A simple model of a steady state differentiating cell system

A simple theoretical model is hypothesized to describe the steady state behavior of a differentiating cell system as exemplified by blood cells. The cell system consists of several morphologically distinguishable cell classes which develop sequentially. Each cell class except the last one is mitotically capable. Mitosis is assumed to be either heteromorphogenic, homomorphogenic, or asymmetric. Some algebraic equations are derived which are conservation equations describing the flux of cells from one class to another. The theoretical considerations have been applied to some experimental observations in humans concerning neutrophil production, particularly in reference to relative cell numbers and mitotic fractions of the myeloblast, promyelocyte, and myelocyte cell classes. These observations are utilized to help determine the values of the parameters which characterize the model. Among these parameters are the generation times of the various cell classes, and the predicted values of the generation times are found to be in excellent agreement with observed grain-count halving times. However, the predicted mitotic times are in disagreement with their observed values.     

Reactivation of stationary Tetrahymena : A contribution to the question of G0 state

Stationary cells of Tetrahymena were reactivated to exponential growth phase by transfer to fresh medium. The sequence of resuming cell cycle events was analysed by scoring the division index, the labelling index for macro- and micronuclei and the increase in cell number. By long-term labelling it was found that all cells replicate in stationary phase cultures. They also divide eventually. Upon transfer to fresh medium a small fraction of cells (about 3%) divide immediately, whereas the rest divide 3 h later after having replicated their macronuclear DNA. The kinetics of entry into the S phase indicates that these cells have a lag period of about 2 h before they resume progress through the cell cycle. It takes more than 1 h until all cells have begun replication. These data show that in stationary cultures all cells proceed through the events of the cell cycle. The cell cycle phases are extended differentially, G1 taking the largest part. During G2 cells pass very slowly through a certain stage close to division. Under the present conditions there is no indication for cells being in a resting state that is not part of the cell cycle, from which they can be restimulated and which has been called the G0 state. The criteria to demonstrate a resting state of this nature are discussed.     

Allo-Ia reactive murine T-cell lines. II. Mechanisms of clonal expansion of T cells explored by use of the allo-Ia reactive T cell clones

Murine T cell clones, which were retrieved from an A.TH anti-A.TL(lak) T cell line and had been long-term cultured in the medium supplemented with T cell growth factor (TCGF) and mitomycin C(MMC)-treated feeder cells of either Is or Ik haplotype, were found to survive in TCGF-free medium for a long time, quite in contrast to so far reported TCGF-dependent T cell clones. When T cells of these clones at the full growth in the TCGF-medium were transferred to TCGF-free medium, they survived at resting state for a long time, and half-life, i.e., the time when 50% of the transferred cells were still viable, of some clones reached 20 days. The cloned T cells at the resting state retained full responsiveness to the specific lak antigen but lost the responsiveness to TCGF as determined by [3H]thymidine uptake, whereas the same T cells harvested from TCGF-medium did not show the antigen-specific responsiveness. The cloned T cells at the resting state showed marked DNA synthesis in response to the specific antigen but never entered the phase of the cell division. Addition of TCGF to the antigen-activated cloned T cells at their peak DNA synthesis triggered the cell division without time lag. Thus, it was confirmed at a single clone level that two sequential signals, one via the antigen-receptor reacting with specific antigen and another via the TCGF-receptor accepting TCGF, are required for clonal expansion of T cells reacting with antigen. The mitogen-responsiveness among five clones was examined at their resting state; two clones responded to Con A and PHA only in the presence of accessory cells (MMC-treated, T cell-depleted syngeneic spleen cells), and one clone responded well to Con A and PHA in the absence of accessory cells. Thus, most of our clones retained physiologic characteristics of T cells directly collected from mice even after long-term culture in TCGF-medium.     

Effect of gamma radiation on resting B lymphocytes. I. Oxygen-dependent damage to the plasma membrane results in increased permeability and cell enlargement

