Auxin Transport Synchronizes the Pattern of Cell Division in a Tobacco Cell Line

doi:10.1104/pp.103.027953

Auxin Transport Synchronizes the Pattern of Cell Division in a Tobacco Cell Line¹

Prisca Campanoni^*, Bernd Blasius and Peter Nick

Biologisches Institut II, Albert-Ludwigs-Universität Freiburg, Schänzlestrasse 1, D-79104 Freiburg, Germany (P.C., P.N.); and Nonlinear Dynamics, Institute of Physics, University of Potsdam, Am Neuen Palais 10, D–14469 Potsdam, Germany (B.B.)

ABSTRACT

TOP
ABSTRACT
RESULTS
DISCUSSION
CONCLUSIONS
MATERIALS AND METHODS
LITERATURE CITED

The open morphogenesis of plants requires coordination of patterningby intercellular signals. The tobacco (Nicotiana tabacum cvVirginia Bright Italia) cell line VBI-0 provides a simple modelsystem to study the role of intercellular communication in patterning.In this cell line, singular cells divide axially to producelinear cell files of distinct polarity. The trigger for thisaxial division is exogenous auxin. When frequency distributionsof files are constructed over the number of cells per file duringthe exponential phase of the culture, even numbers are foundto be frequent, whereas files consisting of uneven numbers ofcells are rare. We can simulate these distributions with a mathematicalmodel derived from nonlinear dynamics, which describes a chainof cell-division oscillators where elementary oscillators arecoupled unidirectionally and where the number of oscillatorsis not conserved. The model predicts several nonintuitive propertiesof our experimental system. For instance, files consisting ofsix cells are more frequent than expected from a strictly binarydivision system. More centrally, the model predicts a polartransport of the coordinating signal. We therefore tested thepatterns obtained after treatment with 1-N-naphthylphthalamicacid, an inhibitor of auxin efflux carriers. Using low concentrationsof 1-N-naphthylphthalamic acid that leave cell division andaxiality of division unaltered, we observe that the frequenciesof files with even and uneven cell numbers are equalized. Ourfindings are discussed in the context of auxin transport assynchronizing signal in cell patterning.

Pattern formation in living organisms culminates in a predictableand reproducible relation between the various elements of thebody plan. There are two principal modes that might lead tothis nonrandom organization: (a) A stereotypic sequence of asymmetric,formative cell divisions could define differential developmentalfates for the prospective descendants originating from thiscell division (Weismann, 1892

). As a characteristic of this"mosaic-mode" development, a removed element cannot be replacedby redefinition of neighboring elements, even at a stage whentheir differentiation has not become manifest. (b) The patternoriginates from coordinative signaling between the elementsthat are patterned. In this "regulation mode" development, theremoval of one element can be buffered by the remaining elementsthat are redefined with respect to their developmental fate.In the extreme case, a complete new body plan is established,although the resulting organism will be smaller (Spemann andMangold, 1924

). In the attempt to explain this so-called proportionalharmony that is highly robust against stochastic fluctuationsin the initial situation, the mathematics of Turing systemswas adapted to biology (Turing, 1952

). First developed to explainpatterning in Hydra sp., a locally constrained, self-amplifyingfeedback loop of an activator was linked to a far-ranging mutualinhibition (Gierer and Meinhard, 1972

). This socalled Gierer-Meinhardmodel was later found to be a very powerful tool to simulatea great number of biological patterns from segmentation in fruitfly(Drosophila melanogaster; Meinhard, 1986

) to the formation ofleaf veins (Meinhard, 1976

As a developmental consequence of their sessile lifestyle, plantsare characterized by extreme developmental flexibility. Thisincludes so-called open morphogenesis, i.e. the body plan iscontinuously enlarged by addition of new elements and thereis no innate limit to this reiterative enlargement. Consequently,a mosaic mode of patterning would not work in plants. The principaltotipotency of plant cells highlights impressively the regulationmode of plant development. Almost independently of its developmentalhistory, each plant cell can reestablish a complete new organism(somatic embryogenesis), and the body plan of such somatic embryosis indistinguishable from those originating from normal (zygotic)development.

Among the putative signals that regulate pattern formation inplants, the polar transport of auxin seems to play a centralrole. The pattern of vascular tissue (Aloni, 1987; Warren Wilsonet al., 1994; Sachs, 2000), leaf veins (Mattsson et al., 1999),and the position of meristems (Hadfi et al., 1998; Reinhardet al., 2000) represent good examples for patterning eventsthat are coordinated by polar auxin fluxes. For the patterningof vascular tissue, the model runs as follows: Initially, allcells are more or less equal in their competence to form a vessel.In response to environmental stimuli or stochastic fluctuations,one of them begins to transport more auxin than the neighbors,causing a draining effect. This will reinforce the polarityof this cell leading to an even stronger auxin transport ina self-amplifying feedback loop. This auxin-transporting celldifferentiates into a vessel, whereas the depletion of auxinfrom the neighboring cells prevents them from differentiatinginto vascular tissue. By channeling the flow of auxin, the vesselprecursor will capacitate the differentiation of its adjacent,downstream neighbor cell. Thus, the adjacent cells will coordinatetheir development such that they form a functional transporttissue. In this context, synchrony and coordination betweenneighboring cells are of extreme importance (Sachs, 1993; forreview, see Sachs, 1991a, 1991b, 2000). Formally, the self-amplificationof cell polarity by a polar auxin flow corresponds to the localactivator in the Gierer-Meinhard model. Interestingly, the lateralinhibition is brought about by the competition of neighboringcells for limited resources of the activator, i.e. not by areal inhibitor molecule, but by the absence of an activatingmolecule. The same mechanism was later invoked to explain otherpatterning events, such as growth of new leaves, formation ofside roots, or initiation of meristem, and is supported by mutantstudies (for review, see Berleth and Sachs, 2001).

