|
|
|
|
|
|
|
||
Original Article |
Correspondence to: Zhenbiao Yang, Department of Botany and Plant Sciences, University of California, Riverside, CA 92521. Tel:(909) 787-7351 Fax:(909) 787-4437 E-mail:zhenbiao.yang{at}ucr.edu.
 |
Abstract |
|---|
 Top Abstract IntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
|---|
Tip-growing pollen tubes provide a useful model system to study polar growth. Although roles for tip-focused calcium gradient and tip-localized Rho-family GTPase in pollen tube growth is established, the existence and function of tip-localized F-actin have been controversial. Using the green fluorescent protein–tagged actin-binding domain of mouse talin, we found a dynamic form of tip-localized F-actin in tobacco pollen tubes, termed short actin bundles (SABs). The dynamics of SABs during polar growth in pollen tubes is regulated by Rop1At, a Rop GTPase belonging to the Rho family. When overexpressed, Rop1At transformed SAB into a network of fine filaments and induced a transverse actin band behind the tip, leading to depolarized growth. These changes were due to ectopic Rop1At localization to the apical region of the plasma membrane and were suppressed by guanine dissociation inhibitor overexpression, which removed ectopically localized Rop1At. Rop GTPase–activating protein (RopGAP1) overexpression, or Latrunculin B treatments, also recovered normal actin organization and tip growth in Rop1At-overexpressing tubes. Moreover, overexpression of RopGAP1 alone disrupted SABs and inhibited growth. Finally, SAB oscillates and appears at the tip before growth. Together, these results indicate that the dynamics of tip actin are essential for tip growth and provide the first direct evidence to link Rho GTPase to actin organization in controlling cell polarity and polar growth in plants.
Key Words: Rho GTPase, cell polarity, polar growth, actin cytoskeleton, RopGAP
|
Introduction |
|---|
|
TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
|---|
The pollen tube has been used as a model system to study tip growth and the actin cytoskeleton for decades because of its uniform cell morphology, rapid growth, and the abundance of actin and its associated proteins (
Unlike in yeast and algal systems, where cortical actin patches are known to establish sites for polar growth (
Recent studies instead suggest the presence of F-actin structures just behind the apical dome of pollen tubes. In tobacco, an actin ring was reported in the subapical region of pollen tubes expressing GFP-talin (
5 µm behind the tip and a dense meshwork of actin filaments in the collar region were observed in chemically fixed maize and Papaver pollen tubes, respectively (
Pharmacological studies suggest that subapical F-actin structures may have a role distinct from that for axial actin cables. Low concentrations of cytochalasin D disrupt subapical fine actin bundles and inhibit root hair elongation, but do not affect axial actin cables and streaming (
It is well established that the organization and dynamics of the actin cytoskeleton are controlled by the RHO family of small GTPases in yeast and animal systems (
Overexpression of CA-Atrac2/rop5At mutants caused axial actin cables to become spiral cables, whereas DN-Atrac2/rop5At mutants induced apparent reduction in the thickness of actin cables in tobacco pollen tubes (
In this report, we demonstrate the presence of a dynamic form of tip-localized F-actin in living tobacco pollen tubes using the actin-binding domain of mTalin tagged with an enhanced GFP mutant. Importantly, using a combined genetic and chemical approach, we show that the dynamics of tip actin are regulated by Rop signaling and are critical for cell polarity development and tip growth in pollen tubes.
|
Materials and Methods |
|---|
|
TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
|---|
DNA Manipulation and Plasmid Constructs
All plasmids used for transient expression in pollen were constructed in a derivative of the pBI221 vector (CLONTECH Laboratories, Inc.), termed pLAT52, in which CaMV 35S::GUS was replaced with the LAT52 promoter (
Particle Bombardment–mediated Transient Expression in Tobacco Pollen
Nicotiana tabacum plants were grown in growth chambers at 22°C under a light regime of 12 h darkness and 12 h light. Pollen grains collected from these plants were used for transient expression using a particle bombardment procedure (8 or 11 cm, respectively). Rupture disks of 1,100 psi were chosen to accelerate macrocarriers under a vacuum of 27 inches of mercury.
