Mesocestoides corti in the rat: The cellular response in the peritoneal cavity of rats infected with Mesocestoides corti

The tetrathyridium (second larval stage) of Mesocestoides corti elicits an extensive cellular response in the peritoneal cavity of rats which was monitored over a period of 40 days following infection. The total white cell count of female Wistar rats rose in the peritoneal cavity during the first 10 days of infection, then declined slowly. Eosinophilia was characteristic, as it is in most helminth infections. Cellular adherence to the surface of some tetrathyridia was noted. In rats infected with a large number of tetrathyridia, many parasites were found trapped in the mesenteries.     

Histopathological changes in livers of mice infected with tetrathyridia of Mesocestoides corti and exposed to different environmental temperatures

Novak M. 1982. Histopathological changes in livers of mice infected with tetrathyridia of Mesocestoides corti and exposed to different environmental temperatures. International Journal for Parasitology12: 41–45. Observations on the histopathology of the liver of mice infected with Mesocestoides corti and kept for 20 days p.i. (post-infection) at low (5 ± 1°C), room (21 ± 1°C) or high (35 ± 1°C) temperature revealed that the degree of liver pathology was directly proportional to the intensity of liver infection, which in turn was the result of the temperature effect. The most severe pathological changes occured in the heavily infected organs of mice kept at low temperature, followed by less prominent changes in moderately infected livers of mice kept at room temperature and the smallest changes in lightly infected livers of mice kept at high temperature. The pathological changes in infected and uninfected livers of hosts exposed to different environmental temperatures are described and compared.     

Cross-protection between the metacestodes of Mesocestoides corti and Taenia crassiceps in mice

Novak M. 1984. Cross-protection between the metacestodes of Mesocestoides corti and Taenia crassiceps in mice. International Journal for Parasitology14: 497–501. Infection with M. corti generated significant resistance against a challenge with T. crassiceps introduced either 2 or 6 weeks after primary infection. Challenge infection with T. crassiceps did not influence primary infection with M. corti. Infection with T. crassiceps protected significantly against challenge with M. corti given 2 weeks but not 6 weeks after the primary infection. Challenge infection with M. corti significantly suppressed primary infection with T. crassiceps.     

Mesocestoides corti in the rat: Comparisons of Mesocestoides corti infections in rats and mice

Infections of M. corti in rats were compared with those in mice. The recoveries of parasites and their distribution were examined for 60 days after infection. During this period continuous and extensive multiplication occurred in mice. In rats there was an initial multiplication of tetrathyridia in the first 10 days followed by a decline in numbers. The relative distribution of tetrathyridia between the peritoneal cavity and liver was similar in both hosts.     

T-cell dependent collagenous encapsulating response in the mouse liver to Mesocestoides corti (Cestoda)

Pollacco S., Nicholas W.L., Mitchell G.F. and Chaicharn Stewart A. 1978. T-cell dependent collagenous encapsulating response in the mouse liver to Mesocestoides corti (Cestoda). International Journal for Parasitology8: 457–462. Experiments with genetically hypothymic mice show that the tetrathyridial larvae of Mesocestoides corti (Cestoda) multiply much more rapidly in the liver than in normal mice. In the hypothymic mouse, collagen fibres are not laid down and the parasite is not encapsulated as it is in the normal mouse. Encapsulation probably restricts the parasite's multiplication, and it is suggested that the failure to encapsulate the parasite accounts for its more rapid multiplication in the hypothymic mouse. Fibrogenesis and encapsulation is restored to hypothymic mice by transferring syngeneic thymus cells, spleen cells or peritoneal exudate cells. It is concluded that the encapsulation of M. corti is a T-cell dependent process.     

Spontaneous sexual differentiation of Mesocestoides corti tetrathyridia in vitro

Barrett N. J., Smyth J. D. and Ong S. J. 1982. Spontaneous sexual differentiation of Mesocestoides corti tetrathyridia in vitro. International Journal for Parasitology12: 315–322. Tetrathyridia of Mesocestoides corti, from the body cavity of mice, maintained in the laboratory by intraperitoneal infection, were used for in vitro culture. In an initial experiment, after 50 days asexual multiplication in vitro one tetrathyridium spontaneously segmented and developed into a sexually mature adult. Further experiments were carried out in an attempt to determine the conditions favouring segmentation and sexual differentiation. A combination of 5 or 10 ml liquid medium S1OE.H (basically composed of CMRL 1066 and foetal calf serum with supplements) changed every 3 days, in a Leighton tube (19 × 105 mm), rotated at 38°C and gassed with 10 or 20% CO₂, containing between 100 and 200 tetrathyridia, has proved to be most suitable so far. Numerous adult worms with normal male and female genitalia have been obtained in this system. However, segmentation is sporadic, rather than consistent and only a few shelled eggs with hooked oncospheres have so far been obtained, suggesting that impregnation and fertilization in vitro is not fully comparable with that in vivo.     

