The Regulator of Nitrate Assimilation in Ascomycetes Is a Dimer Which Binds a Nonrepeated, Asymmetrical Sequence

ABSTRACT The regulation of nitrate assimilation seems to follow the same pattern in all ascomycetes where this process has been studied. We show here by in vitro binding studies and a number of protection and interference techniques that the transcription factor mediating nitrate induction in Aspergillus nidulans, a protein containing a binuclear zinc cluster DNA binding domain, recognizes an asymmetrical sequence of the form CTCCGHGG. We further show that the protein binds to its consensus site as a dimer. We establish the role of the putative dimerization element by its ability to replace the analogous element of the cI protein of phage λ. Mutagenesis of crucial leucines of the dimerization element affect both the binding ability of the dimer and the conformation of the resulting protein-DNA complex. This is the first case to be described where a dimer recognizes such an asymmetrical nonrepeated sequence, presumably by each monomeric subunit making different contacts with different DNA half-sites.

Download Full-text

EWS, but Not EWS-FLI-1, Is Associated with Both TFIID and RNA Polymerase II: Interactions between Two Members of the TET Family, EWS and hTAFII68, and Subunits of TFIID and RNA Polymerase II Complexes

Molecular and Cellular Biology ◽

10.1128/mcb.18.3.1489 ◽

1998 ◽

Vol 18 (3) ◽

pp. 1489-1497 ◽

Cited By ~ 161

Author(s):

Anne Bertolotti ◽

Thomas Melot ◽

Joël Acker ◽

Marc Vigneron ◽

Olivier Delattre ◽

...

Keyword(s):

Rna Polymerase ◽

Rna Polymerase Ii ◽

Chromosomal Translocation ◽

Binding Studies ◽

Pol Ii ◽

Nuclear Extracts ◽

Vitro Binding ◽

Tfiid Complex

ABSTRACT The t(11;22) chromosomal translocation specifically linked to Ewing sarcoma and primitive neuroectodermal tumor results in a chimeric molecule fusing the amino-terminus-encoding region of theEWS gene to the carboxyl-terminal DNA-binding domain encoded by the FLI-1 gene. As the function of the protein encoded by the EWS gene remains unknown, we investigated the putative role of EWS in RNA polymerase II (Pol II) transcription by comparing its activity with that of its structural homolog, hTAFII68. We demonstrate that a portion of EWS is able to associate with the basal transcription factor TFIID, which is composed of the TATA-binding protein (TBP) and TBP-associated factors (TAFIIs). In vitro binding studies revealed that both EWS and hTAFII68 interact with the same TFIID subunits, suggesting that the presence of EWS and that of hTAFII68 in the same TFIID complex may be mutually exclusive. Moreover, EWS is not exclusively associated with TFIID but, similarly to hTAFII68, is also associated with the Pol II complex. The subunits of Pol II that interact with EWS and hTAFII68 have been identified, confirming the association with the polymerase. In contrast to EWS, the tumorigenic EWS–FLI-1 fusion protein is not associated with either TFIID or Pol II in Ewing cell nuclear extracts. These observations suggest that EWS and EWS–FLI-1 may play different roles in Pol II transcription.

Download Full-text

Dynamics of Ankyrin-containing Complexes in Chicken Embryonic Erythroid Cells: Role of Phosphorylation

Molecular Biology of the Cell ◽

10.1091/mbc.12.12.3864 ◽

2001 ◽

Vol 12 (12) ◽

pp. 3864-3874 ◽

Cited By ~ 6

Author(s):

Sourav Ghosh ◽

John V. Cox

Keyword(s):

