Mechanism of action of a repressor of dioxin-dependent induction of Cyp1a1 gene transcription.

A dominant mutant of Hepa-1 cells, c31, expresses a repressor that prevents 2,3,7,8-tetrachlorodibenzo-p-dioxin (TCDD)-dependent stimulation of Cyp1a1 transcription. The repressor acts via the xenobiotic-responsive elements (XREs), which are the DNA-binding sites for the aryl hydrocarbon (Ah) receptor-TCDD complex during transcriptional activation of the gene. High-salt nuclear extracts prepared from c31 cells grown with TCDD contained normal levels of the Ah receptor which bound the XRE with normal affinity, as judged by in vitro gel mobility shift assays. Furthermore, extracts prepared from these cells, grown either with or without TCDD, contained no novel XRE-binding proteins compared with extracts from wild-type Hepa-1 cells. However, in vivo genomic footprinting demonstrated that TCDD treatment leads to binding of the Ah receptor to the XREs in Hepa-1 but not mutant cells. This finding suggests that the repressor associates with the Ah receptor to prevent its binding to the XREs and that high-salt treatment either causes dissociation of the receptor/repressor complex or fails to extract the repressor from nuclei. The results underscore the importance of using both in vivo and in vitro assays for analyzing DNA-protein interactions.

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Mechanism of action of a repressor of dioxin-dependent induction of Cyp1a1 gene transcription

Molecular and Cellular Biology ◽

10.1128/mcb.12.5.2115-2123.1992 ◽

1992 ◽

Vol 12 (5) ◽

pp. 2115-2123

Author(s):

A J Watson ◽

K I Weir-Brown ◽

R M Bannister ◽

F F Chu ◽

S Reisz-Porszasz ◽

...

Keyword(s):

Protein Interactions ◽

Transcriptional Activation ◽

High Salt ◽

In Vitro Assays ◽

Ah Receptor ◽

Mobility Shift ◽

Nuclear Extracts ◽

Gel Mobility Shift

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Characterization of Combinatorial Stat3/GATA-1 Complexes in the γ-Globin 5′UTR.

Blood ◽

10.1182/blood.v108.11.1223.1223 ◽

2006 ◽

Vol 108 (11) ◽

pp. 1223-1223

Author(s):

Xiao Yao ◽

James K. Dzandu ◽

Betty S. Pace

Keyword(s):

Protein Interactions ◽

Transcriptional Activation ◽

Residual Activity ◽

K562 Cells ◽

Fold Increase ◽

Competitive Binding ◽

Proximal Promoter ◽

Mobility Shift

Abstract Regulation of human γ-globin expression depends on localized combinatorial interactions of trans-factors with cis-elements in the proximal promoter however, the full complement of proteins involved in γ-gene regulation remains obscure. We previously demonstrated the ability of Stat3 α to bind a +9 site in the Aγ-globin 5′untranslated region (Aγ5′UTR) to activate transcription. To expand on this observation we identified an overlapping Stat3/GATA-1 site (GAGATTATCAA) at nucleotide +21γ. Recently Stat3 and GATA-1 were shown to participate in protein-protein interactions to regulate cell differentiation. Therefore we hypothesized that GATA-1 and Stat3 may regulate γ-gene transcription through a similar mechanism. Initial chromatin immunoprecipitation (ChIP) assays were performed to demonstrate in vivo GATA-1 and Stat3 binding to the γ-promoter. ChIP assay for the Aγ-globin region between −122 to +65 produced 9-fold and 4-fold chromatin enrichment in K562 cells with GATA-1 and Stat3α antibodies respectively compared to no enrichment with IgG. Treatment with Interleukin-6 mediated a 12-fold increase in bound Stat3α and a concomitant 2-fold decrease in GATA-1 interactions. TFIID binding increased from 25-fold to 40-fold supporting transcriptional activation. To provide in vitro evidence for competitive binding in the +21γsite, electrophoretic mobility shift assays (EMSA) were performed with K562 nuclear extracts and 32P- labeled γ41 (+1 to +41), +21γ, and Stat3 and GATA-1 consensus probes. Four specific DNA-protein complexes were established with γ41. Stat3 and GATA-1 antibody studies with the four probes demonstrated that Stat3 dimers and GATA-1 dimers were bound in the Band 1 and Band 4 complexes respectively; in contrast Stat3/GATA-1 heterodimers were present in the Band 3 complex. Studies with the +21γ probe confirmed our findings with γ41. The data are consistent with our hypothesis that GATA-1 and Stat3 compete for binding to the +21γ cis-element. To further our understanding of the in vivo consequences of GATA-1/Stat3 interactions, preliminary transient transfections were performed in K562 cells. The wild type -210γLuc reporter containing the −210 to +36 γ-promoter (10μg) and this mutant −201γ(+21mStat3)Luc reporter were co-transfected individually with β-galactosidase. The luciferase activity of −201γLuc increased 110-fold after enforced pZeoStat3α (30μg) expression which dropped 75-fold when tested with the mutant Stat3 reporter. Residual activity was attributed to the intact +9γ Stat3 site. Enforced pGFP-GATA-1 expression activated the −201γLuc reporter 35-fold which increased further to 70-fold for the mutant reporter. Additional cotransfection studies will be completed to determine whether competitive interactions of Stat3 and GATA-1 occur to regulate γ-globin transcription in vivo. To confirm and verify these observations, vitro competitive binding utilizing purified Stat3 and GATA-1 proteins will be performed. 2-Dimensional EMSA coupled with mass spectroscopy will be used for comprehensive identification of the protein components of complexes bound to the Aγ5′UTR.

