The fine structure of the female reproductive tract of adult Loa loa

Weber P. 1987. The fine structure of the female reproductive tract of adult Loa loa. International Journal for Parasitology17: 927–934. The wall of the female reproductive tract of Loa loa was studied by electron microscopy. The wall is composed of a monolayered epithelium covered by a basal lamina. The epithelium of the ovary has a moderately developed basal labyrinth, abundant organelles, and a few secretory granules. In the oviduct, the basal lamina intrudes septa-like into the epithelium. Abundant myofilaments are attached to it. Microvilli cover the luminal cell border. The seminal receptacle contains few muscle cells in its basal lamina. It shows a highly developed spongy zone at its luminal surface. The uterine epithelium contains glycogen deposits and lipid droplets. In its anterior parts it shows a highly developed basal labyrinth and an abundance of secretory granules. The vagina has several layers of muscle cells in the basal lamina. Its epithelium contains few organelles, a small number of secretory granules, and is devoid of storage deposits.     

Genetic heterogeneity in Loa loa parasites from southern Cameroon: A preliminary study

Ivermectin (or Mectizan trade mark ) is widely used by onchocerciasis and lymphatic filariasis control programs worldwide. Generally, Mectizan trade mark is both safe and well tolerated. An exception to this general pattern is in some areas co-endemic for Onchocerca volvulus and Loa loa, where a number of severe adverse reactions to Mectizan trade mark have been noted in L. loa infected individuals. The vast majority of these severe adverse events have occurred in Southern Cameroon. This suggested the hypothesis that the parasites endemic to Southern Cameroon might form a distinct population that exhibited a phenotype of eliciting severe adverse reactions in Loa-infected individuals upon Mectizan trade mark exposure. To test this hypothesis, the DNA sequences of three potentially polymorphic loci were compared among L. loa parasites from Southern Cameroon and other endemic foci in Sub-Saharan Africa. Analysis of these data suggested that parasites from Southern Cameroon were at least as genetically diverse as those from other foci. Furthermore, no polymorphisms were noted that were unique to and shared among the parasite isolates from Southern Cameroon. Although a limited number of parasite isolates were tested, these results do not appear to support the hypothesis that L. loa parasites from Southern Cameroon represent a unique, genetically isolated population.     

Electron microscope study ofLeptospira

A leptospira consists of the cytoplasmic cylinder (contained within its own wall) which winds helically anticlockwise around the axistyle; both these components are enclosed by the outer covering membrane enveloping the whole organism.     

Rapid molecular assays for specific detection and quantitation of Loa loa microfilaremia

Background

Accurate diagnosis of Loa loa infection is essential to the success of mass drug administration efforts to eliminate onchocerciasis and lymphatic filariasis, due to the risk of fatal encephalopathic reactions to ivermectin occurring among highly microfilaremic Loa-infected individuals living in areas co-endemic for multiple filarial species.

Methodology/Principal Findings

From a pool of over 1,800 L. loa microfilaria (mf) expressed sequence tags, 18 candidate L. loa mf-specific PCR targets were identified. Real-time PCR (qPCR) assays were developed for two targets (LLMF72 and LLMF269). The qPCR assays were highly specific for L. loa compared with related filariae and also highly sensitive, with detection limits of 0.1 pg genomic DNA, or 1% of DNA extracted from normal blood spiked with a single L. loa microfilaria. Using various DNA extraction methods with dried blood spots obtained from Cameroonian subjects with parasitologically proven loiasis, the LLMF72 qPCR assay successfully estimated mf burden in 65 of 68 samples (50–96,000 mf/mL by microscopy), including all 12 samples subjected to a simple 10-minute boiling extraction. Additionally, the assay detected low-level microfilaremia among 5 of 16 samples from patients thought to be amicrofilaremic by microscopy.

Conclusions/Significance

This novel, rapid, highly sensitive and specific qPCR assay is an important step forward in the laboratory diagnosis of L. loa infection.     

