes, probably originating from Golgi apparatus, and amylopectin granules are produced later, when daughter merozoites separate from the residuum. The genesis of these various organelles and the relation between the last mitosis and differentiation are discussed.     

Fine Structure of the Schizont and Merozoite of Isospora sp. (Sporozoa: Eimeriidae) Parasitic in Gehyra variegata (Dumeril and Bibron, 1836) (Reptilia: Gekkonidae)

SYNOPSIS. A study was made of the fine structure of some stages in the life cycle of an undesignated species of Isospora parasitic in a gecko. The merozoites which lay within a membrane-bound periparasitic vacuole in the host epithelial cell, had a striking similarity to Plasmodium, Lankesterella, Toxoplasma, Besnoitia, Sarcocystis, Eimeria and the M-organism. Each merozoite was invested with a triple-layered pellicle, the outer membrane of which was loosely applied. At the anterior end of the merozoite were conoid and apical rings; microtubules terminated in the posterior apical ring. Other organelles included nucleus, endoplasmic reticulum, mitochondria, micropyle, paired organelle, toxonemes and a variety of vacuoles. Although the sequence of development of the merozoite was not completely followed, some events in this process were recorded. The evidence suggests that anterior ends are formed early and that merozoites develop subsequently by a process of budding. The merozoite pellicle appears to be continuous with, altho structurally different from, the investing membrane of the parent cell.     

High Yield Purification of Plasmodium falciparum Merozoites For Use in Opsonizing Antibody Assays

Plasmodium falciparum merozoite antigens are under development as potential malaria vaccines. One aspect of immunity against malaria is the removal of free merozoites from the blood by phagocytic cells. However assessing the functional efficacy of merozoite specific opsonizing antibodies is challenging due to the short half-life of merozoites and the variability of primary phagocytic cells. Described in detail herein is a method for generating viable merozoites using the E64 protease inhibitor, and an assay of merozoite opsonin-dependent phagocytosis using the pro-monocytic cell line THP-1. E64 prevents schizont rupture while allowing the development of merozoites which are released by filtration of treated schizonts.  Ethidium bromide labelled merozoites are opsonized with human plasma samples and added to THP-1 cells. Phagocytosis is assessed by a standardized high throughput protocol. Viable merozoites are a valuable resource for assessing numerous aspects of P. falciparum biology, including assessment of immune function. Antibody levels measured by this assay are associated with clinical immunity to malaria in naturally exposed individuals. The assay may also be of use for assessing vaccine induced antibodies.       

Eimeria tenella: use of a monoclonal antibody in determining the intracellular fate of the refractile body organelles and the effect on in vitro development

A monoclonal antibody, which recognizes the refractile body of Eimeria sporozoites, was used to study the developmental fate of this organelle during asexual development of E. tenella and to determine the effect of this monoclonal antibody on in vitro development of the parasite. Through use of immunofluorescent antibody and gold-labeling techniques at the light and electron microscopy level, the refractile body at 48 to 96 hr postinoculation was found to separate into 6 to 10 small globules, then diffuse throughout the schizont cytoplasm, and eventually reconcentrate as a small dot of material in each of the mature first-generation merozoites. The schizont did not develop to maturity if diffusion of the refractile body did not occur. The refractile body material was quickly lost as the merozoite left the schizont and invaded new cells and was not detected in any later developmental stages. The in vitro development of first- and second-generation schizonts of E. tenella was greatly inhibited (up to 100%) with exposure to the monoclonal antibody. There was an increase in the number of schizonts with nondispersed refractile body in the monoclonal antibody-treated cells when compared to the untreated controls, and the few mature schizonts seen had up to a 50-fold decrease in the number of merozoites. Immunofluorescent antibody labeling of the refractile body of intracellular sporozoites and schizonts treated in vitro with the monoclonal antibody for 24-96 hr postinoculation indicated that the antibody had crossed the host cell and parasite plasma membrane during incubation.     

Visualization and quantification of <Emphasis Type="Italic">Plasmodium falciparum</Emphasis> intraerythrocytic merozoites

Malaria, a leading parasitic killer, is caused by Plasmodium spp. The pathology of the disease starts when Plasmodium merozoites infect erythrocytes to form rings, that matures through a large trophozoite form and develop into schizonts containing multiple merozoites. The number of intra-erythrocytic merozoites is a key-determining factor for multiplication rate of the parasite. Counting of intraerythrocytic merozoites by classical 2-D microscopy method is error prone due to insufficient representation of merozoite in one optical plane of a schizont. Here, we report an alternative 3-D microscopy based automated method for counting of intraerythrocytic merozoites in entire volume of schizont. This method offers a considerable amount of advantages in terms of both, ease and accuracy.