Web Topic 12.3 Experiments on Phloem Loading

Susan Dunford, University of Cincinnati, Cincinnati, OH, USA

Revised by Alexander Schulz, University of Copenhagen, Copenhagen, Denmark
(September 2021)

In its narrow sense, the term “phloem loading” refers only to the last step of assimilate transfer from bundle sheath or phloem parenchyma into the sieve element-companion cell complexes. The steps before are called pre-phloem transport that generally makes use of plasmodesmata between all cells up to the bundle sheath. The driving force for this transport is diffusion in apoplastically loading plants, but might contain a component of mass flow (advective flow) in symplasmically loading plant species (Schulz, 2015; Comtet et al., 2017).

Evidence for Apoplastic Loading of Sieve Elements

Early research on phloem loading focused on the apoplastic pathway (see textbook Figure 6.4). Many studies devoted to testing these predictions have provided solid evidence for apoplastic loading in several species. Some of the more important evidence is:

1. Transport sugars are found in the apoplast. Sucrose is the predominant apoplastic sugar in species that transport mainly sucrose in the phloem, for example, sugar beet (Beta vulgaris) and broad bean (Vicia faba). Treatments and events that alter the rate of translocation from the source leaf also change the flux of sucrose through the apoplast (Geiger et al., 1974) or the apoplastic sucrose level.
2. Sucrose supplied exogenously to a source leaf of sugar beet accumulates in the sieve elements and companion cells of the minor veins, as does sucrose derived from photosynthetic CO₂ fixation (see textbook Figure 12.11). Similar observations have been made in broad bean, pea (Pisum sativum), castor bean (Ricinus communis), and other species.
3. PCMBS (p-chloromercuribenzenesulfonic acid) is a reagent that inhibits the transport of sucrose across plasma membranes but does not enter the symplasm. PCMBS inhibits the uptake of sucrose from the apoplast when the sugar is supplied exogenously to sugar beet. Of greater importance, PCMBS also inhibits the export of sucrose synthesized from CO₂ in the mesophyll, implying that short-distance transport in sugar beet normally includes an apoplastic step (Giaquinta, 1976; Web Figure 12.3.A). Assimilate loading is also inhibited by PCMBS in broad bean, pea, and other species.
4. Experiments with transgenic plants further support the interpretation that sucrose moves through the apoplast. (Transgenic organisms carry cloned genes integrated into their DNA by a variety of recombinant-DNA techniques.) Transgenic tomato plants that have a sucrose-cleaving enzyme (invertase) in their apoplast show a very slow growth rate and fail to mobilize the starch in their source leaves during a prolonged dark period (Dickinson et al., 1991). Apparently, hydrolyzing sucrose in the apoplast inhibits phloem loading in source leaves of this species. This result is expected only if the phloem-loading pathway includes an apoplastic step.

Web Figure 12.3.A Effects of PCMBS on phloem transport from a sugar beet leaf. Export pf labeled photosynthate from a sugar beet leaf decreases upon addition of PCMBS. Photosynthesis was not affected, indicating that PCMBS did not alter the photosynthetic carbon fixation of the leaf. (From Fischer, 2000; after Giaquinta, 1976.)

Some Substances Enter the Phloem by Diffusion

Many substances, such as organic acids and plant hormones, are found in the phloem sap at lower concentrations than carbohydrates. These substances are probably not actively loaded into the sieve element–companion cell complex but enter the sieve elements via other pathways and mechanisms. They may be taken up directly by diffusion across the phospholipid bilayer of the plasma membrane of the sieve element–companion cell complex or by a passive transporter in the plasma membrane of those cells, or they may diffuse into the sieve elements via the symplasm.

Once in the sieve elements, these substances are swept along in the translocation stream by bulk flow, the motive force being generated by the active loading of only certain sugars or amino acids. Many substances not normally found in plants, such as herbicides and fungicides, can be transported in the phloem because of their ability to diffuse through membranes at an intermediate rate. In other words, they diffuse through membranes rapidly enough to allow considerable accumulation in the sieve elements, but slowly enough that they are not lost from the sieve elements completely before reaching a sink tissue. In addition, compounds that are weakly acidic tend to be “trapped” within the sieve elements, becoming negatively charged in the basic environment (low H⁺ concentration) of the sieve elements and thus less likely to diffuse out of the cells across the hydrophobic membrane (Kleier, 1988). Substances that are not transported in the phloem (such as calcium ions) may not enter the sieve elements at all. The Arabidopsis gene AUX1 (auxin influx carrier) encodes an auxin permease that appears to function as an auxin carrier (Swarup et al., 2001; Marchant et al., 2002; see textbook Figure 4.29). AUX1 has been localized in protophloem cells in the root (Swarup et al., 2001). Gene expression studies have shown that AUX1 facilitates IAA loading into the leaf vascular transport system, and IAA unloading in the primary root apex and developing lateral root primordium (Marchant et al., 2002).

