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Plant Physiol, September 2001, Vol. 127, pp. 119-130
Cytoplasmic pH Dynamics in Maize Pulvinal Cells Induced by
Gravity Vector Changes1,[w]
Eva
Johannes,*
David A.
Collings,2
Jochen C.
Rink,3 and
Nina Strömgren
Allen
Department of Botany, Box 7612, North Carolina State University,
Raleigh, North Carolina 27695-7612
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ABSTRACT |
In maize (Zea mays) and other grasses, changes in
orientation of stems are perceived by pulvinal tissue, which responds
to the stimulus by differential growth resulting in upward bending of
the stem. The amyloplast-containing bundle sheath cells are the sites
of gravity perception, although the initial steps of gravity perception
and transmission remain unclear. In columella cells of Arabidopsis
roots, we previously found that cytoplasmic pH (pHc) is a
mediator in early gravitropic signaling (A.C. Scott, N.S. Allen
[1999] Plant Physiol 121: 1291-1298). The question arises whether
pHc has a more general role in signaling gravity vector
changes. Using confocal ratiometric imaging and the fluorescent pH
indicator carboxy seminaphtorhodafluor acetoxymethyl ester acetate, we
measured pHc in the cells composing the maize pulvinus. When stem slices were gravistimulated and imaged on a horizontally mounted confocal microscope, pHc changes were only apparent
within the bundle sheath cells, and not in the parenchyma cells. After turning, cytoplasmic acidification was observed at the sides of the
cells, whereas the cytoplasm at the base of the cells where plastids
slowly accumulated became more basic. These changes were most apparent
in cells exhibiting net amyloplast sedimentation. Parenchyma cells and
isolated bundle sheath cells did not show any gravity-induced
pHc changes although all cell types responded to external
stimuli in the predicted way: Propionic acid and auxin treatments
induced acidification, whereas raising the external pH caused
alkalinization. The results suggest that pHc has an important role in the early signaling pathways of maize stem gravitropism.
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INTRODUCTION |
The vector of the gravitational
force is one of the main cues that determines the spatial orientation
of plant organs (Masson, 1995 ; Tasaka et al., 1999; Kiss, 2000). A
plant's ability to respond to the direction of gravity, the process of
gravitropism, ensures the correct positioning of the seedling after
germination and also enables mature plants to correct their position
after a forced reorientation, e.g. by strong wind. In most cases,
gravity perception occurs in specialized cells that contain dense
particles, such as starch-filled plastids (amyloplasts; Sack, 1997;
Tasaka et al., 1999). These shift their location within the cell when
the normal plant orientation gets disturbed, thereby generating a cellular signal that sets up a chemical gradient between top and bottom
of the plant organ resulting in differential growth.
Whereas the gravity-induced growth response in plants is well
documented, little is known about the mechanism of gravity perception and the nature of the early steps of the signaling cascade. Research has focused on gravity perception in roots that occurs in
amyloplast-containing root cap cells. Some of the earliest
measurable responses induced by gravistimulation occur in and
around these cells, and include complex changes in cytosolic and
apoplastic pH (Scott and Allen, 1999; Fasano et al., 2001), changes in
plasma membrane potential (Sievers et al., 1995), and the induction of
ion flux changes around the root cap (Behrens et al., 1985;
Björkman and Leopold, 1987). It is intriguing that in
Arabidopsis, cytoplasmic pH (pHc) changes occur
only in the inner collumella cells of the root cap (Scott and Allen,
1999; Fasano et al., 2001), which are the most competent in gravity
perception (Blancaflor et al., 1998). Furthermore, artificial
modification of pHc alters the gravitropic
response (Scott and Allen, 1999; Fasano et al., 2001). This suggests
that pHc changes play a key role in
gravity-induced signaling.
Induced changes in pHc occur in response to a
wide array of stimuli, apart from gravitropism, including phytohormones
(Felle, 1988a; Gehring et al., 1990a, 1994; Beffagna et al., 1994),
light (Felle and Bertl, 1986; Okazaki et al., 1994), Nod factors (Allen et al., 1994; Felle et al., 1996), and other elicitors (Mathieu et al.,
1996). Furthermore, protons are implicated as a mediator in plant
signal transduction (Felle, 1989; Guern et al., 1992; Roos et al.,
1998; Zhou et al., 2000). Whether the gravity-induced pHc changes measured in roots have a general role
in gravity perception in plants is still unknown because
pHc changes in shoots have only been linked to
the later phases of the gravitropic response (Gehring et al., 1990b).
The objective of this study was to elucidate whether gravity-induced
changes in pHc occur in shoot tissues that are
specialized in gravity perception such as the maize (Zea mays) pulvinus.
The stem pulvinus of maize is a disc-shaped tissue that is located
above each stem node and has a specific role in both gravity perception
and the bending response (Collings et al., 1998; for review, see
Kaufman et al., 1987, 1995). When the stem is placed horizontally, amyloplast sedimentation occurs in bundle sheath cells,
and a growth response follows characterized by cell elongation specifically within the pulvinal cells, causing the stem to bend upwards. Pulvinal cells retain the capacity to elongate in the presence
of an appropriate stimulus even after the surrounding tissue has fully
differentiated, allowing the normal growth responses to be spatially
and temporally separated from those induced by changes in the gravity
vector (Collings et al., 1998). These properties make the maize
pulvinus an ideal system to investigate biochemical (Winter et al.,
1997; Perera et al., 1999), structural, and physiological changes at
the cellular level (Collings et al., 1998) during gravitropism.
