Synchronization and signal transmission in protoplasmic strands of Physarum

The importance of endoplasmic streaming in the synchronization of contraction activites in plasmodial strands of Physarum was investigated under experimental conditions allowing simultaneous observation of the endoplasmic flow in the middle part of a strand mounted as a trapeze and the measurement of isometric contraction activities of the arms of the trapeze, as well as of the activities of the strand portion connecting the arms. The correlation of longitudinal and radial contraction activities in different regions of a trapeze was examined. Whereas the arms and the middle part of a trapeze contract synchronously in a longitudinal direction (in-phase behaviour), an antiphase correlation appeared when comparing the longitudinal contraction activity of the arms and the radial activity of the middle part. This result is interpreted to mean that the middle part is able to perform isotonic contractions which induce radial dilatation of the strands. No clear-cut correlation between longitudinal and radial activities could be found when measuring simultaneously both activities in one and the same arm of a trapeze by combining tensiometry and cinematography. Protoplasmic shuttle streaming within a strand mounted as a trapeze is found to run regularly out of one arm through the middle part into the other arm, and vice versa. There is no correlation between the time points of streaming reversal and a certain stage of contraction cycles as presented by the contraction curves of the arms. However, there is a good correlation between the points of streaming reversal and the phase deviations of the longitudinal contraction activities of the arms. The importance of these phase deviations for the control of streaming reversal, i.e., for the generation of hydrostatic pressure differences in a system working with phase synchrony, is discussed. The role of endoplasmic streaming as a pacemaker for synchronization phenomena of contraction activities is stressed. The possibility is discussed that shuttle streaming of endoplasm acts as a mechanical coupling within the regulation phenomena resulting in spatial monorhythmicity.Partly presented at the Cell Motility workshop, 8^th European Muscle Conference, Heidelberg 17.–20. September 1979     

THE CHANGING PATTERN OF BIREFRINGENCE IN PLASMODIA OF THE SLIME MOLD, PHYSARUM POLYCEPHALUM

Plasmodia of the acellular slime mold, Physarum polycephalum, reveal a complex and changing pattern of birefringence when examined with a sensitive polarizing microscope. Positively birefringent fibrils are found throughout the ectoplasmic region of the plasmodium. In the larger strands they may be oriented parallel to the strand axis, or arranged circularly or spirally along the periphery of endoplasmic channels. Some fibrils exist for only a few minutes, others for a longer period. Some, particularly the circular fibrils, undergo changes in birefringence as they undergo cyclic deformations. In the ramifying strand region and the advancing margin there is a tendency for fibrils of various sizes to become organized into mutually orthogonal arrays. In some plasmodia the channel wall material immediately adjacent to the endoplasm has been found to be birefringent. The sign of endoplasmic birefringence is negative, and its magnitude is apparently constant over the streaming cycle. The pattern of plasmodial birefringence and its changes during the shuttle streaming cycle of Physarum are considered in the light of several models designed to explain either cytoplasmic streaming alone or the entire gamut of plasmodial motions. The results of this and other recent physical studies suggest that both streaming and the various other motions of the plasmodium may very likely be explained in terms of coordinated contractions taking place in the fibrils which are rendered visible in polarized light.     

Bidirectional flow of endoplasm inPhysarum plasmodium under centrifugal acceleration

Summary The behavior of cytoplasmic streaming in plasmodial strand ofPhysarum polycephalum was studied under centrifugal acceleration using a centrifuge microscope of the stroboscopic type. Cytoplasmic streaming in the plasmodium was greatly affected by changes in the acceleration. The endoplasmic flow in the centrifugal direction was accelerated, while that in the centripetal was retarded, by centrifugal acceleration. The centrifugal acceleration required to stop the endoplasmic flow in the centripetal direction did not cause total cessation of streaming but always induced a bidirectional flow of endoplasm in one and the same strand. Each profile of velocity distribution of the bidirectional flow was both parabola with flattened apex. One possible cause of the bidirectional flow is discussed.Dedicated to Emeritus Professor Noburo Kamiya on the occasion of his 80th birthday     

Dynamics of the ectoplasmic walls during pulsation of plasmodial veins ofPhysarum polycephalum

Summary The thickness of ectoplasmic walls decreases at the contraction phase and increases at the expansion phase of each pulsation cycle. In average, 29% of material forming the walls of expanded veins is evacuated during contraction with the endoplasm streaming.     