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Analysis of Saccharomyces cerevisiae his3 transcription in vitro: biochemical support for multiple mechanisms of transcription

Molecular and Cellular Biology ◽

10.1128/mcb.10.6.2832-2839.1990 ◽

1990 ◽

Vol 10 (6) ◽

pp. 2832-2839

Author(s):

A S Ponticelli ◽

K Struhl

Keyword(s):

Saccharomyces Cerevisiae ◽

Transcriptional Activation ◽

Transcription Initiation ◽

Molecular Mechanisms ◽

Initiation Site ◽

Activator Proteins ◽

Nuclear Extracts ◽

Transcription In Vitro

The promoter region of the Saccharomyces cerevisiae his3 gene contains two TATA elements, TC and TR, that direct transcription initiation to two sites designated +1 and +13. On the basis of differences between their nucleotide sequences and their responsiveness to upstream promoter elements, it has previously been proposed that TC and TR promote transcription by different molecular mechanisms. To begin a study of his3 transcription in vitro, we used S. cerevisiae nuclear extracts together with various DNA templates and transcriptional activator proteins that have been characterized in vivo. We demonstrated accurate transcription initiation in vitro at the sites used in vivo, transcriptional activation by GCN4, and activation by a GAL4 derivative on various gal-his3 hybrid promoters. In all cases, transcription stimulation was dependent on the presence of an acidic activation region in the activator protein. In addition, analysis of promoters containing a variety of TR derivatives indicated that the level of transcription in vitro was directly related to the level achieved in vivo. The results demonstrated that the in vitro system accurately reproduced all known aspects of in vivo his3 transcription that depend on the TR element. However, in striking contrast to his3 transcription in vivo, transcription in vitro yielded approximately 20 times more of the +13 transcript than the +1 transcript. This result was not due to inability of the +1 initiation site to be efficiently utilized in vitro, but rather it reflects the lack of TC function in vitro. The results support the idea that TC and TR mediate transcription from the wild-type promoter by distinct mechanisms.

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c-Fos-induced activation of a TATA-box-containing promoter involves direct contact with TATA-box-binding protein

Molecular and Cellular Biology ◽

10.1128/mcb.14.9.6021-6029.1994 ◽

1994 ◽

Vol 14 (9) ◽

pp. 6021-6029

Author(s):

R Metz ◽

A J Bannister ◽

J A Sutherland ◽

C Hagemeier ◽

E C O'Rourke ◽

...