It is obvious, however, that polar auxin flux can be only onecomponent of patterning and must interact with local differencesin cellular competence (for review, see Scheres, 2000). Thehigh complexity of plant organs or even tissue explants witha great number of different cell types makes it extremely difficultto study intercellular coordination on the cellular level. Anideal system should meet the following requirements: (a) Itshould consist only of one or few cell types. (b) It shouldpossess the ability to establish axiality and polarity. (c)It should be predictable in its developmental responses. (d)It should be amenable to control by exogenous signals. (e) Itshould be easy to handle. (f) It should be accessible to cellbiological analysis.

The tobacco (Nicotiana tabacum cv Virginia Bright Italia) cellline VBI-0 meets all of these requirements. It derives fromstem pith parenchyma, i.e. the cells that can differentiateinto vascular tissue in response to auxin flow. In the sameway as its ancestor cells within the tissue, this cell linegrows in cell files exhibiting basic characteristics in patternformation such as clear axis and polarity of cell division andgrowth (Opatrn $y$ and Opatrná, 1976; Petrá $s$ ek et al.,1998). The progression into the culture cycle, the durationof the lag phase, the rate of cell division, and the lengthof the exponential phase are strongly dependent on auxin actionin this cell line (Za $z$ ímalová et al., 1995, 1996).Polarity and axiality of VBI-0 cells were recently shown todepend on the transport of auxin (Petrá $s$ ek et al., 2002).The cell files are formed from singular cells, such that positionalinformation inherited from the mother tissue does not play arole. If there are patterns of competence within a cell file,they must originate de novo during the culture cycle.

Using this cell line as a model system, we demonstrate thatcell division within the file is partially synchronized, leadingto a much higher frequency of cell files with even cell numbersas compared with files with uneven cell numbers. We can simulateour experimental data by a mathematical model derived from nonlineardynamics, where elementary celldivision oscillators are coupledunidirectionally, and where the number of oscillators is notconserved. The model predicts several nonintuitive propertiesof our experimental system, among them a polar transport ofthe coordinating signal. We tested whether this signal is polarauxin flux and observed that we can remove the synchronizationof cell division by low concentrations of 1-N-naphtylphthalamicacid (NPA), a well-known inhibitor of polar auxin transport(for review, see Morris, 2000). It has been shown repeatedlythat auxin is necessary for the progress of the cell cycle andthus can be used to synchronize the cell cycle in plant-cellcultures (Stals and Inzé, 2001; Himanen et al., 2002).However, to our knowledge, this is the first time that auxinhas been found to participate in the coordination of adjacentcell divisions.

RESULTS

TOP
ABSTRACT
RESULTS
DISCUSSION
CONCLUSIONS
MATERIALS AND METHODS
LITERATURE CITED

Cell Division Is Synchronized by the Addition of Exogenous Auxins in VBI-0

The culture cycle in VBI-0 consists of two distinct phases:Cell divisions are confined to the first phase of the cycle,whereas the second phase is characterized by prominent cellelongation (Fig. 1). Figure 1A shows examples of morphologicalchanges in VBI-0 cells along the culture cycle. A classicalgrowth curve in Figure 1B plots cell density against time. Understandard conditions, the singular, polar cells prevailing atthe time of subcultivation initiate strictly axial divisionsaround 2 to 3 d after subcultivation. The subsequent divisionsin the cell file follow the axiality manifest from the firstdivision. The two terminal cells show a clear polarity: Thebasal cell is rounder with the nucleus in the apical half ofthe cell, almost adjacent to the cross wall, whereas the apicalcell is more pointed with a nucleus that is situated in thebasal half of the cell but with a greater distance between nucleusand cross wall. After 10 to 12 d, the elongation phase initiates:The cells stop to divide and elongate in the direction of thefile axis. At the end of the elongation phase (around 18 d aftersubcultivation) the files disintegrate, and the cells returnto the status of the starting point. The total culture cyclelasts 21 d.

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Figure 1. Schematic representation of the culture cycle in the tobacco cell line VBI-0. After inoculation in presence of auxin, singular cells divide into cell files presenting a clear axis of cell division and polarity. After 10 to 12 d, the cells stop to divide and elongate in the direction of the file axis. At the end of the elongation phase (around 18 d after subcultivation), the files disintegrate, and the cells return to the initial status. The images are confocal sections of cells stained with rhodamin-G6-chloride, a fluorescent membrane dye. Bars = 50 µm.