Complex Formation ◽

Anion Exchanger ◽

Erythroid Cells ◽

Binding Studies ◽

Phosphatase Inhibitors ◽

In Vitro Binding ◽

Vitro Binding

Chicken erythroid ankyrin undergoes a fairly rapid cycle of cytoskeletal association, dissociation, and turnover. In addition, the cytoskeletal association of ankyrin is regulated by phosphorylation. Treatment of erythroid cells with serine and threonine phosphatase inhibitors stimulated the hyperphosphorylation of the 225- and 205-kDa ankyrin isoforms, and dissociated the bulk of these isoforms from cytoskeletal spectrin. In vitro binding studies have shown that this dissociation of ankyrin from spectrin in vivo can be attributed to a reduced ability of hyperphosphorylated ankyrin to bind spectrin. Interestingly, a significant fraction of detergent insoluble ankyrin accumulates in a spectrin-independent pool. At least some of this spectrin-independent pool of ankyrin is complexed with the AE1 anion exchanger, and the solubility properties of this pool are also regulated by phosphorylation. Treatment of cells with serine and threonine phosphatase inhibitors had no effect on ankyrin/AE1 complex formation. However, these inhibitors were sufficient to shift ankyrin/AE1 complexes from the detergent insoluble to the soluble pool. These analyses, which are the first to document the in vivo consequences of ankyrin phosphorylation, indicate that erythroid ankyrin-containing complexes can undergo dynamic rearrangements in response to changes in phosphorylation.

Download Full-text

IC-P-199: Comparing [3 H]MK-6240 and [3 H]AV-1451(T-807) In In vitro Binding Studies in Brain Tissues

Alzheimer s & Dementia ◽

10.1016/j.jalz.2016.06.230 ◽

2016 ◽

Vol 12 ◽

pp. P144-P144

Author(s):

Zhizhen Zeng ◽

Patricia J. Miller ◽

Brett M. Connolly ◽

Stacey S. O’Malley ◽

Idriss Bennacef ◽

...

Keyword(s):

Binding Studies ◽

In Vitro Binding ◽

Vitro Binding ◽

Brain Tissues

Download Full-text

Organization of the regulatory region of the yeast CYC7 gene: multiple factors are involved in regulation

Molecular and Cellular Biology ◽

10.1128/mcb.7.9.3252-3259.1987 ◽

1987 ◽

Vol 7 (9) ◽

pp. 3252-3259

Author(s):

T Prezant ◽

K Pfeifer ◽

L Guarente

Keyword(s):

Cytochrome C ◽

Regulatory Region ◽

Carbon Sources ◽

Binding Studies ◽

Multiple Factors ◽

Vitro Binding ◽

Genes Encoding ◽

Nonfermentable Carbon Source

Regulation of the CYC7 gene of Saccharomyces cerevisiae, encoding iso-2-cytochrome c, was studied. Expression was induced about 20-fold by heme and derepressed 4- to 8-fold by a shift from glucose medium to one containing a nonfermentable carbon source. Deletion analysis showed that induction by heme depends upon sequences between -250 and -228 (from the coding sequence) and upon the HAP1 activator gene, previously shown to be required for CYC1 expression (L. Guarente et al., Cell 36:503-511, 1984). Thus, HAP1 coordinates expression of CYC7 and CYC1, the two genes encoding isologs of cytochrome c in S. cerevisiae. HAP1-18, a mutant allele of HAP1, which increased CYC7 expression more than 10-fold, also acted through sequences between -250 and -228. In vitro binding studies showed that the HAP1 product binds to these sequences (see also K. Pfeifer, T. Prezant, and L. Guarente, Cell 49:19-28, 1987) and an additional factor binds to distal sequences that lie between -201 and -165. This latter site augmented CYC7 expression in vivo. Derepression of CYC7 expression in a medium containing nonfermentable carbon sources depended upon sequences between -354 and -295. The interplay of these multiple sites and the factors that bind to them are discussed.

Download Full-text

Different Forms of TFF2, A Lectin of the Human Gastric Mucus Barrier: In Vitro Binding Studies

International Journal of Molecular Sciences ◽

10.3390/ijms20235871 ◽

2019 ◽

Vol 20 (23) ◽

pp. 5871 ◽

Cited By ~ 10

Author(s):

Franziska Heuer ◽

René Stürmer ◽

Jörn Heuer ◽

Thomas Kalinski ◽

Antje Lemke ◽

...