In this study, we focused on early gravity-induced responses and
monitored pHc changes in pulvinal cell regions
after rotation on a horizontally mounted confocal microscope using the
ratiometric pH indicator carboxy seminaphtorhodafluor acetoxymethyl
ester acetate (SNARF-1 AM). We compared the responses of
amyloplast-containing bundle sheath cells with those of parenchyma
cells to find out whether pHc changes similar to
those found in Arabidopsis root cells occur and whether they are
associated with the cells that perceive the gravity stimulus.
Furthermore, we dissected the pHc responses of
base and side regions (relative to the gravity vector) of the
stimulated cells and compared cells that exhibited amyloplast sedimentation with those that did not. That pHc
changes were most pronounced in cells in which there was net amyloplast
sedimentation, with these changes confined to specific sites within
these cells, is discussed in light of current models for the mechanism
of gravity perception and the rising importance of
pHc as a messenger in cellular signaling.
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RESULTS |
Specimen Preparation and Dye Loading
The pulvinus is a region of cells found between the differentiated
node and elongated cells of the internode. The unelongated pulvinal
cells surrounding the vascular strands are of two types. Several layers
of bundle sheath cells occur immediately adjacent to the vascular
tissue. Potassium iodide staining confirms that these cells contain
starch-filled amyloplasts, and that these plastids are effectively
confined to the pulvinus (Fig. 1, A-C). Surrounding the bundle sheath are numerous files of ground
parenchyma.
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Figure 1.
Cellular organization of the pulvinus. The image
in A was taken of a hand cross section on an upright microscope
(Zeiss, Thornwood, NJ) equipped with a CCD camera (Hamamatsu,
Bridgewater, NJ) and the Image 1 software system (Universal Imaging,
West Chester, PA), whereas the images shown in B and C were taken of
longitudinal hand sections using a dissecting microscope (Leica,
Wetzlar, Germany) and a Hamamatsu color CCD camera. Bars in A through C
represent 50, 1,000, and 200 µm, respectively. B, Bundle sheath cells
with amyloplasts (stained with 0.2% [w/v] iodine in 5% [w/v]
KI). C, Collenchyma, P, parenchyma; Phl, phloem; V, vascular
bundle; X, xylem.
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To measure cytosolic pH (pHc) in maize pulvinal
cells, both before and after gravistimulation, we investigated several
specimen preparation protocols. Two methods proved satisfactory for
imaging on a sideways-mounted microscope. In the first method, mild
enzymatic digestion of cell wall material resulted in the isolation of
long files of healthy cells that showed vigorous cytoplasmic streaming. These files could either be parenchymal cells or amyloplast-containing bundle sheath cells. When files of bundle sheath cells were incubated in a vertical position for 30 min and then gravistimulated, net amyloplast sedimentation occurred over the next several minutes (Fig. 2, A-C; for video sequence, see
www.plantphysiol.org). In these cells, the average rate of
plastid sedimentation was visibly slower than the streaming velocities
for individual amyloplasts. However, amyloplast sedimentation in files
of bundle sheath cells, as shown in Figure 2, A through C, was a
relatively rare event, seen in only two out of 15 independent
rotations. The second specimen preparation method involved taking 0.3- to 0.5-mm thick longitudinal sections through the pulvinus. Cells in
these preparation also showed vigorous cytoplasmic streaming, but it is
significant that sections were more likely to show amyloplast
sedimentation following gravistimulation (Fig. 2, D-F; for video
sequence, see www.plantphysiol.org), with this being seen in
67% of sections (n = 12).
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Figure 2.
Dynamics of amyloplast sedimentation. A through C,
Amyloplast sedimentation in isolated files of bundle sheath cells.
Amyloplasts follow the tracks of intracellular particle movement as
well as the path predicted by physical parameters such as plastid
density and cytosolic viscosity leading to net sedimentation of
plastids to the new bottom of the cell. A, Thirty seconds before
rotation of cell files through 180°. QuickTime movie located at
www.plantphysiol.org. B, Thirty seconds after rotation. C,
Seven minutes after rotation. D through E, Plastid
sedimentation in bundle sheath cells of maize. Ratio images
E2 (620-670 nm)/E1
(550-600 nm) of SNARF-1 AM-loaded longitudinal pulvinal sections,
excitation 514 nm. D, Before rotation; E, 2 min after rotation by
90°. QuickTime movie located at www.plantphysiol.org. F, 12 Minutes after rotation, bar = 50 µm; v, vascular tissue; b,
bundle sheath cells; p, parenchyma cells.
