Propidium Iodide Competes with Ca2+ to Label Pectin in Pollen Tubes and Arabidopsis Root Hairs

We have used propidium iodide (PI) to investigate the dynamic properties of the primary cell wall at the apex of Arabidopsis (Arabidopsis thaliana) root hairs and pollen tubes and in lily (Lilium formosanum) pollen tubes. Our results show that in root hairs, as in pollen tubes, oscillatory peaks in PI fluorescence precede growth rate oscillations. Pectin forms the primary component of the cell wall at the tip of both root hairs and pollen tubes. Given the electronic structure of PI, we investigated whether PI binds to pectins in a manner analogous to Ca²⁺ binding. We first show that Ca²⁺ is able to abrogate PI growth inhibition in a dose-dependent manner. PI fluorescence itself also relies directly on the amount of Ca²⁺ in the growth solution. Exogenous pectin methyl esterase treatment of pollen tubes, which demethoxylates pectins, freeing more Ca²⁺-binding sites, leads to a dramatic increase in PI fluorescence. Treatment with pectinase leads to a corresponding decrease in fluorescence. These results are consistent with the hypothesis that PI binds to demethoxylated pectins. Unlike other pectin stains, PI at low yet useful concentration is vital and specifically does not alter the tip-focused Ca²⁺ gradient or growth oscillations. These data suggest that pectin secretion at the apex of tip-growing plant cells plays a critical role in regulating growth, and PI represents an excellent tool for examining the role of pectin and of Ca²⁺ in tip growth.The apical wall of tip-growing cells participates directly in the process of growth regulation (McKenna et al., 2009; Winship et al., 2010), yet few methods permit monitoring the wall properties of living cells. Despite this, several recent studies have enhanced our understanding of the apical cell wall. Chemical analyses of isolated pollen tube wall material have revealed a complex mixture of pectic polysaccharides with regions comprising long sequences of polygalacturonic acid. Important patterns of pectin methoxylation have been detected using immunocytochemical approaches, but these are limited to fixed cells (Dardelle et al., 2010). In a recent study, Parre and Geitmann (2005) used microindentation to show significant correlations between wall strength and growth rate. None of these techniques allow for easy investigation of the cell wall during growth.In an earlier study, we found that propidium iodide (PI) vitally stains pollen tubes of lily (Lilium formosanum) and tobacco (Nicotiana tabacum) and in particular reveals with great clarity the thickened apical cell wall (Fig. 1; McKenna et al., 2009). In addition, the apical PI fluorescence oscillates and in lily pollen tubes correlates tightly with oscillations in wall thickness measured by differential interference contrast (DIC) optics. Finally, these studies indicated that the PI fluorescence predicted cell growth rates with high confidence, suggesting that PI binding may provide useful information about the physical and chemical properties of the cell wall.Open in a separate windowFigure 1.PI fluorescence and growth rate oscillate in lily pollen tubes (A and B), Arabidopsis root hairs (C–E), and Arabidopsis pollen tubes (F and G). A, The top panel shows a DIC image of a lily pollen tube, and the bottom panel shows PI fluorescence of the same tube. The PI fluorescence is pseudocolored, with white representing high signal and blue representing low signal. Bar = 10 μm. B, Growth rate (blue) and PI fluorescence (red) are plotted on a line graph. Both oscillate with the same period but with different phases. C, DIC image (top panel) and PI fluorescence image (bottom panel) of an Arabidopsis root hair. Bar = 10 μm. D, Two PI fluorescence images of the same root hair focused on the apex representing peak (top) and trough (bottom) PI signals. Bar = 5 μm. E, A line graph showing the growth rate (blue) and peak PI fluorescence at the apex (red) for the same root hair shown in C and D. F, The top panel shows a DIC image of an Arabidopsis pollen tube, and the bottom panel shows PI fluorescence of the same tube. The PI fluorescence is pseudocolored, with white representing high signal and blue representing low signal. Bar = 5 μm. G, Growth rate (blue) and PI fluorescence (red) are plotted on a line graph. Both oscillate with the same period but with different phases. The growth rate between individual 3-s frames was smaller than the pixel size for our optics in both Arabidopsis cell types; to remove the noise this generated, a four-image (pollen) or five-image (root hair) running average is shown. A.U., Arbitrary units.PI is commonly used to visualize plant cell walls by wide-field fluorescence and confocal microscopy (Fiers et al., 2005; Tian et al., 2006; Estevez et al., 2008) and to select viable cells during cell sorting (Deitch et al., 1982; Jones and Senft, 1985). A positively charged phenanthridine derivative, the propidium ion stains cell walls but does not pass through the intact cell membranes of living cells. It readily diffuses into dead cells and forms highly fluorescent complexes by intercalation between base pairs of double-stranded nucleic acids, thus acting as an excellent indicator for cell vitality (Hudson et al., 1969). Binding to cell walls presumably occurs by a different mechanism, since it is not accompanied by the dramatic increase in fluorescence and shift in absorption and emission maxima observed when PI binds to nucleic acids. The mechanism of PI binding needs further exploration, as does the potential for broader use in other tip-growing plant cells.In this report, we test two hypotheses: first, that PI stains other tip-growing cells with pectin-containing cell walls; and second, that PI and Ca²⁺ bind to the same sites in these walls. This binding would occur through the interaction of partial positive charges caused by localized deficits in π-orbital electrons associated with three of the four nitrogen atoms of PI (Luedtke et al., 2005) coordinating with negatively charged carboxyl and hydroxyl groups on homogalacturonans (HGs), as has been suggested in Oedogonium bharuchae (Estevez et al., 2008).Our findings indicate that both hypotheses are satisfied. Notably, oscillatory changes in apical PI fluorescence occur and are observed to anticipate oscillations in growth rate in Arabidopsis (Arabidopsis thaliana) root hairs and Arabidopsis pollen tubes. In addition, competition studies indicate that PI and Ca²⁺ bind to the same sites in cell walls. Supporting these studies, we demonstrate that pectin methyl esterase (PME) creates more sites for PI binding, presumably by demethoxylating HGs as they are secreted, and that pectinase reduces PI fluorescence dramatically. However, unlike other pectin-binding dyes, PI does not block Ca²⁺ channels at the concentration used in live cell studies, nor does it alter oscillatory growth characteristics. Our findings provide evidence that PI may be employed as a quantitative measure of Ca²⁺-binding sites and thus may have use as an indicator of the degree of cross-linking of HGs and of cell wall extensibility.