To test whether the initiation of cell division is triggeredby auxin or just by the supply with fresh nutrients, we inoculatedthe cells at time 0 (21 d old from the previous culture cycle)in fresh Heller medium that was either complemented with thestandard concentrations of auxins or in fresh medium withoutauxins. The number of cells per cell file as measure for divisionactivity was scored at 2 d after inoculation (Fig. 2A, secondand third bars). Under auxin starvation, the average numberof cells per file was virtually identical to that of the originalinoculum with the vast majority of cells still being in thesingular state. In contrast, in the presence of auxin, mostcells had already undergone the first division. The blockedcell division in the auxin-starved population was not due toreduced viability. In all of the samples, the cell viabilitywas higher than 90% (data not shown).

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Figure 2. Auxin controls cell division in VBI-0 and is responsible for even cell numbers within individual files. Cells were either inoculated into fresh medium supplied with auxins (+auxin) or in auxin-free fresh medium (-auxin); in the "refeeding experiment," cells that had been grown for 2 d in auxin-free medium were complemented with auxin and cultivated for further 4 d either without (-auxin) or with (+auxin) exogenous auxins. A, The average numbers of cells per file were determined for the initial state (0 d), and after 2 and 6 d, respectively. The frequency distributions over cell number per file are shown for 2 d after inoculation (B), for 6 d after inoculation, and for the refeeding experiment at 6 d after inoculation (C). Each experiment was repeated three times, scoring more than 10³ cells per sample every time. Error bars indicate SE.

Auxin starvation has been shown to stimulate production andaccumulation of endogenous auxins, mainly indole-3-acetic acid(Za $z$ ímalová et al., 1995). Therefore, the starvationexperiment was prolonged to test whether endogenous auxin influencescell division during later stages of the exponential phase (Fig. 2A,forth and fifth bars). Cell division remained suppressedin the auxin-starved population as compared with the controlcultivated in presence of auxin. Again, the viability of theauxin-starved samples was the same as in the controls (datanot shown). These data show that exogenous auxin is necessaryto trigger cell division. In the context of the present work,exogenous auxin is defined as a 1:1 combination of 1-naphthaleneaceticacid (NAA) and 2,4-dichlorophenoxyacetic acid (2,4-D).

To test, whether auxin is sufficient to trigger cell division,we asked whether exogenous auxin can restore division in cellsthat had undergone auxin starvation for 2 d and therefore wereblocked in their division. We observed that 4 d after this delayedaddition of auxin (i.e. 6 d after inoculation), the averagenumber of cells per file had reached the level of cells thathad been continuously cultivated in presence of auxin (Fig. 2A,last bar). This refeeding experiment demonstrates that evenunder favorable conditions (i.e. when nutrients are freshlysupplied), exogenous auxin is strictly necessary to triggercell division.

In addition to the average cell numbers per file, we determinedthe corresponding frequency distributions over the cell population(Fig. 2, B and C). Two days after subcultivation (Fig. 2B),the presence of auxin shifted most of the cells into division(just around 25% of the files in the culture are still singular).In contrast, the addition of fresh medium without auxins blockedthe population in the original situation with more than 70%of the files being singular. The level of cell coordinationat 2 d after the addition of auxin is remarkable: up to 70%of the cell files had just undergone the first division. Whenthe frequency distributions are analyzed after 6 d in the presenceof auxins (Fig. 2C), pluricellular files have become very frequent.In contrast, the distribution of cells that had been cultivatedunder auxin starvation for 6 d is strongly shifted to low cellnumber files, close to the behavior of the original inoculum.Interestingly, cells cultured in the presence of auxins showan oscillatory behavior of the frequency distribution, withpeaks of frequency for even cell number files. This alternatingbehavior was observed in every single independent experiment(data not shown) used for the pooled distribution in Figure 2C,suggesting that a high level of synchronization is maintainedeven at 6 d after subcultivation. We have recorded similar distributionsthrough the entire exponential phase (5–9 d after subcultivation).This indicates that the oscillations represent a characteristicfeature of exponential growth for this cell line in standardconditions. Moreover, when the frequency distributions weredetermined for the refeeding experiment, no significant differenceswere observed between prestarved cells that had been complementedwith auxins at d 2 and cells that had been continuously cultivatedin presence of auxin. Addition of auxin after 2 d of auxin starvationcompletely restored the oscillatory distribution observed inthe controls.

Summarizing our data, we observed that (a) auxin is the triggerfor cell division in VBI-0, (b) cell division is synchronizedsuch that files with even cell numbers are much more frequentthan files with uneven cell numbers, and (c) auxin can triggernot only cell division, but also the synchrony of cell division.

Mathematical Modeling

In a strictly binary system of cell division, files consistingof 2ⁿ cells (2, 4, 8, 16...) should be most frequent. In oursystem, however, we observe that files consisting of six cellsare highly frequent, even more than files consisting of eightcells, which is difficult to reconcile with a strictly binarysystem. Thus, we conjecture the existence of some exchange ofinformation (coupling) between the cells that coordinates andsynchronizes cell division. To test whether the observed deviationfrom a binary system could be caused by coupling, we developeda simple mathematical model to simulate the dynamics of cellnumber for different combinations of coupling and innate cellcycle variability.

In the terminology of nonlinear dynamics, our cell culture systemcan be described as a one-dimensional array of coupled oscillators,where the number of oscillators is not conserved over time.Instead, a new oscillator is generated and inserted adjacentto the "parent" cell, whenever a certain oscillator has finishedone cell cycle. In this framework, a given oscillator couldrun its loop freely (no coupling). Alternatively, it could sensean interference with the two neighboring oscillators (bilateralcoupling) or just with one of them (unilateral coupling). Usingthis theoretical background, the patterns of cell number canbe modeled with a reiterative algorithm from the singular cellstate through the formation of a pluricellular file of N cells.The growth of cell number per file can thus be simulated asa function of time, N(t).