Although the susceptibility of resting B lymphocytes to radiation-induced interphase death is well known, the mechanism by which this occurs is not understood. In this report, we use three measures of plasma membrane integrity (increase in cell volume, uptake of trypan blue, and release of 51Cr) to assess the effect of radiation on the resting B cell plasma membrane. The delivery of 500 to 1000 rad caused the majority of resting B cells to enlarge slightly, whereas 3000 rad caused virtually all of the cells to approximately double in size within 3 to 4 hr. Measurement of the release of 51Cr from resting B cells revealed a similar relationship between the dose of radiation and the loss of radioactive label. Trypan blue exclusion was also found to diminish as a function of radiation dose. An analysis of a variety of lymphoid cells suggested that sensitivity to the membrane damaging effects of gamma radiation was in the order of resting B cells greater than resting T cells greater than a long-term L3T4+ T cell clone greater than a B cell lymphoma. LPS-induced B cell blasts treated with 3000 rad were equivalent to 1000 rad-treated resting B cells. The effects of the gamma radiation could be ameliorated by excluding oxygen (a diradical molecule that can potentially enhance the generation and propagation of highly reactive free radicals) at the time of irradiation, or by adding the free radical scavenging agent cysteamine. These data are compatible with the hypothesis that gamma radiation results in damage to the plasma membrane of resting lymphocytes via the generation of highly reactive free radical species. This damage is reflected in a rapid increase in plasma membrane permeability and swelling of the cells, and may play a major role in causing interphase death.     

On the distribution of cell cycle generation times

The problem of whether the cell cycle is a deterministic or probabilistic process is widely discussed in the current literature (P. Nurse, Nature, 286, pp. 9–10, 1980). In this report the question of fluctuations of cell cycle period is treated in the limits of the membrane model of cell division regulation. The parametric analysis of the equations set both for normal and tumour cells is carried out. We describe the bifurcation parameters in the neighbourhood of which the system can amplify the small fluctuations. The presence of white noise in parameters describing the lipids and antioxidants influxes into membrane is examined by methods of Marcovian processes and also by direct stochastic computer simulation. The equation for the distribution function of generation times is obtained and the increase of dispersion and mean cycle time during the changes of those parameters which would be connected with cell culture density is calculated.The influence of parameter fluctuations upon the cycle period for both normal and tumour cells is compared in the framework of model assumptions. The ratio of dispersion of generation time distribution to mean period value for an ensemble of tumour cells is shown to be several times greater than that for normal ones.In the discussion the problem of the presence of a premitotical (G₀₂) resting state and of the possibility of its experimental detection is considered.     

Morphological phase-contrast cinematographic studies on the behavior of bone marrow cells in vitro. X. Myeloblasts and monoblasts]

The myeloblast is nearly of the same size as the lymphozyte and has the same nucleus cytoplasma ratio of 0.7 but differs from it in its morphology, its high frequency of multiplication, and by its kinetic behaviour. By phase contrast observation the transformation of the myeloblast into the promyelocyte has been seen several times. The myeloblast like the lymphocyte is able to move although at a much slower speed. By locomotion the myeloblast, and likewise the lymphocyte can move between blood and bone marrow. Of the granulocytopoietic series only the promyelocyte and the myelocyte with their nuclear cytoplasm relation of 0.3 are found in the bone marrow. The monoblast but is about twice its size, and moves less often. Apart from its transformation into promonocyte, monocyte and histiocyte, the monoblast may evalue in another way: it grows into a cell of doubled size with the same nucleus cytoplasm ratio 0.7 in whose cytoplasm are seen a lot of big granules. The cell may now be characterized as a tissue macrophage or mastcell. In consequence a frequently multiplying basophilic cell with a coarse nuclear structure and nucleoli, grows from a diameter of 6.5 to one of 13.0 mum without marked morphologic change apart from becoming alpha-NA-Esterase positive and acquiring big lysosomes. When this haemocytoblast is small (K 1/4 to K 1/2), it can be triggered into the granulocytopoietic series, when it is bigger (K 1/2 to K1) into the monocytopoietic series, or in the size K1 to K2 by erythropoietin into the erythropoietic series. If no triggering takes place, the cell degenerates after having granulated. The lymphopoietic system is not connected to this system of stem cells committed to the granulocytopoietic, the monocytopoietic and the erythropoietic series. Therefore we postulate a dual haematopoietic system. In acute leukemias the spread of size of cells and nuclei is wider and kinetically active stem cells are rarer. Only leukemic promyelocytes are in locomotion vividly, in contrast to the normal ones. In leukemic myeloblasts there are fewer mitoses than in normal ones, but in leukemic promyelocytes and monoblasts the mitotic frequency is not reduced.     

Deterministic model of steady-state cell proliferation

A new approach to the kinetics of cell proliferation, based on the postulated restriction of the number of cell divisions in an organism gives the possibility to determine the individual lifetimes of cells. In the model, a necessary condition for a steady-state population is that two sister cells have distinct lifetimes. A steady state was obtained as a consequence of constant rate of cell production in each generation, when sister cell divisions alternated. The mean value of the generation time of cells is in the direct proportion to the number of cells in each generation and connected (with a coefficient of 2) with the generation number. In consequence, we attach great importance to the identification of cells belonging to distinct generations. Corresponding mathematical method to determine the cell population parameters is given and conclusions about stem cells' organization have been drawn.     

