Your search keyword '"Gaynor, R. B."' showing total 13 results

1. Differential transcriptional activation by human T-cell leukemia virus type 1 Tax mutants is mediated by distinct interactions with CREB binding protein and p300.

Author

Bex F, Yin MJ, Burny A, and Gaynor RB

Subjects

Activating Transcription Factor 1, Animals, Binding Sites, CREB-Binding Protein, Cell Line, Cell Nucleus metabolism, Cell Transformation, Viral, Cricetinae, Cyclic AMP Response Element Modulator, DNA-Binding Proteins metabolism, Gene Products, tax genetics, Human T-lymphotropic virus 1 genetics, Humans, Mutation, NF-kappa B metabolism, Transcription Factor RelA, Transcription, Genetic, Tumor Cells, Cultured, Gene Expression Regulation, Viral, Gene Products, tax metabolism, Human T-lymphotropic virus 1 physiology, Nuclear Proteins metabolism, Repressor Proteins, Trans-Activators, Transcription Factors metabolism, Transcriptional Activation

Abstract

The human T-cell leukemia virus type 1 Tax protein transforms human T lymphocytes, which can lead to the development of adult T-cell leukemia. Tax transformation is related to its ability to activate gene expression via the ATF/CREB and the NF-kappaB pathways. Transcriptional activation of these pathways is mediated by the actions of the related coactivators CREB binding protein (CBP) and p300. In this study, immunocytochemistry and confocal microscopy were used to localize CBP and p300 in cells expressing wild-type Tax or Tax mutants that are able to selectively activate gene expression from either the NF-kappaB or ATF/CREB pathway. Wild-type Tax colocalized with both CBP and p300 in nuclear bodies which also contained ATF-1 and the RelA subunit of NF-kappaB. However, a Tax mutant that selectively activates gene expression from only the ATF/CREB pathway colocalized with CBP but not p300, while a Tax mutant that selectively activates gene expression from only the NF-kappaB pathway colocalized with p300 but not CBP. In vitro and in vivo protein interaction studies indicated that the integrity of two independent domains of Tax delineated by these mutants was involved in the direct interaction of Tax with either CBP or p300. These studies are consistent with a model in which activation of either the NF-kappaB or the ATF/CREB pathway by specific Tax mutants is mediated by distinct interactions with related coactivator proteins.

Published

1998

2. Role of the human homolog of the yeast transcription factor SPT5 in HIV-1 Tat-activation.

Author

Wu-Baer F, Lane WS, and Gaynor RB

Subjects

Amino Acid Sequence, Chromatography, Ion Exchange, DNA, Complementary, Electrophoresis, Polyacrylamide Gel, HeLa Cells, Herpes Simplex Virus Protein Vmw65 metabolism, Humans, Molecular Sequence Data, Open Reading Frames, Transcription Factors chemistry, Transcription Factors isolation & purification, tat Gene Products, Human Immunodeficiency Virus, Chromosomal Proteins, Non-Histone, Fungal Proteins metabolism, Gene Products, tat metabolism, HIV-1 metabolism, Nuclear Proteins metabolism, Saccharomyces cerevisiae metabolism, Trans-Activators metabolism, Transcription Factors metabolism, Transcriptional Elongation Factors

Abstract

The transactivator protein Tat stimulates transcriptional elongation from the HIV-1 LTR. One mechanism by which Tat increases HIV-1 transcription is by interacting with RNA polymerase II and TFIIH to increase phosphorylation of the polymerase C-terminal domain. Recent studies indicate that specific elongation factors may also be required to modulate Tat function. Here, we used biochemical analysis and in vitro transcription assays to identify cellular factors required for Tat activation. This analysis resulted in the purification of a cellular factor Tat-CT1 which is a human homolog of the yeast transcription factor SPT5. Immunodepletion of Tat-CTl from HeLa extract demonstrated that this factor was involved in transcriptional activation by Tat. However, the absence of this factor from HeLa extract did not prevent transcriptional activation by VP16. These findings are consistent with a model in which Tat-mediated effects on transcriptional elongation are mediated in part by the action of the human homolog of the yeast transcription factor SPT5., (Copyright 1998 Academic Press Limited.)