In this model, the state of each oscillator, i = 1.N(t), issimply defined by a real number, called the phase ${tau}$ _i, which describesthe time the cell will need to accomplish its cell cycle inthe absence of coupling. Each simulation starts with the singularcell state, N(0)=1. Then, time is increased until the firstoscillator i has completed one cycle. As a consequence, itsphase is reduced to zero, ${tau}$ _i (t)=0. At this time point, the followingtwo events are introduced:

(a) To describe unidirectional coupling, the phase of the rightneighbor of the dividing cell, i + 1, is reduced by ${epsilon}$ (degreeof coupling strength),

Here, we have taken into account that the remaining time tocell division cannot be lower than zero. Thus, the length ofthe neighboring cell cycle is reduced due to interfering signalsfrom the dividing cell. In this way, a higher chance of divisionis induced in the neighbor. In the case of bidirectional coupling,the phases of both the right and left neighbor are reduced bythe same amount ${epsilon}$ ; whereas in the scheme without coupling, theneighboring phases are left unchanged.

(b) The mother cell is removed and replaced by two newly generateddaughter cells. Thereby the total number of cells in the fileincreases by one.

The two newborn cells are inserted in the cell file at the positionof the mother cell. Each of the two daughter cells is assignedwith a new independent random phase, which describes its naturalperiod length in the absence of coupling. This value is a randomnumber taken from a Gaussian distribution with mean period lengthT and SD ${sigma}$ .

This algorithm is repeated until a certain large time is passed,in this way successively generating a chain of cells. The totalnumber of cells is scored as a function of time, N(t). Notethat the model is based on the assumption that cell files continueto divide to arbitrary size. This means that the model doesnot incorporate the elongation phase with a division stop aftera certain time. Second, both daughter cells originating froma division are treated equally and in particular are independentof the previous state (i.e. period length) of their mother cell.

The model depends on only three basic parameters. (a) The averagefree-running period length T. This parameter does not inflictany dynamical consequence because a change in T only resultsin an overall rescaling of time and can easily be fitted tothe experimental data. However, note that the observed periodlength is shorter than the free-running period length T, becauseit is reduced by the coupling. The observed period length canbe estimated from the average number of cells per file at differenttime points of the culture cycle (Table I). In our model, weused for the free-running period length a somewhat increasedvalue of T = 4 d as first approximation. (b) The variabilityof natural period length ${sigma}$ . This parameter describes the disorderof the cell cycle measured as the SD of the natural period lengthin percent of the mean natural period T. In our simulations,we varied ${sigma}$ in the range from 5% up to 50%. (c) Degree of coupling ${epsilon}$ . Because in our model, coupling results in a reduction of periodlength, we measure the coupling strength in percent of the meanperiod length, T. In our simulation we vary ${epsilon}$ in the range from0% to 100%.

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Table I. Estimation of the cell cycle length from the data shown in Figure 2

The time course of cell division can be approximated by an exponential curve: N(t) = N(0)·e^kt with k being the average time of the cell cycle, t the time after inoculation, N(t) the average cells per file at time t, and N(0) the initial number of cells in the inoculum. This approximation leads to an estimate for k of 2.9 d.

To describe the growth over a population of files and to obtaingood statistics, the whole program was repeated for a largenumber files, and the results were averaged over a large numberof simulation runs (here at least 2,000). For each of thesepossibilities, the algorithm was calculated for a large numberof files (at least 2,000), and the simulated frequency distributionsof cell number (as estimate for the probability) were plottedas number of cells per file at a given time point.

Figure 3 depicts the simulation results. Plotted are the distributionof percentage of files with a certain number of cells per fileat successive days. To indicate probability frequencies, a grayscale was used, in which the white color represents a probabilityof 0% and the black color a probability of 100%.

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Figure 3. Simulation of the temporal dynamics for the number of cells in individual files using a model based on coupling of elementary oscillators. The probability distributions of cell number per file are plotted for different combinations of coupling and cell-cycle variability after averaging more than 2,000 simulation runs. Left, Predicted dynamics of cell number per file during successive days (percentage). The probability for each number at a given time point is coded by a gray scale in which the white color represents a probability of 0% and the black color a probability of 100%. Time is given in days elapsed from the initial state where there is only one cell with random phase. Therefore, the average number of cells at total division time 0 equals one. Right, Probability distributions predicted for d 0 (dashed line, circles), d 2 (dotted line, triangles), and d 6 (solid line, stars). These distributions take into account that the initial cell number per file at time 0 was 1.23 (see Table I). The details of the model are explained in the text. A and B, Low variability ( ${sigma}$ = 8%) and strong degree of coupling ( ${epsilon}$ = 100%). C and D, Medium variability ( ${sigma}$ = 40%) strong degree of coupling ( ${epsilon}$ = 100%). E and F, Medium variability ( ${sigma}$ = 40%) weak degree of coupling ( ${epsilon}$ = 40%). G and H, Medium variability ( ${sigma}$ = 40%) no coupling ( ${epsilon}$ = 0%).

