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Molecular and Cellular Biology, September 2002, p. 6321-6335, Vol. 22, No. 18
0270-7306/02/$04.00+0     DOI: 10.1128/MCB.22.18.6321-6335.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.

MINIREVIEW

Classification of Human B-ZIP Proteins Based on Dimerization Properties

Charles Vinson,^* Max Myakishev, Asha Acharya, Alain A. Mir, Jonathan R. Moll, and Maria Bonovich

Laboratory of Metabolism, National Cancer Institute, National Institutes of Health, Bethesda, Maryland 20892

B-ZIP transcription factors (98) are exclusively eukaryotic proteins that bind to sequence-specific double-stranded DNA as homodimers or heterodimers to either activate or repress gene transcription (34). We have examined both of the recently published DNA sequences of the human genome (51, 95) and identified 56 genes that contain the B-ZIP motif. Three sequences were identical, giving a total of 53 unique B-ZIP domains with the potential to form 2,809 dimers. This creates the possibility for a tremendous range of transcriptional control (23, 50, 52). While significant effort has been directed at identifying dimerization partners of B-ZIP proteins, the full complement of dimerization partners remains to be elucidated. This review highlights two topics: (i) the known structural rules that regulate leucine zipper dimerization specificity and (ii) experimental data addressing mammalian B-ZIP dimerization partners.

We have annotated the leucine zippers of all human B-ZIP domains, highlighting amino acids in the a, d, e, and g positions that appear critical for leucine zipper dimerization specificity. These data were used to group B-ZIP proteins into 12 families with similar dimerization properties: (i) those that strongly favor homodimerization within the family (PAR, CREB, Oasis, and ATF6), (ii) those that have the ability to both homodimerize and heterodimerize with similar affinities (C/EBP, ATF4, ATF2, JUN, and the small MAFs), and (iii) those that favor heterodimerization with other families (FOS, CNC, and large MAFs).

BACKGROUND

In the late 1980s, several mammalian B-ZIP proteins were purified by double-stranded DNA affinity chromatography, and the genes encoding these proteins were cloned. Among the first cloned were the AP-1 (c-FOS and c-JUN) heterodimer, (4), the CREB homodimer (65), and the C/EBP homodimer (37, 53). These newly isolated genes were used as probes in low-stringency DNA hybridizations to identify new sequence-related B-ZIP proteins (5, 78, 101). In addition, new B-ZIP proteins (25, 36, 102) were isolated by screening lambda phage protein expression libraries with radiolabeled DNA binding elements (29, 85, 97). These functional DNA binding assays successfully isolated B-ZIP proteins because the B-ZIP motif is compact and refolds easily (87). The wealth of new sequences led to a confusing nomenclature, because multiple groups independently isolated and named the same B-ZIP proteins. Moreover, initial classification into families was often based on apparent DNA binding activity, resulting in grouping of proteins with different dimerization properties. Several reviews have helped clarify these issues, including a comprehensive review by Hurst in 1995 (34), one focusing on ATF proteins (24), and another focusing on FOS and JUN proteins (6). We hope this review will further contribute to a systematic B-ZIP classification.

B-ZIP STRUCTURE

Amino acid alignment of B-ZIP proteins allowed the identification of the B-ZIP motif, a long bipartite -helix that is 60 to 80 amino acids long (98). The N-terminal half contains two clusters of basic amino acids responsible for sequence-specific DNA binding, while the C-terminal half contains an amphipathic protein sequence of variable length with a leucine every seven amino acids. The shorter leucine zippers have less protein sequence flexibility, because amino acids must be optimized for dimerization stability. Longer leucine zippers allow better regulation of dimerization specificity, because they can contain amino acids that are suboptimal for stability but favor interaction with a particular partner. This amphipathic sequence, termed the "leucine zipper" (52), mediates homo- and heterodimerization of B-ZIP proteins (3, 20, 41, 44, 54, 77, 86, 91). Figure 1 shows the X-ray crystal structure of the B-ZIP domain from yeast GCN4 bound to DNA (15). B-ZIP DNA binding stabilizes the basic region inducing the random coil to form an -helical extension of the leucine zipper (73, 84). Several B-ZIP proteins, including the small and large MAF proteins (13, 42), contain additional DNA binding elements N terminal to the basic region that increase the number of specific DNA bases that can be bound.

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FIG. 1. X-ray structure of the yeast B-ZIP homodimer, GCN4 (blue -helices) bound to DNA (red helices). The N-terminal DNA recognition helix lies in the major groove of the DNA. An almost invariant leucine present every two turns of the C-terminal -helix (at the d position) is shown in gray.

The leucine zipper dimerization domain forms a parallel coiled coil (75) that consists of four to five heptads, in which each heptad is composed of two -helical turns or seven amino acids, labeled a, b, c, d, e, f, and g (61). Amino acids in the a, d, e, and g positions regulate leucine zipper oligomerization, dimerization stability, and dimerization specificity.

Amino acids in the a and d positions are on the same surface of the -helix and are typically hydrophobic. The a and d amino acids from one monomer interact with the complementary a' and d' amino acid positions in the opposite monomer (' refers to the second -helix in the dimer). This interaction creates a hydrophobic core essential for dimer stability (87). The g and e positions typically contain charged amino acids (8, 96). X-ray crystallography reveals ge' interhelical interactions between amino acids in the g position and oppositely charged amino acids in the e', which is five amino acids C terminal (2, 15, 19, 21, 75, 80). Electrostatic interactions between the amino acids in the ge' pair can be either attractive or repulsive and thus can regulate both homodimerization and heterodimerization. Furthermore, Van der Waal interactions between the g and e' methylene groups and the underlying a and d amino acids contribute to stability (2).

LIST OF ALL HUMAN B-ZIP PROTEINS GROUPED BY DIMERIZATION PROPERTIES

We have examined two versions of the DNA sequence of the human genome (51, 95) and identified 56 genes that contain the B-ZIP motif. Three of these motifs were identical, resulting in 53 unique B-ZIP domains. Four of the proteins were found only in the Celera database. Table 1 provides the chromosomal location, unique database search identifiers, and the number of amino acids found N terminal and C terminal of the B-ZIP domain. We have generated three dendrograms that examine the relatedness of the amino acid sequences of the 53 human B-ZIP domains. One dendrogram is based on the entire B-ZIP domain, one is based on the basic region that is critical for DNA binding, and the last is based on the leucine zipper region that regulates dimerization specificity (Fig. 2). The three dendrograms are similar. The differences are interesting, because they reveal whether similarities are based on DNA binding properties or dimerization specificities. For example, the basic region dendrogram places the CREB, ATF6, and Oasis families together, reflecting their binding to the CRE DNA sequence (5'-TGACGTCA-3'). In contrast, the leucine zipper dendrogram places the Oasis family separately from the CREB and ATF6 families, reflecting their different dimerization properties. It is possible that these families could compete for binding to the CRE DNA sequence to give a range of transcriptional control. Another example is the XBP protein, which is not related to any sequence when its basic region is examined, but clusters with the ATF6 proteins when its leucine zipper is examined.

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TABLE 1. Human B-ZIP proteinsaa

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FIG. 2. Dendrogram of 53 human B-ZIP proteins. Phylogenetic trees were generated by Align X module of Vector NTI, 7.0 with default parameters. (A) Alignment based on the entire B-ZIP domain. (B) Alignment based on the basic region. (C) Alignment based on the leucine zipper defined from the first leucine shown in the consensus on Fig. 3.

To achieve a functional classification of the B-ZIP proteins, we have considered the dimerization properties of the B-ZIP domains. We have examined the amino acids in the g, a, d, and e positions of the leucine zipper region of the B-ZIP domains to rationalize the known and predict the unknown dimerization properties of the 53 human B-ZIP domains whose amino acid sequences are presented in Fig. 3. Using this analysis, we have grouped B-ZIP proteins with similar dimerization properties into 12 families. Our grouping is consistent with the dendrograms and agrees particularly with the dendrogram based on the leucine zipper sequence. An examination of the human genome by Green and colleagues (90) grouped B-ZIP proteins into eight previously identified families, (PAR, CREB, C/EBP, FOS, JUN, Maf, CNC, and ATF6) based on amino acid similarity throughout the B-ZIP domain. Our analysis divides their FOS family into FOS, ATF2, and ATF4; the MAF family into the small MAFs and large MAFs; and the CREB family into the CREB and Oasis families. We also reassigned two sequences, XBP1 was moved from the FOS family to the ATF6 family, and NFLI3 was moved from the C/EBP to the PAR family.

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FIG. 3. Amino acid sequence of all 53 human B-ZIP domains. Proteins are placed in to 12 groups based on predicted dimerization properties. We have placed the well-studied yeast B-ZIP protein GCN4 at the bottom of the figure for reference. The natural C terminus is denoted with an asterisk. Leucine zipper heptads are grouped (gabcdef) to help visualize potential ge' pairs. If both the g and e positions contain charged amino acids, we have colored the gabcde amino acids. Our description of "attractive" and "repulsive" refers to pairs that would be present in the homodimer. We use the four colors to describe the ge' pairs. Green is for the attractive basic-acidic pairs (RE and KE), orange is for the attractive acidic-basic pairs (ER, EK, DR, and DK), red is for the repulsive acidic pairs (EE, ED, EQ, and QE), and blue is for the repulsive basic pairs (KK, RK, QK, RQ, and KQ (Table 3). If only one of the two amino acids in the ge' pair is charged, we color only that amino acid: red if it is acidic and blue if it is basic. If the a or d positions contain polar or charged amino acids, they are colored black.

We divide these 12 families into three general groups: (i) those that strongly favor homodimerization within the family (PAR, CREB, Oasis, and ATF6), (ii) those that homodimerize and heterodimerize (C/EBP, ATF4, ATF2, JUN, and the small MAFs), and (iii) those that strongly favor heterodimerization with other families (FOS, CNC, and large MAFs). Amino acids in the leucine zipper region of each human B-ZIP domain that regulate attractive and repulsive interactions are color-coded in Fig. 3 and reveal similar interaction patterns within each family. Figure 4 presents a helical wheel representation of homo- and heterodimers to help explain the color code used in Fig. 3. A similar annotation for Drosophila B-ZIP proteins indicates that the 12 families we have identified are conserved in the insects (17).

