ORIGINAL RESEARCH article
The Arabidopsis Lipid Transfer Protein 2 (AtLTP2) Is Involved in Cuticle-Cell Wall Interface Integrity and in Etiolated Hypocotyl Permeability
- 1Laboratoire de Recherche en Sciences Végétales, Université de Toulouse, Centre National de la Recherche Scientifique (CNRS), Université Paul Sabatier (UPS), Castanet-Tolosan, France
- 2Plateforme Imagerie-Microscopie, Fédération de Recherche FR3450–Agrobiosciences, Interactions et Biodiversité, Centre National de la Recherche Scientifique (CNRS), Université de Toulouse, Université Paul Sabatier (UPS), Castanet-Tolosan, France
- 3Laboratoire de Biogenèse Membranaire, UMR 5200 CNRS Université de Bordeaux–INRA Bordeaux Aquitaine, Villenave d’Ornon, France
- 4Centre de Microscopie Electronique Appliquée à la Biologie (CMEAB), Faculté de Médecine Rangueil, Toulouse III, Université Paul Sabatier (UPS), Toulouse, France
Plant non-specific lipid transfer proteins (nsLTPs) belong to a complex multigenic family implicated in diverse physiological processes. However, their function and mode of action remain unclear probably because of functional redundancy. Among the different roles proposed for nsLTPs, it has long been suggested that they could transport cuticular precursor across the cell wall during the formation of the cuticle, which constitutes the first physical barrier for plant interactions with their aerial environment. Here, we took advantage of the Arabidopsis thaliana etiolated hypocotyl model in which AtLTP2 was previously identified as the unique and abundant nsLTP member in the cell wall proteome, to investigate its function. AtLTP2 expression was restricted to epidermal cells of aerial organs, in agreement with the place of cuticle deposition. Furthermore, transient AtLTP2-TagRFP over-expression in Nicotiana benthamiana leaf epidermal cells resulted in its localization to the cell wall, as expected, but surprisingly also to the plastids, indicating an original dual trafficking for a nsLTP. Remarkably, in etiolated hypocotyls, the atltp2-1 mutant displayed modifications in cuticle permeability together with a disorganized ultra-structure at the cuticle-cell wall interface completely recovered in complemented lines, whereas only slight differences in cuticular composition were observed. Thus, AtLTP2 may not play the historical purported nsLTP shuttling role across the cell wall, but we rather hypothesize that AtLTP2 could play a major structural role by maintaining the integrity of the adhesion between the mainly hydrophobic cuticle and the hydrophilic underlying cell wall. Altogether, these results gave new insights into nsLTP functions.
In many instances, lipid synthesis and metabolism require the cooperation of various organelles and cellular structures implicating the transport of lipidic precursors/intermediates from one cellular compartment to another (Ohlrogge and Browse, 1995). Lipid Transfer Proteins (LTPs), primarily defined by their capability of transferring lipids between lipid bilayers in vitro, are good candidates to convey hydrophobic lipids within the hydrophilic intracellular spaces (Kader, 1996). In addition, plant non-specific LTPs (nsLTPs) share highly conserved structures characterized by four disulfide bridges formed by eight cysteine residues that delineate an internal hydrophobic cavity able to bind various hydrophobic compounds in vitro (Carvalho and Gomes, 2007; Liu et al., 2015). The nsLTPs are encoded by a large multigenic family in flowering plants (Boutrot et al., 2008; Edstam et al., 2011; Liu et al., 2015). Based on (i) sequence similarity, (ii) calculated molecular mass of the mature protein, (iii) presence or not of a glycosylphosphatidylinositol (GPI) modification site, and (iv) intron position, terrestrial plant nsLTPs have been grouped in 10 clades (Edstam et al., 2011). Most plant nsLTPs possess a predicted N-terminal signal peptide to target them to the secretory pathway (Edstam et al., 2011). The absence of identification of additional sorting signals to endomembrane compartments has suggested their bulk transport to the extracellular compartment and particularly to the cell wall. Some nsLTPs have been detected to the outer side of the plasma membrane where they are attached by a GPI-anchor (Liu et al., 2015). However, a recent study has shown that a sunflower nsLTP, could be re-localized intra-cellularly by endocytosis during seed imbibition, thus possibly contributing to intra-cellular transport of lipids (Pagnussat et al., 2012).
The knowledge of nsLTPs has considerably increased in recent years with the first characterization of a NMR 3D-structure, insight into their biochemical properties, description of spatio-temporal patterns of expression, and sub-cellular localization (Yeats and Rose, 2008; Liu et al., 2015). Several roles have been proposed for a few nsLTPs in diverse physiological processes, for example, cell wall loosening (Nieuwland et al., 2005), pollen exine assembly (Huang et al., 2013), sexual reproduction (Chae et al., 2010), seed development (Wang et al., 2015), response to biotic/abiotic stress (Lee et al., 2009; Guo et al., 2013; Deeken et al., 2016), symbiotic nodulation (Lei et al., 2014), and cutin and wax assembly. In the latter case, a few studies provided experimental evidence of a possible role for two plasma membrane-localized GPI-anchored nsLTPs (AtLTPG/LTPG1, AtLTPG2) in the control of the cuticle lipid composition (Debono et al., 2009; Lee et al., 2009; Kim et al., 2012). However, the description of nsLTPs mode of action remains unclear and the identification of their genuine physiological substrates is still lacking. The difficulties encountered to decipher their function are probably due to the large size of the nsLTP multigenic family implicating possible functional redundancy.
The cuticle provides a primary barrier to prevent non-stomatal water-loss, but also plays various roles during development and in response to environmental stresses (Yeats and Rose, 2013). This protective layer is a complex structure mainly composed of a lipid polymer, i.e., cutin, which is impregnated and covered by cuticular waxes (Yeats and Rose, 2013; Lee and Suh, 2015; Fernandez et al., 2016). The cuticle coats the outermost layer of periclinal cell walls of all aerial organ epidermal cells. The biosynthetic pathways of the fatty acid derivatives constituting the waxes and the cutin polymer are now well described (Yeats and Rose, 2013), but their intra-cellular trafficking is still poorly understood. In addition, if the transport across the plasma membrane of both wax and cutin precursors has been shown to be dependent on ATP-binding cassette (ABC) transporters, the transfer through the cell wall to the cuticle and the assembly mechanisms within the cuticle are still a matter of debate (Samuels et al., 2008; Bernard and Joubes, 2013; Domínguez et al., 2015). One particular paradigm that remains to be solved is how the hydrophobic cuticle layer is structurally stabilized next to the highly hydrophilic polysaccharidic cell wall.
Etiolated hypocotyls of Arabidopsis thaliana constitute a well-documented model of cell elongation (Gendreau et al., 1997; Refregier, 2004; Derbyshire et al., 2007; Pelletier et al., 2010). During a short period of active growth in darkness, no cell division occurs in hypocotyls and, consequently, growth only proceeds by cell elongation. Furthermore, the outer cuticle-periclinal wall zone has been observed to be thicker than in light-growth condition (Gendreau et al., 1997). Thus, in addition to their primary interest for elongation studies, etiolated hypocotyls could be a new attractive model to gain insight into the understanding of cuticle formation.
In this study, we have taken advantage of the fact that AtLTP2 (NP_181387/At2g38530) is the unique and abundant nsLTP that has been identified in the cell wall proteome of etiolated hypocotyls (Irshad et al., 2008) among the 49 (Boutrot et al., 2008) or 79 (Edstam et al., 2011) nsLTPs of A. thaliana. We have assumed that this feature would facilitate the search for its function and the exploration of its possible role in cuticle biogenesis. We provide evidence for spatio-temporal restricted accumulation of AtLTP2 transcripts in epidermal cells where the cuticle is synthesized and for a dual sub-cellular localization of AtLTP2 to the cell wall and plastids. We also use a reverse genetics approach to demonstrate its contribution to the control of the permeability of etiolated hypocotyls, but not to the cuticle composition and content. Finally, a topochemical ultra-structural study enables us to propose a role of AtLTP2 in maintaining the integrity of the cuticle-cell wall interface.
Generation of an atltp2-1 Mutant Line Strongly Affected at the Transcript and Protein Levels
In order to investigate the function of AtLTP2, the A. thaliana SALK_026257 insertion line in which the AtLTP2 promoter is disrupted by a T-DNA insertion (Figure 1A), was studied. A homozygous mutant line (atltp2-1) and its wild type counterpart (WT) were selected during a genotyping screen. The genomic sequence of AtLTP2 (2,783 bp), including native regulatory sequences (promoter and terminator sequences) and the unique intron (Figure 1A), was used to transform homozygous atltp2-1 plants, finally leading to the selection of 12 homozygous independent complemented lines (comp). Three of them (i.e., 5′2, 6′4, and 14′3) were selected for further studies.
FIGURE 1. atltp2-1 is a strong knock-down mutant. (A) Organization of the AtLTP2 (At2g38530) genomic sequence showing the T-DNA insertion in the SALK_026257 (atltp2-1) mutant. The displayed 2,783 bp sequence containing native regulatory sequences was cloned and used for complementation of atltp2-1. Legend: exon (ex); intron (int); UTR (untranslated region). The arrows show the position of primers used for RT-qPCR. (B) Relative AtLTP2 expression was determined by RT-qPCR for etiolated seedling kinetics at eight developmental stages in wild type (WT) (black) and atltp2-1 (white). Results represent the mean values ± SD (n = 3). Significant differences were assessed by a Student’s t-test (∗p-value < 0.05; ∗∗∗p-value < 0.001). (C) 1D-electrophoresis (1D-E) profiles of proteins extracted from cell walls of 5-day-old WT and atltp1-2 seedlings. The numbers on the left indicate the position of protein molecular mass markers (MM) in kDa. The arrow shows the position of the 9.6 kDa band containing AtLTP2.