Electron microscope study on meiosis

Summary The cycle of the nucleolus and sex chromosome was studied with the electron microscope during the following stages of spermatogenesis and spermiogenesis of Gryllus argentinus: (1) spermatogonia; (2) prophase cyte I, leptotene, part of pachytene, and end of diplotene till breakdown of the nuclear envelope; (3) division I, metaphase and anaphase; (4) cyte II, prometaphase; (5) division II, metaphase, anaphase and telophase; (6) early and late spermatids. Some observations were also carried out in the primary oocyte until beginning of the growth period.It was found that nucleolus and sex chromosome are associated, at first without mixture of their components (leptotene) and afterwards interchanging components (pachytene). The interchange takes place by the passage from one element to another of filamentous units ot low electron density, similar in appearance to those existing in the medial plane of tripartite groups (synaptinemal complexes).At pachytene the primary results of interchange are: (1) the nucleolus contains filaments of chromosomal nature; (2) the nucleolus emits a long rod-like prolongation containing a cylindrical bundle of filaments, and an axial unit of the same nature; two equidistant clear spaces separate the axial unit from the cylindrical bundle and the latter from the dark wall of nucleolar material. At the end of diplotene these components are found organized in two bodies and a prolongation. One of the bodies is formed by a number of alternatively dark and light bands, the other by a pack of tubular units each showing the structure of the former nucleolar prolongation. The prolongation is either formed as in the preceding stage or it is composed of five ribbons, two dark ones outside and three light ones between them. It is supposed that both bodies are united by the prolongation but no definite proof was obtained. It is assumed that the complex thus constituted represents the sex chromosome.The sex chromosome was found at any phase of both divisions as well as at the intermediate stages between them; at the division phase the chromosome is separated from the autosomes and moves independently of them.The element could not be traced at telophase II but it reappears within the reorganized nuclei of spermatids. Amorphous nucleolar-like material and chromosome-like material are found associated at this stage with banded complexes like those seen at the end of prophase I. All these components undergo involution during spermatid maturation. At the final step of maturation no traces of them are found.A similar association of nucleolus and chromosome was found at prophase of primary oocytes of the same species. The associated body is of the same structure as that described for primary spermatocytes. The structures existing in the primary oocytes disorganize at the beginning of growth. At this time the nucleolus has developed into a large body containing masses of chromatin-like material.This investigation was supported in part by U.S. Public Health Service, Research Grant No. GM-08337 from the National Institute of General Medical Sciences.     

Electron microscope study on spermatogenesis

Summary The morphogenesis of chromosomes at early prophase of spermatocytes I is studied in three ortoptherian species: Grillus argentinus (Grillidae), Laplatacris dispar (Acrididae) and Blaptica dubia (Blaptidae).The first chromosome component appearing at the beginning of meiosis is a thread (single elementary thread; S.E.T.) of low electron density measuring about 700 Å to 0.1 width. A group having the same width and integrated by three helically twisted ribbon-like components develops from S.E.T. and is called primary tripartite group, P.T.G. The three components are at first of the same width (about 200 Å) but the lateral arms progressively increase in thickness and in that way the group becomes coated by a layer of dense microfibrils supposed to be chromatin.Late stages of prophase were not thoroughly investigated in this study, but many evidences were however found helping to identify synaptene stage. In accordance with these evidences each homologous chromosome is integrated by an axial component (tripartite groups) coated by chromatin.The medial component of tripartite groups of Blaptica dubia is double and also shows multistranded regions which are called puffy regions.A comparative optical and electron microscope study was made in order to better understand the above described process. This study includes the comparison of the thickness of chromosomes as measured in light and electron micrographs.On the other hand, rubber models were made to illustrate the same process and pohotographs of these models are exhibited in the text.The nuclear structure of early spermatids of the same species is also studied in this paper. It was found that Blaptica and Grillus early spermatids nuclei contain groups similar to those found at the beginning of prophase of spermatocyte I, with the only difference that in many cases composite groups, formed by fusion of the lateral arms of two or more than two single groups, were found.The nuclear structure of late spermatids was also considered in this paper. Notwithstanding the study only aimed to point out that the pattern of organization of the spermatozoon chromatin greatly differs in the species examined.     

