Putrescine export from leaves in relation to floral transition in Sinapis alba

Sinapis alba L. was induced to flower by either a long day or a displaced short day. Following collection of leaf (phloem) and root (xylem) exudates from induced and non-induced plants, polyamines in the exudates were extracted, separated and analyzed quantitatively. The titers of free and conjugated putrescine the major polyamine fractions in all samples, increased early and markedly in leaf exudates during the floral transition, coinciding closely with movement of the floral stimulus out of the induced leaf. By contrast, putrescine titer in the root exudate did not increase. A spray of difluoromethylornithine (DFMO), an irreversible inhibitor of the putrescine-biosynthetic enzyme ornithine decarboxylase, at hour 8 of the long day considerably reduced the titer of free and conjugated putrescine in leaf exudates, and at the same time, markedly decreased the flowering response of induced plants. This effect of DFMO on flowering was substantially reversed by a simultaneous application of putrescine to the roots. DFMO sprayed on induced plants also suppressed early activation of indices of both mitosis and DNA synthesis in the shoot apical meristem. These results support the view that the extra putrescine synthesized in induced leaves is a necessary component of the floral stimulus in Sinapis.     

Radiolabeled Ligands Specific for the G Protein-Coupled State of Neurotensin Receptors

Abstract: Radiolabeled analogues of neuromedin N have been prepared by acylation of the α, ε1, and ε2 amino groups of [Lys²]neuromedin N (Lys-Lys-Pro-Tyr-Ile-Leu) either with the ¹²⁵I-labeled Bolton-Hunter reagent or with N -succinimidyl[2,3-³H]propionate. The binding properties of the purified analogues toward newborn mouse brain homogenate or toward membranes of cells transitorily (COS) or permanently (AA1) transfected with the cloned rat brain neurotensin receptor cDNA were evaluated and compared with those of radiolabeled neurotensin. The α-modified analogue of [Lys²]neuromedin N behaves exactly like neurotensin in these binding experiments, whereas the ε1- and ε2-modified analogues selectively recognize the fraction of neurotensin binding sites that is sensitive to GTPγS. The proportion of neurotensin receptors coupled to GTP binding proteins is ∼50% in membranes of newborn mouse brain or of AA1 cells that respond to neurotensin by an increase of the intracellular inositol trisphosphate concentration. By contrast, membranes of transitorily transfected COS cells that do not respond to neurotensin exhibit very low levels of GTP-sensitive receptors labeled with the ε1- or ε2-modified analogues. These radiolabeled peptides offer new tools to selectively detect active neurotensin receptors.     

Evolution ofDrosophila repetitive-dispersed DNA

We have examined the phylogenetic distribution of a spectrum of Drosophila repetitive-dispersed DNAs ranging from structurally complex transposable elements to scrambled middle repetitive sequences. Our data suggest that unlike typical "genes" these DNAs are unstable components of the drosophilid genome. The unusual behavior of these repetitive-dispersed DNAs raises the possibility that this type of sequence may have an important role in the evolution of the family Drosophilidae.     

Methionine-enkephalin-like immunoreactivity in the nervous ganglion and the ovary of a protochordate,Ciona intestinalis

Summary When methionine-enkephalin antiserum was applied to paraffin sections of adult Ciona intestinalis it reacted with neurons in the ganglion and along the visceral nerve. The fluorescence was strong before and during spawning season, but partially disappeared at the end of August.With the same antibody a positive immunoreactivity was detected in the ovary during the growth of oocytes. The distribution of positive granules in the cytoplasm did not change significantly with varying lighting conditions (normal photoperiod, permanent light or darkness) in which the animals were maintained. In contrast, treatment with a substance isolated from crude extracts of Ciona (peroxide 1) induced a dense, crescent-like concentration of positive granules near the nucleus of oocytes. The follicular cells did not show any immunofluorescent reaction.This research was supported in part by a grant from CNRS (ATP JV/DP:N 4696-4697)A Gift from Dr. M. Bosc (I.N.R.A., Nouzilly, France)A Gift from Ciba Laboratory     

Neurofilament Phosphorylation in Cultured Bovine Adrenal Chromaffin Cells Is Stimulated by Phorbol Ester

Primary cultures of bovine adrenal chromaffin cells contain neurofilament proteins that are hypophosphorylated. When the cells were grown in medium containing 32Pi and 0.1 microM 12-O-tetradecanoyl-phorbol 13-acetate (TPA), 32P-labelling of the three neurofilament subunits was increased 6- to 20-fold relative to controls, the highest level of stimulation occurring for the mid-sized subunit. Addition of the protease inhibitor leupeptin to the growth medium had no effect on TPA-stimulated phosphorylation. The increased 32P incorporation was accompanied by a marked reduction in the gel electrophoretic mobilities of the two largest subunits. The augmented phosphorylation was observed 10 min after addition of TPA to a concentration of 0.1 microM or after 1 h of incubation in the presence of 0.01 microM TPA. One-dimensional peptide mapping and phosphoamino acid analysis indicated that TPA stimulated the phosphorylation of seryl residues at new sites in the mid-sized subunit. All of the latter subunit contained in the cytoskeletal fraction of chromaffin cells was converted to a more highly phosphorylated state after the cells were grown in the presence of TPA for 1 h.     