Firstly, AtLTP2 expression was investigated by RT-qPCR on etiolated seedlings during 7 days, timing starting at the time of transfer to dark after synchronization of germination by light exposure for 4 h. In WT seedlings, the level of accumulation of AtLTP2 transcripts showed a significant 15-fold increase between 24 and 48 h, and peaked at 72 h before decreasing to the same level as at 48 h (Figure 1B). A 5- to 64-fold reduction in the accumulation of AtLTP2 transcripts was observed in atltp2-1 seedlings as compared to WT between 24 h and 7 days (Figure 1B). An AtLTP2 expression pattern similar to that of WT was retrieved in the three selected independent complemented lines (Supplementary Figure S1).
To further characterize these lines, we have performed a MALDI-TOF MS analysis of proteins extracted from cell walls of 5-day-old etiolated seedlings of WT and atltp2-1. Proteins were separated by 1D-electrophoresis (1D-E). A band around 9.6 kDa, in which AtLTP2 was previously identified (Irshad et al., 2008), was clearly visible after Coomassie blue staining in the WT extract, but appeared much fainter in the atltp2-1 extract (Figure 1C). MALDI-TOF MS analysis after tryptic digestion of the 9.6 kDa band from WT displayed four peptides specific for AtLTP2 allowing its identification: one major peptide (m/z 955.5321) and three minor ones (m/z 1008.4359, 992.4441, and 1236.5724; Supplementary Figure S2). In atltp2-1, only a small peak corresponding to the major peptide (m/z 955.5321) was detected in the 9.6 kDa band, suggesting that this band also contained AtLTP2. No other protein could be identified in the 9.6 kDa band. Even though MALDI-TOF MS was not quantitative, combined SDS-PAGE and MALDI TOF MS analyses indicated that the amount of AtLTP2 was lower in atltp2-1 in comparison to WT.
Altogether, these experiments have confirmed the strong reduction of the level of accumulation of AtLTP2 gene products in atltp2-1, both at the transcript and protein levels. Furthermore, these results have demonstrated that the selected AtLTP2 genomic region, carrying the native regulatory sequences, was sufficient to rescue the WT AtLTP2 expression level in atltp2-1, and that the use of these genetic lines (WT, atltp2-1, and comp) was relevant for the following phenotyping studies.
In Dark-Grown Seedlings, AtLTP2 Expression Is Restricted to the Epidermal Cells of Aerial Organs
To characterize the spatio-temporal expression pattern of AtLTP2, in situ RNA hybridization (ISH) was performed on serial sections from young etiolated seedlings (24 or 30-h-old, timing starting as described for RT-qPCR experiments). The AtLTP2 sense (S) probe, used as a negative control, displayed no significant background on WT seedling cross-sections (Figure 2A). The natural brown color observed on seed coats in all samples did not correspond to ISH labeling (Figure 2). By comparison, the subsequent serial section hybridized with the AtLTP2 antisense (AS) probe displayed an intense purple signal restricted to the epidermis of both the hypocotyl and, to a lesser extent, the cotyledons (Figure 2B). Cross-section of the atltp2-1 seedlings, at the same developmental stage, did not show such a labeling with the AtLTP2 AS probe (Figure 2C), in agreement with the RT-qPCR data (Figure 1B). The epidermal AtLTP2 hybridization signal was retrieved in the epidermis from aerial organs of the 5′2 complemented line (Figure 2D). Interestingly, the ISH performed with the AtLTP2 AS probe on a longitudinal section of WT etiolated seedlings clearly illustrated the restriction of the AtLTP2 expression to epidermal cell of aerial organs which are covered by a cuticle (hypocotyl and cotyledons) and the absence of such an expression in the cuticle-deprived radicle (Figure 2E).
FIGURE 2. AtLTP2 expression is restricted to epidermal cells of cuticle-containing hypocotyl and cotyledons from etiolated seedlings. (A–E) ISH was performed with AtLTP2 antisense (AS) and sense (S) probes on 24-h-old serial cross-sections (A–D) and 30-h-old etiolated seedling longitudinal sections (E) of WT, atltp2-1 and one complemented line (5′2 comp). The AtLTP2 S probe (A) allowed showing the low hybridization background level within the etiolated seedling tissues (C, cotyledons; H, hypocotyls; R, radicle) and in the endosperm (EN), and to visualize the natural brown color of the seed coat (SC). Scale bars: 100 μm.
AtLTP2 Is Dually Localized to the Cell Wall and the Plastids
Like most nsLTPs, AtLTP2 carries a predicted N-terminal signal peptide of 23 amino acids in length most likely directing AtLTP2 to the secretory pathway (Edstam et al., 2011). The mature 9.6 kDa protein accumulated in the cell wall proteome of dark-grown hypocotyls (Irshad et al., 2008) in agreement with the assumed localization of nsLTPs (Kader, 1996). In order to confirm its sub-cellular localization in vivo, AtLTP2 fused to the fluorescent protein TagRFP (Red Fluorescent protein, Merzlyak et al., 2007) was transiently produced in Nicotiana benthamiana leaves (Figure 3A). The TagRFP is characterized by its low 3.8 pKa especially well-adapted to fluorescence emission in various cell compartments including at the acidic pH of the cell wall compartment (Albenne et al., 2014).
FIGURE 3. AtLTP2-TagRFP is dually targeted to the cell wall and the plastids. The fusion protein AtLTP2-TagRFP displayed in (A) was produced together with the plasma membrane (PM) marker PIP2A-YFP in Nicotiana benthamiana leaves. Detached leaves were observed under hypotonic (B–G) or hypertonic (H–M) conditions. The Tag-RFP fluorescence signal is false-colored in magenta in the left column. The PM and the plastid markers (chlorophyll auto-fluorescence) are false-colored in green in the second column and the merge is presented in white in the right column. Note that under plasmolysis, the AtLTP2-TagRFP fluorescence in the cell wall is excluded from the PM fluorescence of PIP2A-YFP and that the additional co-localization of AtLTP2-TagRFP fluorescence with the chlorophyll auto-fluorescence indicates its plastid localization. Scale bars: 50 μm.
A specific TagRFP fluorescence signal was observed at the cell periphery, but was difficult to distinguish from the co-transformed PIP2A-YFP plasma membrane marker (Nelson et al., 2007) (Figures 3B–D). To overcome this difficulty, the detached transformed leaves were plasmolysed in 0.5 M mannitol, allowing the distinction between the peripheral fluorescence of the AtLTP2-TagRFP fusion protein and the retracted PIP2A-YFP fluorescence (Figures 3H–J), thus clearly demonstrating the cell wall localization of AtLTP2-TagRFP. Surprisingly, we also observed in the same cells a strong additional fluorescent signal of AtLTP2-TagRFP that co-localized with the chlorophyll auto-fluorescence both in hypotonic and hypertonic conditions (Figures 3E–G,K–M). In addition, AtLTP2 fused to the YFP coding sequence was transiently expressed in N. benthamiana leaves (Supplementary Figure S3). AtLTP2-YFP was strongly visualized in plastids, thus confirming this unexpected localization (Supplementary Figure S3). However, certainly due to the YFP instability in the cell wall acidic compartment (pKa 6.9; Albenne et al., 2014), AtLTP2-YFP fluorescence was not detected in cell wall contrary to that of AtLTP2-TagRFP. Altogether, these results showed that AtLTP2 had an original dual localization to the cell wall and the plastids.
To further clarify the mechanism of AtLTP2 transport to the plastids, AtLTP2-TagRFP was produced in N. benthamiana leaves in the presence of Brefeldin A (BFA), a drug used to prevent the endoplasmic reticulum (ER)-to-Golgi trafficking (Daskalova et al., 2010). In presence of BFA (Figure 4), the AtLTP2-TagRFP fluorescence was strictly restricted to the ER-Golgi hybrid and BFA compartments (Nebenführ et al., 2002; Ritzenthaler et al., 2002). It co-localized with the sp-YFP-HDEL marker of the ER compartment (Nelson et al., 2007) suggesting that AtLTP2-TagRFP was redistributed in the oversized ER-Golgi modified structures as previously described (Ritzenthaler et al., 2002). In the control experiment without BFA, AtLTP2-TagRFP was still observed in the cell wall and in plastids (Supplementary Figure S4). In presence of BFA, AtLTP2-TagRFP was no longer localized to the cell wall and to plastids suggesting that AtLTP2 needed to go through the ER/Golgi apparatus to reach these two compartments. Therefore, it was assumed that the full length AtLTP2 pre-protein was first targeted to the secretory pathway thanks to its signal peptide, prior to be sorted to both the cell wall and plastids.
FIGURE 4. The secretory pathway is involved in both cell wall and plastids AtLTP2-TagRFP localization. The AtLTP2-TagRFP fusion protein was produced together with the endoplasmic reticulum (ER) marker sp-YFP-HDEL in N. benthamiana leaves which were subjected to Brefeldin A (BFA) treatment. The AtLTP2-TagRFP fluorescence signal is false-colored in magenta in (A,D,G). The bright-field (B) is displayed to visualize the cell morphology. ER marker (E) and chlorophyll auto-fluorescence (H) are false-colored in green and the merge is presented in white in the right column (C,F,I). Note that in presence of BFA, AtLTP2-TagRFP fluorescence is restricted to the ER-Golgi hybrid and BFA compartments. Scale bars: 40 μm.
