伍氏游仆虫接合过程中老大核后碎块的去向

在伍氏游仆虫(Euplotes woodruffi)接合后体发育过程中,已呈退化状态的老大核后碎块,在细胞第二次形态发生时,逐渐恢复其正常形态结构。T形新大核原基向后延伸而与恢复正常形态的老大核后碎块紧密靠拢。此时在光镜下观察,很容易误认为二者已融合为一。但在接合后体分裂之前,老大核后碎块再次瓦解,T形大核原基缩短成棒状而与老大核后碎块分开,此时二者界限分明。细胞分裂后,残存的老大核后碎块停留于后子虫中,最后被吸收。几个关键时期大核原基和老大核后碎块DNA含量的测定,也证明新老大核不融合。本文还讨论了老大核后碎块在有性过程中的功能。     

Persistence of Cell Division Synchrony in Spirogyra Insignis (Gamophyceae): Membrane Proteoglycans Transmitting Synchronizing Information Throughout Generations

Spirogyra insignis shows a long-term persistence of cell division synchrony in the absence of the synchronizing Zeitgeber, so that at least six generations are involved in the process. This tentatively suggests that a mechanism of transmission throughout generations of synchronizing information could maintain this synchrony. Apparently, a vital part of the molecular basis of this mechanism is a membrane proteoglycan complex. This complex could obtain temporal information from a synchronizing Zeitgeber and be transmitted to the progeny by distribution of plasma membrane between daughter cells.     

Purine nucleosides and nucleotides stimulate proliferation of a wide range of cell types

Summary Presumptive astrocytes isolated from 10-day white Leghorn chick embryos, Factor VIII-positive human brain capillary endothelial cells, meningeal fibroblasts from 10-day chick embryos, Swiss mouse 3T3 cells, and human astrocytoma cell lines, SKMG-1 and U373, were rendered quiescent when placed in culture medium that contained 0 or 0.2% serum for 48 h; their proliferation was markedly reduced and they incorporated [³H]thymidine at a low rate. [³H]Thymidine incorporation and cell proliferation were induced in all types of cells by addition of guanosine, GMP, GDP, GTP, and to a lesser extent, adenosine, AMP, ADP or ATP to the culture medium. The stimulation of proliferation by adenosine and guanosine was abolished by 1,3-dipropyl-7-methylxanthine (DPMX), an adenosine A₂ receptor antagonist, but not by 1,3,-dipropyl-8-(2-amino-4-chorophenyl)xanthine (PACPX), an A₁ antagonist. Stimulation of proliferation by the nucleotides was not abolished by either DPMX or PACPX. The P₂ receptor agonists,α,β-methyleneATP and 2-methylthioATP, also stimulated [³H]thymidine incorporation into the cells with peak activity at approximately 3.5 and 0.03 nM, respectively. These data imply that adenosine and guanosine stimulate proliferation of these cell types through activation of an adenosine A₂ receptor, and the stimulation of cell proliferation by the nucleotides may be due to the activation of purinergic P_2y receptors. As the primary cultures grew older their growth rate slowed. The capacity of the purine nucleosides and nucleotides to stimulate their growth diminished concomitantly. The 3T3 cells showed neither decreased growth with increased passages nor reduced response to the purines. In contrast, although the doubling time of the immortalized human astrocytoma cell lines SKMG-1 and U373 remained constant, the responsiveness to purinergic stimulation of the U373 cells decreased but that of the SKMG-1 did not. These data are compatible with a decrease in the number, or the ligand-binding affinity of the purinergic receptors, or a decreased coupling of purinergic receptors to intracellular mediators in primary cells aged in tissue culture.     

On the precision and accuracy achieved by Escherichia coli cells at fission about their middle

Length and width of each of the prospective siblings of constricted Escherichia coli cells from different strains and culture conditions were measured from electron micrographs. The data were statistically analyzed to investigate how equally the length and volume of one cell was divided into two. The analysis showed that, for all cultures, bipartition is unbiased or very nearly so, i.e. sibling cells were on the average equally long and large. The precision of bipartition attained by the cells was usually high; it was related to the average cell shape (length/width): slender E. coli cells divided into two less precisely than squat cells. Absolute size, growth rate and strain specificity affected the precision of bipartition only indirectly, i.e. in as much as they influenced cell shape.     

