Ferredoxin/thioredoxin system plays an important role in the chloroplastic <scp>NADP</scp> status of Arabidopsis

Hashida, Shin‐nosuke; Miyagi, Atsuko; Nishiyama, Maho; Yoshida, Keisuke; Hisabori, Toru; Kawai‐Yamada, Maki

doi:10.1111/tpj.14000

Cited by 40 publications

(42 citation statements)

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“…De novo synthesis of NADP + in cytosol, chloroplasts, and peroxisomes is carried out by the ATP-dependent NAD kinases: NADK1, NADK2, and NADK3 43 , among which NADK2 in chloroplasts, is a light-dependent enzyme 44 . Illumination of 3week-old plants for 5 min to 1 h gradually increases the NADP + and NADPH pools in the rosette leaves of WT plants but not in a nadk2 mutant, indicating that, under illumination, the synthesis of NADP + from NAD + by NADK2 in the chloroplasts is the major NADP + synthesis pathway.…”

Section: Discussionmentioning

confidence: 99%

“…Illumination of 3week-old plants for 5 min to 1 h gradually increases the NADP + and NADPH pools in the rosette leaves of WT plants but not in a nadk2 mutant, indicating that, under illumination, the synthesis of NADP + from NAD + by NADK2 in the chloroplasts is the major NADP + synthesis pathway. The newly synthesized NADP + is then reduced to NADPH by FNR, and the NADPH/NADP + ratio is maintained at~1 in the first 5 min of illumination, and gradually decreases to~0.7 after 60 min of illumination 44 .…”

Section: Discussionmentioning

confidence: 99%

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In planta study of photosynthesis and photorespiration using NADPH and NADH/NAD+ fluorescent protein sensors

et al. 2020

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The challenge of monitoring in planta dynamic changes of NADP(H) and NAD(H) redox states at the subcellular level is considered a major obstacle in plant bioenergetics studies. Here, we introduced two circularly permuted yellow fluorescent protein sensors, iNAP and SoNar, into Arabidopsis thaliana to monitor the dynamic changes in NADPH and the NADH/ NAD + ratio. In the light, photosynthesis and photorespiration are linked to the redox states of NAD(P)H and NAD(P) pools in several subcellular compartments connected by the malate-OAA shuttles. We show that the photosynthetic increases in stromal NADPH and NADH/ NAD + ratio, but not ATP, disappear when glycine decarboxylation is inhibited. These observations highlight the complex interplay between chloroplasts and mitochondria during photosynthesis and support the suggestions that, under normal conditions, photorespiration supplies a large amount of NADH to mitochondria, exceeding its NADH-dissipating capacity, and the surplus NADH is exported from the mitochondria to the cytosol through the malate-OAA shuttle.

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Section: Discussionmentioning

confidence: 99%

Section: Discussionmentioning

confidence: 99%

In planta study of photosynthesis and photorespiration using NADPH and NADH/NAD+ fluorescent protein sensors

et al. 2020

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“…TRX-f1 and TRX-f2 function in activation of Calvin-Benson-Bassham cycle (CBB) enzymes and γ-subunit of F-ATP synthase [4]. TRX-m1, -m2, -m3 and-m4 are suggested to regulate targets which control the NADPH/NADP ratio [5] which is linked to their ability to efficiently activate the NADPH-dependent malate dehydrogenase [6]. TRX-x, NTRC and TRX-lilium1 (ACHT4a) were identified as reductants of the 2-cysteine peroxiredoxin (2CysPRX) [7][8][9], and TRX-y1 and-y2 as reductant of PRX-Q [10].…”

Section: Introductionmentioning

confidence: 99%

Computational simulation of the reactive oxygen species and redox network in the regulation of chloroplast metabolism

et al. 2020

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Cells contain a thiol redox regulatory network to coordinate metabolic and developmental activities with exogenous and endogenous cues. This network controls the redox state and activity of many target proteins. Electrons are fed into the network from metabolism and reach the target proteins via redox transmitters such as thioredoxin (TRX) and NADPHdependent thioredoxin reductases (NTR). Electrons are drained from the network by reactive oxygen species (ROS) through thiol peroxidases, e.g., peroxiredoxins (PRX). Mathematical modeling promises access to quantitative understanding of the network function and was implemented by using published kinetic parameters combined with fitting to known biochemical data. Two networks were assembled, namely the ferredoxin (FDX), FDX-dependent TRX reductase (FTR), TRX, fructose-1,6-bisphosphatase (FBPase) pathway with 2cysteine PRX/ROS as oxidant, and separately the FDX, FDX-dependent NADP reductase (FNR), NADPH, NTRC-pathway for 2-CysPRX reduction. Combining both modules allowed drawing several important conclusions of network performance. The resting H 2 O 2 concentration was estimated to be about 30 nM in the chloroplast stroma. The electron flow to metabolism exceeds that into thiol regulation of FBPase more than 7000-fold under physiological conditions. The electron flow from NTRC to 2-CysPRX is about 5.32-times more efficient than that from TRX-f1 to 2-CysPRX. Under severe stress (30 μM H 2 O 2) the ratio of electron flow to the thiol network relative to metabolism sinks to 1:251 whereas the ratio of eflow from NTRC to 2-CysPRX and TRX-f1 to 2-CysPRX rises up to 1:67. Thus, the simulation provides clues on experimentally inaccessible parameters and describes the functional state of the chloroplast thiol regulatory network.