Reduced Expression of AtLTP2 Leads to an Increase in Cuticle Permeability without Major Modification of the Cuticle Lipid Profile
According to (i) the putative function of nsLTPs, and (ii) the above-demonstrated expression profile of AtLTP2 restricted to the aerial organ epidermal cells, we have performed cuticle-dedicated phenotyping experiments. Given that a crucial function of the cuticle is its role as a primary barrier to water-loss, the cuticle permeability was determined in 5-day-old etiolated seedlings of WT, atltp2-1, and atltp2-1 (comp) seedlings. At this developmental stage, following AtLTP2 expression peak (Figure 1B), AtLTP2 has been shown to be strongly accumulated in etiolated hypocotyl cell walls by previous proteomic studies (Irshad et al., 2008). The water-loss rate of the etiolated seedlings was faster in atltp2-1 than in WT following exit from the in vitro conditions operated in order to mimic a desiccation stress by quickly reducing the in vitro water-saturated atmosphere (Figure 5A). The water-loss rates of the 5′2 and 14′3 complemented lines were slightly slower than the WT one (Figure 5A). A link was found between relative AtLTP2 transcript level and the water-loss rate: the higher the AtLTP2 transcript level is (Supplementary Figure S1), the more the seedlings resist to water-loss (Figure 5A). To ensure that the observed weight differences were due to water-loss, the dry mass of the seedlings of the different genotypes was measured. No significant difference was detected between them (Figure 5A). The observed faster desiccation in atltp2-1 etiolated seedlings could be visualized after exit from in vitro conditions (Figure 5B). Although both the WT and atltp2-1 hypocotyls displayed similar diameters at the time they were put in normal atmospheric conditions, a clear shrinkage quickly appeared in atltp2-1 hypocotyls, whereas the WT ones resisted better to dehydration during the time course of experiments (Figure 5B). These observations were confirmed by biometrical data showing that atltp2-1 hypocotyl diameters became significantly smaller than the WT ones a few minutes after their transfer to normal atmospheric conditions (Figure 5B).
FIGURE 5. atltp2-1 etiolated seedlings show increased water-loss and toluidine blue (TB) permeability. (A) Water-loss kinetics of WT, atltp2-1 and complemented lines (5′2 and 14′3; expressed as % of fresh mass) were performed at 25°C. Points represent mean values ± SE (n = 3). Significant differences from WT were assessed by a Wilcoxon rank-sum test (∗p-value ≤ 0.05). Dry mass was measured after 3 days at 25°C. No significant differences between the different lines were assessed using a Wilcoxon rank-sum test (p-value > 0.05) (B) Arabidopsis thaliana etiolated seedlings from 5-day-old WT and atltp2-1 were imaged along a 25 min kinetics following exit from the in vitro conditions. atltp2-1 hypocotyls displayed a gradually shrinkage whereas WT hypocotyls resisted better to the induced desiccation (n = 11). Hypocotyl diameters were measured using the ImageJ software. The results were analyzed by ANOVA and Tukey HSD test (α = 0.01) using R software. Different letters indicate significant differences at p-value < 0.01. (C) Permeability of etiolated hypocotyls was examined using the TB staining test. TB uptake was quantified spectrophotometrically at OD626 nm. Results are presented as mean values ± SD (n = 5). Significant differences from WT were assessed by a Student’s t-test (∗∗p-value < 0.01).
Moreover, non-functional cuticle often showed an increased permeability to water-soluble molecules that can be monitored with toluidine blue (TB) hydrophilic dye uptake (Tanaka et al., 2004). The atltp2-1 hypocotyls showed an intense TB coloration (Figure 5C) as compared to those of the WT and of the two selected complemented lines which remained mostly white. Toluidine blue was extracted for quantification from stained aerial organs. Significant 6- to 10-fold higher stain intensity was revealed for atltp2-1 seedlings as compared to WT and complemented lines, in agreement with the macroscopic observations (Figure 5C).
In order to determine if this permeability phenotype was linked to defects in the cuticle, the composition and content of the cuticular waxes and cutin polymer were determined by GC-MS using 5-day-old etiolated hypocotyls. To our knowledge, no work has yet reported the cuticle composition of dark-grown seedlings. Therefore, the cuticle lipid profiles obtained were compared to those of light-grown A. thaliana stems and leaves (Suh et al., 2005; Kosma et al., 2009). The wax profile of etiolated hypocotyls was dominated by C29 and C31 alkanes, like in leaves, but also contained substantial amounts of very long-chain fatty acids with less than 28 carbon atoms (mainly C24) and very long-chain fatty alcohols with less than 26 carbon atoms (mainly C22; Figure 6A). Such compounds were found as very minor components of A. thaliana leaf and stem waxes, which usually contained similar compounds (i.e., fatty acids and alcohols), but with more than 26 carbon atoms. Moreover, A. thaliana stems were characterized by high amounts of C29 ketone and secondary alcohols, which were not detected in hypocotyls (Figure 6A). The cutin polymer of etiolated hypocotyls was dominated by 18:2 dicarboxylic acid, as in leaves and stems, but also contained high amounts of polyhydroxy C18 fatty acids (Figure 6B). In addition, very long-chain fatty acids with more than 24 carbon atoms were detected. Nevertheless, the waxes and cutin polymer composition and content of WT and atltp2-1 presented only slight differences (Figure 6). The waxes profile of atltp2-1 was characterized by very minor increases in the amounts of C30 fatty acids, and C22 and C30 fatty alcohols, while the major alkanes (C29 and C31) were not significantly decreased (Figure 6A). More interestingly, at the cutin level, atltp2-1 was characterized by a one third increase of the major component (18:2-DCA) when compared to WT (Figure 6B). These analyses therefore suggested that alterations in the cutin polymer, rather than in the cuticular waxes, could be related to the observed increased permeability.
FIGURE 6. atltp2-1 and WT etiolated hypocotyls have very similar cuticle composition and content. Cuticular waxes (A) and cutin monomers (B) were quantified by GC-MS. The different aliphatic compounds, sorted into individual chain length, are presented. Mean values are shown in μg/mg of fresh weight (FW) ± SD (n = 4). 18:X stands for the sum of all unsaturated C18 fatty acids (18:1+18:2+18:3). Significant differences were assessed by a Student’s t-test (∗p-value < 0.05 and ∗∗p-value < 0.01).
atltp2-1 Displays a Collapsed Epidermal Cell Surface and a Disrupted Ultra-Structure at the Cuticle-Cell Wall Interface
To clarify which alteration in the cuticle and/or cell wall could result in the permeability phenotype of atltp2-1, the epidermal cell surface and ultra-structure of etiolated hypocotyls were investigated by electron microscopy techniques. Environmental scanning electron microscopy (ESEM) was used to have an overview of the hypocotyl surface under close-to-native conditions. ESEM was indeed particularly adapted to the observation of the delicate hypocotyls because no fixation of the samples was required, thus preventing/limiting dehydration effect. While WT hypocotyls showed extremely elongated epidermal cells evenly aligned, the architecture of the atltp2-1 epidermal cells displayed pronounced modifications both in the shape and cell organization leading to some points of disruption along their surface (Figures 7A,B). This collapsed phenotype was observed from 3 to 11 days post-germination for atltp2-1 (Supplementary Figure S5), whereas a WT phenotype was repeatedly observed for the three complemented lines (Supplementary Figure S6). Whether these different phenotypes actually corresponded to the native state of the hypocotyls or were accentuated by the vacuum during ESEM, they clearly illustrated an impaired hypocotyl cell surface in atltp2-1.
FIGURE 7. Etiolated hypocotyls of atltp2-1 show dramatic surface and cuticle-cell wall interface defects. Hypocotyls from 5-day-old WT (A,C,E) and atltp2-1 (B,D,F) etiolated seedlings were imaged using ESEM (A,B), osmium tetroxide lipophilic staining at the transmission electron microscopy (TEM) level (C,D), and PATAg cell wall polysaccharide staining at the TEM level (E,F). Note the dramatic perturbation of the atltp2-1 hypocotyl surface imaged by environmental scanning electron microscopy (ESEM). Legend: cuticle (Cut); cytoplasm (Cyt); cell wall (CW); cuticle-cell wall detachment zone (DZ).
The ultra-structure of both epidermis periclinal cell wall and cuticle was observed by transmission electron microscopy (TEM) using the osmium tetroxide lipophilic staining (Figures 7C,D) and the PATAg polysaccharide staining (Figures 7E,F). A typical ∼50 nm thick electron-dense layer corresponding to the cuticle was observed on the outer part covering the periclinal cell wall in hypocotyl cross-sections from both WT and atltp2-1 (Figures 7C,D). However, the atltp2-1 cuticle was clearly no longer sealed to the cell wall at several points, especially at the junction zone between two cells, thus delineated detachment zones (DZ) between the atltp2-1 cuticle and the underlying periclinal cell wall. On the contrary, the WT cuticle consistently appeared attached to the cell wall (Figures 7C,D). While the PATAg strongly stained both the WT and the atltp2-1 epidermis cell walls (Figures 7E,F), the DZ were lightly and specifically stained by PATAg, but not by osmium tetroxide (Figures 7C,D), indicating that they were mainly composed of fibrillar cell wall polysaccharides which were pulled up during the cuticle-cell wall separation. This repeatedly observed phenotype was reinforced by a quantitative analysis of the DZ area stained with PATAg, at the junction zone between two cells. The ratio of detached cuticle length normalized relatively to the length of outer periclinal cell wall was significantly higher in atltp2-1 (75% +/- 8.8 %) than in WT (14.6% +/- 5.9 %; Supplementary Figure S7). Furthermore, light microscopy (LM) observation of cross-sections confirmed the remarkable impaired morphology of atltp2-1 hypocotyls in which the epidermal cells were particularly collapsed and thereby modified the overall shape of hypocotyls (Figure 8). By performing correlated LM and TEM-PATAg polysaccharide staining, it was shown that the DZ were distributed along the hypocotyl surface and were indeed made of empty space with little cell wall material, especially at the position covering the epidermal radial cell wall (Figure 8). Altogether, these results have demonstrated marked ultra-structural alterations on the epidermal surface of the atltp2-1 etiolated hypocotyls, suggesting a role for AtLTP2 at the cuticle-cell wall interface.