Published

1998

3. Purification of a Tat-associated kinase reveals a TFIIH complex that modulates HIV-1 transcription.

Author

García-Martínez LF, Mavankal G, Neveu JM, Lane WS, Ivanov D, and Gaynor RB

Subjects

Dichlororibofuranosylbenzimidazole pharmacology, Gene Expression Regulation, Viral, Neoplasm Proteins metabolism, Nucleic Acid Synthesis Inhibitors pharmacology, Phosphorylation, Positive Transcriptional Elongation Factor B, Protein Binding, Protein Serine-Threonine Kinases isolation & purification, Sequence Analysis, Transcription Factor TFIIH, Transcription Factors isolation & purification, tat Gene Products, Human Immunodeficiency Virus, Cyclin-Dependent Kinase-Activating Kinase, Cyclin-Dependent Kinases, Gene Products, tat metabolism, HIV-1 genetics, Protein Serine-Threonine Kinases metabolism, RNA Polymerase II metabolism, Transcription Factors metabolism, Transcription Factors, TFII, Transcription, Genetic

Abstract

The Tat protein is a transcriptional activator which is required for efficient human immunodeficiency virus 1 (HIV-1) gene expression Tat stimulates HIV-1 transcriptional elongation by increasing the processivity of RNA polymerase II. To address whether Tat-mediated effects on HIV-1 gene expression are due to modulation in the phosphorylation of the RNA polymerase II C-terminal domain (CTD), we developed a purification protocol to identify cellular kinases that are capable of binding to Tat and hyperphosphorylating the RNA polymerase II CTD. A 600 kDa protein complex with these properties was isolated, and specific components were identified using peptide microsequence analysis. This analysis indicated that proteins comprising the multi-subunit TFIIH complex, in addition to several novel factors, were associated with Tat using both in vitro and in vivo analysis. The Tat-associated kinase bound to the activation domain of Tat, and its ability to hyperphosphorylate RNA polymerase II was markedly stimulated by Tat. Furthermore, the addition of the Tat-associated kinase to in vitro transcription assays stimulated the ability of Tat to activate HIV-1 transcription. These results define a cellular kinase complex whose activity is modulated by Tat to result in activation of HIV-1 trancription.

Published

1997

4. Constitutive binding of the transcription factor interleukin-2 (IL-2) enhancer binding factor to the IL-2 promoter.

Author

Nirula A, Moore DJ, and Gaynor RB

Subjects

Binding Sites, DNA metabolism, DNA-Binding Proteins metabolism, Gene Expression, Humans, Interleukin-2 metabolism, Jurkat Cells, Molecular Sequence Data, NFATC Transcription Factors, Protein Binding, Enhancer Elements, Genetic, Interleukin-2 genetics, Nuclear Proteins, Promoter Regions, Genetic, Transcription Factors metabolism

Abstract

A positive regulatory element in the interleukin-2 (IL-2) promoter, designated the antigen receptor response element-2, is essential for the induction of IL-2 gene expression upon the binding of an inducible multiprotein complex of proteins known as nuclear factor of activated T cells. In the current study, we demonstrated that the winged-helix transcription factor IL-2 enhancer binding factor (ILF) is constitutively expressed in both resting and activated Jurkat cells and binds to two adjacent sequence motifs immediately downstream of the binding site for NFAT. One of these elements has a high degree of homology with consensus binding sites for a variety of winged-helix DNA binding proteins, and the second site functions to modulate ILF binding. Mutagenesis of each of the two sequence elements required for ILF binding decreased IL-2 promoter activity when assayed in transfection assays. Although ILF bound constitutively to the IL-2 promoter, it was not detected as a component of the NFAT complex. These results suggest that important regulatory sequences in the IL-2 promoter are bound by ILF and that this binding may be involved in the control of IL-2 gene expression.

Published

1997

5. Expression patterns of immediate early transcription factors in human non-small cell lung cancer. The Lung Cancer Study Group.

