A Direct Transposon Insertion Tool for Modification and Functional Analysis of Viral Genomes

Vilen, Heikki; Aalto, Juha-Matti; Kassinen, Anna; Paulín, Lars; Savilahti, Harri

doi:10.1128/jvi.77.1.123-134.2003

Cited by 35 publications

(28 citation statements)

References 62 publications

(50 reference statements)

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“…However, these methods can produce variable or biased insertions, and library generation efficiencies are often too low to apply to larger genes. Transposon-based insertional mutagenesis has recently emerged as an efficient means of studying the features of viral genomes (1,5,22,25,44). We hypothesized that a transposonbased approach for saturation insertional mutagenesis, coupled with a high-throughput viral-based library selection process, could rapidly identify optimal sites within VSV-G that could functionally incorporate a novel peptide sequence.…”

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confidence: 99%

Selection of Novel Vesicular Stomatitis Virus Glycoprotein Variants from a Peptide Insertion Library for Enhanced Purification of Retroviral and Lentiviral Vectors

Schaffer

2006

J Virol

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The introduction of new features or functions that are not present in an original protein is a significant challenge in protein engineering. For example, modifications to vesicular stomatitis virus glycoprotein (VSV-G), which is commonly used to pseudotype retroviral and lentiviral vectors for gene delivery, have been hindered by a lack of structural knowledge of the protein. We have developed a transposon-based approach that randomly incorporates designed polypeptides throughout a protein to generate saturated insertion libraries and a subsequent high-throughput selection process in mammalian cells that enables the identification of optimal insertion sites for a novel designed functionality. This method was applied to VSV-G in order to construct a comprehensive library of mutants whose combined members have a His 6 tag inserted at likely every site in the original protein sequence. Selecting the library via iterative retroviral infections of mammalian cells led to the identification of several VSV-G-His 6 variants that were able to package high-titer viral vectors and could be purified by Ni-nitrilotriacetic acid affinity chromatography. Column purification of vectors reduced protein and DNA impurities more than 5,000-fold and 14,000-fold, respectively, from the viral supernatant. This substantially improved purity elicited a weaker immune response in the brain, without altering the infectivity or tropism from wild-type VSV-G-pseudotyped vectors. This work applies a powerful new tool for protein engineering to construct novel viral envelope variants that can greatly improve the safety and use of retroviral and lentiviral vectors for clinical gene therapy. Furthermore, this approach of library generation and selection can readily be extended to other challenges in protein engineering.

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confidence: 99%

Selection of Novel Vesicular Stomatitis Virus Glycoprotein Variants from a Peptide Insertion Library for Enhanced Purification of Retroviral and Lentiviral Vectors

Schaffer

2006

J Virol

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“…strain ER72M2 cells were cultured in SB broth or on SB agar plates (33) at 28°C. Escherichia coli K-12 DH5␣ (Life Technologies) was used for transposon preparation as described previously (20,50).…”

Section: Methodsmentioning

confidence: 99%

“…One of the most versatile methods is based on the bacteriophage Mu in vitro DNA transposition reaction, which can be used to disseminate custom-designed mini-Mu transposons into any DNA, including viral genomes. This strategy has been used successfully for the functional characterization of linear dsDNA genomes of bacteriophages PRD1 (50) and YeO3-12 (31). A related strategy employing transposon ends has been applied to human immunodeficiency virus (34) and potato virus A (30) RNA genome characterization.…”

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confidence: 99%

“…Recently, we have initiated a structural characterization of phage PM2 as a model phage system (2,26). Since no genetic tools are available in this system, we set out to probe the PM2 genome using the phage Mu-derived in vitro transposition mutagenesis technology, which represents an efficient alternative strategy for functional genome characterization (50).…”

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confidence: 99%

“…Transposon mutagenesis can be used to map essential versus nonessential regions in viral genomes (8,48,50,54). One of the most versatile methods is based on the bacteriophage Mu in vitro DNA transposition reaction, which can be used to disseminate custom-designed mini-Mu transposons into any DNA, including viral genomes.…”

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confidence: 99%

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Genome Characterization of Lipid-Containing Marine Bacteriophage PM2 by Transposon Insertion Mutagenesis

Krupovìč

Vilen

Bamford

et al. 2006

J Virol

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Bacteriophage PM2 presently is the only member of the Corticoviridae family. The virion consists of a protein-rich lipid vesicle, which is surrounded by an icosahedral protein capsid. The lipid vesicle encloses a supercoiled circular double-stranded DNA genome of 10,079 bp. PM2 belongs to the marine phage community and is known to infect two gram-negative Pseudoalteromonas species. In this study, we present a characterization of the PM2 genome made using the in vitro transposon insertion mutagenesis approach. Analysis of 101 insertion mutants yielded information on the essential and dispensable regions of the PM2 genome and led to the identification of several new genes. A number of lysis-deficient mutants as well as mutants displaying delayed-and/or incomplete-lysis phenotypes were identified. This enabled us to identify novel lysis-associated genes with no resemblance to those previously described from other bacteriophage systems. Nonessential genome regions are discussed in the context of PM2 genome evolution.

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Current awareness on comparative and functional genomics

2003

Comp Funct Genom

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In order to keep subscribers up‐to‐date with the latest developments in their field, this current awareness service is provided by John Wiley & Sons and contains newly‐published material on comparative and functional genomics. Each bibliography is divided into 16 sections. 1 Reviews & symposia; 2 General; 3 Large‐scale sequencing and mapping; 4 Genome evolution; 5 Comparative genomics; 6 Gene families and regulons; 7 Pharmacogenomics; 8 Large‐scale mutagenesis programmes; 9 Functional complementation; 10 Transcriptomics; 11 Proteomics; 12 Protein structural genomics; 13 Metabolomics; 14 Genomic approaches to development; 15 Technological advances; 16 Bioinformatics. Within each section, articles are listed in alphabetical order with respect to author. If, in the preceding period, no publications are located relevant to any one of these headings, that section will be omitted

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A Direct Transposon Insertion Tool for Modification and Functional Analysis of Viral Genomes

Cited by 35 publications

References 62 publications

Selection of Novel Vesicular Stomatitis Virus Glycoprotein Variants from a Peptide Insertion Library for Enhanced Purification of Retroviral and Lentiviral Vectors

Selection of Novel Vesicular Stomatitis Virus Glycoprotein Variants from a Peptide Insertion Library for Enhanced Purification of Retroviral and Lentiviral Vectors

Genome Characterization of Lipid-Containing Marine Bacteriophage PM2 by Transposon Insertion Mutagenesis

Current awareness on comparative and functional genomics

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