Abstract
The dynamic remodeling of actin filaments in guard cells functions in stomatal movement regulation. In our previous study, we found that the stochastic dynamics of guard cell actin filaments play a role in chloroplast movement during stomatal movement. In our present study, we further found that tubular actin filaments were present in tobacco guard cells that express GFP-mouse talin; approximately 2.3 tubular structures per cell with a diameter and height in the range of 1–3 µm and 3–5 µm, respectively. Most of the tubular structures were found to be localized in the cytoplasm near the inner walls of the guard cells. Moreover, the tubular actin filaments altered their localization slowly in the guard cells of static stoma, but showed obvious remodeling, such as breakdown and re-formation, in moving guard cells. Tubular actin filaments were further found to be colocalized with the chloroplasts in guard cells, but their roles in stomatal movement regulation requires further investigation.
Key words: actin dynamics, tubular actin filaments, chloroplast, guard cell, stomatal movement
Stomatal movement responses to surrounding environment are mediated by guard cell signaling.1,2 Actin filaments within guard cells are dynamic cytoarchitectures and function in stomatal development and movement.3 Arrays of actin filaments in guard cells that are dependent on different stomatal apertures have also been reported in references 4–7. For example, the random or longitudinal orientations of actin filaments in closed stomata change to a radial orientation or ring-like array after stomata opening.5,6,8 The reorganization of the actin architecture during stomatal movement depends on the depolymerization and repolymerization of actin filaments in guard cells. In contrast to the traditional treadmill model of actin dynamic mechanisms, stochastic dynamics of actin have been revealed in plant cells, such as in the epidermal cells of hypocotyl and root, the pavement cells of Arabidopsis cotyledons, and the guard cells of tobacco (Nicotiana tabacum).9–11 In this alternative system, the short actin fragments generated from severed long filaments can link with each other to form longer filaments by end-joining activity. The actin regulatory proteins, Arp2/3 complex, capping protein and actin depolymerizing factor (ADF)/cofilin, may also be involved in the stochastic dynamics of actin filaments.12,13
Using tobacco GFP-mouse talin expression lines, we have previously analyzed the stochastic dynamics of guard cell actin filaments and their roles in chloroplast displacement during stomatal movement.6,11 We found from these analyses that another arrangement of actin filaments, i.e., tubular actin filaments, exists in the guard cells of these tobacco lines. We first found the circle-like actin filaments in 82% of the guard cells (counting 320 cells) in tobacco expressing GFPmouse talin when analyzing a single optical section (Fig. 1A). In a previous study of BY-2 cells expressing GFP-Lifeact labeled actin filaments, Smertenko et al. found similar structures, i.e., quoit-like structures or acquosomes in all of the plant tissues examined except growing root hairs.10 However, in our present analysis of serial sections, we determined that the circle-like actin filaments in the tobacco guard cells were long tubes (Fig. 1A), as the lengths (about 3–5 µm) of these structures were greater than their diameter (about 1–3 µm). Hence, we denoted these structures as tubular actin filaments to distinguish them from the circular conformations of actin filaments observed previously in other plant cell tissues.10,14–19 About 2.3 of these tubular actin filaments were found per guard cell, which is less than the number of acquosomes reported in BY-2 cells (about 6.7 per cell).10 Analysis of serial optical sections at the z-axis revealed that the tubular actin filaments localize in the cytoplasm near the inner walls of the guard cells (Fig. 1B), which is similar to the distribution of chloroplasts in guard cells.11 Longitudinal sections further revealed a colocalization of tubular actin filaments and chloroplasts (Fig. 1B).
Figure 1.
Tubular actin filaments in the guard cells of a tobacco (Nicotiana tabacum) line expressing GFP-mouse talin. (A) Optical-sections (interval, 1.5 µm) of guard cells in a moving stoma showing tubular actin filaments (arrow heads). Frames (a1) and (a2) are cross sections of 1.5-µm-picture through the yellow and red lines, respectively, revealing the cross section of the circle structures are parallel lines (arrows). (B) Optical-sections of a stoma from the outer periclinal walls to the inner walls of the guard cells (interval, 1 µm). The tubular actin filaments (arrow heads) are localized in the cytoplasm near to the inner periclinal walls of guard cells. Frame (b1) is the guard cell on the right of the frame “4 µm”; (b2) is the cross section of b1 through the red line; and (b3) is a higher magnification image of the area encompassed by the white square in b2. Arrows indicate the colocalization between the tubular actin filaments and the chloroplast (indicated using a red pseudocolor). (C) Time-series imaging showing the movement of tubular actin filaments in the guard cells of static stomata. Frame (c1) comprises three images colored red (0 S), green (40 S) and blue (80 S), that are merged in a single frame to show the translocation of the tubular actin filaments (arrows). (D) Time-series images of the opening stomata showing the breakdown (arrows) and re-formation (arrowheads) of the tubular actin filaments. All images were captured using a Zeiss LSM 510 META confocal laser scanning microscope, as described by Wang et al.11 Bars, 10 µm.
We performed time-lapse imaging and found that the translocation of tubular actin filaments is slow in static stomata in which the distance between two tubular actin filaments typically increased from 2.22 to 2.50 µm after 80 sec (Fig. 1C). In moving stomata, however, the tubular actin filaments showed an obvious dynamic reorganization whereby they could be processed into short fragments and also reemerged after they had disintegrated (Fig. 1D). These results indicate that tubular actin filaments have stochastic dynamics that are similar to the long actin filaments of guard cells.11 In our previous study, we found that the stochastic dynamics of actin filaments correlate with light-induced chloroplast movement in guard cells.11 However, whether the dynamics of the tubular actin filaments are also involved in chloroplast movement during stomatal movement remains to be investigated. In cultured mesophyll cells which had been mechanically isolated from Zinnia elegans, Wilsen et al. previously found a close association between fully closed actin rings and chloroplasts.18 These authors further found that the average percentage of cells with free actin rings increased at the initial culture stage, and then decreased, which indicates that the formation of actin rings might be a response of the actin cytoskeleton to cellular stress or disturbance.18 The turgor pressure of guard cells is the fundamental basis of stomatal movement leading to changes in the shape, volume, wall structure, and membrane surface of guard cells.20–24 We speculate from our current data that there is a relationship between tubular actin filaments and the shape changes of guard cells during stomatal movement.
Acknowledgments
We thank Prof. Xue-Chen Wang (China Agricultural University, Beijing, China) for the kind guidance and help for this work. This work was supported by Research Fund for the Outstanding Young Scientists Foundation Grant of Shandong Province (No.BS2009SW035) and Doctoral Program of Higher Education (No.20093702120010).
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