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FIG. 4. Schematic of leucine zipper dimerization according to the color code used in Fig. 3. End view of a coiled coil with the seven unique positions of the heptad presented as ellipses, looking from the N terminus to the C terminus. The a and d positions are colored black. Three possible combinations of acidic and basic amino acids in the g and e positions are presented and color-coded as in Fig. 3. (Top panel) A coiled coil with a ge' pair containing an acidic amino acid in the g position and a basic amino acid in the following e position (orange in Fig. 3) can form a homo- or heterodimer with a similarly charged -helix. (Middle panel) An -helix with a ge' pair containing a basic amino acid in the g position and an acidic amino acid in the following e position (green in Fig. 3) can form a homo- or heterodimer with a similarly charged -helix. (Bottom panel) A heterodimer between an acidic ge' pair (red in Fig. 3) and a basic ge' pair (blue in Fig. 3).

An examination of the ge' pairs in the first four heptads of human B-ZIP proteins results in several general observations. Thirty percent are attractive, with acidic-basic pairs (orange) predominating; 23% are repulsive with acidic-acidic (red) pairs predominating; and 30% contain a single charged amino acid that can stabilize either homodimerization or heterodimerization.

The d position of the hydrophobic interface typically contains leucine with very few polar and no charged amino acids. The 2nd heptad a position typically contains asparagine. The a position in other heptads typically contains hydrophobic amino acids, but asparagine and basic amino acids are occasionally observed, which are critical for regulating dimerization specificity. The surprisingly limited diversity of amino acids in the a, d, e, and g positions suggests that a limited set of rules might regulate leucine zipper dimerization specificity.

STRUCTURAL RULES REGULATING DIMERIZATION SPECIFICITY

In this section, we will review what is known about the contribution of individual amino acids to leucine zipper dimerization specificity and apply these rules to all human B-ZIP proteins. B-ZIP dimerization stability can be measured by circular dichroism spectroscopy (CD). Ellipticity at 222 nm indicates the presence of -helical structure, and ellipticity decreases as the B-ZIP structure is unfolded by denaturants such as heat or urea. Thermal- or denaturant-induced unfolding of B-ZIP dimers occurs cooperatively and reversibly from an -helical dimer to an unfolded monomer. The homodimerizing B-ZIP domains typically have a melting temperature (T_m [midpoint of thermal transition]) of approximately 50°C, which represents 10 kcal/mol/dimer or 100 nM affinity at 37°C (1, 48, 49). The thermal denaturation is well described by a two-state model so that mutational analysis of specific amino acids allows their contribution to dimerization stability to be measured (47, 87).

The g and e positions.

Seventy-six percent of the g and e positions in the leucine zipper of human B-ZIP proteins contain one of four long-side-chain amino acids: the acidic glutamic acid (E), the basic arginine (R) or lysine (K), or the polar glutamine (Q) (2, 8, 74, 96). Changing the g and e positions in two heptads of the PAR B-ZIP domain from charged amino acids to alanine resulted in the formation of tetramers instead of dimers (48)[]. Thus, charged amino acids in the g and e positions inhibit the higher-order oligomerization that would occur if the g and e positions formed a continuous hydrophobic surface with the a and d positions.

Charged amino acids in the g and e positions contribute to leucine zipper stability. The most common ge' pair has glutamic acid (E) in the g position and an oppositely charged arginine (R) or lysine (K) in the following e' position (ER and EK). These oppositely charged amino acids produce a ge' pair that contributes -1.3 (ER) or -0.9 (EK) kcal/mol/pair more energy to dimer stability than a reference alanine pair (AA) (47). The ge' pairs RR and KK are stabilizing, contributing -0.1 and -0.3 kcal/mol/pair, respectively, relative to the AA pair. Presumably the repulsive electrostatic energies between the like charges in arginine or lysine pairs are overcome by the favorable Van der Waals interactions between the methylenes of arginine or lysine side chains and hydrophobic amino acids in the a and d positions (2). EE is the only pair less stable than AA, contributing +0.4 kcal/mol/pair.

In addition to affecting stability, charged amino acids in the g and e positions also regulate dimerization specificity (2, 3, 48, 57, 67, 74, 96, 104). In the analysis of stability presented above, we considered the stability of a charged ge' pair relative to an AA pair without addressing any potential energetic interaction between the amino acids in the ge' pair; the contribution of the individual E or R side chain to stability can be determined by examining the EA and AR pairs. Any excess stability conferred by the ER pair is due to the energetic interaction between E and R, termed the "coupling energy." This can be calculated by using a double-mutant thermodynamic cycle (31, 81) that involves the analysis of four proteins. This idea is presented graphically in Fig. 5. For example, the coupling energy of the ER pair is derived from a comparison of a protein containing the ER pairs with three additional proteins mutated to contain the pairs AR, EA, and AA (47). The levels of stability of the pairs relative to AA are as follows: ER, -1.3 kcal/mol; EA, -0.1 kcal/mol; and AR, -0.7 kcal/mol. The additional energy of the ER pair compared to the AR and EA pairs is -0.5 kcal/mol/salt-bridge [ER - (AR + EA) = coupling energy] [-1.3 - (-0.7 + -0.1) = -0.5] and represents the energy of interaction (coupling energy) between E and R. Table 2 lists the stability of each ge' pair relative to AA, and Table 3 gives their coupling energy.

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FIG. 5. Schematic describing the four proteins used for a double-mutant thermodynamic cycle. The top panel depicts two alanines in the g and e' positions of a ge'. The second panel shows that an EA pair is 0.1 kcal/mol more stable than an AA pair. The third panel shows that a AR pair is 0.7 kcal/mol more stable than an AA pair. The fourth panel shows a ER pair. Instead of being 0.8 kcal/mol more stable than AA, as would be expected if the two amino acids did not interact, ER is 1.3 kcal/mol more stable. The additional 0.5 kcal/mol is described as the coupling energy indicative of an physical interaction between the E and R side chains.

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TABLE 2. Thermodynamic differences for ge' pairs relative to AA (GAA in kcal mol-1/pair) a

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TABLE 3. Coupling energy of interaction for ge' pairs (Gint in kcal mol-1/pair) a

The larger coupling energy for the ER pair (-0.5 kcal/mol) than that of the EK pair (-0.3 kcal/mol) indicates that the ER pair contributes more to dimerization specificity than EK. The like-charged EE, KK, and RR pairs all have destabilizing coupling energies (+0.7, +0.6, and +0.8 kcal/mol, respectively) that are larger than the ER and EK attractive coupling energies (Table 3). This suggests that preventing a repulsive ge' pair is more important for driving dimerization specificity than forming an attractive pair. The energetic basis of the coupling energy for ge' pairs is a subject of ongoing debate in the literature (47, 56, 59), with some studies suggesting the measured coupling energy does not have a strong electrostatic component.

The suggestion that coupling energy may not be driven by charge interactions is highlighted by the polar glutamine that has a repulsive coupling energy in pairs with either acidic E or basic K (Table 3). Because of the positive calculated coupling energies, we have color-coded EQ and QE pairs in red as depicting repulsive acidic pairs and KQ, RQ, and QK in blue as depicting repulsive basic pairs (Fig. 3).

Many B-ZIP families, including JUN, CNC, and C/EBP, have only one charged amino acid in the ge' pair. These charged amino acids contribute to the stability of the homodimer, as seen in the AR and EA pairs in the double-mutant thermodynamic analysis. Heterodimers, however, may be preferred if they form an attractive ge pair, because of the coupling energy. Thus, incomplete ge' pairs can stabilize both homodimer and heterodimeric interactions.

The a and d positions.

Amino acids in the a and d positions of the leucine zipper are typically hydrophobic, with a variety of amino acids in the a positions and leucine in 84% of the d positions. An exception is the 2nd heptad a position, which contains asparagine in most homodimerizing B-ZIP proteins. The a and d amino acids are packed in the "holes and knobs" pattern predicted by Crick in 1953 (10), which is essential for leucine zipper dimer stability (87). When the GCN4 leucine zipper a and d positions were changed from valine and leucine to other aliphatic residues, trimers and tetramers formed (26). Similar to the role of amino acids in the e and g positions, amino acids in the a and d positions function to prevent higher-order oligomerization.

Several groups have examined the contribution of amino acids in the a and d positions to leucine zipper stability (63, 88). Leucine in the 4th d position is 9.2 kcal/mol/dimer more stable than alanine and 5.9 kcal/mol/dimer more stable than isoleucine. The additional stability conferred by leucine relative to isoleucine, an amino acid of similar size, likely results from the unique packing interactions of the two leucines with each other and with neighboring amino acids (63). The preferential energetic contribution of leucine over other aliphatic amino acids is not observed in the a position (99, 105; Vinson laboratory, unpublished data).

In addition to ge' pairs, amino acids in the a position can also regulate dimerization specificity. The asparagine side chains, which are common in the 2nd heptad a position (Fig. 3), interact interhelically to form a polar pocket in the hydrophobic interface that limits oligomerization and directs the orientation of the -helices (69). Hu and coworkers (103) mutated various a position asparagines to isoleucine and found that the asparagine-containing molecules interact preferentially with each other; thus, asparagine a position interactions are important for homodimerization specificity. In contrast, the basic amino acids lysine and arginine in the a position result in repulsive interactions that destabilize homodimerization and thus favor heterodimerization.

Coupling energies for the ge' pair can be measured in the context of a homodimerizing system because the g and e positions in the monomer (and thus the g and e' positions in the dimer) can be changed independently. In contrast, changing a and a' or d and d' independently requires a heterodimerizing system. The contribution of the d position to heterodimer formation remains to be examined. However, the prevalence of leucine in the d position in mammalian B-ZIPs suggests that this position contributes to stability rather than to specificity. The a position in contrast is more variable than the d position, suggesting this position may be important for regulating dimerization specificity.