FIGURE 8. Correlated light microscopy (LM) and TEM observations of 5-day-old etiolated hypocotyls of WT and atltp2-1. Semi-thin cross-sections of WT (A–E) and of atltp2-1 (F–J) were stained with TB for LM observations (A,B,F,G) and ultra-thin serial sections were PATAg-labeled for TEM observations (C–E,H–J). The frames indicate the magnified zones. Note the overall shrinkage of atltp2-1 hypocotyl, although no particular phenotype was observable at the cuticle-cell wall interface at the correlated high magnification of LM (B,G) and low magnification of TEM (C,H), respectively. In the atltp2-1, higher TEM magnification (I,J) allowed, the visualization of the PATAg-reactive cell wall defibrillated material at the detachment zone located between the cuticle and the cell wall. Legend: cuticle (Cut); cytoplasm (Cyt); cell wall (CW); cuticle-cell wall detachment zone (DZ); vacuole (V).
In Etiolated Seedlings, the Abundance of AtLTP2 Gene Products Is Restricted to Cuticle-Carrying Epidermal Cells
The rationale to study AtLTP2 was primarily linked to the fact that it was the unique and abundant member of the nsLTP multigene family present in the cell wall proteome of etiolated hypocotyls (Irshad et al., 2008). In agreement with the AtLTP2 expression patterns described in the Arabidopsis eFP browser database (Winter et al., 2007), we found that the expression of AtLTP2 was 15–30 times increased over a 7 days period in the dark. In addition, we have demonstrated here that in etiolated seedlings, the AtLTP2 strong expression was restricted to epidermal cells of hypocotyls and to a lesser extent of cotyledons. In contrast, when atltp2-1 plants were grown under a 16 h light/8 h dark photoperiod in soil in a greenhouse to produce seeds, we did not notice any obvious change in germination rate, early vegetative growth, flowering time, and seed production in comparison to WT (data not shown), suggesting low expression under normal conditions. In agreement, using transgenic AtLTP2 promoter::GUS lines, Chae et al. (2010) previously showed that AtLTP2 was only expressed at a low level in hypocotyls in normal growth conditions, but highly induced under abiotic stress such as drought (PEG treatment). More recently, using the same strategy, Deeken et al. (2016) reported that AtLTP2/AtLtpI-4 expression was restricted to very specific cell types under normal conditions, but reached very high level in crown gall tumors which develop on inflorescence stems epidermis of mature plants upon bacterial infection. Finally, abundant AtLTP2 transcripts were also found in the epidermal cells of embryonic aerial organs at late stages of seed development (Francoz et al., 2016). Taken together, these different reports showed that AtLTP2 was poorly expressed in most plant organs under normal exposure, but strongly expressed in WT aerial organ epidermis undergoing cell wall remodeling. Interestingly, the AtLTP2 developmental expression pattern is in addition distinguishable from those of other AtLTPs already studied (Winter et al., 2007; Chae et al., 2010), allowing to hypothesize that AtLTP2 could play a major role in different scenarii related to biotic (crown gall) and abiotic stresses (drought/PEG, continuous darkness/active growth).
AtLTP2 Is Transported through the Secretory Pathway Both to the Cell Wall and the Plastids
As expected from AtLTP2 identification in the cell wall proteome of etiolated hypocotyls (Irshad et al., 2008), we unambiguously visualized over-expressed AtLTP2-TagRFP in the cell wall compartment of N. benthamiana epidermal cells. Unexpectedly, AtLTP2 fused with the red fluorescent protein mCherry was reported as being associated with the plasma membrane (Deeken et al., 2016) despite the absence of GPI anchor necessary for plasma membrane-anchorage (Debono et al., 2009; Lee et al., 2009; Kim et al., 2012). We hypothesize that this discrepancy could be due to the plasmolysis treatments done with 1 M KNO3 (Deeken et al., 2016) or mannitol (this study). Indeed, we have previously shown that salt solutions and not osmotic agents such as glycerol or mannitol, release fluorescent-tagged CWPs from cells walls (Albenne et al., 2014). Furthermore, AtLTP1/AtLtpI.5 (At2g38540), a nsLTP highly homologous to AtLTP2 (81% protein similarity), was demonstrated to have a cell wall localization (Thoma et al., 1993; Potocka et al., 2012; Deeken et al., 2016). Altogether and considering the huge abundance of AtLTP2 in the cell wall proteome of etiolated hypocotyls, these results provide strong clues in favor of its cell wall localization. Other nsLTPs from several plant species have already been shown to be addressed to the apoplastic compartment [see for review (Liu et al., 2015)]. Interestingly, nsLTPs were also found deeply associated with the surface wax (Pyee et al., 1994), the cutin layer (Thoma et al., 1993). Our localization experiments did not allow showing whether AtLTP2 was localized to the cuticle, to the underlying polysaccharidic cell wall or both. However, the sample preparation procedure used for the cell wall proteomics studies in which AtLTP2 was abundantly found, argues for cell wall localization (Irshad et al., 2008). Surprisingly, we consistently additionally detected AtLTP2-TagRFP and AtLTP2-YFP in plastids of N. benthamiana leaves during transient expression assays. Although AtLTP2-mCherry was not detected in this sub-cellular compartment (Deeken et al., 2016), the plastidial localization of both AtLTP2-TagRFP and AtLTP2-YFP was in agreement with the identification of AtLTP2 but also AtLTP1 in the A. thaliana chloroplast proteome (Ferro et al., 2010). It is worth noting that during somatic embryogenesis in A. thaliana, LTP1 epitopes (i.e., AtLTP1 and/or AtLTPs sharing protein similarity with AtLTP1 as AtLTP2), were strongly and clearly detected in plastids (Potocka et al., 2012). Furthermore, the RlemLTP from rough lemon was also localized restrictively to the chloroplast but its principal role remains unknown (Nishimura et al., 2008). Altogether, AtLTP2 appears to be localized both to the cell wall and the plastids. In this study, our results suggest that this dual targeting involves the secretory pathway. Indeed, the transport of AtLTP2 to the cell wall and to plastids was prevented in presence of BFA, a fungal molecule mainly reported as an inhibitor of anterograde trafficking in plants even if in some cases it could also inhibits endocytosis (Jelínková et al., 2015). Recently, three rice Nucleotide Pyrophosphatase/Phosphodiesterases (NPP1, 2 and 6) have been shown to be transported from the secretory pathway to plastids via the trans-Golgi. In particular, their transport to plastids was BFA-sensitive (Nanjo et al., 2006; Kaneko et al., 2016). Only a few proteins have been shown to be targeted to the plastids through the secretory pathway, e.g., NPPs, several α-amylases and a carbonic anhydrase (Radhamony and Theg, 2006; Li and Chiu, 2010; Kaneko et al., 2016). AtLTP2 could then be added to the shortlist of proteins targeted, through the secretory pathway, to non-secretory pathway organelles such as plastids, mitochondrion, or nucleus (Porter et al., 2015).
AtLTP2 Is Required to Maintain the Cuticle-Cell Wall Interface Integrity to Control Etiolated Hypocotyl Permeability
Plant epidermal cells have a huge demand for lipid synthesis and lipid transport as they synthesize the cuticle that covers their surface (Hurlock et al., 2014). Because of their lipophilic properties, the cuticular components may require the use of transporters for their trafficking from the ER to the cuticle. nsLTPs were proposed as such carriers for cuticular lipids through the hydrophilic cell wall compartment (Kader, 1996; Samuels et al., 2008; Domínguez et al., 2015). According to its epidermal localization and to its putative role in cuticle formation, AtLTP2 was assessed for its involvement in cuticle permeability. atltp2-1 knock-down mutant displayed a faster water-loss rate together with an increase in TB staining revealing deep modification in the permeability and possibly in the structure of the cuticle. In in vitro-grown etiolated hypocotyls, no stomata were observed on our ESEM images from all genetic lines strongly suggesting that the water-loss measured mainly occurred at the cuticular level. The dysfunctional cuticle observed in etiolated atltp2-1 seedlings was entirely recovered in complementation lines. However, atltp2-1 and WT etiolated hypocotyls displayed very similar cuticle composition and content. It is considered that distortion of the cuticle can result in an increased permeability (Tanaka et al., 2004) which in many instances, is linked to modifications in the cuticle composition and content. For instance, mutations in ABC transporter encoding genes (Luo et al., 2007; Bessire et al., 2011), in BODYGUARD (BDG) encoding an α/β-hydrolase fold protein (Jakobson et al., 2016), or in lipid biosynthetic enzymes involved in cuticle formation (Tanaka et al., 2004; Kosma et al., 2009; Li et al., 2013), were tightly associated with changes both in cuticle permeability and cuticle composition and content. However, very few reports have clearly demonstrated direct links between nsLTPs and cuticular permeability and/or cuticle lipid profile. Overexpression of BraLTP1 in Brassica napus (Liu et al., 2014) causes both reduced wax deposition and a significant increase in water-loss. In addition, the disruption of genes encoding plasma membrane-anchored LTPG reported to be implicated in cuticular lipid composition did not lead to changes in cuticle permeability and show a slight impact on lipid content and composition (Lee et al., 2009). Our cuticular lipid analyses showed that atltp2-1 was slightly affected in its cutin polymer. Besides, the cuticular waxes were barely affected, although they play the predominant role in limiting non-stomatal water-loss (Jetter and Riederer, 2016). Interestingly, in accordance with these results, in the physiological context of the crown gall, the GK-639E08 atltp2 mutant displayed no difference in lipid composition of the cuticular wax in comparison with WT (Deeken et al., 2016). Thus, AtLTP2 appears to be a new type of nsLTP which could be involved in the barrier primary function of the cuticle by limiting water-loss at the epidermal surface of etiolated hypocotyls without major modification in its wax cuticular lipid profile.
To go further in the understanding of the role of AtLTP2 in controlling cuticular permeability, the structure and ultra-structure of the surface of etiolated hypocotyls were examined. When AtLTP2 expression was strongly reduced, the epidermal cells appeared disorganized and several points of disruption along the hypocotyl surface were observed. Severe ultra-structural alterations at the cuticle-cell wall interface occurred in atltp2-1 leading (i) to the detachment of the cuticle from the underlying cell wall mainly at the radial separation of epidermal cells and (ii) to the appearance of space with remaining cell wall components. It cannot be excluded that both the vacuum and dehydration treatments applied for ESEM and TEM, respectively, could have accentuated the mutant phenotype. However, this phenotype was exclusively observed in atltp2-1 and not in WT or in complemented lines. It indicated that the cuticle-cell wall interface was highly weakened in atltp2-1 in comparison to WT and complemented lines. Besides, no phenotype was observed in the ultra-structure of the cuticle itself.
