Synergistic effects of metabolically related amino acids on the growth of a multicellular plant

The effects of several amino acids related to the metabolism of aspartic acid on the growth and development of gemmalings of the liverwort Marchantia polymorpha were investigated under axenic conditions. Lysine and theonine synergistically inhibit the growth of these plants and cause a loss of normal pigmentation at concentrations as low as 1 μm. These effects are highly specific for this pair of amino acids, are partially reversible upon removal of the effectors, and can be prevented by low concentrations of methionine or its metabolic precursor, homoserine. Alterations in the growth and development of gemmalings in the presence of natural amino acids are discussed in relation to metabolic regulatory mechanisms which have been well established in microorganisms.     

Salmonellae Associated with Further-processed Turkey Products

"Further-processed" turkey products, prepared from chilled, eviscerated, and thawed carcasses at two commercial turkey-processing plants, were evaluated, for the presence of salmonellae. These organisms were isolated from swab samples from 12% of chilled, eviscerated turkey carcasses, 27% of finished products, and 24% of processing equipment. The same serotypes as those found throughout a plant on any one visit were recovered from 31% of rinse-samples taken from hands and gloves of processing personnel. Salmonellae were found in samples taken on 37 of 48 visits; a greater number of recoveries were made on days when freshly killed turkeys were processed (87%) than when frozen-defrosted carcasses were processed (59%). The predominant serotype isolated from meat and environment usually changed from visit to visit. Salmonella sandiego and Salmonella anatum were the most frequent among 23 serotypes recovered. Most of the isolated serotypes are commonly associated with turkeys and have been incriminated as causative agents of human salmonellosis. The implication is that further-processed turkey products, if inadequately cooked by the consumer and if improperly refrigerated between the time of manufacture and consumption, could directly transmit salmonellae. These same products might also contaminate other foods by introducing salmonellae into food-preparation areas.     

Histochemistry of implantation in the rabbit

Summary The distribution of glycogen, acid and neutral mucopolysaccharides, hydrolases alkaline phosphatases, and carbohydrate dehydrogenases is described in the rabbit blastocyst and its surroundings over the implantation period from 5 to 9 days.Glycogen is found mainly in the embryonic tissues, where peaks of concentration coincide with differentiation, some is also seen in the uterine epithelium and secretion, and large quantities accumulate in the developing decidua.Neutral mucopolysaccharide is found in the yolk-sac and embryonic endoderm, and as secretion droplets in the uterine epithelium and secretion.Acid mucopolysaccharide occurs in the embryonic coverings and uterine secretion.RNA is associated in the embryo with developing tissues, and accumulates in the developing decidual cells.Hydrolases (acid phosphatase, and B esterase) increase their activity in the trophoblast knobs, in developing syncytiotrophoblast, and in the embryonic endoderm. Degeneration of the uterine epithelium is associated with maximal hydrolase activity.Trophoblastic alkaline phosphatase activity (non-specific and specific) decreases from 5 to 7 days of gestation, then increases markedly in the developing syncytiotrophoblast. AMPase appears in the embryonic mesoderm. In the uterine epithelium intense brush border staining is seen, and TPPase and UDPase become visible for a short period in the Golgi region. Phosphatases increase their activity in the decidua to 8 days and then decrease.Carbohydrate dehydrogenases (except -glycero-phosphate and -hydroxy-butyrate dehydrogenases) increase their activity in embryonic tissues, particularly in the developing syncytiotrophoblast and endoderm. Symplasma formation in the uterine epithelium is also associated with increase in enzyme activity, and a similar increase, up to 8 days of gestation, is seen in the decidua with isocitrate, malate, glucose-6-phosphate, lactate, succinate, and furfuryl alcohol dehydrogenases.Some correlation is found between the histochemical findings and the phenomena of epithelial removal, uterine secretion, decidual formation and function, giant cell function, morphogenesis, and histiotrophic nutrition, and the results are compared with previous findings for the rat in which implantation is morphologically, and probably physiologically a very different process.     

Comparative histochemical distribution of “leucine amino-peptidase” in the placenta and foetal membranes

Summary The distribution of an enzyme, or enzymes hydrolysing l-leucyl--naphthylamide is studied in the placentae, foetal membranes, and uterine structures of the horse, sheep, cat, dog, ferret, rat, rabbit, guinea-pig, and human. Activity is seen mainly in the trophoblast (except that of the cat, dog, and guinea-pig), in the rodent yolk-sac endoderm (except that of the rat), or in the uterine epithelium — surface (sheep and guinea-pig) or glandular (dog). The presence of the enzyme or enzymes is correlated with possible functions in absorption and transport of materials, or in elaboration and release of complex molecules.     

Hormonal stimulation of tyrosinase activity in human foreskin organ cultures

Summary A human foreskin organ culture system has been developed to study the response of human skin to hormonal stimulation. Foreskins are maintained in culture on floating plastic supports which allows the epidermal surface to be exposed to air while the dermis is bathed in nutrient medium. Both black and white human foreskins can be maintained in organ culture for at least 1 wk with no change in the tissue structure or cell viability as determined by histochemical staining and by dopa reaction staining. Tyrosinase activity in both black and white human foreskin cultures decays markedly during the first 2 d of culture to a new steady state level which remains stable throughout the culture period. Both black and white foreskin cultures consistently demonstrate 2- to 10-fold increases in tyrosinase activity when treated with theophylline (1 mM). Approximately 90% of all skin cultures examined showed an increase in enzyme activity when treated with this phosphodiesterase inhibitor. Dibutyryl cAMP (0.1 mM) and [Nle⁴, D-phe⁷]-alpha MSH (10⁻⁸ M), were also found to markedly stimulate tyrosinase activity in some skin cultures, whereas alpha-MSH and prostaglandin E₁ produced only an inconsistent and small increase in the activity of the enzyme. Histamine (1 μM), vitamin D₃ (1 μM), and retinoic acid (1μM) failed to stimulate tyrosinase activity in either white or black foreskin cultures. This hormone-responsive organ culture system can be utilized to characterize the molecular processes responsible for the regulation of tyrosinase and pigmentation in human skin. This work was supported by a research contract from the Oklahoma Center for the Advancement of Science and Technology (OCAST) and by a research grant from the Presbyterian Health Foundation.