We used a heterodimerizing leucine zipper system to determine the contribution of alanine, leucine, isoleucine, valine, asparagine, and lysine in the a position to dimerization specificity. Pairs comprising any combination of the three aliphatic amino acids leucine, isoleucine, and valine have similar coupling energies. Asparagine in contrast, prefers to interact with itself and not with the aliphatic amino acids. The NN and VV interactions are more stable than the NV interactions by 2.3 and 5.3 kcal/mol, respectively. Therefore, asparagine drives interactions with asparagine in the a position. Asparagines in the a position of the 4th heptads of the Oasis family and the 3rd and 5th heptads of the ATF6 families appears to be critical for their predicted homodimerization. In contrast, KK interactions in the a position are repulsive, so that lysine preferentially interacts with asparagine and the aliphatic amino acids (Vinson laboratory, unpublished data). The FOS, CNC, large MAF, and small MAF B-ZIP families use basic amino acids in the a position to create heterodimerizing B-ZIP families

REPULSION BETWEEN LEUCINE ZIPPERS: USING A-ZIP DOMINANT NEGATIVES

A problem with analyzing leucine zipper interactions by CD spectroscopy is that the stability of heterodimers can only be measured if the heterodimer is significantly more stable than either homodimer. To gain further insights into dimerization specificity, we have developed an A-ZIP protein consisting of a leucine zipper and a designed amphipathic acidic -helical sequence that replaces the B-ZIP basic region (Fig. 6). This acidic extension forms a coiled-coil structure with the basic region in the B-ZIP|A-ZIP heterodimer and stabilizes the complex by up to 8 kcal/mol (1, 22, 49, 64, 71). The B-ZIP|A-ZIP heterodimer drives interactions between weakly attractive or even somewhat repulsive leucine zippers and gives us access to measuring a range of dimerization affinities. This is important because in vivo dimerization is often driven by DNA binding. The B-ZIP|A-ZIP heterodimer is more stable than the B-ZIP protein bound to DNA, so that the A-ZIPs specifically prevent B-ZIP DNA binding at equimolar concentrations. Because the acidic extension interacts with all basic regions, the specificity of interaction between A-ZIP and B-ZIP domains is primarily leucine zipper dependent (1, 22, 64, 70). The inhibition of DNA binding provides an assay for dimerization.

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FIG. 6. Schematic of the A-ZIP dominant negative. (A) A model of a B-ZIP dimer with the basic region (blue) unstructured. (B) A B-ZIP dimer bound to DNA with the basic region now -helical. (C) A B-ZIP|A-ZIP heterodimer with the protein-protein interface extending N terminally into the basic region. The basic region (blue) and the designed acidic amphipathic region (red) interact as -helices to extend the coiled-coil domain.

Competition between A-ZIP protein and DNA for interaction with a B-ZIP protein can be analyzed with the gel shift assay. Figure 6 shows the FOS|JUND heterodimer and the C/EBP, CREB, and PAR homodimers binding to their canonical DNA binding sites. One molar equivalent of A-PAR inhibits the DNA binding of PAR; it does not inhibit the DNA binding of FOS|JUND, C/EBP, or CREB, even at 100 molar equivalences (Fig. 7, top panel). Similarly, 1 molar equivalent of A-CREB, A-C/EBP, and A-FOS specifically inhibit the DNA binding of CREB, C/EBP, and FOS|JUND, respectively. In contrast, A-ATF4 has somewhat promiscuous dimerization properties, inhibiting the DNA binding of FOS|JUND and C/EBP at 1 molar equivalent (Fig. 7E).

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FIG. 7. B-ZIP DNA binding is inhibited by specific A-ZIP dominant negatives. Four B-ZIP dimers, the PAR, CREB, and C/EBP homodimers, and the FOS|JUND heterodimer are bound to a 28-bp DNA containing the optimal binding site for each B-ZIP dimer. One, 10, or 100 molar equivalents of the A-ZIP is added to the B-ZIP before addition of DNA, and the solution is electrophoresed with an electrophoretic mobility shift assay. The sequence of the 28-mer DNA probes is shown below with the consensus binding sites underlined: GTCAGTCAGAATGACTCATATCGGTCAG (AP-1), GTCAGTCAGATGACGTCATATCGGTCAG (CREB), GTCAGTCAGATTACGTAATATCGGTCAG (VBP), and GTCAGTCAGATTGCGCAATATCGGTCAG (C/EBP).

We can rationalize the specificity seen in Fig. 7 based on the leucine zipper sequence of each protein. The homodimerizing PAR, CREB, and C/EBP families have similar a and d positions with an asparagine in the a position of the 2nd heptad. The families differ in their attractive ge' pairs, PAR has four attractive ge' pairs, while CREB and C/EBP each have two attractive ge' pairs that are subsets of the PAR pattern. Dimerization between PAR and CREB or PAR and C/EBP is prevented, because PAR preferentially homodimerizes due to the 4.0-kcal/mol/dimer of coupling energy from the eight attractive ge' pairs in the four heptads. Therefore, CREB or C/EBP remain to homodimerize. C/EBP and CREB do not interact because their ge' pairs are in different heptads. To test the validity of this idea, we mutated only three amino acids in the g and e positions of the C/EBP leucine zipper to confer the PAR pattern of ge' pairs. The mutated C/EBP displays dimerization properties similar to those of PAR (64).

THE 13 B-ZIP FAMILIES

We can predict dimerization partners from Fig. 3 by using the following strategy. Heptads that interact to produce attractive ge' pairs and drive dimerization are green-green, orange-orange, red-blue, and blue-red. Heptads that interact to give repulsive ge' pairs and discourage dimerization are green-orange, orange-green, red-red, or blue-blue. As noted previously, biophysical measurements show that repulsive ge' pairs are more important than attractive ge' pairs in driving dimerization specificity. The a and d positions that affect dimerization are colored black. Asparagine in the a position will preferentially dimerize with another a position asparagine, while basic amino acids in the a position repel each other and thus drive heterodimerization. It should be appreciated that these rules are an oversimplification! We expect more detailed work will show more interactions that are critical for mediating dimerization specificity.

In the following section, we describe the known dimerization properties of each B-ZIP family and rationalize these properties based on the leucine zipper amino acid sequences.

The homodimerizing B-ZIP families. The homodimerizing B-ZIP families are PAR, CREB, Oasis, and ATF6. Homodimerizing leucine zippers have two defining properties. First, each B-ZIP family has a distinct pattern of attractive ge' pairs. Second, all have asparagine in the a position of the 2nd heptad. The Oasis family has an additional a position asparagine in the 4th heptad, while the ATF6 family has two additional a position asparagines in the 3rd and 5th heptads that help prevent heterodimerization with other B-ZIP proteins.

(i) PAR family.

The PAR family, named for a conserved proline- and acid-rich domain N terminal of the basic region (14), consists of four family members, TEF/VBP, HLF, DBP, and the more distant NFIL3. PAR family members dimerize within the family (14, 33), but not with C/EBP family members (36). The dimers bind the palindromic DNA consensus sequence (5'-ATTACGTAAT-3'), which differs from the CREB binding site by 1 bp per half-site. We view PAR with its four attractive ge' pairs as the canonical homodimerizing leucine zipper. The 1st heptad contains an RE pair (green), and the 2nd, 3rd, and 4th heptads contain ER or EK pairs (orange). The a and d positions contain aliphatic amino acids, except for an asparagine in the 2nd a position. The attractive ge' pairs and the absence of destabilizing a and d amino acids suggest that these proteins will homodimerize.

(ii) CREB family.

The CREB family, which has one of the shortest leucine zippers, contains three members ATF1, CREM, and CREB. ICRE is an alternative splice product of the CREB gene. These proteins form dimers within the family (11, 12, 60). CREB homodimers bind the palindromic DNA consensus sequence 5'-TGACGTCA-3', termed the cyclic AMP responsive element (CRE).

This family has conserved attractive RE pairs (green) in the 1st heptad and EK pairs (orange) in the 3rd heptad. The crystal structure of CREB bound to a consensus CRE identified the RE and EK interhelical interactions and an additional YE interaction one heptad N-terminal of the leucine zipper, as being important in dimer stability (80). A single asparagine in the 2nd heptad a position and the unique pattern of ge' pairs results in homodimerization among CREB members. Although the ge' pairs are a subset of those found in the PAR family, heterodimerization between PAR and CREB is not predominant, because the PAR|PAR homodimer has greater coupling energy than a PAR|CREB heterodimer.

(iii) Oasis family.

The Oasis family has five proteins, Oasis (30), CREB-H (72), CREB3 (18, 55), hcp201085, and hcp1698600. These proteins also bind the CRE DNA sequence. The 2nd and 3rd heptads contain attractive ge' pairs, and the a positions of the 2nd and 4th heptads contain asparagine. Two characteristics are consistent with this being a homodimerizing family. First, there is a unique pattern of attractive ge' pairs. Second, the asparagine in the 4th a position will encourage dimerization within the family, but not with the other homodimerizing families without an asparagine in the 4th a position.

(iv) ATF6 family.

ATF6 is a group of three proteins, ATF6, CREBL1, and Xbp-1 (7). ATF6 binds to three DNA sequences, termed ERSE-, SRE-, and CRE-like sites (24, 100).

ATF6 proteins have a unique pattern of attractive ge' pairs (orange) in the 2nd, 3rd, and 5th heptads. These three heptads also contain asparagine in the a position. This novel combination of attractive ge' pairs and asparagine placements is likely to promote dimerization within the family and discourage interactions with other B-ZIP proteins. Xbp-1 has a 4th heptad a position threonine that may result in exclusive homodimerization of this protein. However, the interactions in the 2nd, 3rd, and 5th heptads remain the same, so that interaction of Xbp-1 with other ATF6 proteins is a possibility.

The homodimerizing and heterodimerizing B-ZIP families.

The C/EBP, ATF4, ATF2, JUN, and the small MAF families homodimerize and heterodimerize with other B-ZIP families. These proteins have properties found in both the homodimerizing and heterodimerizing proteins.

(i) C/EBP family.

