pSAT RNA Interference Vectors: A Modular Series for Multiple Gene Down-Regulation in Plants

Dafny-Yelin, Mery; Chung, Sang-Min; Frankman, Ellen L.; Tzfira, Tzvi

doi:10.1104/pp.107.106062

Cited by 48 publications

(29 citation statements)

References 56 publications

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“…Furthermore, it also allowed easy modification and removal of the ATG-containing NcoI site from several pSAT-AFP and pSAT.pro.MCS.ter plasmids, allowing for greater versatility while cloning ATG-containing target genes into these vectors (Chung et al, 2005). Other modifications of the basic pSAT-AFP plasmids (Table I) included the introduction of the pSAT-BiFC family of plasmids, useful for the bimolecular fluorescence complementation assay (Citovsky et al, 2006), the construction of pSAT-red fluorescent protein (RFP), for the N-and C-terminal fusion of RFP (enhanced cyan variant of GFP-enhanced cyan fluorescent protein [ECFP], or the monomeric form of DsRed2; Chung et al, 2005;Citovsky et al, 2006), and the assembly of pSAT-RNAi, a set of vectors useful for the expression of hairpin structures for RNAi in plant cells (Dafny-Yelin et al, 2007). Additional plasmids, specifically designed to facilitate the expression of epitope-tagged proteins in plant cells, have also been constructed (T. Tzfira, unpublished data), as have two sets of plant selection-marker expression cassettes, controlled under two different constitutive promoters (Chung et al, 2005;Tzfira et al, 2005), allowing the user the freedom of choosing the preferred selection marker while assembling a multigene binary vector.…”

Section: The Psat Family Of Plasmidsmentioning

confidence: 99%

Delivery of Multiple Transgenes to Plant Cells

2007

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Section: The Psat Family Of Plasmidsmentioning

confidence: 99%

Delivery of Multiple Transgenes to Plant Cells

2007

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“…Wesley et al (2001) tested a variety of constructs of this type and found that the combination of doublestranded RNA, produced after splicing of the intron separating two identical but oppositely-oriented DNA fragments, was far more effective in gene silencing expression than either sense suppression (''co-suppression'') or traditional antisense constructs. Other groups (Dafny-Yelin et al 2007) have produced similar vector sets that contain RNAi elements, but again, these contain only constitutive promoters. We have built one constitutive RNAi cloning vector (plasmid J16), but otherwise, we focused on production of seed-specific plasmids, that will allow for specific silencing of certain types of genes (such as those involved in lipid metabolism) whose complete silencing throughout the plant may be deleterious.…”

Section: Discussionmentioning

confidence: 98%

“…In the years that followed, the auxillary vectors were improved by inclusion of various promoters and terminators (Chung et al 2005). Synthesis of plasmids containing fusion-compatible genes allowing for study of bimolecular fluorescence complementation (BiFC; Citovsky et al 2006), N-and C-terminalfusion compatible fluorescence proteins, and constitutive RNAi interference elements (Dafny-Yelin et al 2007) followed soon after. Other powerful methods have been described recently.…”

Section: Discussionmentioning

confidence: 99%

Development and analysis of a highly flexible multi-gene expression system for metabolic engineering in Arabidopsis seeds and other plant tissues

et al. 2015

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Production of novel value-added compounds in transgenic crops has become an increasingly viable approach in recent years. However, in many cases, product yield still falls short of the levels necessary for optimal profitability. Determination of the limiting factors is thus of supreme importance for the long-term viability of this approach. A significant challenge to most metabolic engineering projects is the need for strong coordinated co-expression of multiple transgenes. Strong constitutive promoters have been well-characterized during the>30 years since plant transformation techniques were developed. However, organ- or tissue-specific promoters are poorly characterized in many cases. Oilseeds are one such example. Reports spanning at least 20 years have described the use of certain seed-specific promoters to drive expression of individual transgenes. Multi-gene engineering strategies are often hampered by sub-optimal expression levels or improper tissue-specificity of particular promoters, or rely on the use of multiple copies of the same promoter, which can result in DNA instability or transgene silencing. We describe here a flexible system of plasmids that allows for expression of 1-7 genes per binary plasmid, and up to 18 genes altogether after multiple rounds of transformation or sexual crosses. This vector system includes six seed-specific promoters and two constitutive promoters. Effective constitutive and seed-specific RNA interference gene-suppression cloning vectors were also constructed for silencing of endogenous genes. Taken together, this molecular toolkit allows combinatorial cloning for multiple transgene expression in seeds, vegetative organs, or both simultaneously, while also providing the means to coordinately overexpress some genes while silencing others.

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“…Then, dsRNA molecules are processed by a RNase III-like enzyme (dicer) into small interfering RNAs (siRNAs) of 21-23 nucleotides in length. Finally, siRNAs are recruited to the RNA induced silencing complex (RISC), which in turn mediates the cleavage of the target mRNA [2,3]. RNA silencing has been investigated in many plants.…”

Section: Introductionmentioning

confidence: 99%

RNA Silencing Mediated by Direct Repeats in Maize: A Potential Tool for Functional Genomics

Zhu

Zhao

et al. 2008

Mol Biotechnol

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It has been shown in tobacco and Arabidopsis that transgenes with multiple direct repeats induce RNA silencing at high frequency. In this study, we tried to establish a direct repeat-induced RNA silencing system in maize and evaluate whether it can be developed as a high throughput tool for functional genomics. Our results showed that the construct phC4, which carries four direct repeats of a chloramphenicol acetyl-transferase (CAT) gene, was able to induce silencing of itself with high efficiency in maize. Using a transient expression system, we further demonstrated that construct phC3G with a beta-glucuronidase (GUS) gene located downstream of three direct repeats of CAT gene silenced not only itself in maize calli but also an "endogenous" GUS gene, which was stably expressed in maize calli. Most importantly, when constructs with the maize iojap (ij) gene inserted in either sense or antisense orientation into the downstream of four direct repeats of CAT gene were transformed into maize plants, co-suppression of endogenous and transgenic ij genes was detected in majority of transgenic maize plants. Our co-suppression results suggest that with improvements, this new approach has the potential to become an efficient research tool for high throughput functional genomics.

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pSAT RNA Interference Vectors: A Modular Series for Multiple Gene Down-Regulation in Plants

Cited by 48 publications

References 56 publications

Delivery of Multiple Transgenes to Plant Cells

Delivery of Multiple Transgenes to Plant Cells

Development and analysis of a highly flexible multi-gene expression system for metabolic engineering in Arabidopsis seeds and other plant tissues

RNA Silencing Mediated by Direct Repeats in Maize: A Potential Tool for Functional Genomics

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