Arabidopsis thaliana aldehyde dehydrogenases ALDH3H1 and ALDH3I1: cysteine mutations, S-nitrosylation and esterase activity
Arabidopsis thaliana aldehyde dehydrogenases ALDH3H1 and ALDH3I1: cysteine mutations, S-nitrosylation and esterase activity
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DissertationPrüfungsdatum
02.09.2015Datum der Veröffentlichung
20.04.2016Erstgutachter
Bartels, DorotheaZweitgutachter
Dörmann, PeterMetadaten
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Inhalt
S-nitrosylation is a posttranslational modification that is known to affect many biochemical processes in plants. In the current study the ability of NO donors to S-nitrosylate aldehyde dehydrogenases ALDH3H1 and ALDH3I1 from A. thaliana was investigated. It was shown that ALDH3H1 is strongly nitrosylated by GSNO than ALDH3I1 showing the differences in nitrosylating capacity between the two enzymes. The experiments proved that oxidative posttranslational modification modulates the dehydrogenase activity in both enzymes in differential ways. It has been demonstrated that the effect of NO donors is related to the physicochemical properties of S-nitrosoglutathione and sodium nitroprusside. The following conclusions were made from this study. (i) Prolonged incubation time and high dose of NO donors (GSNO and SNP) regulate the inactivation and the rate of dehydrogenase activity. (ii) The decrease of dehydrogenase activity during S-nitrosylation of cysteine residues is related to the loss of sulfhydryl groups.
It is also clearly shown that the reducing reagents DTT and GSH have the differential abilities to restore the GSNO and SNP-mediated inhibition of the dehydrogenase activity in both the enzymes. The effect of the reducing agents on dehydrogenase activity was monitored and it was observed that DTT possessed stronger reducing properties than GSH. The concentration of reducing reagents (DTT and GST) regulated the ability to restore the inactivation of the dehydrogenase activity. Additionally, the dual enzyme activity (dehydrogenase and esterase activities) of aldehyde dehydrogenases ALDH3H1 and ALDH3I1 was effectively demonstrated. Further, the effect of GSNO and CuCl2 on the esterase activity was investigated and the results indicated that the reactions of dehydrogenation and hydrolysis are probably catalysed at two separate active sites of the protein. Using the non-direct method for detection of S-nitrosylated aldehyde dehydrogenases it is proved that this application can be successfully used in the case of recombinant, purified enzymes ALDH3H1 and ALDH3I1 as well as for ALDH3H1enzyme S-nitrosylated under in vivo conditions. Altogether it can be concluded that ALDH enzymes used in the current study can undergo nitrosylation and apart from having dehydrogenase activity they also possess esterase activity.
It is also clearly shown that the reducing reagents DTT and GSH have the differential abilities to restore the GSNO and SNP-mediated inhibition of the dehydrogenase activity in both the enzymes. The effect of the reducing agents on dehydrogenase activity was monitored and it was observed that DTT possessed stronger reducing properties than GSH. The concentration of reducing reagents (DTT and GST) regulated the ability to restore the inactivation of the dehydrogenase activity. Additionally, the dual enzyme activity (dehydrogenase and esterase activities) of aldehyde dehydrogenases ALDH3H1 and ALDH3I1 was effectively demonstrated. Further, the effect of GSNO and CuCl2 on the esterase activity was investigated and the results indicated that the reactions of dehydrogenation and hydrolysis are probably catalysed at two separate active sites of the protein. Using the non-direct method for detection of S-nitrosylated aldehyde dehydrogenases it is proved that this application can be successfully used in the case of recombinant, purified enzymes ALDH3H1 and ALDH3I1 as well as for ALDH3H1enzyme S-nitrosylated under in vivo conditions. Altogether it can be concluded that ALDH enzymes used in the current study can undergo nitrosylation and apart from having dehydrogenase activity they also possess esterase activity.
Schlagwörter
aldehyde dehydrogenase, S-nitrosylation, esterase activity, dehydrogenase activity
Klassifikation (DDC)
580 Pflanzen (Botanik)Podgórska, Karolina Anna: Arabidopsis thaliana aldehyde dehydrogenases ALDH3H1 and ALDH3I1: cysteine mutations, S-nitrosylation and esterase activity. - Bonn, 2016. - Dissertation, Rheinische Friedrich-Wilhelms-Universität Bonn.