Motory effects of perforating peripheral cell layers ofAmoeba proteus

Summary Perforation of peripheral cell layers ofA. proteus in any place provokes immediate endoplasm efflux, what supports the view that the hydrostatic pressure is higher in the cell interior than outside. The local effusion of endoplasm results in the reversal of flow in formerly advancing pseudopodia, in agreement with the pressure gradient theories of protoplasmic streaming. Amoebae with destroyed frontal zones squeeze all their endoplasm out through the breach, what disproves the frontal contraction hypothesis of amoeboid movement, but supports the concept of a general contraction of cell cortex.Study supported by the Research Project II.1 of the Polish Academy of Science.     

A continuum model of contraction waves and protoplasm streaming in strands of Physarum plasmodium

We present a mathematical model for continuously distributed mechanochemical autooscillations (autowaves) in a protoplasmic strand of Physarum polycephalum. The model is based on a hypothesis of local positive feedback between deformation and contraction of the contractile apparatus. This feedback is mediated through a cell regulatory system whose kinetics involves coupling to mechanical strain. Mathematical analysis and computer simulations have demonstrated that the solutions of the model agree quantitatively with the available experimental data. In particular, hydrodynamic interaction alone, between different sections of the strand via the streaming endoplasm, is capable of inducing the characteristic contractile behavior.     

Cytoplasmic streaming in internodal cells ofNitella under centrifugal acceleration: a study done with a newly constructed centrifuge microscope

Summary We constructed a new centrifuge microscope of the stroboscopic type, with which the cytoplasmic streaming inNitella internodal cells under centrifugal acceleration was studied. Under moderate centrifugal acceleration (ca. 50–100×g), the direction of cytoplasmic streaming in an internodal cell ofNitella is parallel to the direction of the subcortical fibrils. The speed of endoplasm flowing contiguous to the subcortical fibrils is neither accelerated nor retarded by moderate centrifugal acceleration. The endoplasmic flow, however, stops suddenly following an electrical stimulus. The endoplasm contiguous to the subcortical fibrils is immobilized transiently at the time of streaming cessation induced by an electrical stimulus under centrifugal acceleration at 50–100×g, even at 900×g. It is suggested that transitory cross bridges between the immobilized endoplasm and the subcortical fibrils are formed at the time of streaming cessation. The bulk endoplasm flows as a whole in the direction parallel to that of the subcortical fibrils and stops promptly upon electrical stimulation. Soon after the stoppage the bulk endoplasm starts to flow passively in the direction parallel to that of the centrifugal acceleration as a result of the centrifugal force.Abbreviations APW artificial pond water - CMS centrifuge microscope     

Structural basis of cytoplasmic streaming in Characean internodal cells. A hydrodynamic analysis

Summary Hydrodynamic equations were derived which relate the velocity profile of endoplasmic streaming with the motive force generated by active sliding of endoplasmic organelles in Characean internodal cells, under two implicit assumptions that (1) the sliding velocity of putative organelles is comparable to the streaming velocity of endoplasm, and (2) subcortical endoplasm is far less viscous than bulk endoplasm.The equations were extended so as to calculate the velocity profile in flattened or perfused internodal cells. Calculated profiles were basically consistent with reported patterns of streaming under these conditions.Utilizing published data, we deduce some hydrodynamic parameters of streaming, and predict the dimensions of putative organelles expected to drive entire cytoplasm. A revision for published values of the motive force of streaming is proposed.Hydrodynamic analyses made earlier on the spherical organelles are repeated. The results show that the organelles may generate streaming, depending on the configurationin vivo of fine filaments protruding from the body of the organelles.     