INFLUENCE OF ENVIRONMENTAL FACTORS AND POPULATION COMPOSITION ON THE TIMING OF CELL DIVISION IN THALASSIOSIRA FLUVIATILIS (BACILLARIOPHYCEAE) GROWN ON LIGHT/DARK CYCLES1

Cell division patterns in Thalassiosira fluviatilis grown in a cyclostat were analyzed as a function of temperature, photoperiod, nutrient limitation and average cell size of the population. Typical cell division patterns in populations doubling more than once per day had multiple peaks in division rate each day, with the lowest rates always being greater than zero. Division bursts occurred in both light and dark periods with relative intensities depending on growth conditions. Multiple peaks in division rate were also found, when population growth rates were reduced to less than one doubling per day by lowering temperature, nutrients, or photoperiod and the degree of division phasing was not enhanced. Temperature and nutrient limitation shifted the timing of the major division burst relative to the light/dark cycle. Average cell volume of the inoculum was found to be a significant determinant of the average population growth rate and the timing and magnitude of the peaks in division rate. The results are interpreted in the context of a cell cycle model in which generation times are “quantized” into values separated by a constant time interval.     

Visualization of thrombin receptors on mouse embryo fibroblasts using fluorescein-amine conjugated human α-thrombin

The localization of thrombin receptors on mouse embryo (ME) cells has been examined by direct fluorescence microscopy using a fluorescein aminelabeled thrombin. Two fluorescein amines, 4-(N-6-aminoethyl thioureal)-fluorescein and 4-(N-6-aminohexyl thioureal)-fluorescein, were synthesized and attached to the carbohydrate moiety of highly purified human α-thrombin by periodate oxidation of the carbohydrate and selective reduction of the Schiff's base using sodium cyanoborohydride. Preparations of fluorescent thrombin with from 1 to 4 fluoresceins per molecule of thrombin retained their ability to proteolytically cleave fibrinogin to form fibrin clots, to bind to thrombin receptors on ME cells, and to initiate cell division. After incubating mitogenic concentrations of the fluorescein amine labeled thrombin with ME cells at 4°C, a diffuse fluorescent pattern was observed over the surface of the ME cells. This diffuse pattern was specific: it was not observed on cells from parallel cultures incubated with fluorescent thrombin plus a 20-fold excess of unlabeled thrombin. Thus, thrombin receptors appear to be distributed randomly over the surface of ME cells prior to interaction with thrombin. Increasing the temperature to 37°C following binding at 4° C resulted in a rapid dissociation of the fluorescent pattern from the cells leaving only the autofluorescent vesicles. This result may reflect the unique ability of thrombin to proteolytically cleave its own receptor.     

Précisions Temporelles sur les Processus de la Stomatogenèse de Tetrahymena paravorax analysés en Microscopie Photonique

Resume. Une analyse des séquences morphogénétiques du CiliéTetrahymena paravorax montre que: (A) La durée de la stomatogenèse de bipartition des formes microstomes en croissance exponentielle représente 45% du temps de génération (stade 1—20%; stade 2—3%; stade 3—3%; stade 4—5%; stade 5—5%; stade 6—9%). (B) La division cytoplasmique est inégale (les proters sont plus petits que les opisthes); la différence de taille initiale entre les 2 produits de fission est probablement compensée par une prolongation de la période de croissance chez le proter. (C) Le pourcentage maximum de réorganisation buccale microstome → macrostome pour les populations asynchrones atteint –? 70% au bout de 210 mn d'incubation dans la stomatine. (D) L'initiation de la stomatogenèse de remplacement oral est connectée avec la fin d'une période dont la durée minimale est approximativement celle du stade 0 du cycle normal d'interdivision des microstomes; cette initiation est retardée chez les microstomes exposés à la stomatine dès le début du cycle cellulaire. (E) Le primordium buccal de division peut se résorber en présence de stomatine et la stomatogenèse antérieure peut commencer avant que ne soit terminée cette résorption; la résorption n'est plus induite au-delà d'un point du stade 5 qui précède le début de la constriction du corps cellulaire. SYNOPSIS. An analysis of the morphogenetic sequences in the ciliate Tetrahymena paravorax has shown that: (A) The duration of predivision stomatogenesis in exponentially growing microstomes occupies 45% of the generation time (stage 1—20%; stage 2—3%; stage 3—3%; stage 4—5%; stage 5—5%; stage 6—9%). (B) Cytoplasmic division is unequal (the proters are smaller than opisthes); the initial size difference between the 2 fission products is presumably compensated by an increased growth period in the proter. (C) The maximum percentage of microstome-to-macrostome oral reorganization is –? 70% in asynchronous populations, 210 min after suspension in stomatin. (D) Initiation of oral replacement stomatogenesis is associated with the end of a period which has a minimum duration nearly equal to that of stage 0 characteristic of the normal inter-division cycle of the microstomes; this initiation is delayed if exposure of microstomes to stomatin is begun at the onset of the cell cycle. (E) The buccal primordium formed in division can be resorbed in presence of stomatin and anterior stomatogenesis can start before the resorption is completed: this resorption is not induced if the cells have progressed beyond a point which precedes the beginning of the cell furrowing (stage 5).     

