Albrecht-von-Haller-Institut für Pflanzenwissenschaften,
Universität Göttingen, Untere Karspüle 2, 37073 Göttingen, Germany.
To
explore possible pathways for anions to enter the xylem in the root
during the transport of salts to the shoot, we used the patch-clamp
method on protoplasts prepared from the xylem parenchyma of barley
(Hordeum vulgare L.) plants. K+ currents
were suppressed by tetraethylammonium or
N-methylglucamine in the solutions in the pipette and
the bath, and the permeating anions were Cl
or
NO3. We recorded the activities of three
distinct anion conductances: (a) an inwardly rectifying anion channel
(X-IRAC), characterized by activation at hyperpolarization and open
times of up to several seconds; (b) a quickly activating anion
conductance (X-QUAC), important for anion efflux at voltages between
50 mV and the equilibrium potential of the prevailing anion; and (c)
a slowly activating anion conductance (X-SLAC), activating above 100
mV. Both X-IRAC and X-QUAC were permeable for Cl and
NO3; X-QUAC was also permeable for malate.
The occurrence of X-IRAC became more frequent with an increase in
cytoplasmic Ca2+, while the occurrence of X-QUAC decreased.
Anion currents through X-SLAC, and particularly through X-QUAC, were
estimated to be large enough to account for reported rates of xylem
loading, which is in accordance with the notion that xylem loading is a
passive process.
 |
INTRODUCTION |
Three pathways are thought to exist for the radial transport of
inorganic nutrients from the root cortex into the stele: the apoplastic, the symplastic, and the transcellular routes (Pitman, 1982
;
Clarkson, 1993). However, the hydrophobic Casparian strip in the walls
of the endodermis blocks the apoplastic path for salts (Caspary,
1865-1866; Marschner, 1995), and, therefore, ions can enter the
stele only by passing plasma membranes at least twice to reach the
transport system from the root to the shoot, once upon entry into the
symplast of the root and again during their release into the apoplast
of the stele. It is this discharge that was the subject of the present
study. How it takes place was a matter of speculation for decades (for
instance, see Marschner, 1995). Knowledge of the transport mechanisms
involved in xylem loading and their control would contribute to our
understanding of a controlled nutrient transfer from the root to the shoot.
Results of patch-clamp experiments with isolated protoplasts prepared
from barley (Hordeum vulgare L.) roots showed that salt efflux from cells of the xylem parenchyma can occur passively through
ion channels (Wegner and Raschke, 1994). The activity of an outward
rectifier for K+ would allow cations to pass into
the apoplast of the stele (Wegner and Raschke, 1994; Wegner and De
Boer, 1997). A similar type of channel was found in roots of maize
(Roberts and Tester, 1995). Recently, the amino acid sequence of a
K+-specific outwardly rectifying channel from
Arabidopsis was reported; this protein was expressed exclusively in the
root stele (Gaymard et al., 1998). Salt loading is an electroneutral
process. It requires the presence of anion conductances that match the
cation permeabilities. Little information on such transport proteins is
available to date for the xylem parenchyma. Wegner and Raschke (1994)
described an anion channel in cells from this tissue; however, its
transport capacity seemed insufficient to account for anion loading. We therefore continued the exploration of anion conductances, again using
protoplasts prepared from the xylem parenchyma of barley roots. We
discovered activities for three types of anion conductances exhibiting
different characteristics, and evaluated their importance for the
release of salts into the xylem.
| |
MATERIALS AND METHODS |
Plant Cultivation and Protoplast Isolation
Barley (Hordeum vulgare L. cv Apex; F. von
Lochow-Petkus, Bergen, Germany) was grown in a hydroponic growth
facility on aerated full-strength Long-Ashton
NO3-type solution (Hewitt
and Smith, 1975) that was changed weekly. Plants were grown at 20°C
from 4 to 22 h and at 18°C from 22 to 4 h. They were
illuminated at 300 µmol m2
s1 from fluorescent tubes (L65W/25S, Osram,
Munich, Germany) from 8 to 20 h. Xylem parenchyma protoplasts were
isolated from roots of 3- to 5-week-old plants as described by Wegner
and Raschke (1994). Nodal roots 4 to 6 cm long without lateral root
formation were selected, and the apical 1 to 2 cm cut off. The stele
was pulled out of the cortex, and the distal 1 to 2 cm of the stele was
chopped into millimeter segments and incubated in enzyme solution for
2.5 h at 20°C (2% [w/v] cellulase Onozuka R10, Yakult Honsha, Tokyo; 0.02% [w/v] pectolyase Y-23, Seishin Pharmaceutical, Tokyo; 2% [w/v] bovine serum albumin, 10 mM Na
ascorbate, and 1 mM CaCl2; pH 5.5; 500 mosmol kg1). The enzyme was
filtered in three steps (200-, 100-, and 20-µm mesh) using 500 mM sorbitol augmented with 1 mM CaCl2 as washing medium.
Protoplasts were then isolated by two centrifugation steps (120g for 10 min each).
Electrical Recording and Solutions
Anion currents were investigated with the patch-clamp technique
(Hamill et al., 1981) using an amplifier (EPC-7, List Electronic, Darmstadt, Germany) and a personal computer (Mega ST4, Atari, Sunnyvale, CA) with the E9-screen program (HEKA Elektronik, Lambrecht, Germany) for pulse generation. Capacitive currents were measured and
corrected for with the amplifier. Access resistances (between 5.6 and
20 M
) were measured with the amplifier and corrected for using the
method of Marty and Neher (1995) when current-voltage curves were plotted.
Data were low-pass filtered at the frequencies given in the figure
legends with an eight-pole Bessel filter (3 dB corner frequency;
Frequency Devices, Haverhill, MA) and stored on the computer's hard
drive or on videotape (Panasonic NV-H75, Matsushita Electric
Industrial, Osaka) via an ITC 16 interface (Instrutech, Elmont, NY) or
a VR-10 interface (Instrutech), respectively. For data transfer from
videotape to hard disk, the program Acquire (H. Affolter and F. Sigworth, Instrutech) was used. The sample frequency was at least four
times the filter frequency.