Effects of mebendazole and levamisole on tetrathyridia of Mesocestoides corti in the mouse

Bennet E.-M., Behm C.A. and Bryant C. 1978. Effects of mebendazole and levamisole on tetrathyridia of Mesocestoides corti in the mouse. International Journal for Parasitology8: 463–466. Mebendazole, but not levamisole, administered to mice carrying artificial infections of 50 tetrathyridia of Mesocestoides corti, was effective in killing the parasites. However, simultaneous administration of mebendazole and levamisole was still more effective. Treatment with levamisole before infection had no additional effect.Injection of mice with dead larvae offered some protection against a subsequent challenge with 50 live larvae; however, levamisole did not then improve the anthelmintic efficacy of mebendazole. In mice rendered immunoincompetent by radiation mebendazole was less effective than in non-irradiated controls and levamisole again did not enhance the effect of mebendazole. It is concluded that anthelmintic efficacy of mebendazole depends on its anthelmintic activity supplemented by the host's immune response; and that levamisole stimulates the latter.     

A comparative study of the susceptibility of inbred strains of mice to infection with Mesocestoides corti

White T. R., Thompson R. C. A. and Penhale W. J. 1982. A comparative study of the susceptibility of inbred strains of mice to infection with Mesocestoides corti. International Journal for Parasitology12: 29–33. The susceptibility of 6 strains of inbred mice to infection with Mesocestoides corti was studied following both intraperitoneal and oral inoculation of tetrathyridia. The greatest degree of resistance was seen in C57BL/6 mice and this resistance was independent of route of inoculation. The proliferation of the parasite in C57BL/6 mice was compared with a more susceptible strain (CBA/H) on 7, 14, 21, 35 and 60 days post-infection. Although both strains harboured significantly different parasite burdens during the initial period following infection, these differences were no longer apparent by day 60.     

Immunoregulation by macrophages: differential secretion of prostaglandin E and interleukin 1 during infection with Salmonella enteritidis

We have investigated the temporal relationship between bacterial clearance in vivo, macrophage bactericidal activity in vitro, and the secretion of immunoregulatory molecules, prostaglandin E (PGE) and Interleukin 1 (IL1) in vitro, during infection with an avirulent strain of Salmonella, Salmonella enteritidis 11RX. The two model systems used were normal mice challenged intraperitoneally with SE11RX (NSE) and previously sensitized mice rechallenged 24 days later with SE11RX (SESE). The increasing nonspecific bactericidal activity of the peritoneal macrophages from NSE and SESE mice after the second day of infection paralleled the clearance of bacteria observed in vivo. Prostaglandin secretion by normal macrophages cultured for 4 hr with LPS correlated inversely with intracellular bacterial numbers but showed a positive correlation when cultured with opsonized SRBC or C3-zymosan complexes. PGE was the major arachidonate metabolite secreted. The cells from sensitized mice secreted tittle prostaglandin with any stimulus, and this secretion showed a positive correlation with bacterial number. The capacity to secrete IL1 in response to LPS increased during infection in both NSE and SESE mice. There was an inverse correlation between IL1 secretion and PGE production by cells from sensitized mice. We propose that changes in the capacity of peritoneal macrophages to secrete IL1 and PGE in response to stimulants in vitro reflect the initiation and regulation of the immune response through the course of infection.     

Acceleration of the growth of tetrathyridial populations of Mesocestoides Corti (Cestoda: Cyclophyllidea) by splenectomy

Acceleration of the growth of tetrathyridial populations of Mesocestoides corti (Cestoda: Cyclophyllidea) by splenectomy. International Journal for Parasitology4, 165–168. Experiments with LDF₁ hybrid mice showed that splenectomy 7 days prior to infection, increases the total biomass of tetrathyridial populations of Mesocestoides corti in hosts of both sexes.This increase is accompanied by a decrease in the size of individuals, and by an increase in the percentage of two-suckered and acephalic forms. Splenectomy thus accelerates both the growth of the biomass of populations and the asexual multiplication of the tetrathyridia.     

