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CAGEs 是定位于高尔基体的 GT31 酶,参与拟南芥纤维素的生物合成。

CAGEs are Golgi-localized GT31 enzymes involved in cellulose biosynthesis in Arabidopsis.

机构信息

Department of Forest Genetics and Plant Physiology, Umeå Plant Science Centre, Swedish University of Agricultural Sciences, 901 83, Umeå, Sweden.

出版信息

Plant J. 2022 Jun;110(5):1271-1285. doi: 10.1111/tpj.15734. Epub 2022 Mar 31.

Abstract

Cellulose is the main structural component in the plant cell walls. We show that two glycosyltransferase family 31 (GT31) enzymes of Arabidopsis thaliana, here named cellulose synthesis associated glycosyltransferases 1 and 2 (CAGE1 and 2), influence both primary and secondary cell wall cellulose biosynthesis. cage1cage2 mutants show primary cell wall defects manifesting as impaired growth and cell expansion in seedlings and etiolated hypocotyls, along with secondary cell wall defects, apparent as collapsed xylem vessels and reduced xylem wall thickness in the inflorescence stem. Single and double cage mutants also show increased sensitivity to the cellulose biosynthesis inhibitor isoxaben. The cage1cage2 phenotypes were associated with an approximately 30% reduction in cellulose content, an approximately 50% reduction in secondary cell wall CELLULOSE SYNTHASE (CESA) protein levels in stems and reduced cellulose biosynthesis rate in seedlings. CESA transcript levels were not significantly altered in cage1cage2 mutants, suggesting that the reduction in CESA levels was caused by a post-transcriptional mechanism. Both CAGE1 and 2 localize to the Golgi apparatus and are predicted to synthesize β-1,3-galactans on arabinogalactan proteins. In line with this, the cage1cage2 mutants exhibit reduced levels of β-Yariv binding to arabinogalactan protein linked β-1,3-galactan. This leads us to hypothesize that defects in arabinogalactan biosynthesis underlie the cellulose deficiency of the mutants.

摘要

纤维素是植物细胞壁的主要结构成分。我们表明,拟南芥中有两种糖基转移酶家族 31(GT31)酶,分别命名为纤维素合成相关糖基转移酶 1 和 2(CAGE1 和 2),它们影响初生细胞壁和次生细胞壁纤维素的生物合成。cage1cage2 突变体表现出初生细胞壁缺陷,表现在幼苗和黄化下胚轴生长和细胞扩展受损,同时也表现出次生细胞壁缺陷,表现在花序茎中木质部导管塌陷和木质部细胞壁厚度减小。单突变体和双突变体也表现出对纤维素生物合成抑制剂异羟肟酸的敏感性增加。cage1cage2 表型与纤维素含量降低约 30%、茎中次生细胞壁纤维素合酶(CESA)蛋白水平降低约 50%以及幼苗中纤维素生物合成速率降低有关。cage1cage2 突变体中的 CESA 转录本水平没有显著改变,这表明 CESA 水平的降低是由转录后机制引起的。CAGE1 和 2 都定位于高尔基体,预计在阿拉伯半乳聚糖蛋白上合成β-1,3-半乳糖。与此一致的是,cage1cage2 突变体表现出阿拉伯半乳聚糖蛋白连接的β-1,3-半乳糖的β-Yariv 结合水平降低。这使我们假设突变体中阿拉伯半乳聚糖生物合成的缺陷是纤维素缺乏的基础。

https://cdn.ncbi.nlm.nih.gov/pmc/blobs/1427/9321575/0d9786e03c28/TPJ-110-1271-g005.jpg

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