Author

Levin WJ, Press MF, Gaynor RB, Sukhatme VP, Boone TC, Reissmann PT, Figlin RA, Holmes EC, Souza LM, and Slamon DJ

Subjects

Base Sequence, Carcinoma, Non-Small-Cell Lung metabolism, DNA-Binding Proteins genetics, Early Growth Response Protein 1, Genes, fos, Genes, jun, Humans, Immunohistochemistry, Lung Neoplasms metabolism, Molecular Sequence Data, Oligodeoxyribonucleotides, RNA, Messenger genetics, Carcinoma, Non-Small-Cell Lung genetics, Genes, Immediate-Early, Immediate-Early Proteins, Lung Neoplasms genetics, Transcription Factors genetics

Abstract

In 1995, there will be 172,000 new cases of lung cancer diagnosed and 153,000 deaths from this disease in the United States. While the pathogenesis of the disease process is poorly understood, a growing body of evidence suggests that abnormalities in cellular regulatory genes may play an important role in the induction, maintenance and/or progression of some tumor types. These genes include both growth promoting oncogenes as well as growth inhibitory or suppressor genes. Included among these genetic sequences are several cellular transcription factors. A group of these factors including c-jun, c-fos and EGR1 are members of a class of genes known as immediate early genes whose expression are inducible by a variety of stimuli including mitogenic and differentiation inducing growth factors, indicating a potential important role for these genes in normal growth processes. Since these genes are involved in early regulation of cellular growth properties and at least two (c-jun and c-fos) can act as oncogenes, we wished to determine whether their expression levels were altered in human non-small cell lung cancers (NSCLC) compared to normal lung tissue. To address this, Northern blot analyses were performed using c-fos, c-jun and EGR1 probes on RNA extracted from 101 NSCLC tumor specimens and adjacent uninvolved lung tissue. Analysis of this cohort revealed that 72% of the normal tissues demonstrate significantly greater expression of these transcription factors as compared to adjacent malignant tissue. Moreover, this expression pattern appeared to be coordinate for all three genes in the majority of cases. This differential expression pattern was confirmed at the protein level using an immunohistochemical approach with antibodies directed against the c-jun, c-fos and EGR1 gene products. Southern blot analyses demonstrated no gross alterations of these sequences at the DNA level, indicating that the observed differential expression pattern was not due to gross structural changes in the genes. These data suggest that down-regulation of these genes may be involved in the pathogenesis of lung cancer.

Published

1995

6. Protein domains involved in both in vivo and in vitro interactions between human T-cell leukemia virus type I tax and CREB.

Author

Yin MJ, Paulssen EJ, Seeler JS, and Gaynor RB

Subjects

Base Sequence, Basic-Leucine Zipper Transcription Factors, Cell Line, DNA Primers, DNA-Binding Proteins metabolism, G-Box Binding Factors, Humans, Leucine Zippers, Molecular Sequence Data, Protein Binding, Regulatory Sequences, Nucleic Acid, Repetitive Sequences, Nucleic Acid, Cyclic AMP Response Element-Binding Protein metabolism, Gene Products, tax metabolism, Human T-lymphotropic virus 1 metabolism, Transcription Factors

Abstract

Gene expression from the human T-cell leukemia virus type I (HTLV-I) long terminal repeat (LTR) is mediated by three cis-acting regulatory elements known as 21-bp repeats and the transactivator protein Tax. The 21-bp repeats can be subdivided into three motifs known as A, B, and C, each of which is important for maximal gene expression in response to Tax. The B motif contains nucleotide sequences known as a cyclic AMP response element (CRE) or tax-response element which binds members of the ATF/CREB family of transcription factors. Though mutations of this element in the HTLV-I LTR eliminate tax activation, Tax will not activate most other promoters containing these CRE sites. In this study, we investigated the mechanism by which Tax activates gene expression in conjunction with members of the ATF/CREB family. We found that Tax enhanced the binding of one member of the ATF/CREB family, CREB 1, to each of the three HTLV-I LTR 21-bp repeats but not another member designated CRE-BP1 or CREB2. Tax enhanced the binding of CREB1 to nonpalindromic CRE binding sites such as those found in the HTLV-I LTR, but Tax did not enhance the binding of CREB1 to palindromic CRE binding sites such as found in the somatostatin promoter. This finding may help explain the failure of Tax to activate promoters containing consensus CRE sites. These studies were extended by use of the mammalian two-hybrid system. Tax was demonstrated to interact directly with CREB1 but not with other bZIP proteins, including CREB2 and Jun. Site-directed mutagenesis of both Tax and CREB1 demonstrated that the amino terminus of Tax and both the basic and the leucine zipper regions of CREB1 were required for direct interactions between these proteins both in vivo and in vitro. This interaction occurred in vivo and thus did not require the presence of the HTLV-I 21-bp repeats, as previously suggested. These results define the domains required for interaction between Tax and CREB that are likely critical for the activation of HTLV-I gene expression.

