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受磷酸盐饥饿调控的拟南芥甘露糖结合凝集素(AtGAL1)与分泌型紫色酸性磷酸酶 AtPAP26 的糖型共同纯化。

A glycoform of the secreted purple acid phosphatase AtPAP26 co-purifies with a mannose-binding lectin (AtGAL1) upregulated by phosphate-starved Arabidopsis.

机构信息

Department of Biology, Queen's University, Kingston, Canada.

Oncolytics Biotech Inc., Calgary, Canada.

出版信息

Plant Cell Environ. 2019 Apr;42(4):1139-1157. doi: 10.1111/pce.13432. Epub 2019 Jan 18.

DOI:10.1111/pce.13432
PMID:30156702
Abstract

The purple acid phosphatase AtPAP26 plays a central role in Pi-scavenging by Pi-starved (-Pi) Arabidopsis. Mass spectrometry (MS) of AtPAP26-S1 and AtPAP26-S2 glycoforms secreted by -Pi suspension cells demonstrated that N-glycans at Asn and Asn were modified in AtPAP26-S2 to form high-mannose glycans. A 55-kDa protein that co-purified with AtPAP26-S2 was identified as a Galanthus nivalis agglutinin-related and apple domain lectin-1 (AtGAL1; At1g78850). MS revealed that AtGAL1 was bisphosphorylated at Tyr and Thr and glycosylated at four conserved Asn residues. When AtGAL was incubated in the presence of a thiol-reducing reagent prior to immunoblotting, its cross-reactivity with anti-AtGAL1-IgG was markedly attenuated (consistent with three predicted disulfide bonds in AtGAL1's apple domain). Secreted AtGAL1 polypeptides were upregulated to a far greater extent than AtGAL1 transcripts during Pi deprivation, indicating posttranscriptional control of AtGAL1 expression. Growth of a -Pi atgal1 mutant was unaffected, possibly due to compensation by AtGAL1's closest paralog, AtGAL2 (At1g78860). Nevertheless, AtGAL1's induction by numerous stresses combined with the broad distribution of AtGAL1-like lectins in diverse species implies an important function for AtGAL1 orthologs within the plant kingdom. We hypothesize that binding of AtPAP26-S2's high-mannose glycans by AtGAL1 enhances AtPAP26 function to facilitate Pi-scavenging by -Pi Arabidopsis.

摘要

紫色酸性磷酸酶 AtPAP26 在缺磷(-Pi)拟南芥的 Pi 清除中发挥核心作用。对 -Pi 悬浮细胞分泌的 AtPAP26-S1 和 AtPAP26-S2 糖型的质谱(MS)分析表明,AtPAP26-S2 中 Asn 和 Asn 的 N-糖链被修饰为高甘露糖糖链。与 AtPAP26-S2 共纯化的 55kDa 蛋白被鉴定为雪花莲凝集素相关和苹果结构域凝集素-1(AtGAL1;At1g78850)。MS 显示 AtGAL1 在 Tyr 和 Thr 处双磷酸化,并在四个保守的 Asn 残基处糖基化。当 AtGAL 在免疫印迹前用巯基还原试剂孵育时,其与抗 AtGAL1-IgG 的交叉反应性显著减弱(与 AtGAL1 的苹果结构域中三个预测的二硫键一致)。在缺磷条件下,分泌的 AtGAL1 多肽的上调幅度远高于 AtGAL1 转录物,表明 AtGAL1 表达受到转录后调控。-Pi atgal1 突变体的生长不受影响,这可能是由于 AtGAL1 最接近的同源物 AtGAL2(At1g78860)的补偿作用。尽管如此,AtGAL1 被多种胁迫诱导,并且在不同物种中存在广泛分布的 AtGAL1 样凝集素,这意味着 AtGAL1 同源物在植物界中具有重要功能。我们假设 AtGAL1 结合 AtPAP26-S2 的高甘露糖糖链增强了 AtPAP26 的功能,从而促进了 -Pi 拟南芥的 Pi 清除。

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