Keyword(s):

Protein Interactions ◽

Transcriptional Activation ◽

Binding Protein ◽

Tata Box ◽

Binding Motif ◽

Protein Protein Interactions ◽

High Concentrations ◽

Tata Box Binding Protein

Transcriptional activation in eukaryotes involves protein-protein interactions between regulatory transcription factors and components of the basal transcription machinery. Here we show that c-Fos, but not a related protein, Fra-1, can bind the TATA-box-binding protein (TBP) both in vitro and in vivo and that c-Fos can also interact with the transcription factor IID complex. High-affinity binding to TBP requires c-Fos activation modules which cooperate to activate transcription. One of these activation modules contains a TBP-binding motif (TBM) which was identified through its homology to TBP-binding viral activators. This motif is required for transcriptional activation, as well as TBP binding. Domain swap experiments indicate that a domain containing the TBM can confer TBP binding on Fra-1 both in vitro and in vivo. In vivo activation experiments indicate that a GAL4-Fos fusion can activate a promoter bearing a GAL4 site linked to a TATA box but that this activity does not occur at high concentrations of GAL4-Fos. This inhibition (squelching) of c-Fos activity is relieved by the presence of excess TBP, indicating that TBP is a direct functional target of c-Fos. Removing the TBM from c-Fos severely abrogates activation of a promoter containing a TATA box but does not affect activation of a promoter driven only by an initiator element. Collectively, these results suggest that c-Fos is able to activate via two distinct mechanisms, only one of which requires contact with TBP. Since TBP binding is not exhibited by Fra-1, TBP-mediated activation may be one characteristic that discriminates the function of Fos-related proteins.

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Transcription from a murine T-cell receptor V beta promoter depends on a conserved decamer motif similar to the cyclic AMP response element

Molecular and Cellular Biology ◽

10.1128/mcb.9.11.4835-4845.1989 ◽

1989 ◽

Vol 9 (11) ◽

pp. 4835-4845

Author(s):

S J Anderson ◽

S Miyake ◽

D Y Loh

Keyword(s):

Cyclic Amp ◽

Regulatory Region ◽

Cell Receptor ◽

Transcription Activator ◽

Mobility Shift ◽

Response Element ◽

Cyclic Amp Response Element ◽

Gel Mobility Shift

We identified a regulatory region of the murine V beta promoter by both in vivo and in vitro analyses. The results of transient transfection assays indicated that the dominant transcription-activating element within the V beta 8.3 promoter is the palindromic motif identified previously as the conserved V beta decamer. Elimination of this element, by linear deletion or specific mutation, reduced transcriptional activity from this promoter by 10-fold. DNase I footprinting, gel mobility shift, and methylation interference assays confirmed that the palindrome acts as the binding site of a specific nuclear factor. In particular, the V beta promoter motif functioned in vitro as a high-affinity site for a previously characterized transcription activator, ATF. A consensus cyclic AMP response element (CRE) but not a consensus AP-1 site, can substitute for the decamer in vivo. These data suggest that cyclic AMP response element-binding protein (ATF/CREB) or related proteins activate V beta transcription.

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RNA binding by Sxl proteins in vitro and in vivo

Molecular and Cellular Biology ◽

10.1128/mcb.14.7.4975-4990.1994 ◽

1994 ◽

Vol 14 (7) ◽

pp. 4975-4990

Author(s):

M E Samuels ◽

D Bopp ◽

R A Colvin ◽

R F Roscigno ◽

M A Garcia-Blanco ◽

...

Keyword(s):

Protein Interactions ◽

Target Genes ◽

Rna Binding ◽

Polytene Chromosomes ◽

Regulatory Sequences ◽

Acceptor Site ◽

Nuclear Extracts ◽

Preferential Binding

Sxl has been proposed to regulate splicing of specific target genes by directly interacting with their pre-mRNAs. We have therefore examined the RNA-binding properties of Sxl protein in vitro and in vivo. Gel shift and UV cross-linking assays with a purified recombinant MBP-Sxl fusion protein demonstrated preferential binding to RNAs containing poly(U) tracts, and the protein footprinted over the poly(U) region. The protein did not appear to recognize either branch point or AG dinucleotide sequences, but an adenosine residue at the 5' end of the poly(U) tract enhanced binding severalfold. MBP-Sxl formed two shifted complexes on a tra regulated acceptor site RNA; the doubly shifted form may have been stabilized by protein-protein interactions. Consistent with its proposed role in pre-mRNA processing, in nuclear extracts Sxl was found in large ribonucleoprotein (RNP) complexes which sedimented significantly faster than bulk heterogeneous nuclear RNP and small nuclear RNPs. Anti-Sxl staining of polytene chromosomes showed Sxl protein at a number of chromosomal locations, among which was the Sxl locus itself. Sxl protein could also be targeted to a new chromosomal site carrying a transgene containing splicing regulatory sequences from the Sxl gene, following transcriptional induction. After prolonged heat shock, all Sxl protein was restricted to the heat-induced puff at the hs93D locus. In contrast, a presumptive small nuclear RNP protein was observed at several heat puffs following shock.

