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J. Biol. Chem., Vol. 275, Issue 32, 24392-24399, August 11, 2000
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From the Department of Chemistry and Biochemistry, University of
California San Diego, La Jolla, California 92093
Received for publication, May 4, 2000, and in revised form, May 19, 2000
The DNA binding of three different NF- The Rel/NF- The NF- Rel/NF- Recently, the NMR structures of a 16-base pair duplex DNA containing
the Among NF- Materials--
5'-Fluorescein-labeled oligonucleotides were
purchased from the Keck Oligonucleotide Synthesis Facility at Yale
University (New Haven, CT). Unlabeled oligonucleotides were synthesized
using a Milligen/Biosearch Cyclone Plus DNA synthesizer.
Electrophoresis and fluorescence polarization chemicals were purchased
from Fisher Scientific, except for MOPS and CAPSO buffers, which were
purchased from Sigma. T4-polynucleotide kinase was purchased from New
England Biolabs. [ Site-directed Mutagenesis--
Monomeric p50 and p65 mutants
were generated through a two-step polymerase chain reaction strategy
using internal primers. The N- and C-terminal primers for both mutants
were the same as those used for the wild type proteins (12). For the
p50 Y267D/L269D mutant, the internal primers used were: N-terminal,
5'-GGGGAGGAGATTGATCTAGATTGTGACAAGGTTC-3'; C-terminal,
5'-GAACCTTGTCACAATCTAGATCAATCTCCTCCCC-3'.
For the p65 F213D/L215D mutant, the internal primers used were:
N-terminal, 5'-GGGGATGAGATCGATCTAGATTGCGACAAGGTG-3'; C-terminal, 5'-CACCTTGTCGCAATCTAGATCGATCTCATCCCC-3'.
Electrophoretic Mobility Shift Assay (EMSA)--
The
oligonucleotide used for the EMSAs was
5'-TCTGAGGGACTTTCCTGATC-3', which contains the
heterodimer target site Ig- Fluorescence Anisotropy Assay (FAA)--
Two 5'-fluorescein
labeled oligonucleotides were used for these assays. A 39-mer
containing the Ig- Data Analysis--
First, the fraction of DNA bound in each
reaction was determined. For EMSA the fraction bound was determined by
integrating the area under the peaks for each band and dividing the
area of the bound DNA band by the total area of the bound and free DNA bands. For the FAAs fraction bound was calculated by subtracting the
experimentally determined polarization value for free DNA from the
observed polarization value for each data point, then dividing each by
the polarization value for NF-
Equation 1 was modified to determine the cooperativity of p50/p65
binding as follows.
Kapp values from salt dependence FAAs were then
fit to the following models to determine the number of cations and
H2O molecules displaced upon NF- Binding Affinities of NF-
The affinity of NF-
Anisotropy profiles for each binding experiment show an initial plateau
indicating unbound DNA, followed by a rise in anisotropy as proteins
bind to DNA, and a final plateau showing saturated binding. As
mentioned previously for EMSA experiments, the binding data for
anisotropy experiments fit the cooperative model. The apparent
dissociation constants obtained from these anisotropy experiments are
very similar to those found in EMSA experiments. Next, we measured the
affinity of the p50 homodimer for the IFN-
To further investigate the cooperative nature of binding, it is
important to determine the affinity of a monomer for its Binding Affinities of NF- Binding Affinities of p50/p65 Heterodimer for
The nature of binding isotherm clearly indicates that the heterodimer
binds Effect of pH on Complex Formation--
To test the pH sensitivity
of the interactions between the heterodimer and Ig- Effect of Salt on Complex Formation--
The dependence of the
apparent K for the p50/p65 heterodimer-Ig- Effect of Temperature on Complex Formation--
The dependence of
Kapp on temperature at constant salt
concentration (50 mM) and pH (7.5) was determined for
the heterodimer/Ig- Over the last 5 years, three-dimensional x-ray structures of nine
different complexes of DNA-bound NF- Binding Affinities--
We have used two different methods to
measure binding affinities: gel mobility shift assay and solution-based
fluorescence polarization assay. Binding affinities obtained from both
these assays are comparable for each of the three NF-
Based on the three-dimensional structures of several NF- pH Effect on Binding--
DNA binding by the NF- Salt Effect on Binding--
NF-
From the p50/p65 structure, it appears that a significant fraction of
the binding affinity of NF-
It is interesting to note that, during the original purification of the
p50/p65 heterodimer, it was observed that the protein bound almost as
tightly to nonspecific oligonucleotide columns as to specific ones.
NF-
Ha et al. (14) have successfully derived an equation
describing the effects of monovalent salt and water on DNA-protein complex formation (Equation 4), which has been simplified by O'Brien et al. (15). Using this ion displacement model, we calculate an A value of 6 ions (also the Z value from
Equation 3) and a B value of 426 water molecules released
upon complex formation. The crystal structure of the complex shows
that, upon association, 3800 Å2 of solvent-accessible
surface area is buried (11). Considering 9 Å2 as the
surface area of a water molecule, theoretically 422 molecules of water
would be released from this complex.
