Concerted Assembly and Cloning of Multiple DNA Segments Using In Vitro Site-Specific Recombination: Functional Analysis of Multi-Segment Expression Clones

Cheo, David L.; Titus, Steven A.; Byrd, Devon R.; Hartley, James L.; Temple, Gary F.; Brasch, Michael A.

doi:10.1101/gr.2512204

Cited by 124 publications

(104 citation statements)

References 39 publications

Supporting

Mentioning

103

Contrasting

Unclassified

Order By: Relevance

“…[8][9][10][11][12] Construction of multiple functional DNA elements in tandem on a single plasmid was performed by stepwise LR and BP reactions as indicated in Figure 1b. All functional elements required for Tet regulation were placed on one contiguous DNA fragment of 12 340 bp between att1 and att2 Gateway recombination signals.…”

Section: Resultsmentioning

confidence: 99%

A versatile nonviral vector system for tetracycline-dependent one-step conditional induction of transgene expression

et al. 2009

View full text Add to dashboard Cite

In this study, we describe a novel self-contained, nonviral vector system for the rapid development of tetracycline (Tet)-inducible transgene expression systems in mammalian cell lines. To avoid multiple rounds of clonal selection for the establishment of stably transfected cell clones, as is necessary with conventional systems, we constructed a multicomplementary DNA(cDNA) expression vector that enables both one-step targeted genomic integration and conditional induction of transgene expression. This vector system consists of several modules including a Tet-inducible promoter directing the expression of a transgene and two Tet repressor expression units placed in tandem on a single vector. The cell clones, generated using a one-step fC31 integrase-mediated chromosomal integration of the multi-cDNA expression construct, showed a stable and robust expression with high induction rates upon addition of doxycycline inducer in five different cell lines tested. By using this system, we show c-Src-induced cell transformation and anticancer cell therapy for this transformation in cultured fibroblast cells. The results show a rapid production and accumulation of target protein on addition of the inducer starting from extremely low background levels and reduction to background levels in a matter of days after the inducer was withdrawn from the culture medium.

show abstract

Section: Resultsmentioning

confidence: 99%

A versatile nonviral vector system for tetracycline-dependent one-step conditional induction of transgene expression

et al. 2009

View full text Add to dashboard Cite

show abstract

“…This promoter drives strong expression in somites and heart (Mohun et al, 1986;Ryffel et al, 2003). To facilitate the transference of putative insulator sequences to the reporter vector, we introduced a Gateway entry site between the promoter and the enhancer (Hartley et al, 2000;Cheo et al, 2004;Fig. 2).…”

Section: Implementation Of Insulator Sequences To Minimize Position Ementioning

confidence: 99%

“…First, to drive the expression of the reporter gene encoding the enhanced green fluorescent protein (EGFP), we have used a gata2a minimal promoter (Ellingsen et al, 2005), which has been selected from a test set of several TATA-containing and TATA-less promoters because of its high efficiency of enhancer activity detection. Second, we have placed a Gateway entry site 5Ј of the gata2a minimal promoter to facilitate the insertion of candidate enhancers in the reporter construct (Hartley et al, 2000;Cheo et al, 2004). Third, the enhancer reporter cassette in ZED is flanked by insulator sequences that we show decrease position effects, thereby increasing the specificity of the signal.…”

Section: Introductionmentioning

confidence: 98%

Zebrafish enhancer detection (ZED) vector: A new tool to facilitate transgenesis and the functional analysis of cis‐regulatory regions in zebrafish