The two observed phenotypes in atltp2-1 (increase of permeability and alteration of cuticle-cell wall interface integrity) without strong modification of the cuticle composition, content, and ultra-structure, do not fit with the historical purported role of nsLTPs (Kader, 1996; Samuels et al., 2008). Indeed, nsLTPs have long been assumed to shuttle lipids across the hydrophilic cell wall from the plasma membrane to the cuticle. Given the abundance and the uniqueness of AtLTP2 in the studied model, and the phenotype observed in atltp2-1, one would expect atltp2-1 to display cuticle composition/content and ultra-structure phenotypes, if AtLTP2 would have such a shuttling role. Such relationships between ultra-structural and/or biochemical changes within the cuticle and increased permeability were described in different plant species mutants thought to be defective in the biosynthesis of cuticular compounds (Voisin et al., 2009; Mao et al., 2012; Liu et al., 2014). On the contrary, our results indicate that AtLTP2 could be involved, directly or indirectly, in the integrity of the cuticle-cell wall adhesion in etiolated seedlings to maintain the cuticle barrier properties, but without disturbing the cuticle ultra-structure itself. Two hypotheses could be proposed to explain the AtLTP2 action mode: (i) AtLTP2 could be a carrier of cuticular lipids and its down-expression leads to slight modifications of cuticle composition and ultra-structure (ii) AtLTP2 is not involved in cuticle formation, but rather could play a physical role at the cuticle-cell wall interface. In our opinion, the fact that the observed slight modifications in cuticle composition did not affect the cuticle ultra-structure in atltp2-1, and the abundance of AtLTP2 are not in favor of a role as a carrier for cuticular compounds. It rather suggests that AtLTP2 could play a structural role as an amphiphile molecule with adhesive properties that could allow the accurate sealing between the hydrophobic cuticle and the hydrophilic underlying cell wall. This proposed structural role is strengthened by the spatio-temporal localization of AtLTP2 gene products (Irshad et al., 2008; our results). Even though we were not able to determine the localization of AtLTP2 within the cell wall, the observed ultra-structural phenotype suggests that AtLTP2 may localize at the cuticle-cell wall interface where intra-cuticular waxes are packed in the spaces of the cutin polyester, acting together to maintain the permeability barrier (Goodwin and Jenks, 2005; Bessire et al., 2007). Somehow similar phenotype with the loss of sealing at the cuticle-cell wall interface were observed for mutants of plasma membrane-localized ABC transporters implicated in cutin deposition like AtABCG32 (Bessire et al., 2011) and OsABCG31 (Garroum et al., 2016). Given that the cuticle layer which directly interacts with the cell wall is rich in cutin residues (Yeats and Rose, 2013), we assume that cutin could be bound by AtLTP2, constituting a first level of AtLTP2 structural interaction at the cuticle-cell wall interface.
A second level of hypothesized AtLTP2 structural interactions concerns polysaccharides. The intimate linkage between both polysaccharides and lipid cuticle constituents are proposed to have a drastic impact on cuticle water absorption (Bessire et al., 2007; Fernandez et al., 2016). However, the molecular basis of lipid-polysaccharide interactions is unclear. Based on phylogenetic analysis combined with ESI (Electrostatic Similarity Indice) clustering analysis (Chae et al., 2010), AtLTP2 belongs to the Stigma/style Cysteine-rich Adhesin (SCA-like LTP) positively net charged subset and was closely clusters with the tobacco LTP2 (Chae et al., 2010). Thus, we propose that, in addition to AtLTP2 interaction with hydrophobic lipids in its pocket, the positive electrostatic polarization of AtLTP2 surface could allow additional interaction with negatively charged cell wall polysaccharides such as demethylated homogalacturonans (Chae et al., 2010). Indeed, it was assumed that during pollen tube adhesion-mediated guidance, the positive lily SCA-LTP interact with the negative pectin moieties from the stylar extra cellular matrix (Mollet et al., 2000), then leading to the adhesion of the pollen tube by the formation of an adhesive matrix, due to ionic interactions between the three partners, SCA-LTP, the pectins of both pollen tube walls and stylar surfaces of the transmitting tract epidermis (Mollet et al., 2007). No such interaction has yet been demonstrated for other nsLTPs, but interaction with cellulose has also been proposed for a tobacco nsLTP presenting a cell wall-loosening activity dependent on hydrophobic interactions (Nieuwland et al., 2005).
To conclude, we propose that AtLTP2 contributes to the cuticular main function (e.g., a barrier to non-stomatal water-loss) by preserving the integrity of the sealing/adhesion at the cuticle-cell wall interface in epidermal cells of dark-grown aerial organs. Given its abundance, its amphiphilic nature and the observed phenotypes of atltp2-1, we propose a structural role for AtLTP2 at this interface made of lipidic cuticular compounds and hydrophilic polysaccharides, constituting a novel function for a nsLTP. Interestingly, during growth and expansion of crown gall tumors in which AtLTP2 was highly expressed (Deeken et al., 2016), the epidermal cell layer was disrupted, leading to the loss of an intact cuticule (Gohlke and Deeken, 2014). Thereby, the disrupted crown gall surface has to be sealed and suberization of cell walls most probably occurred to avoid uncontrolled loss of water from the host plant. Similarly, Chae et al. (2010) reported strong AtLTP2 expression in response to PEG treatment, suggesting the involvement of AtLTP2 in osmotic response, where the cuticular barrier is known to be up-regulated (Kosma et al., 2009). Thus, AtLTP2 could present different functions in various developmental conditions or under biotic or abiotic stresses. Remarkably, in all three cases (high elongation rate of etiolated hypocotyls, biotic and abiotic stresses), it seems that the expression of AtLTP2 is induced in specific conditions where reinforcement of the cuticle-cell wall integrity or modification of the cell wall (e.g., suberization) is needed at the epidermal surface.
In addition, AtLTP2 is the first nsLTP shown to have a dual sub-cellular localization to the cell wall and the plastids by trafficking through the secretory pathway. The elucidation of the molecular mechanisms by which AtLTP2 establish cell wall-cuticle homeostasis and the exact function of the dual targeting will be challenging tasks in the future.
Materials and Methods
The atltp2-1 mutant for At2g38530 (Salk N526257.5, Col-0 background) was ordered from the NASC collection1. The homozygous atltp2-1 and its WT counterpart were obtained from this Salk line during a genotyping process of its progeny. This screening was done by PCR with the primers listed in Supplementary Table S1. For phenotyping experiments, seeds were sown in Magenta boxes on Murashige and Skoog (MS) medium (Sigma–Aldrich)2 with 1% (w/v) agar. Seeds were kept in the dark at 4°C during 48 h and subsequently exposed to light for 4 h to synchronize germination. In vitro seedlings were grown in the dark at 23°C for various periods of time up to 11 days. For complementation/transformation experiments, atltp2-1 plants were grown in growth chamber under a 15 h light/9 h dark cycle (22/20°C, 70% humidity) until flowering. For transient transformation experiments, N. benthamiana plants were cultivated in growth chambers (16 h light/8 h dark cycle, 25/22°C, 80% humidity) during 3 weeks.
Plasmid Construction and Stable Plant Transformation of atltp2-1
A 2.8 kb genomic fragment comprising the AtLTP2 promoter, the coding region and the terminator regions was amplified from genomic DNA by PCR using primers listed in Supplementary Table S1. It was cloned into pAM-PAT-D35S-GWY-3HA-RRS1-RT which derived from binary vectors previously described (Tasset et al., 2010), to generate the promAtLTP2::AtLTP2::TermAtLTP2 construct. The Agrobacterium tumefaciens GV3101::pMP90 strain (Koncz and Schell, 1986) was transformed with the recombinant vector and used to stably transform atltp2-1 plants with the floral dip method (Clough and Bent, 1998).
In situ Hybridization (ISH)
In situ hybridization was performed as previously described for developing seeds (Francoz et al., 2016). Tissue microarrays encompassed early developmental kinetics for hundreds of etiolated seedlings of A. thaliana WT, atltp2-1, and the complemented line 5′2. Slides have been scanned with a Nanozoomer HT slide scanner (Hamamatsu)3.
RNA Extraction and cDNA Synthesis
Total RNA extractions were performed from three biological replicates for each sample. For the youngest samples, whole seedlings were sampled, whereas for 5- and 11-day-old seedlings, only aerial organs were sampled. Samples were ground in liquid nitrogen and RNA extraction was performed using the E.Z.N.A® Plant DNA Kit (Omega BioTech Inc)4. For each extraction, 70 mg of fresh material were used. RNA concentration and quality were determined using a N-100 NanoDrop5. For cDNA synthesis, 400 ng of total RNAs were used to perform reverse transcription using the High-Capacity cDNA reverse transcription kit (Applied Biosystems)6. The cDNAs were stored at -20°C.
RT-qPCRs were laid out in 384 well-plates, including three reference genes (At5g15710 encoding a F-box protein, At1g49240 encoding actin 8 and At4g34270 encoding a TIP-41 like protein; Czechowski et al., 2005). A. thaliana gene-specific primers are listed in Supplementary Table S1. Three biological and two technical replicates were included for each cDNA-primer combination. Individual reactions contained 3 μl of cDNA, 0.5 μl of each primer (10 μM), and 4 μl of 2x SYBR GREENTM (Roche)7 in a final volume of 8 μl. Plates were sealed using a clear, adhesive PCR film (Thermo Scientific)8. They were run in a LightCycler® 480 (Roche) at 95°C for 5 min, followed by 45 cycles with 95°C for 15 s and 60°C for 1 min, and finally 40°C for 1 min. Data were collected and analyzed using Microsoft Excel 20109. The geometric mean value generated from the three reference genes was used to calculate the relative gene expression levels using the 2-ΔΔCT method (Livak and Schmittgen, 2001). Significant differences were assessed by a Student’s t-test.