Mathematical description and analysis of cell cycle kinetics and the application to Ehrlich ascites tumor

The linear and nonlinear aspects of the dynamics of the cell cycle kinetics of cell populations are studied. The dynamics are represented by difference equations. The characteristics of cell population systems are analyzed by applying the model to Ehrlich ascites tumor. The model applied for the simulations of the growth of Ehrlich ascites tumor cells incorporates processes of cell division, cell death, transition of cells to resting states and clearance of dead cells. Comparison of the results obtained with the model and the experimental data suggests that the duration of the mean generation time of the proliferating EAT cells increases with aging of the tumor. An attempt is made to relate the prolongation of cell mean generation time with processes of cell death and dead cell clearance. Studying the transition of cells to the resting states, it becomes apparent that in fact transition of proliferating cells to the resting states occurs somewhere close to the end of the cell cycle and with a rate that varies with the age of the tumor. Time course behavior of the cell age, cell size, and cell DNA distribution with aging of the tumor are obtained. Variations in average size and average DNA contents are determined.     

The messenger RNA sequences in growing and resting mouse fibroblasts.

The sequences present in messenger RNA in resting and growing 3T6 cells have been examined. First, the abundance and complexity classes of mRNA in growing 3T6 were compared to those in other established cell lines. The overall complexities measured for mRNA from HeLa cells and the three mouse fibroblast lines, 3T6, SV-PY-3T3, and L, are qualitatively similar and correspond to approximately 10,000 sequences. The relative amount of the two major abundance classes and their complexities appear identical in the three mouse fibroblast lines despite their different histories. HeLa cell mRNA is significantly different both in the amount and the complexity of the two major classes. The complexity of the two mRNA classes appears the same in resting and growing 3T6, although there is a small difference in relative amounts. Cross hybridizing cDNA and mRNA from resting and growing cells shows that the majority of mRNA sequences are the same in the two states. However, cross hybridization after the common sequences are removed shows that about 3% of the mRNA in resting cells is not present in the growing state, while the opposite cross shows 3% of the mRNA in growing cells is not present in resting cells. These differences may result from alterations in gene expression which are related to the growth state of the cell.     

The biological essence of resting cells in cell populations

Turnover of cell macromolecules and the diversity of turnover rates in cycling and resting cells is proposed as the underlying fundamental basis for a set of biological phenomena that involve growth, aging, and resistance of normal and tumor cell populations to damage by alkylating agents.It is postulated that in cycling cells the degradation rates are minimal or approaching zero, while in resting cells they are reaching the maximal possible values which are inherent characteristic features of each biological species. The biological advantage of the resting state lies in the ability of these cells to turn to maximal rates of degradation of cell macromolecules. During this process the level of accumulated cellular misinformation infthe form of altered misfunctioning macromolecules is substantially reduced and the cell becomes partially or completely rejuvenated. All cell populations are thought to contain a pool of rejuvenating resting cells, which have a certain probability of reverting to the cycling state.     

Chicken hematopoietic cells transformed by seven strains of defective avian leukemia viruses display three distinct phenotypes of differentiation.

Chicken hematopoietic cells transformed in vitro and in vivo by seven strains of replication-defective avian leukemia viruses were assayed for the expression of six erythroid and five myeloid differentiation parameters, including differentiation-specific surface antigens as detected by newly developed antisera. The transformed cells were found to display three distinct phenotypes of differentiation. First, cells transformed by AEV resemble erythroblasts. They express heme, globin, carbonic anhydrase and erythrocyte cell surface antigen at low levels, and histone H5 and erythroblast cell surface antigen at high levels. Second, cells transformed by MC29, CMII, OK10 and MH2 viruses have macrophage-like properties. They strongly express Fc receptors, phagocytic capacity and macrophage cell surface antigen, but only weakly express myeloblast cell surface antigen and are negative for ATPase activity. Third, cells transformed by AMV and E26 viruses resemble myeloblasts in that they weakly express Fc receptors, phagocytic capacity and macrophage cell surface antigen but strongly express myeloblast cell surface antigen and ATPase activity. No difference was found between in vitro- and in vivo-transformed cells in the parameters tested. In light of recent genetic and biochemical evidence, we believe that these phenotypes reflect the action of three new types of viral-transforming genes, designated erb (erythroblast), mac (macrophage) and myb (myeloblast).     