Published

1995

7. Regulatory elements involved in tax-mediated transactivation of the HTLV-I LTR.

Author

Seeler JS, Muchardt C, Podar M, and Gaynor RB

Subjects

Base Sequence, Cell Line, Chloramphenicol O-Acetyltransferase biosynthesis, Chloramphenicol O-Acetyltransferase genetics, DNA Mutational Analysis, DNA-Binding Proteins genetics, DNA-Binding Proteins metabolism, Gene Expression Regulation, Viral, Lymphocytes, Molecular Sequence Data, Proto-Oncogene Protein c-ets-1, Proto-Oncogene Proteins genetics, Proto-Oncogene Proteins metabolism, Proto-Oncogene Proteins c-ets, Recombinant Proteins biosynthesis, TATA Box, Transfection, Gene Products, tax genetics, Human T-lymphotropic virus 1 genetics, Regulatory Sequences, Nucleic Acid genetics, Repetitive Sequences, Nucleic Acid genetics, Transcription Factors, Transcriptional Activation

Abstract

HTLV-I is the etiologic agent of adult T-cell leukemia. In this study, we investigated the regulatory elements and cellular transcription factors which function in modulating HTLV-I gene expression in response to the viral transactivator protein, tax. Transfection experiments into Jurkat cells of a variety of site-directed mutants in the HTLV-1 LTR indicated that each of the three motifs A, B, and C within the 21-bp repeats, the binding sites for the Ets family of proteins, and the TATA box all influenced the degree of tax-mediated activation. Tax is also able to activate gene expression of other viral and cellular promoters. Tax activation of the IL-2 receptor and the HIV-1 LTR is mediated through NF-kappa B motifs. Interestingly, sequences in the 21-bp repeat B and C motifs contain significant homology with NF-kappa B regulatory elements. We demonstrated that an NF-kappa B binding protein, PRDII-BF1, but not the rel protein, bound to the B and C motifs in the 21-bp repeat. PRDII-BF1 was also able to stimulate activation of HTLV-I gene expression by tax. The role of the Ets proteins on modulating tax activation was also studied. Ets 1 but not Ets 2 was capable of increasing the degree of tax activation of the HTLV-I LTR. These results suggest that tax activates gene expression by either direct or indirect interaction with several cellular transcription factors that bind to the HTLV-I LTR.

Published

1993

8. Localization of the gene-encoding upstream stimulatory factor (USF) to human chromosome 1q22-q23.

Author

Shieh BH, Sparkes RS, Gaynor RB, and Lusis AJ

Subjects

Animals, Base Sequence, Chromosome Mapping, DNA genetics, DNA Probes, Humans, Hybrid Cells, In Situ Hybridization, Mice, Molecular Sequence Data, Upstream Stimulatory Factors, Chromosomes, Human, Pair 1, DNA-Binding Proteins genetics, Transcription Factors genetics

Abstract

The upstream stimulatory factor, USF, is a ubiquitously expressed cellular transcription factor that binds to a symmetrical DNA sequence that is found in a variety of viral and cellular promoters. A full-length cDNA encoding the 43-kDa USF protein has previously been isolated. USF contains both helix-loop-helix and leucine repeats, which are involved in regulating its DNA binding and dimerization properties. We report the use of mouse-human somatic cell hybrids and in situ hybridization in localizing the gene-encoding USF to human chromosome 1q22-q23.

