Genetic analysis of adeno-associated virus: properties of deletion mutants constructed in vitro and evidence for an adeno-associated virus replication function

Tratschin, Jon-Duri; Miller, I L; Carter, B J

doi:10.1128/jvi.51.3.611-619.1984

Cited by 252 publications

(184 citation statements)

References 47 publications

(65 reference statements)

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“…Analysis of the factors which affect AAV vector production will provide insights into the development of more efficient rAAV production systems. Since Rep78/68, whose expression is driven from the p5 promoter, are the only AAV gene products required for replication and regulate both p19 and p40 promoters (21,28,34), we constructed various AAV helper plasmids in which the p5 promoter was replaced with heterologous promoters (EF, CMV, SV40, B l9p6 and CAG) to modulate the expression of AAV proteins, and examined the relation between the expression patterns of AAV proteins and the efficiency of rAAVLacZ production using these helper plasmids.…”

Section: Discussionmentioning

confidence: 99%

“…The AAV rep gene is transcribed from p5 and p19 promoters, and the AAV cap gene is transcribed from p40 promoter. Transcription from p5 promoter generates spliced and unspliced transcripts which encode Rep68 and Rep78, respectively (34). Rep78/68 are required to regulate transcription from all three promoters and to replicate the viral DNA (9,34).…”

mentioning

confidence: 99%

“…Transcription from p5 promoter generates spliced and unspliced transcripts which encode Rep68 and Rep78, respectively (34). Rep78/68 are required to regulate transcription from all three promoters and to replicate the viral DNA (9,34). In the absence of a helper virus, Rep78/68 repress both p5 and p19 transcription (18).…”

mentioning

confidence: 99%

“…Since Rep78/68 proteins are required for replication from an AAV origin within the ITR and transactivate both p19 and p40 promoters during productive infection in the presence of adenovirus (21,28,34), a change in the expression level of Rep78/68 would affect the expression of other AAV proteins and thereby alter the efficiency of AAV vector production. In this study, we constructed various helper plasmids in which p5 promoter was replaced with heterologous promoters [human polypeptide chain elongation factor 1-oc (EF) (24), cytomegalovirus immediate-early (CMV-LE) (36), simian virus 40 early (SV40), B19 parvovirus p6 (B 19p6) (27) and chicken P-actin promoter plus cytomegalovirus enhancer (CAG) (25) promoters] to examine the effect of different amounts of Rep78/68 on the expression of Rep52/40 and Cap, rAAV DNA replication and the efficiency of AAV vector production.…”

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confidence: 99%

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The Use of Heterologous Promoters for Adeno‐Associated Virus (AAV) Protein Expression in AAV Vector Production

Ogasawara

Urabe

Ozawa

1998

Microbiology and Immunology

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Although adeno-associated virus (AAV) vectors are potentially useful gene transfer vehicles for gene therapy, the vector production system is currently at the developmental stage. We constructed AAV helper plasmids (Rep and Cap expression plasmids) by replacing a native AAV promoter, p5, with various heterologous promoters to examine whether the efficiency of AAV vector production was influenced by modulating the AAV protein expression pattern. The helper plasmids containing heterologous promoters (EF, CMV, SV40, B19p6, and CAG promoters, respectively) expressed Rep78/68 more efficiently than a conventional helper plasmid (pIM45), but the expression of Rep52/40 and Cap decreased, resulting in a significant reduction in AAV vector production. Furthermore, the efficiency of vector production never fully recovered even if the Cap proteins were supplied by an additional expression plasmid. A large amount of Rep78/68 and/or a reduced level of Rep52/40 may have deleterious effects on AAV vector production. The present findings will aid in the development of a more efficient AAV vector production system.

