Lectin AtGAL1 interacts with high‐mannose glycoform of the purple acid phosphatase AtPAP26 secreted by phosphate‐starved <i>Arabidopsis</i>

Ghahremani, Mina; Park, Joonho; Anderson, Erin M.; Marty‐Howard, Naomi J.; Mullen, Robert T.; Plaxton, William C.

doi:10.1111/pce.13463

Cited by 18 publications

(12 citation statements)

References 36 publications

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“…Since their discovery in mammals, many PAP isoforms have also been purified from plant tissues ( del Pozo et al , 1999 ; Miller et al , 2001 ; Bozzo et al , 2004 ), and the physiological functions of a number of them have been characterized, most of which are related to P nutrition ( Tran et al , 2010b ; Wang et al , 2011 ; Robinson et al , 2012 ; Lu et al , 2016 ; Li et al , 2017 ; Mehra et al , 2017 ; Wu et al , 2018 ). In Arabidopsis, AtPAP12 and AtPAP26 have been shown to be the predominant PAP isozymes that are secreted into the medium under Pi starvation ( Tran et al , 2010b ; Ghahremani et al , 2019 ). Mutations of AtPAP12 and AtPAP26 result in a significant reduction in the activity of secreted APases and hence in the ability to utilize extracellular Po ( Robinson et al , 2012 ).…”

Section: Introductionmentioning

confidence: 99%

Purple acid phosphatase 10c encodes a major acid phosphatase that regulates plant growth under phosphate-deficient conditions in rice

Deng

et al. 2020

Journal of Experimental Botany

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Abstract Whilst constitutive overexpression of particular acid phosphatases (APases) can increase utilization of extracellular organic phosphate, negative effects are frequently observed in these transgenic plants under conditions of inorganic phosphate (Pi) sufficiency. In this study, we identified rice purple acid phosphatase 10c (OsPAP10c) as being a novel and major APase that exhibits activities associated both with the root surface and with secretion. Two constructs were used to generate the OsPAP10c-overexpression plants by driving its coding sequence with either a ubiquitin promoter (UP) or the OsPAP10c-native promoter (NP). Compared with the UP transgenic plants, lower expression levels and APase activities were observed in the NP plants. However, the UP and NP plants both showed a similar ability to degrade extracellular ATP and both promoted root growth. The growth performance and yield of the NP transgenic plants were better than the wild-type and UP plants in both hydroponic and field experiments irrespective of the level of Pi supply. Overexpression of APase by its native promoter therefore provides a potential way to improve crop production that might avoid increased APase activity in untargeted tissues and its inhibition of the growth of transgenic plants.

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Section: Introductionmentioning

confidence: 99%

Purple acid phosphatase 10c encodes a major acid phosphatase that regulates plant growth under phosphate-deficient conditions in rice

Deng

et al. 2020

Journal of Experimental Botany

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“…A combination of systemic 'omic' (Li et al, 2008;Tran and Plaxton, 2008;Plaxton and Tran, 2011;Plaxton and Shane, 2015;Pan et al, 2019) and targeted biochemical (Gregory et al, 2009;Liang et al, 2012;Shane et al, 2013;Ghahremani et al, 2019) studies have indicated that multiple PTMs play important roles in the PSR. These PTMs include phosphorylation, ubiquitination and glycosylation signatures that affect gene expression profiles and the activities of intra-and extracellular metabolic enzymes (Shane et al, 2013;Plaxton and Shane, 2015;Ghahremani et al, 2019;Pan et al, 2019). Targeted studies involving protein phosphorylation indicate that calcium-dependent protein kinases (CDPKs) are probably protein-level PTM regulators of the PSR (Saito and Uozumi, 2020), which aligns with observed fluctuations in calcium levels under changing Pi conditions (Matthus et al, 2019).…”

Section: Introductionmentioning

confidence: 99%

Phosphate and phosphite have a differential impact on the proteome and phosphoproteome of Arabidopsis suspension cell cultures