The C/EBP family consists of seven members: C/EBP, C/EBPß, C/EBP, C/EBP, C/EBP, CAA60698, and CHOP10. C/EBP proteins form dimers within the family (5, 101) that bind to the palindromic DNA consensus sequence 5'-ATTGCGCAAT-3' and the related CRE and PAR sites (16). The CHOP10 basic region is unique among the listed B-ZIP proteins with a proline in the basic region that likely distorts the -helical basic region and alters DNA binding. The CHOP10|C/EBP dimer binds a unique DNA sequence (92). Dimerization within the family is driven by attractive ge' (orange) pairs in the 2nd and 4th heptads and a single asparagine at the 2nd heptad a position.

Heterodimeric interactions have been reported between C/EBP and other B-ZIP families, such as the FOS, JUN (32), ATF4 (93, 96), and ATF2 (83) families. C/EBPß has also been reported to interact with CREB (89), however, A-C/EBP and A-CREB fail to inhibit the DNA binding of CREB and C/EBP, respectively (Fig. 6), suggesting repulsion between the leucine zippers of C/EBP and CREB. Heterodimerization between C/EBP and other B-ZIP proteins may be promoted by incomplete ge' pairs found in the 1st and 3rd heptad g positions of C/EBP.

One of the C/EBP members, C/EBP, may have dimerization properties similar to those found in the FOS and JUN families described later. These properties include a repulsive RK (blue) pair in the 1st heptad found in JUN, a repulsive EE (red) pair in the 2nd heptad found in FOS, and a histidine in the 5th d position, as found in JUN, FOS, and ATF2.

(ii) ATF4.

The ATF4 family has three members, ATF4, ATF5, and hcp1709392. Besides homodimerizing, ATF4 heterodimerizes with C/EBP (93, 96), FOS (23), and NRF2 (27). This family is noteworthy in having acidic and basic repulsive ge' pairs as well as attractive ge' pairs, which may explain their promiscuous dimerization properties. The interface contains the 2nd heptad asparagine in the a position found in homodimerizing B-ZIP proteins.

(iii) ATF2 family.

The ATF2 family contains three proteins: ATF2, ATF7, and CRE-BPa (68). These proteins contain an asparagine in the 2nd heptad a position and attractive ge' pairs (orange) in the 3rd and 4th heptads, structural features that favor homodimerization. The 5th heptad d position contains a histidine that is also found in the FOS and JUN families and may be important for interaction with both of these families.

ATF2 has been reported to heterodimerize with JUN (23, 58), FOS (28), and C/EBP (83) family members. Heterodimerization with FOS could be driven by an incomplete ge' pair in the 1st heptad of C/EBP interacting with the EE pair in the 1st heptad of FOS to form an attractive KE pair.

Heterodimerization between C/EBP and ATF2 has been observed on a chimeric DNA sequence composed of a C/EBP half site and an ATF2 half site (83). CEBP and ATF2 homodimers have four attractive interhelical salt bridges and no repulsive ge' pairs, while a ATF2|C/EBP heterodimer has two attractive and one repulsive ge' pair, suggesting that these two proteins would prefer to homodimerize. The formation of heterodimerization on a chimeric site demonstrates the importance of DNA sequence in modulating dimerization specificity.

(iv) JUN family.

The JUN family is comprised of three proteins, c-JUN, JUND, and JUNB. The best-studied JUN partner is FOS. JUN and FOS heterodimerize to form the AP-1 transcription factor, originally isolated as a biochemical activity, that binds the 5'-TGAGTCA-3' DNA sequence, termed the "TRE" (12-O-tetradecanoylphorbol-13-acetate response element) (79, 82). Many other proteins have been reported to heterodimerize with JUN family members, among them CNC, ATF2 (58, 68), ATF3, and c-Maf. JUN family members can also homodimerize, but these complexes bind DNA poorly, bringing into question their biological function (70).

The amino acid sequence of the JUN leucine zipper is consistent with the experimentally observed promiscuous dimerization. Properties that drive heterodimerization are repulsive KK (blue) and QK pairs (blue) in the 1st and 4th heptads, respectively. An incomplete ge' pair in the 3rd heptad also promotes promiscuous heterodimerization. In contrast, the asparagine in the 2nd heptad a position is commonly found in homodimerizing B-ZIP proteins. Heterodimerization with ATF2 creates a canonical interface and attractive ge' pairs. An elegant study (94) showed that by changing amino acids in the e and g positions, the promiscuous dimerization of JUN could be restricted to either FOS or ATF2 with a corresponding change in the biological activity of the JUN mutants. The large number of basic amino acids in the g and e positions encourages heterodimerization with acidic proteins such as FOS. A histidine (H) in the 5th heptad d position is conserved among the JUN, FOS, and ATF2 proteins and contributes to dimer stability (9), but its contribution to dimerization specificity has yet to be elucidated.

(v) Small MAF family.

There are three small MAF (S-MAF) musculoaponeurotic fibrosarcome proteins, MafF, MafG, and MafK. The S-MAFs homodimerize, but do not contain, a transactivation domain and thus repress transcription. However, they also heterodimerize with CNC and FOS family members to activate gene expression (35, 40, 43). The S-MAF leucine zipper contains attractive ER (orange) in the 3rd and 4th heptads that favor homodimerization (also observed in the ATF2 family) and an asparagine in the 3rd a heptad. Features that promote heterodimerization include a lysine in the 1st heptad a position (also found in the L-MAFs) and an incomplete glutamic acid ge' pair (red) in the 2nd heptad.

The heterodimerizing B-ZIP families.

The heterodimerizing B-ZIP families are FOS, CNC, and the large Maf. Three general properties are apparent for these proteins: (i) repulsive ge' pairs that inhibit homodimerization; (ii) amino acids in the a positions include lysine or arginine, which discourages homodimerization; (iii) incomplete ge' pairs that promote promiscuous heterodimerization.

(i) FOS family. There are nine FOS family proteins: c-Fos, FosB, Fra1, Fra2, hcp34067, ATF3, JDP2, SNFT, and BATF. FOS family members heterodimerize with the JUN, CNC, and small Maf families (reviewed in reference 6). The FOS family has acidic amino acids in the g and e positions and heterodimerize with basic JUN zippers (74). Specifically, FOS dimerization properties can be divided into three sets of characteristics that are slightly variable. Five of the proteins (c-Fos, FosB, Fra1, Fra2, and hcp34067) contain conserved repulsive EE or QE pairs (red) in the 1st and 4th heptads and repulsive EQ or EE pairs (red) in the 2nd and 3rd heptads. The hydrophobic interface is composed of a threonine in the 1st a position, lysines in the 2nd and 4th a positions, and a histidine in the 5th heptad. The lysines in the a position inhibit homodimerization and drive heterodimerization.

The remaining FOS family members, ATF3, JDP2, SNFT, and BATF, are not as acidic and do not contain as many repulsive lysines in the a position as the prototypical FOS leucine zipper. They can be further divided into two groups: SNFT and BATF, which do not contain the repulsive 4th heptad a position basic amino acid found in ATF3 and JDP2.

(ii) CNC family. The second acidic leucine zipper family is named after the founding member, cap'n'collar (CNC), a Drosophila protein (62). There are six members: BACH1, CNC1/NRF1, NF-E2, BACH2, CNC2/NRF2, and NF-E2L3. These proteins heterodimerize with the S-MAF family (35, 66). These proteins have either a repulsive acidic ge' pair or an acidic incomplete ge' pair in the 1st heptad. The presence of multiple incomplete ge' pairs is expected to confer promiscuous dimerization properties. Like the FOS family, the CNC family has lysines in the a positions that drive heterodimerization. However, in contrast to the FOS family, where the lysines are in the 2nd and 4th heptad a positions, CNC proteins contain a basic amino acid in the 2nd and 3rd heptad a positions. This arrangement should alter the heterodimerization partners for the CNC proteins compared to FOS proteins. Interestingly, the CNC|S-MAF heterodimer forms a 3rd heptad a position interaction between N and K, similar to the 2nd heptad interaction found between FOS and JUN in the 2nd heptad.

(iii) Large MAF family. The large MAF (L-MAF) family contains three members: NRL, c-MAF, and MAF-B. These proteins can homodimerize and heterodimerize with FOS and JUN proteins (39, 43).

L-MAF family members form heterodimers driven by the repulsive QK (blue) or QR pairs (blue) in the 2nd heptad, while homodimerization is mediated through attractive EK pairs (orange) in the 4th heptad. Along with the small MAF proteins, these are the only B-ZIP proteins with aliphatic amino acids in the 2nd a position. The 1st and 4th heptad a position lysine or arginine discourages homodimerization. Features that promote promiscuous heterodimerization include incomplete ge' pairs composed of glutamic acid (red) in the 1st and 3rd heptads.

(iv) HCF family. The HCF (host cell factor) protein, also known as C1 (45), VCAF (76), or CFF (38), exists in human cells as a family of proteolytic cleavage products of the primary HCF protein (46).

HCF has a unique pattern of interactions that suggest it will homodimerize. This protein contains attractive ge' pairs (orange) in the 1st and 4th heptads. The a positions contain asparagine in the 1st and 2nd heptad a positions and serine (a small polar amino acid similar to asparagine) in the 4th heptad. HCF was found to interact with Luman (18, 55).

SUMMARY

We have reviewed the literature on the dimerization properties of mammalian B-ZIP proteins and made predictions about the amino acids in the a, d, e, and g positions of the leucine zipper that mediate their known dimerization specificities. We have extended these predictions to all the identified B-ZIP proteins in the human genome. These predictions appear more robust for the homodimerizing proteins than for the heterodimerizing proteins. This type of analysis will be valuable in predicting the dimerization properties of B-ZIP proteins from newly sequenced genomes for which much less experimental data exists. Additional experimental data is needed to quantify the attraction and repulsion between different B-ZIP leucine zippers to gain insight into which dimers may form in vivo. In addition, the contribution of DNA binding to B-ZIP stability needs to be quantified to gain insight into how DNA sequences can regulate B-ZIP dimer partner choice.

ACKNOWLEDGMENTS

We thank Tsonwin Hai, Jon Shuman, and an anonymous reviewer for comments on the manuscript.

 
* Corresponding author. Mailing address: Building 37, Room 2D24, Laboratory of Metabolism, National Cancer Institute, National Institutes of Health, Bethesda, MD 20892. Phone: (301) 496-8753. Fax: (301) 496-8419. E-mail: Vinsonc{at}dc37a.nci.nih.gov.