Bessa

Tena

Calle‐Mustienes

et al. 2009

Developmental Dynamics

150

207

View full text Add to dashboard Cite

The identification and characterization of the regulatory activity of genomic sequences is crucial for understanding how the information contained in genomes is translated into cellular function. The cisregulatory sequences control when, where, and how much genes are transcribed and can activate (enhancers) or repress (silencers) gene expression. Here, we describe a novel Tol2 transposon-based vector for assessing enhancer activity in the zebrafish (Danio rerio). This Zebrafish Enhancer Detector (ZED) vector harbors several key improvements, among them a sensitive and specific minimal promoter chosen for optimal enhancer activity detection, insulator sequences to shield the minimal promoter from position effects, and a positive control for transgenesis. Additionally, we demonstrate that highly conserved noncoding sequences homologous between humans and zebrafish largely with enhancer activity largely retain their tissue-specific enhancer activity during vertebrate evolution. More strikingly, insulator sequences from mouse and chicken, but not conserved in zebrafish, maintain their insulator capacity when tested in this model.

show abstract

“…Only a handful of dedicated vector assembly systems have been developed in the past several years for the assembly of multigene transformation vectors (Cheo et al, 2004;Sasaki et al, 2004;Karimi et al, 2005;Chen et al, 2006Chen et al, , 2010Wakasa et al, 2006). Most of these vector assembly systems have a rather limited capacity and hence have been utilized for the delivery of only a small number (i.e.…”

mentioning

confidence: 99%

“…The system was used to construct several multitransgene binary vectors and led to the production of transgenic plants with eight transgenes (Chen et al, 2010). A number of other recombination-based cloning strategies have also been developed for the construction of multigene plant transformation vectors (Cheo et al, 2004;Sasaki et al, 2004;Karimi et al, 2005;Chen et al, 2006Chen et al, , 2010Wakasa et al, 2006). However, here too, the irreversible nature of the recombination-based reactions does not enable the modification of existing binary vectors, and users of such systems may be required to completely rebuild their transformation vectors to give different gene combinations.…”

mentioning

confidence: 99%

Zinc Finger Nuclease and Homing Endonuclease-Mediated Assembly of Multigene Plant Transformation Vectors

Zeevi¹,

Liang²,

Arieli³

et al. 2011

Plant Physiol.

View full text Add to dashboard Cite

Binary vectors are an indispensable component of modern Agrobacterium tumefaciens-mediated plant genetic transformation systems. A remarkable variety of binary plasmids have been developed to support the cloning and transfer of foreign genes into plant cells. The majority of these systems, however, are limited to the cloning and transfer of just a single gene of interest. Thus, plant biologists and biotechnologists face a major obstacle when planning the introduction of multigene traits into transgenic plants. Here, we describe the assembly of multitransgene binary vectors by using a combination of engineered zinc finger nucleases (ZFNs) and homing endonucleases. Our system is composed of a modified binary vector that has been engineered to carry an array of unique recognition sites for ZFNs and homing endonucleases and a family of modular satellite vectors. By combining the use of designed ZFNs and commercial restriction enzymes, multiple plant expression cassettes were sequentially cloned into the acceptor binary vector. Using this system, we produced binary vectors that carried up to nine genes. Arabidopsis (Arabidopsis thaliana) protoplasts and plants were transiently and stably transformed, respectively, by several multigene constructs, and the expression of the transformed genes was monitored across several generations. Because ZFNs can potentially be engineered to digest a wide variety of target sequences, our system allows overcoming the problem of the very limited number of commercial homing endonucleases. Thus, users of our system can enjoy a rich resource of plasmids that can be easily adapted to their various needs, and since our cloning system is based on ZFN and homing endonucleases, it may be possible to reconstruct other types of binary vectors and adapt our vectors for cloning on multigene vector systems in various binary plasmids.

show abstract

Concerted Assembly and Cloning of Multiple DNA Segments Using In Vitro Site-Specific Recombination: Functional Analysis of Multi-Segment Expression Clones

Cited by 124 publications

References 39 publications

A versatile nonviral vector system for tetracycline-dependent one-step conditional induction of transgene expression

A versatile nonviral vector system for tetracycline-dependent one-step conditional induction of transgene expression

Zebrafish enhancer detection (ZED) vector: A new tool to facilitate transgenesis and the functional analysis of cis‐regulatory regions in zebrafish

Zinc Finger Nuclease and Homing Endonuclease-Mediated Assembly of Multigene Plant Transformation Vectors

Contact Info

Product

Resources

About