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To measure pHc, both before and after
gravistimulation, we also investigated numerous ratiometric pH
indicators. The most promising dye was carboxy seminaphtorhodafluor
(SNARF-1) because of a range of technical issues, and because when
excited at 514 nm, pulvinal cells showed little autofluorescence at the
emission peaks of SNARF's acidic and basic forms, recorded at 550 to
600 and 620 to 670 nm, respectively. After 1 h of incubation in
the membrane permeant AM ester form of SNARF (10 µM), dye
loaded predominantly into the cytoplasm and was largely excluded from
the vacuole. However, SNARF fluorescence was also observed within
amyloplasts. SNARF loaded rapidly into isolated file cells, whereas in
tissue sections the dye loaded first into the vascular tissue then
proceeded into bundle sheath cells and finally was found in the
parenchyma. Attempts to load SNARF via the vascular bundles into
excised pulvini without prior sectioning failed.
pHc Measurements in Maize Pulvinal Cells: Effects of
Weak Acids, External pH Changes, and Indole Acetic Acid (IAA)
To determine the reliability of our confocal ratiometric imaging
system, we measured pHc with SNARF-1 in
non-gravistimulated file cells and tissue slices, observing both bundle
sheath and parenchyma cells, and determined whether these cells
responded to known stimuli in the normal way. Ratios of the two
emission intensities (620-670 nm/550-600 nm) were generally stable in
non-stimulated cells for the duration of experiments. In vitro
calibrations with dextran-linked SNARF (10 kD) were carried out after
each experiment. In most cases, these in vitro calibrations gave
calculated pHc values of about pH 6.6 (or lower)
that were more acidic than the pHc values
reported in earlier studies (Smith and Raven, 1979; Kurkdjian and
Guern, 1989; Guern et al., 1991, 1992). However, the cells appeared
healthy, showing normal intracellular particle movement, and could
react to weak acid and other treatments with similar ratio shifts as
those cells whose calibrations reported a resting
pHc around 7. Thus, results are presented in this
paper as changes in ratio rather than changes in
pHc, with an increase in ratio reflecting
alkalinization and a decrease in ratio reflecting acidification.
Adjustments in the photomultiplier settings for the two emission
windows led mainly to a parallel ratio shift in the calibration curve
and only had a small effect on the slope of the pH dependence (Fig.
3). Therefore, the change in ratio obtained from data sets with different starting ratios can be compared
even though the pH dependence is not linear. It should, however, be
noted that the bulk of the data were obtained within a more narrow
range of photomultiplier adjustments than those depicted in Figure
3.
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Figure 3.
In vitro calibrations with 50 µM
SNARF-1 dextran (10 kD): pH dependence of emission intensity ratio
E2 (620-670 nm)/E1
(550-600 nm) for different photomultiplier settings. An increase in
the photomultiplier setting for E2 leads to an
approximately parallel shift in the ratio values with only a slight
increase in slope.
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In vivo calibrations with nigericin in the presence of high
K+ (Vercesi et al., 1994) are not reported in
this paper because such experiments did not lead to sustained ratio
changes and required complex solution changing that could not be
performed for the majority of measurements that were made with a
sideways-mounted microscope.
To test whether SNARF-1 AM can be used reliably to monitor
pHc changes in maize pulvinal cells, a range of
conditions were applied that are known to increase or decrease
pHc in a large variety of plant cells. When
subjected to 0.5 mM propionic acid applied at an external
pH of 5.5, bundle sheath cells from tissue sections responded with a
drop in ratio by  r =  0.171 ± 0.009 (n = 16; acidification, Fig. 4A). Streaming
remained visibly unaffected in these cells. After removal of the weak
acid, the ratio returned to the resting value, and occasionally showed
a transient overshoot to more positive values (alkalinization). The
kinetics with which these ratio changes occurred are comparable to the
weak acid-induced pHc changes measured with
ion-selective microelectrodes (Felle, 1987; Frachisse et al., 1988) and
31P NMR spectroscopy (Guern et al., 1986) in a
variety of other plant cells. Conditions that evoke alkalinizations
were also tested. It is known from previous reports that changes in
external pH lead to corresponding changes in pHc
by about 0.1 pHc unit per pH unit change in
external pH (for review, see Smith and Raven, 1979; Felle, 1988b).
Figure 4B shows the response of pulvinal bundle sheath cells to a
change in external pH from 5.5 to 9.0 that caused a rise in the ratio
(alkalinization) by r = 0.077 ± 0.008 (n = 18).
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Figure 4.
Ratio changes E2 (620-670
nm)/E1 (550-600 nm) in maize pulvinal cells from
tissue slices following: A, application of 0.5 mM propionic
acid; B, a change in external pH from pH 5.5 to 9.0; and C, addition of
0.1 mM IAA. Representative measurements are shown and
statistics are given in the text. Substances were applied in buffer C
(pH 5.5). Increase in ratio reflects alkalinization, decrease in ratio
reflects acidification.
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The phytohormone auxin (e.g. IAA), which plays an important role in the
gravity-induced differential growth response (Evans, 1991; Estelle,
1996), also evoked ratio changes in maize pulvinal cells (Fig. 4C).
Application of 0.1 mM IAA evoked a transient rise in the
ratio (alkalinization) by r = 0.027 ± 0.004 (n = 12), which was apparent in 72% of analyzed
recordings. This was followed by a drop in r (acidification) by
0.175 ± 0.015 (n = 18). IAA concentrations of
10 µM IAA caused a rise in r
(alkalinization) by 0.040 ± 0.002 (n = 3, one
data set), which returned to the resting level within about 10 min
(data not shown). Although the acidification evoked by higher IAA
concentrations might in part be attributable to a weak acid effect, the
initial alkalinization could reflect a change in membrane transport
activity. Previous studies concerning pHc changes
in maize coleoptiles induced by auxins (1 µM)
showed either an oscillatory pattern of pHc
changes (Felle, 1988a) or a sustained acidification by 0.1 to 0.2 pH
units (Gehring et al., 1990a).
