Expression of stress-responsive ubiquitin genes in potato tubers

Garbarino, Joan E.; Rockhold, David R.; Belknap, William R.

doi:10.1007/bf00014491

Cited by 77 publications

(80 citation statements)

References 26 publications

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“…The possible multi-regulated clones encoded putative cytochrome P450, MADS box transcription factor, Proline-rich protein precursor, seed maturation protein and so on. Together with the results that ethylene-response protein was regulated by ABA (Fig 2, clone Xd439, AJ437339), although the detailed analysis on the regulation by both hormones is still required, these may indicate the complicated interIdentification of ABA-responsive genes in rice [47][48][49]. Although there was no report about the connection of auxin and ubiquitin, but the promoter of GLP3b gene has a single putative auxin-response element, which was physically linked to the polyubiquitin 4 gene [50].…”

Section: Interaction Of Aba With Auxin and Brsmentioning

confidence: 64%

Identification of ABA-responsive genes in rice shoots via cDNA macroarray

Lin

et al. 2003

Cell Res

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Phytohormone abscisic acid (ABA) was critical for many plant growth and developmental processes including seed maturation, germination and response to environmental factors. With the purpose to detect the possible ABA related signal transduction pathways, we tried to isolate ABA-regulated genes through cDNA macroarray technology using ABA-treated rice seedling as materials (under treatment for 2, 4, 8 and 12 h). Of 6144 cDNA clones tested, 37 differential clones showing induction or suppression for at least one time, were isolated. Of them 30 and 7 were up-or down-regulated respectively. Sequence analyses revealed that the putative encoded proteins were involved in different possible processes, including transcription, metabolism and resistance, photosynthesis, signal transduction, and seed maturation. 6 cDNA clones were found to encode proteins with unknown functions. Regulation by ABA of 7 selected clones relating to signal transduction or metabolism was confirmed by reverse transcription PCR. In addition, some clones were further shown to be regulated by other plant growth regulators including auxin and brassinosteroid, which, however, indicated the complicated interactions of plant hormones. Possible signal transduction pathways involved in ABA were discussed.

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Section: Interaction Of Aba With Auxin and Brsmentioning

confidence: 64%

Identification of ABA-responsive genes in rice shoots via cDNA macroarray

Lin

et al. 2003

Cell Res

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“…Polyubiquitin genes have been isolated from different plants (Causing and Barkardottir, 1986;Burke et al, 1988;Christensen and Quail, 1989;Jamet et al, 1990;Genschik et al, 1992;Garbarino et al, 1992;Reynolds and Hooley, 1992), including sunflower (Binet et al, 1989(Binet et al, , 1991. The nucleotide sequences of these genes are highly conserved, mainly in their coding regions and in a characteristic 5' flanking intron (Binet et al, 1991, and refs.…”

Section: Discussionmentioning

confidence: 99%

“…therein). Sequence divergence in their 3' flanking regions (Joshi et al, 1991) and the expression of different sized messengers (Causing and Barkardottir, 1986;Burke et al, 1988;Genschik et al, 1992) have allowed detection of the differential accumulation of polyubiquitin mRNAs, mainly in response to heat shock (Christensen and Quail, 1989;Binet et al, 1991;Christensen et al, 1992;Genschik et al, 1992) and other stress treatments (Garbarino et al, 1992;Genschik et al, 1992) but also during leaf (Causing and Barkardottir, 1986;Burke et al, 1988) or flower (Causing and Barkardottir, 1986;Binet et al, 1989) development and in cell dedifferentiation (Jamet et al, 1990). The finding of multiple, differentially regulated polyubiquitin genes in Arabidopsis and in all plants studied so far has suggested (Burke et al, 1988) that evolutionary divergence of their regulation provides basic, conserved functions (reviewed by Monia et al, 1990;Finley and Chau, 1991;Hershko and Ciechanover, 1992;Jentsch, 1992;Vierstra, 1993) in specific temporal or spatial environments.…”