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Section: Discussionmentioning

confidence: 99%

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confidence: 99%

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confidence: 99%

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confidence: 99%

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The Use of Heterologous Promoters for Adeno‐Associated Virus (AAV) Protein Expression in AAV Vector Production

Ogasawara

Urabe

Ozawa

1998

Microbiology and Immunology

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“…Rep78/68 are required to regulate transcription from all three promoters and to replicate the viral DNA. 10,11) Furthermore, Rep78/68 are also involved in the preferential integration of AAV genomes into the AAVS1 locus. 12) Spliced and unspliced transcripts from the p19 promoter encode Rep40 and Rep52, respectively.…”

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confidence: 99%

Efficient Production of Adeno‐associated Virus Vectors Using Split‐type Helper Plasmids

Ogasawara

Urabe

Kogure

et al. 1999

Japanese Journal of Cancer Research

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Adeno-associated virus (AAV) vectors are potentially useful vehicles for the delivery of therapeutic genes into human cells. To determine the optimal expression pattern of AAV proteins (Rep78, Rep68, Rep52, Rep40, and Cap proteins) for packaging the recombinant AAV genome, helper plasmids were split into two portions. In this study, two sets of split-type helper plasmids were prepared; i.e., 1) a Rep expression plasmid (pRep) and Cap expression plasmid (pCap), and 2) a large Rep expression plasmid (pR78/68) and small Rep plus Cap expression plasmid (pR52/ 40Cap). When AAV vectors were produced using these sets of split-type helper plasmids at various ratios, the optimal ratio of (large) Rep expression plasmid and Cap expression plasmid was 1 to 9 for both sets. More importantly, the titers were comparable to or even higher than that of a conventional helper plasmid (pIM45) (4.9 ± ± ± ±2.1× × × ×10 11 vector particles/10 cm dish for pRep and pCap; 2.9 ± ± ± ±1.6× × × ×10 11 vector particles/10 cm dish for pR78/68 and pR52/40Cap; and 1.8 ± ± ± ±0.16× × × ×10 11 particles/10 cm dish for pIM45). Western analysis of AAV proteins suggests that the expression of a relatively small amount of large Rep and a large amount of Cap is important for optimal vector production. The present study shows that the AAV helper plasmid can be split without losing the ability to package the recombinant AAV genome, and provides us with valuable basic information for the development of efficient AAV packaging cell lines.

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Molecular epidemiology of adenovirus type 7 in Israel: Identification of two new genome types, Ad7k and Ad7d2

Azar

Varsano

Mileguir

et al. 1998

Journal of Medical Virology

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The molecular epidemiology of Adenovirus type 7 in Israel was investigated. Fifty-seven adenovirus isolates identified as serotypes 7 or 7a which were recovered from patients in Israel between 1968 and 1995 were analyzed by restriction enzymes digestion using BamHI for primary discrimination and identification of genome types and by six additional enzymes: BstEII, HpaI, BglI, BglII, BclI, and XbaI for confirmation and determination of genomic subtypes. Four digestion patterns were identified with BamHI; one of them was new. Using BstEII, two patterns were obtained, one of them new. Digestion with the other five enzymes yielded known patterns. The analysis revealed four different genomic types and subtypes, which circulated in Israel in different years: subtype 7a1; type 7b, a type with a new BamHI pattern which was designated type 7K, and a subtype with a new BstEII pattern which differed from type 7d by one restriction site and was designated type 7d2. Twenty-two isolates from 1968 through 1975 and from 1984 were Ad7a1. Three isolates from 1973-1974 were Ad7b. Five isolates from 1968 through 1973 were Ad7K and 27 isolates from 1992 through 1995 were Ad7d2. This demonstrates the temporal change in the circulating genome types with up to three genome types cocirculating in 1 year (1973). The two new types, Ad7k and Ad7d2 could have evolved in Israel or could have been imported by travellers and immigrants from neighboring or distant countries.

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Genetic analysis of adeno-associated virus: properties of deletion mutants constructed in vitro and evidence for an adeno-associated virus replication function

Cited by 252 publications

References 47 publications

The Use of Heterologous Promoters for Adeno‐Associated Virus (AAV) Protein Expression in AAV Vector Production

The Use of Heterologous Promoters for Adeno‐Associated Virus (AAV) Protein Expression in AAV Vector Production

Efficient Production of Adeno‐associated Virus Vectors Using Split‐type Helper Plasmids

Molecular epidemiology of adenovirus type 7 in Israel: Identification of two new genome types, Ad7k and Ad7d2

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