Cell Wall Purification, Extraction of Proteins, and Identification of AtLTP2 by MALDI-TOF MS
Cell wall purification and extraction of proteins were performed as described (Feiz et al., 2006) with 5 g of etiolated hypocotyls and cotyledons. Proteins were dialysed and concentrated by successive centrifugation using the Amicon Ultra-15 centrifugal filter Ultracel® (Merck Millipore Corporation)10. Proteins were separated by denaturing 1D-E using 12.5% (m/v) polyacrylamide gel. Proteins were stained with CoomassieTM Brilliant Blue (Scheler et al., 1998). Colored bands around 9.6 kDa were sampled and digested with trypsin. MALDI-TOF MS analyses were performed as reported (Boudart et al., 2005).
Transient Transformation of N. benthamiana Plants for Sub-cellular Localization of AtLTP2
To generate the AtLTP2-TagRFP construct, the A. thaliana full-length cDNA AtLTP2 clone (pda02841) was ordered at the RIKEN Genomic Sciences Complex (RIKEN11; Seki et al., 2002). It was amplified by PCR using the primers listed in Supplementary Table S1 (AttB1-At2g38530-F and Spacer-At2g38530-R). The TagRFP coding sequence was amplified separately from the pTagRFP-C vector (FP141, Evrogen, Euromedex, Souffelweyersheim, France) with the sense and AS primers (Spacer-TarRFP-F and AttB2-TagRFP-stop listed in Supplementary Table S1). Both the AtLTP2 and the TagRFP PCR products were fused by the overlap extension PCR method and the corresponding fused DNA product was amplified with the primers listed in Supplementary Table S1 (attB1-F-adapter and attB2-R-adapter). Then, it was cloned into the entry vector pDONR207 prior to be transferred into the pEAQ-DEST1-HT destination vector (Sainsbury et al., 2009) by homologous recombination using the Gateway® technology (InvitrogenTM-ThermoFisher)12. The A. tumefaciens GV3101 strain was transformed with the recombinant binary vector.
Agrobacterium tumefaciens were grown in Yeast Extract Broth (YEB) liquid medium at 28°C under shaking until OD600 reached 1. Bacteria were centrifuged 5 min at 4000 × g. The pellet was re-suspended in agromix (10 mM MES-KOH pH 5.6, 0.15 mM acetosyringone, 10 mM MgCl2) until OD600 = 1, and incubated overnight at room temperature. Nicotiana benthamiana leaves of 3-week-old plants were infiltrated at their abaxial side with the bacterial suspension(s). In the case of co-infiltration of two bacterial suspensions carrying different constructs, a ratio of 2/1 was used [TagRFP-construct/YFP-tagged organelle markers for plasma membrane (pm-yb CD3-1006) or ER (ER-yb CD3-958)] (Nelson et al., 2007). Nicotiana benthamiana plants were kept in the growth chamber room until observation 48 h after infiltration.
An upright confocal laser scanning microscope (LEICA SP2 AOBS13) using a 40 x apochromatic water immersion lens was used to visualized YFP fluorescence (excitation: 488 nm; emission: 514–551 nm), TagRFP fluorescence (excitation: 561 nm; emission: 582–622 nm), and chlorophyll auto-fluorescence (excitation: 488 nm; emission: 680–720 nm). Fluorescence in different channels was acquired for the same field using a sequential acquisition mode. Plasmolysis assays were performed using 0.5 M mannitol.
For the ER-Golgi trafficking assay, BFA (Sigma–Aldrich) was used at a concentration of 35 μM. One milliliter BFA was co-infiltrated with transformed A. tumefaciens in N. benthamiana leaves and 1 ml was infiltrated 24 h before observation (Daskalova et al., 2010).
Water-Loss and Toluidine Blue Assays
Five-day-old etiolated seedlings from WT and atltp2-1 (n = 11) were aligned on a microscopy slide and imaged with an Axiozoom V 1614 during a 25 min kinetics to follow their degree of desiccation. Hypocotyl diameters were measured using the ImageJ software15. The results were analyzed by ANOVA and Tukey HSD test (α = 0.01) using the R software (R Core Team, 2016). In parallel, 500 mg of WT, atltp2-1, and complemented lines (5′2 and 14′3) seedlings were put in Petri dishes. They were placed in a 25°C oven and weighted with a precision balance during a 3 h kinetics to monitor water-loss. Dry mass was measured after 3 days at 25°C. Significant differences were assessed by a Wilcoxon rank-sum test using the R software. TB staining was performed as described (Tanaka et al., 2004). Quantification of TB was performed using 20 mg of etiolated hypocotyls (Xing et al., 2013). Significant differences were assessed by a Student’s t-test. Root and seed coats were carefully removed prior to immersion in ethanol.
Wax and Cutin Monomer Analysis
Five-day-old etiolated hypocotyls were harvested, the cotyledons removed, and the fresh mass immediately measured. Waxes were extracted by dipping in chloroform for 30 s and analyzed as described (Bourdenx et al., 2011). The hypocotyls were then delipidated and the cutin monomer composition and content determined as described (Domergue et al., 2010). Significant differences were assessed by a Student’s t-test.
Environmental Scanning Electron Microscopy Analysis
Wild type and atltp2-1 etiolated seedlings were used for ESEM analysis. Samples were observed without fixation following their sampling from in vitro cultures. Micrographs were obtained with a Quanta 250FEG ESEM (FEI Company)16 using a 10 kV acceleration voltage, a spot size of 3, and a chamber pressure of 800 Pa, at 5°C and 94% humidity.
Transmission Electron Microscopy Analysis
Five-day-old etiolated seedlings of WT and atltp2-1 were fixed for 2 h in 1.25% glutaraldehyde/2% paraformaldehyde (Oudin et al., 2007). Half of the samples were post-fixed for 1 h in 1% (v/v) aqueous OsO4 solution (Electron Microscopy Sciences)17. All the samples were further dehydrated, infiltrated, and embedded in LR White resin (Oudin et al., 2007). For OsO4 post-fixed samples, ultrathin cross-sections (100 nm thick) of the hypocotyls base were cut and directly observed on 200 mesh-copper grids using a HT7700 TEM (Hitachi)18 operated at 80 kV with a Gatan numeric camera19. For the other samples, semi- (1 μm) and ultra-thin (100 nm) sections were sequentially cut from the same sample. Semi-thin sections were stained in 0.5% (w/v) TB solution for 15 min for correlative microscopy with TEM observations. Ultra-thin sections were handled on plastic rings for PATAg staining (Reis and Roland, 1974) and eventually transferred to 200 mesh-nickel grids. TEM observations were performed as described above. For quantitative analysis of DZ on PATAg images, wide views (×5K magnification) were chosen to provide the widest surface of analysis enabling to keep the ultrastructural details of PATAg-labeling, WT (n = 8) and atltp2-1 (n = 8) hypocotyl epidermal cell cross-sections were carefully analyzed for quantification of DZ. The TEM images were individually computer-labeled using Corel Photopaint with red lines (detached cuticle) and green lines (outer periclinal cell wall). These color marks (length of red lines and length of green lines, both in μm) were measured with ImageJ on calibrated images. For each image, the ratio of detached cuticle length/total outer periclinal cell wall length (sum of red lines whenever present/green line) was calculated as %, and the results were expressed as mean % +/- standard error. Significant difference in atltp2-1 as compared to WT was assessed by a Wilcoxon rank-sum test.
AJ and CP performed the experiments. YM and BP contributed to the histological analysis. FD performed the cuticular lipids analysis. EJ initiated the research. VB and VP conceived and designed the study, supervised the assays, analyzed and discussed the results. VP coordinated the writing of the manuscript. All authors participated to the writing and/or the drafting of the paper. All authors read and approved the final manuscript.
The authors are thankful to Université Paul Sabatier (Toulouse, France) and CNRS for supporting their research work. This work was also supported by the French Laboratory of Excellence project entitled “TULIP” (ANR-10-LABX-41; ANR-11-IDEX-0002-02).
Conflict of Interest Statement
The authors declare that the research was conducted in the absence of any commercial or financial relationships that could be construed as a potential conflict of interest.
MALDI-TOF MS analyses were performed on the Toulouse Proteomics platform (http://proteomique.ipbs.fr/). Microscopy analyses were performed on the Toulouse Imaging platform (http://trigenotoul.com). The authors also wish to thank Dr. Cécile Albenne and Carole Pichereaux for help in MALDI-TOF MS analyses and Dr. Laurent Deslandes for the gift of the two pAM-PAT derived binary vectors. They are also grateful to Olivier Catrice, Josiane Chourré, and David Roujol for technical support. Lipid analyses were performed at the Functional Genomic Center of Bordeaux – Metabolome/Lipidome platform, which is supported by the MetaboHUB-ANR-11-INBS-0010 grant (http://metabolome.cgfb.u-bordeaux.fr/).
