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盐胁迫上调周质阿拉伯半乳聚糖蛋白:利用盐胁迫分析阿拉伯半乳聚糖蛋白的功能

Salt stress upregulates periplasmic arabinogalactan proteins: using salt stress to analyse AGP function.

作者信息

Lamport Derek T A, Kieliszewski Marcia J, Showalter Allan M

机构信息

School of Life Sciences, John Maynard Smith Building, University of Sussex, Falmer, Brighton BN1 9QG, UK.

出版信息

New Phytol. 2006;169(3):479-92. doi: 10.1111/j.1469-8137.2005.01591.x.

Abstract

Arabinogalactan proteins (AGPs) are implicated in cell expansion by unknown mechanisms, thus AGP content and cell-expansion rate might be correlated. We used Yariv reagent to quantify release rates and distribution of AGP at the cell surface of tobacco BY-2 cells: plasma membrane (M); soluble periplasmic AGPs released by cell rupture (S); cell wall (W); and growth medium (Gsink). In contrast to earlier reports, we observed massive upregulation of AGPs in salt-stressed cells, and hence the absence of a simple, direct cause-and-effect relationship between growth rate and AGP release. There was a more subtle connection. A dynamic flux model, M-->S-->W-->Gsink, indicated that turnover was nondegradative, with little free diffusion of AGPs trapped in the pectic matrix of nonadapted cells where transmural migration of high molecular-weight AGPs occurred mainly by plug flow (apposition and extrusion). In contrast, however, an up to sixfold increased AGP release rate in the slower-growing salt-adapted cells indicated a greatly increased rate of AGP diffusion through a much more highly porous pectic network. We hypothesize that classical AGPs act as pectin plasticizers. This explains how beta-D-glycosyl Yariv reagents might inhibit expansion growth by crosslinking monomeric AGPs, and thus mimic an AGP loss-of-function mutation.

摘要

阿拉伯半乳聚糖蛋白(AGPs)通过未知机制参与细胞扩张,因此AGP含量与细胞扩张速率可能相关。我们使用亚力夫试剂来量化AGP在烟草BY - 2细胞表面的释放速率和分布:质膜(M);细胞破裂释放的可溶性周质AGPs(S);细胞壁(W);以及生长培养基(Gsink)。与早期报告相反,我们观察到盐胁迫细胞中AGPs大量上调,因此生长速率与AGP释放之间不存在简单的直接因果关系。存在一种更微妙的联系。一个动态通量模型,M→S→W→Gsink,表明周转是非降解性的,被困在未适应细胞果胶基质中的AGPs几乎没有自由扩散,在未适应细胞中,高分子量AGPs的跨膜迁移主要通过活塞流(附着和挤出)发生。然而,相比之下,在生长较慢的盐适应细胞中AGP释放速率增加了高达六倍,这表明AGP通过一个孔隙率高得多的果胶网络的扩散速率大大增加。我们假设经典AGPs充当果胶增塑剂。这解释了β - D - 糖基亚力夫试剂如何通过交联单体AGPs来抑制扩张生长,从而模拟AGP功能丧失突变。

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