PHOTOTACTIC ORIENTATION BY THE CILIATE, STENTOR COERULEUS

Stentor coeruleus exhibits negative phototaxis to visible light, in addition to a step-up photophobic response. The negative phototaxis was established by demonstrating the swimming of Stentor toward a focused beam away from the light source. The action spectrum showed a maximum at 610–620 nm and is essentially identical to that of the step-up photophobic response. Proton uncouplers such as micromolar concentrations of FCCP and TPMP⁺ inhibited the negative phototaxis.     

Stentor coeruleus SHOWS POSITIVE PHOTOKINESIS

Abstract— Stentor coeruleus responds to a sudden increase in light intensity with a step-up photophobic response (avoiding reaction), and to collimated light with negative phototaxis. The peaks of the action spectra for the photophobic response and for the phototaxis are in common, 610 nm.
5. coeruleus showed changes in its steady-state swimming velocity induced with varying intensities of light (photokinesis). The cells swam fast in light regions but slowly in dark ones (positive photokinesis); the mean velocity of swimming was about 0.6 mm/s at 100 lx but reached about 1.0 mm/s at 50000 lx. The peak of the action spectrum for this photokinesis was about 680 nm.
The organism is the first protozoan cell reported to show three types of photoresponse: photophobic response, phototaxis and photokinesis.     

BEHAVIORAL RESPONSES IN Paramecium multimicronucleatum TO VISIBLE LIGHT

Specimens of colorless Paramecium multimicronucleatum were found to respond to visible light. They accumulated in the shaded region (photodispersal) of a half-shaded glass tube during 2 min exposure to visible light. The specimens showed avoiding reaction upon both spatial and temporal increase in light intensity (step-up photophobic response). Steady-state swimming velocity (orthokinesis) was higher, while steady-state frequency of spontaneous change in swimming direction (klinokinesis) was lower when the light intensity was kept higher. In a light with wavelength of 440 nm the velocity was highest, while the frequency was lowest. The specimens did not show phototaxis (light direction-oriented locomotion). Spectral sensitivity curves for both the photodispersal and the step-up photophobic response showed a major peak at 520 nm and a minor peak at 680 nm. The photodispersal seems to be caused mainly by the step-up photophobic response exhibited by the specimens at the dark-light border. The photokinetic responses enhance the degree of the photodispersal.     

PHOTORECEPTOR PIGMENT IN Blepharisma: H+ RELEASE FROM RED PIGMENT

In faded cells of Blepharisma kept in a standard saline solution containing bacteria which had been cultured on agar plates containing glucose and polypepton, threshold light intensity for step-up photophobic response elevated. This result suggests that red pigment (blepharismin) contained in Blepharisma cells is involved in the step-up photophobic response. The pH of the aqueous solution of the red pigment was found to decrease when light was applied, indicating that the pigment releases H⁺ in response to light stimulation. However, faded pigment preparation by light irradiation did not show pH decrease. In the living cells faded by light irradiation, threshold light intensity for the step-up photophobic response was raised. Results suggest that H⁺ release from the red pigment induced by light irradiation might be responsible for the step-up photophobic response of the cells.     

Mechanism and computer simulation of the phototactic accumulation of Euglena in a beam of light

Abstract— A mechanistic model is proposed which describes the phototactic behavior of Euglena during accumulation in an illuminated region. Measurements of the lag time occurring between illumination of the culture and net accumulation in the lighted zone as a function of culture density indicate that the relative strengths of the negative phototactic response inside and of the positive phototactic response outside this region are the prime factors controlling the lag phenomenon. Further evidence for this is provided by studies of the temperature dependence of the phototactic responses to polarized actinic light. It is shown that negative phototaxis as measured in the 7lsquo;phototaxigraph’ is not directed, but rather a shock-mediated response. A ‘FOCAL’ computer program for simulation of experiments in the phototaxigraph has been written on the basis of our model. It correctly predicts the observed results under a variety of simulated experimental conditions. Measurements of the lag time and of the rate of accumulation in different parts of the actinic zone allow the calculation of motilities of the organisms with illumination and in the dark, the latter value being 0.08 mm/sec. For a 2–3-weekold culture, the rate of negative phototaxis remained constant at light intensities above 40 ergs/cm²sec at 500 nm. At this wavelength, the threshold for the positive photophobic response was 100 ergs/cm² sec.     

LIGHT REACTIONS OF THE CILIATE Stentor coeruleus-A THREE-DIMENSIONAL ANALYSIS

A computer-controlled three-dimensional tracking and motion analysis system was developed to study the responses of Stentor coeruleus to short light pulses and to evaluate its distribution patterns. In addition to photokinesis and phototaxis, the step-up photophobic response was analyzed, which includes a gravity-controlled component at higher fluence rates and a light direction-dependent component at lower fluence rates.     

