4.4 Article

Peroxisomal hydroxypyruvate reductase is not essential for photorespiration in Arabidopsis but its absence causes an increase in the stoichiometry of photorespiratory CO2 release

期刊

PHOTOSYNTHESIS RESEARCH
卷 108, 期 2-3, 页码 91-100

出版社

SPRINGER
DOI: 10.1007/s11120-011-9651-3

关键词

Photosynthesis; Photorespiration; Peroxisomes; Hydroxypyruvate reductase

资金

  1. Australian Research Council [FF0457721, CE0561495]
  2. Centres of Excellence of the Government of Western Australia
  3. NSF [0842182, 0923562]
  4. Direct For Biological Sciences
  5. Div Of Biological Infrastructure [0923562] Funding Source: National Science Foundation
  6. Division Of Integrative Organismal Systems
  7. Direct For Biological Sciences [0842182] Funding Source: National Science Foundation

向作者/读者索取更多资源

Recycling of carbon by the photorespiratory pathway involves enzymatic steps in the chloroplast, mitochondria, and peroxisomes. Most of these reactions are essential for plants growing under ambient CO2 concentrations. However, some disruptions of photorespiratory metabolism cause subtle phenotypes in plants grown in air. For example, Arabidopsis thaliana lacking both of the peroxisomal malate dehydrogenase genes (pmdh1pmdh2) or hydroxypyruvate reductase (hpr1) are viable in air and have rates of photosynthesis only slightly lower than wild-type plants. To investigate how disruption of the peroxisomal reduction of hydroxypyruvate to glycerate influences photorespiratory carbon metabolism we analyzed leaf gas exchange in A. thaliana plants lacking peroxisomal HPR1 expression. In addition, because the lack of HPR1 could be compensated for by other reactions within the peroxisomes using reductant supplied by PMDH a triple mutant lacking expression of both peroxisomal PMDH genes and HPR1 (pmdh1pmdh2hpr1) was analyzed. Rates of photosynthesis under photorespiratory conditions (ambient CO2 and O-2 concentrations) were slightly reduced in the hpr1 and pmdh1pmdh2hpr1 plants indicating other reactions can help bypass this disruption in the photorespiratory pathway. However, the CO2 compensation points (Gamma) increased under photorespiratory conditions in both mutants indicating changes in photorespiratory carbon metabolism in these plants. Measurements of Gamma*, the CO2 compensation point in the absence of mitochondrial respiration, and the CO2 released per Rubisco oxygenation reaction demonstrated that the increase in Gamma in the hpr1 and pmdh1pmdh2hpr1 plants is not associated with changes in mitochondrial respiration but with an increase in the non-respiratory CO2 released per Rubisco oxygenation reaction.

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