REFERENCES

1
1. Ahn, S., M. Olive, S. Aggarwal, D. Krylov, D. D. Ginty, and C. Vinson. 1998. A dominant-negative inhibitor of CREB reveals that it is a general mediator of stimulus-dependent transcription of c-fos. Mol. Cell. Biol. 18:967-977.[Abstract/Free Full Text]
2
2. Alber, T. 1992. Structure of the leucine zipper. Curr. Opin. Genet. Dev. 2:205-210.[CrossRef][Medline]
3
3. Baxevanis, A. D., and C. R. Vinson. 1993. Interactions of coiled coils in transcription factors: where is the specificity? Curr. Opin. Genet. Dev. 3:278-285.[CrossRef][Medline]
4
4. Bohmann, D., T. J. Bos, A. Admon, T. Nishimura, P. K. Vogt, and R. Tjian. 1987. Human proto-oncogene c-jun encodes a DNA binding protein with structural and functional properties of transcription factor AP-1. Science 238:1386-1392.[Abstract/Free Full Text]
5
5. Cao, Z., R. M. Umek, and S. L. McKnight. 1991. Regulated expression of three C/EBP isoforms during adipose conversion of 3T3-L1 cells. Genes Dev. 5:1538-1552.[Abstract/Free Full Text]
6
6. Chinenov, Y., and T. K. Kerppola. 2001. Close encounters of many kinds: Fos-Jun interactions that mediate transcription regulatory specificity. Oncogene 20:2438-2452.[CrossRef][Medline]
7
7. Clauss, I. M., M. Chu, J. L. Zhao, and L. H. Glimcher. 1996. The basic domain/leucine zipper protein hXBP-1 preferentially binds to and transactivates CRE-like sequences containing an ACGT core. Nucleic Acids Res. 24:1855-1864.[Abstract/Free Full Text]
8
8. Cohen, C., and D. Parry. 1990. A-helical coiled coils and bundles: how to design an -helical protein. Protein 7:1-14.
9
9. Cohen, D. R., and T. Curran. 1990. Analysis of dimerization and DNA binding functions in Fos and Jun by domain-swapping: involvement of residues outside the leucine zipper/basic region. Oncogene 5:929-939.[Medline]
10
10. Crick, F. 1953. The packing of -helices: simple coiled-coils. Acta Crystallogr. 6:689-697.[CrossRef]
11
11. Daniel, P. B., W. H. Walker, and J. F. Habener. 1998. Cyclic AMP signaling and gene regulation. Annu. Rev. Nutr. 18:353-383.[CrossRef][Medline]
12
12. De Cesare, D., G. M. Fimia, and P. Sassone-Corsi. 1999. Signaling routes to CREM and CREB: plasticity in transcriptional activation. Trends Biochem. Sci. 24:281-285.[CrossRef][Medline]
13
13. Dlakic, M., A. V. Grinberg, D. A. Leonard, and T. K. Kerppola. 2001. DNA sequence-dependent folding determines the divergence in binding specificities between Maf and other bZIP proteins. EMBO J. 20:828-840.[CrossRef][Medline]
14
14. Drolet, D. W., K. M. Scully, D. M. Simmons, M. Wegner, K. T. Chu, L. W. Swanson, and M. G. Rosenfeld. 1991. TEF, a transcription factor expressed specifically in the anterior pituitary during embryogenesis, defines a new class of leucine zipper proteins. Genes Dev. 5:1739-1753.[Abstract/Free Full Text]
15
15. Ellenberger, T., C. Brandl, K. Struhl, and S. Harrison. 1992. The GCN4 basic region leucine zipper binds DNA as a dimer of uninterrupted helices: crystal structure of the protein-DNA complex. Cell 71:1223-1237.[CrossRef][Medline]
16
16. Falvey, E., L. Marcacci, and U. Schibler. 1996. DNA-binding specificity of PAR and C/EBP leucine zipper proteins: a single amino acid substitution in the C/EBP DNA-binding domain confers PAR-like specificity to C/EBP. Biol. Chem. 377:797-809.[Medline]
17
17. Fassler, J., D. Landsman, A. Acharya, J. Moll, M. Bonovich, et al. B-ZIP proteins encoded by the Drosophila genome: evaluation of potential dimerization partners. Genome Res., in press.
18
18. Freiman, R. N., and W. Herr. 1997. Viral mimicry: common mode of association with HCF by VP16 and the cellular protein LZIP. Genes Dev. 11:3122-3127.[Abstract/Free Full Text]
19
19. Fujii, Y., T. Shimizu, T. Toda, M. Yanagida, and T. Hakoshima. 2000. Structural basis for the diversity of DNA recognition by bZIP transcription factors. Nat. Struct. Biol. 7:889-893.[CrossRef][Medline]
20
20. Gentz, R., F. J. Rauscher III, C. Abate, and T. Curran. 1989. Parallel association of Fos and Jun leucine zippers juxtaposes DNA binding domains. Science 243:1695-1699.[Abstract/Free Full Text]
21
21. Glover, J. N., and S. C. Harrison. 1995. Crystal structure of the heterodimeric bZIP transcription factor c-Fos-c-Jun bound to DNA. Nature 373:257-261.[CrossRef][Medline]
22
22. Greenwel, P., S. Tanaka, D. Penkov, W. Zhang, M. Olive, J. Moll, C. Vinson, M. Di Liberto, and F. Ramirez. 2000. Tumor necrosis factor alpha inhibits type I collagen synthesis through repressive CCAAT/enhancer-binding proteins. Mol. Cell. Biol. 20:912-918.[Abstract/Free Full Text]
23
23. Hai, T., and T. Curran. 1991. Cross-family dimerization of transcription factors Fos/Jun and ATF/CREB alters DNA binding specificity. Proc. Natl. Acad. Sci. USA 88:3720-3724.[Abstract/Free Full Text]
24
24. Hai, T., and M. G. Hartman. 2001. The molecular biology and nomenclature of the activating transcription factor/cAMP responsive element binding family of transcription factors: activating transcription factor proteins and homeostasis. Gene 273:1-11.[CrossRef][Medline]
25
25. Hai, T., F. Liu, W. Coukos, and M. Green. 1989. Transcription factor ATF cDNA clones: an extensive family of leucine zipper proteins able to selectively form DNA-binding heterodimers. Genes Dev. 3:2083-2090.[Abstract/Free Full Text]
26
26. Harbury, P. B., T. Zhang, P. S. Kim, and T. Alber. 1993. A switch between two-, three-, and four-stranded coiled coils in GCN4 leucine zipper mutants. Science 262:1401-1417.[Abstract/Free Full Text]
27
27. He, C. H., P. Gong, B. Hu, D. Stewart, M. E. Choi, A. M. Choi, and J. Alam. 2001. Identification of activating transcription factor 4 (ATF4) as an Nrf2-interacting protein. Implication for heme oxygenase-1 gene regulation. J. Biol. Chem. 276:20858-20865.[Abstract/Free Full Text]
28
28. Hoeffler, J. P., J. W. Lustbader, and C. Y. Chen. 1991. Identification of multiple nuclear factors that interact with cyclic adenosine 3',5'-monophosphate response element-binding protein and activating transcription factor-2 by protein-protein interactions. Mol. Endocrinol. 5:256-266.[Abstract/Free Full Text]
29
29. Hoeffler, J. P., T. E. Meyer, Y. Yun, J. L. Jameson, and J. F. Habener. 1988. Cyclic AMP-responsive DNA-binding protein: structure based on a cloned placental cDNA. Science 242:1430-1433.[Abstract/Free Full Text]
30
30. Honma, Y., K. Kanazawa, T. Mori, Y. Tanno, M. Tojo, H. Kiyosawa, J. Takeda, T. Nikaido, T. Tsukamoto, S. Yokoya, and A. Wanaka. 1999. Identification of a novel gene, OASIS, which encodes for a putative CREB/ATF family transcription factor in the long-term cultured astrocytes and gliotic tissue. Mol. Brain Res. 69:93-103.[Medline]
31
31. Horovitz, A., L. Serrano, B. Avron, M. Bycroft, and A. R. Fersht. 1990. Strength and cooperativity of contributions of surface salt bridges to protein stability. J. Mol. Biol. 216:1031-1044.[Medline]
32
32. Hsu, W., T. K. Kerppola, P.-L. Chen, T. Curran, and S. Chen-Kiang. 1994. Fos and Jun repress transcription activation by NF-IL6 through association at the basic zipper region. Mol. Cell. Biol. 14:268-276.[Abstract/Free Full Text]
33
33. Hunger, S. P., K. Ohyashiki, K. Toyama, and M. L. Cleary. 1992. Hlf, a novel hepatic bZIP protein, shows altered DNA-binding properties following fusion to E2A in t(17;19) acute lymphoblastic leukemia. Genes Dev. 6:1608-1620.[Abstract/Free Full Text]
34
34. Hurst, H. C. 1995. Transcription factors 1: bZIP proteins. Protein Profile 2:101-168.[Medline]
35
35. Igarashi, K., K. Kataoka, K. Itoh, N. Hayashi, M. Nishizawa, and M. Yamamoto. 1994. Regulation of transcription by dimerization of erythroid factor NF-E2 p45 with small Maf proteins. Nature 367:568-572.[CrossRef][Medline]
36
36. Iyer, S. V., D. L. Davis, S. N. Seal, and J. B. E. Burch. 1991. Chicken vitellogenin gene-binding protein, a leucine zipper transcription factor that binds to an important control element in the chicken vitellogenin II promoter, is related to rat DBP. Mol. Cell. Biol. 11:4863-4875.[Abstract/Free Full Text]
37
37. Johnson, P. F., W. H. Landschulz, B. J. Graves, and S. L. McKnight. 1987. Identification of a rat liver nuclear protein that binds to the enhancer core element of three animal viruses. Genes Dev. 1:133-146.[Abstract/Free Full Text]
38
