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| DC Field | Value | Language |
|---|---|---|
| dc.creator | Loscos Aranda, Jorge | - |
| dc.creator | Naya, Loreto | - |
| dc.creator | Ramos Escribano, Javier | - |
| dc.creator | Clemente, María Rebeca | - |
| dc.creator | Matamoros Galindo, Manuel Ángel | - |
| dc.creator | Becana Ausejo, Manuel | - |
| dc.date | 2008-04-29T09:00:05Z | - |
| dc.date | 2008-04-29T09:00:05Z | - |
| dc.date | 2006-02 | - |
| dc.date.accessioned | 2017-01-31T01:06:49Z | - |
| dc.date.available | 2017-01-31T01:06:49Z | - |
| dc.identifier | Plant Physiology 140(4): 1213–1221 (2006) | - |
| dc.identifier | 0032-0889 | - |
| dc.identifier | http://hdl.handle.net/10261/3874 | - |
| dc.identifier | 10.1104/pp.105.073635 | - |
| dc.identifier.uri | http://dspace.mediu.edu.my:8181/xmlui/handle/10261/3874 | - |
| dc.description | 9 páginas. | - |
| dc.description | Phytochelatin synthases (PCS) catalyze phytochelatin (PC) synthesis from glutathione (GSH) in the presence of certain metals. The resulting PC-metal complexes are transported into the vacuole, avoiding toxic effects on metabolism. Legumes have the unique capacity to partially or completely replace GSH by homoglutathione (hGSH) and PCs by homophytochelatins (hPCs). However, the synthesis of hPCs has received little attention. A search for PCS genes in the model legume Lotus (Lotus japonicus) resulted in the isolation of a cDNA clone encoding a protein (LjPCS1) highly homologous to a previously reported homophytochelatin synthase (hPCS) of Glycine max (GmhPCS1). Recombinant LjPCS1 and Arabidopsis (Arabidopsis thaliana) PCS1 (AtPCS1) were affinity purified and their polyhistidine-tags removed. AtPCS1 catalyzed hPC synthesis from hGSH alone at even higher rates than did LjPCS1, indicating that GmhPCS1 is not a genuine hPCS and that a low ratio of hPC to PC synthesis is an inherent feature of PCS1 enzymes. For both enzymes, hGSH is a good acceptor, but a poor donor, of {gamma}-glutamylcysteine units. Purified AtPCS1 and LjPCS1 were activated (in decreasing order) by Cd2+, Zn2+, Cu2+, and Fe3+, but not by Co2+ or Ni2+, in the presence of 5 mM GSH and 50 µM metal ions. Activation of both enzymes by Fe3+ was proven by the complete inhibition of PC synthesis by the iron-specific chelator desferrioxamine. Plants of Arabidopsis and Lotus accumulated (h)PCs only in response to a large excess of Cu2+ and Zn2+, but to a much lower extent than did with Cd2+, indicating that (h)PC synthesis does not significantly contribute in vivo to copper, zinc, and iron detoxification. | - |
| dc.description | This work was supported by the Ministerio de Educación y Ciencia-Fondos Europeos de Desarrollo Regional (grant nos. AGL2002–2876 and AGL2005–1404) and by Gobierno de Aragón-Fondo Social Europeo (group E33) | - |
| dc.description | Peer reviewed | - |
| dc.format | 24753 bytes | - |
| dc.format | application/pdf | - |
| dc.language | eng | - |
| dc.publisher | American Society of Plant Biologists | - |
| dc.relation | http://dx.doi.org/10.1104/pp.105.073635 | - |
| dc.rights | closedAccess | - |
| dc.title | A Reassessment of Substrate Specificity and Activation of Phytochelatin Synthases from Model Plants by Physiologically Relevant Metals | - |
| dc.type | Artículo | - |
| Appears in Collections: | Digital Csic | |
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