Online-Ausgabe in bonndoc: https://nbn-resolving.org/urn:nbn:de:hbz:5n-42932
Online-Ausgabe in bonndoc: https://nbn-resolving.org/urn:nbn:de:hbz:5n-42932
@phdthesis{handle:20.500.11811/6724,
urn: https://nbn-resolving.org/urn:nbn:de:hbz:5n-42932,
author = {{Karolina Anna Podgórska}},
title = {Arabidopsis thaliana aldehyde dehydrogenases ALDH3H1 and ALDH3I1: cysteine mutations, S-nitrosylation and esterase activity},
school = {Rheinische Friedrich-Wilhelms-Universität Bonn},
year = 2016,
month = apr,
note = {S-nitrosylation is a posttranslational modification that is known to affect many biochemical processes in plants. In the current study the ability of NO donors to S-nitrosylate aldehyde dehydrogenases ALDH3H1 and ALDH3I1 from A. thaliana was investigated. It was shown that ALDH3H1 is strongly nitrosylated by GSNO than ALDH3I1 showing the differences in nitrosylating capacity between the two enzymes. The experiments proved that oxidative posttranslational modification modulates the dehydrogenase activity in both enzymes in differential ways. It has been demonstrated that the effect of NO donors is related to the physicochemical properties of S-nitrosoglutathione and sodium nitroprusside. The following conclusions were made from this study. (i) Prolonged incubation time and high dose of NO donors (GSNO and SNP) regulate the inactivation and the rate of dehydrogenase activity. (ii) The decrease of dehydrogenase activity during S-nitrosylation of cysteine residues is related to the loss of sulfhydryl groups.
It is also clearly shown that the reducing reagents DTT and GSH have the differential abilities to restore the GSNO and SNP-mediated inhibition of the dehydrogenase activity in both the enzymes. The effect of the reducing agents on dehydrogenase activity was monitored and it was observed that DTT possessed stronger reducing properties than GSH. The concentration of reducing reagents (DTT and GST) regulated the ability to restore the inactivation of the dehydrogenase activity. Additionally, the dual enzyme activity (dehydrogenase and esterase activities) of aldehyde dehydrogenases ALDH3H1 and ALDH3I1 was effectively demonstrated. Further, the effect of GSNO and CuCl2 on the esterase activity was investigated and the results indicated that the reactions of dehydrogenation and hydrolysis are probably catalysed at two separate active sites of the protein. Using the non-direct method for detection of S-nitrosylated aldehyde dehydrogenases it is proved that this application can be successfully used in the case of recombinant, purified enzymes ALDH3H1 and ALDH3I1 as well as for ALDH3H1enzyme S-nitrosylated under in vivo conditions. Altogether it can be concluded that ALDH enzymes used in the current study can undergo nitrosylation and apart from having dehydrogenase activity they also possess esterase activity.},
url = {https://hdl.handle.net/20.500.11811/6724}
}
urn: https://nbn-resolving.org/urn:nbn:de:hbz:5n-42932,
author = {{Karolina Anna Podgórska}},
title = {Arabidopsis thaliana aldehyde dehydrogenases ALDH3H1 and ALDH3I1: cysteine mutations, S-nitrosylation and esterase activity},
school = {Rheinische Friedrich-Wilhelms-Universität Bonn},
year = 2016,
month = apr,
note = {S-nitrosylation is a posttranslational modification that is known to affect many biochemical processes in plants. In the current study the ability of NO donors to S-nitrosylate aldehyde dehydrogenases ALDH3H1 and ALDH3I1 from A. thaliana was investigated. It was shown that ALDH3H1 is strongly nitrosylated by GSNO than ALDH3I1 showing the differences in nitrosylating capacity between the two enzymes. The experiments proved that oxidative posttranslational modification modulates the dehydrogenase activity in both enzymes in differential ways. It has been demonstrated that the effect of NO donors is related to the physicochemical properties of S-nitrosoglutathione and sodium nitroprusside. The following conclusions were made from this study. (i) Prolonged incubation time and high dose of NO donors (GSNO and SNP) regulate the inactivation and the rate of dehydrogenase activity. (ii) The decrease of dehydrogenase activity during S-nitrosylation of cysteine residues is related to the loss of sulfhydryl groups.
It is also clearly shown that the reducing reagents DTT and GSH have the differential abilities to restore the GSNO and SNP-mediated inhibition of the dehydrogenase activity in both the enzymes. The effect of the reducing agents on dehydrogenase activity was monitored and it was observed that DTT possessed stronger reducing properties than GSH. The concentration of reducing reagents (DTT and GST) regulated the ability to restore the inactivation of the dehydrogenase activity. Additionally, the dual enzyme activity (dehydrogenase and esterase activities) of aldehyde dehydrogenases ALDH3H1 and ALDH3I1 was effectively demonstrated. Further, the effect of GSNO and CuCl2 on the esterase activity was investigated and the results indicated that the reactions of dehydrogenation and hydrolysis are probably catalysed at two separate active sites of the protein. Using the non-direct method for detection of S-nitrosylated aldehyde dehydrogenases it is proved that this application can be successfully used in the case of recombinant, purified enzymes ALDH3H1 and ALDH3I1 as well as for ALDH3H1enzyme S-nitrosylated under in vivo conditions. Altogether it can be concluded that ALDH enzymes used in the current study can undergo nitrosylation and apart from having dehydrogenase activity they also possess esterase activity.},
url = {https://hdl.handle.net/20.500.11811/6724}
}
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