Elucidating the Role of Transport Processes in Leaf Glucosinolate Distribution

In Arabidopsis (Arabidopsis thaliana), a strategy to defend its leaves against herbivores is to accumulate glucosinolates along the midrib and at the margin. Although it is generally assumed that glucosinolates are synthesized along the vasculature in an Arabidopsis leaf, thereby suggesting that the margin accumulation is established through transport, little is known about these transport processes. Here, we show through leaf apoplastic fluid analysis and glucosinolate feeding experiments that two glucosinolate transporters, GTR1 and GTR2, essential for long-distance transport of glucosinolates in Arabidopsis, also play key roles in glucosinolate allocation within a mature leaf by effectively importing apoplastically localized glucosinolates into appropriate cells. Detection of glucosinolates in root xylem sap unambiguously shows that this transport route is involved in root-to-shoot glucosinolate allocation. Detailed leaf dissections show that in the absence of GTR1 and GTR2 transport activity, glucosinolates accumulate predominantly in leaf margins and leaf tips. Furthermore, we show that glucosinolates accumulate in the leaf abaxial epidermis in a GTR-independent manner. Based on our results, we propose a model for how glucosinolates accumulate in the leaf margin and epidermis, which includes symplasmic movement through plasmodesmata, coupled with the activity of putative vacuolar glucosinolate importers in these peripheral cell layers.Feeding behavior of herbivorous insects and distribution of defense compounds in plants have been suggested to be a result of an arms race between plants and insects that has spanned millions of years (Ehrlich and Raven, 1964). Whether insects adapted first to plants or the other way around is an ongoing debate in this research field (Schoonhoven et al., 2005; Ali and Agrawal, 2012). Leaf margin accumulation of defense compounds has been demonstrated in various plant species (Gutterman and Chauser-Volfson, 2000; Chauser-Volfson et al., 2002; Kester et al., 2002; Cooney et al., 2012). In the model plant Arabidopsis (Arabidopsis thaliana), higher concentration of glucosinolates, which constitute a major part of the chemical defense system in this plant (Kliebenstein et al., 2001a; Halkier and Gershenzon, 2006), was found at the leaf midrib and margins compared with the leaf lamina (Shroff et al., 2008; Sønderby et al., 2010). This nonuniform leaf distribution of glucosinolates appeared to explain the feeding pattern of a generalist herbivore (Helicoverpa armigera), as it avoided feeding at the leaf margin and midrib (Shroff et al., 2008). A similar feeding pattern on Arabidopsis was observed for a different generalist herbivore, Spodoptera littoralis (Schweizer et al., 2013). Interestingly, S. littoralis was shown to favor feeding from Arabidopsis leaf margins in glucosinolate-deficient mutants (Schweizer et al., 2013), which could indicate an inherent preference for margin feeding and that Arabidopsis adapted to such behavior by accumulating defense compounds here. A damaged leaf margin may be more critical for leaf stability than damage to inner leaf parts (Shroff et al., 2008), further motivating protection of this tissue. The margin-feeding preference of S. littoralis might be explained by better nutritional value of the leaf margin cells (Schweizer et al., 2013), which has been shown to consist of specialized elongated cell files (Koroleva et al., 2010; Nakata and Okada, 2013).Other distribution patterns have been reported for glucosinolates in an Arabidopsis leaf. A study investigating spatiotemporal metabolic shifts during senescence in Arabidopsis reported that fully expanded mature leaves exhibited a glucosinolate gradient from base to tip, with highest level of glucosinolates at the leaf base (Watanabe et al., 2013). In contrast to the horizontal plane, less has been reported on distribution of glucosinolates in the vertical plane of a leaf. A localization study of cyanogenic glucosides, defense molecules related to glucosinolates (Halkier and Gershenzon, 2006), determined that these compounds primarily