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烟草花粉管生长过程中类葡聚糖合酶蛋白NaGSL1的分子调控及胼胝质合成

Molecular control of the glucan synthase-like protein NaGSL1 and callose synthesis during growth of Nicotiana alata pollen tubes.

作者信息

Brownfield Lynette, Wilson Sarah, Newbigin Ed, Bacic Antony, Read Steve

机构信息

Plant Cell Biology Research Centre, School of Botany, University of Melbourne, VIC 3010, Australia.

出版信息

Biochem J. 2008 Aug 15;414(1):43-52. doi: 10.1042/BJ20080693.

DOI:10.1042/BJ20080693
PMID:18462191
Abstract

The protein NaGSL1 (Nicotiana alata glucan synthase-like 1) is implicated in the synthesis of callose, the 1,3-beta-glucan that is the major polysaccharide in the walls of N. alata (flowering tobacco) pollen tubes. Here we examine the production, intracellular location and post-translational processing of NaGSL1, and relate each of these to the control of pollen-tube callose synthase (CalS). The 220 kDa NaGSL1 polypeptide is produced after pollen-tube germination and accumulates during pollen-tube growth, as does CalS. A combination of membrane fractionation and immunoelectron microscopy revealed that NaGSL1 was present predominantly in the endoplasmic reticulum and Golgi membranes in younger pollen tubes when CalS was mostly in an inactive (latent) form. In later stages of pollen-tube growth, when CalS was present in both latent and active forms, a greater proportion of NaGSL1 was in intracellular vesicles and the plasma membrane, the latter location being consistent with direct deposition of callose into the wall. N. alata CalS is activated in vitro by the proteolytic enzyme trypsin and the detergent CHAPS, but in neither case was activation associated with a detectable change in the molecular mass of the NaGSL1 polypeptide. NaGSL1 may thus either be activated by the removal of a few amino acids or by the removal of another protein that inhibits NaGSL1. These findings are discussed in relation to the control of callose biosynthesis during pollen germination and pollen-tube growth.

摘要

蛋白质NaGSL1(烟草葡聚糖合酶样蛋白1)与胼胝质的合成有关,胼胝质是一种1,3-β-葡聚糖,是烟草花粉管细胞壁中的主要多糖。在此,我们研究了NaGSL1的产生、细胞内定位和翻译后加工,并将其中每一项与花粉管胼胝质合酶(CalS)的调控联系起来。220 kDa的NaGSL1多肽在花粉管萌发后产生,并在花粉管生长过程中积累,CalS也是如此。膜分级分离和免疫电子显微镜相结合的方法显示,当CalS大多处于无活性(潜伏)形式时,NaGSL1主要存在于较年轻花粉管的内质网和高尔基体膜中。在花粉管生长的后期阶段,当CalS以潜伏和活性两种形式存在时,更大比例的NaGSL1存在于细胞内囊泡和质膜中,后者的位置与胼胝质直接沉积到细胞壁中一致。烟草CalS在体外可被蛋白酶胰蛋白酶和去污剂CHAPS激活,但在这两种情况下,激活都与NaGSL1多肽分子量的可检测变化无关。因此,NaGSL1可能通过去除几个氨基酸或去除另一种抑制NaGSL1的蛋白质而被激活。本文结合花粉萌发和花粉管生长过程中胼胝质生物合成的调控对这些发现进行了讨论。

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