Suppression of B-cell differentiation by natural killer (asialo GM1+) cells in mice

Mice were injected intravenously with rabbit antiserum to ganglio-n-tetraosylceramide (asialo GM1, ASGM1), a neutral glycosphingolipid present at high quantities on the surface of natural killer (NK) cells. Spleen cells prepared from the mice were then examined for NK activity against YAC-1 targets, for phagocytic cells and by flow cytometric analysis for Thy1, Lyt1, Lyt2, ASGM1 and surface Ig (SIg) phenotypes. Administration of anti-ASGM1 in mice resulted in a complete depletion of NK activity and ASGM+1 cells in the spleen, but no changes in the proportions of Thy1+ cells and their Lyt1+ and Lyt2+ subsets and phagocytic cells. Corresponding to this selective depletion of ASGM+1 cells and NK activity, the spleen cells showed an increased number of SIg+ B cells and augmented mitogenic responses to B-cell but not T-cell mitogens. These NK-depleted spleen cells also showed production of pokeweek mitogen (PWM)-driven plaque-forming cells (PFC) to much higher levels than those of control spleens. In the spleens of mice treated with varying concentrations of anti-ASGM+1, a good correlation was found between the decreased NK activity and the enhanced PFC response. To directly test the possible suppressor activity of NK cells on PWM-induced PFC response, NK (ASGM+1) cells were highly purified from the spleen by a combination of Percoll gradients and cytolysis of T cells by monoclonal antibodies followed by indirect panning. When added to NK-depleted spleen cells, they suppressed the augmented PFC response of NK-depleted spleen cells, depending on the number of cells added. These results suggest that NK (ASGM+1) cells in mice exhibit a suppressor property on B cells, which are undergoing spontaneous or mitogen-induced differentiation.     

Extrapyramidaler Kern und extrapyramidale Fasern im Accessorius und Hypoglossus

Zusammenfassung Die kleinen Zellen im Accessoriuskern und Hypoglossuskern, die in Form und Bau der Neben- und Mittelzelle Waldeyers im Rückenmark sehr nahe stehen, zeigen deutliche retrograde Veränderung nach der Durchtrennung des Accessorius bzw. Hypoglossus. Wir möchten dem-nach diese Zellen als extrapyramidalen Kern und die kleine markhaltige Faser im N. accessorius und hypoglossus als extrapyramidale Faser betrachten.     

Correlation Between Urea and Other Chemical and Biological Parameters in Waters of Lake Suwa,Japan

The vertical profiles of chemical and biological parameters, including urea concentration, have been measured periodically since February of 1977 at a central station in Lake Suwa, which is one of the typical eutrophic lakes in Japan. The seasonal trend in the standing stock of urea in the central water column, together with the ratio of urea versus total inorganic nitrogen in the euphotic zone from 12 March, 1977 to 25 July, 1978, are presented. The possible importance of bacterial decomposition of dead phytoplankton as a urea source in natural waters is demonstrated by this study. At times, a highly significant correlation between the vertical profile of urea and vertical distributions of other chemical and biological parameters which were also measured was found. An apparent in situ utilization of urea by phytoplankton is suggested on the basis of vertical profiles of urea and other chemical and biological parameters.     

Tumor DNA circulating in the plasma might play a role in metastasis. The hypothesis of the genometastasis.

BACKGROUND: Clinical and experimental observations suggest that more than one pathway might be involved in the development of metastases. In the present study, we examined the presence of tumor DNA in plasma using an experimental model in which tumor cells were modified with a genome-associated tag. We also investigated whether plasma of tumor-bearing rats had any effect on cultured cells and healthy animals. METHODS: Transfected cancer cells (DHD/K12-PROb stably transfected with pCDNA3.1CAT.) were injected subcutaneously into the chest of BD-IX rats. Animals were divided into ten groups according to the time between injection of tumor cells and euthanasia. Prior to euthanasia (2-14 week), blood samples were collected by cardiac puncture. To detect circulating tumor cells and CAT-encoding DNA in plasma, we performed PCR with nested primers. Fifty samples of plasma were chosen at random to supplement the medium of fifty cultures of DHD cells for 10-12 days. PCR for the detection of CAT DNA in cells was performed approximately one to two months later. Four healthy rats received an intraperitoneal injection of plasma from a tumor-bearing rat five times at week for 4 to 6 weeks. Animals were sacrificed and samples of liver, kidney, spleen, omentum, blood and lung were processed by PCR for the detection of CAT DNA. RESULTS: Detection of CAT DNA in plasma was slightly more frequent than in the buffy-coat fraction. All surviving cultures that had been supplemented with plasma were positive at some point for CAT DNA. In all four healthy animals injected with plasma of tumor-bearing rats, the marker gene for CAT was found in extracts of lungs. CONCLUSION: Our present observation lead us to propose the following hypothesis. Metastases might develop as a result of transfection of susceptible cells in distant target organs with dominant oncogenes that are present in the circulating plasma and are derived from the primary tumor.