Although the data shown in Figure 4 relate to inducible
pHc changes in bundle sheath cells from tissue
slices, we observed similar changes in the emission ratio in isolated
files of bundle sheath cells (Fig. 5A),
and in parenchyma cells in both slices and isolated files (data not
shown).
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Figure 5.
Ratio changes E2 (620-670
nm)/E1 (550-600 nm) in isolated pulvinal cell
files following: A, application of 1 mM propionic acid; and
B, after rotation by 90°. Representative measurements are shown.
Substances were applied in buffer B (pH 5.5). The average ratio change
was: A, 0.214 ± 0.019 (n = 10) in response to
propionic acid; and B, 0.003 ± 0.005 (n = 10)
after rotation.
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Gravistimulation Experiments Demonstrate pHc Changes in
Bundle Sheath Cells
Protocols for isolation of bundle sheath cell files were developed
because these cells provide a much more favorable system for high
resolution imaging than pulvinal slices. Although it was possible to
measure pHc changes in this system in response to
propionic acid (Fig. 5A), gravistimulation never led to any visible
change in the ratio (Fig. 5B). Because plastid sedimentation was only
rarely retained in isolated cell files, it might be argued that the
lengthy isolation and dye loading procedure, the potential for
cytoskeletal reorganization, or the loss of cell wall material and cell
positioning information, led to disruption in cell function that might
have affected early steps in the signaling cascade.
In longitudinal stem sections that were loaded with SNARF-1 AM,
rotation by 90° resulted in significant ratio changes, indicative of
pHc changes, in cells that contained sedimentable
amyloplasts, as depicted in Figure 6, B
and C, and summarized in Table I. Parenchyma cells that lack amyloplasts provided an ideal control for
these experiments because they did not exhibit any notable change in
the emission ratio after turning (Fig. 6A) either at the base of the
cell or at the side of the cell (Table I). In bundle sheath cells that
showed amyloplast sedimentation, cytoplasmic regions at the sides of
the cells often responded with a drop in ratio (acidification), whereas
regions at the base of cells showed a rise in ratio (alkalinization;
Figs. 6B and 7). When cytoplasmic areas
of whole cells were measured, the acidification often prevailed. In
about 12% of cases, a transient alkalinization was followed by an
acidification at the sides of cells but not at the base
(Fig. 6C). Rotation by 360° (no gravistimulation) did not
elicit any significant changes in the pHc of
bundle sheath cells, suggesting that touch responses that might occur
during rotation do not contribute to the ratio change (Fig.
6D).
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Figure 6.
Ratio changes E2 (620-670
nm)/E1 (550-600 nm) in maize pulvinal cells from
tissue slices before and after rotation by 90° (A-C) and 360° (D).
A, Response of parenchyma cells (no amyloplasts); B, typical response
of bundle sheath cells with amyloplast sedimentation base region of
cells ( ) and side regions of cells ( ); C, transient response
measured in side regions of bundle sheath cells showing amyloplast
sedimentation, observed in 12% of recordings; D, response of bundle
sheath cells to a full 360° rotation. Average values ± SEs of representative data sets are shown and statistics
are given in Table I.
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Table I.
pH ratio changes in stem slices following
gravistimulation
t, Student's t distribution; P,
significance level; nd, not determined as invalid comparison.
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Figure 7.
Histograms summarizing data represented in Figure
6B. The rate of ratio change after rotation was determined over a 15- to 20-min period using linear regression and least-square fit. Data
obtained from bundle sheath cells showing amyloplast sedimentation
(light shaded bars) were compared with those in which no amyloplast
sedimentation occurred (dark shaded bars). A, Ratio changes in base
regions; B, ratio changes in side regions. The maximum rates of ratio
changes observed in data sets obtained from parenchyma cells
(exemplified in Fig. 6A) fell within the range of r = ±0.0025
min 1 and were designated as no response. The
bin width was r = 0.005 min1; however,
rates of acidification larger than r = 0.0125
min1 were included in the left column.
Statistics are given in Table I.
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In contrast to these observations of changes in
pHc in bundle sheath cells that showed amyloplast
sedimentation, bundle sheath cells that failed to show amyloplast
sedimentation within 30 min after rotation lacked pronounced changes in
pHc. The results are summarized in the histograms
presented in Figure 7 and the statistics in Table I. In bundle sheath
cells not exhibiting plastid sedimentation, a higher percentage of
cells showed no pHc response compared with cells
that showed sedimentation; furthermore, alkalinization did not occur at
the base of cells. The magnitude and rate of acidification measured in
side regions was also markedly lower than that measured in cells with
sedimenting plastids (at the 90% confidence interval; Fig. 7B, Table
I).
In Table I, the rate of ratio change after rotation was compared
statistically (Student's t test for two independent
samples) for data sets obtained from side and base regions of
parenchyma cells, and bundle sheath cells with and without plastid
sedimentation. Bundle sheath cells showed a significantly different
response than parenchyma cells (control), except for base regions of
bundle sheath cells not exhibiting plastid sedimentation, which
responded in a manner similar to the control. When cells with and
without plastid sedimentation were compared the responses measured in the base regions were significantly different (95% confidence interval) between the two data sets, whereas those measured at the
sides of the cells were different at the 90% confidence interval. Bundle sheath cells that were rotated 360° did not exhibit
significant ratio changes (Fig. 6D) and their response was
significantly different from bundle sheath cells that were rotated
90°.
