Sequences required for coordinate induction of adeno-associated virus p19 and p40 promoters by Rep protein

McCarty, Doug; Christensen, Merrill J.; Muzyczka, Nicholas

doi:10.1128/jvi.65.6.2936-2945.1991

Cited by 97 publications

(114 citation statements)

References 55 publications

(42 reference statements)

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“…A possible explanation for the decrease in Cap expression is that the amount of Rep78/68 may not be sufficient to enhance the Cap expression, because Rep78/68 is required to transactivate both the p19 and p40 promoters in the presence of adenovirus. 25) Since Rep78/68 is also required to replicate the vector DNA, the AAV vector yields may be reduced when the levels of Rep78/68 expression are very low. Thus, for AAV vector production it is important to express appropriate amounts of Rep78/68.…”

Section: Discussionmentioning

confidence: 99%

“…1, pIM45 contains the wild-type rep and cap genes at nt 145 to 4493 in a Bluescript M13+ vector. 25) To construct the Rep expression plasmid (pRep), a polylinker containing recognition sites for the enzymes 5′-SacI-ClaI-EcoRI-SmaI-BamHI-XbaI-HincII-PstI-EcoRV-HindIII-XhoI-KpnI-3′ was cloned into the BssHII site of pUC-MCS, 8) and then the following fragments were cloned into the plasmid; an AAV fragment containing the rep gene (nt 145-2252 in the AAV genome) into SpeI-PstI and the 135-bp HpaI-BamHI blunt-end modified SV40 early polyadenylation signal from pCMV-β plasmid (CLONETECH Laboratories, Palo Alto, CA) into the HpaI site. The Rep78/68 expression plasmid (pR78/68) was derived from pRep with a mutation of the first ATG of Rep52/40 to GGA as described previously.…”

Section: Cell Line and Plasmidsmentioning

confidence: 99%

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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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Section: Discussionmentioning

confidence: 99%

Section: Cell Line and Plasmidsmentioning

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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“…Plasmids. The pCMVRep78 construct was made by inserting the XbaI fragment of pIM29 (31), containing the genomic DNA and promoters of AAV but lacking the 145-bp terminal repeats (TRs), 45 bp immediately 3 0 of the left TR, and 42 bp immediately 5 0 of the right TR, into the XbaI site of pRc/CMV (Invitrogen), which contains the human cytomegalovirus immediate-early promoter (hCMV IEP).…”

Section: Methodsmentioning

confidence: 99%

Adeno‐Associated Virus Rep78 Binds to E2‐Responsive Element 1 of Bovine Papillomavirus Type 1

Chon

Rim

1999

IUBMB Life

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Adeno-associated virus type-2 (AAV-2) is a helper-dependent parvovirus that has been implicated in the inhibition of replication and oncogenic transformation of bovine papillomavirus type-1 (BPV-1) and other transforming DNA viruses. Previous studies have suggested that the Rep78 protein of AAV-2 is a key player mediating this effect. In this report we have analyzed the effect of AAV-2 Rep78 protein on the regulation of gene expression of a reporter gene under the control of the long control region (LCR) of BPV-1. Our results show that Rep78 is capable of down-regulating the promoter activity of the LCR in vivo in tissue culture cells. Inhibition of LCR activity in vivo suggested the need for Rep78 to bind to a region of the LCR promoter spanning the E2-responsive elements of BPV-1. This observation was further confirmed in vitro with gel shift assays showing specific binding of Rep78 to DNA oligonucleotides containing E2-responsive element 1 (E2RE1) sequences of BPV-1 LCR. Our results expand the understanding of the mechanism of trans-regulation mediated by Rep78 and involving this protein and DNA sequences with complex secondary structure.

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“…In the absence of a helper virus, Rep78/68 repress both p5 and p19 transcription (18). In the presence of a helper virus, the AAV promoters, particularly p5, are transactivated by the adenovirus ElA and host YY1 proteins, and Rep78/68 positively regulate the p19 and p40 promoters (19,21,28). Transcription from p19 promoter generates spliced and unspliced tran-*Address correspondence to Dr .…”

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.…”

mentioning

confidence: 99%

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.

show abstract

Sequences required for coordinate induction of adeno-associated virus p19 and p40 promoters by Rep protein

Cited by 97 publications

References 55 publications

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

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

Adeno‐Associated Virus Rep78 Binds to E2‐Responsive Element 1 of Bovine Papillomavirus Type 1

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

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