©1995 by The American Society for Biochemistry and Molecular Biology, Inc.
Reconstitution of a High Affinity Binding Site for Type I Interferons (*)

(Received for publication, June 8, 1995; and in revised form, August 1, 1995)

Dean Russell-Harde (1) Haifeng Pu (2) Melissa Betts (1) Richard N. Harkins (1) H. Daniel Perez (3) Ed Croze (1)(§)

From the  (1)Departments of Protein Biochemistry and Biophysics, (2)Cell and Molecular Biology, and (3)Immunology, Berlex Biosciences Inc., Richmond, California 94804-0099

ABSTRACT
INTRODUCTION
EXPERIMENTAL PROCEDURES
RESULTS AND DISCUSSION
FOOTNOTES
ACKNOWLEDGEMENTS
REFERENCES

ABSTRACT

The type I interferon (IFN) receptor complex is assumed to be composed of multiple protein subunits. Recently, two proteins have been identified as potential receptor components, both of which share a high degree of structural homology with the immunoglobulin superfamily. One of these proteins, referred to as the human interferon alpha receptor (IFNAR), has been shown to be involved in interferon signal transduction, but it does not bind IFN with high affinity. A second putative receptor protein, named FLP40, has been cloned from human Daudi cells. Transfection of FLP40 into murine NIH 3T3 cells does not result in high affinity IFN binding. In this study, we demonstrate that when expressed in murine L929 cells neither IFNAR nor FLP40 by themselves are capable of binding human IFN-alpha8. Co-expression of IFNAR and FLP40 results in cells capable of binding IFN-alpha8 and IFN-alpha2. Scatchard analysis of binding demonstrated the presence of high (K 350 pM) and low (K 4.0 nM) affinity binding sites. Binding of radiolabeled IFN-alpha8 can be competed with either unlabeled IFN-alpha8 or a recombinant form of human interferon beta, IFN-beta1b, but not with IFN-. Ligand binding of IFN-alpha8 can be inhibited by antibodies directed against IFNAR providing further support for a role for this protein in the formation of a ligand binding site. This is the first demonstration indicating that two previously identified IFN receptor proteins, which individually do not bind type I IFN with high affinity, cooperate in the formation of a type I IFN receptor ligand binding complex.


INTRODUCTION

Ligand-receptor cross-linking experiments (1, 2) suggest that a functional type I interferon (IFN) (^1)receptor complex is comprised of multiple components much like that of the previously described IFN-, interleukins, and granulocyte-macrophage colony-stimulating factor receptor families(3, 4, 5, 6) . However, the identity and mechanism of interaction between proteins comprising the human type I IFN receptor is unclear. Two proteins have recently been identified as potential components of the human type I IFN receptor complex(7, 8) . One, the human interferon alpha receptor (IFNAR) was identified by its ability to reconstitute an antiviral response to IFN-alpha8 in a murine cell line(7, 9) . Monoclonal antibodies directed against the extracellular region of IFNAR have been shown to block the antiviral activity of a number of type I IFNs(10) . It appears, however, that neither human IFNAR nor the purified extracellular domain of IFNAR is able to mediate high affinity binding(11, 12) . Although Daudi cells, from which IFNAR was cloned, bind high levels of type I IFN at 20 °C, murine cells expressing human IFNAR could only be demonstrated to bind ligand at 37 °C in which binding values were expressed as cellular uptake rather that direct receptor binding(7) . Indeed, it was later shown that murine cells expressing IFNAR did not bind detectable levels of type I IFN when ligand binding was measured under conditions which minimized endocytosis(11) . Recent studies in which human IFNAR was expressed in Xenopus laevis oocytes (13) confirmed the notion that IFNAR alone binds type I IFN with very low affinity. Finally, it has been shown that IFNAR becomes phosphorylated by IFN-alpha and IFN-beta but not IFN- in a ligand-dependent manner demonstrating again its involvement in type I IFN signaling(14) .

A second IFN receptor protein, P40, identified by Novick et al.(8) , was purified as a soluble protein from human urine by its ability to bind to an IFN-alpha2 affinity column. A variation of this protein also appears as a membrane-bound form in Daudi cells where it contains a transmembane and cytoplasmic domain(8) . We refer to the membrane-bound form of this protein as full-length P40 (FLP40). Antibodies directed against the soluble form of this protein block the antiviral activity of a number of human type I IFNs on human WISH cells (8) . Although P40 binds to immobilized IFN-alpha2, it appears to do so with only low affinity. This is implied by the observation that the membrane-bound form of this protein when expressed on murine NIH 3T3 cells could only be demonstrated to bind low levels of ligand after extensive cross-linking(8) .

Neither IFNAR nor FLP40 alone appears to be able to act as a receptor capable of high affinity ligand binding. Therefore, it seems likely that in the case of the type I IFN receptor a ligand-induced association between two or more proteins would be required to form a functional type I IFN receptor complex capable of specific high affinity ligand binding. In this report we describe the results of co-expressing IFNAR and FLP40 in a L929 murine cell line. The co-expression of these two proteins in L929 cells results in the formation of a high affinity ligand binding site for human type I IFNs in a cell type initially lacking the ability to bind type I IFNs.