Temperature Effect of Binding--
The dependence of the apparent
binding constants on temperature at constant salt (50 mM
NaCl) and pH (7.5) was determined. As shown in Fig. 7, apparent binding
constants essentially remain unchanged at temperatures ranging from
4 °C to 42 °C. This suggests that the intrinsic enthalpy change
upon complex formation is negligible. It therefore appears that the
binding of Ig-
X-ray crystallographic analyses of various NF- We acknowledge Partho Ghosh, Simpson Joseph,
and the members of the G. Ghosh laboratory for critical reading of this
manuscript, as well as the C. Zucker laboratory for the use of the
PhosphorImager and storage screens.
*
This work was supported in part by National Institutes of
Health Grant CA-71871 and fellowships from the Alfred P. Sloan and Hellman Foundations.The costs of publication of this
article were defrayed in part by the
payment of page charges. The article
must therefore be hereby marked
"advertisement" in
accordance with 18 U.S.C. Section
1734 solely to indicate this fact.
§
Supported by a predoctoral fellowship from the American Heart Association.
¶
To whom correspondence should be addressed. Tel.:
858-822-0469; Fax: 858-534-7042; E-mail:
gghosh@ucsd.edu.
Published, JBC Papers in Press, May 23, 2000, DOI 10.1074/jbc.M003784200
The abbreviations used are:
RHR, Rel homology
region;
HIV-LTR, human immunodeficiency virus-long terminal repeat;
MES, 2-(N-morpholino)ethanesulfonic acid;
MOPS, 3-(N-morpholino)propanesulfonic acid;
CAPSO, 3-(cyclohexylamino)-2-hydroxy-1-propanesulfonic acid;
IFN, interferon;
EMSA, electrophoretic mobility shift assay;
FAA, fluorescence
anisotropy assay.
Mechanism of
B DNA binding by Rel/NF-B dimers*
,
ABSTRACT
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
B
dimers, the p50 and p65 homodimers and the p50/p65 heterodimer, has
been examined using a combination of gel mobility shift and
fluorescence anisotropy assays. The NF-B p50/p65 heterodimer is
shown here to bind the B DNA target site of the immunoglobulin enhancer (Ig-B) with an affinity of approximately 10 nM. The p50 and p65 homodimers bind to the same site
with roughly 5- and 15-fold lower affinity, respectively. The nature of
the binding isotherms indicates a cooperative mode of binding for all
three dimers to the DNA targets. We have further characterized the role
of pH, salt, and temperature on the formation of the p50/p65
heterodimer-Ig-B complex. The heterodimer binds to the Ig-B DNA
target in a pH-dependent manner, with the highest affinity
between pH 7.0 and 7.5. A strong salt-dependent interaction
between Ig-B and the p50/p65 heterodimer is observed, with optimum
binding occurring at monovalent salt concentrations below 75 mM, with binding becoming virtually nonspecific at a salt
concentration of 200 mM. Binding of the heterodimer to DNA was unchanged across a temperature range between 4 °C and 42 °C. The sensitivity to ionic environment and insensitivity to temperature indicate that NF-B p50/p65 heterodimers form complexes with specific DNA in an entropically driven manner.
INTRODUCTION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
B transcription factors constitute one of the most
important families of regulatory transcription factors. Members of the
Rel/NF-B family are essential for diverse biological functions such
as the regulation of innate and adaptive immunity, development, and
apoptosis in a wide array of eukaryotes from Drosophila to man (1-4). Like most transcription factors, dimers of NF-B proteins modulate transcription by directly binding to enhancer sequences located in the regulatory regions of numerous genes. These DNA sequences are collectively known as B DNA sequences. In mammals, the
Rel/NF-B dimers arise from five polypeptides, p50, p52, p65, c-Rel,
and RelB. The most abundant of these dimers are the p50/p65 heterodimer
and the p50 homodimer. The existences of some, but not all, of the
other possible dimers have been shown to exist in cells.
B family can be divided into two subgroups based on the
presence or absence of an activation domain. p50 and p52 do not contain
a distinct activation domain and belong to class I. The other three
members constitute the class II subfamily. It is generally believed
that the homodimers of p50 and p52 and the p50/p52 heterodimer function
as transcriptional repressors. The remaining combinations of dimeric
NF-B proteins, containing at least one monomer of p65, c-Rel, or
RelB, act as activators.