PHOTOBEHAVIOR OF EUGLENA GRACILIS: ACTION SPECTRUM FOR THE STEP-DOWN PHOTOPHOBIC RESPONSE OF INDIVIDUAL CELLS

Abstract—Light-induced behavioral responses of Euglena gracilis have been investigated in single cells by means of a video system coupled to an optical microscope. Light intensity-effect curves at different wavelengths in the near UV and visible range have been determined. From these curves the action spectrum for the step-down photophobic response of Euglena has been calculated. From a comparison with the results obtained using a population method by means of a phototaxigraph, it is concluded that a single photomotile reaction is responsible for cell accumulation, brought about by trapping in the light spot and possibly by phototaxis towards scattered light from organisms already in the light field.     

Effect of preillumination on photomotile responses of the marine ciliate Fabrea salina

Fabrea salina is a marine ciliate that shows photomotile responses such as positive phototaxis and a step-down photophobic reaction. We found that preilluminated F. salina cells show a phototactic response significantly greater than that of dark-adapted cells when exposed to the same phototactic light stimulus. In particular, positive phototaxis is strongly enhanced by preillumination. This enhancement effect depends on the preillumination light irradiance, on the total preillumination dose, and on the duration of the dark interval between preillumination and the phototaxis measurement. Our results show that the determining factor is the total preillumination dose given to the sample. The enhancement effect shows an asymptotic behavior over a certain range of energy values (10-200 W/m2). Further, the effect is transient; after 120 s in the dark, the cells lose any memory of the preillumination, independent of the preillumination energy received. These results are tentatively discussed in terms of light-driven membrane potential or membrane channel conductances.     

DOUBLET Stentor DO NOT DISPLAY PHOTODISPERSAL

Normal Stentor, called singlets since they have a single membranellar band and oral groove surrounding their frontal field, swim away from light sources and collect in the darker areas of an unevenly illuminated container (photodispersal). Phenotypic variants, called doublets since they have 2 membranellar bands and 2 oral grooves, do not exhibit this behavior. Doublets produce photophobic responses and contractions when illuminated at the same fluence rates which produce those responses in singlets, hence their sensitivity to light is normal. Illumination of the frontal field of doublets produces a photophobic response at lower fluence rates than does illumination of their side or posterior. This directional sensitivity is quantitatively similar to that observed in singlets. However, doublets do not reorient their swimming direction after a phobic response as extensively as do singlets. This failure in reorientation is the probable reason that doublets fail to show photodispersal. These results imply that the mechanism producing photodispersal in singlets depends on photophobic responses or some other, presently undescribed, response which requires an asymmetric frontal field.     

Photosensory Functions of Channelrhodopsins in Native Algal Cells†

Photomotility responses in flagellate alga are mediated by two types of sensory rhodopsins (A and B). Upon photoexcitation they trigger a cascade of transmembrane currents which provide sensory transduction of light stimuli. Both types of algal sensory rhodopsins demonstrate light‐gated ion channel activities when heterologously expressed in animal cells, and therefore they have been given the alternative names channelrhodopsin 1 and 2. In recent publications their channel activity has been assumed to initiate the transduction chain in the native algal cells. Here we present data showing that: (1) the modes of action of both types of sensory rhodopsins are different in native cells such as Chlamydomonas reinhardtii than in heterologous expression systems, and also differ between the two types of rhodopsins; (2) the primary function of Type B sensory rhodopsin (channelrhodopsin‐2) is biochemical activation of secondary Ca²⁺‐channels with evidence for amplification and a diffusible messenger, sufficient for mediating phototaxis and photophobic responses; (3) Type A sensory rhodopsin (channelrhodopsin‐1) mediates avoidance responses by direct channel activity under high light intensities and exhibits low‐efficiency amplification. These dual functions of algal sensory rhodopsins enable the highly sophisticated photobehavior of algal cells.     

光驱动一维活性凝胶自发定向运动

许多生物都具备一种自发响应环境刺激进行自动运动的本能。光照是一种强有力的外部刺激,且对生物系统具有正负驱动的双重效应;本实验设计了一个一维活性BZ凝胶体系,利用钌催化BZ反应的光敏性,控制凝胶振荡频率,驱动凝胶进行定向自发运动。同时,我们修正了V. V. Yashin 提出的BZ响应胶模型活性凝胶光强频率曲线进行模拟,揭示光驱动活性凝胶运动的本质。这有助于研发新型仿生智能机器人来对生物系统响应外部刺激的自发运动进行研究。     

CAFFEINE-ENHANCED PHOTOMOVEMENT IN THE CILIATE, STENTOR COERULEUS

The effects of caffeine, ionophores and calcium flux blockers on the step-up photophobic response, phototactic orientation and the intracellularly recorded, light-induced electrical action potential were studied in the ciliate, Stentor coeruleus . Caffeine alters the absorption and CD spectra and enhances the fluorescence of the photoreceptor pigment, stentorin. Independent of its effects on the spectroscopic properties of the photoreceptor pigment, caffeine shortens the photophobic response time by enhancing the Ca²⁺ conductivity of membranes, while Ca²⁺ flux blockers (LaCI₃ or ruthenium red) prolong it; both effects cancel each other. Evidence is presented that phototactic orientation is brought about by repetitive photophobic responses, since a change in the phobic response time results in a decreased accuracy of phototaxis.     