38. Katan, M., A. Haigh, C. P. Verrijzer, P. C. van der Vliet, and P. O'Hare. 1990. Characterization of a cellular factor which interacts functionally with Oct-1 in the assembly of a multicomponent transcription complex. Nucleic Acids Res. 18:6871-6880.[Abstract/Free Full Text]
39
39. Kataoka, K., K. T. Fujiwara, M. Noda, and M. Nishizawa. 1994. MafB, a new Maf family transcription activator that can associate with Maf and Fos but not with Jun. Mol. Cell. Biol. 14:7581-7591.[Abstract/Free Full Text]
40
40. Kataoka, K., K. Igarashi, K. Itoh, K. T. Fujiwara, M. Noda, M. Yamamoto, and M. Nishizawa. 1995. Small Maf proteins heterodimerize with Fos and may act as competitive repressors of the NF-E2 transcription factor. Mol. Cell. Biol. 15:2180-2190. (Erratum, 15:3461.)
41
41. Kerppola, T., and T. Curran. 1991. Transcription factor interactions: basics on zippers. Curr. Opin. Struct. Biol. 1:71-79.
42
42. Kerppola, T. K., and T. Curran. 1994. A conserved region adjacent to the basic domain is required for recognition of an extended DNA binding site by Maf/Nrl family proteins. Oncogene 9:3149-3158.[Medline]
43
43. Kerppola, T. K., and T. Curran. 1994. Maf and Nrl can bind to AP-1 sites and form heterodimers with Fos and Jun. Oncogene 9:675-684.[Medline]
44
44. Kouzarides, T., and E. Ziff. 1988. The role of the leucine zipper in the fos-jun interaction. Nature 336:646-651.[CrossRef][Medline]
45
45. Kristie, T. M., J. H. LeBowitz, and P. A. Sharp. 1989. The octamer-binding proteins form multi-protein-DNA complexes with the HSV alpha TIF regulatory protein. EMBO J. 8:4229-4238.[Medline]
46
46. Kristie, T. M., J. L. Pomerantz, T. C. Twomey, S. A. Parent, and P. A. Sharp. 1995. The cellular C1 factor of the herpes simplex virus enhancer complex is a family of polypeptides. J. Biol. Chem. 270:4387-4394.[Abstract/Free Full Text]
47
47. Krylov, D., J. Barchi, and C. Vinson. 1998. Inter-helical interactions in the leucine zipper coiled coil dimer: pH and salt dependence of coupling energy between charged amino acids. J. Mol. Biol. 279:959-972.[CrossRef][Medline]
48
48. Krylov, D., I. Mikhailenko, and C. Vinson. 1994. A thermodynamic scale for leucine zipper stability and dimerization specificity: e and g interhelical interactions. EMBO J. 13:2849-2861.[Medline]
49
49. Krylov, D., M. Olive, and C. Vinson. 1995. Extending dimerization interfaces: the bZIP basic region can form a coiled coil. EMBO J. 14:5329-5337.[Medline]
50
50. Lamb, P., and S. L. McKnight. 1991. Diversity and specificity in transcriptional regulation: the benefits of heterotypic dimerization. Trends Biochem. Sci. 16:417-422.[CrossRef][Medline]
51
51. Lander, E. S., L. M. Linton, B. Birren, C. Nusbaum, M. C. Zody, J. Baldwin, K. Devon, K. Dewar, M. Doyle, W. FitzHugh, R. Funke, D. Gage, K. Harris, A. Heaford, J. Howland, L. Kann, J. Lehoczky, R. LeVine, P. McEwan, K. McKernan, J. Meldrim, J. P. Mesirov, C. Miranda, W. Morris, J. Naylor, C. Raymond, M. Rosetti, R. Santos, A. Sheridan, C. Sougnez, N. Stange-Thomann, N. Stojanovic, A. Subramanian, D. Wyman, J. Rogers, J. Sulston, R. Ainscough, S. Beck, D. Bentley, J. Burton, C. Clee, N. Carter, A. Coulson, R. Deadman, P. Deloukas, A. Dunham, I. Dunham, R. Durbin, L. French, D. Grafham, S. Gregory, T. Hubbard, S. Humphray, A. Hunt, M. Jones, C. Lloyd, A. McMurray, L. Matthews, S. Mercer, S. Milne, J. C. Mullikin, A. Mungall, R. Plumb, M. Ross, R. Shownkeen, S. Sims, R. H. Waterston, R. K. Wilson, L. W. Hillier, J. D. McPherson, M. A. Marra, E. R. Mardis, L. A. Fulton, A. T. Chinwalla, K. H. Pepin, W. R. Gish, S. L. Chissoe, M. C. Wendl, K. D. Delehaunty, T. L. Miner, A. Delehaunty, J. B. Kramer, L. L. Cook, R. S. Fulton, D. L. Johnson, P. J. Minx, S. W. Clifton, T. Hawkins, E. Branscomb, P. Predki, P. Richardson, S. Wenning, T. Slezak, N. Doggett, J. F. Cheng, A. Olsen, S. Lucas, C. Elkin, E. Uberbacher, M. Frazier et al. 2001. Initial sequencing and analysis of the human genome. Nature 409:860-921.[CrossRef][Medline]
52
52. Landschultz, W. H., P. F. Johnson, and S. L. McKnight. 1988. The leucine zipper: a hypothetical structure common to a new class of DNA binding proteins. Science 240:1759-1764.[Abstract/Free Full Text]
53
53. Landschulz, W. H., P. F. Johnson, E. Y. Adashi, B. J. Graves, and S. L. McKnight. 1988. Isolation of a recombinant copy of the gene encoding C/EBP. Genes Dev. 2:786-800.[Abstract/Free Full Text]
54
54. Landschulz, W. H., P. F. Johnson, and S. L. McKnight. 1989. The DNA binding domain of the rat liver nuclear protein C/EBP is bipartite. Science 243:1681-1688.[Abstract/Free Full Text]
55
55. Lu, R., P. Yang, P. O'Hare, and V. Misra. 1997. Luman, a new member of the CREB/ATF family, binds to herpes simplex virus VP16-associated host cellular factor. Mol. Cell. Biol. 17:5117-5126.[Abstract]
56
56. Lumb, K. J., and P. S. Kim. 1995. Measurement of interhelical electrostatic interactions in the GCN4 leucine zipper. Science 268:436-439.[Abstract/Free Full Text]
57
57. Lupas, A. 1996. Coiled coils: new structures and new functions. Trends Biochem. 21:375-382.[CrossRef][Medline]
58
58. Macgregor, P. F., C. Abate, and T. Curran. 1990. Direct cloning of leucine zipper proteins: Jun binds cooperatively to the CRE with CRE-BP1. Oncogene 5:451-458.[Medline]
59
59. Marti, D. N., I. Jelesarov, and H. R. Bosshard. 2000. Interhelical ion pairing in coiled coils: solution structure of a heterodimeric leucine zipper and determination of pKa values of Glu side chains. Biochemistry 39:12804-12818.[CrossRef][Medline]
60
60. Mayr, B., and M. Montminy. 2001. Transcriptional regulation by the phosphorylation-dependent factor CREB. Nat. Rev. Mol. Cell Biol. 2:599-609.[CrossRef][Medline]
61
61. McLachlan, A., and M. Stewart. 1975. Tropomyosin coiled-coil interactions: evidence for an unstaggered structure. J. Mol. Biol. 98:293-304.[CrossRef][Medline]
62
62. Mohler, J., K. Vani, S. Leung, and A. Epstein. 1991. Segmentally restricted, cephalic expression of a leucine zipper gene during Drosophila embryogenesis. Mech. Dev. 34:3-9.[CrossRef][Medline]
63
63. Moitra, J., L. Szilak, D. Krylov, and C. Vinson. 1997. Leucine is the most stabilizing aliphatic amino acid in the d position of a dimeric leucine zipper coiled coil. Biochemistry 36:12567-12573.[CrossRef][Medline]
64
64. Moll, J. R., M. Olive, and C. Vinson. 2000. Attractive interhelical electrostatic interactions in the proline- and acidic-rich region (PAR) leucine zipper subfamily preclude heterodimerization with other basic leucine zipper subfamilies. J. Biol. Chem. 275:34826-34832.[Abstract/Free Full Text]
65
65. Montminy, M. R., and L. M. Bilezikjian. 1987. Binding of a nuclear protein to the cyclic-AMP response element of the somatostatin gene. Nature 328:175-178.[CrossRef][Medline]
66
66. Motohashi, H., J. A. Shavit, K. Igarashi, M. Yamamoto, and J. D. Engel. 1997. The world according to Maf. Nucleic Acids Res. 25:2953-2959.[Abstract/Free Full Text]
67
67. Nicklin, M., and G. Casari. 1991. A single site mutation in a truncated Fos protein allows it to interact with the TRE in vitro. Oncogene 6:173-179.[Medline]
68
68. Nomura, N., Y. L. Zu, T. Maekawa, S. Tabata, T. Akiyama, and S. Ishii. 1993. Isolation and characterization of a novel member of the gene family encoding the cAMP response element-binding protein CRE-BP1. J. Biol. Chem. 268:4259-4266.[Abstract/Free Full Text]
69
69. Oakley, M. G., and P. S. Kim. 1998. A buried polar interaction can direct the relative orientation of helices in a coiled coil. Biochemistry 37:12603-12610.[CrossRef][Medline]
70
70. Olive, M., D. Krylov, D. R. Echlin, K. Gardner, E. Taparowsky, and C. Vinson. 1997. A dominant negative to activation protein-1 (AP1) that abolishes DNA binding and inhibits oncogenesis. J. Biol. Chem. 272:18586-18594.[Abstract/Free Full Text]
71
71. Olive, M., S. C. Williams, C. Dezan, P. F. Johnson, and C. Vinson. 1996. Design of a C/EBP-specific, dominant-negative bZIP protein with both inhibitory and gain-of-function properties. J. Biol. Chem. 271:2040-2047.[Abstract/Free Full Text]
72
72. Omori, Y., J. Imai, M. Watanabe, T. Komatsu, Y. Suzuki, K. Kataoka, S. Watanabe, A. Tanigami, and S. Sugano. 2001. CREB-H: a novel mammalian transcription factor belonging to the CREB/ATF family and functioning via the box-B element with a liver-specific expression. Nucleic Acids Res. 29:2154-2162.[Abstract/Free Full Text]
73