Gold particles (1.0 µm diameter) were coated with plasmid DNA according to the manufacturer's procedures (Bio-Rad Laboratories) immediately before bombardment. Routinely, 0.5-mg particles were coated with 0.8 µg of pLAT52::GFP-mTalin DNA or a mixture of 0.8 µg of pLAT52::GFP-mTalin DNA with 0.4 µg of a second plasmid DNA containing a gene of interest. As control, the pLAT52 vector DNA was cobombarded with the pLAT52::GFP-mTalin.
Bombarded pollen grains were incubated at room temperature for 30 min before being washed into petri dishes with 0.5 ml GM. The pollen grains were then either treated with Latrunculin B or incubated for an additional 3–6 h before observation under a inverted microscope (model TE300; Nikon) equipped with a cooled CCD camera (model C4742-95; Hamamatsu) or confocal microscope as described below.
Drug Treatments
To determine the effect of caffeine or Latrunculin B on the actin organization in tobacco pollen tubes, pollen grains bombarded with pLAT52::GFP-mTalin were incubated for 3.5 h before the addition of drugs. For caffeine treatment, a stock solution of 0.5 M caffeine (Sigma-Aldrich) was added to germinated pollen to a final concentration of 0.3 mM. For Latrunculin B treatment, a stock solution of 5 mM Latrunculin B (Calbiochem) prepared in anhydrous DMSO (Sigma-Aldrich) was added to germinated pollen for a final concentration of 5 nM. Because the final concentration of DMSO in the medium was 1 ppm after Latrunculin B was added, an equivalent concentration of DMSO was added to the medium of all untreated controls. Pollen tubes were incubated for an additional 30 min before observation.
To study the effects of Latrunculin B treatment on pollen tubes overexpressing Rop1At or DN-rop1At, Latrunculin B was added to germinated pollen 1.5 h after bombardment. Treated pollen tubes were incubated for an additional 3 h before being analyzed for polar growth or actin organization as described below.
Visualization and Analyses of F-actin using GFP-mTalin and Confocal Microscopy
To visualize F-actin in pollen tubes, the GFP-mTalin chimeric gene was transiently expressed in pollen as described above. Tubes expressing GFP-mTalin were identified using epifluorescence microscopy and observed either under an OPTIPHOT upright microscope (Nikon) equipped with an MRC 600 laser scanning device (Bio-Rad Laboratories) or an Axioplan2 microscope equipped with an LSM 510 laser scanning system (ZEISS). In either case, 1-µm optical sections were scanned and captured using Comos or LSM 510 software, respectively. Confocal images were analyzed using the Metamorph v4.5 software (Universal Imaging Corp.) and processed using Adobe Photoshop® v5.5. For three-dimensional reconstruction, serial optical sections were taken for each tube. For a given treatment, 40–70 pollen tubes were observed from several independent experiments and the percentage of tubes with a specific actin-staining pattern was determined. For time–sequence analyses, either midplane sections or cortical sections of the tip were scanned every 15 s.
Analyses of Correlation between Tip F-actin and Elongation Rates
To analyze the correlation between tip-localized F-actin and pollen tube elongation, we used the time serials of midplane optical sections scanned every 15 s from pollen tubes expressing GFP-mTalin. Using Metamorph v4.5, a region of the apical dome (17.5 µm2, 4 µm from the extreme tip) was created. Using the measurement function, the average fluorescence intensity in this region was measured and subtracted from background fluorescence, which was determined using background function in a region created from the darkest area near the tip of the tube. The corrected average intensity of GFP fluorescence was used to represent relative amounts of F-actin at the tip. Elongation rates were determined from the same images used for measuring apical F-actin. Using the Metamorph v4.5 measurement function, the distance between the base and the leading edge of the images was determined. Pollen tube elongation rates (µm/min) were calculated as differences in distances between two images over the time interval of 15 s.
