Studies on the stimulation of cAMP metabolism in human lymphocytes by latex polymers

The purpose of this investigation was to further characterize the marked increase in intracellular cAMP which follows the interaction of human lymphocytes and latex polymers. Six distinct cell types, each of which either bind or ingest these latex particles, were studied; however, only lymphocytes responded with increases in intracellular cAMP. The initial attachment of the latex particles to the lymphocyte surface was independent of temperature, cyclic nucleotides and divalent cations in the external milieu. The subsequent cAMP response was maximal at physiologic temperatures and modulated by agents thought to alter microfilament and microtubule function. Four different types of polymers produced increases in intralymphocytic cAMP and the maximal increases were confined to particles having a mean diameter of 0.4–2.02 μm. Within this latter size range, there was a close correlation between the number of membrane-associated particles and the magnitude of the cAMP response. Similarities to the lymphocyte-lectin activation system included:

1. 1. A requirement for binding of the latex polymers to the external plasma membrane.

2. 2. A biphasic cAMP response characterized by an early rise followed by a later fall.

3. 3. Modulation of this response by pharmacologic agents which compromise microtubule and microfilament function.

In contrast to the lectin-induced activation, latex beads inhibited amino acid transport and phosphatidylinositol turnover and did not lead to later increases in DNA synthesis. These data suggest that latex polymers attach to receptors on the plasma membrane different from those responsible for lymphocyte activation, and through cAMP induce metabolic responses dissimilar to those associated with lectin activation.     

Chemotaxis in Physarum polycephalum : Effects of chemicals on isometric tension of the plasmodial strand in relation to chemotactic movement

The effects of chemicals were examined on the isometric tension of the plasmodial strand of the true slime mold Physarum polycephalum, and chemotactic motive forces were compared with the contractile properties of the strand. The results were:

1. 1. Isometric tension changed rhythmically within a period of 3–4 min and a few mg in amplitude. Application of attractants (glucose, galactose, maltose, Ca(H₂PO₄)₂, and K(H₂PO₄) led to a decrease in the amplitude of the tension. Contrary to this, repellents (sucrose, inorganic salts) increased the amplitude of the tension. The base line of the tension did not change appreciably unless the concentration of chemicals applied was not too high as compared with respective thresholds.

2. 2. Changes in the isometric tension, F, induced by application of chemicals were analysed quantitatively in terms of integral of isometric tension with respect to time during a period as defined by S=F dt. The values of S changed gradually with increase of concentration of chemicals above their respective thresholds.

3. 3. The threshold concentrations of chemicals determined by measurements of the isometric tension agreed with those obtained from chemotactic motive force and from membrane potential changes.

4. 4. The plasmodium of Physarum polycephalum moved away vigorously from high osmolarity by producing a large transient increase of motive force of the protoplasmic movement. Similarly, the isometric tension increased transiently with a high peak when the concentration of sugars and glycerol exceeded 0.2 M. The maximum tension was linearly proportional to the diameter of the strand.

These results indicate that contraction or relaxation of the plasma gel is the primary cause of the negative and positive chemotaxis in the slime molds.     

Heterochromatin diversity in Cymbidium, and its relationship to differential DNA replication

1. 1. DNA was extracted from aseptical cultures of protocorms of the orchid Cymbidium and analysed by thermal denaturation. The denaturation profiles revealed an AT-rich fraction of about 18% of total DNA.

2. 2. Mitotic chromosomes and diploid and endopolyploid nuclei of in vitro cultured protocorms and root tips were differentially stained with quinacrine (Q), 33258 Hoechst (H) and a novel compound 4′-6-diamidino-2-phenylindole (DAPI) [10], as well as by the Giemsa C-banding technique. The centromeric regions display very bright fluorescence with all three fluorochromes and stain intensely following the Giemsa procedure. It is proposed that the AT-rich fraction of the Cymbidium DNA is located within the centromeric heterochromatin.

3. 3. In interphase nuclei differential Q, H, and DAPI fluorescence both within and between the chromocenters occurs. In nuclei with enlarged chromocenters, i.e. with amplified DNA in heterochromatin [2], the increased size of chromocenters is mainly caused by enlargement of the less brightly fluorescing fractions of the heterochromatin. The proportion of the very brightly fluorescing heterochromatin is similar in all nuclei (about 7%).

4. 4. A comparison of nucleolar size and differential Giemsa staining of the nucleolus organizers showed that there is no disproportional increase of nucleoli and nucleolus organizing heterochromatin during endopolyploidization. That means, there is no indication for amplification of ribosomal DNA.

