Protein interactions with DNA elements in variant equine infectious anemia virus enhancers and their impact on transcriptional activity

doi:10.1128/JVI.67.11.6586-6595.1993

. 1993 Nov;67(11):6586-95.

doi: 10.1128/JVI.67.11.6586-6595.1993.

Protein interactions with DNA elements in variant equine infectious anemia virus enhancers and their impact on transcriptional activity

M Carvalho¹, M Kirkland, D Derse

Affiliations

PMID: 8411361
PMCID: PMC238096
DOI: 10.1128/JVI.67.11.6586-6595.1993

Protein interactions with DNA elements in variant equine infectious anemia virus enhancers and their impact on transcriptional activity

M Carvalho et al. J Virol. 1993 Nov.

. 1993 Nov;67(11):6586-95.

doi: 10.1128/JVI.67.11.6586-6595.1993.

Authors

M Carvalho¹, M Kirkland, D Derse

Affiliation

¹ Laboratory of Viral Carcinogenesis, National Cancer Institute, Frederick, Maryland 21702-1201.

PMID: 8411361
PMCID: PMC238096
DOI: 10.1128/JVI.67.11.6586-6595.1993

Abstract

The long terminal repeats (LTRs) from various cloned equine infectious anemia virus (EIAV) proviruses differ significantly, but all contain cis-acting DNA elements identical to MDBP-, PEA2-, AP-1-, and PU.1 (ets)-binding sites. A prototype EIAV LTR would contain one of each of these conserved elements. The LTR variations originate from the insertion of novel sequences between the PEA2 and AP-1 elements in the transcriptional enhancer unit. Viewed in this way, the LTR from provirus clone lambda 12 has an 11-bp insertion containing a PEA2 site and the LTR of the lambda 6 provirus has a 31-bp insertion/duplication containing PEA2, AP-1, and PU.1 sites. Two other LTRs were cloned by amplification of cDNAs from the persistently infected cell line, EIAV-FEA. A third LTR was generated by site-directed mutagenesis of one of the LTRs from EIAV-FEA cells. The latter three had a single base change in the element next to the TATA box that abolished PU.1 binding; however, the variable regions of these LTRs were shown by gel mobility shift assays to contain one or two PU.1 sites. One variable region was shown to have an octamer site overlapping its tandem PU.1 elements. Basal, PMA-activated, and Tat trans-activated transcriptional activities of the LTRs were compared in several different cell lines by transient transfection. The various promoters displayed different relative levels of activity depending on the cell line used and the condition of activation. This natural set of variant promoters may help define how changes in the components of the transcription complex influence transactivation by Tat. The diverse LTRs could endow their respective proviruses with a unique pattern of expression and activation in vivo.

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[1] Am J Pathol. 1971 Feb;62(2):283-94 - PubMed

[2] Am J Pathol. 1971 Feb;62(2):283-94 - PubMed

[3] Oncogene. 1990 May;5(5):663-8 - PubMed

[4] Oncogene. 1990 May;5(5):663-8 - PubMed

[5] Intervirology. 1981;16(4):225-32 - PubMed

[6] Intervirology. 1981;16(4):225-32 - PubMed

[7] Mol Cell Biol. 1982 Sep;2(9):1044-51 - PubMed

[8] Mol Cell Biol. 1982 Sep;2(9):1044-51 - PubMed

[9] Nucleic Acids Res. 1983 Mar 11;11(5):1475-89 - PubMed

[10] Nucleic Acids Res. 1983 Mar 11;11(5):1475-89 - PubMed

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Protein interactions with DNA elements in variant equine infectious anemia virus enhancers and their impact on transcriptional activity

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Protein interactions with DNA elements in variant equine infectious anemia virus enhancers and their impact on transcriptional activity

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