Morphological Analyses of Pollen Tubes
To determine the effect of Latrunculin B treatment on changes in polar growth of pollen tubes caused by Rop1At or DN-rop1At overexpression, we measured the width and length of pollen tubes cobombarded with the GFP-mTalin construct after Latrunculin B treatment. Exactly 3 h after pollen tubes were treated with different concentrations of Latrunculin B as described above, images of fluorescent tubes were rapidly recorded through a cooled CCD camera (model C4742-95; Hamamatsu) attached on an Eclipse inverted microscope (model TE300; Nikon). The images were analyzed using the Metamorph v4.5 measurement function. The degree of depolarized growth was determined by measuring the diameter of the widest region of the tube, and the degree of polar growth was determined by measuring the length of pollen tubes. For each treatment, data were collected from three independent experiments (40–80 tubes). Data were subjected to a statistic test using Sigmastat (Hallogram).
Online Supplemental Material
A video (available at http://www.jcb.org/cgi/content/full/152/5/1019/DC1) of images of the tip-localized short actin bundle (SAB) was prepared using QuickTime® v4.0. The images were a time serial (15 s intervals for a period of 12 min) of mid-plane optical sections of a tube expressing GFP-mTalin. Images for the first 2 min 45 s are also shown in Fig 1 C.
|
|
Results |
|---|
|
TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
|---|
F-actin Is Present at the Tip of Pollen Tubes and Is Highly Dynamic
To visualize actin dynamics in pollen tubes, we constructed a chimeric gene encoding an enhanced GFP mutant (24% of tubes expressing GFP-mTalin (Fig 1 B). We also observed short bundles or patches apparently composed of short and fine actin filaments in the extreme apex in 85% of tubes examined (Fig 1 A). We termed this F-actin short actin bundle (SAB).
Our observations suggest that the subapical actin collar and apical SAB may represent one or more populations of highly dynamic F-actin. Thus, we performed a temporal analysis of GFP-mTalin localization by scanning the midplane or the cortex of the apical region. Because repeated laser scanning caused fluorescence bleaching and growth inhibition, we had to limit our minimal time intervals of laser scanning to 15 s, which allowed visualizing F-actin over a period of 5–10 min without significant fluorescence bleaching or growth inhibition. As shown in Fig 1C and Fig D (Fig 1 C is also shown in a video, available at http://www.jcb.org/cgi/content/full/152/5/1019/DC1), both SAB and the actin collar were very dynamic. The appearance of these structures seems to alternately oscillate every 60–75 s in actively growing tubes, i.e., the appearance of SAB was generally associated with reduction or disappearance of the actin collar and vice versa. These results support the notion that these two types of actin structures belong to the same actin population that is subject to both temporal and spatial regulation.
Overexpression of DN-rop1At Mutants Disrupted SAB at the Tip but Induced a Transverse Actin Band behind the Tip
To assess the involvement of Rop in the regulation of tip F-actin, we coexpressed GFP-mTalin with a DN-rop1At mutant in tobacco pollen tubes, which has been shown to inhibit tube growth and cause slight tube expansion when overexpressed in Arabidopsis pollen (32% of them had drastically reduced SAB levels; only 8% of pollen tubes were seen with a similar amount of apical actin as wild-type tubes. We did not observe significant changes in axial actin cables in DN-rop1At tubes (Fig 2 B). Surprisingly, we also observed a transverse actin band composed of cortical actin hoops just behind the apical dome in DN-rop1At cells. Time–sequence analyses showed that the transverse actin band was quite stable and actually widened over time, apparently due to actin polymerization behind the apical dome (data not shown). The DN-rop1At–induced transverse actin band could be caused by DN-rop1At–induced growth inhibition, direct effects of DN-rop1At, or indirect effects of DN-rop1At that result in increased Rop activity behind the tip, because DN-rop1At overexpression causes ectopic localization of wild-type Rop proteins in the subapical region of the PM (Wu, G., Y. Fu, and Z. Yang, unpublished data).