73. O'Neil, K. T., R. H. Hoess, and W. F. DeGrado. 1990. Design of DNA binding peptides based on the leucine zipper motif. Science 243:774-778.
74
74. O'Shea, E., R. Rutkowski, and P. Kim. 1992. Mechanism of specificity in the fos-jun oncoprotein heterodimer. Cell 68:699-708.[CrossRef][Medline]
75
75. O'Shea, E. K., J. D. Klemm, P. S. Kim, and T. Alber. 1991. X-ray structure of the GCN4 leucine zipper, a two-stranded, parallel coiled-coil. Science 254:539-544.[Abstract/Free Full Text]
76
76. Popova, B., P. Bilan, P. Xiao, M. Faught, and J. P. Capone. 1995. Transcriptional activation by DNA-binding derivatives of HSV-1 VP16 that lack the carboxyl-terminal acidic activation domain. Virology 209:19-28.[CrossRef][Medline]
77
77. Ransone, L. J., J. Visvader, P. Sassone-Corsi, and I. M. Verma. 1989. Fos-Jun interaction: mutational analysis of the leucine zipper domain of both proteins. Genes Dev. 3:770-781.[Abstract/Free Full Text]
78
78. Ryder, K., A. Lanahan, E. Perez-Albuerne, and D. Nathans. 1989. jun-D: a third member of the jun gene family. Proc. Natl. Acad. Sci. USA 86:1500-1503.[Abstract/Free Full Text]
79
79. Ryseck, R. P., and R. Bravo. 1991. c-JUN, JUN B, and JUN D differ in their binding affinities to AP-1 and CRE consensus sequences: effect of FOS proteins. Oncogene 6:533-542.[Medline]
80
80. Schumacher, M. A., R. H. Goodman, and R. G. Brennan. 2000. The structure of a CREB bZIP.somatostatin CRE complex reveals the basis for selective dimerization and divalent cation-enhanced DNA binding. J. Biol. Chem. 275:35242-35247.[Abstract/Free Full Text]
81
81. Serrano, L., A. Horovitz, B. Avron, M. Bycroft, and A. R. Fersht. 1990. Estimating the contribution of engineered surface electrostatic interactions to protein stability by using double-mutant cycles. Biochemistry 29:9343-9352.[CrossRef][Medline]
82
82. Shaulian, E., and M. Karin. 2001. AP-1 in cell proliferation and survival. Oncogene 20:2390-2400.[CrossRef][Medline]
83
83. Shuman, J. D., J. Cheong, and J. E. Coligan. 1997. ATF-2 and C/EBPalpha can form a heterodimeric DNA binding complex in vitro. Functional implications for transcriptional regulation. J. Biol. Chem. 272:12793-12800.[Abstract/Free Full Text]
84
84. Shuman, J. D., C. R. Vinson, and S. L. McKnight. 1990. Evidence of changes in protease sensitivity and subunit exchange rate on DNA binding by C/EBP. Science 249:771-774.[Abstract/Free Full Text]
85
85. Singh, H., J. H. LeBowitz, A. S. Baldwin, Jr., and P. A. Sharp. 1988. Molecular cloning of an enhancer binding protein: isolation by screening of an expression library with a recognition site DNA. Cell 52:415-423.[CrossRef][Medline]
86
86. Smeal, T., P. Angel, J. Meek, and M. Karin. 1989. Different requirements for formation of Jun:Jun and Jun:Fos complexes. Genes Dev. 3:2091-2100.[Abstract/Free Full Text]
87
87. Thompson, K. S., C. R. Vinson, and E. Freire. 1993. Thermodynamic characterization of the structural stability of the coiled-coil region of the bZIP transcription factor GCN4. Biochemistry 32:5491-5496.[CrossRef][Medline]
88
88. Tripet, B., K. Wagschal, P. Lavigne, C. T. Mant, and R. S. Hodges. 2000. Effects of side-chain characteristics on stability and oligomerization state of a de novo-designed model coiled-coil: 20 amino acid substitutions in position "d." J. Mol. Biol. 300:377-402.[CrossRef][Medline]
89
89. Tsukada, J., K. Saito, W. R. Waterman, A. C. Webb, and P. E. Auron. 1994. Transcription factors NF-IL6 and CREB recognize a common essential site in the human prointerleukin 1ß gene. Mol. Cell. Biol. 14:7285-7297.[Abstract/Free Full Text]
90
90. Tupler, R., G. Perini, and M. R. Green. 2001. Expressing the human genome. Nature 409:832-833.[CrossRef][Medline]
91
91. Turner, R., and R. Tjian. 1989. Leucine repeats and an adjacent DNA binding domain mediate the formation of functional cFos-cJun heterodimers. Science 243:1689-1694.[Abstract/Free Full Text]
92
92. Ubeda, M., X.-Z. Wang, H. Zinszner, I. Wu, J. F. Habener, and D. Ron. 1996. Stress-induced binding of the transcriptional factor CHOP to a novel DNA control element. Mol. Cell. Biol. 16:1479-1489.[Abstract]
93
93. Vallejo, M., D. Ron, C. P. Miller, and J. F. Habener. 1993. C/ATF, a member of the activating transcription factor family of DNA-binding proteins, dimerizes with CAAT/enhancer-binding proteins and directs their binding to cAMP response elements. Proc. Natl. Acad. Sci. USA 90:4679-4683.[Abstract/Free Full Text]
94
94. van Dam, H., S. Huguier, K. Kooistra, J. Baguet, E. Vial, A. J. van der Eb, P. Herrlich, P. Angel, and M. Castellazzi. 1998. Autocrine growth and anchorage independence: two complementing Jun-controlled genetic programs of cellular transformation. Genes Dev. 12:1227-1239.[Abstract/Free Full Text]
95
95. Venter, J. C., M. D. Adams, E. W. Myers, P. W. Li, R. J. Mural, G. G. Sutton, H. O. Smith, M. Yandell, C. A. Evans, R. A. Holt, J. D. Gocayne, P. Amanatides, R. M. Ballew, D. H. Huson, J. R. Wortman, Q. Zhang, C. D. Kodira, X. H. Zheng, L. Chen, M. Skupski, G. Subramanian, P. D. Thomas, J. Zhang, G. L. Gabor Miklos, C. Nelson, S. Broder, A. G. Clark, J. Nadeau, V. A. McKusick, N. Zinder, A. J. Levine, R. J. Roberts, M. Simon, C. Slayman, M. Hunkapiller, R. Bolanos, A. Delcher, I. Dew, D. Fasulo, M. Flanigan, L. Florea, A. Halpern, S. Hannenhalli, S. Kravitz, S. Levy, C. Mobarry, K. Reinert, K. Remington, J. Abu-Threideh, E. Beasley, K. Biddick, V. Bonazzi, R. Brandon, M. Cargill, I. Chandramouliswaran, R. Charlab, K. Chaturvedi, Z. Deng, V. Di Francesco, P. Dunn, K. Eilbeck, C. Evangelista, A. E. Gabrielian, W. Gan, W. Ge, F. Gong, Z. Gu, P. Guan, T. J. Heiman, M. E. Higgins, R. R. Ji, Z. Ke, K. A. Ketchum, Z. Lai, Y. Lei, Z. Li, J. Li, Y. Liang, X. Lin, F. Lu, G. V. Merkulov, N. Milshina, H. M. Moore, A. K. Naik, V. A. Narayan, B. Neelam, D. Nusskern, D. B. Rusch, S. Salzberg, W. Shao, B. Shue, J. Sun, Z. Wang, A. Wang, X. Wang, J. Wang, M. Wei, R. Wides, C. Xiao, C. Yan, et al. 2001. The sequence of the human genome. Science 291:1304-1351.[Abstract/Free Full Text]
96
96. Vinson, C. R., T. Hai, and S. M. Boyd. 1993. Dimerization specificity of the leucine zipper-containing bZIP motif on DNA binding: prediction and rational design. Genes Dev. 7:1047-1058.[Abstract/Free Full Text]
97
97. Vinson, C. R., K. L. LaMarco, P. F. Johnson, W. H. Landschulz, and S. L. McKnight. 1988. In situ detection of sequence-specific DNA-binding activity specified by a recombinant bacteriophage. Genes Dev. 2:801-806.[Abstract/Free Full Text]
98
98. Vinson, C. R., P. B. Sigler, and S. L. McKnight. 1989. A scissors-grip model for DNA recognition by a family of leucine zipper proteins. Science 246:911-916.[Abstract/Free Full Text]
99
99. Wagschal, K., B. Tripet, P. Lavigne, C. Mant, and R. S. Hodges. 1999. The role of position a in determining the stability and oligomerization state of alpha-helical coiled coils: 20 amino acid stability coefficients in the hydrophobic core of proteins. Protein Sci. 8:2312-2329.[Medline]
100
100. Wang, Y., J. Shen, N. Arenzana, W. Tirasophon, R. J. Kaufman, and R. Prywes. 2000. Activation of ATF6 and an ATF6 DNA binding site by the endoplasmic reticulum stress response. J. Biol. Chem. 275:27013-27020.[Abstract/Free Full Text]
101
101. Williams, S. C., C. A. Cantwell, and P. F. Johnson. 1991. A family of C/EBP-related proteins capable of forming covalently linked leucine zipper dimers in vitro. Genes Dev. 5:1553-1567.[Abstract/Free Full Text]
102
102. Yoshimura, T., J. Fujisawa, and M. Yoshida. 1990. Multiple cDNA clones encoding nuclear proteins that bind to the tax-dependent enhancer of HTLV-1: all contain a leucine zipper structure and basic amino acid domain. EMBO J. 9:2537-2542.[Medline]
103
103. Zeng, X., A. M. Herndon, and J. C. Hu. 1997. Buried asparagines determine the dimerization specificities of leucine zipper mutants. Proc. Natl. Acad. Sci. USA 94:3673-3678.[Abstract/Free Full Text]
104
104. Zhou, N., C. Kay, and R. Hodges. 1994. The net energetic contribution of interhelical electrostatic attractions to coiled-coil stability. Protein Eng. 7:1365-1372.[Abstract/Free Full Text]
105
105. Zhu, H., S. A. Celinski, J. M. Scholtz, and J. C. Hu. 2000. The contribution of buried polar groups to the conformational stability of the GCN4 coiled coil. J. Mol. Biol. 300:1377-1387.[CrossRef][Medline]