The Roles of Sucrose-H⁺ Symporters in the Phloem of Apoplastic Loaders

Sucrose transporters are postulated to load photosynthetically produced sucrose into the sieve elements of apoplastic loaders (see textbook Figure 12.12). The carriers are found in plasma membranes of either sieve elements or companion cells. Carriers found in sieve element membranes includ1e SUT1, SUT2, and SUT4, in potato (Solanum tuberosum) and tomato. SUC2 has been found in the companion cell plasma membranes of Arabidopsis and plantain

As shown in Web Figure 12.3.B, SUC2, one of the major sucrose transporters involved in phloem loading, is found in the companion cells. Mutant Arabidopsis plants containing transferred DNA insertions in the gene encoding SUC2 have been recently identified by reverse genetics (Gottwald et al., 2000). In the homozygous state, these mutations resulted in stunted growth, retarded development, and sterility. The source leaves of mutant plants contained a great excess of starch, and radiolabeled sugar failed to be transported efficiently to roots and inflorescences.

Web Figure 12.3.B This micrograph shows a single companion cell from broad-leaved plantain (Plantago major) stained with two fluorescent dyes. One of the dyes (green) is (indirectly) linked to an antibody that is specific for the PmSUC2 sucrose–H⁺ symporter. The second dye (blue) binds to DNA. Since the two dyes are found on a single phloem cell, which is always adjacent to a sieve element, the sucrose symporter is located in the companion cell membrane in this species. (From (Stadler et al., 1995). Interestingly, expression of the SUC2 transporter begins in the tip and proceeds to the base in developing leaves during a sink-to-source transition, the same pattern shown by photosynthate export capacity.

Work with SUT1 has shown that the messenger RNAs for symporters found in the sieve element membrane are synthesized in the companion cells (Kühn et al., 1997; Vaughn et al., 2002). This finding agrees with the fact that sieve elements lack nuclei. The symporter protein is probably also synthesized in the companion cells since ribosomes do not appear to persist in mature sieve elements.

All sucrose transporters fall into one of three large subfamilies; the roles played by the many of the carriers are still being investigated. SUT1 and SUC2 appear to be the major sucrose transporters in phloem loading, into either companion cells or sieve elements. Additional functions of these and the other sucrose transporters include sucrose retrieval from the apoplast following leakage from the transport stream, transport of sucrose from the vacuole to the cytoplasm, sucrose uptake into germinating pollen, and sucrose release into the apoplast of developing seeds. (See Section 12.6 Phloem Unloading and Sink-to-Source Transition in the textbook.)

Studies Supporting the Oligomer-Trapping Model of Symplasmic Loading

Many studies support the oligomer-trapping model. For instance, the enzymes required to synthesize stachyose from sucrose are localized in intermediary cells. In melon, raffinose and stachyose are present in high concentrations in intermediary cells, but not in mesophyll cells. Some plants seem to be able to making use of different loading strategies (Slewinski et al., 2013). Not only for passive symplasmically loading plants, mostly trees, but also for the oligomer-trapping model, a mass flow via plasmodesmata has also been proposed as a mechanism for symplasmic entry of solutes into the phloem (Dölger et al., 2014; Comtet et al., 2017).

Relationships between Loading Characteristics and Loading Mechanisms

What characteristic—type of companion cell, transport sugars, or abundance of plasmodesmata—is the best predictor of symplasmic loading? The number of plasmodesmata linking the sieve element–companion cell complex and surrounding cells has often been considered to be diagnostic for loading type. However, some species that had been classified as symplasmic loaders based on plasmodesmatal frequencies have now been shown to load apoplastically. Plants with abundant plasmodesmata in the minor vein phloem also tend to possess abundant plasmodesmata between mesophyll cells, so plasmodesmatal frequencies may be related to some other plant characteristic. In conclusion, the presence of abundant plasmodesmata is necessary for the symplasmic loading type, but not sufficient to predict this mode.

The type of transport sugar (sucrose alone or sucrose plus larger oligosaccharides) can differentiate between oligomer trapping and the other loading strategies. Autoradiographs of leaf discs fed ¹⁴C-sucrose can then be used to distinguish between apoplastic loading and passive symplasmic loading. In species which concentrate sugars in the phloem (apoplastic loading and oligomer trapping), the veins should be clearly visible on the autoradiographs. In species which move sugars from the mesophyll into the phloem by means of diffusion down a concentration gradient, veins should not be visible on the autoradiographs. Web Figure 12.3.C confirms these expectations in the three loading types.