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Inhibition of the activation of heat shock factor in vivo and in vitro by flavonoids.

Molecular and Cellular Biology ◽

10.1128/mcb.12.8.3490 ◽

1992 ◽

Vol 12 (8) ◽

pp. 3490-3498 ◽

Cited By ~ 151

Author(s):

N Hosokawa ◽

K Hirayoshi ◽

H Kudo ◽

H Takechi ◽

A Aoike ◽

...

Keyword(s):

Heat Shock ◽

Transcriptional Activation ◽

Heat Shock Factor ◽

Mobility Shift ◽

Human Colon Cancer ◽

Heat Shock Element ◽

Mrna Accumulation ◽

Cell Extracts

Transcriptional activation of human heat shock protein (HSP) genes by heat shock or other stresses is regulated by the activation of a heat shock factor (HSF). Activated HSF posttranslationally acquires DNA-binding ability. We previously reported that quercetin and some other flavonoids inhibited the induction of HSPs in HeLa and COLO 320DM cells, derived from a human colon cancer, at the level of mRNA accumulation. In this study, we examined the effects of quercetin on the induction of HSP70 promoter-regulated chloramphenicol acetyltransferase (CAT) activity and on the binding of HSF to the heat shock element (HSE) by a gel mobility shift assay with extracts of COLO 320DM cells. Quercetin inhibited heat-induced CAT activity in COS-7 and COLO 320DM cells which were transfected with plasmids bearing the CAT gene under the control of the promoter region of the human HSP70 gene. Treatment with quercetin inhibited the binding of HSF to the HSE in whole-cell extracts activated in vivo by heat shock and in cytoplasmic extracts activated in vitro by elevated temperature or by urea. The binding of HSF activated in vitro by Nonidet P-40 was not suppressed by the addition of quercetin. The formation of the HSF-HSE complex was not inhibited when quercetin was added only during the binding reaction of HSF to the HSE after in vitro heat activation. Quercetin thus interacts with HSF and inhibits the induction of HSPs after heat shock through inhibition of HSF activation.

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Fused protein domains inhibit DNA binding by LexA.

Molecular and Cellular Biology ◽

10.1128/mcb.12.7.3006 ◽

1992 ◽

Vol 12 (7) ◽

pp. 3006-3014 ◽

Cited By ~ 105

Author(s):

E A Golemis ◽

R Brent

Keyword(s):

Dna Binding ◽

Protein Interactions ◽

In Vitro Assays ◽

Dimerization Domain ◽

Activation Domains ◽

Dna Binding Domains ◽

Binding Domains ◽

Operator Binding

Many studies of transcription activation employ fusions of activation domains to DNA binding domains derived from the bacterial repressor LexA and the yeast activator GAL4. Such studies often implicitly assume that DNA binding by the chimeric proteins is equivalent to that of the protein donating the DNA binding moiety. To directly investigate this issue, we compared operator binding by a series of LexA-derivative proteins to operator binding by native LexA, by using both in vivo and in vitro assays. We show that operator binding by many proteins such as LexA-Myc, LexA-Fos, and LexA-Bicoid is severely impaired, while binding of other LexA-derivative proteins, such as those that carry bacterially encoded acidic sequences ("acid blobs"), is not. Our results also show that DNA binding by LexA derivatives that contain the LexA carboxy-terminal dimerization domain (amino acids 88 to 202) is considerably stronger than binding by fusions that lack it and that heterologous dimerization motifs cannot substitute for the LexA88-202 function. These results suggest the need to reevaluate some previous studies of activation that employed LexA derivatives and modifications to recent experimental approaches that use LexA and GAL4 derivatives to detect and study protein-protein interactions.

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Mutational and in vitro protein-binding studies on centromere DNA from Saccharomyces cerevisiae.

