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Sieve Tube Unloading and Post-Phloem Transport of Fluorescent Tracers and Proteins Injected into Sieve Tubes via Severed Aphid Stylets1

机译:筛管卸载以及通过切断的蚜虫Stylets注入筛管的荧光示踪剂和蛋白质的韧皮部后转运1

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摘要

A variety of fluorescent tracers and proteins were injected via severed aphid stylets into the sieve tubes of wheat (Triticum aestivum L.) grains to evaluate the dimensions of plasmodesmal channels involved in sieve element/companion cell (SE/CC) unloading and post-phloem transport. In the post-phloem pathway, where diffusion is the predominant mode of transport, the largest molecule to show mobility was 16-kD dextran, with a Stokes radius of 2.6 nm. This suggests that the aqueous channels for cell-to-cell transport must be about 8 nm in diameter. Even the largest tracer injected into the sieve tubes, 400-kD fluorescein-labeled Ficoll with a Stokes radius of about 11 nm, was unloaded from the SE/CC complex. However, in contrast to smaller tracers (≤3 kD, with a Stokes radius ≤ 1.2 nm), the unloading of fluorescein-labeled Ficoll and other large molecules from the SE/CC complex showed an irregular, patchy distribution, with no further movement along the post-phloem pathway. Either the plasmodesmal channels involved in SE/CC unloading are exceptionally large (perhaps as much as 42 nm in diameter), with only a very small fraction of plasmodesmata being conductive, or the larger tracers damage the plasmodesmata in some way, enlarging smaller channels.
机译:通过切断的蚜虫探针将各种荧光示踪剂和蛋白质注入小麦(Triticum aestivum L.)谷物的筛管中,以评估参与筛分/伴侣细胞(SE / CC)卸载和韧皮部后的胞膜通道的尺寸运输。在韧皮部后途径中,扩散是主要的运输方式,显示迁移率的最大分子是16 kD葡聚糖,斯托克斯半径为2.6 nm。这表明用于细胞间运输的水通道的直径必须约为8 nm。即使是注入到筛管中的最大示踪剂,400 kD荧光标记的Ficoll,斯托克斯半径约为11 nm,也已从SE / CC复合物中卸载。但是,与较小的示踪剂(≤3 kD,斯托克斯半径≤1.2 nm)相比,荧光素标记的Ficoll和其他大分子从SE / CC络合物中的卸载显示出不规则的,斑片状分布,并且没有进一步的移动韧皮部后途径。 SE / CC卸载所涉及的质膜通道异常大(直径可能高达42 nm),只有极小部分的质膜导电,或者较大的示踪剂以某种方式破坏了质膜,扩大了较小的通道。

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