Web Figure 12.3.C Autoradiographs of leaf discs from species which load by oligomer trapping (left, twining snapdragon, Asarina scandens), from the apoplast (middle, celery, Apium graveolens), and by passive diffusion through the symplasm (right, cherry laurel, Prunus laurocerasus). The leaves were treated just like the sugar beet leaf in textbook Figure 12.11, except that the labeling period was 1 h. Label (black) accumulated in the species which concentrate sugars in the minor veins, by oligomer trapping (left) and by active loading from the apoplast (middle), but not in the species that loads via passive diffusion (right). (Rennie and Turgeon, 2009.)

Several species have more than one type of companion cell in their minor veins. For example, coleus has both intermediary cells and ordinary companion cells. It has been suggested that active and passive loading may coexist in some species, simultaneously or at different times, in different sieve elements in the same vein. However, symplasmic and apoplastic pathways do not exist in the same sieve element-companion cell complex, due to restrictions imposed by anatomical features, such as plasmodesmatal frequencies.

References

Comtet J, Turgeon R, Stroock A (2017) Phloem Loading through Plasmodesmata: A Biophysical Analysis. Plant Physiology 175: 904–915.

Dickinson CD, Altabella T, Chrispeels MJ (1991) Slow-growth phenotype of transgenic tomato expressing apoplastic invertase. Plant Physiology 95: 420–425.

Dölger J, Rademaker H, Liesche J, Schulz A, Bohr T (2014) Diffusion and bulk flow in phloem loading: a theoretical analysis of the polymer trap mechanism for sugar transport in plants. Phys Rev E Stat Nonlin Soft Matter Phys 90: 042704.

Fischer DB (2000) Long-distance transport. In B Buchanan, W Gruissem, RL Jones, eds, Biochemistry and Molecular Biology of Plants. American Society of Plant Physiologists, Rockville, Md., pp 730–784.

Geiger DR, Sovonick SA, Shock TL, Fellows RJ (1974) Role of Free Space in Translocation in Sugar-Beet. Plant Physiology 54: 892–898.

Giaquinta R (1976) Evidence for Phloem Loading from Apoplast - Chemical Modification of Membrane Sulfhydryl-Groups. Plant Physiology 57: 872–875.

Gottwald JR, Krysan PJ, Young JC, Evert RF, Sussman MR (2000) Genetic evidence for the in planta role of phloem-specific plasma membrane sucrose transporters. Proc Natl Acad Sci USA 97: 13979–13984.

Kleier DA (1988) Phloem Mobility of Xenobiotics .1. Mathematical-Model Unifying the Weak Acid and Intermediate Permeability Theories. Plant Physiology 86: 803–810.

Kühn C, Franceschi VR, Schulz A, Lemoine R, Frommer WB (1997) Macromolecular trafficking indicated by localization and turnover of sucrose transporters in enucleate sieve elements. Science 275: 1298–1300.

Marchant A, Bhalerao R, Casimiro I, Eklof J, Casero PJ, Bennett M, Sandberg G (2002) AUX1 promotes lateral root formation by facilitating indole-3-acetic acid distribution between sink and source tissues in the Arabidopsis seedling. Plant Cell 14: 589–597.

Rennie EA, Turgeon R (2009) A comprehensive picture of phloem loading strategies. Proc Natl Acad Sci USA 106: 14162–14167.

Schulz A (2015) Diffusion or bulk flow: how plasmodesmata facilitate pre-phloem transport of assimilates. J Plant Res 128: 49–61.

Slewinski TL, Zhang C, Turgeon R (2013) Structural and functional heterogeneity in phloem loading and transport. Front Plant Sci 4: 244.

Stadler R, Brandner J, Schulz A, Gahrtz M, Sauer N (1995) Phloem loading by the PMSUC2 sucrose carrier from Plantago-major occurs into companion cells. Plant Cell 7: 1545–1554.

Swarup R, Friml J, Marchant A, Ljung K, Sandberg G, Palme K, Bennett M (2001) Localization of the auxin permease AUX1 suggests two functionally distinct hormone transport pathways operate in the Arabidopsis root apex. Genes Dev 15: 2648–2653.

Vaughn MW, Harrington GN, Bush DR (2002) Sucrose-mediated transcriptional regulation of sucrose symporter activity in the phloem. Proc Natl Acad Sci USA 99: 10876–10880.