The contractile basis of amoeboid movement : IV. The viscoelasticity and contractility of amoeba cytoplasm in vivo

The viscoelasticity and contractility of amoeba cytoplasm has been studied in vivo and in vitro. A gradient of increasing viscoelasticity and contractility was identified in the endoplasm of intact cells from the uroid (tail) to the fountain zone (tip of advancing pseudopod). Anterior endoplasm, as well as all of the ectoplasm, contracted in response to the microinjection of a threshold calcium ion concentration (ca 7.0 × 10⁻⁷ M). In contrast, there were only delayed weak contractions in the uroid endoplasm upon the microinjection of a threshold calcium ion concentration. Contractions induced in the ectoplasm by microinjecting the contraction solution readily caused the endoplasm to stream. However, the endoplasm at the tips of the extending pseudopods were also contractile and transmitted applied tensions. Furthermore, the microinjection of subthreshold calcium ion concentrations caused the loss of distinct endoplasmic structure and the cessation of streaming in both the uroid and the anterior third of the cell. In addition, the relationship between contractility and cytoplasmic streaming was characterized in “relaxed” cytoplasm placed in a gradient of calcium ion concentration inside quartz capillaries. The results of these experiments demonstrated that the mechanochemical conversion of endoplasm to ectoplasm caused the cytoplasm to become more structured and contractile. Therefore, physiological contractions are possible during and after the conversion of endoplasm to ectoplasm.     

Differential treatment ofAcetabularia with cytochalasin B and N-Ethylmaleimide with special reference to their effects on cytoplasmic streaming

Summary Cytoplasmic streaming in the stalk ofAcetabularia, ryukyuensis at the vegetative stage was reversibly inhibited by cytochalasin B (cB) of 50 g/ml and irreversibly by N-Ethylmaleimide (NEM) above concentrations of 0.25 mM.After the endoplasm and the chloroplasts were pushed forward one end of the stalk by gentle centrifugation at about 500 × g for 3 minutes, numerous ectoplasmic striations remainedin situ in the stalk cortex. The striations ran in parallel with the longitudinal axis of the stalk at unequal intervals. The endoplasm streamed back only along these striations.By combining centrifugation and a double chamber technique, the endoplasm and the cortex of the stalk were treated separately with CB or NEM. CB treatment of the cortex arrested streaming; when treatment was restricted to the endoplasm, streaming continued at an normal rate. NEM treatment restricted to the cortex permitted normal streaming rates. Treatment restricted to the moving endoplasm inhibited streaming.These results suggest that microfilaments and a moiety, possibly myosin, play an active role in the streaming. Microfilaments must reside in the cortex, especially in the ectoplasmic striations, while the putative myosin must reside in the moving endoplasm.     

Velocity distributions of the streaming protoplasm in Nitella flexilis.

Laser light is Doppler-shifted in frequency by the streaming endoplasm of living cells of Nitella flexilis. The frequency spectrum of the scattered light can be interpreted as the histogram of velocities within the organism, with the exception of the intense low-frequency portion of the spectrum. We demonstrate that the lowest-frequency component is the result of amplitude modulation of the scattered light by the array of chloroplasts in the cell. Measurement of the streaming endoplasm in a photobleached "window" region allows correction of the frequency distribution for the modulation component. The complete velocity histogram for the streaming endoplasm is calculated directly from the corrected frequency distribution. Measurements of vacuolar and endoplasmic motions show that the tonoplast, the membrane separating the vacuole and the endoplasm, seems to be flowing along with the endoplasm and vacuolar sap. Placing the cell in medium containing ATP in concentrations greater than 10(-3) M greatly increases the contribution of low velocities to the velocity histogram. Cytochalasin B at high dosages (10-50 mug/ml) does not noticably change the shape of the velocity histogram, while at low dosages (1 mug/ml) there is an increase in the contribution of low velocities to the velocity histogram. Colchicine in high concentrations (1%) has no observable effect on the velocity histogram.     

Progress in plasmodial differentiation improves regularity of oscillating contractions in Physarum polycephalum

Based on the knowledge about subcellular morphogenetic processes in the acellular slime mold Physarum polycephalum, we hypothesized that during differentiation of undifferentiated endoplasm to the highly differentiated complex structure of the contractile apparatus of this organism, the regularity of oscillating contractions must improve. We measured the endogenous contraction automaticity starting from the de novo generation within minutes after sampling small portions of undifferentiated endoplasm. The standard deviation of the normalized period duration of these samples was compared to the respective values of radial contractions of differentiated protoplasmic plasmodial strands. The mean normalized standard deviation in endoplasmic drops was 28.3+/-12.2%. Respective values in protoplasmic strands were 10.0+/-3.7%. The difference between the experimental groups was highly significant (p<0.0001). We interpret the verification of our hypothesis as an indication that the very regular oscillating contractions in fully differentiated stages of Physarum require the complex structure of the sophisticated contractile apparatus, represented by the circular plasmalemma invagination system of protoplasmic strands, while the regularity is lower in stages, where the differentiation is still in progress. We believe that this is due to deficits in coordination capabilities, which need a directional and spatially oriented protoplasmic streaming as a precondition.     