PHOTOSENSORY TRANSDUCTION IN CILIATES. III. THE TEMPORAL RELATION BETWEEN MEMBRANE POTENTIALS AND PHOTOMOTILE RESPONSES IN Blepharisma japonic urn

Abstract— Blepharisma japonicum exhibits a step-up photophobic response when subjected to an increase in light stimulus intensity. This response is characterized by the stop reaction after a period of delay followed by backward swimming (lateral rotation). The latency of the stop response decreased and duration of the lateral rotation increased as the intensity of light stimuli was raised. A step-increase in light intensity elicited a graded membrane depolarization (photic receptor potential), as measured by intracellular microelectrode. When the amplitude of receptor potential exceeded a threshold depolarization for membrane excitation (15–25 mV), an all-or-none action potential of 50–65 mV in amplitude was evoked which also occurred with some latency. Light stimuli of higher intensity (suprathreshold) elicited action potential which was followed by a membrane after-depolarization. Increasing the intensity of stimuli caused generation of an action potential with shorter lag period and prolonged after-depolarization. The action spectra for the latency of stop reaction, receptor potential amplitude and cell photoresponsiveness showed maxima at 460, 530 and 580 nm. The analysis of temporal relationships between the electrophysiological responses and the motile events showed that latency of an action potential, induced by the receptor potential, correlates well with the latency of a cell stop response. Also the duration of membrane after-depolarization resembled the time period of the cell's backward swimming (cell rotation). The data obtained indicate that the primary reaction initiated by light absorption in the photoreceptor pigment (blepharismin) is converted into the observed electrical potential changes, which in turn results in the photomotile response of Blepharisma cells.     

Photodegradation of polyacetaldehyde in solution. I. Direct photolysis

The quantum yields measured for the random scission of main-chain bonds of polyacetaldehyde in benzene solution by 254 nm irradiation at 298°K are on the order of 10^?3–10^?4 scissions per quantum absorbed by the polymer. The quantum yields are unaffected by oxygen but are dependent upon initial polymer concentration and upon the inverse square root of absorbed light intensity. The direct photochemistry involves excitation of carbonyl chromophores in their ¹nπ^* bands, and a Norrish type I process is believed to be responsible for subsequent free-radical random-chain scissions. It has been established that direct photoexcitation processes do not lead to sequential depolymerization of polyacetaldehyde to monomer.     

A videomicroscopic study of the effect of l-cis-diltiazem on the photobehavior of Stentor coeruleus

The protozoan ciliate Stentor coeruleus displays a step-up photophobic response to an increase in light intensity in its environment. The motile response consists of a delayed stop of ciliary beating and transient ciliary reversal period. Such light-avoiding behavior was significantly influenced by an incubation of cells with l-cis-diltiazem, a common blocker of cyclic guanosine monophosphate (cGMP)-gated ion channel conductance. The introduction of l-cis-diltiazem to the medium induced ciliary reversal in control cells, mimicking the step-up photophobic response. In light-stimulated ciliates, the presence of this inhibitor caused a substantial decrease of the latency of ciliary stop response, prolongation of the ciliary reversal duration and also an increase of cell photoresponsiveness in a dose- and time-dependent manner. The obtained behavioral results support the suggestion that the photosensitive ciliate S. coeruleus possesses cGMP-gated channels, which may be involved in the process of light signal transduction for the motile photophobic response.     

PHOTOTAXIS IN DICTYOSTELIUM DISCOIDEUM AMOEBAE

Abstract— An apparatus has been developed to measure phototactic movement in a population of amoebae of Dictyostelium discoideum. Fluence–response curves in white light show a positive phototaxis to light below 100mW/m². Higher intensities cause a negative phototaxis. An action spectrum, based on the zero-crossing points in fluence–response curves for monochromatic light, shows a major peak at about 405nm and secondary maxima at about 450, 520, 580 and 640nm. This action spectrum resembles the action spectra for accumulations of amoebae in and dispersal from light traps and that of inhibition of aggregation by light, but is distinctly different from the action spectrum for phototaxis by D. discoideum pseudoplasmodia.     