B proteins share a region that shows over 45% sequence
similarity across the entire family. This region, known as the Rel
homology region (RHR),1 is
responsible for DNA binding and subunit dimerization. High resolution
x-ray crystal structures of RHRs are known for four homodimers, p50,
p52, p65, and c-Rel in their DNA-bound conformations (5-8). These
structures show that, as expected, Rel/NF-B proteins also share
similar structures. Most of the RHR is folded into two
immunoglobulin-like domains connected by a 10-amino acid linker; the
N-terminal domain confers sequence specificity in DNA binding, and the
C-terminal domain is involved in dimerization as well as DNA backbone
recognition. These structures show that, unlike most other
transcription factors, NF-B dimers do not use any secondary
structure for contacting DNA. All the DNA-contacting residues emanate
from loops connecting secondary structures. Crystal structures of these
complexes suggest that in their free form the N-terminal domains should
be flexible with respect to the dimerization domain.
B target from the HIV-LTR, which is identical to the B site
in the immunoglobulin light chain gene (Ig-B), and a mutant form
of the target site that abolishes DNA binding have been solved (9, 10).
These show that the phosophodiester bonds of the sugar-phosphate
backbone of the native duplex preferentially adopt a distinct
conformation in the 5' and 3' regions of the B site. The mutant site
is incapable of adopting the native DNA's conformation, suggesting
that B-DNA sequence also plays a role in NF-B-DNA complex
formation. The combined flexibility of the NF-B dimers and their
target DNA allows NF-B to adopt multiple conformations in a promoter
specific manner.
B's most well characterized DNA targets are the B DNA
sites of the immunoglobulin light chain gene and HIV-LTR (Ig-B)
and the interferon 
gene (IFN-B). A crystal structure of the
NF-B p50/p65 heterodimer bound to the Ig-B DNA target has been
completed (11). In order to understand the mechanism of DNA binding by
NF-B, thermodynamic parameters need to be determined for various
NF-B dimers and B DNA target sites. In this study we have
analyzed binding of Ig-B and IFN-B DNA targets with three
different NF-B dimers: p50 homodimer, p65 homodimer, and p50/p65
heterodimer, using both a gel mobility assay and a solution-based fluorescence anisotropy assay. The binding of NF-B p50/p65
heterodimer to Ig-B DNA has been further tested for its dependence
on pH, salt, and temperature.
EXPERIMENTAL PROCEDURES
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ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
-32P]ATP and poly(dI-dC) carrier DNA
were purchased from Amersham Pharmacia Biotech. The Nucleotide Removal
Kit was purchased from Qiagen. All proteins were purified according to
Refs. 5, 6, 8, and 12.
B (underlined). This oligonucleotide was
annealed to its complimentary strand and end radiolabeled with
32P using T4-polynucleotide kinase and
[-32P]ATP. The labeled DNA was then purified using a
Nucleotide Removal Kit. Binding reactions were performed using constant
DNA concentration (100 pM for the p50/p65 heterodimer or 1 nM for the p50 and p65 homodimers) in 20 µl of binding
buffer (20 mM Tris (pH 8.0), 50 mM NaCl, 1 mM MgCl2, 1 mM dithiothreitol, 1 µg of poly(dI-dC) DNA, 0.25 mg/ml bovine serum albumin, and 5%
glycerol (v/v)) at 20 °C for 30 min. The reaction mixes were then
loaded onto a 6% 0.25× Tris borate-EDTA-polyacrylamide gel and run
for 2 h at 120 V. The gels were then dried and exposed to a
phosphorimage storage plate for a Molecular Dynamics Storm 860 scanner,
which was used to visualize the gels. Gels were quantified using
ImageQuant version 1.2 from Molecular Dynamics.
B target site from the HIV-LTR (underlined)
(5'-GATCGCTGGGGACTTTCCAGGGAGGCGTGGCCTGAGTCC-3') and a 17-mer containing the IFN-B site (underlined)
(5'-AGTGGGAAATTCCTCGG-3'). Both were annealed to
their complimentary strands prior to use. p50, p65, or the p50/p65
heterodimer were then serially diluted into 0.6-ml binding reactions.
After the dilutions, each tube was blanked and the labeled
oligonucleotides were added at constant concentration (100 pM, 1 nM, or 10 nM for p50/p65,
p50, and p65, respectively), and the reactions were incubated at
20 °C for 45 min to 1 h. For the monomeric p50 (Y267D/L269D),
reactions were set up using a hairpin oligonucleotide with the sequence
5'-AAAGTCCCCACCCCCTGGGGACTTT-3' containing the
p50 Ig-B half-site from the HIV-LTR (underlined) added to the
titrated protein at 1 nM. The anisotropy value of each
reaction tube was then measured using a Beacon 2000 fluorescence polarization analyzer (Panvera, WI). Buffers used in the assays were as
follows: Temperature Dependence, 20 mM Tris (pH 8.0), 50 mM NaCl; Salt Dependence, 20 mM Tris (pH 8.0),
and 0, 25, 50, 75, 100, 150, and 200 mM NaCl or KCl; pH
Dependence, 20 mM buffer (pH 6.0, 6.2, and 6.5 MES, pH 6.8 and 7.0 MOPS, pH 7.5, 8.0, and 8.5 Tris, and pH 9.0 CAPSO). All salt
and pH experiments were carried out at 37 °C; temperature dependence
assays were carried out at 4, 8, 16, 22, 30, 37, and 42 °C.