5. 5. Electron micrographs particularly of heterochromatin-rich nuclei revealed areas of different chromatin density within and between the chromocenters. However, the differences in fiber packaging density are much smaller than the observed differences in fluorescence brightness.

6. 6. The data obtained are interpreted as evidence for differential replication of AT-rich and non-AT-rich heterochromatin. It is suggested that DNA amplification [2, 4] is restricted to a non-AT-rich component which apparently is located neither in the brightly fluorescent centromeric nor in the nucleolus-associated heterochromatin.

     

Changes in the activities of mitochondrial carriers during the development of Xenopus laevis

The transport of the substrates phosphate, pyruvate, malate, fumarate, α-ketoglutarate, citrate, isocitrate and glutamate has been determined in mitochondria isolated from various developmental stages of Xenopus laevis. The carriers may be sub-divided into three groups with respect to the pattern of changes in activity:

1. 1. Pyruvate, tricarboxylate and glutamate/OH carriers, distinguished by low activities during the pregastrula stages and a subsequent increase in activity.

2. 2. Phosphate and α-ketoglutarate carriers, with a constant activity throughout development.

3. 3. Malate and fumarate carriers, highly active initially, but decreasing already after gastrulation.

The results are discussed in relation to mitochondrial differentiation and the change from embryonic to adult metabolism.     

Countercurrent distribution and multiple sedimentation of Chlorella pyrenoidosa during its life cycle

Synchronously and normally grown Chlorella pyrenoidosa cell populations were analysed by countercurrent distribution in aqueous two-polymer phase systems and by a multiple sedimentatation technique. Partition of cells in aqueous phases reflects the surface properties of cells (primarily surface charge) and multiple sedimentation reflects the cells' size-density parameters. It was found that:

1. 1. Synchronized cells that have just divided have the lowest partition of any in the population. Surface charge (as reflected by partition) increases with time after cell division. Cells have the highest partition just prior to division.

2. 2. Synchronized cells that have just divided are the smallest of any in the population. Since size and sedimentation rate increase with time after cell division multiple sedimentation permits the separation of cells of different ages.

3. 3. Both countercurrent distribution and multiple sedimentation studies reveal considerable heterogeneity of synchronized Chlorella populations. The increase in both surface charge and size with cell age does not appear to proceed in a continuous fashion. Rather, it seems to go in a stepwise manner.

4. 4. Non-synchronized cells examined by either countercurrent distribution or multiple sedimentation show two distinct sub-populations. One of these corresponds to the youngest, just divided cells; and the other to cells just prior to cell division. It is suggested that a lag time just prior to cell division and just after cell division explains these results.

5. 5. Countercurrent distribution in two-polymer phases and multiple sedimentation at unit gravity in a suspension medium best suited for the cell under investigation seem to be methods of choice for tracing cell changes during division, maturation and aging and for sub-fractionating such cell populations.

     

Induction of cell spreading by substratum-adsorbed ligands directed against the cell surface

Studies were carried out to compare the spreading of baby hamster kidney (BHK) cells, which occurs by an interaction between the cells and a specific serum glycoprotein (ASF) adsorbed onto the substratum surface, with the spreading of BHK cells that occurs by an interaction between the cells and substrata coated with ligands directed at various cell surface determinants. The ligands tested were polycationic ferritin, concanavalin A (ConA) and antibody directed against BHK plasma membranes. Cell spreading onto ASF and ligand-coated substrata were similar even though different cell surface components were apparently involved. The similarities were:

1. 1. The shape of the spread cells.

2. 2. The inhibition of cell spreading by conditions that interfere with metabolic activity, block free sulfhydryl groups, or interfere with microtubules and microfilaments.

3. 3. The similar reorganization of certain cell surface antigenic determinants during cell spreading onto any of the substrata.

The results indicate that cell spreading is a general cellular response to specific cell-substratum interactions but does not depend upon binding between a unique cell surface receptor and the substratum.     