Molecular and Cellular Biology ◽

10.1128/mcb.7.12.4522 ◽

1987 ◽

Vol 7 (12) ◽

pp. 4522-4534 ◽

Cited By ~ 47

Author(s):

R Ng ◽

J Carbon

Keyword(s):

Saccharomyces Cerevisiae ◽

Protein Binding ◽

In Vitro Assays ◽

Binding Studies ◽

Mobility Shift ◽

Sequence Element ◽

Sequence Elements ◽

Mobility Shift Assay

Centromeres on chromosomes in the yeast Saccharomyces cerevisiae contain approximately 140 base pairs (bp) of DNA. The functional centromere (CEN) region contains three important sequence elements (I, PuTCACPuTG; II, 78 to 86 bp of high-AT DNA; and III, a conserved 25-bp sequence with internal bilateral symmetry). Various point mutations or deletions in the element III region have a profound effect on CEN function in vivo, indicating that this DNA region is a key protein-binding site. This has been confirmed by the use of two in vitro assays to detect binding of yeast proteins to DNA fragments containing wild-type or mutationally altered CEN3 sequences. An exonuclease III protection assay was used to demonstrate specific binding of proteins to the element III region of CEN3. In addition, a gel DNA fragment mobility shift assay was used to characterize the binding reaction parameters. Sequence element III mutations that inactivate CEN function in vivo also prevent binding of proteins in the in vitro assays. The mobility shift assay indicates that double-stranded DNAs containing sequence element III efficiently bind proteins in the absence of sequence elements I and II, although the latter sequences are essential for optimal CEN function in vivo.

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Host Protein Interactions with the 3′ End of Bovine Coronavirus RNA and the Requirement of the Poly(A) Tail for Coronavirus Defective Genome Replication

Journal of Virology ◽

10.1128/jvi.74.11.5053-5065.2000 ◽

2000 ◽

Vol 74 (11) ◽

pp. 5053-5065 ◽

Cited By ~ 85

Author(s):

Jeannie F. Spagnolo ◽

Brenda G. Hogue

Keyword(s):

Protein Interactions ◽

Helper Virus ◽

Host Protein ◽

Genome Replication ◽

Mobility Shift ◽

Bovine Coronavirus ◽

Replication Assay ◽

Infected Cells ◽

Gel Mobility Shift

ABSTRACT RNA viruses have 5′ and 3′ untranslated regions (UTRs) that contain specific signals for RNA synthesis. The coronavirus genome is capped at the 5′ end and has a 3′ UTR that consists of 300 to 500 nucleotides (nt) plus a poly(A) tail. To further our understanding of coronavirus replication, we have begun to examine the involvement of host factors in this process for two group II viruses, bovine coronavirus (BCV) and mouse hepatitis coronavirus (MHV). Specific host protein interactions with the BCV 3′ UTR [287 nt plus poly(A) tail] were identified using gel mobility shift assays. Competition with the MHV 3′ UTR [301 nt plus poly(A) tail] suggests that the interactions are conserved for the two viruses. Proteins with molecular masses of 99, 95, and 73 kDa were detected in UV cross-linking experiments. Less heavily labeled proteins were also detected in the ranges of 40 to 50 and 30 kDa. The poly(A) tail was required for binding of the 73-kDa protein. Immunoprecipitation of UV-cross-linked proteins identified the 73-kDa protein as the cytoplasmic poly(A)-binding protein (PABP). Replication of the defective genomes BCV Drep and MHV MIDI-C, along with several mutants, was used to determine the importance of the poly(A) tail. Defective genomes with shortened poly(A) tails consisting of 5 or 10 A residues were replicated after transfection into helper virus-infected cells. BCV Drep RNA that lacked a poly(A) tail did not replicate, whereas replication of MHV MIDI-C RNA with a deleted tail was detected after several virus passages. All mutants exhibited delayed kinetics of replication. Detectable extension or addition of the poly(A) tail to the mutants correlated with the appearance of these RNAs in the replication assay. RNAs with shortened poly(A) tails exhibited less in vitro PABP binding, suggesting that decreased interactions with the protein may affect RNA replication. The data strongly indicate that the poly(A) tail is an important cis-acting signal for coronavirus replication.

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