Epidemiology of concomitant infection due to Loa loa and Mansonella perstans in Gabon

Background

The filarial parasites Loa loa and Mansonnella perstans are endemic in the central and western African forest block. Loa loa is pathogenic and represents a major obstacle to the control of co-endemic filariae because its treatment can cause fatal complications such as encephalitis.

Methodology/Principal Findings

4392 individuals aged over 15 years were studied both by direct examination and a concentration technique. The overall prevalence rates were 22.4% for Loa loa microfilaremia, 10.2% for M. perstans microfilaremia, and 3.2% for mixed infection. The prevalence of both filariae was higher in the forest ecosystem than in savannah and lakeland (p<0.0001). The intensity of microfilariae (mf) was also higher in the forest ecosystem for both parasites. The prevalence and intensity of microfilaria were both influenced by age and gender. Correlations were found between the prevalence and intensity of Loa loa microfilariae (r = 0.215 p = 0.036), and between the prevalence of Loa loa and the prevalence of individuals with microfilaria >8000 mf/ml (r = 0.624; p<0.0001) and microfilariae >30 000 mf/ml (r = 0.319, p = 0.002). In contrast, the prevalence of pruritis and Calabar swellings correlated negatively with the prevalence of Loa loa microfilaria (r = −0.219, p = 0.032; r = −0.220; p = 0.031, respectively). Pruritis, Calabar swellings and eye worm were not associated with L. loa mf intensity (r = −0.144, p = 0.162; r–0.061, p = 0.558; and r = 0.051, p = 0.624, respectively), or with the prevalence or intensity of M. perstans microfilariae.

Conclusions/Significance

This map of the distribution of filariae in Gabon should prove helpful for control programs. Our findings confirm the spatial uniformity of the relationship between parasitological indices. Clinical manifestations point to a relationship between filariae and allergy.     

Macaca fascicularis, a nonpermissive host for the human filarial parasite Loa loa

The ability of the filarial nematode Loa loa to infect 2 species of primates was studied. The primate species selected were closely related to species known to be susceptible. A mandrill (Mandrillus sphinx) and 6 cynomolgus monkeys (Macaca fascularis) were infected by subcutaneous injection of third-stage larvae of human L. loa from Gabon. The mandrill developed microfilaremia with an estimated prepatent period of 147 days, but microfilariae were not detected in any of the cynomolgus monkeys. Thus, mandrills appear permissive to human L. loa, whereas cynomolgus monkeys are not. Serum antibody responses were examined on western blots of adult L. loa antigens. Preinfection sera from all animals gave no reactions, but, after infection, sera from cynomolgus monkeys reacted more intensely and with more antigens than mandrill sera. Antibodies were still detectable in cynomolgus monkeys 15 mo postinfection. These reactions were compared with those found using human infection sera. Reactions with the cynomolgus monkey sera resembled those found with resistant endemic and amicrofilaremic human sera.     

Electron microscope study of Cryptostroma corticale

An ultrastructural study of Cryptostroma corticale has been carried out with scanning and transmission electron microscopes. The usual features in fungi, as well as features characteristic of the family, were shown. It was noted that lomasomes and myelin-type structures were demonstrated by the two fixatives used. Their significance is discussed.     