Commitment to differentiation in Friend cells and initiation of globin mRNA synthesis occurs during the G1 phase of the cell cycle

We have measured the kinetics of specific globin mRNA and Friend virus (FV) RNA synthesis by hybridization to immobilized cDNA after induction of differentiation of two erythroleukemia cell lines (F4N, B8) by butyrate and Me₂SO. The induction with butyrate in these cell lines occurs very rapidly (16–24 h). Cell cycle analysis was made of the populations throughout induction by flow cytofluorometry. The kinetics of commitment of cell populations to terminal differentiation by butyrate was determined by removal of inducer at various times and scoring of benzidine staining cells (hemoglobin producing). In addition, the cell cycle dependence of commitment was determined by flow sorting out of G1 and S+G2 cells various times after addition of inducer and scoring benzidine-stained colonies after growth in methylcellulose. Cells exposed to inducer were also sorted by cell cycle phase using an elutriator rotor. The amount of globin mRNA synthesis in the different cell populations was then determined.

1. 1. It was found that an 8–12 h period in butyrate was required before (a) globin specific mRNA was synthesized; and (b) commitment to differentiation occurred. The time course of globin mRNA synthesis was positively correlated with G1 arrest, as has been also found by others.

2. 2. The increase of FV RNA synthesis was not found during G1 arrest. It occurred early and before commitment.

3. 3. Commitment of cells to irreversible differentiation upon butyrate induction occurs only during the G1 phase of the cell cycle.

4. 4. Globin mRNA synthesis occurs first only in G1 cells.

5. 5. Globin mRNA is synthesized later in all phases of the cell cycle.

These data suggest that (a) commitment to differentiation and globin mRNA accumulation are coupled; and (b) that both events occur only in G 1 cells after a pre-commitment phase of about 12 h.     

The effect of copper on frog skin. The role of sulphydryl groups

1. 1. Cu²⁺ at a concentration of 10⁻⁴ M, when applied to the external side of the frog skin produces an increase in the short-circuit current (I_sc).

2. 2. This effect was studied in skins of Rana temporaria adapted to cold (5°C) and room temperature (20°C), skins of Rana pipiens adapted to cold, and the results compared with those obtained previously with Rana ribibunda.

3. 3. The observed effect is less dependent upon the adaptation to cold than upon the functional state of the skin: skins with low short circuit currents have a bigger response to Cu²⁺ than skins with high I_sc.

4. 4. A species difference cannot be ruled out since skins of Rana ribibunda exhibiting high I_sc give good responses to Cu²⁺.

5. 5. 5,5′-dithiobis(2-nitrobenzoic acid), a sulphydryl-oxidizing reagent, produces an effect similar to that of Cu²⁺, and dithiothreitol an SH-reducing agent, reverses the effect of this ion.

6. 6. Cu²⁺ also induces an increase in the unidirectional K⁺ fluxes and unmasks a net outward potassium flux.

7. 7. The outward K⁺ flux induced by Cu²⁺ is sensitive to ouabain.

8. 8. It is concluded that Cu²⁺ increases the permeability of the external barrier of the frog skin to Na⁺ and K⁺, probably by reacting with SH groups.

Fluorimetric determination of the resting potential changes associated with the chemotactic response in Paramecium

1. (1) Evidence is presented which indicates that the carbocyanine dye (3,3′ dipropyl thiadicarbocyanine) can be used as a spectroscopic probe for monitoring the resting potential across the plasma membrane of the ciliated protozoan Paramecium.

2. (2) The dye at low concentrations ( 1 μM) does not affect either the viability or the motility of the cells, nor does it induce a chemotactic response.

3. (3) The fluorescence of the dye bound to the cells alters as the potential across the membrane is changed by increasing the external cation concentration.

4. (4) The absorbance of the bound dye also changes in response to an alteration of the membrane potential.

5. (5) The membrane potential changes as measured by the fluorescence method have been correlated with the measurements of the potential estimated by microelectrode methods.

6. (6) Both cations which induce a negative chemotactic response in Paramecium (K⁺, Na⁺, Ba²⁺) and several non-toxic cations bring about a rapid depolarization of the plasma membrane. The significance of these rapid changes in relation to the swimming behaviour of the ciliate is discussed.

Mechanical properties of the surface of the sea urchin egg at fertilization and during cleavage

1. 1. Changes in stiffness of the cell surface at fertilization and during cleavage in sea urchin eggs were determined by the magnetic particle method.

2. 2. The stiffness of the cell surface increased at fertilization, reached a maximum after about 1.5 min, then decreased and reached a minimum about 4 min after insemination, followed by a gradual increase, in the eggs of Temnopleurus toreumaticus at 25.5 to 26.5 °C.