The Supplementary Material for this article can be found online at: https://www.frontiersin.org/article/10.3389/fpls.2017.00263/full#supplementary-material
- ^ http://arabidopsis.info/
- ^ https://www.sigmaaldrich.com
- ^ http://www.hamamatsu.com
- ^ www.omegabiotek.com/
- ^ www.nanodrop.com
- ^ www.appliedbiosystems.com
- ^ www.lifescience.roche.com
- ^ www.thermofisher.com
- ^ www.microsoft.com
- ^ www.merckmillipore.com
- ^ http://www.riken.jp/en/
- ^ www.thermofisher.com
- ^ www.leica-microsystems.com
- ^ www.zeiss.fr/microscopy
- ^ https://imagej.nih.gov/ij/
- ^ www.fei.com/
- ^ www.emsdiasum.com/microscopy/
- ^ www.hitachi-hightech.com
- ^ www.gatan.com
Bessire, M., Borel, S., Fabre, G., Carraca, L., Efremova, N., Yephremov, A., et al. (2011). A member of the PLEIOTROPIC DRUG RESISTANCE family of ATP binding cassette transporters is required for the formation of a functional cuticle in Arabidopsis. Plant Cell 23, 1958–1970. doi: 10.1105/tpc.111.083121
Bessire, M., Chassot, C., Jacquat, A.-C., Humphry, M., Borel, S., Petétot, J. M.-C., et al. (2007). A permeable cuticle in Arabidopsis leads to a strong resistance to Botrytis cinerea. EMBO J. 26, 2158–2168. doi: 10.1038/sj.emboj.7601658
Boudart, G., Jamet, E., Rossignol, M., Lafitte, C., Borderies, G., Jauneau, A., et al. (2005). Cell wall proteins in apoplastic fluids of Arabidopsis thaliana rosettes: identification by mass spectrometry and bioinformatics. Proteomics 5, 212–221. doi: 10.1002/pmic.200400882
Bourdenx, B., Bernard, A., Domergue, F., Pascal, S., Leger, A., Roby, D., et al. (2011). Overexpression of Arabidopsis ECERIFERUM1 promotes wax very-long-chain alkane biosynthesis and influences plant response to biotic and abiotic stresses. Plant Physiol. 156, 29–45. doi: 10.1104/pp.111.172320
Boutrot, F., Chantret, N., and Gautier, M. F. (2008). Genome-wide analysis of the rice and Arabidopsis non-specific lipid transfer protein (nsLtp) gene families and identification of wheat nsLtp genes by EST data mining. BMC Genomics 9:86. doi: 10.1186/1471-2164-9-86
Chae, K., Gonong, B. J., Kim, S. C., Kieslich, C. A., Morikis, D., Balasubramanian, S., et al. (2010). A multifaceted study of stigma/style cysteine-rich adhesin (SCA)-like Arabidopsis lipid transfer proteins (LTPs) suggests diversified roles for these LTPs in plant growth and reproduction. J. Exp. Bot. 61, 4277–4290. doi: 10.1093/jxb/erq228
Czechowski, T., Stitt, M., Altmann, T., Udvardi, M. K., and Scheible, W. R. (2005). Genome-wide identification and testing of superior reference genes for transcript normalization in Arabidopsis. Plant Physiol. 139, 5–17. doi: 10.1104/pp.105.063743
Daskalova, S. M., Radder, J. E., Cichacz, Z. A., Olsen, S. H., Tsaprailis, G., Mason, H., et al. (2010). Engineering of N. benthamiana L. plants for production of N-acetylgalactosamine-glycosylated proteins–towards development of a plant-based platform for production of protein therapeutics with mucin type O-glycosylation. BMC Biotechnol. 10:62. doi: 10.1186/1472-6750-10-62
Debono, A., Yeats, T. H., Rose, J. K., Bird, D., Jetter, R., Kunst, L., et al. (2009). Arabidopsis LTPG is a glycosylphosphatidylinositol-anchored lipid transfer protein required for export of lipids to the plant surface. Plant Cell 21, 1230–1238. doi: 10.1105/tpc.108.064451
Deeken, R., Saupe, S., Klinkenberg, J., Riedel, M., Leide, J., Hedrich, R., et al. (2016). The nonspecific lipid transfer protein AtLtpI-4 is involved in suberin formation of Arabidopsis thaliana crown galls. Plant Physiol. 172, 1911–1927. doi: 10.1104/pp.16.01486
Derbyshire, P., Findlay, K., McCann, M. C., and Roberts, K. (2007). Cell elongation in Arabidopsis hypocotyls involves dynamic changes in cell wall thickness. J. Exp. Bot. 58, 2079–2089. doi: 10.1093/jxb/erm074
Domergue, F., Vishwanath, S. J., Joubes, J., Ono, J., Lee, J. A., Bourdon, M., et al. (2010). Three Arabidopsis fatty acyl-coenzyme A reductases, FAR1, FAR4, and FAR5, generate primary fatty alcohols associated with suberin deposition. Plant Physiol. 153, 1539–1554. doi: 10.1104/pp.110.158238
Feiz, L., Irshad, M., Pont-Lezica, R. F., Canut, H., and Jamet, E. (2006). Evaluation of cell wall preparations for proteomics: a new procedure for purifying cell walls from Arabidopsis hypocotyls. Plant Methods 2:10. doi: 10.1186/1746-4811-2-10
Fernandez, V., Guzman-Delgado, P., Graca, J., Santos, S., and Gil, L. (2016). Cuticle structure in relation to chemical composition: re-assessing the prevailing model. Front. Plant Sci. 7:427. doi: 10.3389/fpls.2016.00427
Ferro, M., Brugière, S., Salvi, D., Seigneurin-Berny, D., Court, M., Moyet, L., et al. (2010). AT_CHLORO, a comprehensive chloroplast proteome database with subplastidial localization and curated information on envelope proteins. Mol. Cell. Proteomics 9, 1063–1084. doi: 10.1074/mcp.M900325-MCP200
Francoz, E., Ranocha, P., Pernot, C., Ru, A. L., Pacquit, V., Dunand, C., et al. (2016). Complementarity of medium-throughput in situ RNA hybridization and tissue-specific transcriptomics: case study of Arabidopsis seed development kinetics. Sci. Rep. 6:24644. doi: 10.1038/srep24644
Garroum, I., Bidzinski, P., Daraspe, J., Mucciolo, A., Humbel, B. M., Morel, J. B., et al. (2016). Cuticular defects in Oryza sativa ATP-binding cassette transporter G31 mutant plants cause dwarfism, elevated defense responses and pathogen resistance. Plant Cell Physiol. 57, 1179–1188. doi: 10.1093/pcp/pcw066
Guo, L., Yang, H., Zhang, X., and Yang, S. (2013). Lipid transfer protein 3 as a target of MYB96 mediates freezing and drought stress in Arabidopsis. J. Exp. Bot. 64, 1755–1767. doi: 10.1093/jxb/ert040
Huang, M. D., Chen, T. L., and Huang, A. H. (2013). Abundant type III lipid transfer proteins in Arabidopsis tapetum are secreted to the locule and become a constituent of the pollen exine. Plant Physiol. 163, 1218–1229. doi: 10.1104/pp.113.225706
Irshad, M., Canut, H., Borderies, G., Pont-Lezica, R., and Jamet, E. (2008). A new picture of cell wall protein dynamics in elongating cells of Arabidopsis thaliana: confirmed actors and newcomers. BMC Plant Biol. 8:94. doi: 10.1186/1471-2229-8-94
Jakobson, L., Lindgren, L. O., Verdier, G., Laanemets, K., Brosche, M., Beisson, F., et al. (2016). BODYGUARD is required for the biosynthesis of cutin in Arabidopsis. New Phytol. 211, 614–626. doi: 10.1111/nph.13924
Jetter, R., and Riederer, M. (2016). Localization of the transpiration barrier in the epi- and intracuticular waxes of eight plant species: water transport resistances are associated with fatty acyl rather than alicyclic components. Plant Physiol. 170, 921–934. doi: 10.1104/pp.15.01699
Kaneko, K., Takamatsu, T., Inomata, T., Oikawa, K., Itoh, K., Hirose, K., et al. (2016). N-Glycomic and microscopic subcellular localization analyses of NPP1, 2 and 6 strongly indicate that trans-Golgi compartments participate in the Golgi to plastid traffic of Nucleotide Pyrophosphatase/Phosphodiesterases in rice. Plant Cell Physiol. 57, 1610–1628. doi: 10.1093/pcp/pcw089
Kim, H., Lee, S. B., Kim, H. J., Min, M. K., Hwang, I., and Suh, M. C. (2012). Characterization of glycosylphosphatidylinositol-anchored lipid transfer protein 2 (LTPG2) and overlapping function between LTPG/LTPG1 and LTPG2 in cuticular wax export or accumulation in Arabidopsis thaliana. Plant Cell Physiol. 53, 1391–1403. doi: 10.1093/pcp/pcs083
Koncz, C., and Schell, J. (1986). The promoter of TL-DNA gene 5 controls the tissue-specific expression of chimaeric genes carried by a novel type of Agrobacterium binary vector. Mol. Gen. Genet. 204, 383–396. doi: 10.1007/bf00331014
Kosma, D. K., Bourdenx, B., Bernard, A., Parsons, E. P., Lu, S., Joubes, J., et al. (2009). The impact of water deficiency on leaf cuticle lipids of Arabidopsis. Plant Physiol. 151, 1918–1929. doi: 10.1104/pp.109.141911
Lee, S. B., Go, Y. S., Bae, H. J., Park, J. H., Cho, S. H., Cho, H. J., et al. (2009). Disruption of glycosylphosphatidylinositol-anchored lipid transfer protein gene altered cuticular lipid composition, increased plastoglobules, and enhanced susceptibility to infection by the fungal pathogen Alternaria brassicicola. Plant Physiol. 150, 42–54. doi: 10.1104/pp.109.137745
Lei, L., Chen, L., Shi, X., Li, Y., Wang, J., Chen, D., et al. (2014). A nodule-specific lipid transfer protein AsE246 participates in transport of plant-synthesized lipids to symbiosome membrane and is essential for nodule organogenesis in Chinese milk vetch. Plant Physiol. 164, 1045–1058. doi: 10.1104/pp.113.232637
Li, C., Wang, A., Ma, X., Pourkheirandish, M., Sakuma, S., Wang, N., et al. (2013). An eceriferum locus, cer-zv, is associated with a defect in cutin responsible for water retention in barley (Hordeum vulgare) leaves. Theor. Appl. Genet. 126, 637–646. doi: 10.1007/s00122-012-2007-3