|
To determine whether growth inhibition was responsible for transverse actin band formation, we treated pollen tubes with Latrunculin B or caffeine. As shown in Fig 2C and Fig D, neither caffeine (3 mM) nor Latrunculin B (5 nM) induced a transverse actin band, although both drugs inhibited tube elongation dramatically (see Table 1), indicating that growth inhibition itself does not cause transverse actin band formation. Latrunculin B treatment disrupted both the actin collar and SAB, leading to the protrusion of actin cables to the extreme tip (Fig 2 D and 5 D). These results also suggest that the subapical actin collar and apical SAB represent the population of F-actin that is highly sensitive to Latrunculin B, as proposed by
|
Rop1At Overexpression Induced the Formation of an Apical Actin Network and Transverse Actin Band
If the abnormal transverse actin band is caused by Rop proteins ectopically localized to PM behind the apex, we expect that overexpression of wild-type Rop1At would also induce the transverse actin band. Indeed, Rop1At overexpression resulted in an actin band very similar to that induced by DN-rop1At overexpression (Fig 3). However, the cortical actin band in Rop1At-overexpressing cells was somewhat narrower than seen with DN-rop1At tubes (Fig 3). More importantly, Rop1At overexpression induced the formation of an apical actin network composed of fine long actin filaments in place of SAB seen in wild-type tubes. This is in sharp contrast with the F-actin–free apex in DN-rop1At–overexpressing tubes.
|
Because Rop1At overexpression induces tube expansion or tip swelling, we sought to assess the causal relationship between depolarized growth and the transverse actin band. Time–sequence analyses indicate that the transverse actin band appeared before or at the onset of tip swelling in tubes overexpressing Rop1At. As shown in Fig 3 C, a few transverse actin filaments began to accumulate near the apex at time 0, when the shape of the tube was still normal. At 5 min, an intense transverse actin band was already formed, whereas the tip just started to expand slightly. In the next 15 min, the tip had expanded considerably, whereas the intensity of the transverse actin band did not increase accordingly. These results suggest that transverse actin band formation was not the direct consequence of depolarization of tube growth, but was directly induced by ectopically localized Rop1At as a result of its overexpression (
Guanine Nucleotide Dissociation Inhibitor Suppressed Transverse Actin Band Formation Induced by Rop1At or DN-rop1At
To test the hypothesis that the transverse actin band is caused by ectopically localized Rop1At, we investigated the effect of guanine nucleotide dissociation inhibitor (GDI) overexpression on actin organization. In mammalian cells, GDIs act to recycle Rho GTPases from PM, and thus we suspect that Arabidopsis GDIs may have a similar role in pollen tubes. We found that overexpression of an Arabidopsis GDI in tobacco pollen tubes indeed suppressed transverse actin band formation (Fig 4, B–E). As shown in Fig 4 H, the transverse actin band was observed in 65% of tubes overexpressing Rop1At alone, but only in 20% of tubes cooverexpressing Rop1At and GDI. Similarly, 59% of tubes overexpressing DN-rop1At had a transverse actin band, whereas cooverexpression with GDI reduced the transverse actin band–containing tubes to 3.7% (Fig 4 H). The GDI suppression of Rop1At-induced depolarized growth was tightly correlated with that of the transverse actin band (i.e., none of the tubes devoid of the transverse actin band had swollen tips or expanded tubes). Interestingly, a meshwork composed of SABs was observed in tubes cooverexpressing Rop1At and GDI, whereas tubes cooverexpressing DN-rop1At and GDI had an actin-free apex, as in tubes overexpressing DN-rop1At alone. Hence, these results not only provide evidence that ectopically localized Rop is responsible for the formation of abnormal actin bands behind the apex, but also suggest that Rop1At is involved in the regulation of SABs found in the extreme apex.
|
RopGAP1 Overexpression Disrupted SABs at the Tip and Suppressed DN-rop1At– or Rop1At-induced Transverse Actin Band Formation
To further understand the role of Rop1At activity in regulating the dynamics of F-actin in pollen tubes, we investigated the effect of overexpressing RopGAPs on actin organization in pollen tubes. Biochemical studies indicate that RopGAP1 is a negative regulator of Rop1At by promoting the conversion of the GTP-bound form of Rop1At to the GDP-bound form (
Overexpression of RopGAP1 alone reduced or disrupted SAB, but had no effects on axial actin cables (Fig 4 F), analogous to the effect of DN-rop1At overexpression. However, in contrast to DN-rop1At, RopGAP1 overexpression did not cause transverse actin band formation behind the apex (Fig 4 F), further confirming that the actin band was not induced by Rop1At inactivation or by tube elongation inhibition as shown above. On the contrary, the actin collar observed in normal tubes was never found in RopGAP1-overexpressing tubes. The disruption of both SAB and the actin collar is tightly associated with the reduction in both elongation and expansion of pollen tubes induced by RopGAP1 overexpression (Fig 4; Wu, G., Y. Fu, and Z. Yang, unpublished data).