Genome-Wide Chromatin Remodeling Identified at GC-Rich Long Nucleosome-Free Regions

To gain deeper insights into principles of cell biology, it is essential to understand how cells reorganize their genomes by chromatin remodeling. We analyzed chromatin remodeling on next generation sequencing data from resting and activated T cells to determine a whole-genome chromatin remodeling landscape. We consider chromatin remodeling in terms of nucleosome repositioning which can be observed most robustly in long nucleosome-free regions (LNFRs) that are occupied by nucleosomes in another cell state. We found that LNFR sequences are either AT-rich or GC-rich, where nucleosome repositioning was observed much more prominently in GC-rich LNFRs — a considerable proportion of them outside promoter regions. Using support vector machines with string kernels, we identified a GC-rich DNA sequence pattern indicating loci of nucleosome repositioning in resting T cells. This pattern appears to be also typical for CpG islands. We found out that nucleosome repositioning in GC-rich LNFRs is indeed associated with CpG islands and with binding sites of the CpG-island-binding ZF-CXXC proteins KDM2A and CFP1. That this association occurs prominently inside and also prominently outside of promoter regions hints at a mechanism governing nucleosome repositioning that acts on a whole-genome scale.     

Electrophysiological characteristics of the unicellular green alga Micrasterias torreyi

The electrophysiological characteristics of the unicellular green alga Micrasterias torreyi Bail. are studied here for the first time using microelectrode techniques. The resting potential of the plasma membrane varied between –39.5 and –42.2 mV for different developmental stages of the dividing cell and was –41.7 mV ( se = 3.2, n = 9) in the interphase cells. The resting potential of the chloroplast envelope was lower, –53.9 mV ( se = 3.6, n = 15). Supraoptimal K⁺ (20 m M ) had no clear effects on the plasma membrane but caused a depolarization of 10 mV in the chloroplast. Additional external Ca²⁺ (10 m M ) depolarized the membrane potential quite strongly (by 23 mV). Low external pH did not affect the resting potential of the cell. There is a marked difference in the resting potential values between non-vacuolated cells (about –40 mV), to which Micrasterias belongs, and vacuolated plant cells (–100 to –250 mV). This indicates the participation of the tonoplast in the transport of ions and charged molecules in vacuolated cells. Na⁺ and Cl⁻, which play an important role in ion metabolism in most plant cells, are not needed by Micrasterias .     

The kinetic significance of cell size : II. Size distributions of resting and proliferating cells during interphase

This second part in a two part report describes the kinetic, cell size and nuclear size characteristics of S phase cells and cells with greatly protracted generation times (‘resting’ cells) in a cell line of human lymphoid cells. The median cell and nuclear sizes of S phase cells were greater than the corresponding median sizes observed in the whole population. Resting cells (operationally defined as unlabelled cells after 5 days of continuous labelling with [³H]TdR) have cell and nuclear size distributions overlapping with the cell and nuclear size distributions of the whole population. These resting cells are kinetically characterized by means of the observed labelling index vs time data during continuous labelling. The implication of these results are discussed.     

HIV Latency Is Established Directly and Early in Both Resting and Activated Primary CD4 T Cells

Highly active antiretroviral therapy (HAART) suppresses human immunodeficiency virus (HIV) replication to undetectable levels but cannot fully eradicate the virus because a small reservoir of CD4⁺ T cells remains latently infected. Since HIV efficiently infects only activated CD4⁺ T cells and since latent HIV primarily resides in resting CD4⁺ T cells, it is generally assumed that latency is established when a productively infected cell recycles to a resting state, trapping the virus in a latent state. In this study, we use a dual reporter virus—HIV Duo-Fluo I, which identifies latently infected cells immediately after infection—to investigate how T cell activation affects the estab-lishment of HIV latency. We show that HIV latency can arise from the direct infection of both resting and activated CD4⁺ T cells. Importantly, returning productively infected cells to a resting state is not associated with a significant silencing of the integrated HIV. We further show that resting CD4⁺ T cells from human lymphoid tissue (tonsil, spleen) show increased latency after infection when compared to peripheral blood. Our findings raise significant questions regarding the most commonly accepted model for the establishment of latent HIV and suggest that infection of both resting and activated primary CD4⁺ T cells produce latency.     

Growth factors and gangliosides: A possible new perspective in neuronal growth control

For many permanent cell lines the transition from a growing (P) to a resting (R) state is reversibly controlled by growth factors present in serum. This P-to-R transition was studied in a neuronal cell line (B 104) with respect to the action of serum, dibutyryl cyclic AMP (DBcAMP), gangliosides, and a glioma cell-produced growth factor GGF. In this cell system gangliosides seem to act as differentiation and survival factors. The kinetics of uptake of radioactively labeled gangliosides and survival experiments both support the idea of the stable incorporation of exogenously added gangliosides into the cells. Based on the experimental evidence a new model of cell development is proposed. Thus in addition to the R or G₀ state, which in this cell system is rather unstable and probably regulated by cyclic nucleotides, we postulate a differentiated D state, which is controlled by gangliosides and which is characterized by its stability (survival time). This D compartment seems to be closer to the in vivo differentiated neuron than does the R or P state. The possible mechanisms for the action of gangliosides are discussed.     

