Characterization of the peroxiredoxin 1 subfamily from Tetrahymena thermophila.

Al-Asadi, S; Malik, A; Bakiu, R; Santovito, G; Menz, I; Schuller, K

Characterization of the peroxiredoxin 1 subfamily from Tetrahymena thermophila.

Al-Asadi, S Malik, A Bakiu, R Santovito, G Menz, I Schuller, K

Permalink

Publisher:: Springer Science and Business Media LLC
Publication Type:: Journal Article
Citation:: Cell Mol Life Sci, 2019, 76, (23), pp. 4745-4768
Issue Date:: 2019-12

Closed Access

	Filename	Description	Size
	s00018-019-03131-3.pdf	Published version	3.85 MB		View/Open

Copyright Clearance Process

Recently Added
In Progress
Closed Access

This item is closed access and not available.

Full metadata record

Field	Value	Language
dc.contributor.author	Al-Asadi, S
dc.contributor.author	Malik, A
dc.contributor.author	Bakiu, R
dc.contributor.author	Santovito, G
dc.contributor.author	Menz, I
dc.contributor.author	Schuller, K
dc.date.accessioned	2022-10-30T02:23:01Z
dc.date.available	2019-05-02
dc.date.available	2022-10-30T02:23:01Z
dc.date.issued	2019-12
dc.identifier.citation	Cell Mol Life Sci, 2019, 76, (23), pp. 4745-4768
dc.identifier.issn	1420-682X
dc.identifier.issn	1420-9071
dc.identifier.uri	http://hdl.handle.net/10453/162900
dc.description.abstract	Peroxiredoxins are antioxidant enzymes that use redox active Cys residues to reduce H2O2 and various organic hydroperoxides to less reactive products, and thereby protect cells against oxidative stress. In yeasts and mammals, the Prx1 proteins are sensitive to hyperoxidation and consequent loss of their peroxidase activity whereas in most bacteria they are not. In this paper we report the characterization of the Prx1 family in the non-parasitic protist Tetrahymena thermophila. In this organism, four genes potentially encoding Prx1 have been identified. In particular, we show that the mitochondrial Prx1 protein (Prx1m) from T. thermophila is relatively robust to hyperoxidation. This is surprising given that T. thermophila is a eukaryote like yeasts and mammals. In addition, the proliferation of the T. thermophila cells was relatively robust to inhibition by H2O2, cumene hydroperoxide and plant natural products that are known to promote the production of H2O2. In the presence of these agents, the abundance of the T. thermophila Prx1m protein was shown to increase. This suggested that the Prx1m protein may be protecting the cells against oxidative stress. There was no evidence for any increase in Prx1m gene expression in the stressed cells. Thus, increasing protein stability rather than increasing gene expression may explain the increasing Prx1m protein abundance we observed.
dc.format	Print-Electronic
dc.language	eng
dc.publisher	Springer Science and Business Media LLC
dc.relation.ispartof	Cell Mol Life Sci
dc.relation.isbasedon	10.1007/s00018-019-03131-3
dc.rights	info:eu-repo/semantics/closedAccess
dc.subject	0601 Biochemistry and Cell Biology, 0606 Physiology, 1103 Clinical Sciences
dc.subject.classification	Biochemistry & Molecular Biology
dc.subject.mesh	Amino Acid Motifs
dc.subject.mesh	Amino Acid Sequence
dc.subject.mesh	Antioxidants
dc.subject.mesh	Benzene Derivatives
dc.subject.mesh	Biological Products
dc.subject.mesh	Gene Expression Regulation
dc.subject.mesh	Humans
dc.subject.mesh	Hydrogen Peroxide
dc.subject.mesh	Oxidative Stress
dc.subject.mesh	Peroxiredoxins
dc.subject.mesh	Phylogeny
dc.subject.mesh	Protozoan Proteins
dc.subject.mesh	Sequence Alignment
dc.subject.mesh	Tetrahymena thermophila
dc.subject.mesh	Humans
dc.subject.mesh	Tetrahymena thermophila
dc.subject.mesh	Hydrogen Peroxide
dc.subject.mesh	Benzene Derivatives
dc.subject.mesh	Protozoan Proteins
dc.subject.mesh	Biological Products
dc.subject.mesh	Antioxidants
dc.subject.mesh	Sequence Alignment
dc.subject.mesh	Phylogeny
dc.subject.mesh	Gene Expression Regulation
dc.subject.mesh	Amino Acid Sequence
dc.subject.mesh	Amino Acid Motifs
dc.subject.mesh	Oxidative Stress
dc.subject.mesh	Peroxiredoxins
dc.title	Characterization of the peroxiredoxin 1 subfamily from Tetrahymena thermophila.
dc.type	Journal Article
utslib.citation.volume	76
utslib.location.activity	Switzerland
utslib.for	0601 Biochemistry and Cell Biology
utslib.for	0606 Physiology
utslib.for	1103 Clinical Sciences
pubs.organisational-group	/University of Technology Sydney
pubs.organisational-group	/University of Technology Sydney/Faculty of Science
pubs.organisational-group	/University of Technology Sydney/Faculty of Science/School of Life Sciences
utslib.copyright.status	closed_access	*
dc.date.updated	2022-10-30T02:22:47Z
pubs.issue	23
pubs.publication-status	Published
pubs.volume	76
utslib.citation.issue	23

Abstract:

Peroxiredoxins are antioxidant enzymes that use redox active Cys residues to reduce H2O2 and various organic hydroperoxides to less reactive products, and thereby protect cells against oxidative stress. In yeasts and mammals, the Prx1 proteins are sensitive to hyperoxidation and consequent loss of their peroxidase activity whereas in most bacteria they are not. In this paper we report the characterization of the Prx1 family in the non-parasitic protist Tetrahymena thermophila. In this organism, four genes potentially encoding Prx1 have been identified. In particular, we show that the mitochondrial Prx1 protein (Prx1m) from T. thermophila is relatively robust to hyperoxidation. This is surprising given that T. thermophila is a eukaryote like yeasts and mammals. In addition, the proliferation of the T. thermophila cells was relatively robust to inhibition by H2O2, cumene hydroperoxide and plant natural products that are known to promote the production of H2O2. In the presence of these agents, the abundance of the T. thermophila Prx1m protein was shown to increase. This suggested that the Prx1m protein may be protecting the cells against oxidative stress. There was no evidence for any increase in Prx1m gene expression in the stressed cells. Thus, increasing protein stability rather than increasing gene expression may explain the increasing Prx1m protein abundance we observed.

Please use this identifier to cite or link to this item:

http://hdl.handle.net/10453/162900