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“…TRX-f1 and TRX-f2 function in activation of Calvin-Benson-Cycle (CBC) enzymes and γ-subunit of F-ATP synthase [4]. TRX-m1, -m2, -m3 and -m4 are suggested to regulate targets which control the NADPH/NADP ratio [5] which is linked to their ability to efficiently activate the NADPH-dependent malate dehydrogenase [6]. TRX-x, NTRC and TRX-lilium1(ACHT4a) were identified as reductants of the 2-cysteine peroxiredoxin (2-CysPRX) [7–9], and TRX-y1 and –y2 as reductant of PRX-Q [10].…”

Section: Introductionmentioning

confidence: 99%

Computational simulation of the reactive oxygen species and redox network in the regulation of chloroplast metabolism

Dietz

Gerken

Kakorin

et al. 2019

Preprint

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38Cells contain a thiol redox regulatory network to coordinate metabolic and developmental 39 activities with exogenous and endogenous cues. This network controls the redox state and 40 activity of many target proteins. Electrons are fed into the network from metabolism and reach 41 the target proteins via redox transmitters such as thioredoxin (TRX) and NADPH-dependent 42 thioredoxin reductases (NTR). Electrons are drained from the network by reactive oxygen 43 species (ROS) through thiol peroxidases, e.g., peroxiredoxins (PRX). Mathematical modeling 44 promises access to quantitative understanding of the network function and was implemented for 45 the photosynthesizing chloroplast by using published kinetic parameters combined with fitting to 46 known biochemical data. Two networks were assembled, namely the ferredoxin (FDX), FDX-47 dependent TRX reductase (FTR), TRX, fructose-1,6-bisphosphatase pathway with 2-cysteine 48 PRX/ROS as oxidant, and separately the FDX, FDX-dependent NADP reductase (FNR), 49NADPH, NTRC-pathway for 2-CysPRX reduction. Combining both modules allowed drawing 50 several important conclusions of network performance. The resting H 2 O 2 concentration was 51 estimated to be about 30 nM in the chloroplast stroma. The electron flow to metabolism exceeds 52 that into thiol regulation of FBPase more than 7000-fold under physiological conditions. The 53 electron flow from NTRC to 2-CysPRX is about 5.46-times more efficient than that from TRX-54 f1 to 2-CysPRX. Under severe stress (30 µM H 2 O 2 ) the ratio of electron flow to the thiol 55 network relative to metabolism sinks to 1:251 whereas the ratio of electron flow from NTRC to 56 2-CysPRX and TRX-f1 to 2-CysPRX rises up to 1:80. Thus, the simulation provides clues on 57 experimentally inaccessible parameters and describes the functional state of the chloroplast thiol 58 regulatory network.59 60 Keywords: Calvin-Benson cycle, fructose-1,6-bisphosphatase, peroxiredoxin, reactive 61 oxygen species, redox regulation, thioredoxin 3 62Authors summary 63 The state of the thiol redox regulatory network is a fundamental feature of all cells and 64 determines metabolic and developmental processes. However, only some parameters are 65 quantifiable in experiments. This paper establishes partial mathematical models which enable 66 simulation of electron flows through the regulatory system. This in turn allows for estimating 67 rates and states of components of the network and to tentatively address previously unknown 68 parameters such as the resting hydrogen peroxide levels or the expenditure of reductive power 69 for regulation relative to metabolism. The establishment of such models for simulating the 70 performance and dynamics of the redox regulatory network is of significance not only for 71 photosynthesis but also, e.g., in bacterial and animal cells exposed to environmental stress or 72 pathological disorders. 73 4 74 75 Reduction-oxidation reactions drive life. In aerobic metabolism, electrons from reduced 76 compounds pass on to oxygen t...

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Ferredoxin/thioredoxin system plays an important role in the chloroplastic NADP status of Arabidopsis

Cited by 40 publications

References 67 publications

In planta study of photosynthesis and photorespiration using NADPH and NADH/NAD+ fluorescent protein sensors

In planta study of photosynthesis and photorespiration using NADPH and NADH/NAD+ fluorescent protein sensors

Computational simulation of the reactive oxygen species and redox network in the regulation of chloroplast metabolism

Computational simulation of the reactive oxygen species and redox network in the regulation of chloroplast metabolism

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