When RopGAP1 was cooverexpressed with Rop1At, the transverse actin band was no longer formed (Fig 4 G). As shown in Fig 4 I, increasing the ratio of RopGAP1 to Rop1At led to a decreasing percentage of tubes containing the cortical actin band. The absence of the transverse actin band was consistently associated with the actin pattern seen in wild-type tubes, i.e., the presence of the dynamic SAB and actin collar. Furthermore, the reversal of Rop1At-induced actin pattern by RopGAP1 was also tightly associated with the restoration of wild-type pollen tube morphology and elongation rate. These results strongly suggest that Rop regulates polar growth at least in part through the control of the organization of dynamic F-actin at the tip of pollen tubes. These observations also suggest that the tip-localized activation of Rop most likely turns on actin assembly at the tip.
Acting as a negative control, cooverexpression with a RopGAP mutant (in which Rop interaction domains were removed) or an empty vector did not affect the changes in actin organization and tube morphology induced by Rop1At (data not shown), demonstrating that RopGAP1 or GDI co-overexpression had no effects on the expression of Rop1At or DN-rop1At.
Latrunculin B Reversed the Abnormal Actin Patterns and Depolarized Growth Induced by Rop1At Overexpression
We next sought to test whether the Rop1At-induced transverse actin band is due to stabilization of the actin collar and increased actin assembly at the subapical region by ectopically localized Rop using the actin-depolymerizing drug Latrunculin B. Latrunculin B disassembles F-actin specifically through sequestering G-actin (202 µm, much shorter than untreated tubes (352 µm). Latrunculin B did not significantly affect pollen tube morphology, as both treated and untreated tubes have a tube diameter 10 µm.
|
Interestingly, 20–30 min after Latrunculin B treatment, the transverse actin band disappeared from the majority of tubes overexpressing DN-rop1At (only 5.6% of tubes with transverse actin band compared with 54.5% in untreated tubes) or Rop1At (17.2% compared with 56.7% in untreated tubes) (Fig 5E, Fig G, and Fig H). Moreover, treatments of Rop1At-overexpressing tubes with 5 nM Latrunculin B restored the dynamic apical F-actin observed in wild-type tubes (Fig 5 E). Time–sequence analyses of tip-localized F-actin showed that the amount of tip-localized actin fluctuated in a comparable manner between wild-type tubes and Latrunculin B–treated Rop1At-overexpressing tubes (Fig 5 H). In contrast, the amount of tip-localized F-actin exhibited little fluctuation in untreated Rop1At-overexpressing tubes (Fig 5 H). Finally, Latrunculin B–treated DN-rop1At tubes showed F-actin localization patterns similar to those of tubes overexpressing RopGAP1 and those cooverexpressing DN-rop1At and GDI (compare Fig 5 G with Fig 4E and Fig F). These results strongly indicate that Rop GTPases play a crucial role in controlling the dynamics of tip F-actin in pollen tubes.
We then determined whether the rescue of actin organization in Rop1At-overexpressing cells by Latrunculin B leads to the recovery of normal tip growth. 3 h after Latrunculin B treatment, the length and the maximal width of pollen tubes were measured. As shown in Table 1 and Fig 6, Latrunculin B treatments suppressed tube expansion or tip swelling induced by either Rop1At or DN-rop1At overexpression. Latrunculin B treatment reduced the width of Rop1At-overexpressing pollen tubes from 19 to 12 µm. Similarly, this treatment also reduced the width of DN-rop1At tubes from 14 to 12 µm. These results suggest that Rop controls the polarity of pollen tube growth via dynamic tip-localized F-actin.
|
Latrunculin B–induced reduction in tip expansion in tubes overexpressing Rop1At or DN-rop1At was correlated with an increase in tube elongation. At 4.5 h after bombardment, Rop1At tubes elongated significantly faster, to 438 µm when treated with 5 nM Latrunculin B compared with 339 µm in untreated tubes (Table 1 and Fig 6). Latrunculin B–treated DN-rop1At tubes (128 µm) were also longer than nontreated tubes (96 µm) on the average, though the difference is not statistically significant. Interestingly, Latrunculin B–treated Rop1At-overexpressing tubes (438 µm) elongated much faster than the control, wild-type tubes (352 µm). This surprising result provides strong evidence for the role of actin dynamics in the regulation of pollen tube growth.
