| Literature DB >> 26829715 |
Yan Wang1, Wenhui Lyu1, Oliver Berkowitz1, Jordan D Radomiljac1, Simon R Law2, Monika W Murcha3, Chris Carrie4, Pedro F Teixeira5, Beata Kmiec5, Owen Duncan3, Olivier Van Aken3, Reena Narsai1, Elzbieta Glaser5, Shaobai Huang3, Ute Roessner6, A Harvey Millar3, James Whelan7.
Abstract
At12Cys-1 (At5g64400) and At12Cys-2 (At5g09570) are two closely related isogenes that encode small, twin cysteine proteins, typically located in mitochondria. At12Cys-2 transcript is induced in a variety of mutants with disrupted mitochondrial proteins, but an increase in At12Cys protein is only detected in mutants with reduced mitochondrial complex I abundance. Induction of At12Cys protein in mutants that lack mitochondrial complex I is accompanied by At12Cys protein located in mitochondria, chloroplasts, and the cytosol. Biochemical analyses revealed that even single gene deletions, i.e., At12cys-1 or At12cys-2, have an effect on mitochondrial and chloroplast functions. However, only double mutants, i.e., At12cys-1:At12cys-2, affect the abundance of protein and mRNA transcripts encoding translation elongation factors as well as rRNA abundance. Blue native PAGE showed that At12Cys co-migrated with mitochondrial supercomplex I + III. Likewise, deletion of both At12cys-1 and At12cys-2 genes, but not single gene deletions, results in enhanced tolerance to drought and light stress and increased anti-oxidant capacity. The induction and multiple localization of At12Cys upon a reduction in complex I abundance provides a mechanism to specifically signal mitochondrial dysfunction to the cytosol and then beyond to other organelles in the cell.Entities:
Keywords: chloroplast; complex I; cytosol; mitochondria; retrograde signaling
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Year: 2016 PMID: 26829715 DOI: 10.1016/j.molp.2016.01.009
Source DB: PubMed Journal: Mol Plant ISSN: 1674-2052 Impact factor: 13.164