B saturated DNA. The apparent
dissociation constant (Kapp) was determined
graphically as the point where fraction bound equals 0.5. Data from all
homodimer experiments were globally fit to a cooperative binding model
using the following equation.
Kmonomer is the equilibrium dissociation
constant of one monomer interacting with its DNA half-site, and
a is a cooperativity factor for the binding of the second
monomer. The statistical factor of 2 in the denominator arises due to
the two equivalent monomer-binding sites available prior to the binding
of the first monomer.
![<UP>Fraction DNA bound </UP>(<UP>FB</UP>)=<FR><NU>([<UP>NF-&kgr;B</UP>]/K<SUB><UP>monomer</UP></SUB>)+([<UP>NF-&kgr;B</UP>]<SUP>2</SUP>/aK<SUP>2</SUP><SUB><UP>monomer</UP></SUB>)</NU><DE>1+(2[<UP>NF-&kgr;B</UP>]/K<SUB><UP>monomer</UP></SUB>)+([<UP>NF-&kgr;B</UP>]<SUP>2</SUP>/aK<SUP>2</SUP><SUB><UP>monomer</UP></SUB>)</DE></FR>](/content/vol275/issue32/fulltext/24392/img001.gif)
(Eq. 1)
Kmonomer(p65) is the affinity of the p65
monomer for its DNA half-site, Kmonomer(p50) is
the affinity of the p50 monomer for its DNA half-site, and a
is a cooperativity factor for the binding of the second monomer.
![<UP> FB</UP>=<FR><NU><AR><R><C>([<UP>NF-&kgr;B</UP>]/K<SUB><UP>monomer</UP>(<UP>p65</UP>)</SUB>+[<UP>NF-&kgr;B</UP>]/K<SUB><UP>monomer</UP>(<UP>p50</UP>)</SUB>)</C></R><R><C>+([<UP>NF-&kgr;B</UP>]<SUP>2</SUP>/aK<SUB><UP>monomer</UP>(<UP>p65</UP>)</SUB> K<SUB><UP>monomer</UP>(<UP>p50</UP>)</SUB>)</C></R></AR></NU><DE><AR><R><C>1+(2[<UP>NF-&kgr;B</UP>]/K<SUB><UP>monomer</UP>(<UP>p65</UP>)</SUB>+2[<UP>NF-&kgr;B</UP>]/K<SUB><UP>monomer</UP>(<UP>p50</UP>)</SUB>)</C></R><R><C>+([<UP>NF-&kgr;B</UP>]<SUP>2</SUP>/aK<SUB><UP>monomer</UP>(<UP>p65</UP>)</SUB> K<SUB><UP>monomer</UP>(<UP>p50</UP>)</SUB>)</C></R></AR></DE></FR>](/content/vol275/issue32/fulltext/24392/img002.gif)
(Eq. 2)
B binding.
K0 is the extrapolated apparent
Ka at 1 M NaCl concentration,
Z is the number of cations displaced, and
![<UP>log</UP>(K<SUB>a,<UP>app</UP></SUB>)=<UP>log</UP>(K<SUB>0</SUB>) Z*&psgr;*<UP>log</UP>[<UP>NaCl</UP>]](/content/vol275/issue32/fulltext/24392/img003.gif)
(Eq. 3)
is the number
of cations thermodynamically bound to each DNA backbone phosphate
previously determined to be 0.88 (13).
K0 is the same as in Equation 3, and
A is the total ion (cation and anion) stoichiometry
released. B is the number of H2O molecules
released upon binding. The equation is a simplified version of the
equation used by Ha et al. (14) from O'Brien et
al. (15).
![<UP>log</UP>(K<SUB>a,<UP>app</UP></SUB>)=<UP>log</UP>(K<SUB>0</SUB>)−A*<UP>log</UP>[<UP>NaCl</UP>]+B*0.016*[<UP>NaCl</UP>]](/content/vol275/issue32/fulltext/24392/img004.gif)
(Eq. 4)
RESULTS
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
B p50 Homodimers for B-DNA
Targets--
We used only the RHR portions of both p50 and p65
subunits for binding experiments. The RHR of p50 and p65 homodimers and the p50/p65 heterodimer have been overexpressed and purified from overexpressing E. coli clones. We have measured the DNA
binding of the p50 homodimer using a gel mobility shift assay. The DNA probe used for this assay was a 20-mer duplex DNA containing a centrally located 10-base pair Ig-B site. Fig.
1 shows the free and bound DNA for the
p50 homodimer, as well as the p65 homodimer and p50/p65 heterodimer.
The data fit best to a cooperative binding model (Equations 1 and 2)
describing two subunits assembling sequentially on the DNA. Fig.