Participation of Ca2+ in cessation of cytoplasmic streaming induced by membrane excitation inCharaceae internodal cells

Summary The mechanism of the cessation of cytoplasmic streaming upon membrane excitation inCharaceae internodal cells was investigated.Cell fragments containing only cytoplasm were prepared by collecting the endoplasm at one cell end by centrifugation. In such cell fragments lacking the tonoplast, an action potential induced streaming cessation, indicating that an action potential at the plasmalemma alone is enough to stop the streaming.The active rotation of chloroplasts passively flowing together with the endoplasm also stopped simultaneously with the streaming cessation upon excitation. The time lag or interval between the rotation cessation and the electrical stimulation for inducing the action potential increased with the distance of the chloroplasts from the cortex. The time lag was about 1 second/15 m, suggesting that an agent causing the rotation cessation is diffused throughout the endoplasm.Using internodes whose tonoplast was removed by replacing the cell sap with EGTA-containing solution (tonoplast-free cells,Tazawa et al. 1976), we investigated the streaming rate with respect to the internal Ca²⁺ concentration. The rate was roughly identical to that of normal cells at a Ca²⁺ concentration of less than 10^–7 M. It decreased with an increase in the internal Ca²⁺ concentration and was zero at 1 mM Ca²⁺.The above results, together with the two facts that Ca²⁺ reversibly inhibits chloroplast rotation (Hayama andTazawa, unpublished) and the streaming in tonoplast-free cells does not stop upon excitation (Tazawa et al. 1976), lead us to conclude that a transient increase in the Ca²⁺ concentration in the cytoplasm directly stops the cytoplasmic streaming. Both Ca influxes across the resting and active membranes were roughly proportional to the external Ca²⁺ concentration, which did not affect the rate of streaming recovery. Based on these results, several possibilities for the increase in Ca²⁺ concentration in the cytoplasm causing streaming cessation were discussed.     

Myosin and Ca2+-sensitive streaming in the alga Chara: detection of two polypeptides reacting with a monoclonal anti-myosin and their localization in the streaming endoplasm

A monoclonal antibody to the heavy chain of myosin from mouse 3T3 cells was used to detect and localize related proteins in the green alga Chara. Proteins of 200,000 and 110,000 Mr reacted on immunoblots of proteins precipitated rapidly with trichloroacetic acid to minimize proteolysis. Immunofluorescence of whole cells localized these proteins to organelles of the streaming endoplasm, to a system of endoplasmic strands and to the subcortical actin bundles. Except that fewer endoplasmic strands and organelles were found and the strands were tangled, the localization pattern was similar in cells rapidly perfused to remove the bulk of the streaming endoplasm. Actin was confined almost entirely to the system of subcortical actin bundles in both whole and perfused cells. Myosin that was associated with the tangled endoplasmic strands but not that associated with the organelles or actin bundles was removed by concentrations of Ca2+ inhibiting ATP-dependent streaming in perfused cells. ATP extracted both organelles and endoplasmic strands but left a continuous pattern of myosin immunostaining along the actin bundles. The findings are discussed in relation to the possible existence of two forms of myosin and of separate mechanisms moving the bulk endoplasm and individual organelles.     

Cytoplasmic streaming in giant algal cells: A historical survey of experimental approaches

Various methods have been used to study cytoplasmic streaming in giant algal cells during the past three decades. Simple techniques can be used with characean internodal cells to modify the cell constitution in various ways to gain insight into the mechanism of cytoplasmic streaming. Another method involves isolatingin vitro a huge drop of uninjured endoplasm, to examine its physical and dynamic properties. The motive force responsible for streaming has been measured by three different techniques with similar results. Subcortical fibrils consisting of bundles of F-actin with the same polarity are indispensable for streaming. Differential treatment of the endoplasm and ectoplasm has shown that putative characean myosin is localized in the endoplasm. Studies of the roles of ATP, Mg²⁺, Ca²⁺, H⁺ etc. in the streaming have been conducted by cellular perfusion, which allows removal of the tonoplast, or by techniques permeabilizing the protoplasmic membrane. A slow version of the movement can even be artificially reproduced by combining characean actinin situ and exogenous myosin in the presence of Mg-ATP. The findings thus far obtained support the hypothesis that cytoplasmic streaming in characean cells is caused by an active shearing force produced by interaction of the actin filament bundles on the cortex with myosin in the endoplasm.     