3. 3. The stiffness of the cell surface increased during the diaster stage, reached a maximum 2 to 3 min before the onset of cleavage, then decreased to a minimum about 1 min before the onset of cleavage, increased again, reached a maximum during cleavage and then diminished, in the eggs of Temnopleurus toreumaticus at 25.5 to 26.5 °C. A similar stiffness change was observed in the eggs of Hemicentrotus pulcherrimus at 17 to 19 °C, occurring almost in parallel in both the equatorial and polar surfaces.

     

Chemical modification by trinitrobenzenesulfonate of a lipid and proteins of intracytoplasmic membranes isolated from Chromatium vinosum and Azotobacter vinelandii

1. 1. The structure of intracytoplasmic membranes of a photosynthetic bacterium Chromatium vinosum and a nitrogen-fixing bacterium Azotobacter vinelandii was studied by chemical modification of amino groups of phospatidylethanolamine and proteins with trinitrobenzensulfonate.

2. 2. Almost all the constituents of intracytoplasmic membranes of C. vinosum were solubilized in a mixture of chloroform, methanol and trichloroacetic acid. One-third of proteins in the intracytoplasmic membranes of C. vinosum was found solubilized in a mixture of chloroform and methanol. By using a column chromatography with Sephadex LH-20 in organic solvents, the unmodified as well as the trinitrophenylated proteins and also the trinitrophenylated phosphatidylethanolamine were separated from the other colored substances.

3. 3. In the chemical modification of the intracytoplasmic membrane preparations, 30% of phosphatidylethanolamine and 15% of protein amino groups in C. vinosum and 45% of phosphatidylethanolamine and 20% of protein amino groups in A. vinelandii were estimated to be exposed to the aqueous phase. In the single-layered liposomes composed of phosphatidylethanolamine and phospatidylglycerol with a ratio of 2:1, 40% of phosphatidylethanolamine were estimated to be exposed to the aqueous phase.

The use of fluorescein-conjugated Bandeiraea simplicifolia B4-isolectin as a histochemical reagent for the detection of α- -galactopyranosyl groups : Their occurrence in basement membranes

The Bandeiraea simplicifolia B₄-isolectin, which combines specifically with α- -galactopyranosyl groups, has been conjugated with fluorescein isothiocyanate and demonstrated to be a reliable histochemical probe for the detection of these groups in normal tissues of mouse, rabbit, rat and man. Specificity of binding of the fluorescein-conjugated B. simplicifolia B₄-isolectin to native cryostat tissue sections was demonstrated in two ways:

1. 1. The hapten inhibitor methyl α- -galactopyranoside prevented the binding of the lectin to tissues whereas the non-hapten methyl α- -glucopyranoside did not.

2. 2. Pretreatment of tissue sections with coffee bean α-galactoside abolished lectin binding whereas pretreatment with A. niger or E. coli β-galactosidase did not. The fluorescein-conjugated isolectin visualized α- -galactopyranosyl groups in basement membranes and on the surface of certain epithelial cells of mouse, rat, rabbit, and on the surface of the TA3 murine mammary carcinoma. These studies suggest that the B. simplicifolia B₄-isolectin may be of great utility in studying the family of α- -galactosyl-containing glycoconjugates of basement membranes in pathological states accompanied by basement membrane changes, such as diabetes mellitus, and in neoplasms that secrete basement membrane.

     

C-NMR detection of lipid polymorphism in model and biological membranes

1. 1. The application of the ¹³C-NMR technique to the study of lipid polymorphism is described for various model and biological membranes.

2. 2. The ¹³C-NMR line-width of various resonances of the lipid molecule are sensitive to the bilayer hexagonal and the bilayer ‘isotropic’ phase transition. The latter transition in some cases is accompanied by the occurrence of lipidic particles as detected by freeze-fracturing. Thus, specific ¹³C-labeling experiments allow the study of the individual phase behaviour of lipids in mixed lipid systems.

3. 3. In diet experiments using rats, the choline group of phosphatidylcholine present in erythrocyte, endoplasmic and sarcoplasmic reticulum membranes could be specifically ¹³C-labeled. The ¹³C line-widths of the resonance from the erythrocyte are typical for a lamellar arrangement of the membrane lipids. In strong contrast, the line-width observed at 37°C for the endoplasmic and sarcoplasmic reticulum membranes is much smaller, typical of the isotropic phases observed in model membranes. In isolated rat liver microsomes and liver slices, the ¹³C line-width is strongly temperature dependent. At lower temperatures the line-widths strongly increase towards values typical of lipids in a bilayer structure.