Pipettes were pulled (L/M-3P-A, List Electronic, Darmstadt, Germany)
from borosilicate glass capillaries (Kimax-51, Kimble Products,
Vineland, NY), insulated with Sylgard (Dow Corning, Midland, MI),
and fire-polished (L/M-CPZ-101, List Electronic). Tip resistances
were 5 to 20 M. Electrode tip potentials were nulled during the
patch-clamp procedure. All recordings were made at temperatures between
22°C and 24°C. The reference electrode was fixed in a tube filled
with 200 mM KCl (agar bridge) or with the external solution.
Solutions were designed for the detection of anion currents.
K+ currents were suppressed by tetraethylammonium
(TEA+) or N-methylglucamine
(NMG+). The standard extracellular solution
contained: 30 mM TEA-Cl (or NMG-Cl), 5 mM Ca(Glc)2, 2 mM MgCl2, and 10 mM 2-(N-morpholino)-ethanesulfonic acid (MES),
and was adjusted to pH 5.8 with Tris. The osmolality was adjusted to
500 mosmol kg1 with mannitol. Two intracellular
solutions were used: the low-Ca2+ solution
contained 120 mM TEA-Cl (or NMG-Cl), 0.15 µM free Ca2+ as 4.3 mM Ca(Glc)2, 10 mM EGTA, 2 mM MgATP, 2 mM MgCl2, and 10 mM Tris, and was adjusted to pH 7.2 with MES; the
high Ca2+solution was the same as the low
Ca2+, except with 5 µM free Ca2+ as 4.5 mM Ca(Glc)2 and 10 mM N-hydroxyethyl-EDTA in place of 10 mM EGTA. In each case, osmolality was
adjusted to 530 mosmol kg1 with mannitol. This
was verified by a water-vapor pressure osmometer (5100 C, Wescor,
Logan, UT). Total and free concentrations of divalent cations were
computed using the program Calcium (Führ et al., 1993).
Variations of the solutions are indicated in the figure legends. All
solutions were filtered with a 0.22-µm filter before use and stored
at 20°C.
Data Analysis
Data were analyzed with the software packages Review (Instrutech),
Tac (Instrutech), and SigmaPlot (Jandel, San Rafael, CA). Liquid
junction potentials between pipette and bath solutions have been
measured and all membrane voltages were corrected for according to the
method of Neher (1992). Correction was done if the magnitudes of the
liquid junction potentials were larger than 3 mV. This was the case
when 30 mM TEA-Cl (7 mV) or 30 mM NMG-Cl (8
mV) was in the bath. Liquid junction potentials were the same with low-
or high-Ca2+ solutions in the pipette. In the
tests for ion selectivity, starting with TEA-NO3
or (TEA)2-malate, 7 or 8 mV were subtracted,
respectively. Ion activities were calculated when ionic equilibrium
potentials were critical for data interpretation. Means of measured
data are given with SD.
For single-channel analysis, current versus voltage curves were
constructed from single-channel amplitudes determined by measuring the
amplitudes in continuous recordings and fitting the resulting histograms with Gaussian functions, or by calculation of the mean single-channel current according to:
|
(1)
|
Fast-voltage ramps were applied for the recording of the current
through an open channel. For correction of the background current, the
current flowing when the channel was closed was subtracted (see Tyerman
and Findlay, 1989).
The mean open time was calculated according to:
|
(2)
|
Since there was more than one channel active in the experiments,
the channel activity, or the number of channels (n) times the open probability (P) was calculated:
|
(3)
|
The current at the baseline was measured to ensure that all
channels were closed. If this was not the case, the nP value was corrected.
Current-voltage curves derived from whole-cell recordings were
constructed from a series of voltage steps, which are given in the
figures. Usually the current 10 ms into a voltage step (the
"instantaneous current") and the current at the end of a voltage
step (after a new steady state had been established) were plotted
against the voltage. Between voltage steps, voltage was clamped at the
holding potential for the current to settle.
Protoplasts varied in size. Their capacities were between 8 and 23 pF.
Note that each parenchyma cell disintegrated into an average of six
protoplasts during preparation (Wegner and Raschke, 1994). To compare
measurements on different cells, channel activities and currents were
related to the membrane area. The specific capacity of xylem
parenchyma protoplast was 0.9 µF cm2
(Wegner and Raschke, 1994).
Permeability ratios were determined under bi-ionic conditions. The
intracellular solution contained 120 mM TEA-Cl and the extracellular solution contained 30 mM
TEA-NO3 or (TEA)2-malate, respectively. After determination of the reversal potential,
permeability ratios were calculated by the Goldman-Hodgkin-Katz-voltage
equation (Hille, 1992):
|
(4)
|
where P is the permeability, z is the
valence, Erev is the reversal
potential, F is Faraday's constant, R is the gas
constant, T is the absolute temperature, a is the
activity, m and n are the ion species, and
o and i are the extracellular and intracellular sides. This equation was derived from the condition that at the reversal potential the sum of the ion currents is zero:
|
(5)
|
where I is the ion flux density,
z
is the valence of the ion species
, and 
is the flux
density of ion species . Ion flux densities () were
estimated by applying the Nernst-Planck equation (Adam et al., 1988):
|
(6)
|
where P is the permeability
coefficient for ion species , and E is the
membrane voltage. Substitution of Equation 6 (for = m and for = n) into Equation 5,
followed by rearrangement, led to Equation 4.
Sign Convention and Estimation of Ion Fluxes from Xylem Parenchyma
into the Apoplast
Membrane potentials are defined as the voltage on the cytoplasmic
side of the membrane with respect to the physiological outside. In the
"whole-cell"
and in the "outside-out"configuration, the inner side of the membrane is turned toward the pipette. Thus, the
voltage between the pipette and the reference electrode corresponds to
the membrane potential. A negative current corresponds to an anion
efflux from the protoplast and to a K+ influx
into the protoplast.