2 shows the data for NF-B p50
homodimer binding to Ig-B DNA fit to the cooperative model.
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Fig. 1.
Sample electrophoretic mobility shift assays
of p50/p65 heterodimer, p50 homodimer, and p65 homodimers
(left to right). DNA concentration
was held constant in each lane and titrated with decreasing NF- B
concentrations. Arrows indicate the location of the NF-B
dimer-DNA complex and free duplex DNA.
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Fig. 2.
NF- B dimers bind DNA
cooperatively. Semi-logarithmic plot of sample DNA binding data
from an electrophoretic mobility shift assay with p50 homodimer. Data
points are represented as solid circles (
),
and the cooperative fit (Equation 1) is represented as a
solid line.
B p50 homodimer for Ig-B DNA was further
examined using fluorescence anisotropy assays. The binding conditions were similar to those for gel mobility shift assays. This
solution-based assay circumvents the problems of artifactual
dissociation of a protein-DNA complex as it migrates through a gel
matrix. Fig. 3 shows titrations of
Ig-B DNA with the three different NF-B dimers. The total
fluorescence intensity did not change during the assay, indicating that
anisotropy signals were not due to changes in fluorescence lifetime or
other experimental artifacts. To determine the time required for each
reaction to reach equilibrium anisotropy, a kinetic experiment was
performed in which each sample was measured at different times until no
change in anisotropy was observed. Accordingly, sufficient time
was allowed before recording the final anisotropy value. Control
experiments showed that the presence or absence of carrier DNA
poly(dI-dC) (2 µg/ml) and glycerol (5%) had no effect in
binding. Additionally, we have verified the activities of each protein
sample used for the assays by measuring anisotropy at various
stoichiometric protein-DNA ratios (over a range from 20/1 to 1/20). We
observe that approximately 85% of the NF-B in each preparation is
fully active (data not shown).
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Fig. 3.
The p50/p65 heterodimer binds DNA tighter
than either homodimer. Semi-logarithmic plot of concentration
(nM) of p50/p65, p50, and p65 versus fraction
DNA bound from fluorescence anisotropy data for representative data
sets. p50/p65 ( ) binds tightest, followed by p50 (
) and then p65
(
).
B site. These results are
presented in Table I. Our results show that the NF-B p50 homodimer has similar affinities for both Ig-B and IFN-B DNA targets.
NF-B binding to Ig-B and IFN-B DNA
B binding to Ig-B and IFN-B DNA
and from electrophoretic mobility shift experiments on Ig-B. Errors
for Kapp and Kmonomer values are
the standard deviation from the reported average of a minimum of three
independent experiments, except the Kmonomer value
for p65, which was derived from fitting to Equation 1 (see
"Experimental Procedures"). The cooperativity factors
(a) were also derived from global fits using Equation 1 for
p50 and p65 homodimer and Equation 2 for the p50/p65 heterodimer. As
such, the reported errors for these values are the standard errors of
the fits.
B half-site
target. The cooperative model predicts that the monomers bind
sequentially to their DNA half-sites, with the second monomer binding
to its half-site with much higher affinity due to its interaction with
the pre-bound first subunit. In order to test this hypothesis, we
created a monomeric mutant p50 using information from crystallographic
models and biochemical studies of the p50 homodimer (16, 17). The
tyrosine at position 267 and leucine at position 269 are critical for
subunit dimerization of p50. These residues are located away from the
protein-DNA interface and are not involved in DNA contacts. We have
created and purified the Tyr267 
Asp/Leu269
Asp double mutant to homogeneity. Size exclusion chromatography clearly shows that the mutant p50 is monomeric even at a high protein
concentration (5 mg/ml, Fig.
4A). Binding experiments have
been performed with a DNA probe that bears only a single half-site
(Fig. 4B). This eliminates any possible binding of two molecules of mutant p50 monomer in a non-cooperative manner. The p50
monomer binds to this target with an affinity of 210 nM
(Kmonomer). Using this value in Equation 1
yields a cooperativity factor of 0.050, suggesting that the second
subunit binds to the DNA with 20 times higher affinity compared with
the first monomer, 10.5 nM. The apparent equilibrium
constant (Kapp) for 2 monomers binding to DNA is
2.2 × 10
15 M2.
However, in the pH, salt, and temperature studies, we focus on the
overall Kapp, the concentration where half of
the DNA is bound, which represents the affinity of the entire NF-B
dimer-DNA complex.
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Fig. 4.
Dimerization is critical for cooperative DNA
binding. A, size exclusion chromatography traces of the
wild-type and Y267D/L239D p50 RHRs showing that the mutant is
monomeric, even at high protein concentration (5 mg/ml). B,
representative data sets comparing p50 RHR ( ) binding to p50
Y267D/L269D (
) on a semi-logarithmic plot of concentration
versus fraction DNA bound.