In vitro development of the strobilar stage of Mesocestoides corti

Thompson R. C. A., Jue Sue L. P. and Buckley S. J. 1982. In vitro development of the strobilar stage of Mesocestoides corti. International Journal for Parasitology12: 303–314. Sexually mature strobilated adults of Mesocestoides corti were grown consistently from undifferentiated tetrathyridia in vitro using a conventional diphasic culture system. Development (growth, strobilisation and maturation) was compared in vitro and in vivo. Although growth and strobilisation were comparable in vitro and in vivo, during the first 18 days, total length and numbers of proglottids decreased in vivo but continued to increase in vitro after day 18. Both male and female reproductive systems appeared to develop normally in vitro and self copulation was frequently observed in cultured worms. However, fully developed oncospheres were not produced in vitro.     

Gonadectomy and the development of polycephalic tetrathyridia of Mesocestoides corti (Cestoda: Cyclophyllidea) in mice

The number of polycephalic tetrathyridia present in 150-day-old intraperitoneal larval populations of Mesocestoides corti was markedly increased in mice gonadectomized 1 month prior to infection. This effect was more pronounced in male hosts. In both sexes it was inversely correlated with the size of the populations: the smaller the population, the larger was the number of polycephalic tetrathyridia. These forms are probably produced when the separation of daughter individuals lags behind the growth and organogenesis of these peculiar cestodes.     

Fasciola hepatica: Comparative studies on fascioliasis in rats and mice

Chapman C. B. and Mitchell G. F. 1982. Fasciola hepatica: comparative studies on fascioliasis in rats and mice. International Journal for Parasitology12: 81–91. Certain characteristics of infection differ between rats and mice exposed to metacercariae of the trematode parasite, Fasciola hepatica. Rats develop a degree of age-related resistance (and infected older females contain fewer parasites than older males), resistance to reinfection in infected rats is demonstrated readily though is partial, and a comparable degree of resistance can be obtained in recipients of infected rat serum provided the serum is given at about the time of challenge. None of these features of F. hepatica infection is seen in mice. Rats also differ from mice in that they can be vaccinated against infection (although again, resistance is incomplete) using larval antigen mixtures in adjuvants. Mice do respond to infection by production of antilarval antibodies and a slight IgG₁ hypergammaglobulinaemia and larvae will sensitize mice for delayed hypersensitivity. The results of this study indicate that sera from infected rats versus infected mice will be useful in pinpointing antigens of F. hepatica larvae which are involved in expression of partial host protection.     

Age-associated responses in susceptible and resistant rats to infection with Fasciola hepatica

Rajasekariah G. R. and Howell M. J. 1981. Age-associated responses in susceptible and resistant rats to infection with Fasciola hepatica. International Journal for Parasitology11: 59–65. Groups of susceptible (5-week-old) and age resistant (25-week-old) outbred male Wistar rats were infected with metacercariae of Fasciola hepatica and the establishment of the parasite was assessed in terms of worm reocvery, and haematological, histopathological and immunological criteria, 2, 4, 6 and 8 weeks after infection. Apart from 2 weeks after infection, there was a significant difference between groups in the recovery of F. hepatica, with resistant rats infected with consistently fewer parasites than susceptible animals. The juvenile worms which invaded the livers of resistant rats elicited a number of host reactions, marked by an intensive cellular infiltration into migratory tracks of the parasite, heavy deposition of fibrous tissue in the liver parenchyma and a rapid antibody response. These responses were not as striking in susceptible animals even though more worms were present. The ability of resistant rats to mount an enhanced response seems related to the maturation of their haemopoietic system.     

Localization and associated histopathology of asexually proliferative Mesocestoides corti tetrathyridia (cestoda) infecting mouse mammary glands

Female mice of pregnant random-bred, or unmated BALB/c groups were exposed per os to Mesocestoides corti tetrathyridia and necropsied at various intervals postexposure. The right posterior subcutaneous fat pad with two mammary glands was removed from each mouse, stained, mounted whole and examined microscopically for localization of worms. The left fat pad/gland set was processed, sectioned and stained using standard histological techniques. In pregnant mice, tetrathyridia were localized primarily in the fat pad's posteroventral lobe. Unmated mice had few worms in the mammary glands or associated fat pads. The difference in infection levels between the two host groups may result from mouse strain difference or the pregnant condition of one group.     

Experimental Salmonellosis

An immune ribonucleic acid (RNA) preparation was obtained from the spleens of mice immunized with a live vaccine of Salmonella enteritidis. When peritoneal macrophages were infected with S. enteritidis 116–54 which had been treated by mixed cultivation with the peritoneal exudate cells of mice previously treated with an immune RNA preparation, they showed cellular resistance against the infecting bacteria. According to the results described previously and those described in this article, it can be concluded that the cellular resistance against an infection with S. enteritidis is traceable to a cellular antibody (or antibodies) detected in macrophages of mice immunized with a live vaccine of the same organism or of mice treated in vivo (or in vitro) with an immune RNA preparation.     