To evaluate the putative role of anion conductances in xylem loading,
ionic fluxes were calculated from electrophysiological data. Since salt
export is an electroneutral process, anion efflux must equal cation
efflux. Based on the assumptions that ion efflux occurred through
K+-selective outwardly rectifying channels (KORC)
(data from Wegner and De Boer, 1997) and through one of the anion
conductances each time, and that the membrane potential is a pure
diffusion potential, a hypothetical membrane potential at which salt
efflux would be possible was determined. Ion fluxes from cytoplasm into
the xylem vessels (JCX) were
calculated from current densities (j) at this hypothetical membrane:
|
(7)
|
Where A is the cell surface, b is the fresh
weight, z is the valence, and F is
Faraday's constant. All xylem parenchyma cells from the
differentiated metaxylem likely participate in xylem loading (see Fig.
1 in Wegner and Raschke, 1994).
Therefore, the current density was multiplied with the cell surface to
obtain ion fluxes, which then were related to fresh weight. Values of cell surface (0.42 cm2
cm1 root length) and
fresh weight (3.9 mg cm1
root length) were provided by L.H. Wegner (personal communication). Whole-cell currents through inwardly rectifying anion channels (X-IRAC)
were determined by multiplying the single-channel current by the
channel activity (nP).
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Figure 1.
Example of single-channel recordings of X-IRAC in
the whole-cell configuration (from one protoplast out of seven). The
data were filtered at 100 Hz. In the pipette was high-Ca2+
solution; in the bath was the standard solution (see "Materials and
Methods"). The letter "c" at the beginning of each trace
indicates the current level at the closed state. Downward changes
correspond to channel openings. Arrows point to changes in open-channel
conductance levels (presumed subconductance states).
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RESULTS |
Because we wished to discover anion conductances, we suppressed
K+ currents by the use of
TEA+ or NMG+ in the place
of K+ in the solutions of our patch-clamp
experiments. Considering that usually Ca2+ is
required to activate anion channels (Hedrich et al., 1990; Tester,
1990), we began our experimentation with 5 µM
Ca2+ in the pipette. Under these conditions,
X-IRAC (X stands for xylem parenchyma) appeared as the predominant
anion conductance. It was active in 34% of the examined protoplasts
and was readily recognized in the whole-cell configuration by the
appearance of single-channel events. During the experimental
characterization of X-IRAC, we applied short hyperpolarizing and
depolarizing voltage pulses and discovered rapidly activating and
inactivating currents, which we interpreted as displays of the quickly
activating anion conductance (X-QUAC). This anion conductance could
further be identified by a concavity in the current-voltage curve that
was displayed when voltages were raised above 40 mV. The conductance X-QUAC also occurred when the Ca2+ concentration
in the pipette was lowered to 0.15 µM. A third anion
conductance appeared during long voltage pulses, which deactivated slowly. We called it the slowly activating anion conductance (X-SLAC), which occurred in 7% of the tested protoplasts. The current-voltage relationships of all three anion conductances had in common a change in
sign at or close to the Nernst potential of the major anion in the
solutions (Cl or
NO3).
X-IRAC
Single-channel events with slow gating characteristics became
visible in the whole-cell configuration, and indicated low channel density or activity of X-IRAC (Fig. 1). This anion channel was active
between 180 and 50 mV. Different levels of open-channel conductances
appeared (Fig. 1), especially in the negative voltage range. In the
experiments, some of which lasted as long as 40 min, no inactivation of
X-IRAC occurred. The mean open time was in the range of seconds; for
instance, at 73 mV, it was 1.2 ± 0.5 s (n = 6, 5 µM Ca2+ in the
pipette). Current-voltage relationships were derived from single-channel recordings (Fig. 2). They
showed that the sign of the current reversed near
ECl. Using
standard solutions, the Nernst potential of Cl
was 30 mV, whereas the Nernst potentials of TEA+
or NMG+, and that of Ca2+
were located at 32 and 143 mV, respectively. Currents recorded during
the application of voltage ramps while an X-IRAC channel stayed open
were zero at 27 ± 4 mV (n = 16) (see also
comparison of the currents with Cl and
NO3 in the bath in Fig.
4). Gaussian functions were fitted to the single-channel current
frequencies (the inset in Fig. 2 shows an example). They were spaced at
equal current intervals, indicating that usually more than one channel
was active in a protoplast; up to 14 simultaneously active channels
could be distinguished in a single (sub) protoplast. Single-channel
currents did not depend on internal Ca2+
concentrations (Fig. 2).
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Figure 2.
Current-voltage relationship of X-IRAC. Currents
were derived from single-channel recordings on six different cells
exposed to 0.15 µM Ca2+ in the pipette (white
symbols, five of the upright triangles are hidden behind other symbols)
and on six different cells exposed to 5 µM
Ca2+ in the pipette (black symbols). A line was fitted to
the means of currents at voltages between 159 and 93 mV; it did not
pass through the origin (r2 = 0.89),
which would have been the case if rectification was the result of a
concentration gradient, as described by the Goldman-Hodgkin-Katz
current equation (Hille, 1992). Inset, Logarithm of the frequency of
discrete current events as they appeared in recordings such as the one
shown in Figure 1, plotted against current. This example was taken from
a recording obtained at 13 mV. Such distributions were used to
determine the number of simultaneously active channels in a protoplast
(here it was 5). Distances between the means of Gaussian functions
fitted to the data indicate magnitudes of single-channel currents. In
the pipette was either the high- or low-Ca2+ solution; in
the bath was the standard solution (see "Materials and Methods").
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Currents increased with hyperpolarization, but remained small at
positive potentials (Fig. 2). This inward rectification by X-IRAC was
not caused by a concentration gradient (legend to Fig. 2). In standard
solutions the chord conductance of X-IRAC decreased from 71 pS at 133
mV (n = 2) to 47 pS at 73 mV (n = 5)
and further to 13 pS at 3 mV (n = 3).