Peaks of probability for even cell numbers were neither obtainedwhen the algorithm was run at a large degree of cell-cycle variability,nor for bilateral coupling (data not shown). However, underthe assumption of strong unilateral coupling, even cell numbersare more frequent than uneven cell numbers. For low or mediumvariability of cell-cycle length, the simulation fits to ourexperimental data, showing peaks of probability in correspondenceof even cell number files and a relatively high incidence offiles consisting of six cells (Fig. 3, A–D), which wasnever observed in any of the other combinations (data not shown).

When the model is run at complete absence of coupling, it culminatesinto a binary distribution with probability peaks at 2, 4, 8,....2ⁿ cells per file, when the variability of the cell cycle islow (data not shown). When the variability of the cell cycleis intermediate and the coupling is weak (Fig. 3, E and F) orabsent (Fig. 3, G and H), files with two and four cells becomefrequent, but files with three cells are also more frequentas compared with the strong unilateral coupling (Fig. 3, C and D).Under these conditions, the model predicts complete randomizationfor the incidence of files with more than four cells.

To test the reliability of our model, we compared the simulateddistributions with our experimental data. To generate a highlysignificant data set, we determined division distribution in17 independent experiments comprising more than 10³ cells eachtime. We observed the described oscillatory synchrony in eachsingle experiment (the pooled distribution is shown in Fig. 4).This highly reproducible pattern indicates that the mechanismresponsible for this synchronicity must be very robust. In particular,the simulation using strong unilateral coupling at medium cell-cyclevariability leads to a predicted frequency distribution thatclosely fits to the experimental data that had been collectedat d 6 after inoculation (Fig. 4).

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Figure 4. Comparison between experimental data and simulation. The distribution observed after 6 d in presence of auxin is shown as a solid line (experimental data). The distribution pools the data of more than 17 x 10³ cells from 17 independent experiments. The distribution predicted by the model for strong unilateral coupling at medium cell-cycle variability (simulated data) is indicated by the dotted line. Error bars indicate SE.

NPA, an Inhibitor of Polar Auxin Transport, Eliminates the Coupling

The mathematical model could approximate the observed frequencydistribution under the assumption of strong unilateral coupling.Because auxins can already trigger cell division per se (Fig. 2A)but in addition can restore the peculiar frequency distributionover cell number per file (Fig. 2C), we asked whether the couplingsignal might be auxin.

We therefore inoculated VBI-0 cells either under standard conditions(control) or in presence of 5 µM NPA, an inhibitor ofpolar auxin transport. The concentration was chosen such thatauxin transport is impaired, but not completely eliminated (Petrá $s$ eket al., 2002) to avoid unspecific side effects of auxin hyperaccumulation.This treatment did not affect the overall rate of cell division(Fig. 5A, first two bars), and, consistently, we did not detectany reduction in viability (data not shown). However, the distributionof cell division is strongly affected (Fig. 5C, compare thesolid curve for the control with the dotted line for the sampletreated with 5 µM of NPA). Especially for files with ahigher number of cells, the difference in the incidence of evenand uneven numbers vanished completely. Only a slightly reducedfrequency of files with three cells as compared with those withtwo or four persisted the treatment with this inhibitor. Thisfrequency distribution is predicted by the model for intermediatevariability in the length of the cell cycle and weak coupling(Fig. 3, E and F). It should be noted that at this concentration,the polarity of the cell file was mostly unaltered, and we observedabsolutely no effect on the axiality of cell files (data notshown). We also did not observe any stimulation of cell elongation(Fig. 5B, first two bars). However, when we performed this analysiswith a high concentration of NPA that causes a complete blockof polar auxin transport (50 µM), we observed an inhibitionof cell division (Fig. 5A, last bar), a stimulation of cellelongation (Fig. 5B, last bar), and a dramatic loss of filepolarity and axiality (data not shown), consistent with recentlypublished data (Petrá $s$ ek et al., 2002). Under these conditions,files with more than four cells are very rare (Fig. 5C, whitesymbols and dashed curve). Again, the probability of files composedof three cells is almost the same as that for files with fourcells.

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Figure 5. Effect of NPA on cell division and cell elongation in VBI-0. Cells were either inoculated under standard conditions with auxin alone (control) or in presence of auxin combined with 5 µM or 50 µM NPA, respectively, and the effects on cell division and elongation were assayed at d 6 after inoculation. A, Average cell number per file. B, Average ratio of cell length to width. C, Frequency distribution over cell number per file. The data are pooled from more than 5 x 10³ cells from five independent experiments. For the ratio of cell length and width, more than 300 individual cells from three independent experiments were viewed by confocal microscopy and images recorded for the central section of the cell. Error bars indicate SE.

Summarizing the inhibitor experiments, we observe that low concentrationsof NPA that do not affect the overall degree of cell division,the proportionality of cell expansion, axiality or polarityof the files, or their viability eliminate more or less completelythe synchrony of cell division mirrored in the predominanceof even-numbered cell files.

NPA Impairs the Coordination of Cell Cycles along the Cell File

To better understand the dynamics of file growth, the cellswere fixed in early exponential phase (4 d after inoculation),and images were recorded after staining the DNA with Hoechst.This allowed location of mitotic events along the cell file.The observed division patterns were grouped into different categories:synchronous division (i.e. all of the cells in the file undergomitosis in the same moment), division starting from one edgeof the file, division initiating from the center of the file,or random (no visible connection between division events withina file). The frequency of these categories was scored eitherin standard condition (control) or under 5 µM of NPA (Fig. 6A).This concentration was chosen to avoid side effects dueto inhibition of cell division.