EXPERIMENTAL PROCEDURES

Cell Lines

Human Daudi cells and murine L929 cells were obtained from the American Type Tissue Culture (ATTC). Murine L929 cells were maintained in Dulbecco's modified Eagle's media and Daudi cells in RPMI 1640. Media in both cases were supplemented with 10% fetal bovine serum, 2.0 mML-glutamine, 200 units/ml penicillin, and 60 µg/ml streptomycin. Following transfection, murine cells were selected in media supplemented with 1.5 mg/ml Geneticin (Life Technologies, Inc.) or 0.6 mg/ml hygromycin.

Plasmid Construction and Transfection Protocol

IFNAR cDNA was kindly provided by Dr. Gilles Uzé, Institut de Genetique Moleculaire, CNRS, Montpellier, Cedex 1, France and cloned into a plasmid containing the cytomegalovirus promoter, SV40 origin of replication (pbSER99), and a neomycin gene for resistance to Geneticin (G418). FLP40 was cloned from Daudi cell mRNA using the reverse transcriptase-polymerase chain reaction (PCR). Single-strand cDNA was synthesized from mRNA isolated from Daudi cell using Superscript II (BRL).

Two primers (5`-GCGAGAGCTGCAAAGTTTAATT and 5`-AGAAAACATTGACAAACGAGAAA) corresponding to the 5`- and 3`-untranslated region of P40 (8) were used to generate a full-length form of P40 cDNA (FLP40) by reverse transcriptase-PCR. The PCR fragment was then cloned into pTA vector (Invitrogen). Nucleotide sequence analysis of the cloned cDNA showed two nucleotide changes when compared to the published sequence (8) which resulted in an amino acid change in the signal peptide region (Val to Phe), and one in the intracellular region (Thr to Ala). For expression in mammalian cells, FLP40 cDNA was first cloned into an expression vector (pbSER97) which contains the myeloproliferative sarcoma virus promoter, a hygromycin resistance gene, and an SV40 origin of replication(15) .

L929 cells were transfected using LipofectAMINE according to the protocol from the supplier (5 µg/ml LipofectAMINE for 5 h in Opti-MEM I media) (Life Technologies, Inc.). After transfection, cells were placed in selection media, and individual clones were selected by limited dilution. The resultant cell line expressing only IFNAR was referred to as L929R(1), and L929 cells expressing FLP40 were referred to as L929R(2). For co-expression of both IFNAR and FLP40, murine L929 cells expressing IFNAR (L929R(1) cells) were transfected with pbSER97 containing the FLP40 coding sequence and selected in media containing both Geneticin and hygromycin. The resultant cell line containing both IFNAR and FLP40 was referred to as L929R.

Northern Blot Analysis

Total RNA (10 µg) isolated from stable transformants was electrophoresed through a formaldehyde-containing agarose gel and transferred to nylon membrane. The membrane was hybridized with a specific P-labeled full-length RNA probe (Riboprobe) for FLP40 using conditions described previously (15) and exposed to x-ray film.

Ligand Binding Assay

A phosphorylatable form of human recombinant IFN-alpha8 and IFN-alpha2 were obtained from Pestka Biomedical (16) . All ligands were phosphorylated (specific activities of 60-61.2 µCi/µg) following previously described procedures(16) . Phosphorylated ligands retained full activity after radiolabeling as judged by their ability to generate an antiviral effect on human WISH cells using a cytopathic effect-antiviral assay (not shown). Direct binding assays on Daudi (10^6 cells/ml) and murine L929 (10^5 cells/ml) were performed at 20 °C for 90 min. After ligand binding, Daudi cells were collected by centrifugation through a cushion of silicone oil prior to determination of bound radioactivity. Binding assays using adherent mouse L929 cells were performed on 35-mm dishes in which cells were grown to near confluency. After ligand binding, cells were washed in cold media as described above and solubilized in 2.0% sodium dodecyl sulfate (SDS) prior to scintillation counting. Nonspecific binding was determined by incubation with 100-fold excess unlabeled ligand. Recombinant human IFN-alpha8 was kindly provided by Ciba-Geigy AG, Basel, and recombinant human IFN-beta1b was purified as described previously(17) . Binding data were analyzed according to Scatchard(18) . For neutralization studies using polyclonal antibodies directed against IFNAR, cells were preincubated with preimmune or immune sera (1:100 dilution) for 60 min at 4 °C prior to addition of ligand.

IFNAR Antibody Production

A soluble form of IFNAR was expressed in baculovirus and purified, and the resultant material was used to generate both monoclonal and polyclonal antibodies. The production of monoclonal antibodies recognizing the native form of IFNAR has been described previously(12) . The monoclonal antibody 4B1 was iodinated using the IODOBEADS following procedures described by the manufacturer (Pierce). The polyclonal antiserum used in these studies was developed in rabbits.