If the Ca2+ concentration in the pipette was
raised from 0.15 to 5 µM, the probability of appearance
of X-IRAC increased. At 0.15 µM, X-IRAC was active in
nine out of 84 protoplasts, corresponding to 11% of the examined
protoplasts; and at 5 µM, activity appeared in 25 out of
74 protoplasts, corresponding to 34%. A 
2
test showed that the association between increasing the concentration of Ca2+ and increasing activity of X-IRAC was
significant at a level of P = 0.005 (2 = 7.98 > 7.88). The channel activity
(nP) of X-IRAC fluctuated strongly (Fig.
3), varying between 0.05 × 106 cm2 and 0.9 × 106 cm2. The mean value
of nP over the whole voltage range was 0.26 ± 0.27 × 106 cm2 with
0.15 µM Ca2+ in the
pipette (n = 33) and 0.25 ± 0.21 × 106 cm2 with 5 µM Ca2+ in the pipette
(n = 39, calculated from the data shown in Fig. 3).
Nevertheless, with 0.15 µM
Ca2+ in the pipette, channel activity declined
with increasing voltage in two out of the four protoplasts tested (Fig.
3A); however, in general, the intracellular Ca2+
concentration did not affect channel activity of X-IRAC significantly. Changes in the external Ca2+ concentration from 5 to 40 mM, or to 1 mM, did
not influence the occurrence of X-IRAC or its current-voltage
relationship (not shown).
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Figure 3.
Channel activity (nP) per unit
membrane area (A) of X-IRAC with low-Ca2+
solution (0.15µm) (A) and high-Ca2+ solution (5 µM) (B) in the pipette.; in the bath was the standard
solution (see "Materials and Methods"). Results are from four (A)
and six (B) protoplasts (identified by different symbols). Lines in A
represent regressions of data from two individual protoplasts; in these
two instances, channel activity declined with increasing voltage, with
r2 of 0.97 and 0.57, respectively.
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X-IRAC was equally permeable for
NO3 and
Cl. Replacement of Cl
by NO3 in the bath did
not alter the current-voltage curves (n = 5); current
responses and reversal potentials were nearly identical with either one
of the anions present (Fig. 4); with
external NO3 the reversal
potential was 27 ± 2 mV (n = 5). Single-channel currents were determined at membrane potentials of 93, 23, and 97 mV, and were found to have been 7.6 ± 1 pA, 1.6 ± 0.1 pA and 0.6 ± 0.3 pA, respectively (n = 5). With
external Cl, the corresponding single-channel
currents were 7.5 ± 0.8 pA, 1.3 ± 0.6 pA, and 0.5 ± 0.3 pA (n = 6). External
NO3 did not affect
channel activity (nP), which was 0.3 ± 0.28 (n = 28, four protoplasts). In one case, nP
decreased linearly with increasing potentials (not shown).
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Figure 4.
Current responses of X-IRAC to voltage ramps of
50-ms duration (inset), showing that replacement of external
Cl by NO3 had no effect.
Residual currents (flowing when all anion channels were closed) were
subtracted. The current-voltage curve with external Cl is
an average of eight ramps; that with external
NO3 of 17 ramps. This experiment was
conducted on one protoplast in the whole-cell configuration (replicated
with four more protoplasts). The filter frequency was 100 Hz. In the
pipette was low-Ca2+ solution; in the bath was the standard
solution with the indicated changes in the major anion (see
"Materials and Methods").
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X-QUAC
Typical for this conductance was its rapid activation upon voltage
jumps from a holding potential of 43 mV to both more positive and
more negative values (Fig. 5). X-QUAC was
active between 200 and 100 mV. In all experiments in which X-QUAC
dominated cell conductance, the sign of the currents reversed at
25 ± 5 mV (n = 20), a value slightly more
negative than the Nernst potential of Cl. Leak
currents were not subtracted from the recorded values; they may have
caused this shift, and they could have included the activity of an
electrogenic pump (Köhler and Raschke, 1998b). The
current-voltage curves exhibited a maximum near 40 mV, where the
magnitude of the current was small, and a minimum near 0 mV. The
magnitude of the currents through X-QUAC varied among protoplasts; the
current density at the minimum was 2.2 ± 2 µA
cm2 (n = 20). To bring out
common current-voltage characteristics of X-QUAC, currents of six
protoplasts were normalized with respect to their minimum at 0 mV and
shown in Figure 5C. At hyperpolarization, X-QUAC inactivated partially
(Fig. 5A). Tail current experiments were performed after partial and
complete inactivation of the inward current. Currents reversed between
27 and 37 mV, near the Nernst potential of Cl
(n = 6); they were carried by
Cl (Fig. 6). The
same conclusion applied to the outward currents (n = 6, not shown, but confirmed by pulse experiments such as the one presented
in Fig. 5).
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Figure 5.
Activation and current-voltage relationship of
X-QUAC. A, From a holding potential of 43 mV (for 10 s), pulses
of 500-ms duration were applied in decrements of 20 mV, covering the
voltage range between 77 and 163 mV; whole-cell configuration. The
filter frequency was 1 kHz. In the pipette was low-Ca2+
solution; in the bath was the standard solution (see "Materials and
Methods"). B, Current-voltage relationship of X-QUAC derived from the
data shown in A. Current densities (j) measured 10 ms ( ) and 500 ms
( ) after initiation of a voltage step (arrows in A) were plotted
against voltage. C, Currents measured on six protoplasts (identified by
different symbols) at the end of 500 ms-pulses plotted against voltage.
Relationships were normalized with respect to the current minimum,
jmin, appearing at a membrane voltage near 0 mV. Data from
the experiment shown in A and B are included () and joined by a
line.
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Figure 6.
X-QUAC, tail-current experiments. After clamping
the voltage at 143 mV for 100 ms (A) or 1 s (B), voltage pulses
with a duration of 100 ms were applied between 57 and 53 mV (insets).
Erev, The currents reversed between 17 and 27 mV (A) or
between 27 and 37 mV (B). Whole-cell configuration, filter frequency
was 1 kHz. In the pipette was low-Ca2+ solution; in the
bath was the standard solution (see "Materials and Methods").