Calcium Control of the Sign of Phototaxis in Brown Algal Gametes of Mutimo cylindricus

Brown algal swarmers usually exhibit positive or negative phototaxis. Such behaviors influence the increasing or decreasing dispersal distance or colonization on the new substratum. We confirmed that the sign of phototaxis (negative or positive) in male gametes of Mutimo cylindricus was affected by extracellular Ca²⁺ influx through Ca²⁺ channels. Under the control condition (10^?2 m [Ca²⁺]), male gametes swimming with a helical rotation of their cell body mostly showed positive phototaxis. At 10^?3 m [Ca²⁺], more than half of the male gametes showed positive phototaxis, whereas the others showed negative phototaxis. From 10^?4–10^?5 m [Ca²⁺], the phototactic sign changed to negative. When these negative phototactic gametes were transferred back to the control condition, the phototactic sign reverted to positive. At 10^?6 m [Ca²⁺], some of male gametes showed negative phototaxis, but most showed no phototaxis or flagellar beating. Lanthanum, a Ca²⁺ channel blocker, affected the sign of phototaxis at 10^?4 m [La³⁺] under 10^?2 m [Ca²⁺], and male gametes mostly showed negative phototaxis. A further increase in [La³⁺] inhibited phototaxis and flagellar beating. These results pointed out the involvement of Ca²⁺ channels that were blocked by La³⁺ in phototaxis and flagellar beating.     

PHOTOPHOBIC BEHAVIORAL RESPONSES OF EUGLENA IN A LIGHT INTENSITY GRADIENT AND THE KINETICS OF PHOTORECEPTOR PIGMENT INTERCONVERSIONS*

Abstract— Accumulation of Euglena gracilis in small illuminated regions called light traps is due to a phobic response to the diminished light intensity at the boundary of the region. The rate of such accumulation of cells was measured as functions of both the light intensity within the trap and the change of intensity at the boundary of the trap. The initial rate of accumulation of a population of cells was taken to be a direct measure of the phobic response of a single typical cell. The data indicate that the strength of the behavioral response in a single cell may be described as being proportional, to the rate of change of the amount of photochemically active form of a photoreceptor pigment molecule which can exist in two predominant forms.     

PHOTOTACTIC BEHAVIOR OF INDIVIDUAL CELLS OF CRYPTOMONAS SP. IN RESPONSE TO CONTINUOUS AND INTERMITTENT LIGHT STIMULI

Abstract— The phototactic response of cells of Cryptomonas sp. to stimulation with continuous or intermittent lateral light was determined by an individual cell method using photomicrography and videomicrography. The cells showed positive phototaxis under the conditions studied. The phototactic orientation of individual cells was induced most effectively by irradiation with light of 570 nm; blue light was less effective, and no orientation was found in red light. An intermittent stimulus regime with a long dark interval (250 ms) elicited a weaker phototactic orientation than did a regime with a short dark interval (63 ms) irrespective of the duration of light pulses (16, 250 and 1000 ms). The swimming rate was ca. 240 ums ^-1 and the rotation period ca. 450 ms in the dark, neither of which was greatly affected by stimulation with continuous or intermittent light. Neither step-up nor step-down photophobic responses were observed at the time of onset or removal of the light stimulus under the experimental conditions. The swimming direction of individual cells became gradually oriented toward the light source. Phototactic response was detectable within 4 s after the onset of light stimulation, reaching a saturation level after more than 30 s.     

BLUE LIGHT PERCEPTION BY ENDOGENOUS REDOX COMPONENTS OF THE PLANT PLASMA MEMBRANE

b-Type cytochromes of the higher plant plasma membrane may be reduced by irradiation with actinic blue light (light-induced absorbance change). Although this reaction has been reported to depend on the presence of an exogenous oxygen-scavenging system, significant cytochrome reduction was obtained in bean hook (Phaseolus vulgaris L. cv. “Limburgse Vroege”) plasma membranes without any addition. An endogenous oxygen-consuming reaction is apparently sufficient to achieve a proper redox balance. A blue light-mediated absorbance change with absorbance minima at 450 and 475 nm precedes cytochrome b reduction and indicates the presence of a flavoprotein in the plasma membrane fraction. Cytochrome b reduction by blue light in the absence of an oxygen scavenger is highly sensitive to flavin photosensitizers. Glucose oxidase, which has previously been used to lower the oxygen concentration in membrane samples, was demonstrated to have a photosensitizing effect. Inhibitors of flavin photochemical reactions (KI and phenylacetic acid) were highly effective in preventing cytochrome b reduction. These results indicate that the blue light-mediated reaction probably involves an endogenous plasma membrane flavoprotein as the photoreceptor. As plasma membrane NADH-dependent oxidoreductases potentially are flavoproteins these experiments raise the question whether a plasma membrane cytochrome b and a flavin-enzyme may cooperate in blue light reactions. Evidence is also discussed, suggesting the possible involvement of oxygen radicals in the blue light-induced cytochrome b reduction.