Keyword(s):

Molecular Mass ◽

Gastric Mucus ◽

Binding Studies ◽

Binding Characteristics ◽

Duodenal Glands ◽

Vitro Binding ◽

Trefoil Factor Family ◽

Mucus Barrier ◽

Mass Form

Trefoil factor family 2 (TFF2) and the mucin MUC6 are co-secreted from human gastric and duodenal glands. TFF2 binds MUC6 as a lectin and is a constituent of the gastric mucus. Herein, we investigated human gastric extracts by FPLC and identified mainly high- but also low-molecular-mass forms of TFF2. From the high-molecular-mass forms, TFF2 can be completely released by boiling in SDS or by harsh denaturing extraction. The low-molecular-mass form representing monomeric TFF2 can be washed out in part from gastric mucosa specimens with buffer. Overlay assays with radioactively labeled TFF2 revealed binding to the mucin MUC6 and not MUC5AC. This binding is modulated by Ca2+ and can be blocked by the lectin GSA-II and the monoclonal antibody HIK1083. TFF2 binding was also inhibited by Me-β-Gal, but not the α anomer. Thus, both the α1,4GlcNAc as well as the juxtaperipheral β-galactoside residues of the characteristic GlcNAcα1→4Galβ1→R moiety of human MUC6 are essential for TFF2 binding. Furthermore, there are major differences in the TFF2 binding characteristics when human is compared with the porcine system. Taken together, TFF2 appears to fulfill an important role in stabilizing the inner insoluble gastric mucus barrier layer, particularly by its binding to the mucin MUC6.

Download Full-text

Identification and purification of a protein that binds DNA cooperatively with the yeast SWI5 protein.

Molecular and Cellular Biology ◽

10.1128/mcb.13.9.5524 ◽

1993 ◽

Vol 13 (9) ◽

pp. 5524-5537 ◽

Cited By ~ 24

Author(s):

R M Brazas ◽

D J Stillman

Keyword(s):

Zinc Finger Protein ◽

Cooperative Interaction ◽

Protein Fusion ◽

Glutathione S Transferase ◽

Binding Studies ◽

Eukaryotic Transcription ◽

Low Concentrations ◽

Vitro Binding

The Saccharomyces cerevisiae SWI5 gene encodes a zinc finger protein required for the expression of the HO gene. A protein fusion between glutathione S-transferase and SWI5 was expressed in Escherichia coli and purified. The GST-SWI5 fusion protein formed only a low-affinity complex in vitro with the HO promoter, which was inhibited by low concentrations of nonspecific DNA. This result was surprising, since genetic evidence demonstrated that SWI5 functions at the HO promoter via this site in vivo. A yeast factor, GRF10 (also known as PHO2 and BAS2), that promoted high-affinity binding of SWI5 in the presence of a large excess of nonspecific carrier DNA was purified. Final purification of the 83-kDa GRF10 protein was achieved by cooperative interaction-based DNA affinity chromatography. In vitro binding studies demonstrated that SWI5 and GRF10 bind DNA cooperatively. Methylation interference and missing-nucleoside studies demonstrated that the two proteins bind at adjacent sites, with each protein making unique DNA contacts. SWI5 and GRF10 interactions were not detected in the absence of DNA. The role of cooperative DNA binding in determining promoter specificity of eukaryotic transcription factors is discussed.

Download Full-text

Lyn Physically Associates With the Erythropoietin Receptor and May Play a Role in Activation of the Stat5 Pathway

Blood ◽

10.1182/blood.v91.10.3734 ◽

1998 ◽

Vol 91 (10) ◽

pp. 3734-3745 ◽

Cited By ~ 128

Author(s):

Hiroshi Chin ◽

Ayako Arai ◽

Hiroshi Wakao ◽

Ryuichi Kamiyama ◽

Nobuyuki Miyasaka ◽

...

Keyword(s):

