Growth of Trypanosoma cruzi in Cultures of Chick Embryo Cells, and Effects of Furazolidone and Tris (p-Aminophenyl)Carbonium Chloride

SYNOPSIS. Monolayers of cells of coverslips were produced by culturing known numbers of trypsinized chick cells in growth medium (solution 199 plus 20% calf serum) at 37 C for 2 days. The fluid was then replaced with maintenance medium (solution 199 plus 5% calf serum) containing various known numbers of T. cruzi and the preparations were incubated at 33 C for 5 days; fresh maintenance medium was substituted on the 2nd or 3rd day. The inocula of parasites were obtained from T. cruzi -cell cultures, supplemented with 2% sterile NNN overlay, or from NNN cultures.
The numbers of extracellular parasites, proportions of infected cells, and percentage distribution of infected cells relative to the number of intracellular leishmanial bodies were determined on days 2 or 3 and 5 of parasite cultivation in many experiments. Analyses of the data gave the following results. Extracellular parasites increased 2- to 14-fold during the first 2 or 3 days, depending upon the source and size of the inocula, and 10- to 20-fold during the last 2 or 3 days. Cell infection continued throughout incubation at daily rates of 1.4-4.5%; 8-22% of the cells became infected during the 5 days of incubation. Intracellular growth was reflected most clearly by increases in the proportion of cells having >10 leishmanial bodies. This increase was about 5% daily during the last 2 or 3 days of incubation.
A useful test procedure for assessing the antiparasitic action and chick embryo cell toxicity of drugs is illustrated by data obtained with furazolidone and tris ( p -aminophenyl)carbonium chloride.     

Population systematics of Russell's viper: a multivariate study

A multivariate analysis of the population systematics of Russell's viper, based on scalation and colour pattern characters, reveals that the populations of this viper constitute two well-defined taxa: a western form, comprising all populations from the Indian subcontinent, and an eastern form, comprising all populations from east of the Bay of Bengal. The two forms could be considered either as subspecies of one species, or as two separate species, depending on the species concept used. Within the western form, there is no clear pattern of geographic variation. Within the eastern form, the populations from the Lesser Sunda Islands are clearly divergent from the populations of mainland Asia and Java. The conventionally recognized subspecies of Vipera russelli fail to portray this pattern of geographic variation. There is no clear relationship between the pattern of geographic variation in morphology and the pattern of geographic variation in the clinical effects of the venom in human bite victims: some populations with considerable differences in venom effects are equally distinct morphologically, whereas other populations with equally strong venom differences are morphologically very similar. The distribution of Russell's viper can be attributed to Pleistocene changes in climate and sea level, coupled with the viper's ecological requirements, which appear to include a seasonally dry climate.     

Biochemical Analysis of a Mutant Tetrahymena Lacking Outer Dynein Arms

ABSTRACT. Tetrahymena thermophila mutants homozygous for the oad mutation become nonmotile when grown at the restrictive temperature, and axonemes isolated from nonmotile mutants lack approximately 90% of their outer dynein arms. Electrophoretic analyses of axonemes isolated from nonmotile mutants ( oad axonemes) indicate they contain significantly fewer of the 22 S dynein heavy chains that axonemes isolated from wild-type cells (wild-type axonemes) contain. The 22 S dynein heavy chains that remain in axonemes isolated from nonmotile, oad mutants are assembled into 22 S dynein particles that exhibit wild-type levels of ATPase activity. Two-dimensional gel electrophoresis of oad axonemes show that they are deficient in no proteins other than those proteins thought to be components of 22 S dynein. This report is the first formal proof that outer dynein arms in Tetrahymena cilia are composed of 22 S dynein.     

The Structure and Function of the Spore Outer Membrane in Dormant and Germinating Spores of Bacillus megaterium

Attempts to demonstrate the presence of the spore outer membrane in mature, dormant spores of a strain of Bacillus megaterium are described. The outer, integument, layers of this organism were found to contain one-third of the total spore cytochrome content, several enzymes of the electron transport chain (specifically NADH oxidase, dehydrogenase, cytochrome c reductase and NADPH dehydrogenase) and a large number of polypeptides extractable with sodium dodecylsulphate in the presence of dithiothreitol and protease inhibitors. These all suggest the presence of a membraneous element. Electron microscopic evidence is presented on the structure of the dormant integument enzymes. Changes in the integument enzymes and in the gel electrophoresis profile of the extractable integument polypeptides which occur during spore gemination, are described and compared with those that take place in the spore inner membrane. The heat sensitivity of the integument enzymes is compared with that of the inner membrane enzymes and the implications for theories of spore heat resistance discussed.     

Comparative Toxicity of Gonyaulax monilata and Gymnodinium breve to Annelids, Crustaceans, Molluscs and a Fish

SYNOPSIS. Toxicities of laboratory cultures of the dinoflagellates Gonyaulax monilata and Gymnodinium breve were compared using fish, annelids, crustaceans and molluscs. Toxicity was evaluated as mortality over a 48-hr test period in 100%, 75% 50%, 25% and 10% concentrations of dinoflagellate cultures. Responses of the assay animals indicated that the dinoflagellates do not produce the same toxins. Effects of the toxins seemed uniform within each major group of animals tested. Fish were most sensitive to both G. breve and Gonyaulax monilata; crustaceans were resistant to both; annelids and molluscs were more sensitive to G. monilata than to G. breve.     

The Antigens Associated with the Cell Walls of Members of the Genus Pseudomonas

Three antigens were associated with the cell walls of pseudomonads. A highly antigenic, strain-specific antigen of high molecular weight and protein or lipoprotein in nature, occurred as an envelope around the cells. It could be washed off the cells closely associated with carbohydrate material but its antigenicity was not dependent on the carbohydrate present. Another antigen, common to all strains tested, was situated below the first antigen. This was less antigenic than the strain-specific antigen and was polysaccharide or lipopolysaccharide in nature. A second common antigen was the mucopeptide of the cell walls. This had an antigenicity similar to that of the second antigen and was dependent on both the carbohydrate and polypeptide components of the macromolecule. There appears to be some correlation between these findings and the structure of cell walls of pseudomonads are shown by electron microscopy.