Taenia crassiceps: Fate of cysticerci following ingestion by the mouse

Cysticerci of Taenia crassiceps were administered to mice by gavage to determine whether enteral or parenteral infections would establish consistently. Some worms survived in the small intestine up to 16 days, whereas others penetrated through the gut wall into the peritoneal cavity within 24 hr. Similar proportions of different doses of worms reached the peritoneal cavity regardless of the size of the inoculum and sex or strain of mice used. In addiiton, it was shown that mice may acquire an intraperitoneal infection with T. crassiceps by eating the carcass of an infected mouse.     

Infectivity of a microsporidium of mosquitoes (Nosema algerae) to larval stages of Schistosoma mansoni in Biomphalaria glabrata

Lai P. F. and Canning E. U. 1980. Infectivity of a microsporidium of mosquitoes (Nosema algerae) to larval stages of Schistosoma mansoni in Biomphalaria glabrata. International Journal for Parasitology10: 293–301. Nosema algerae derived from a closed colony of Anopheles stephensi was fed to Biomphalaria glabrata infected with Schistosoma mansoni. Mother and daughter sporocysts became hyperinfected but the snail tissues remained free of the microsporidia except for rare small aggregates of spores. These lay close to the sites occupied by mother or daughter sporocysts and were probably liberated from them. Irrespective of dose, fewer snails contained infected sporocysts when spores were given at 7 days post-miracidial infection than when given at 14 days. These periods corresponded respectively to stages when mother sporocysts only or daughter sporocysts as well were present in the snails. Infection of the sporocysts began in the tegumental cells, spread to the brood chamber and ultimately to the cercariae themselves. Heavily infected sporocysts contained fewer developing embryos. Doses of 10⁶ and 10⁷ spores/snail caused significant depression of cercaria output when given at 14 days but not at 7 days.     

Effect of Capsular Polysaccharide of Klebsiella pneumoniae on Host Resistance to Bacterial Infections

When Klebsiella pneumoniae capsular polysaccharide (CPS-K) from type 1, Kasuya strain, was injected intraperitoneally (i.p.) immediately before i.p. bacterial challenge, the survival time of mice infected with Salmonella enteritidis NUB 1 (virulent strain) was shortened and the mortality rate for mice infected with S. enteritidis NUB 31 (avirulent strain) was enhanced. The promotion of infection with S. enteritidis NUB 1 by CPS-K depended upon its dose, the effect of CPS-K being demonstrable up to as little as 0.2 μg per mouse. In the case of S. enteritidis NUB 31, the effect of CPS-K was detectable only when more than 20 μg per mouse was injected. As a result of enumeration of bacterial populations in the peritoneal washing, blood, liver and spleen, it was revealed that CPS-K promoted in vivo growth of S. enteritidis NUB 1 and NUB 31. In addition, CPS-K enhanced the mortality rate in mice infected with Streptococcus pyogenes or Streptococcus pneumoniae. The peak CPS-K effect on infection with S. enteritidis NUB 1 was seen when given immediately before bacterial challenge. The active substance responsible for the infection-promoting effect of CPS-K was neutral CPS-K, which is distinct from the O antigen and from acidic CPS-K (the type-specific capsular antigen). Preparations of neutral CPS-K isolated from the other three strains of K. pneumoniae exhibited a marked infection-promoting effect comparable with that of preparations from the Kasuya strain. Neutral CPS-K, with identical antigenicity to that from the Kasuya strain, has already been found to exert a strong adjuvant effect on antibody responses to various antigens in mice. No parallelism exists between infection-promoting activity and adjuvant activity of neutral CPS-K.     

Interactions between Trichinella spiralis and Hymenolepis nana in the intestine of the mouse

Ferretti G., Gabriele F., Palmas C. and Wakelin D. 1984. Interactions between Trichinella spiralis and Hymenolepis nana in the intestine of the mouse. International Journal for Parasitology14: 29–33. The rejection of the intestinal phase of Trichinella spiralis in outbred CD₁ mice is associated with an inflammatory response. The effects of this inflammation were studied in mice concurrently infected with an unrelated parasite, Hymenolepis nana, which stimulates a slight inflammation but is also immunologically rejected by this strain of mice. Moreover though Cd(In)1 mice seem to be ‘slow responders’, in concurrent infections with T. spiralis and H. nana there was a marked effect upon the cesode survival. At the highest level of T. spiralis infection, H. nana failed to establish at all. On the other hand, if 300 T. spiralis were administered 10 weeks earlier, H. nana become established in all mice and the distribution of parasites suggests that immunodepression is involved. An accelerated loss of the nematode, when H. nana was present, was also demonstrated. There was no evidence of any reciprocal or specific cross-immunity between the two parasites.