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A low concentration of Ca2+ in the
"cytoplasm" enhanced the activity of X-QUAC, in contrast to the
Ca2+ dependence of the activity of X-IRAC: With 5 µM Ca2+ in the pipette, X-QUAC
appeared in seven out of 68 protoplasts, corresponding to 10% of the
examined protoplasts; with 0.15 µM Ca2+, X-QUAC activity was seen in 16 out of 59 protoplasts, corresponding to 27% of the examined protoplasts. A
2 test resulted in a value of 4.16, which
indicated that the association between increasing
Ca2+ concentration in the "cytoplasm" and
decreasing activity of X-QUAC was significant at a level of
P = 0.05 (2 > 3.84). Changes
in the extracellular Ca2+ concentration between 1 and 40 mM did not affect the occurrence of X-QUAC
nor its current-voltage relationship (not shown).
The conductance X-QUAC was permeable not only for
Cl, but also for
NO3 and
malate2 (Fig. 7).
In the presence of external
NO3 (30 mM),
the reversal potential was near 9 mV; it shifted to 55 mV after
replacement by 30 mM malate (Table
I). From the reversal potentials,
relative permeabilities (with respect to that for Cl) were calculated (Table I). For
PNO3
/PCl, the ratio was 3. Because, at pH 5.8 in the external solution, 83% of
the malate was charged 2-fold (pK1 = 3.5;
pK2 = 5.1), we assumed that
malate2 permeated the membrane, and we
estimated
Pmalate2/PCl to have been about 0.28 (for single-charged malate, the permeability ratio would have been about 48; Table I). Most of these experiments were done on different protoplasts.
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Figure 7.
A, Current-voltage relationships of X-QUAC for
three different anions in the external solution, Cl
( ), NO3 ( ), and malate2
(). The data shown for NO3 and
malate2 were obtained on one protoplast after replacing
external TEA-NO3 with (TEA)2-malate. B,
Currents were normalized with respect to their minima that appeared at
membrane voltages between 50 mV and the reversal potentials, average
currents of Cl (n = 5) and
NO3 (n = 4), and two
individual examples for currents of malate2 (white
symbols). A and B, Lines extending to the borders of the diagrams
indicate that some data points were outside the ranges of the panels.
Experimental procedure similar to that shown in Figure 5. In the
pipette was low-Ca2+ solution; in the bath was the standard
solution with the indicated changes in the major anion (see
"Materials and Methods").
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Table I.
X-QUAC is permeable for
NO3 and malate
Permeability ratios with respect to Cl were calculated
from reversal potentials as described in "Material and Methods."
For the determination of reversal potentials, anions were varied in the
bath. The low-Ca2+ solution was used in the pipette.
Px, Permeability for
NO3 (n = 4) or malate
(n = 2). In the case of malate, permeability ratios
were calculated for both the double- and the single-charged form.
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To facilitate comparisons, current-voltage curves were normalized with
respect to the current minimum that in each case appeared in the
voltage range between 50 mV and the particular reversal potentials;
Figure 7B). (This voltage range is probably the most important one for
salt release into the xylem; see "Discussion"). The position of the
minimum depended on the species of the external anion. With external
NO3, it was about 20 mV
more negative than with external Cl, and with
external malate, it was about 15 mV more positive than with external
Cl. Considering the absolute magnitudes of the
anion effluxes in the mentioned voltage range (Fig. 7A), we recognize
that replacement of external
NO3 by malate led to a
reduction of anion loss, although the electromotive force acting on the
anion in the cell was larger with malate than with
NO3. This result was
obtained on one and the same protoplast; it could not have been
accidental, despite the generally wide variation among cells in the
magnitude of their anion currents. We do not know yet whether the
disparity between malate currents that appeared at negative membrane
voltages (Fig. 7B) points to variations in a hypothetical binding site
for malate.
X-SLAC
This conductance appeared in seven out of 104 experiments when the
internal Ca2+ concentration was kept relatively
low (at 0.15 µM), and activated at potentials higher than
100 mV. In the experiment shown in Figure
8, it was activated at a holding
potential of 37 mV. Polarizing pulses resulted in gradual
deactivations, illustrating the slow gating behavior of X-SLAC. The
increase in current following the step from 37 to 67 mV made it clear
that at 37 mV, X-SLAC was not yet fully activated (Fig. 8A). The
reversal potential of about 30 mV affirms a selectivity of X-SLAC for
the anion Cl, and the current densities of both
the instantaneous current (measured 10 ms after the voltage step, white
symbols in Fig. 8B) and the steady-state current (as extrapolated from
exponential functions fitted to the deactivation records, black symbols
in Fig. 8B), reversed near the equilibrium potential of
Cl. (The instantaneous current represents the
current through channels that were activated during the time at the
conditioning voltage of 37 mV).
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Figure 8.
A, Deactivation of X-SLAC recorded while running
the voltage protocol shown in the inset; between pulses, the voltage
was clamped to 37 mV for 60 s each. Filter frequency was 400 Hz.
At negative potentials, currents were noisy occasionally. B,
Current-voltage relationship of X-SLAC in three protoplasts. Current
densities determined 10 ms after triggering a voltage pulse (white
symbols) and after a new steady state had been established (black
symbols) were plotted against the voltage. Squares indicate values
derived from the records shown in A. Steady-state currents were
determined by extrapolation of exponential functions fitted to the
deactivation curves. Nernst potentials were 30 mV (Cl),
32 mV (TEA+), and 143 mV (Ca2+). In the
pipette was low-Ca2+ solution; in the bath was the standard
solution (see "Materials and Methods").
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The steady-state current-voltage curve proves that X-SLAC stays active
at membrane voltages greater than 100 mV (more positive than 100
mV). Clamping the voltage at hyperpolarized values led to a closure of
X-SLAC; this is demonstrated in Figure 9.
