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PLANT PHYSIOLOGY , Vol 104, Issue 1 17-27, Copyright © 1994 by American Society of Plant Biologists
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DEVELOPMENT AND GROWTH REGULATION |
The Use of Fluorescent Tracers to Characterize the Post-Phloem Transport Pathway in Maternal Tissues of Developing Wheat Grains
N. Wang and D. B. Fisher
Department of Botany, Washington State University, Pullman, Washington 99164-4238
Various polar fluorescent tracers were used to characterize the pathways
for apoplastic and symplastic transport in the "crease tissues" (i.e. the
vascular strand, chalaza, nucellus, and adjacent pericarp) of developing
wheat (Triticum aestivum L.) grains. With mostly minor exceptions, the
results strongly support existing views of phloem unloading and post-phloem
transport pathways in the crease. Apoplastic movement of Lucifer yellow CH
(LYCH) from the endosperm cavity into the crease was virtually blocked in
the chalazal cell walls before reaching the vascular tissue. However, LYCH
could move slowly along the cell wall pathway from the chalaza into the
vascular parenchyma. Slow uptake of LYCH into nucellar cell cytoplasm was
observed, but no subsequent symplastic movement occurred.
Carboxyfluorescein (CF) imported into attached grains moved symplastically
from the phloem across the chalaza and into the nucellus, but was not
released from the nucellus. In addition, CF moved in the opposite direction
(nucellus to vascular parenchyma) in attached grains. Thus, the post-phloem
symplastic pathway can accommodate bidirectional transport even when there
is an intense net assimilate flux in one direction. When fresh sections of
the crease were placed in fluorochrome solutions (e.g. LYCH or pyrene
trisulfonate), dye was rapidly absorbed into intact cells, apparently via
unsealed plasmodesmata. Uptake was not visibly reduced by cold or by
respiratory inhibitors, but was greatly reduced by plasmolysis. Once
absorbed, the dye moved intercellularly via the symplast. Based on this
finding, a size-graded series of fluorescein-labeled dextrans was used to
estimate the size-exclusion limits (SEL) for the post-phloem symplastic
pathway. In most, and perhaps all, cells of the crease tissues except for
the pericarp, the molecular diameter for the SEL was about 6.2 nm. The SEL
in much of the vascular parenchyma may be smaller, but it is still at least
3.6 nm. Channel diameters would likely be about 1 nm larger, or about 4.5
to 7.0 nm in the vascular parenchyma and 7.0 nm elsewhere. These dimensions
are substantially larger than those for "conventional" symplastic
connections (about 3 nm), and would have a greater than proportionate
effect on the per channel diffusive and hydraulic conductivities of the
pathway. Thus, relatively small and probably ultrastructurally undetectable
adjustments in plasmodesmatal structure may be sufficient to account for
assimilate flux through the crease symplast.
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