To further assess the role of actin dynamics in pollen tube growth, we tested the effect of various concentrations of Latrunculin B on tubes overexpressing Rop1At. As shown in Table 2, treatments with Latrunculin B as low as 1 nM somewhat reduced the width of tubes and promoted tube elongation. However, 5 nM Latrunculin B was optimal for promoting elongation, as well as inhibiting expansion. High concentrations of Latrunculin B (e.g., 30 nM) inhibited elongation more severely than expansion (shorter tubes with greater width to length ratio than untreated Rop1At tubes), presumably due to the disruption of actin cables (Fig 5 F;
|
The Abundance of Tip-localized SABs Oscillates and Increases before Growth
To understand how the dynamics of the tip-localized actin are involved in the control of tip growth, we determined the relationship between actin dynamics and growth oscillation. Growth oscillation has been shown to occur in pollen tubes from various plant species, including tobacco (15–30 s, although a more refined time-lapse imaging may allow deciphering of a more accurate phasic relationship. However, the amplitude of a GFP peak correlated with that of the following growth peak. Interestingly, the apex of a GFP peak generally coincided with the base of a growth peak. These results provide evidence that tip F-actin plays a role in events that precede tip growth.
|
|
Discussion |
|---|
|
TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
|---|
In this study, we have used chemical genetic analysis in conjunction with live imaging of the actin cytoskeleton to demonstrate that the dynamics of an actin structure localized to the site of growth plays an essential role in the development of cell polarity and polar growth in pollen tubes. Importantly, the dynamics of this actin is dependent on the signaling of a plant-specific Rho-type GTPase, Rop. This study provides the first direct evidence to link F-actin to polarity development through a Rho GTPase in plant cells. This extends the common theme of Rho GTPase–mediated cell polarity control to the plant system (
The Apex of Pollen Tubes Contains a Highly Dynamic Cortical Actin Structure
The actin cytoskeleton has been implicated in many aspects of plant cell growth, division, and development (
One of the major challenges in studying the actin cytoskeleton in the plant cell has been difficulties in faithfully visualizing F-actin and its dynamics. Chemical fixation methods frequently fail to detect dynamic and fine actin filaments and may cause dramatic structural alteration (
Our current study, using an enhanced GFP mutant (S65C) to tag mTalin, has uncovered a dynamic population of tip-localized SABs in tobacco pollen tubes. We believe that the use of this improved GFP mutant was critical, because it produces much more intense fluorescence compared with the GFP (S65T) mutant used previously (
In addition to SAB, GFP-mTalin also revealed another F-actin structure localized just behind the extreme apex, similar to an actin ring or actin collar described previously (
Rop Controls the Formation and the Dynamics of F-actin at the Tip of Pollen Tubes
Our current results indicate that the formation and the dynamics of tip F-actin are controlled by Rop GTPase activity localized to the apex of the pollen tube PM. Several lines of evidence strongly support this conclusion. First, RopGAP1 overexpression in tobacco pollen tubes drastically reduced SAB and completely removed the actin collar. Second, Rop1At overexpression, which led to ectopic accumulation of Rop proteins to the apical region of PM (
Our results suggest that Rop controls the dynamics of tip actin by promoting actin assembly, as do Rop-related Cdc42 and Rac GTPases in mammalian cells. First, Rop1At overexpression induced the formation of long actin filaments in the apex of pollen tubes, suggesting that increased actin polymerization allows SAB to become long filaments. Second, treatments of Rop1At-overexpressing tubes with the G-actin sequestering drug Latrunculin B completely recovered normal actin dynamics by suppressing the formation of the apical long actin filaments and subapical transverse actin band. Finally, SAB was disrupted by either deactivation of Rop or by Latrunculin B treatments in wild-type tubes. A role for Rop in promoting actin polymerization is also supported by a recent study suggesting that a phosphatidylinositol 4,5-bisphosphate (PIP) kinase and PIP2 may be a Rop effector in tobacco pollen (
Both transient deactivation of Rop and actin disassembly at the tip could contribute to the dynamics of the tip actin. Potential factors that control actin disassembly at the tip include profilin, actin-depolymerizing factor, gelsolin, and calcium (
|
The calcium-dependent actin disassembly at the tip may also explain the formation of the actin collar in normal tubes and the transverse actin band in Rop1At-overexpressing tubes. Although actin disassembly at the tip is activated by high calcium, polymerization just behind the tip may continue, contributing to the formation of the actin collar. Moreover, as discussed below, Rop1At overexpression-induced transverse actin band probably results from the stabilization of the collar actin by ectopically localized Rop in the subapical region, where calcium-dependent actin disassembly is absent or minimal.