After a holding voltage of 123 mV, voltage steps elicited only
insignificant current changes during the 500 ms-pulses (Fig. 9B), in
contrast to steps starting from a holding potential of 37 mV (Fig. 9A). The activation of X-SLAC appearing during long pulses was very slow;
after a change from 123 mV to 67 mV, only a small fraction of the
steady-state conductance had just come into view after 5 s (not
shown). The ensuing small increase in current caused a shift of the
reversal voltage to positive values (n = 2, not shown).
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Figure 9.
No activation of X-SLAC at hyperpolarization.
After holding the protoplast for 60 s at conditioning voltages of
37 mV (A) or 123 mV (B), pulses of 500-ms duration were applied in
20-mV steps to voltages between 87 mV and 137 mV. C, Current-voltage
relationships of three protoplasts determined 10 ms after a voltage
change from a conditioning voltage of 37 mV (black symbols) or of 123
mV (white symbols). Circles joined by lines represent values derived
from the experiment shown in A. Filter frequency was 400 Hz. In the
pipette was low-Ca2+ solution; in the bath was the standard
solution (see "Materials and Methods").
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The gating characteristics of X-QUAC and X-SLAC were clearly distinct.
Only minute time-dependent changes of current through X-SLAC occurred
during pulses of 500 ms duration, in contrast to the pronounced changes
of currents through X-QUAC.
Simultaneous Activity of X-QUAC and KORC
A condition sine qua non for the loading of salts into the xylem
is the concurrent activity of anion and cation conductances. In
solutions containing KCl, a slow activation of the KORC appeared superimposed on the traces of the quickly activated X-QUAC (Fig. 10A). After replacement of the external
KCl with TEA-Cl, K+ currents were inhibited and
the currents through X-QUAC retained (Fig. 10B) their typical
current-voltage characteristics (Fig. 10C). The reversal potential
shifted to ECl. An
activity of the inwardly rectifying K+ channel
(KIRC) was never observed simultaneously with that of X-QUAC, although
KIRC appeared more often than KORC. The conductance KIRC was active in
14 out of 43 protoplasts, KORC only in three.
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Figure 10.
A, Simultaneous activity of X-QUAC and KORC. B,
Inhibition of KORC in the same protoplast by changing from 30 mM KCl in the bath to 30 mM TEA-Cl. Steps of
500-ms duration started from a holding potential of 30 mV and went to
voltages between 70 and 10 mV, and between 40 and 100 mV, in
decrements of 20 mV. C, Currents measured in the experiment shown in A
and B, at 500 ms into each pulse, were plotted against voltage. ,
KCl in the bath; , TEA-Cl in the bath. Filter frequency, 100 Hz.
Solutions: Pipette, 120 mM KCl, 0.15 µM free
Ca2+, 2 mM MgATP, 10 mM EGTA, and
10 mM Tris, pH 7.2; bath, 30 mM KCl or TEA-Cl,
1 mM CaGlc2, 2 mM
MgCl2, and 10 mM MES, pH 5.8.
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DISCUSSION |
Diversity of the Anion Conductances
In our investigation, we suppressed all K+
currents through the plasmalemma of the xylem parenchyma protoplasts by
the use of TEA+ or NMG+ in
the solutions, and therefore K+ currents were not
detected. Currents appearing in response to voltage ramps or sequences
of voltage pulses were zero at the equilibrium potentials of
Cl or
NO3; these were anion
currents. The analysis of these electrical responses indicated the
presence of three distinctly different anion conductances, which we
called X-IRAC, X-QUAC, and X-SLAC (Table
II; Fig.
11).
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Table II.
Relative frequencies of activity of the three anion
conductances in protoplasts prepared from the xylem parenchyma of roots
of barley
Percentage of protoplasts in which the respective conductance was
active at a low and a high intracellular concentration of
Ca2+. Absolute numbers of protoplasts investigated are
given in parentheses. The activities of X-IRAC and X-QUAC were
significantly correlated with the internal Ca2+
concentration (2-test, *, P = 0.05, **,
P = 0.005). Determinations of X-QUAC and X-IRAC were
made in external standard solution. Data on the activity of X-SLAC
included measurements with external 1 and 40 mM
Ca2+. If data obtained solely with external standard
solution were considered, X-SLAC was active in four out of 59 protoplasts, which again resulted in a percentage of 7.
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Figure 11.
Representative current-voltage curves of
the three anion conductances X-QUAC, X-SLAC, and X-IRAC juxtaposed to
that of the KORC to recognize the voltage range in which anions and the
cation K+ could be released simultaneously into the xylem.
The curve for X-IRAC depicts a series of products of nP
by single-channel currents at the respective voltages. Data for KORC
are from Wegner and Raschke (1994). Hatched area, Voltage range in
which salt release appears possible; dotted lines, examples for
simultaneous anion and K+ currents of equal magnitude but
opposite sign through X-SLAC and KORC in one case, and through X-QUAC
and KORC in the other.
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The X-IRAC appeared in 11% of the protoplasts if the
Ca2+ concentration in the pipette was 0.15 µM, and in 34% if Ca2+ was 5 µM. It was characterized by open times of up to several seconds and was active in the voltage range from 180 to 50 mV (Fig.
1). This is most likely identical to the "slow" anion channel described by Wegner and Raschke (1994), which had a mean open time of
1 s. The conductance X-IRAC is an inward rectifier. We showed in
Figure 2 that this property could not have been the consequence of a
concentration gradient, but must have resulted from intrinsic
properties of the channel. The single-channel conductance of X-IRAC
increased with hyperpolarization. At 130 mV, the chord conductance
was 71 pS, and decreased to less than 13 pS near
ECl. Without
taking the rectifying effect into account, Wegner and Raschke (1994)
estimated the conductance to be in the range of 46 to 85 pS at the same
Cl concentrations we used; thus, the magnitudes
of the conductances agreed with each other.
The channel X-IRAC shares features with an anion channel from amaranth
cotyledons (Terry et al., 1991) and an anion channel in suspension
cells derived from barley embryos (Amtmann et al., 1997). Both
possessed slow gating characteristics and large conductances, and were
selective for Cl. Similar to X-IRAC, the anion
channel from barley embryos was strongly inward rectifying. It was
active in the voltage range between 150 and 70 mV, and the open
probability was only weakly voltage dependent (Amtmann et al., 1997).