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DISCUSSION |
pHc Measurements in Pulvinal Cells with SNARF-1
AM
Lipophilic derivatives of ion sensitive fluorescent dyes such as
SNARF-1 AM can permeate intracellular organelles and cause errors in
the determination of cytoplasmic ion concentrations (Fricker et al.,
1993; Williams et al., 1993; Roos, 2000). In pulvinal bundle sheath
cells, dye accumulation into the central vacuole is minimal during the
first 60 to 90 min following SNARF-1 AM incubation. However, a large
amount of dye accumulates in amyloplasts, an observation previously
noted in barley (Hordeum vulgare) pulvinal cells
where amyloplasts accumulate fluorescence following esterase cleavage
of fluorescein diacetate (Dayanandan et al., 1982). The result of this
dye accumulation is frequent signal saturation from amyloplasts under
the conditions used for our experiments. To minimize errors in the
pHc measurements arising from SNARF-1 AM-loaded
amyloplasts, we used the following precautions. If possible, cytoplasmic regions free of amyloplasts were selected for measurement, and a thresholding method was used to determine the emission ratio eliminating most of the amyloplast-derived signal.
Quantification of Changes in the Emission Ratio
Because in vitro calibrations did not report reliable
pHc values, it was difficult to quantify the
observed ratio changes. However, taking into account measurements that
reported normal pHc values when compared with in
vitro calibration, and by comparing our results obtained with weak
acids and external pH changes with those obtained by other
investigators, we can estimate the range within which the
gravity-induced pHc changes might fall. A
lipohilic weak acid, propionic acid, was used to induce a cytosolic
acidification. In the absence of a transporter, lipophilic weak acids
enter the cell solely in their undissociated form, and it is this
concentration that determines the magnitude of the pH change in a
particular system (Frachisse et al., 1988; Felle and Johannes, 1991).
The responses to lipophilic weak acids show variability among different plant species that could be due to variation in the buffer capacity of
the cytoplasm and the ability of the plant to regulate its pHc (Smith and Raven, 1979; Kurkdjian and Guern,
1989; Guern et al., 1991, 1992).
Bundle sheath cells from tissue slices responded to 0.5 mM
propionic acid (0.1 mM undissociated acid) with a drop in
ratio (acidification) by r = 0.171 ± 0.009 (n = 16; Fig. 4A). Compared with in vitro calibrations
that showed reliable pHc values, these changes
fell within a range of 0.4 to 0.5 pH units and were similar to those
measured in Riccia fluitans after addition of the same concentration of weak acids (Frachisse et al., 1988). Changes in
external pH are known to evoke corresponding changes in
pHc by about 0.1 unit per 1 unit change in
extracellular pH in a large variety of plants (for review, see Felle,
1988b). In pulvinal bundle sheath cells, a change in external pH from
5.5 to 9 evoked a rise in the emission ratio by r = 0.077 ± 0.035 (Fig. 4B) that reflects an alkalinization by approximately
0.35 pH unit.
Amyloplast Redistribution following Gravistimulation Induces
pHc Changes
We argue that the observed changes in emission ratio seen
following gravistimulation indicate that pHc
changes are a genuine consequence of amyloplast relocation following
gravistimulation. Although measurement errors cannot be excluded, we
base this contention on the following observations. Bundle sheath and
parenchyma cells in both tissue slices and isolated files respond
similarly to propionic acid and IAA, yet ratio changes following
turning were only seen in bundle sheath cells in tissue slices.
Furthermore, gravity-induced changes strongly correlated with
amyloplast sedimentation. In 25% of bundle sheath cells exhibiting
amyloplast sedimentation, no change in ratio was observed although
other cells within the same preparation did show a response. This
indicates that sedimentation per se does not change the emission ratio.
In cells that did respond to gravistimulation, the ratio change
persisted over the measuring period after most plastids had settled to
the bottom of the cell. Again, this supports our view that the measured
ratio changes reflect pHc changes induced by gravity.
Gravity-Induced pHc Changes: An Early Step in Gravity
Perception?
The present investigation shows that gravity induces
pHc changes in the amyloplast-containing bundle
sheath cells of the maize pulvinus, indicating that
pHc changes might have a generally important role
in early gravity-induced signaling. Average ratio changes evoked in
bundle sheath cells (with plastid sedimentation) within 30 min
following rotation were about r = 0.06 (alkalinization) in
bottom regions and r = 0.15 (acidification) in side regions (see Table I and Fig. 6B). Taking into account the considerations discussed in the previous section, the gravity-induced ratio changes are likely to reflect pHc changes in the range of
0.3 to 0.5 pH units. These changes are similar to stimulus-induced
pHc changes reported in other plant systems where
changes in pHc have a wide array of physiological
effects in plant cells and can act as mediators in many signal
transduction pathways (Felle, 1989; Guern et al., 1992; Putnam, 1998).
Changes in pHc affect proton translocation by
pumps and carriers (Felle and Johannes, 1991; Portillo, 2000), and can
modulate the activity of various anion (Schulz-Lessdorf et al., 1996;
Johannes et al., 1998) and cation (Grabov and Blatt, 1997; Lacombe et
al., 2000) channels.