Change of contractile behavior in plasmodia ofPhysarum polycephalum during mitosis

Summary Oscillations of ectoplasmic contraction in plasmodia of the myxomycetePhysarum polycephalum growing on agar containing semidefined medium were studied to determine if the contractile force is altered during the synchronous mitosis. In interphase the regular oscillations of contraction in the plasmodial sheet had an average period of 0.93 minutes in plasmodia growing at 24 °C. During mitosis the amplitude of these oscillations gradually decreased, ceasing for an average time of 2.7 minutes in 74% of the 23 plasmodia studied. Cessation of oscillating contractions in mitosis was accompanied by a decrease in the width of the channels embedded in the plasmodial sheet, and a decrease in the velocity of endoplasmic shuttle streaming usually to a complete standstill. Of 13 plasmodia in which the mitotic stage was very accurately determined, the stop in oscillating contractions occurred during metaphase in 10 plasmodia, and in prometaphase, anaphase, telophase in the 3 others. The cessation of contractile oscillations or of streaming did not occur absolutely simultaneously during mitosis in widely separated locations within one plasmodium, indicating mitotic asynchrony over a period of a few minutes within each plasmodium. We suggest that the halt of plasmodial migration during mitosis reported by others is caused by a decrease or cessation at slightly different times in the amplitude of ectoplasmic contractile oscillations in different areas of a plasmodium in mitosis resulting in an overall lack of coordination of endoplasmic flow throughout the plasmodium, thus temporarily halting migration. Possible physiological mechanisms linking a decrease in actomyosin contraction with the metaphase stage of mitosis are discussed.     

A study of protoplasmic streaming inPhysarum by laser Doppler spectroscopy

Summary Protoplasmic streaming in the slime moldPhysarum polycephalum has been characterized using laser Doppler spectroscopy. Measurement of the spectrum of scattered laser light permits simultaneous determination of the velocities of all particles in the laser beam, with the relative intensity from each particle proportional to its light scattering cross-section. Simple experimental modifications allow the tracking of the oscillations of the streaming velocities. Rhythmic wall contractions can be monitored simultaneously with the flow velocities. Interpretation of the Doppler spectra shows that a small fraction of the particles in the flowing protoplasm are moving with velocities two to four times greater than the characteristic velocities reported by optical microscopy. Transverse velocities in the tubes are nearly as great as the longitudinal velocities. The shape of the Doppler spectrum at the maximum of the oscillation cycle is consistent with a spatial velocity profile which is sharper than parabolic, presumably because of a viscosity gradient from the center to the walls of the plasmodial tubes. The shape of the Doppler spectrum of depolarized scattered light is of approximately the same form. The response of the plasmodium to increased temperature is an increase in the frequency of the velocity oscillations with little change in the magnitude of the velocities. The response of the plasmodium to very high intensities of laser light is to gel at the point of incidence.     

Laser light-scattering analysis of protoplasmic streaming in the slime mold Physarum polycephalum

Laser light scattering is shown to be an effective means of obtaining a rapid, objective assessment of dynamic changes in the intact plasmodium of the myxomycete Physarum polycephalum during bidirectional (shuttle) streaming. The motion of material in a 100 mum diameter region of a plasmodial vein was studied by following changes in the autocorrelation function of the fluctuations in the scattered light intensity. The autocorrelation function was recorded at 10 s intervals and analyzed to follow changes in the flow velocity of protoplasm associated with shuttle streaming. Rhythmic velocity changes and a "beating" pattern of velocity maxima were readily observed. In an attempt to locate the site of underlying structural changes in the vein responsible for the changing pattern of flow, the average scattered intensity was separated into components derived from moving and stationary scatterers. Periodic variations in the light intensity due to stationary scatterers are related to the streaming cycle and indicate the occurrence of important structural changes in the vein walls. Two possible interpretations of the data are offered; one involving gross dynamic changes in vein structure, the other involving the formation, contraction, or breakdown of fibrillar material in the vein wall during the streaming cycle.