Tyrosine Kinase ◽

Tyrosine Phosphorylation ◽

Kinase Domain ◽

Sh2 Domain ◽

Erythropoietin Receptor ◽

Tyrosine Kinase Domain ◽

Binding Studies ◽

In Vitro Binding ◽

Vitro Binding

Abstract Protein tyrosine phosphorylation plays a crucial role in signaling from the receptor for erythropoietin (Epo), although the Epo receptor (EpoR) lacks the tyrosine kinase domain. We have previously shown that the Jak2 tyrosine kinase couples with the EpoR to transduce a growth signal. In the present study, we demonstrate that Lyn, a Src family tyrosine kinase, physically associates with the EpoR in Epo-dependent hematopoietic cell lines, 32D/EpoR-Wt and F36E. Coexpression experiments in COS7 cells further showed that Lyn induces tyrosine phosphorylation of the EpoR and that both LynA and LynB, alternatively spliced forms of Lyn, bind with the membrane-proximal 91-amino acid region of the EpoR cytoplasmic domain. In vitro binding studies using GST-Lyn fusion proteins further showed that the Src homology (SH)-2 domain of Lyn specifically binds with the tyrosine-phosphorylated EpoR in lysate from Epo-stimulated cells, whereas the tyrosine kinase domain of Lyn binds with the unphosphorylated EpoR. Far-Western blotting and synthetic phosphopeptide competition assays further indicated that the Lyn SH2 domain directly binds to the tyrosine-phosphorylated EpoR, most likely through its interaction with phosphorylated Y-464 or Y-479 in the carboxy-terminal region of the EpoR. In vitro binding studies also demonstrated that the Lyn SH2 domain directly binds to tyrosine-phosphorylated Jak2. In vitro reconstitution experiments in COS7 cells further showed that Lyn induces tyrosine phosphorylation of Stat5, mainly on Y-694, and activates the DNA-binding and transcription-activating abilities of Stat5. In agreement with this, Lyn enhanced the Stat5-dependent transcriptional activation when overexpressed in 32D/EpoR-Wt cells. In addition, Lyn was demonstrated to phosphorylate the EpoR and Stat5 on tyrosines in vitro. These results suggest that Lyn may play a role in activation of the Jak2/Stat5 and other signaling pathways by the EpoR.

Download Full-text

Trefoil Factor Family (TFF) Modules Are Characteristic Constituents of Separate Mucin Complexes in the Xenopus laevis Integumentary Mucus: In Vitro Binding Studies with FIM-A.1

International Journal of Molecular Sciences ◽

10.3390/ijms21072400 ◽

2020 ◽

Vol 21 (7) ◽

pp. 2400 ◽

Cited By ~ 1

Author(s):

René Stürmer ◽

Jana Reising ◽

Werner Hoffmann

Keyword(s):

Molecular Mass ◽

Complex I ◽

Size Exclusion ◽

Trefoil Factor ◽

Binding Studies ◽

In Vitro Binding ◽

Vitro Binding ◽

Exclusion Chromatography ◽

Trefoil Factor Family

The skin of the frog Xenopus laeevis is protected from microbial infections by a mucus barrier that contains frog integumentary mucins (FIM)-A.1, FIM-B.1, and FIM-C.1. These gel-forming mucins are synthesized in mucous glands consisting of ordinary mucous cells and one or more cone cells at the gland base. FIM-A.1 and FIM-C.1 are unique because their cysteine-rich domains belong to the trefoil factor family (TFF). Furthermore, FIM-A.1 is unusually short (about 400 amino acid residues). In contrast, FIM-B.1 contains cysteine-rich von Willebrand D (vWD) domains. Here, we separate skin extracts by the use of size exclusion chromatography and analyze the distribution of FIM-A.1 and FIM-C.1. Two mucin complexes were detected, i.e., a high-molecular-mass Complex I, which contains FIM-C.1 and little FIM-A.1, whereas Complex II is of lower molecular mass and contains the bulk of FIM-A.1. We purified FIM-A.1 by a combination of size-exclusion chromatography (SEC) and anion-exchange chromatography and performed first in vitro binding studies with radioactively labeled FIM-A.1. Binding of 125I-labeled FIM-A.1 to the high-molecular-mass Complex I was observed. We hypothesize that the presence of FIM-A.1 in Complex I is likely due to lectin interactions, e.g., with FIM-C.1, creating a complex mucus network.