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Molecular and Cellular Biology, September 2002, p. 6321-6335, Vol. 22, No. 18
0270-7306/02/$04.00+0     DOI: 10.1128/MCB.22.18.6321-6335.2002
Copyright © 2002, American Society for Microbiology. All Rights Reserved.

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• Yoshida, T., Ohkumo, T., Ishibashi, S., Yasuda, K. (2005). The 5'-AT-rich half-site of Maf recognition element: a functional target for bZIP transcription factor Maf. Nucleic Acids Res 33: 3465-3478 [Abstract] [Full Text]  
• Misra, V., Rapin, N., Akhova, O., Bainbridge, M., Korchinski, P. (2005). Zhangfei Is a Potent and Specific Inhibitor of the Host Cell Factor-binding Transcription Factor Luman. J. Biol. Chem. 280: 15257-15266 [Abstract] [Full Text]  
• Yeagley, D., Quinn, P. G. (2005). 3',5'-Cyclic Adenosine Monophosphate Response Element-Binding Protein and CCAAT Enhancer-Binding Protein Are Dispensable for Insulin Inhibition of Phosphoenolpyruvate Carboxykinase Transcription and for Its Synergistic Induction by Protein Kinase A and Glucocorticoids. Mol. Endocrinol. 19: 913-924 [Abstract] [Full Text]  
• Chin, K.-T., Zhou, H.-J., Wong, C.-M., Lee, J. M.-F., Chan, C.-P., Qiang, B.-Q., Yuan, J.-G., Ng, I. O.-l., Jin, D.-Y. (2005). The liver-enriched transcription factor CREB-H is a growth suppressor protein underexpressed in hepatocellular carcinoma. Nucleic Acids Res 33: 1859-1873 [Abstract] [Full Text]  
• Agou, F., Courtois, G., Chiaravalli, J., Baleux, F., Coic, Y.-M., Traincard, F., Israel, A., Veron, M. (2004). Inhibition of NF-{kappa}B Activation by Peptides Targeting NF-{kappa}B Essential Modulator (NEMO) Oligomerization. J. Biol. Chem. 279: 54248-54257 [Abstract] [Full Text]  
• Chun, J. T., Di Dato, V., D'Andrea, B., Zannini, M., Di Lauro, R. (2004). The CRE-Like Element Inside the 5'-Upstream Region of the Rat Sodium/Iodide Symporter Gene Interacts with Diverse Classes of b-Zip Molecules that Regulate Transcriptional Activities through Strong Synergy with Pax-8. Mol. Endocrinol. 18: 2817-2829 [Abstract] [Full Text]  
• West, M. J., Webb, H. M., Sinclair, A. J., Woolfson, D. N. (2004). Biophysical and Mutational Analysis of the Putative bZIP Domain of Epstein-Barr Virus EBNA 3C. J. Virol. 78: 9431-9445 [Abstract] [Full Text]  
• Ganss, B., Jheon, A. (2004). ZINC FINGER TRANSCRIPTION FACTORS IN SKELETAL DEVELOPMENT. CROBM 15: 282-297 [Abstract] [Full Text]  
• FitzGerald, P. C., Shlyakhtenko, A., Mir, A. A., Vinson, C. (2004). Clustering of DNA Sequences in Human Promoters. Genome Res 14: 1562-1574 [Abstract] [Full Text]  
• Agou, F., Traincard, F., Vinolo, E., Courtois, G., Yamaoka, S., Israel, A., Veron, M. (2004). The Trimerization Domain of Nemo Is Composed of the Interacting C-terminal CC2 and LZ Coiled-coil Subdomains. J. Biol. Chem. 279: 27861-27869 [Abstract] [Full Text]  
• Deppmann, C. D., Acharya, A., Rishi, V., Wobbes, B., Smeekens, S., Taparowsky, E. J., Vinson, C. (2004). Dimerization specificity of all 67 B-ZIP motifs in Arabidopsis thaliana: a comparison to Homo sapiens B-ZIP motifs. Nucleic Acids Res 32: 3435-3445 [Abstract] [Full Text]  
• Thuerauf, D. J., Morrison, L., Glembotski, C. C. (2004). Opposing Roles for ATF6{alpha} and ATF6{beta} in Endoplasmic Reticulum Stress Response Gene Induction. J. Biol. Chem. 279: 21078-21084 [Abstract] [Full Text]  
• Euskirchen, G., Royce, T. E., Bertone, P., Martone, R., Rinn, J. L., Nelson, F. K., Sayward, F., Luscombe, N. M., Miller, P., Gerstein, M., Weissman, S., Snyder, M. (2004). CREB Binds to Multiple Loci on Human Chromosome 22. Mol. Cell. Biol. 24: 3804-3814 [Abstract] [Full Text]  
• Gietzen, D. W., Ross, C. M., Hao, S., Sharp, J. W. (2004). Phosphorylation of eIF2{alpha} Is Involved in the Signaling of Indispensable Amino Acid Deficiency in the Anterior Piriform Cortex of the Brain in Rats. J. Nutr. 134: 717-723 [Abstract] [Full Text]  
• Schwieger, M., Lohler, J., Fischer, M., Herwig, U., Tenen, D. G., Stocking, C. (2004). A dominant-negative mutant of C/EBP{alpha}, associated with acute myeloid leukemias, inhibits differentiation of myeloid and erythroid progenitors of man but not mouse. Blood 103: 2744-2752 [Abstract] [Full Text]  
• Rishi, V., Gal, J., Krylov, D., Fridriksson, J., Boysen, M. S., Mandrup, S., Vinson, C. (2004). SREBP-1 Dimerization Specificity Maps to Both the Helix-Loop-Helix and Leucine Zipper Domains: USE OF A DOMINANT NEGATIVE. J. Biol. Chem. 279: 11863-11874 [Abstract] [Full Text]  
• Borkovich, K. A., Alex, L. A., Yarden, O., Freitag, M., Turner, G. E., Read, N. D., Seiler, S., Bell-Pedersen, D., Paietta, J., Plesofsky, N., Plamann, M., Goodrich-Tanrikulu, M., Schulte, U., Mannhaupt, G., Nargang, F. E., Radford, A., Selitrennikoff, C., Galagan, J. E., Dunlap, J. C., Loros, J. J., Catcheside, D., Inoue, H., Aramayo, R., Polymenis, M., Selker, E. U., Sachs, M. S., Marzluf, G. A., Paulsen, I., Davis, R., Ebbole, D. J., Zelter, A., Kalkman, E. R., O'Rourke, R., Bowring, F., Yeadon, J., Ishii, C., Suzuki, K., Sakai, W., Pratt, R. (2004). Lessons from the Genome Sequence of Neurospora crassa: Tracing the Path from Genomic Blueprint to Multicellular Organism. Microbiol. Mol. Biol. Rev. 68: 1-108 [Abstract] [Full Text]  
• Rose, A., Manikantan, S., Schraegle, S. J., Maloy, M. A., Stahlberg, E. A., Meier, I. (2004). Genome-Wide Identification of Arabidopsis Coiled-Coil Proteins and Establishment of the ARABI-COIL Database. Plant Physiol. 134: 927-939 [Abstract] [Full Text]  
• Kamaraju, A. K., Adjalley, S., Zhang, P., Chebath, J., Revel, M. (2004). C/EBP-{delta} Induction by gp130 Signaling: ROLE IN TRANSITION TO MYELIN GENE EXPRESSING PHENOTYPE IN A MELANOMA CELL LINE MODEL. J. Biol. Chem. 279: 3852-3861 [Abstract] [Full Text]  
• Sen, E., Alam, S., Meyers, C. (2004). Genetic and Biochemical Analysis of cis Regulatory Elements within the Keratinocyte Enhancer Region of the Human Papillomavirus Type 31 Upstream Regulatory Region during Different Stages of the Viral Life Cycle. J. Virol. 78: 612-629 [Abstract] [Full Text]  
• Zhang, J.-W., Tang, Q.-Q., Vinson, C., Lane, M. D. (2004). Dominant-negative C/EBP disrupts mitotic clonal expansion and differentiation of 3T3-L1 preadipocytes. Proc. Natl. Acad. Sci. USA 101: 43-47 [Abstract] [Full Text]  
• Richie-Jannetta, R., Francis, S. H., Corbin, J. D. (2003). Dimerization of cGMP-dependent Protein Kinase I{beta} Is Mediated by an Extensive Amino-terminal Leucine Zipper Motif, and Dimerization Modulates Enzyme Function. J. Biol. Chem. 278: 50070-50079 [Abstract] [Full Text]  
• Storlazzi, C. T., Mertens, F., Nascimento, A., Isaksson, M., Wejde, J., Brosjo, O., Mandahl, N., Panagopoulos, I. (2003). Fusion of the FUS and BBF2H7 genes in low grade fibromyxoid sarcoma. Hum Mol Genet 12: 2349-2358 [Abstract] [Full Text]  
• Matsuoka, T.-a., Zhao, L., Artner, I., Jarrett, H. W., Friedman, D., Means, A., Stein, R. (2003). Members of the Large Maf Transcription Family Regulate Insulin Gene Transcription in Islet {beta} Cells. Mol. Cell. Biol. 23: 6049-6062 [Abstract] [Full Text]  
• Newman, J. R. S., Keating, A. E. (2003). Comprehensive Identification of Human bZIP Interactions with Coiled-Coil Arrays. Science 300: 2097-2101 [Abstract] [Full Text]  
• Miller, M., Shuman, J. D., Sebastian, T., Dauter, Z., Johnson, P. F. (2003). Structural Basis for DNA Recognition by the Basic Region Leucine Zipper Transcription Factor CCAAT/Enhancer-binding Protein alpha. J. Biol. Chem. 278: 15178-15184 [Abstract] [Full Text]  
• Gupta, P., Prywes, R. (2002). ATF1 Phosphorylation by the ERK MAPK Pathway Is Required for Epidermal Growth Factor-induced c-jun Expression. J. Biol. Chem. 277: 50550-50556 [Abstract] [Full Text]  

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