The sequence of signaling events that follow gravistimulation, and the
involvement of pHc, remain largely unknown.
However, in root gravitropism, many of the earliest measurable
gravity-induced effects involve ionic fluxes in and around the root
cap. These include membrane potential and ion flux measurements that
showed gravity-induced hyperpolarizations and proton fluxes indicative of stimulation of the plasma membrane H+ ATPase
(Behrens et al., 1985; Björkman and Leopold, 1987; Sievers et
al., 1995). Fasano et al. (2001) also observed a uniform acidification of the Arabidopsis root cap apoplast from pH 5.5 to 4.5 within 2 min of
gravistimulation. However, because the plasma membrane H+ pump can effect pHc
changes as well as respond to them, it is difficult to tell which of
these two early responses might come first.
Early Events in Gravisignaling and the Role of
pHc
Three investigations have now shown that
pHc changes are a key player in early
gravity-induced signaling in root caps. First, Scott and Allen
(1999) showed that microinjection of the pH-sensitive dye
1',7'-bis-(2-carboxymethyl)-5-(and-6)-carboxyfluorescein
into gravity-perceiving root cap cells of Arabidopsis revealed a rapid alkalinization in tier 2 cells and a slower acidification in tier 3 cells (Scott and Allen, 1999), the sites with the greatest competence for gravity perception (Blancaflor et al., 1998). When
pHc changes were induced solely within the root
cap by various pHc modifiers, the gravitropic
response was also altered, with acidification of the columella causing
enhanced bending, whereas alkalinization resulted in inhibition of
bending. These observations were expanded by Fasano et al. (2001)
who demonstrated, using both dye
1',7'-bis-(2-carboxymethyl)-5-(and-6)-carboxyfluorescein-dextran microinjection and the constitutive expression of a pH-sensitive green fluorescent protein, that rapid alkalinization occurred in the
Arabidopsis columella following gravistimulation. Furthermore, in a
starchless Arabidopsis mutant, where plastid sedimentation and bending
were reduced, pHc changes were also markedly
smaller (Fasano et al., 2001). Taken together with our observations in the pulvinus, these results indicate that pHc
changes might have a generally important role in early gravity-induced signaling.
Concurrent with rapid pHc changes in the
pulvinus, gravity also induces rapid changes in the inositol phosphate
metabolism in pulvini of maize and oats (Avena
sativa) beginning within minutes of gravistimulation and resulting
in oscillations of phosphatidylinositol 4,5-bisphosphate and inositol
1,4,5-trisphosphate (IP3; Perera et al., 1999,
2001). Increases in the second messenger IP3 are known to open Ca2+ channels in the vacuolar
membrane of plant cells (Alexandre et al., 1990; Allen et al., 1995),
and suggest a role of cytosolic free Ca2+
([Ca2+]c) in the
gravity-induced signaling cascade. Although direct measurements of
[Ca2+]c in
gravity-perceiving cells in the root cap of Arabidopsis failed to
reveal such changes in response to gravistimulation (Legué et
al., 1997), a role for
[Ca2+]c has long been
implicated by indirect experimental evidence (for review, see Chen et
al., 1999). It is conceivable that
[Ca2+]c changes occur and
act locally in cellular microdomains and that high resolution imaging
techniques in conjunction with more sensitive
Ca2+ dyes are required to make them detectable.
However, several significant questions remain unclear. First, how does
amyloplast sedimentation cause changes in pHc,
phophatidylinositol 4,5-bisphosphate/IP3 levels,
and possibly also
[Ca2+]c, and how are
these changes linked? Second, how is this signal integrated from the
cellular to the tissue level, such that pHc changes visible in the majority of cells with amyloplast sedimentation can generate a chemical gradient between the top and bottom of the
plant organ that results in differential growth and the bending response? And third, how does auxin, thought to be a key regulator of
the bending response (Evans, 1991; Estelle, 1996), fit into this
system? One possible integrating system that could satisfy all these
questions would be the actin cytoskeleton.
Although subject to some debate (for review, see Balu ka and
Hasenstein, 1997), it has now been shown that the amyloplasts in the
columella cells of the root cap from various plant species are
surrounded by endoplasmic reticulum and actin filaments (Collings et
al., 2001). In a similar manner, the dynamics of amyloplast streaming
in the maize pulvinus (this study), and amyloplast motility in other
gravitropic tissues (Sack and Leopold, 1985), indicate extensive
interactions between amyloplasts and the actin cytoskeleton. Thus, it
is possible that while moving to the new cell bottom, amyloplasts might
interact with actin and/or membranes, thereby eliciting
pHc changes in cellular microdomains. The actin
cytoskeleton has several features that make it suitable for regulating
gravitropic signaling and response generation. Actin-binding proteins
that regulate the equilibrium between F actin and G actin, such as actin-depolymerizing factor, are modulated by pHc
with depolymerization occurring at higher pHc
values (Gungabissoon et al., 1998; Kovar and Staiger, 2000). Various
actin-binding proteins, including actin-depolymerizing factor and
profilin (Gibbon and Staiger, 2000; Kovar and Staiger, 2000), also
interact extensively with signaling by phospholipids. Furthermore,
actin modulates auxin transport through its regulation of the auxin
efflux carrier (Muday, 2000).