Liu, F., Xiong, X., Wu, L., Fu, D., Hayward, A., Zeng, X., et al. (2014). BraLTP1, a lipid transfer protein gene involved in epicuticular wax deposition, cell proliferation and flower development in Brassica napus. PLoS ONE 9:e110272. doi: 10.1371/journal.pone.0110272
Liu, F., Zhang, X., Lu, C., Zeng, X., Li, Y., Fu, D., et al. (2015). Non-specific lipid transfer proteins in plants: presenting new advances and an integrated functional analysis. J. Exp. Bot. 66, 5663–5681. doi: 10.1093/jxb/erv313
Livak, K. J., and Schmittgen, T. D. (2001). Analysis of relative gene expression data using real-time quantitative PCR and the 2(-Delta Delta C(T)) method. Methods 25, 402–408. doi: 10.1006/meth.2001.1262
Luo, B., Xue, X. Y., Hu, W. L., Wang, L. J., and Chen, X. Y. (2007). An ABC transporter gene of Arabidopsis thaliana, AtWBC11, is involved in cuticle development and prevention of organ fusion. Plant Cell Physiol. 48, 1790–1802. doi: 10.1093/pcp/pcm152
Mao, B., Cheng, Z., Lei, C., Xu, F., Gao, S., Ren, Y., et al. (2012). Wax crystal-sparse leaf2, a rice homologue of WAX2/GL1, is involved in synthesis of leaf cuticular wax. Planta 235, 39–52. doi: 10.1007/s00425-011-1481-1
Merzlyak, E. M., Goedhart, J., Shcherbo, D., Bulina, M. E., Shcheglov, A. S., Fradkov, A. F., et al. (2007). Bright monomeric red fluorescent protein with an extended fluorescence lifetime. Nat. Methods 4, 555–557. doi: 10.1038/nmeth1062
Nanjo, Y., Oka, H., Ikarashi, N., Kaneko, K., Kitajima, A., Mitsui, T., et al. (2006). Rice plastidial N-glycosylated nucleotide pyrophosphatase/phosphodiesterase is transported from the ER-golgi to the chloroplast through the secretory pathway. Plant Cell 18, 2582–2592. doi: 10.1105/tpc.105.039891
Nelson, B. K., Cai, X., and Nebenfuhr, A. (2007). A multicolored set of in vivo organelle markers for co-localization studies in Arabidopsis and other plants. Plant J. 51, 1126–1136. doi: 10.1111/j.1365-313X.2007.03212.x
Nieuwland, J., Feron, R., Huisman, B. A., Fasolino, A., Hilbers, C. W., Derksen, J., et al. (2005). Lipid transfer proteins enhance cell wall extension in tobacco. Plant Cell 17, 2009–2019. doi: 10.1105/tpc.105.032094
Nishimura, S., Tatano, S., Gomi, K., Ohtani, K., Fukumoto, T., and Akimitsu, K. (2008). Chloroplast-localized nonspecific lipid transfer protein with anti-fungal activity from rough lemon. Physiol. Mol. Plant Pathol. 72, 134–140. doi: 10.1016/j.pmpp.2008.07.003
Oudin, A., Mahroug, S., Courdavault, V., Hervouet, N., Zelwer, C., Rodriguez-Concepcion, M., et al. (2007). Spatial distribution and hormonal regulation of gene products from methyl erythritol phosphate and monoterpene-secoiridoid pathways in Catharanthus roseus. Plant Mol. Biol. 65, 13–30. doi: 10.1007/s11103-007-9190-7
Pagnussat, L., Burbach, C., Baluska, F., and de la Canal, L. (2012). An extracellular lipid transfer protein is relocalized intracellularly during seed germination. J. Exp. Bot. 63, 6555–6563. doi: 10.1093/jxb/ers311
Pelletier, S., Van Orden, J., Wolf, S., Vissenberg, K., Delacourt, J., Ndong, Y. A., et al. (2010). A role for pectin de-methylesterification in a developmentally regulated growth acceleration in dark-grown Arabidopsis hypocotyls. New Phytol. 188, 726–739. doi: 10.1111/j.1469-8137.2010.03409.x
Porter, B. W., Yuen, C. Y., and Christopher, D. A. (2015). Dual protein trafficking to secretory and non-secretory cell compartments: Clear or double vision? Plant Sci. 234, 174–179. doi: 10.1016/j.plantsci.2015.02.013
Potocka, I., Baldwin, T. C., and Kurczynska, E. U. (2012). Distribution of lipid transfer protein 1 (LTP1) epitopes associated with morphogenic events during somatic embryogenesis of Arabidopsis thaliana. Plant Cell Rep. 31, 2031–2045. doi: 10.1007/s00299-012-1314-0
Pyee, J., Yu, H., and Kolattukudy, P. E. (1994). Identification of a lipid transfer protein as the major protein in the surface wax of broccoli (Brassica oleracea) leaves. Arch. Biochem. Biophys. 311, 460–468.
Reis, D., and Roland, J. C. (1974). Mise en évidence de l’organisation des parois des cellules végétales en croissance par extractions ménagées des polysaccharides associés à la cytochimie ultrastructurale. J. Microsc. 20, 271–284.
Ritzenthaler, C., Nebenfuhr, A., Movafeghi, A., Stussi-Garaud, C., Behnia, L., Pimpl, P., et al. (2002). Reevaluation of the effects of brefeldin A on plant cells using tobacco Bright Yellow 2 cells expressing Golgi-targeted green fluorescent protein and COPI antisera. Plant Cell 14, 237–261. doi: 10.1105/tpc.010237
Sainsbury, F., Thuenemann, E. C., and Lomonossoff, G. P. (2009). pEAQ: versatile expression vectors for easy and quick transient expression of heterologous proteins in plants. Plant Biotechnol. J. 7, 682–693. doi: 10.1111/j.1467-7652.2009.00434.x
Scheler, C., Lamer, S., Pan, Z., Li, X. P., Salnikow, J., and Jungblut, P. (1998). Peptide mass fingerprint sequence coverage from differently stained proteins on two-dimensional electrophoresis patterns by matrix assisted laser desorption/ionization-mass spectrometry (MALDI-MS). Electrophoresis 19, 918–927. doi: 10.1002/elps.1150190607
Seki, M., Narusaka, M., Kamiya, A., Ishida, J., Satou, M., Sakurai, T., et al. (2002). Functional annotation of a full-length Arabidopsis cDNA collection. Science 296, 141–145. doi: 10.1126/science.1071006
Suh, M. C., Samuels, A. L., Jetter, R., Kunst, L., Pollard, M., Ohlrogge, J., et al. (2005). Cuticular lipid composition, surface structure, and gene expression in Arabidopsis stem epidermis. Plant Physiol. 139, 1649–1665. doi: 10.1104/pp.105.070805
Tanaka, T., Tanaka, H., Machida, C., Watanabe, M., and Machida, Y. (2004). A new method for rapid visualization of defects in leaf cuticle reveals five intrinsic patterns of surface defects in Arabidopsis. Plant J. 37, 139–146. doi: 10.1046/j.1365-313X.2003.01946.x
Tasset, C., Bernoux, M., Jauneau, A., Pouzet, C., Brière, C., Kieffer-Jacquinod, S., et al. (2010). Autoacetylation of the Ralstonia solanacearum effector PopP2 targets a lysine residue essential for RRS1-R-mediated immunity in Arabidopsis. PLoS Pathog. 6:e1001202. doi: 10.1371/journal.ppat.1001202
Voisin, D., Nawrath, C., Kurdyukov, S., Franke, R. B., Reina-Pinto, J. J., Efremova, N., et al. (2009). Dissection of the complex phenotype in cuticular mutants of Arabidopsis reveals a role of SERRATE as a mediator. PLoS Genet. 5:e1000703. doi: 10.1371/journal.pgen.1000703
Wang, X., Zhou, W., Lu, Z., Ouyang, Y., O, C. S., and Yao, J. (2015). A lipid transfer protein, OsLTPL36, is essential for seed development and seed quality in rice. Plant Sci. 239, 200–208. doi: 10.1016/j.plantsci.2015.07.016
Winter, D., Vinegar, B., Nahal, H., Ammar, R., Wilson, G. V., and Provart, N. J. (2007). An “Electronic Fluorescent Pictograph” browser for exploring and analyzing large-scale biological data sets. PLoS ONE 2:e718. doi: 10.1371/journal.pone.0000718
Xing, Q., Creff, A., Waters, A., Tanaka, H., Goodrich, J., and Ingram, G. C. (2013). ZHOUPI controls embryonic cuticle formation via a signalling pathway involving the subtilisin protease ABNORMAL LEAF-SHAPE1 and the receptor kinases GASSHO1 and GASSHO2. Development 140, 770–779. doi: 10.1242/dev.088898
Keywords: Arabidopsis thaliana, AtLTP2, At2g38530, non-specific lipid transfer protein, cell wall, cuticle, plastid, plant
Citation: Jacq A, Pernot C, Martinez Y, Domergue F, Payré B, Jamet E, Burlat V and Pacquit VB (2017) The Arabidopsis Lipid Transfer Protein 2 (AtLTP2) Is Involved in Cuticle-Cell Wall Interface Integrity and in Etiolated Hypocotyl Permeability. Front. Plant Sci. 8:263. doi: 10.3389/fpls.2017.00263
Received: 20 September 2016; Accepted: 13 February 2017;
Published: 27 February 2017.
Edited by:John Love, University of Exeter, UK
Reviewed by:Patrick H. Masson, University of Wisconsin-Madison, USA
Heather E. McFarlane, University of Melbourne, Australia
Copyright © 2017 Jacq, Pernot, Martinez, Domergue, Payré, Jamet, Burlat and Pacquit. This is an open-access article distributed under the terms of the Creative Commons Attribution License (CC BY). The use, distribution or reproduction in other forums is permitted, provided the original author(s) or licensor are credited and that the original publication in this journal is cited, in accordance with accepted academic practice. No use, distribution or reproduction is permitted which does not comply with these terms.
*Correspondence: Valérie B. Pacquit, email@example.com
†Present address: Clémentine Pernot, University of Quebec in Abitibi-Témiscamingue, Rouyn-Noranda, QC, Canada