Autophagic degradation of the chloroplastic 2-phosphoglycolate phosphatase TaPGLP1 in wheat

Jiayao Ni; Yuru Li; Yue Xiang; Xiangyun Yang; Lei Jia; Jieyu Yue; Huazhong Wang

doi:10.1007/s00299-021-02820-3

Autophagic degradation of the chloroplastic 2-phosphoglycolate phosphatase TaPGLP1 in wheat

Plant Cell Rep. 2022 Feb;41(2):473-487. doi: 10.1007/s00299-021-02820-3. Epub 2022 Jan 4.

Authors

Jiayao Ni¹, Yuru Li¹, Yue Xiang¹, Xiangyun Yang¹, Lei Jia¹, Jieyu Yue¹, Huazhong Wang²

Affiliations

¹ College of Life Sciences, Tianjin Key Laboratory of Animal and Plant Resistance, Tianjin Normal University, 393#, BinShuiXi Road, Xiqing, Tianjin, 300387, China.
² College of Life Sciences, Tianjin Key Laboratory of Animal and Plant Resistance, Tianjin Normal University, 393#, BinShuiXi Road, Xiqing, Tianjin, 300387, China. skywhz@tjnu.edu.cn.

PMID: 34981152
DOI: 10.1007/s00299-021-02820-3

Abstract

TaPGLP1, a chloroplast stromal 2-phosphoglycolate phosphatase of wheat, is an ATG8-interacting protein and undergoes autophagic degradation in starvation-treated wheat mesophyll protoplasts. Selective autophagy in plants has been shown to target diverse cellular cargoes including whole chloroplasts (Chlorophagy) and several chloroplast components (Piecemeal chlorophagy). Most cargoes of selective autophagy are captured by the autophagic machinery through their direct or indirect interactions with the autophagy-essential factor ATG8. Here, we reported a new ATG8-interacting cargo of piecemeal chlorophagy, the wheat photorespiratory 2-phosphoglycolate phosphatase TaPGLP1. The TaPGLP1-mCherry fusions expressed in wheat protoplasts located in the chloroplast stroma. Strikingly, these fusions are translocated into newly formed chloroplast surface protrusions after a long time incubation of protoplasts in a nutrition-free solution. Visualization of co-expressed TaPGLP1-mCherry and the autophagy marker GFP-TaATG8a revealed physical associations of TaPGLP1-mCherry-accumulating chloroplast protrusions with autophagic structures, implying the delivery of TaPGLP1-mCherry fusions from chloroplasts to the autophagic machinery. TaPGLP1-mCherry fusions were also detected in the GFP-TaATG8a-labelled autophagic bodies undergoing degradation in the vacuoles, which suggested the autophagic degradation of TaPGLP1. This autophagic degradation of TaPGLP1 was further demonstrated by the enhanced stability of TaPGLP1-mCherry in protoplasts with impaired autophagy. Expression of TaPGLP1-mCherry in protoplasts stimulated an enhanced autophagy level probably adopted by cells to degrade the over-produced TaPGLP1-mCherry fusions. Results from gene silencing assays showed the requirement of ATG2s and ATG7s in the autophagic degradation of TaPGLP1. Additionally, TaPGLP1 was shown to interact with ATG8 family members. Collectively, our data suggest that autophagy mediates the degradation of the chloroplast stromal protein TaPGLP1 in starvation-treated mesophyll protoplasts.

Keywords: 2-Phosphoglycolate phosphatase (PGLP); Autophagy; Chloroplast; Wheat (Triticum aestivum L.).

MeSH terms

Autophagy / physiology*
Autophagy-Related Proteins / genetics
Autophagy-Related Proteins / metabolism
Chloroplasts / metabolism*
Luminescent Proteins / genetics
Luminescent Proteins / metabolism
Mesophyll Cells / metabolism
Phosphoric Monoester Hydrolases / genetics
Phosphoric Monoester Hydrolases / metabolism*
Plant Proteins / genetics
Plant Proteins / metabolism*
Plants, Genetically Modified
Protein Transport
Red Fluorescent Protein
Triticum / cytology
Triticum / genetics
Triticum / metabolism*

Substances

Autophagy-Related Proteins
Luminescent Proteins
Plant Proteins
phosphoglycolate phosphatase
Phosphoric Monoester Hydrolases

Abstract

MeSH terms

Substances

Grants and funding