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Figure 6. Effect of NPA on the localization of cell division events along individual cell files. After 4 d of cultivation in either standard conditions with auxin alone or with auxin in combination with 5 µM NPA, the cells were fixed, and the DNA was stained with Höchst for pictures recording. Individual files were grouped according to the spatial pattern of division (A) or to the transitions between different cell numbers (B), and corresponding frequency distributions were constructed. A, Spatial pattern of cell divisions in relation to cell number per file. Synchronous, All cells of a file divide simultaneously; edge, division is initiated at one edge of the file and spreads into the file; central, division initiates in one center of the file; random, division initiates at different locations of a cell file. B, Dynamics of file growth. Files of a given cell number n were grouped, and within this population (defined as 100%), the frequency of transitions into the subsequent cell numbers (n + 1, n + 2) was plotted.

We observed that mitosis along the cell file is rarely an isolatedevent: Commonly, several cells of the same file region dividesimultaneously generating waves of mitosis. In the control,synchronous division was frequent only among bicellular files(around 50%), whereas division waves from the edge prevailedfor files composed of three or more cells. For files with fouror more cells, an increasing number of division "hot-spots"in the file center was noted, and for long cell files (fiveor more), random division could be observed. However, not asingle case for a quadricellular file with random division wasever noted.

NPA was affecting mostly files composed of two and three cells.In both cases, the frequency of synchronous divisions was higherafter treatment with NPA as compared with the control, whereasthe frequency of division waves from the edge of the file wasreduced. For higher cell numbers, NPA increased the frequenciesof central and random division events as compared with the respectivecontrol values.

We asked then, whether we could trace preferential transitionsfrom a given cell number to certain, higher cell numbers. Wedefined the total number of files of a given cell number n as100% and then scored how many of those files chose the transitionto the number n + 1, n + 2, and so forth (Fig. 6B). Under standardconditions, almost all bi- or tricellular files pass directlyinto the quadricellular state, and from there, they preferentiallypass into the six- and the eight-cell stage. The treatment withNPA affects the first division steps (until the formation ofquadricellular files) only marginally. However, quadricellularfiles loose their preference for a transition into evennumberedfiles, but more often they form files composed of five or sevencells.

DISCUSSION

TOP
ABSTRACT
RESULTS
DISCUSSION
CONCLUSIONS
MATERIALS AND METHODS
LITERATURE CITED

In plants with their open morphogenesis, the patterning of cellsand tissues must cope with the continuous expansion of the bodyplan through reiterative addition of new elements. Several experimentsdemonstrated the central role of basipetal auxin transport inmediating plant pattern formation (Friml et al., 2002; Friml,2003; for review, see Berleth and Sachs, 2001). However, theidea of auxin as morphogen acting on a homogenous populationof cells that respond exclusively to the local concentrationof the morphogen does not completely explain all of the aspectsof patterning in plants: High levels of synchronization andcoordination between different parts must play an importantrole, as well as specific local differences in cell competence.Therefore it would be extremely important to study the finecellular events that characterize the control of patterning.

The VBI-0 tobacco cv Virginia Bright Italia cell line representsan ideal system to study cellular aspects of pattern formation.This cell line is a relatively homogenous system easily accessibleto cell biological analysis and endowed with the ability toestablish axiality and polarity.

Our first data shown in Figure 2 demonstrated that the systemis amenable to an external control by exogenous auxin. It isexogenous auxin that triggers a new culture cycle in VBI-0 (Fig. 2A),and it is exogenous auxin that synchronizes the cell cycle(Fig. 2B). Even at 6 d after inoculation, cell division remainsmostly blocked when the cells are left without exogenous auxin(Fig. 2, A and C). The slight, residual division activity persistingunder these conditions could be due to endogenously producedauxin (Za $z$ ímalová et al., 1995) or more probablycould be caused by a small exogenous auxin pool present in theoriginal inoculum. The effect is anyway marginal compared withthe induction of cell division in response to exogenous auxin.

In the presence of exogenous auxins, a clear pattern of celldivision consisting in elevated frequencies of even-numberedcell files becomes manifest (Figs. 2C and 4). Through refeedingexperiments (Fig. 2, A, last bar, and C), we were able to demonstratethat the expression of this pattern depends on exogenous auxin.However, it is astonishing that the patterning program willlead to a correct pattern independently from the time when auxinis added. To get insight into the mechanism of this highly robustpatterning program, we ventured to model the pattern using anonlinear dynamics approach.

The VBI-0 cell culture can be conceived as an array of oscillators,the number of which is not conserved on time. This allowed usto mathematically model the division pattern during the exponentialphase. The in silico simulation performed according to thismodel could approximate our experimental data when a specificprecondition was met. When the probability of a given cell todivide is enhanced by a neighboring cell and the enhancing signalmoves unidirectionally through the cell file (Fig. 3, A–D),predicted and observed distributions match almost perfectly(Fig. 4).