Published

1993

9. Cloning and chromosomal mapping of a human immunodeficiency virus 1 "TATA" element modulatory factor.

Author

Garcia JA, Ou SH, Wu F, Lusis AJ, Sparkes RS, and Gaynor RB

Subjects

Amino Acid Sequence, Chromosome Mapping, Chromosomes, Human, Pair 3, Cloning, Molecular, Humans, Molecular Sequence Data, RNA, Messenger genetics, Sequence Alignment, Transcription, Genetic, DNA-Binding Proteins genetics, Gene Expression Regulation, Viral, HIV-1 genetics, TATA Box, Transcription Factors genetics

Abstract

A critical regulatory element in many promoters transcribed by RNA polymerase II is the "TATA" box, which is located 25-30 nucleotides upstream of the transcription initiation site. TFIID is a biochemically defined HeLa cell nuclear fraction containing a transcription factor activity that binds specifically to the TATA box and is critical in determining both basal and regulated promoter activity. Recently, the gene for a TATA-binding protein was cloned and found to bind to various TATA elements and to substitute for TFIID in stimulating basal gene expression in in vitro transcription systems. However, it is possible that additional cellular factors can bind to the TATA element and influence the level of gene expression. By using lambda gt11 expression cloning with oligonucleotides corresponding to the human immunodeficiency virus 1 TATA element, we report the identification of a cellular protein with a calculated molecular mass of 123 kDa that we designate TATA element modulatory factor (TMF). TMF binds to the human immunodeficiency virus 1 TATA element in gel-retardation assays and inhibits activation of the viral long terminal repeat by the TATA-binding protein in in vitro transcription assays. TMF contains leucine-zipper amino acid motifs and exhibits homology in its DNA binding domain with the phage-encoded DNA binding protein Ner. Chromosomal mapping localizes the TMF gene to human chromosome 3p12-p21, which is a site of frequent rearrangements in lung and renal carcinomas. Thus, TMF is a transcription factor that likely regulates the expression of both viral and cellular genes.

Published

1992

10. Localization of the gene for the DNA-binding protein AP-2 to human chromosome 6p22.3-pter.

Author

Gaynor RB, Muchardt C, Xia YR, Klisak I, Mohandas T, Sparkes RS, and Lusis AJ

Subjects

Animals, Blotting, Southern, Chromosome Banding, Chromosome Mapping, DNA genetics, DNA isolation & purification, Humans, Hybrid Cells physiology, Mice, Transcription Factor AP-2, Chromosomes, Human, Pair 6, DNA-Binding Proteins genetics, Transcription Factors genetics

Abstract

A variety of cellular proteins bind to cellular and viral enhancer elements. One such factor, known as AP-2, is a 52-kDa transcription factor identified by its interaction with the SV40 and metallothionein enhancers. In addition, it has been found that AP-2 binds to the SV40 T-antigen. AP-2 activity is mediated by both the state of cellular differentiation and changes in signal transduction pathways, suggesting a potential role of AP-2 in the regulation of diverse cellular processes. As part of an effort to examine the chromosomal organization of cellular genes encoding transcription factors, we report the mapping of the gene encoding AP-2 to human chromosome 6p22.3-24 by analysis of somatic cell hybrids and in situ hybridization to chromosomes.

Published

1991

11. Purification of the human immunodeficiency virus type 1 enhancer and TAR binding proteins EBP-1 and UBP-1.

Author

Wu FK, Garcia JA, Harrich D, and Gaynor RB

Subjects

Base Sequence, Gene Expression Regulation, HeLa Cells metabolism, Humans, Molecular Sequence Data, Molecular Weight, Promoter Regions, Genetic, Proto-Oncogene Proteins c-jun, Transcription, Genetic, DNA, Viral isolation & purification, DNA-Binding Proteins metabolism, Enhancer Elements, Genetic, Genes, Viral, HIV genetics, Transcription Factors metabolism