Download Full-text

Zur Interaktion von Anthracyclinen und Anthracyclinonen mit DNS / Interaction of Anthracyclines and Anthracyclinones with DNA

Zeitschrift für Naturforschung B ◽

10.1515/znb-1970-0406 ◽

1970 ◽

Vol 25 (4) ◽

pp. 362-367 ◽

Cited By ~ 31

Author(s):

H. Berg ◽

K. Eckardt

Keyword(s):

Binding Constants ◽

Cooperative Interaction ◽

Sugar Residue ◽

Binding Mechanism ◽

Buffer Solution ◽

Binding Ability ◽

Weak Binding ◽

Order Of Magnitude ◽

Dna Complex

It was shown by the polarographic data of the complexes between antracycline antibiotics and DNA that in contrast to their biological inactive aglycones and other antracyclinones, a cooperative interaction of the intercalating chromophore as well as the sugar residue of the anthracycline molecules, is generally responsible for the complex formation with DNA.The high complex binding constants of the antracyclines daunomycin, nogalamycin, galirubin A and galirubin B measured in dimethylsulfoxid-buffer solution are in the same order of magnitude as those of actinomycins. On the other hand, only a weak binding ability of the aglycones daunomycinon, ε-pyrromycinon and aklavinon, as well as of other investigated anthracyclinones and model hydroxyanthraquinones, could be observed.No significant influence of the number and positions of the chromophore hydroxyls could be noticed.The results suggest that the first outerphase addition of the sugar residues to the backbone of the helix gives the necessary space of time for the slower intercalation process of the planar chromophore.In the case of denatured DNA, the antibiotic-DNA-complex has a lowered stability.The important role of the sugar residue for the binding mechanism strongly suggests that modifications of the nature and position of the basic sugar residue should be most valuable for the synthesis of new effective anthracyclines.

Download Full-text

Physical and functional interactions between Stat5 and the tyrosine- phosphorylated receptors for erythropoietin and interleukin-3

Blood ◽

10.1182/blood.v88.12.4415.bloodjournal88124415 ◽

1996 ◽

Vol 88 (12) ◽

pp. 4415-4425 ◽

Cited By ~ 64

Author(s):

H Chin ◽

N Nakamura ◽

R Kamiyama ◽

N Miyasaka ◽

JN Ihle ◽

...

Keyword(s):

Tyrosine Phosphorylation ◽

Sh2 Domain ◽

Binding Studies ◽

Interleukin 3 ◽

In Vitro Binding ◽

Vitro Binding ◽

Docking Sites ◽

Carboxy Terminal

Erythropoietin (Epo) and interleukin-3 (IL-3) stimulate activation of the Jak2 tyrosine kinase and induce tyrosine phosphorylation and activation of Stat5. In the present study, we have shown that Epo or IL-3 stimulation induces binding of Stat5 to the tyrosine-phosphorylated Epo receptor (EpoR) or IL-3 receptor beta subunit (betaIL3), respectively, in IL-3-dependent 32D cells expressing the EpoR. The binding of Stat5 to these cytokine receptors was shown to be rapid and transient, occurring within 1 minute of stimulation of cells and significantly decreasing after 5 minutes of cell treatment. In vivo binding experiments in COS cells showed that binding of Stat5 to the EpoR was mediated through the Stat5 Src homology 2 (SH2) domain. In vitro binding studies further showed that Stat5, but not other Stats examined, bound specifically to tyrosine-phosphorylated recombinant EpoR fusion proteins. In these in vivo and in vitro binding studies, Stat5 bound, albeit to a lesser degree, to truncated EpoR mutants in which all the intracellular tyrosines except Y-343 were removed. Furthermore, EpoR-derived synthetic phosphotyrosine peptides corresponding to Y-343, Y-401, Y-431, and Y-479 inhibited the in vitro binding of Stat5. When expressed in 32D cells, a mutant EpoR in which all the intracellular tyrosines were removed by carboxy-terminal truncation showed a significantly impaired ability to induce tyrosine phosphorylation of Stat5, particularly at low concentrations of Epo, but exhibited an increased sensitivity to Epo for growth signaling as compared with the wild-type EpoR. These results indicate that Stat5 specifically and transiently binds to the EpoR through the interaction between the Stat5 SH2 domain and specific phosphorylated tyrosines, including Y-343, in the EpoR cytoplasmic domain. It was implied that betaIL3 may also have similar Stat5 docking sites. The Stat5 docking sites in the EpoR were shown to facilitate specific activation of Stat5, which, however, may not be required for the EpoR-mediated growth signaling.

Download Full-text