The current state of knowledge suggests that changes in membrane
transport (Behrens et al., 1985; Björkman and Leopold, 1987; Sievers and Busch, 1992; Sievers et al., 1995), actin dynamics (Collings et al., 2001), and phophoinositol metabolism (Perera et al.,
1999, 2001) are early responses to a change in the gravity vector. It
is likely that the observed pHc changes have an
integral role in the gravity-induced signaling cascade because
pHc alone or in conjunction with
[Ca2+]c modulates the
activity of membrane transport proteins (Felle and Johannes, 1991;
Schulz-Lessdorf et al., 1996; Grabov and Blatt, 1997; Johannes et al.,
1998; Lacombe et al., 2000; Portillo, 2000), cytoskeletal
polymerization (Gungabissoon et al., 1998; Kovar and Staiger, 2000),
organization of the endoplasmic reticulum (Quader and Fast, 1990), and
enzymatic reactions (Putnam, 1998; Paterson and Nimmo, 2000),
all of which are likely to play a role in the initial steps of
gravity-induced signal transduction. It will be a challenge for future
investigators to elucidate how the gravity signal is integrated and to
dissect the sequence of events leading from gravity perception to the
gravitropic response. Progress in this field will be aided by the
availability of mutants impaired in perception or transduction of the
gravity signal (Sedbrook et al., 1999; Firn et al., 2000) and through
the use of more refined techniques for visualization of ionic changes
in cellular microdomains using pH-sensitive green fluorescent protein
constructs that can be targeted to specific cellular compartments
(Miesenböck et al., 1998).
| |
MATERIALS AND METHODS |
Plant Material
Maize (Zea mays) plants (line 3183; Pioneer, Des
Moines, IA) were grown in greenhouses (22°C -27°C), three plants
per 22-cm pot. Pulvini 2 and 3 (the second and third pulvinus from the
base of the stem) from 5- to 6-week-old plants were used for all
experiments. These pulvini exhibit the strongest response to
gravitistimulation, and lie adjacent to internodes that have ceased
elongation (Collings et al., 1998).
Isolation of Stem Slices
Longitudinal hand sections, approximately 0.2 to 0.5 mm thick,
were made with a razor blade through the pulvinal regions of pulvini 2 and 3. Replicate sections were stained to reveal and confirm the
location of starch-containing amyloplasts with 0.2% (w/v) iodine in
5% (w/v) KI (10 min).
Isolation of Cell Files
Pulvini 2 and 3 from one or several maize plants were harvested,
chopped in 1- to 2-mm3 pieces, and incubated for 40 to 50 min in cell wall-digesting enzymes (1% [w/v] Cellulase YC, 0.1%
[w/v] Pectolyase Y23, 0.5% [w/v] bovine serum albumin, and
0.3 M mannitol in Murashige and Skoog medium, pH 5.3).
Following enzyme digestion, the tissue was mechanically disrupted by
gentle stirring and tapping at the tissue pieces with a glass rod to
release files of cells. Buffer A {100 mM KCl, 0.285 M mannitol, and 10 mM PIPES
[piperazine-N,N'-bis(2-ethanesulfonic acid)]/KOH, pH 6.8} was added
and the suspension was allowed to sediment for 30 to 45 min at
1g (4°C), and this fast-sedimenting debris removed. Files
of cells were recovered by further sedimentation of the suspension at
1g (4°C) over the next several hours. The pelleted
cell files then were resuspended in buffer A to remove residual enzyme
and again pelleted at 1g (4°C) for several hours. Centrifugation to accelerate the recovery of cell files was not feasible because low-speed centrifugation (<80g)
ruptured the amyloplast-containing bundle sheath cells.
Ester Loading of SNARF1-AM and Mounting of Cells
Cell files were incubated for 60 min in 10 µM
SNARF1-AM (0.8 mL of buffer A and 1% [v/v] dimethyl
sulfoxide, 22°C). Cell files settled at the bottom of the
Eppendorf tube and were resuspended in the recording buffer B {5
mM KCl, 0.475 M mannitol, 0.1 mM CaCl2, and 10 mM MES [-(N-morpholino)
ethanesulfonic acid]/KOH, pH 5.5, standard recording medium for cell
files) to remove external dye. After sedimentation at room temperature,
cell files were embedded in a thin layer of low-melting-point agarose
(1.3% [w/v] agarose VII, in buffer B, applied at about
40°C) on a prewarmed welled slide.
Freshly prepared longitudinal sections through the pulvinal region were
rinsed and incubated for 60 min in 10 µM SNARF-1AM (1%
[v/v] dimethyl sulfoxide, 22°C). Following dye loading they were washed three times with buffer C (0.1 mM
CaSO4, 0.2 mM K2SO4, 0.1 mM NaCl, 0.5 mM MgCl2, and 10 mM MES/Tris, pH 5.5, standard recording medium for tissue
sections) to remove excess dye. The slices were then embedded in a thin
agarose layer (1.3% [w/v] agarose VII, in buffer C, applied
at about 40°C) on a prewarmed welled slide.
For gravity experiments, welled slides were sealed with a coverslip
using melted valap (vaseline:lanolin:paraffin, 1:1:1, w/w), whereas for
perfusion experiments, the slide well (approximate volume 0.3 mL) was
left open on two sides and had a small reservoir on each side. This
allowed rapid media exchange using filter paper.