Female turtles from hot nests: is it duration of incubation or proportion of development at high temperatures that matters?

Summary Mean daily temperature in natural nests of freshwater turtles with temperature-dependent sex determination is known to be a poor predictor of hatchling sex ratios when nest temperatures fluctuate. To account for this, a model was developed on the assumption that females will emerge from eggs when more than half of embryonic development occurs above the threshold temperature for sex determination rather than from eggs that spend more than half their time above the threshold. The model is consistent with previously published data and in particular explains the phenomenon whereby the mean temperature that best distinguishes between male and female nests decreases with increasing variability in nest temperature. The model, if verified by controlled experiments, has important implications for our understanding of temperature-dependent sex determination in natural nests. Both mean nest temperature and hours spent above the threshold will be poor predictors of hatchling sex ratios. Studies designed to investigate latitudinal trends and inter-specific differences in the threshold temperature will need to consider latitudinal and inter-specific variation in the magnitude of diel fluctuations in nest temperature, and variation in factors influencing the magnitude of those fluctuations, such as nest depth. Furthermore, any factor that modifies the relationship between developmental rate and temperature can be expected to influence hatchling sex ratios in natural nests, especially when nest temperatures are close to the threshold.     

In vitro inhibition of the helper activity of GAT-specific T-cell lines by a syngeneic anti-idiotypic serum: preferential effect on the IgG response

We described in this paper the characteristics of a syngeneic anti-idiotypic serum made in BALB/c against BALB/c anti-poly (Glu⁶⁰ Ala³⁰ Tyr¹⁰) (GAT) antibodies. This serum recognizes idiotypic determinants present in all anti-GAT sera whatever the allotypic markers of the mice used to prepare the sera. The functional effect of this serum on two helper cell lines is also described. Cell line BDF₁/52 was obtained from GAT immunized lymph node cells (LNC). Cell line BDF₁/E₃ was selected from splenic T-cells educated in vitro on GAT-pulsed adherent cells. Both lines were propagated in presence of filler cells, antigen, and medium containing T-cell growth factor(s) from splenic cells activated with concanavalin A. Both cell lines exhibit a helper activity as measured by the plaque-forming cell (PFC) response they induce in vitro in the presence of DNP-GAT and DNP sensitized B cells. Their helper activity is specific and they require a hapten-carrier bridge to activate B cells. These lines are able to induce IgG₁, IgG_2a and IgG_2b anti-TNP PFC. Syngeneic anti-idiotypic serum B 658 inhibits specifically the function of these two lines but does not affect the helper activity of an OVA-specific T-cell line. The blocking activity of the serum can be adsorbed on a hybridoma protein with anti-GAT activity. This inhibition affects more dramatically the IgG₁ response than the IgG_2a and IgG_2b responses.     

Elements causing hybrid dysgenesis on the second chromosome ofDrosophila melanogaster

Summary Hybrid dysgenesis inDrosophila melanogaster is a syndrome of germline abnormalities including temperature-dependent gonadal dysgenesis (GD sterility), high rates of mutation and male recombination. In theP-M system, hybrid dysgenesis results from interaction between chromosomally-linked factors (P factors) and a particular extrachromosomal state refered to as theM cytotype. TheT007/Cy strain, shown by other authors to induce a high level of mutation and male recombination, is presently studied with respect to gonadal dysgenesis. TheP activity appears mainly linked with theT007 second chromosome and has been essentially mapped to a 0.6 centimorgan long interval, i.e. betweenhk andpr. On the other hand, 14 strains balanced for deficiencies on the left arm of the second chromosome are studied for their relative level ofM cytotype activity.In F1 females, inheriting the same maternal cytotype and the same paternalT007 chromosome, significant differences inGD sterility are found between flies receiving the maternal deficiency and those receiving the alternate non-deleted chromosome. This effect appears only when the chromosomes are deleted for a common region (37F5-38A7), suggesting the presence of elements intervening in the determinism ofGD sterility in this zone. As this region is included in the correspondinghk-pr interval (37C1-38B6), these results state the problem of the nature of the elements located in this interval and two hypotheses are discussed.