Live imaging of companion cells and sieve elements in Arabidopsis leaves.
The phloem is a complex tissue composed of highly specialized cells with unique subcellular structures and a compact organization that is challenging to study in vivo at cellular resolution. We used confocal scanning laser microscopy and subcellular fluorescent markers in companion cells and sieve e...
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doaj-082128a78fa2427fa4c51c8f5f2459fb2020-11-24T21:12:39ZengPublic Library of Science (PLoS)PLoS ONE1932-62032015-01-01102e011812210.1371/journal.pone.0118122Live imaging of companion cells and sieve elements in Arabidopsis leaves.Thibaud CaylaBrigitte BataillerRozenn Le HirFrédéric ReversJames A AnsteadGary A ThompsonOlivier GrandjeanSylvie DinantThe phloem is a complex tissue composed of highly specialized cells with unique subcellular structures and a compact organization that is challenging to study in vivo at cellular resolution. We used confocal scanning laser microscopy and subcellular fluorescent markers in companion cells and sieve elements, for live imaging of the phloem in Arabidopsis leaves. This approach provided a simple framework for identifying phloem cell types unambiguously. It highlighted the compactness of the meshed network of organelles within companion cells. By contrast, within the sieve elements, unknown bodies were observed in association with the PP2-A1:GFP, GFP:RTM1 and RTM2:GFP markers at the cell periphery. The phloem lectin PP2-A1:GFP marker was found in the parietal ground matrix. Its location differed from that of the P-protein filaments, which were visualized with SEOR1:GFP and SEOR2:GFP. PP2-A1:GFP surrounded two types of bodies, one of which was identified as mitochondria. This location suggested that it was embedded within the sieve element clamps, specific structures that may fix the organelles to each another or to the plasma membrane in the sieve tubes. GFP:RTM1 was associated with a class of larger bodies, potentially corresponding to plastids. PP2-A1:GFP was soluble in the cytosol of immature sieve elements. The changes in its subcellular localization during differentiation provide an in vivo blueprint for monitoring this process. The subcellular features obtained with these companion cell and sieve element markers can be used as landmarks for exploring the organization and dynamics of phloem cells in vivo.http://europepmc.org/articles/PMC4340910?pdf=render |
collection |
DOAJ |
language |
English |
format |
Article |
sources |
DOAJ |
author |
Thibaud Cayla Brigitte Batailler Rozenn Le Hir Frédéric Revers James A Anstead Gary A Thompson Olivier Grandjean Sylvie Dinant |
spellingShingle |
Thibaud Cayla Brigitte Batailler Rozenn Le Hir Frédéric Revers James A Anstead Gary A Thompson Olivier Grandjean Sylvie Dinant Live imaging of companion cells and sieve elements in Arabidopsis leaves. PLoS ONE |
author_facet |
Thibaud Cayla Brigitte Batailler Rozenn Le Hir Frédéric Revers James A Anstead Gary A Thompson Olivier Grandjean Sylvie Dinant |
author_sort |
Thibaud Cayla |
title |
Live imaging of companion cells and sieve elements in Arabidopsis leaves. |
title_short |
Live imaging of companion cells and sieve elements in Arabidopsis leaves. |
title_full |
Live imaging of companion cells and sieve elements in Arabidopsis leaves. |
title_fullStr |
Live imaging of companion cells and sieve elements in Arabidopsis leaves. |
title_full_unstemmed |
Live imaging of companion cells and sieve elements in Arabidopsis leaves. |
title_sort |
live imaging of companion cells and sieve elements in arabidopsis leaves. |
publisher |
Public Library of Science (PLoS) |
series |
PLoS ONE |
issn |
1932-6203 |
publishDate |
2015-01-01 |
description |
The phloem is a complex tissue composed of highly specialized cells with unique subcellular structures and a compact organization that is challenging to study in vivo at cellular resolution. We used confocal scanning laser microscopy and subcellular fluorescent markers in companion cells and sieve elements, for live imaging of the phloem in Arabidopsis leaves. This approach provided a simple framework for identifying phloem cell types unambiguously. It highlighted the compactness of the meshed network of organelles within companion cells. By contrast, within the sieve elements, unknown bodies were observed in association with the PP2-A1:GFP, GFP:RTM1 and RTM2:GFP markers at the cell periphery. The phloem lectin PP2-A1:GFP marker was found in the parietal ground matrix. Its location differed from that of the P-protein filaments, which were visualized with SEOR1:GFP and SEOR2:GFP. PP2-A1:GFP surrounded two types of bodies, one of which was identified as mitochondria. This location suggested that it was embedded within the sieve element clamps, specific structures that may fix the organelles to each another or to the plasma membrane in the sieve tubes. GFP:RTM1 was associated with a class of larger bodies, potentially corresponding to plastids. PP2-A1:GFP was soluble in the cytosol of immature sieve elements. The changes in its subcellular localization during differentiation provide an in vivo blueprint for monitoring this process. The subcellular features obtained with these companion cell and sieve element markers can be used as landmarks for exploring the organization and dynamics of phloem cells in vivo. |
url |
http://europepmc.org/articles/PMC4340910?pdf=render |
work_keys_str_mv |
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