Abstract

Transcription of the human immunodeficiency virus type 1 (HIV-1) is regulated by viral proteins and cellular factors that bind to the viral long terminal repeat (LTR). At least five regions of the HIV LTR serve as binding sites for HeLa cellular proteins. One region containing two copies of the sequence GGGACTTTCC functions as an enhancer element for HIV transcriptional regulation. Another region between -17 and +44 known as the TAR region contains two copies of the sequence CTCTCTGG and is also important in tat-induced activation of the HIV LTR. HeLa cell extracts were used to purify cellular proteins binding to portions of the enhancer region (EBP-1) and the TAR region (UBP-1) by a combination of conventional and DNA affinity chromatography. Several species of proteins of between 55 and 60 kd were found to bind to specific sequences in the enhancer region and these proteins also bound to a portion of the NF-kappa B binding site in the immunoglobulin kappa enhancer. Two proteins of between 61 and 63 kd were the major species found to bind to specific sequences in the TAR region and fractions containing these proteins also bind to the TATA region. Both UBP-1 and EBP-1 exhibited specific binding as demonstrated by both UV cross-linking and DNase I footprinting. Mutations of either the enhancer or TAR regulatory regions prevented binding of these purified factors. These results demonstrate the binding of highly purified cellular proteins to important transcriptional regulatory regions in the HIV LTR.

Published

1988

12. Functional domains required for tat-induced transcriptional activation of the HIV-1 long terminal repeat.

Author

Garcia JA, Harrich D, Pearson L, Mitsuyasu R, and Gaynor RB

Subjects

DNA Mutational Analysis, Gene Expression Regulation, Nuclear Proteins genetics, Oligodeoxyribonucleotides genetics, Regulatory Sequences, Nucleic Acid, Repetitive Sequences, Nucleic Acid, Structure-Activity Relationship, Transcription, Genetic, DNA-Binding Proteins genetics, HIV genetics, Retroviridae Proteins genetics, Transcription Factors genetics

Abstract

The transcriptional regulation of the human immunodeficiency virus (HIV) type I involves the interaction of both viral and cellular proteins. The viral protein tat is important in increasing the amount of viral steady-state mRNA and may also play a role in regulating the translational efficiency of viral mRNA. To identify distinct functional domains of tat, oligonucleotide-directed mutagenesis of the tat gene was performed. Point mutations of cysteine residues in three of the four Cys-X-X-Cys sequences in the tat protein resulted in a marked decrease in transcriptional activation of the HIV long terminal repeat. Point mutations which altered the basic C-domain of the protein also resulted in decreases in transcriptional activity, as did a series of mutations that repositioned either the N or C termini of the protein. Conservative mutations of other amino acids in the cysteine-rich or basic regions and in a series of proline residues in the N terminus of the molecule resulted in minimal changes in tat activation. These results suggest that several domains of tat protein are involved in transcriptional activation with the cysteine-rich domain being required for complete activity of the tat protein.

Published

1988

13. Interactions of cellular proteins involved in the transcriptional regulation of the human immunodeficiency virus.

Author

Garcia JA, Wu FK, Mitsuyasu R, and Gaynor RB

Subjects

Chromosome Deletion, HeLa Cells metabolism, Humans, Mutation, Transfection, Gene Expression Regulation, Genes, Genes, Viral, HIV genetics, Neoplasm Proteins physiology, Transcription Factors genetics, Transcription, Genetic

Abstract

The human immunodeficiency virus (HIV) is a human retrovirus which is the etiologic agent of the acquired immunodeficiency syndrome. To study the cellular factors involved in the transcriptional regulation of this virus, we performed DNase I footprinting of the viral LTR using partially purified HeLa cell extracts. Five regions of the viral LTR appear critical for DNA binding of cellular proteins. These include the negative regulatory, enhancer, SP1, TATA and untranslated regions. Deletion mutagenesis of these binding domains has significant effects on the basal level of transcription and the ability to be induced by the viral tat protein. Mutations of either the negative regulatory or untranslated regions affect factor binding to the enhancer region. In addition, oligonucleotides complementary to several of the binding domains specifically compete for factor binding. These results suggest that interactions between several distinct cellular proteins are required for HIV transcriptional regulation.

Published

1987