The anion channel from amaranth also activated at hyperpolarization
(Terry et al., 1991). As also found in X-IRAC, activation was favored
by a high intracellular Ca2+ concentration. A
role of this channel was seen in the control of the membrane potential
(Terry et al., 1991). Subconductance states are known to occur in anion
channels in the plasma membrane of higher plants (Schauf and Wilson,
1987; Terry et al., 1991) and algae (Coleman, 1986; Laver, 1991).
Figure 1 shows that, at hyperpolarization, subconductance states also
occurred in X-IRAC.
Typical for X-QUAC was an activation within milliseconds (Fig. 5).
Plasma membrane anion channels with similar characteristics occur
in various plant species. Some of these channels activated rapidly with
depolarization (Keller et al., 1989; Cerana and Colombo, 1992; Skerrett
and Tyerman, 1994; Zimmermann et al., 1994; Thomine et al., 1995),
others with hyperpolarization (Schauf and Wilson, 1987; Barbara et al.,
1994; Elzenga and Van Volkenburgh, 1997).
The current-voltage curve of X-QUAC displayed a local maximum,
followed, with increasing voltage, by a concavity (in Fig. 5, the
maximum appeared at 40 mV and the minimum near 0 mV). This concavity
resembles that of the current-voltage relationship of the rapidly
activating anion channel of guard cells (Keller et al., 1989; Hedrich
et al., 1990); however, currents through X-QUAC increased with
hyperpolarization, whereas currents through the rapidly activating
anion channel of guard cells declined. The inactivation of X-QUAC after
voltage steps going to negative values (Fig. 5) is shared with other
hyperpolarization-activated anion channels (Barbara et al., 1994;
Elzenga and Van Volkenburgh, 1997).
One could consider the possibility that the two branches of the
current-voltage relationship of X-QUAC (at negative and at positive
voltages) were manifestations of two separate anion conductances, one
inward rectifier and one outward rectifier. Indeed, tail currents recorded after returning from negative and from positive pulses to the
holding voltage differed in their time courses. However, the
anion-channel blocker DIDS (4,4'-diisothiocyanostilbene-2,2'-disulfonic acid) inhibited currents evoked by negative voltages as much as those
produced by positive voltages (Köhler and Raschke, 1998a), and we
never saw the sole activation of just one of the two branches. Alternatively, the conductance X-QUAC could have been only apparent, resulting from a summation of simultaneous activities of X-IRAC and
X-SLAC; but the clearly distinct kinetics of X-QUAC and X-SLAC preclude
this possibility (compare the current responses of these two
conductances with the voltage pulses shown in Figs. 5A, 8A, and 9,A and
B). We consider the one-conductance hypothesis of X-QUAC as the
simplest explanation of our experimental results and are elaborating on
it further at present (B. Köhler, L.H. Wegner, and K. Raschke,
unpublished data).
The anion conductance with slow responses, X-SLAC, appeared in 7% out
of a population of 104 protoplasts. Although its slow gating
characteristics was reminiscent of those of X-IRAC, it differed from it
in its voltage dependency. X-IRAC was active well below 100 mV (Figs.
1 and 2), whereas X-SLAC was active at voltages above 100 mV (Fig.
8). Deactivation of X-SLAC (Fig. 8A) was much slower than that of
X-QUAC (Fig. 5A). After a voltage step, it took more than 30 s
before a new steady state was established (Fig. 8). In this respect,
there is some resemblance to the slowly activating anion channel of
guard cells (Linder and Raschke, 1992; Schroeder and Keller, 1992),
whose half-time of deactivation was 10 s after a voltage step from
20 to 120 mV (Schmidt and Schroeder, 1994). The slow anion
conductance of guard cells was active over a wide voltage range,
extending from below 200 to 50 mV and had a current minimum
(corresponding to a maximum of anion efflux) near 40 mV (Linder and
Raschke, 1992).
In three out of 23 experiments in which X-QUAC was active, a
simultaneous activity of X-IRAC appeared, and three of our voltage-ramp experiments indicated a concurrent activity of X-QUAC and X-SLAC. The
display of two types of anion conductance in one cell type was reported
from guard cells of Vicia faba and Xanthium
strumarium (Linder and Raschke, 1992; Schroeder and Keller, 1992)
and epidermal cells of the Arabidopsis hypocotyl (Thomine et al., 1995;
Cho and Spalding, 1996). An apparent interconversion between quick and slow gating modes of an anion channel in guard cells of V. faba was reported by Dietrich and Hedrich (1994). Anion channels in tobacco suspension cells and epidermal cells of the Arabidopsis hypocotyl also appear to switch between quick and slow gating modes
(Zimmermann et al., 1994; Thomine et al., 1995). It was suggested that
these changes were caused by changes in the channel protein; this
modulation depended on phosphorylation (Zimmermann et al., 1994) or the
presence of ATP (Thomine et al., 1995).
Alternations between gating modes of anion channels also occur in
animal cells, and are controlled by voltage, nucleotides, phosphorylation, or other, unknown factors (Fischer and Machen, 1994;
Larsen et al., 1996). Although we have not yet obtained evidence for
transitions between X-QUAC, X-SLAC, and X-IRAC in xylem parenchyma
cells, we cannot exclude the possibility that just one protein accounts
for the observed diversity, as an alternative to the activity of three
different channel proteins. We also have to consider the fact that each
xylem parenchyma cell disintegrated into an average of six protoplasts
during the isolation procedure (Wegner and Raschke, 1994). If one
protoplast of a preparation displayed only one type of anion
conductance and a second protoplast another type, this could have been
the result of an inhomogeneity in the distribution of conductances in
the plasmalemma of the whole cell and a disconnection of the
conductance ensemble during the division into subprotoplasts.