The Rop-dependent Tip F-actin Controls Cell Polarity Development in Pollen Tubes
Our previous studies indicate that localized Rop activity specifies the site for tip growth (
The Dynamics of Apical SABs Couple Cell Polarity Control with Growth Control
Our study suggests that SAB is also critical for pollen tube growth. The actin cable–independent effect of Latrunculin B treatments suggests that a population of F-actin is required for pollen tube growth but not cytoplasmic streaming (
The requirement of Rop-mediated SAB for both growth and polarity controls is consistent with our previous finding that Rop couples growth and polarity control during pollen tube tip growth. Together, our studies provide strong evidence for the model of Rop-mediated tip growth: a localized tip growth cue activates Rop at the extreme apex of the tube and activated Rop then controls polarized organization of SAB to the site of growth. It remains to be determined how polarized SAB regulates tip growth. An attractive model is that SAB targets vesicles to the site of growth. A high density of vesicles accumulates at the extreme apex of the tube (
Regardless of the mode of action for SAB, it is intriguing that the function of Rop and SAB in pollen tubes is very analogous to that of Cdc42 and cortical actin patches in the tip-growing fission yeast: Cdc42 and actin patches are involved in both cell polarity establishment and growth control (
Potential Cross-Talk between Actin and Calcium via Rop in Pollen Tube Growth
Rop also regulates the formation of the tip-focused calcium gradient (
We favor the model that Rop regulates actin and calcium independently (Fig 8 A). Tip-localized Rop could activate two distinct Rop effectors that are involved in the control of calcium gradient formation and tip actin dynamics, respectively. Alternatively, Rop could activate a single effector, and the calcium and actin pathways bifurcate downstream of this effector. A potential Rop effector of this sort is a phosphotidylinositol phosphate kinase and its product, PIP2 (
|
Footnotes |
|---|
The online version of this article contains supplemental material. 
1 Abbreviations used in this paper: CA, constitutively active; DN, dominant negative; GAP, GTPase-activating protein; GDI, guanine nucleotide dissociation inhibitor; GFP, green fluorescent protein; GM, germination medium; mTalin, mouse talin; PIP, phosphatidylinositol 4,5-bisphosphate; PM, plasma membrane; SAB, short actin bundle.
|
Acknowledgements |
|---|
|
TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgementsReferences |
|---|
We would like to thank Elizabeth Lord and Eugene Nothnagel for critical reading and comments on this manuscript, and Veronica Franklin-Tong, Chris Staiger, Ming Yuan, and members of Z. Yang's laboratory for helpful discussion.
This work is supported by a grant to Z. Yang from the National Science Foundation (MCB-0096026).
Submitted: 20 November 2000
Revised: 16 January 2001
Accepted: 16 January 2001
|
References |
|---|
|
TopAbstractIntroductionMaterials and MethodsResultsDiscussionAcknowledgements |
|---|
) and elongation rates (
) of this tube were determined using Metamorph v4.5 software as described in Materials and Methods. Y-axis values are arbitrary units of fluorescence intensity; x-axis indicates times after the first laser section.