Consistent with previously published data (Za $z$ ímalováet al., 1996), we find that auxin has a highly synchronizingeffect on cell division in VBI-0 (Fig. 2). In addition, auxinis known in planta to be transported unidirectionally throughthe tissues. For the context of VBI-0, auxin transport was shownto be required for cell division, cell axiality, and file polarity(Petrá $s$ ek et al., 2002). Therefore, we have chosen auxinas a potential candidate for the unilaterally transported couplingagent, and we have tested this hypothesis experimentally. Weobserve that the inhibition of auxin transport produces a frequencydistribution (Fig. 5C) where files with three cells are almostas frequent as those with two and four cells and where filesof higher cell numbers are rare and do not show a predominanceof even numbers. This would be predicted by our model for areduction or elimination of coupling (Fig. 3, E–H), whichis evidence for intrafile auxin transport being required forthe patterning of cell division.

When we analyzed the dynamics of file growth (Fig. 6), we noticedthat, under standard conditions, mitosis within a given cellfile is rarely an isolated event, but that the individual cellsof a file divide coordinately preferentially following divisionwaves that start from one edge and "move" polarly through thefile. This is especially true for low-numbered cell files (composedof two, three, and four cells), whereas files of higher cellnumber display an increased frequency of central divisions (Fig. 6A).As a consequence of this coordinated wave of mitoses, thefiles develop preferentially into even-numbered states (sixand eight cells), independently from their original cell number(Fig. 6B).

In contrast, treatment with 5 µM NPA impairs the formationof division waves in bi- and tricellular files as compared withthe control. Instead, central (in tri- and quadricellular files)and random divisions (in the longer cell files) become morefrequent (Fig. 6A). Although the initial divisions leading tothe tri- or quadricellular state seem to proceed mostly in thesame way as for the controls, the impaired coordination of celldivision becomes manifest during the subsequent division events:tri- and quadricellular files generate odd-numbered files athigh frequency, such that the frequency peaks for even-numberedfiles typical for cells grown in standard conditions do notemerge after treatment with NPA (Fig. 6B).

Together with the data shown in Figure 2, these results allowus to draw a model on the dynamics of division coordinationin standard conditions: The first cell division is triggeredby the exogenous auxin added at the time of inoculation. Inmost of the newborn bicellular files, both daughter cells dividesimultaneously to generate files composed of four cells. Thissecond division-step could either still be controlled throughthe added auxin or could alternatively already be coordinatedby an internal signal. For the next two divisions, a clear coordinationvia the coupling signal (most likely polar auxin transport)reinforces the formation of even-numbered files. When the cellnumber per file increases, these polar division waves are progressivelyoverlaid by newly emerging hot spots of mitosis in the internalregions of the file and eventually even randomly localized mitoses.This indicates that for an increasing number of cells in a file,the relative influence of the coupling weakens progressively.This model of division dynamics is perfectly compatible withthe observed frequency distribution (Fig. 5) and the frequencydistribution predicted for unilateral coupling.

In the original situation within the plant tissue, the ancestorsof the VBI-0 cell line can respond to auxin fluxes by formingcontiguous vessels. In a classical experiment by Sachs (1981),auxin was provided in a way that no flux of auxin could occur.Under these conditions, no vessels could be regenerated. However,as soon as an outlet was created such that auxin could flow,new vessels formed in the direction of the flow. This meansthat the pattern is not generated by auxin per se, but by theflux of auxin. This means that auxin acts just as a triggerthat allows local, intrinsical differences between neighboringcells to generate a visible pattern. In the terminology of theGierer and Meinhard (1972) model, polar auxin flow acts as self-amplifyingactivator, whereas mutual competition of neighboring cells forauxin plays the role of lateral inhibition. Our refeeding experimentsshow that there exists an intrinsic prepattern that is independentof auxin but is rendered manifest in response to exogenous auxin.Already, a mild inhibition of polar auxin transport that leavescell division rate as such as well as cell axiality and polarityuntouched can remove the preponderance of even-numbered cellfiles. This indicates that the pattern is intimately linkedto a flow of auxin. In other words, our experimental systemhas truly preserved the patterning principles of its ancestortissue.

CONCLUSIONS

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ABSTRACT
RESULTS
DISCUSSION
CONCLUSIONS
MATERIALS AND METHODS
LITERATURE CITED

From this study, we find that the tobacco cell line VBI-0 isan ideal basic system for studying cellular events controllingauxin-induced pattern formation in plants. Our NPA experiments,in combination with the in silico simulations we performed,clearly demonstrated that auxin polar transport, and not auxinper se, mediates pattern formation. In particular, our NPA experimentshighlighted another very interesting issue. Consistent withrecently published data (Petrá $s$ ek et al., 2002), high(50 µM) concentrations block axiality and polarity inVBI-0 and slow down cell division (Fig. 5A) in favor of enhancedcell elongation (Fig. 5B). However, cells treated with 5 µMNPA did not show any effect on division rate and axiality, butalready a dramatic loss of the signal coordinating cell division(Fig. 5). This means that the cells are much more sensitiveto manipulation of the coupling signal compared with other auxin-dependenteffects. This finding opens the interesting question of howa cell flooded by exogenous auxin can distinguish between auxininflux from the medium and intrafile auxin flux.

We are presently investigating the patterns of division andelongation in response to altered balance between differentauxins. To understand how a dividing cell can convey throughauxin transport a coordinative signal to a neighboring cell,it will be necessary to visualize auxin abundance and dynamicson the cellular level.

