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对于人工筛管的某些性能。

Forisome performance in artificial sieve tubes.

机构信息

School of Biological Sciences, Washington State University, Pullman, WA 99164-4236, USA.

出版信息

Plant Cell Environ. 2012 Aug;35(8):1419-27. doi: 10.1111/j.1365-3040.2012.02499.x. Epub 2012 Mar 14.

Abstract

In the legume phloem, sieve element occlusion (SEO) proteins assemble into Ca(2+)-dependent contractile bodies. These forisomes presumably control phloem transport by forming reversible sieve tube plugs. This function, however, has never been directly demonstrated, and appears questionable as forisomes were reported to be too small to plug sieve tubes, and failed to block flow efficiently in artificial microchannels. Moreover, plugs of SEO-related proteins in Arabidopsis sieve tubes do not affect phloem translocation. We improved existing procedures for forisome isolation and storage, and found that the degree of Ca(2+)-driven deformation that is possible in forisomes of Vicia faba, the standard object of earlier research, has been underestimated substantially. Forisomes deform particularly strongly under reducing conditions and high sugar concentrations, as typically found in sieve tubes. In contrast to our previous inference, Ca(2+)-inducible forisome swelling certainly seems sufficient to plug sieve tubes. This conclusion was supported by 3D-reconstructions of forisome plugs in Canavalia gladiata. For a direct test, we built microfluidics chips with artificial sieve tubes. Using fluorescent dyes to visualize flow, we demonstrated the complete blockage of these biomimetic microtubes by Ca(2+)-induced forisome plugs, and concluded by analogy that forisomes are capable of regulating phloem flow in vivo.

摘要

在豆科植物韧皮部中,筛分子阻塞(SEO)蛋白组装成依赖 Ca2+的收缩体。这些胞间连丝可能通过形成可逆的筛管塞来控制韧皮部运输。然而,这个功能从未被直接证明过,而且似乎值得怀疑,因为胞间连丝被报道过小到无法堵塞筛管,并且在人工微通道中不能有效地阻止流动。此外,拟南芥筛管中与 SEO 相关的蛋白质塞并不影响韧皮部转运。我们改进了胞间连丝的分离和储存的现有程序,并发现蚕豆中胞间连丝的 Ca2+驱动变形程度被大大低估了,蚕豆是早期研究的标准对象。胞间连丝在还原条件和高糖浓度下特别强烈变形,如通常在筛管中发现的那样。与我们之前的推断相反,Ca2+诱导的胞间连丝肿胀似乎足以堵塞筛管。这一结论得到了 Canavalia gladiata 中胞间连丝塞的 3D 重建的支持。为了进行直接测试,我们构建了带有人工筛管的微流控芯片。我们使用荧光染料来可视化流动,证明了 Ca2+诱导的胞间连丝塞完全阻塞了这些仿生微管,并通过类比得出结论,胞间连丝能够在体内调节韧皮部流动。

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