Section: Discussionmentioning

confidence: 99%

“…This, together with observation of differential regulation of severa1 plant ubiquitin genes, has suggested that their multiplicity and diversity reflect an evolutionary divergence of their gene regulation to cope with different specific tasks, such as functions related to cell proliferation and dedifferentiation (Gausing and Barkardottir, 1986;Jamet et al, 1990;Genschik et al, 1992); stress, light, or hormone responses (Burke et al, 1988;Binet et al, 1991;Hoffman et al, 1991;Garbarino et al, 1992;Genschik et al, 1992;Reynolds and Hooley, 1992); and organ (flower, leaf, etc.) development (Gausing and Barkardottir, 1986;Burke et al, 1988;Hoffman et al, 1991;Garbarino et al, 1992). The differential regulation of tetraubiquitin mRNAs during seed maturation and detection of putative, seed-specific, protein-ubiquitin conjugates reported in this study suggest that distinct ubiquitin genes could perform specific functions during plant zygotic embryogenesis.…”

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confidence: 99%

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Differential Accumulation of Sunflower Tetraubiquitin mRNAs during Zygotic Embryogenesis and Developmental Regulation of Their Heat-Shock Response

Almoguera¹,

Coca²,

Jordano³

1995

Plant Physiol.

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We have isolated and sequenced Ha UbiS, a cDNA for a dryseed-stored mRNA that encodes tetraubiquitin. We have observed differential accumulation of tetraubiquitin mRNAs during sunflower (Helianthus annuus 1.) zygotic embryogenesis. These mRNAs were up-regulated during late embryogenesis and reached higher prevalence in the dry seed, where they were found to be associated mainly with provascular tissue. UbiS mRNA, as confirmed by RNase A protection experiments, accumulated also in response to heat shock, but only in leaves and later during postgerminative development. These novel observations demonstrate expression during seed maturation of specific plant polyubiquitin transcripts and developmental regulation of their heat-shock response. Using ubiquitin antibodies we also detected discrete, seed-specific proteins with distinct temporal expression patterns during zygotic embryogenesis. Some of these patterns were concurrent with UbiS mRNA accumulation in seeds. The most abundant ubiquitin-reacting proteins found in mature seeds were small (16-22 kD) and acidic (isoelectric points of 6.1-7.4). Possible functional implications for UbiS expression elicited from these observations are discussed.

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“…AY566555) flanked by HindIII and SpeI sites was inserted into the corresponding sites of the resulting plasmid, and an expression cassette comprising the Agrobacterium ipt gene preceded by the Ubi-3 promoter (Garbarino and Belknap, 1994) and followed by the Ubi-3 terminator was introduced as a 2.6-kb SacII fragment. The P-DNA vector pSIM108 contains the nptII gene, driven by the Ubi-7 promoter (Garbarino et al, 1992) and followed by the terminator of the yeast (Saccharomyces cerevisiae) alcohol dehydrogenase gene (GenBank accession no. V01292), positioned within the P-DNA region.…”

Section: P-dna Vectorsmentioning

confidence: 99%

Crop Improvement through Modification of the Plant's Own Genome

et al. 2004

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Plant genetic engineering has, until now, relied on the incorporation of foreign DNA into plant genomes. Public concern about the extent to which transgenic crops differ from their traditionally bred counterparts has resulted in molecular strategies and gene choices that limit, but not eliminate, the introduction of foreign DNA. Here, we demonstrate that a plant-derived (P-) DNA fragment can be used to replace the universally employed Agrobacterium transfer (T-) DNA. Marker-free P-DNAs are transferred to plant cell nuclei together with conventional T-DNAs carrying a selectable marker gene. By subsequently linking a positive selection for temporary marker gene expression to a negative selection against marker gene integration, 29% of derived regeneration events contain P-DNA insertions but lack any copies of the T-DNA. Further refinements are accomplished by employing Ω-mutated virD2 and isopentenyl transferase cytokinin genes to impair T-DNA integration and select against backbone integration, respectively. The presented methods are used to produce hundreds of marker-free and backbone-free potato (Solanum tuberosum) plants displaying reduced expression of a tuber-specific polyphenol oxidase gene in potato. The modified plants represent the first example of genetically engineered plants that only contain native DNA

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Expression of stress-responsive ubiquitin genes in potato tubers

Cited by 77 publications

References 26 publications

Identification of ABA-responsive genes in rice shoots via cDNA macroarray

Identification of ABA-responsive genes in rice shoots via cDNA macroarray

Differential Accumulation of Sunflower Tetraubiquitin mRNAs during Zygotic Embryogenesis and Developmental Regulation of Their Heat-Shock Response

Crop Improvement through Modification of the Plant's Own Genome

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