B p65 Homodimer for B-DNA
Targets--
We have performed analogous binding experiments with p65
homodimer for both Ig-B and IFN-B DNA targets (Table I). Binding with Ig-B DNA has been tested through both EMSA and polarization experiments at pH 8.0. EMSA experiments show that p65 homodimer binds
the DNA with an affinity of 464 nM and fluorescence
anisotropy gives a value of 341 nM. At pH 7.5 the p65
homodimer binds Ig-B more tightly, with an affinity of approximately
150 nM. We also observe that the binding affinity of p65
homodimer IFN-B DNA is similar to its affinity for Ig-B DNA (414 nM versus 341 nM at pH 8.0). The
nature of binding isotherms also suggests a cooperative mode of
binding. We therefore set out to determine the cooperativity of
interactions between p65 and B targets. We have created monomeric p65 by mutating Phe231 and Leu233 located at
the subunit interface to aspartic acid. These two residues are located
at the equivalent positions to that of Tyr267 and
Leu269, respectively, in p50. We overexpressed, purified,
and tested the oligomeric nature by size exclusion chromatography. As
expected, this double mutant was monomeric. However, the mutant tends
to aggregate, preventing us from using it in binding experiments. We
have overexpressed the monomeric DNA binding N-terminal domain of p65.
X-ray crystal structures show that this fragment provides most of the
sequence-specific binding of target DNA while lacking the phosphate
backbone contacts contributed by the dimerization domain. This fragment
binds a B half-site with an affinity of approximately 1,800 nM at pH 7.5. Considering this as the absolutely upper
limit, and the affinity of p50 RHR monomer, 210 nM, being the lower limit, we fit the Kmonomer and
a values in Equation 1, with Kmonomer
constrained to be less than 1,800 nM, to the p65 RHR data
at pH 7.5. This yielded a Kmonomer of 379 nM and a cooperativity value (a) of 0.16, suggesting that the second molecule of p65 monomer binds the second
half-site of DNA with 6-7-fold higher affinity.
B-DNA
Targets--
In addition to the homodimers, we have also extensively
studied the NF-B p50/p65 heterodimer. We have determined the
apparent binding affinities of the heterodimer for the Ig-B DNA
target using both gel mobility shift and fluorescence anisotropy
assays. Similar to the results observed for the homodimers, we do not see any difference in binding affinities between these two methods. The
Kapp values of the p50/p65 heterodimer for
Ig-B are approximately 20 nM at pH 8.0 in both assays.
We observe that the heterodimer binds to IFN-B with a relatively
lower affinity compared with its Ig-B targets. The apparent
dissociation constants of Ig-B and IFN-B for the heterodimer are
19 and 27 nM, respectively, at pH 8.0. Our results show
that the p50/p65 heterodimer has the highest affinity for Ig-B DNA,
p50 homodimer binds with intermediate affinity, whereas p65 shows the
lowest binding affinity.
B targets with highest cooperativity of the three dimers
tested here. Using the equilibrium binding constants of the p50 and p65
monomers to their DNA half-sites, we observe that the cooperativity of
the heterodimer is 0.0017 (the second subunit binds 500 times tighter
than the first) using Equation 2.
B DNA, we
performed binding experiments at pH 7.5 and 8.0 using fluorescence
anisotropy assay. These experiments showed approximately 2-fold higher
affinity at pH 7.5 than at pH 8.0. To observe if both the homodimers
also exhibit a similar binding trend, the homodimers were subjected to
similar experiments. The homodimers did not show a large difference in
affinities as was observed for the heterodimer. Nevertheless, both
these dimers did show slightly higher affinities at pH 7.5 compared
with pH 8.0. To further investigate the pH dependence of equilibrium
binding constants of the heterodimer-DNA complex, we tested a wider pH range. The apparent binding constants were determined for the heterodimer/Ig-B DNA complex at seven different pH values ranging from 6.0 to 9.0. At pH 6.0, no change in anisotropy was observed due to
background noise, but a change of intensity was recorded with increases
in protein concentration. Therefore, the binding constant was
determined from the plot of increase of fluorescence intensity
versus protein concentration. As shown in Fig.
5, apparent binding constants vary only
roughly 2-fold between pH 6.8 and 8.0, with the highest affinity is
observed at pH 7.0. Below pH 6.8 binding constants increase
significantly as pH decreases. Similarly, Kapp
increases as pH increases with a 5-6-fold increases of the binding
constant at pH 9.0, the highest pH used in the assay.
View larger version (7K):
[in a new window]
Fig. 5.
pH dependence profile of p50/p65. The
apparent dissociation constant (Kapp,
nM) was measured between pH 6.0 and 9.0, with the lowest
Kapp at pH 7.0. Error bars
represent one standard deviation from the average observed value from
three separate FAAs at each pH.