Mehta¹,

Ghahremani²,

Pérez‐Fernández³

et al. 2020

The Plant Journal

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Phosphorus absorbed in the form of phosphate (H 2 PO 4 À) is an essential but limiting macronutrient for plant growth and agricultural productivity. A comprehensive understanding of how plants respond to phosphate starvation is essential for the development of more phosphate-efficient crops. Here we employed label-free proteomics and phosphoproteomics to quantify protein-level responses to 48 h of phosphate versus phosphite (H 2 PO 3 À) resupply to phosphate-deprived Arabidopsis thaliana suspension cells. Phosphite is similarly sensed, taken up and transported by plant cells as phosphate, but cannot be metabolized or used as a nutrient. Phosphite is thus a useful tool for differentiating between non-specific processes related to phosphate sensing and transport and specific responses to phosphorus nutrition. We found that responses to phosphate versus phosphite resupply occurred mainly at the level of protein phosphorylation, complemented by limited changes in protein abundance, primarily in protein translation, phosphate transport and scavenging, and central metabolism proteins. Altered phosphorylation of proteins involved in core processes such as translation, RNA splicing and kinase signaling was especially important. We also found differential phosphorylation in response to phosphate and phosphite in 69 proteins, including splicing factors, translation factors, the PHT1;4 phosphate transporter and the HAT1 histone acetyltransferasepotential phosphoswitches signaling changes in phosphorus nutrition. Our study illuminates several new aspects of the phosphate starvation response and identifies important targets for further investigation and potential crop improvement.

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“…An obvious hypothesis is that AtGAL1 binds AtPAP26‐S2's high‐mannose glycans and that this association modulates the catalytic activity and physico‐chemical properties of AtPAP26‐S2. Indeed, our companion paper (Ghahremani et al, ) documents that (a) AtGAL1 specifically interacts with AtPAP26‐S2 and (b) AtGAL1 preincubation significantly enhances the APase activity and thermal stability of purified AtPAP26‐S2, but not AtPAP26‐S1. AtGAL1 's induction by numerous stresses combined with the broad distribution of AtGAL1‐like lectins in phylogenetically diverse species (Table , Figure S4) implies an important and conserved function for AtGAL1 orthologs within the plant kingdom.…”

Section: Discussionmentioning

confidence: 97%

“…An obvious hypothesis is that AtGAL1 binds AtPAP26-S2's high-mannose glycans and that this association modulates the catalytic activity and physico-chemical properties of AtPAP26-S2. Indeed, our companion paper (Ghahremani et al, 2018) documents that (a) AtGAL1 specifically interacts with AtPAP26-S2 and (b) AtGAL1 preincubation significantly enhances the APase activity and thermal stability of purified AtPAP26-S2, but not AtPAP26-S1.…”

Section: Atgal1 Undergoes Multiple Posttranslational Modificationsmentioning

confidence: 99%

“…AtGAL1 belongs to Arabidopsis ' Galanthus nivalis agglutinin (GNA)‐related and apple domain lectin family, whose GNA domain binds high‐mannose glycans (Van Damme et al, ). Our companion paper reports that AtGAL1 specifically associates with AtPAP26‐S2 and that this interaction significantly enhances the APase activity and thermal stability of AtPAP26‐S2 (Ghahremani et al, ). To our knowledge, the current study provides the first definitive evidence for involvement of secreted glycoforms, lectins, or a phosphotyrosylated protein in plant Pi‐starvation responses, while representing the first purification and characterization of a GNA‐apple domain lectin from any species.…”

Section: Introductionmentioning

confidence: 98%

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

Ghahremani

Tran

Biglou

et al. 2019

Plant Cell & Environment

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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 post-transcriptional 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.

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Lectin AtGAL1 interacts with high‐mannose glycoform of the purple acid phosphatase AtPAP26 secreted by phosphate‐starved Arabidopsis

Cited by 18 publications

References 36 publications

Purple acid phosphatase 10c encodes a major acid phosphatase that regulates plant growth under phosphate-deficient conditions in rice

Purple acid phosphatase 10c encodes a major acid phosphatase that regulates plant growth under phosphate-deficient conditions in rice

Phosphate and phosphite have a differential impact on the proteome and phosphoproteome of Arabidopsis suspension cell cultures

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

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