Dioscin (saponin)-induced generation of reactive oxygen species through mitochondria dysfunction: a proteomic-based study

It is generally believed that traditional Chinese medicine such as saponins has great value as potent cancer prevention and chemotherapeutic agents; however, the molecular basis for their activities is for the most part lacking. In the present study, we used proteomics to examine the cytotoxic effect of dioscin, a glucoside saponin, on human myeloblast leukemia HL-60 cells. Dioscin induced apoptosis in HL-60 cells in a time-dependent manner. Protein profiling of the microsomal fraction with enriched plasma membrane proteins isolated from HL-60 cells revealed that proteins act as chaperones and/or mediators of protein folding and were substantially altered in expression cells upon dioscin stimuli. Further biochemical study indicated that mitochondria dysfunction caused generation of reactive oxygen species (ROS), leading to the changes in protein expression. The mitochondrial transmembrane potential (DeltaPsi m) inhibitor aristolochic acid (ArA) partially abrogated the dioscin-initiated death receptor apoptosis pathway and cell death. The current study provided detailed evidence to support that dioscin is capable of inducing apoptosis in mammalian cells, in which the mitochondria-initiated apoptosis pathway plays an important role.     

Regulation of thymidylate synthase enzyme synthesis in 5-fluorodeoxyuridine-resistant mouse fibroblasts during the transition from the resting to growing state

Thymidylate synthase (TS) activity is very low in resting mouse 3T6 fibroblasts but increases sharply in growth-stimulated cells at about the same time the cells enter S phase. To study the mechanism responsible for the increase in TS level, we isolated a 5-fluorodeoxyuridine (5-FdUrd)-resistant cell line (LU3-7) that overproduces TS and its mRNA about 50-100-fold. In this paper we show that the LU3-7 cells were able to rest in the G0 state of the cell cycle when maintained in medium containing 0.5% serum. When the serum concentration was increased to 10%, the resting cells reentered the cell cycle and began DNA replication about 12 hr later. TS activity remained at the resting level until DNA replication began, then increased at later times. The increase was not affected when the cells were stimulated in the presence of DNA synthesis inhibitors. The rate of synthesis of TS (as determined in a pulse-labeling experiment) remained at the resting level for the first 10 hr following stimulation, then increased 8-9-fold by 25 hr following serum stimulation. The half-life of TS in growing LU3-7 cells was measured in a pulse-chase experiment and found to be greater than 24 hr. Therefore the increase in TS activity was primarily due to an increase in the rate of synthesis of the enzyme. Since TS gene expression appears to be regulated in a similar manner in LU3-7 cells and in the parental 3T6 cells, the LU3-7 cells should be a good model system for detailed analysis of the mechanism for regulating TS gene expression in mammalian cells.     

Analysis of Escherichia coli cell state by flow cytometry during whole cell catalyzed biotransformation for l-carnitine production

Flow cytometry was used to monitor Escherichia coli cellular state during the biotransformation of crotonobetaine into l-carnitine using growing and resting cells in batch and high-cell-recycle continuous membrane reactors. The cell physiological state and the DNA, RNA and protein cell content were analyzed during the bioprocess. The cell growth cycle was followed by reference to cellular DNA concentration and the entry in the stationary phase resulted in an increase in intracellular protein. The biochemical activity of resting cells was assessed for the first time at the molecular level, protein synthesis being observed despite the absence of nutrients. Freely suspended growing, both in batch and continuous cultures, and, more importantly, resting E. coli cells were seen to be made up of subpopulations differing in reproductive ability, metabolic activity and membrane integrity. In the case of growing cells, biotransformation was mostly performed by fully viable cells (68–75%), while in a resting cell system, also dead cells (1–5%) and cells with doubtful viability (60–70%) appeared to be involved in the process; in later stages, a population made up of phantom cells, containing little or no cellular DNA, was detected. In cell-recycle continuous reactors, the recording of DNA (40 to 60 fg), RNA (50 to 120 fg) and protein (100 to 220 fg) levels per unit of cell, and the evolution of cell population heterogeneity (three different populations of cells) threw light on the stress conditions imposed by high cell densities. The use of FCM allowed to follow the recovery of cell catalytic activity for resting biotransformation batch processes, thus showing its potential for the optimization of bioprocesses.