Morphogenesis in the Heterotrich Ciliate Climacostomum virens. I. Oral Development During Cell Division

The principal characteristics of stomatogenesis during division in Climacostomum virens are: (A) Kinetosomal proliferation on the left side of a variable number of kineties in the ventral somatic cortex forms an oral primordium consisting of several kinetosomal fields, which then fuse to form a single anarchic field. (B) A constant topographical relationship exists between the primordium and a well defined cortical pattern, the zone of discontinuity. (C) The anarchic field primordium divides into 2 unequal parts—to the left, the AZM primordium, and to the right, the paroral primordium, which differentiates into the apical membranelles, the peristomial field, and the buccal tube. (D) Preoral and oblique kineties of the somatic cortex form along the right side of the paroral primordium. (E) Parental oral structures are partially dedifferentiated. Stomatogenesis in C. virens and other heterotrichs is compared.     

RNA Synthesis in Division Synchronized Tetrahymena: Macronuclear and Cytoplasmic RNA*

SYNOPSIS. Synthesis of RNA in the macronucleus and appearance of RNA in the cytoplasm were studied in heat synchronized Tetrahymena pyriformis GL and compared to those found under conditions of logarithmic growth (28 C) and during heat shocks (34 C). In macronuclei of logarithmically growing cells precursors were processed to 2 rRNA species (25S and 17S). In addition, another RNA (15S), more homogeneous than the RNA (8-15S) in the cytoplasm, was observed in the macronucleus. Both 17S and 25S rRNA species were found in the cytoplasm, 17S rRNA appearing more rapidly than 25S rRNA. Synthesis of rRNA was suppressed at 34 C in cells subjected to heat synchronization; 8-15S RNA synthesis appeared to be inhibited to a lesser extent. During the time preceding the first synchronized division, the synthesis of rRNAs in the macronucleus slowly recovered. Early in the cycle, almost no newly synthesized rRNAs were extracted. By 30 min after the last heat shock (EH), most of the RNA synthesized was not identified as rRNA. By 60 min after EH, the pattern of RNA synthesis had not returned to that observed in logarithmically growing cells.     

Nuclear Division in the Ameboflagellate Adelphamoeba galeacystis

Nuclear division in synchronized cultures of the ameboflagellate Adelphamoeba galeacystis has been described. Division in this organism is typically promitotic. It occurs within an intact nuclear membrane and is characterized by the persistence of the nucleolus and its transformation into 2 polar masses. The nucleolus is stained with pyronin-Y by the methyl green pyronin-Y technic, and with Heidenhain's hematoxylin, but is unstained by the Feulgen reaction. The reaction with these stains is removed after digestion of the nucleolus by ribonuclease. During mitosis the nucleolus undergoes an orderly series of vacuolizations before forming the polar masses. The chromatin is Feulgen positive, stains with methyl green by the methyl green pyronin-Y technic and undergoes a series of characteristic changes during the division process. Synchronization of amebae grown on coverglasses was accomplished by transfer of cells from 30 to 38.5 C for a period of 100 min. A temporal sequence of nucleolar and chromatin participation in the nuclear division of this organism is suggested.