were located in the epidermis of sorghum (Sorghum bicolor; Kojima et al., 1979). Whereas epidermis-derived trichomes in Arabidopsis were recently demonstrated to contain glucosinolates and to express glucosinolate biosynthetic genes (Frerigmann et al., 2012), no studies have investigated glucosinolates in the epidermal cell layer.Based on promoter-GUS studies, biosynthesis of glucosinolates in leaves of Arabidopsis has been associated with primarily major and minor veins in leaves and silique walls (Mikkelsen et al., 2000; Reintanz et al., 2001; Tantikanjana et al., 2001; Chen et al., 2003; Grubb et al., 2004; Schuster et al., 2006; Gigolashvili et al., 2007; Li et al., 2011; Redovniković et al., 2012). The discrepancy between vasculature-associated glucosinolate biosynthesis and margin accumulation of glucosinolates suggests that transport processes must be involved in establishing the distribution pattern of glucosinolates within a leaf.Plant transport systems include the apoplastic xylem, the symplastic phloem, and plasmodesmata. Xylem transport is mainly driven by an upward pull generated by transpiration from aerial plant organs, thereby directing transport to sites of rapid evaporation (such as leaf margins; Sattelmacher, 2001). Phloem flow is facilitated by an osmosis-regulated hydrostatic pressure difference between source and sink tissue, primarily generated by Suc bulk flow (Lucas et al., 2013). Plasmodesmata are intercellular channels that establish symplasmic pathways between neighboring cells, and most cell types in a plant are symplastically connected via plasmodesmata (Roberts and Oparka, 2003). Translocation of small molecules in these channels is driven by diffusion and is regulated developmentally as well as spatially to form symplastically connected domains (Roberts and Oparka, 2003; Christensen et al., 2009). To what extent any of these transport processes are involved in establishing specific distribution patterns of glucosinolates within leaves is not known.Recently, two plasma membrane-localized, glucosinolate-specific importers, GLUCOSINOLATE TRANSPORTER1 (GTR1) and GTR2, were identified in Arabidopsis (Nour-Eldin et al., 2012). In leaf, their expression patterns were shown to be in leaf veins (GTR1 and GTR2) and surrounding mesophyll cells (GTR1; Nour-Eldin et al., 2012). Absence of aliphatic and indole glucosinolates in seeds of the gtr1gtr2 double knockout (dKO) mutant (gtr1gtr2 dKO) demonstrated that these transporters are essential for long-distance glucosinolate transport to the seeds and indicates a role in phloem loading (Nour-Eldin et al., 2012). Another study investigating long-distance transport of glucosinolates in the 3-week-old wild type and gtr1gtr2 dKO indicated that GTR1 and GTR2 were involved in bidirectional transport of aliphatic glucosinolates between root and shoot via both phloem and xylem pathways (Andersen et al., 2013). The authors suggested a role for GTR1 and GTR2 in the retention of long-chained aliphatic glucosinolates in roots by removing the compounds from the xylem (Andersen et al., 2013).Identification of the glucosinolate transporters GTR1 and GTR2 has provided a molecular tool to investigate the role of transport processes in establishing leaf glucosinolate distribution. In this study, we have performed a detailed spatial investigation of the distribution of an exogenously fed glucosinolate (sinigrin) and endogenous glucosinolates within mature wild-type and gtr1gtr2 dKO Arabidopsis leaves, achieved by collecting and analyzing leaf parts at the horizontal (y axis: petiole, base, and tip; x axis: midrib, lamina, and margin) as well as at the vertical leaf plane (z axis: abaxial epidermis). Furthermore, we analyze wild-type and gtr1gtr2 dKO root xylem sap and leaf apoplastic fluids for glucosinolates. Based on our results, we propose a model where GTR1 and GTR2 import glucosinolates from the apoplast to the symplast and where the glucosinolate distribution pattern within an Arabidopsis leaf is established via symplasmic movement of glucosinolates through plasmodesmata, coupled with the activity of putative vacuolar glucosinolate importers in peripheral cell layers.