B DNA complex
on salt concentration was determined at pH 8.0 and 37 °C using the
anisotropy method. As shown in Table II, the Kapp of this complex is highly dependent on
the salt concentration. Kapp remained
unchanged between salt concentrations from 0 to 50 mM. Whereas Kapp is approximately 20 nM at 50 mM NaCl, it is reduced by a factor of
3-4 at 100 mM NaCl concentration. A reduction in
Kapp value of 2 orders of magnitude is observed
at 200 mM salt concentration. FAA experiments replacing
NaCl with KCl produced no observable changes in the apparent
equilibrium constants. The salt effect on the heterodimer/Ig-B DNA
complex is shown in a log-log plot of salt concentration
versus Kapp in Fig.
6. The plot fits Equations 3 and 4
relating equilibrium binding constants to ion-water models at NaCl
concentrations where binding is salt-dependent. Log
Kapp exhibits a linear dependence on log salt
concentrations from 75 to 200 mM. From the fit to these
data points, it appears that between 5 and 6 ions and approximately 430 water molecules are released upon the protein-DNA complex formation.
The release of large numbers of water molecules is a hallmark of
specific, protein-DNA complex formation (18). Similar strong salt
dependence of apparent equilibrium binding constants
(Kapp) on salt was also observed for the p50
homodimer/IFN-B DNA complex. Like the heterodimer/Ig-B DNA
complex, the binding constants do not change at salt concentrations between 0 and 50 mM. Above 75 mM NaCl
concentration, p50/IFN-B DNA complex is even more
salt-dependent than the heterodimer. The binding constant
is decreased over 200-fold at 200 mM salt compared with 50 mM salt concentration.
NaCl dependence of p50/p65 heterodimer binding to Ig-B DNA
View larger version (8K):
[in a new window]
Fig. 6.
DNA binding by p50/p65 is strongly
salt-dependent. Log of average apparent association
constants (M 1) is plotted
versus log NaCl concentration. Log 0, 25, and 50 mM NaCl are open symbols, and Log 75, 100, 150, and 200 mM NaCl are solid
symbols. The error bars represent one
standard deviation from the average observed value. The curve was the
fit of the NaCl-dependent data points (75 mM
NaCl and above, solid points) to determine the
number of cations and H2O molecules released upon binding,
6 and 426, respectively.
B DNA complex. The binding constants were
measured at seven different temperatures ranging from 4 °C to
42 °C. The results are shown in a plot of
ln(Kapp) versus temperature (Fig.
7). We do not observe any temperature
dependence of apparent binding constants.
View larger version (8K):
[in a new window]
Fig. 7.
p50/p65's binding to DNA is
temperature-independent. The average of the natural log of
Kapp (in M) is plotted
versus temperature (from 4 °C to 42 °C), with
error bars representing one standard deviation
from the average of measured values. The change in temperature has no
observable effect on the binding constant of p50/p65.
DISCUSSION
TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
REFERENCES
B dimers have been determined.
These structures have provided a wealth of information regarding how
these closely related dimers make contacts with their DNA targets. In
order to understand how NF-B dimers actually recognize DNA, an
energetic profile of NF-B-DNA interactions is essential. In this
study, we have determined relative binding affinities of three NF-B
dimers, p50 and p65 homodimers and p50/p65 heterodimer, for two
different physiological targets. We have also investigated the effects
of monovalent salt concentration, pH, and temperature on DNA binding by
the p50/p65 heterodimer.
B-DNA complexes tested: p50/p65-DNA, p50 homodimer-DNA, and p65 homodimer-DNA complexes. The nature of the binding isotherms indicates a cooperative mode of binding. The source of cooperation is likely to be the stepwise
binding of NF-B monomers to DNA half-sites, followed by subunit
association through the dimerization domains of each protein subunit.
Indeed, our thorough investigation of binding by p50 to Ig-B DNA
clearly suggests that the dimer recognizes the target in a highly
cooperative manner. Our results also show that the major source of the
cooperativity is indeed the dimerization interactions between the two
p50 subunits. Although we could not perform the similar experiment with
p65 due to the aggregation problem of monomeric p65 RHR, binding
affinity of p65 monomer was estimated to fall between the DNA binding
affinity of the N-terminal domain p65 and affinity of monomeric p50
RHR. A binding affinity for p65 monomer for B DNA of 379 nM is a good estimate for two reasons. First, this value
fits our data best (lowest standard errors). Second, this value is
roughly 2-fold lower than the p50 Kmonomer,
which is expected, because of extra DNA base contacts made by the p50
monomer. Using these Kmonomer values for p50 and
p65 in a cooperative model for heterodimer binding gives a
cooperativity factor of 0.0017. This suggests that the heterodimer
binds the DNA much more cooperatively than either of the homodimers.
Nevertheless, the apparent equilibrium binding constants provide the
true affinity of the NF-B dimer-DNA complexes. The apparent
dissociation constants obtained from our experiments are somewhat
higher than previous reports (19-23). Although we cannot explain the
source of discrepancies, it is important to note that different binding
reaction conditions may influence the relative affinity values.