Unless otherwise stated, chemicals were obtained from Sigma Chemical
Co. (St. Louis) and fluorescent dyes were obtained from Molecular
Probes Inc. (Eugene, OR).
Confocal Imaging and Ratiometric pH Measurements
Experiments were conducted with a confocal microscope system
(Leica SP, Leica). The ratiometric pH indicator SNARF-1 AM was excited
with an argon laser at 514 nm, and fluorescence emission windows were
set to 550 to 600 nm (peak of acidic form) and 620 to 670 nm (peak of
basic form). These wavelengths avoided autofluorescence from the
amyloplasts present within the bundle sheath cells. Concurrent differential interference contrast images were also recorded. Images
were acquired with a 20× numerical aperture 0.6 dry objective at 5- to
10-s intervals for up to 40 min. Ratiometric image analysis was
performed with Metafluor 4.01 software (Universal Imaging) with
cytoplasmic regions marked and thresholds set at 3 and 253 (8-bit
image). Ratios are given as emission intensity at 620 to 670 nm divided
by emission intensity at 550 to 600 nm. In vitro calibrations were
carried out with 50 µM SNARF-1 dextran (10 kD) in 100 mM KCl, 1 mM ATP, 1 mM
MgCl2, and 10 mM HEPES
[4-(2-hydroxyethyl)-1-piperazineethanesulfonic acid]/Tris adjusted to
pH 6.0, 6.5, 7.0, 7.5, and 8.0 (Bibikova et al., 1998).
For gravity experiments, the confocal unit was attached to an
"upright" microscope (Leica model DMRX-A) that was mounted sideways in a cradle to give a horizontal light path. Specimens were mounted on
a rotating stage and kept in an upright position for at least 30 min
before the start of an experiment. Specimens were gravistimulated by
rotating the stage, and imaged with centerable lenses adjusted to give
a constant field of view as the stage rotated. Images were recorded
before and after gravistimulation, but images taken during and directly
after rotation were often blurred and could not be used for ratio
analysis, resulting in gaps in the recording of between 25 and 180 s.
Perfusion experiments were performed in the horizontal position on an
inverted microscope (Leica model DM-IRB) to facilitate solution changes.
Data Analysis
Emission ratios were routinely measured at the sides and base of
the turned cells. Throughout the manuscript, the terms "side" and
"base" of cells refers to their position after rotation. Average ratio values were compiled from three to nine independent data sets (if
not indicated otherwise) and are presented as average values ± SE (n = no. of cells or regions
measured). The rate of change in the ratio after gravistimulation was
determined using linear regression and a least-square fit. Data sets
obtained for different cell regions/types were compared statistically
using Student's t test for independent samples.
| |
FOOTNOTES |
Received February 16, 2001; returned for revision April 23, 2001; accepted June 3, 2001.
1
This work was supported by the National
Aeronautics and Space Administration (NASA Specialized Center of
Research and Training grant no. NAGW-4984).
2
Present address: School of Biological Sciences, Macleay
Building A12, Sydney University, NSW 2006, Australia.
3
Present address: Max Planck Institute for Molecular Cell
Biology and Genetics, Pfotenhauerstrasse 108, 01307 Dresden, Germany.
[w]
The online version of this article contains Web-only
data. The supplemental material is available at www.plantphysiol.org.
*
Corresponding author, e-mail eva_johannes{at}ncsu.edu; fax
919-515-3436.
| |
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[Abstract]
[Full Text]
[PDF]
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M. Palmieri and J. Z. Kiss
Disruption of the F-actin cytoskeleton limits statolith movement in Arabidopsis hypocotyls
J. Exp. Bot.,
September 1, 2005;
56(419):
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[Abstract]
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C. Saito, M. T. Morita, T. Kato, and M. Tasaka
Amyloplasts and Vacuolar Membrane Dynamics in the Living Graviperceptive Cell of the Arabidopsis Inflorescence Stem
PLANT CELL,
February 1, 2005;
17(2):
548 - 558.
[Abstract]
[Full Text]
[PDF]
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E. B. Blancaflor and P. H. Masson
Plant Gravitropism. Unraveling the Ups and Downs of a Complex Process
Plant Physiology,
December 1, 2003;
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G. Hou, D. R. Mohamalawari, and E. B. Blancaflor
Enhanced Gravitropism of Roots with a Disrupted Cap Actin Cytoskeleton
Plant Physiology,
March 1, 2003;
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[Abstract]
[Full Text]
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M. Haruta and C. P. Constabel
Rapid Alkalinization Factors in Poplar Cell Cultures. Peptide Isolation, cDNA Cloning, and Differential Expression in Leaves and Methyl Jasmonate-Treated Cells
Plant Physiology,
February 1, 2003;
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[Abstract]
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J. C. Long, W. Zhao, A. M. Rashotte, G. K. Muday, and S. C. Huber
Gravity-Stimulated Changes in Auxin and Invertase Gene Expression in Maize Pulvinal Cells
Plant Physiology,
February 1, 2002;
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[Abstract]
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I. Heilmann, J. Shin, J. Huang, I. Y. Perera, and E. Davies
Transient Dissociation of Polyribosomes and Concurrent Recruitment of Calreticulin and Calmodulin Transcripts in Gravistimulated Maize Pulvini
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[Abstract]
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TOP
ABSTRACT
INTRODUCTION