Electron microscope study of lens fibers

The in vitro swelling action of L-thyroxine on rat liver mitochondria as examined photometrically represents an acceleration of a process which the mitochondria are already inherently capable of undergoing spontaneously, as indicated by the identical kinetic characteristics and the extent of thyroxine-induced and spontaneous swelling, the nearly identical pH dependence, and the fact that sucrose has a specific inhibitory action on both types of swelling. However, thyroxine does not appear to be a "catalyst" or coenzyme since it does not decrease the temperature coefficient of spontaneous swelling. The temperature coefficient is very high, approximately 6.0 near 20 degrees . Aging of mitochondria at 0 degrees causes loss of thyroxine sensitivity which correlates closely with the loss of bound DPN from the mitochondria, but not with loss of activity of the respiratory chain or with the efficiency of oxidative phosphorylation. Tests with various respiratory chain inhibitors showed that the oxidation state of bound DPN may be a major determinant of thyroxine sensitivity; the oxidation state of the other respiratory carriers does not appear to influence sensitivity to thyroxine. These facts and other considerations suggest that a bound form of mitochondrial DPN is the "target" of the action of thyroxine. The thyroxine-induced swelling is not reversed by increasing the osmolar concentration of external sucrose, but can be "passively" or osmotically reversed by adding the high-particle weight solute polyvinylpyrrolidone. The mitochondrial membrane becomes more permeable to sucrose during the swelling reaction. On the other hand, thyroxine-induced swelling can be "actively" reversed by ATP in a medium of 0.15 M KCl or NaCl but not in a 0.30 M sucrose medium. The action of ATP is specific; ADP, Mn(++), and ethylenediaminetetraacetate are not active. It is concluded that sucrose is an inhibitor of the enzymatic relationship between oxidative phosphorylation and the contractility and permeability properties of the mitochondrial membrane. Occurrence of different types of mitochondrial swelling, the intracellular factors affecting the swelling and shrinking of mitochondria, as well as the physiological significance of thyroxine-induced swelling are discussed.     

A possible case of spontaneous Loa loa encephalopathy associated with a glomerulopathy

Background

There is a danger that mass drug administration campaigns may fail to maintain adequate treatment coverage to achieve lymphatic filariasis elimination. Hence, additional measures to suppress transmission might be needed to ensure the success of the Global Program for the Elimination of Lymphatic Filariasis.

Discussion

Vector control successfully eliminated lymphatic filariasis when implemented alone or with mass drug administration. Challenges to lymphatic filariasis elimination include uncertainty of the exact level and duration of microfilarial suppression required for elimination, the mobility of infected individuals, consistent non-participation of some infected individuals with mass drug administration, the possible development of anti-filarial drug resistance and treatment strategies in areas co-endemic with loasis. Integration of vector control with mass drug administration can address some of these challenges. The potential benefits of vector control would include: (1) the ability to suppress filariasis transmission without the need to identify all individual 'foci of infection'; (2) minimizing the risk of reestablishment of transmission from imported microfilaria positive individuals; and (3) decreasing the risk of dengue or malaria transmission where, respectively, Aedes or Anopheles are lymphatic filariasis vectors.

Summary

With adequate sustained treatment coverage, mass drug administration should meet the criteria for elimination of lymphatic filariasis. However, it may be difficult to sustain sufficiently high mass drug administration coverage to achieve lymphatic filariasis elimination in some areas, particularly, where Aedes species are the vectors. Since vector control was effective in controlling and even eliminating lymphatic filariasis transmission, integration of vector control with mass drug administration will ensure the sustainability of transmission suppression and thereby better ensure the success of national filariasis elimination programs. Although trials of some vector control interventions are needed, proven vector control strategies are ready for immediate integration with mass drug administration for many important vectors. Vector control is the only presently available additional lymphatic filariasis control measure with the potential for immediate implementation.     

Electron microscope study of the human neuromuscular junction

A preliminary electron microscope study of human neuromuscular junction is presented. The biopsy material was taken from the palmarus longus, and fixed routinely in osmium tetroxide and embedded in methacrylate. The structure of the motor endings and the relationship of the synaptic vesicles to the axolemmal membrane are described. The synaptic clefts are filled with an homogeneous material in continuity with the basement membrane covering the muscle fiber. The subneural apparatus is described, and special attention is paid to a vesicular component present in the sarcoplasm of the junctional area, which differs from synaptic vesicles and is presumed to be a derivate of the sarcoplasmic reticulum.