Control by Ca2+
There was variability in the appearance of the three anion
conductances. This should not be surprising, since ion transport from
the root to the shoot is likely to be regulated and ion channels are
conceivable effectors in this system, possibly with each type responding to a variety of signals. One presumed messenger is Ca2+. Two of the conductances, X-QUAC and X-IRAC,
responded to variations in "cytoplasmic" Ca2+
but, interestingly, in opposite ways. Whereas X-QUAC was active with
0.15 µM Ca2+ in the pipette and
less so with 5 µM, the activity of X-IRAC grew larger
with the same change. In this context it is worth noting that KORC is
active at intracellular Ca2+ concentrations of
0.15 µM, and is inhibited by increasing
Ca2+ levels (Wegner and De Boer, 1997); KORC
therefore goes hand in hand with X-QUAC in regard to
Ca2+ dependence. This parallel behavior supports
the notion that X-QUAC and KORC provide the main pathways for
electroneutral salt loading into the xylem.
The conductance X-SLAC was active at intracellular
Ca2+ concentrations in the nanomolar range as
well, and it might also be involved in xylem loading. In none of our
experiments did the extracellular Ca2+
concentration appear to be a modulating factor. Variations of external
Ca2+ in the range between 1 and 40 mM
did not affect the anion conductances X-QUAC and X-IRAC (not shown),
and Wegner et al. (1994) and Wegner and De Boer (1997) showed that the
K+ conductances KORC and KIRC were also
insensitive to external Ca2+.
Ca2+ concentrations in xylem sap of various
species range between 0.2 and 13 mM (Allen et al., 1988;
Atkinson et al., 1992; Engels and Marschner, 1993; Schurr and Schulze,
1995; Zornoza et al., 1996).
Permeabilities for NO3 and Malate
NO3 is
quantitatively the most important inorganic anion that is transported
from the root through the xylem to the shoot. The permeability of
X-IRAC for NO3 was equal
to that for Cl (Fig. 4), and X-QUAC was three
times more permeable for
NO3 than for
Cl (Table I). Thus, X-IRAC and X-QUAC may have
a function in xylem loading with
NO3. Although we did not
test the permeability of X-SLAC for
NO3, one can say that, in
general, a high permeability for
NO3 is a common feature
of plant anion channels (Schönknecht et al., 1988; Keller et al.,
1989; Terry et al., 1991; Tyerman, 1992; Hedrich and Marten, 1993;
Schmidt and Schroeder, 1994; Skerrett and Tyerman, 1994). However,
there is another side to the fact that the permeabilities for
NO3 and
Cl of the anion conductances in the barley root
were of about equal magnitude. Apparently, there is little
discrimination against Cl, and barley is known
to be a salt includer (Wolf and Jeschke, 1986). It would be worth
testing whether the anion conductances of roots of salt excluders (such
as maize) possess a reduced permeability for
Cl, relative to that for
NO3. Figure 7 indicates
that NO3 may affect the
electrical properties of X-QUAC. We have begun to explore this possibility.
Malate is thought to move in the plant from the shoot to the root at
least in part through the phloem (Ben-Zioni et al., 1971; Kirkby and
Knight, 1977), to be released into the apoplast of the root and ending
up in the xylem sap. The permeability of X-QUAC for malate turned out
to be smaller than that for
NO3 or
Cl (Table I), and the permeability sequence was
similar to that of the quickly activating anion conductance of guard
cells, NO3 (4.2) > Cl (1) > malate (0.1) (Hedrich and
Marten, 1993). (In both investigations, it was the external malate that
was changed.) Because the response to malate of the quickly activating
anion channel of guard cells did not significantly change with a rise
in pH from 5.6 to 7.2, malate2 seemed to
represent the active form of the metabolite (Hedrich and Marten, 1993).
We assumed that it was also malate2 that
permeated X-QUAC at pH 5.8 in the external solution. At this pH, 83%
of the malate is in the doubly charged form (pK1 = 3.5; pK2 = 5.1). There appeared to be some
relationship with the quickly activating anion channel of guard cells,
in which the current-voltage curve was modified by the presence of
external malate. The activation potential and the concavity of the
current-voltage relationship of the guard cell conductance moved to
more hyperpolarized values with 82 mM malate (Hedrich and
Marten, 1993). This was not the case with X-QUAC. Nevertheless, the
decrease in anion efflux after the addition of external malate (Fig.
7A) is an indication that malate in the xylem sap might have a function
in controlling X-QUAC, for instance by binding to an external site, as
was reported to occur with the quickly activating anion channel of
guard cells (Hedrich and Marten, 1993). Malate can provide negative
charges in the xylem fluid, e.g. in
NH4+-grown plants (Arnozis
and Findenegg, 1986; Marschner, 1995). Further experiments should be
directed at the question of whether malate modifies the properties of
X-QUAC. If so, malate in the xylem sap could act as a messenger by
controlling membrane potential in the xylem parenchyma and anion
currents into the xylem vessels.
Estimation of Salt Fluxes into the Xylem
If salt release into the xylem is passive, two requirements must
be met: the electrochemical potential gradients of the ions to be
transported must be downhill into the xylem, and the voltage across the
plasmalemma must be in a range at which anion and cation conductances
are open simultaneously. Therefore, the equilibrium potentials of
cations and anions set limits within which an electroneutral flux of
anions and cations can occur. Under the conditions we assumed to apply,
this was the case in the range from 30 to 30 mV (hatched area in Fig.
11). We also have to consider the limits set by the voltage
dependencies of the ion conductances. An efflux of
K+ through KORC can occur only at voltages above
50 mV (Wegner and Raschke, 1994). All of the three anion
conductances, X-IRAC, X-QUAC, and X-SLAC are active beyond this
boundary (Fig. 11).
From the current-voltage relationships of the anion conductances we
computed fluxes into the xylem (see "Materials and Methods"). Anion
efflux through X-QUAC was larger than through X-IRAC or X-SLAC. Mean
fluxes relative to fresh weight (in grams) were estimated to have been
11 µmol g1 h1 for
X-QUAC, 8 µmol g1 h1
for X-SLAC, and 5 µmol g1
h1 for X-IRAC. These numbers exce
TOP
ABSTRACT
INTRODUCTION