Assessing Protein Synthesis and Degradation Rates in <i>Arabidopsis thaliana</i> Using Amino Acid Analysis

Ishihara, Hirofumi; Moraes, Thiago Alexandre; Arrivault, Stéphanie; Stitt, Mark

doi:10.1002/cpz1.114

Cited by 2 publications

(3 citation statements)

References 44 publications

(76 reference statements)

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“…When combined with hydroponic cultivation, dual labeling with 13 CO 2 and 15 N (in the form of 15 NH 4 NO 3 , 15 NH 4 15 NO 3 or K 15 NO 3 in nutrient solution) enables simultaneous tracking of C and N allocation [ 41 ]. While 15 N feeding was successfully applied to unveil leaf proteome turnover [ 2 , 3 ], attempts are being made with 13 CO 2 to concomitantly analyze turnover of metabolites and proteins [ 42 , 43 ]. Chambers for long-term 13 CO 2 labeling typically have a large volume to treat multiple plants in parallel [ 41 – 44 ].…”

Section: Discussionmentioning

confidence: 99%

Combination of long-term 13CO2 labeling and isotopolog profiling allows turnover analysis of photosynthetic pigments in Arabidopsis leaves

et al. 2022

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Background Living cells maintain and adjust structural and functional integrity by continual synthesis and degradation of metabolites and macromolecules. The maintenance and adjustment of thylakoid membrane involve turnover of photosynthetic pigments along with subunits of protein complexes. Quantifying their turnover is essential to understand the mechanisms of homeostasis and long-term acclimation of photosynthetic apparatus. Here we report methods combining whole-plant long-term 13CO2 labeling and liquid chromatography - mass spectrometry (LC–MS) analysis to determine the size of non-labeled population (NLP) of carotenoids and chlorophylls (Chl) in leaf pigment extracts of partially 13C-labeled plants. Results The labeling chamber enabled parallel 13CO2 labeling of up to 15 plants of Arabidopsis thaliana with real-time environmental monitoring ([CO2], light intensity, temperature, relative air humidity and pressure) and recording. No significant difference in growth or photosynthetic pigment composition was found in leaves after 7-d exposure to normal CO2 (~ 400 ppm) or 13CO2 in the labeling chamber, or in ambient air outside the labeling chamber (control). Following chromatographic separation of the pigments and mass peak assignment by high-resolution Fourier-transform ion cyclotron resonance MS, mass spectra of photosynthetic pigments were analyzed by triple quadrupole MS to calculate NLP. The size of NLP remaining after the 7-d 13CO2 labeling was ~ 10.3% and ~ 11.5% for all-trans- and 9-cis-β-carotene, ~ 21.9% for lutein, ~ 18.8% for Chl a and 33.6% for Chl b, highlighting non-uniform turnover of these pigments in thylakoids. Comparable results were obtained in all replicate plants of the 13CO2 labeling experiment except for three that were showing anthocyanin accumulation and growth impairment due to insufficient water supply (leading to stomatal closure and less 13C incorporation). Conclusions Our methods allow 13CO2 labeling and estimation of NLP for photosynthetic pigments with high reproducibility despite potential variations in [13CO2] between the experiments. The results indicate distinct turnover rates of carotenoids and Chls in thylakoid membrane, which can be investigated in the future by time course experiments. Since 13C enrichment can be measured in a range of compounds, long-term 13CO2 labeling chamber, in combination with appropriate MS methods, facilitates turnover analysis of various metabolites and macromolecules in plants on a time scale of hours to days.

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Section: Discussionmentioning

confidence: 99%

Combination of long-term 13CO2 labeling and isotopolog profiling allows turnover analysis of photosynthetic pigments in Arabidopsis leaves

et al. 2022

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“…Translation is related mainly to protein biosynthesis and approaches to study translational dynamics typically involve the use of stable isotope mass spectrometry as an empirical measure of protein synthesis (K 𝑠 ) and degradation (K 𝑑 ) (Nelson et al, 2014b,a). The calculation of plant protein K 𝑠 using a stable isotope pulse depends on several parameters that must be considered (Ishihara et al, 2015(Ishihara et al, , 2021Li et al, 2017). The amount of protein fraction that has taken up the externally supplied stable isotope tracer can be determined by isotopolog analysis of proteinogenic amino acids from isolated and hydrolyzed protein fractions or individual purified proteins.…”

Section: Introductionmentioning

confidence: 99%

“…The first two variables are protein content and relative growth rate (RGR), which are required to adjust K S rates between plant systems that differ in these characteristics. A third set of variables describes the dynamics of tracer incorporation into soluble amino acid pools, and label incorporation into these pools may differ between the physiological conditions being compared and between individual proteinogenic amino acids ( Ishihara et al, 2021 ). All of these variables are necessary to correct the isotopic envelopes of proteins or digested peptides based on knowledge of their individual amino acid sequences.…”

Section: Introductionmentioning

confidence: 99%

Remodelled Ribosomes Synthesise a Specific Proteome in Proliferating Plant Tissue during Cold

Martinez‐Seidel

Suwanchaikasem

Gentry-Torfer

et al. 2022

Preprint

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Plant acclimation to low temperatures occurs through system-wide mechanisms that include proteome shifts, some of which occur at the level of protein synthesis. All proteins are synthesised by ribosomes. Rather than being monolithic, transcript-to-protein translation machines, ribosomes can be selective and cause effective proteome shifts required for successful temperature acclimation. Here, we use apical root meristems of germinating seedlings of the monocotyledonous plant barley as a model to study changes in protein abundance and synthesis rates during cold acclimation. We measure metabolic and physiological parameters that allow us to compare protein synthesis rates in different physiological states, e.g., in cold acclimation compared to the optimal temperature state. We show that ribosomal proteins are independently synthesised and assembled into ribosomal complexes in root proliferative tissue, and assess how the ribo-proteome shifts during cold may be associated with changes in synthesis and accumulation of macromolecular complexes. We demonstrate that translation initiation is the limiting step during cold acclimation and based on our data propose a model of a ribosomal code that depends on a reconfigured ribosome population, where as a mode of cold acclimation, specific ribosomal protein compositions may confer selective association capabilities between 60S subunits and 48S initiation complexes.

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Assessing Protein Synthesis and Degradation Rates in Arabidopsis thaliana Using Amino Acid Analysis

Cited by 2 publications

References 44 publications

Combination of long-term 13CO2 labeling and isotopolog profiling allows turnover analysis of photosynthetic pigments in Arabidopsis leaves

Combination of long-term 13CO2 labeling and isotopolog profiling allows turnover analysis of photosynthetic pigments in Arabidopsis leaves

Remodelled Ribosomes Synthesise a Specific Proteome in Proliferating Plant Tissue during Cold

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