Publikation: Analysis of sublethal arsenic toxicity to Ceratophyllum demersum : subcellular distribution of arsenic and inhibition of chlorophyll biosynthesis
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Arsenic (As) pollution is a serious concern worldwide. Recent studies under environmentally relevant conditions revealed that, in the aquatic plant Ceratophyllum demersum, pigments are the first observable target of toxicity, prior to any effect on photosynthetic parameters or to oxidative stress. Lethal toxicity was initiated by a change of As species and their distribution pattern in various tissues. Here, the localization of As was investigated at the subcellular level through X-ray fluorescence using a submicron beam and a Maia detector. Further, it was possible to obtain useful tissue structural information from the ratio of the tomogram of photon flux behind the sample to the tomogram of Compton scattering. The micro-X-ray fluorescence tomograms showed that As predominantly accumulated in the nucleus of the epidermal cells in young mature leaves exposed to sublethal 1 µM As. This suggests that As may exert toxic effects in the nucleus, for example, by interfering with nucleic acid synthesis by replacing phosphorous with As. At higher cellular concentrations, As was mainly stored in the vacuole, particularly in mature leaves. An analysis of precursors of chlorophyll and degradation metabolites revealed that the observed decrease in chlorophyll concentration was associated with hindered biosynthesis, and was not due to degradation. Coproporphyrinogen III could not be detected after exposure to only 0.5 µM As. Levels of subsequent precursors, for example, protoporphyrin IX, Mg-protoporphyrin, Mg-protoporphyrin methyl ester, and divinyl protochlorophyllide, were significantly decreased at this concentration as well, indicating that the pathway was blocked upstream of tetrapyrrole synthesis.
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MISHRA, Seema, Matthias ALFELD, Roman SOBOTKA, Elisa ANDRESEN, Gerald FALKENBERG, Hendrik KÜPPER, 2016. Analysis of sublethal arsenic toxicity to Ceratophyllum demersum : subcellular distribution of arsenic and inhibition of chlorophyll biosynthesis. In: Journal of Experimental Botany. 2016, 67(15), pp. 4639-4646. ISSN 0022-0957. eISSN 1460-2431. Available under: doi: 10.1093/jxb/erw238BibTex
@article{Mishra2016-08-04Analy-35415,
year={2016},
doi={10.1093/jxb/erw238},
title={Analysis of sublethal arsenic toxicity to Ceratophyllum demersum : subcellular distribution of arsenic and inhibition of chlorophyll biosynthesis},
number={15},
volume={67},
issn={0022-0957},
journal={Journal of Experimental Botany},
pages={4639--4646},
author={Mishra, Seema and Alfeld, Matthias and Sobotka, Roman and Andresen, Elisa and Falkenberg, Gerald and Küpper, Hendrik}
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<dcterms:abstract xml:lang="eng">Arsenic (As) pollution is a serious concern worldwide. Recent studies under environmentally relevant conditions revealed that, in the aquatic plant Ceratophyllum demersum, pigments are the first observable target of toxicity, prior to any effect on photosynthetic parameters or to oxidative stress. Lethal toxicity was initiated by a change of As species and their distribution pattern in various tissues. Here, the localization of As was investigated at the subcellular level through X-ray fluorescence using a submicron beam and a Maia detector. Further, it was possible to obtain useful tissue structural information from the ratio of the tomogram of photon flux behind the sample to the tomogram of Compton scattering. The micro-X-ray fluorescence tomograms showed that As predominantly accumulated in the nucleus of the epidermal cells in young mature leaves exposed to sublethal 1 µM As. This suggests that As may exert toxic effects in the nucleus, for example, by interfering with nucleic acid synthesis by replacing phosphorous with As. At higher cellular concentrations, As was mainly stored in the vacuole, particularly in mature leaves. An analysis of precursors of chlorophyll and degradation metabolites revealed that the observed decrease in chlorophyll concentration was associated with hindered biosynthesis, and was not due to degradation. Coproporphyrinogen III could not be detected after exposure to only 0.5 µM As. Levels of subsequent precursors, for example, protoporphyrin IX, Mg-protoporphyrin, Mg-protoporphyrin methyl ester, and divinyl protochlorophyllide, were significantly decreased at this concentration as well, indicating that the pathway was blocked upstream of tetrapyrrole synthesis.</dcterms:abstract>
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