B-DNA
complexes, several important conclusions can be drawn. These complexes
approximately bury 3000-3800 Å2 solvent-exposed surface
area; the dimers make 12-14 direct base-specific hydrogen bonds with
their DNA target and 25-40 nonspecific hydrogen bonding contacts with
the backbone of DNA targets (11). None of these numbers are unusual
when compared with other complexes of dimeric transcription factor-DNA
complexes. Whereas no direct relationship exists between number of
contacts between two complex forming macromolecules and the affinity of
such a complex, it is not unusual that NF-B binds DNA with nanomolar
affinity like most other eukaryotic transcription factors.
Incidentally, NFAT, a NF-B-related transcription factor, is known to
bind DNA with much lower affinity. The N-terminal specificity domain of
NFAT is structurally very similar to the N-terminal domain of NF-B and recognizes specific bases in almost identical manner to that of
NF-B (24).
B heterodimer
was determined as a function of pH. The apparent binding constants of
the heterodimer/Ig-B complex were measured at eight different pH
values ranging from pH 6.0 to 9.0, using appropriate buffers. As
presented in Fig. 5, the interaction of protein with DNA is optimal
between pH 6.8 and 7.5. The affinity decreases below and above this pH
range. However, the affinity decreases more dramatically at low pH. It is likely that partial protonation of certain residues such as Glu39 of p65 and Glu60 and His64 of
p50 that are directly involved in DNA contacts are responsible for this
effect. Conversely, deprotonation of DNA backbone contacting residues,
Tyr36 and Cys38 of p65 and the corresponding
Tyr57 and Cys59 of p50 reduce the affinity of
protein for the DNA. Studies on the dimerization affinity of the p50
homodimer show no pH effects on dimer stability over the range of pH
values used in these assays (16). Thus, the pH dependence of affinity
is due to alterations of the amino acid residues that contribute
directly to the NF-B-DNA interface.
B p50/p65 heterodimer binds
Ig-B DNA in a highly salt-dependent manner. Although no
change in the binding constant is observed at NaCl concentrations
between 0 and 50 mM, an increase of only 100 mM
NaCl reduces the affinity by more than an order of magnitude. At 200 mM NaCl, the heterodimer binds Ig-B practically nonspecifically. Similar strong effects of salt on p50 homodimer binding to IFN-B DNA suggests that all NF-B-DNA complexes are formed in a salt-dependent manner. Additionally, the
formation of p50 dimers in the absence of DNA is not affected by the
salt concentrations used here (16).
B-DNA is likely to come from nonspecific
salt bridges between the DNA phosphate backbone and positively charged
protein side chains. There are at least 20 such contacts observed
between the heterodimer and Ig-B DNA complex (11). Additionally,
from NMR and molecular modeling studies of the HIV-LTR Ig-B DNA, it
appears that the dynamics of the phosphate backbone's conformation in
the 5' and 3' regions of the B sequence play an active role in
NF-B recognition (25). Cooperative interactions with other
transcription factors may provide the higher level of specificity at
physiological salt concentrations, which is approximately 175 mM.
B also eluted from the oligonucleotide columns at much lower salt
concentrations than other DNA-binding proteins (0.2 and 0.4 M, respectively) (26). Our data predict this weak binding
at the salt concentrations used and the low protein concentration of
this initial purification. At this point it is still unclear why
NF-B's DNA binding behavior at low salt concentrations (0-50
mM) differs from that higher concentrations.
B DNA by NF-B p50/p65 heterodimer is an entropic
process driven by the release of counterion and bound waters. This is
not surprising for two reasons. First, release of a large number of
water molecules clearly favors entropy of binding. Second,
crystallographic analysis of various NF-B-DNA complexes reveals that
several DNA contacting amino acid side chains are most likely
pre-organized through interactions with each other. In fact, the
structures of the dimerization domains of the p50 and p65 homodimers
show that the DNA backbone contacting residues contributed by the
dimerization domain adopt similar conformations in the unbound form as
those found in their respective homodimer-DNA complexes (17). These
observations suggest that the ordering of amino acid side chains, and
the resulting loss of entropy, are minimal in the forming of
NF-B-DNA complexes.
B-DNA complexes have
given a strong foundation upon which to initiate thermodynamic studies
of these complexes. In this report we have shown qualitatively the
relative binding behaviors of three NF-B dimers, p50, p65, and
p50/p65, with two different DNA targets. We have further investigated the role of pH, monovalent salt, and temperature on the ability of the
p50/p65 heterodimer to recognize Ig-B DNA. More detailed analyses
are essential to determine the thermodynamic parameters of binding in
more quantitative terms.
ACKNOWLEDGEMENTS
FOOTNOTES
Supported by University of California San Diego Cellular and
Molecular Genetics Training Grant 2-T32-GM07240-24.
ABBREVIATIONS
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TOP
ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS
DISCUSSION
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