MATERIALS AND METHODS

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ABSTRACT
RESULTS
DISCUSSION
CONCLUSIONS
MATERIALS AND METHODS
LITERATURE CITED

Cell Line

The tobacco (Nicotiana tabacum) cell line VBI-0 derives fromstem pith explants of cv Virginia Bright Italia (Opatrn $y$ andOpatrná, 1976) and was cultivated in slightly modifiedHeller's liquid medium (Heller, 1953) supplemented with thesynthetic auxins 2,4-D (4.5 µM; Fluka Chemie AG, Neu-Ulm,Switzerland) and NAA (5.4 µM; Sigma-Aldrich, St. Louis).Cells were subcultured every 3 weeks (Petrá $s$ ek et al.,1998), inoculating 4 mL of stationary cells (5 x 10⁶ cells mL^-1)into 30 mL of fresh medium in 100-mL Erlenmeyer flasks, andincubation at 25°C in darkness on an orbital shaker (KS250basic, IKA Labortechnik, Staufen, Germany) at 120 rpm (1.8 cmdiameter).

Morphometry

Aliquots (0.25 mL) from each sample were stained with 1:100(v/v) Rhodamin-G6-chloride for 10 min on a topover-shaker anddestained twice for 5 min in 1 mL of culture medium. Cells werethen immediately viewed under a confocal laser scanning microscope(DM RBE, Leica, Bensheim, Germany) using a one-channel scanwith an argon-krypton laser at 568-nm excitation, a 575-nm beamsplitter, and 590-nm emission filters. Image stacks were recordedat 200-fold magnification along the z axis, and cell lengthand width were determined from the central section of the cellsusing the Scion Image Software (Scion, Frederick, MD). For eachdata point, 300 individual cells from three independent experimentalseries were scored.

Determination of Cell Viability and Division Pattern

Cell viability was assayed by the Trypan Blue dye exclusiontest (Phillips, 1973). Aliquots (0.5 mL) from each sample werestained with 0.4% (w/v) Trypan Blue solution (Sigma-Aldrich)at a ratio of 1:100 (v/v). After incubation for 3 min, the frequencyof the unstained viable cells was scored as well as the numberof cells per individual file using a Fuchs-Rosenthal hematocytometerunder a bright-field microscope. For each single sample, 10³cells were scored.

Auxin Starvation and Refeeding Experiments

For the auxin starvation experiments, stationary cells (culturedfor 21 d under standard conditions) were inoculated into 30mL of the usual culture medium that was void of exogenous auxins.In the refeeding experiments, the inoculum was first culturedfor 2 d in hormone-free medium, and the hormones were then addeddirectly into the auxin-starved cultures starting from filter-sterilizedstocks of 5 mg mL^-1 NAA and 5 mg mL^-1 2,4-D dissolved in 96%(v/v) ethanol. An equal volume of sterile 96% (v/v) ethanolwas added to the control samples.

In Silico Simulation

Simulations were performed with the MATLAB software and wererun both on a DEC workstation and a Windows PC with identicalresults. The algorithm of the model is detailed in "Results".The MATLAB source code of the program is available from theauthors on demand.

NPA Treatments

NPA was synthesized by Dr. Wolfgang Michalke (Albert-Ludwigs-UniversitätFreiburg, Institut für Biologie III, Freiburg, Germany)according to Thompson et al. (1973). NPA was added at inoculationfrom a filter-sterilized stock of 34 mM NPA in dimethyl sulfoxideto final concentrations of 5 or 50 µM. Equal aliquotsof sterile dimethyl sulfoxide were added to the control samples.

Scoring Division Events along Individual Cell Files

Cells were inoculated in standard conditions with auxin or withauxin in combination with 5 µM of NPA. Four days afterinoculation, aliquots were fixed in Carnoy fixative (3:1 [v/v]96% [v/v] ethanol:acetic acid) plus 0.5% (w/v) Triton X-100and stained with Hoechst 33258 (Molecular Probes, Leiden, Netherlands).Randomly selected files were recorded under a fluorescent microscope(Axioskop 2, Zeiss, Oberkochen, Germany) using a 4',6-diamino-phenylindolefilter set (365-nm excitation, 395-nm beam splitter, and 397-nmemission; Zeiss). The observed patterns were grouped accordingto the cell number and the localization of cell division asspecified in "Results" with a minimum of 50 files scored foreach data point.

ACKNOWLEDGMENTS

NPA was kindly provided by Dr. Wolfgang Michalke (Albert-Ludwigs-UniversitätFreiburg).

Received June 2, 2003; returned for revision July 12, 2003; accepted August 17, 2003.

FOOTNOTES

Article, publication date, and citation information can be foundat www.plantphysiol.org/cgi/doi/10.1104/pp.103.027953.

¹ This work was supported by the Volkswagen-Foundation Nachwuchsgruppen-Programme(grants to P.N. and B.B.).

^* Corresponding author; e-mail prisca.campanoni{at}biologie.unifreiburg.de; fax 49–761–203–2612.

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Auxin Transport Synchronizes the Pattern of Cell Division in a Tobacco Cell Line1

Auxin Transport Synchronizes the Pattern of Cell Division in a Tobacco Cell Line¹