RESULTS AND DISCUSSION

Selection of Murine Cells Expressing Type I IFN Receptor Proteins

Mouse L929 cells (L929) have previously been shown not to be able to bind or produce an antiviral response to human type I IFNs at concentrations which induce such responses in human cells(7, 11, 19) . Therefore, this cell line was chosen for transfection studies in which the function of individual human type I IFN receptor subunits could be examined. As a first step in studying the role of IFNAR and FLP40 in ligand binding, stable L929 cell lines expressing only IFNAR (L929R(1)) were generated. The surface expression of IFNAR on L929R(1) cells was confirmed by making use of a monoclonal antibody (4B1) which is specific for human IFNAR (12, 14) . Iodinated 4B1 was used in direct binding studies to demonstrate the presence of IFNAR on the surface of L929R(1) cells (Fig. 1, A and B). Scatchard analysis of binding curves revealed that binding of 4B1 detected 17,000 ± 2000 antibody sites/cell (mean ± S.E., n = 2) on L929R(1) cells. Scatchard analysis of binding curves was also performed on L929R cells (Fig. 1C) and showed that binding of 4B1 (detected (10,234 ± 3,000 antibody sites/cell, mean ± S.E., n = 2). Therefore, L929R(1) and L929R cells express similar amounts of IFNAR on their cell surface. The expression of IFNAR on these cells was also confirmed by fluorescent-activated cell sorting (FACS) analysis using the monoclonal antibody 4B1 (not shown).


Figure 1: Detection of human IFNAR expression on murine L929R(1) and L929R cells using the anti-human IFNAR monoclonal antibody, 4B1. A, binding of increasing concentrations of 4B1 to L929R(1). Specific binding (open circles), nonspecific binding in the presence of 100-fold excess unlabeled monoclonal antibody (closed circles), and binding of I-4B1 to parental L929 cells (squares) is shown. Data represent mean values of n = 2, and variation between replicates was less than 15%. B, Scatchard analysis of I-4B1 binding to L929R(1) (17,000 ± 2000 antibody sites/cell, mean ± S.E., n = 2) C, Scatchard analysis of I-4B1 binding to L929R cells (10,234 ± 3,000 antibody sites/cell, mean ± S.E., n = 2).



Next we generated L929 cell lines expressing either FLP40 (L929R(2)) or both IFNAR and FLP40 (L929R). L929R cells were produced by transfecting into L929R(1) cells a plasmid containing a gene encoding FLP40 as described under ``Experimental Procedures.'' FLP40 mRNA in L929R(2) and L929R cells was confirmed by demonstrating the presence of a 1.5-kb band corresponding to the expected size of FLP40 mRNA (Fig. 2)(8) . As expected, the 4.3-kb band, presumed to represent a soluble truncated receptor(8) , was visible only in blots using Daudi cell mRNA (8) and was not detected in cells transfected with a plasmid containing only the cDNA encoding FLP40. In all L929R cell lines tested (8 individual clones), it appeared that co-expression of IFNAR and FLP40 resulted in an apparent increase in the amount of FLP40 mRNA. A second faint variable band of 3.0 kb was sometimes observed in L919R cells. However, the presence or absence of this band did not correlate with ligand binding. The monoclonal antibody 4B1 was used to confirm that the expression of IFNAR in L929R cells was similar to that observed in L929R(1) cells (Fig. 1).


Figure 2: Northern blot analysis of FLP40 mRNA. Murine L929 (lane 1), L929R(1) (lane 2), L929R (lane 3), L929R(2) (lane 4), and Daudi (lane 5) cells were probed for the presence of FLP40 mRNA. Total RNA (10 µg) from each cell line was electrophoresed through a formaldehyde-containing agarose gel, transferred to a Nylon membrane, and hybridized to a P-labeled full-length FLP40 RNA probe (Riboprobe). A 1.5-kb band, corresponding to the expected size of FLP40, was observed only in cell lines transfected with a plasmid containing a gene encoding this protein (lanes 3 and 4) and Daudi cells (lane 5). A 4.3-kb band was also detected in Daudi cells as described previously(8) . Occasionally, a second 3.0-kb unidentified band was observed in L929R cells (lane 3), the presence of which had no effect on ligand binding. No FLP40 mRNA was detected in either the parental L929 or L929R(1) cells (lanes 1 and 2). Hybridization with a P-labeled actin probe revealed equal RNA loading between lanes (not shown). The 28 S and 18 S ribosomal RNA is indicated.



Human Type I IFN Binding to Murine Cells

L929R(1) and L929R(2) cells were evaluated for their ability to bind IFN by measuring the binding of increasing concentrations (25-750 pM) of phosphorylated IFN-alpha8 and IFN-alpha2 in the presence or absence of 100-fold excess unlabeled ligand (Fig. 3, A and B). We could not demonstrate ligand binding to either L929R(1) or L929R(2) cells. The lack of ligand binding to L929R(1) cells confirms previous results in which the binding of type I IFNs could not be detected in L929 cells expressing IFNAR(11) . Next, we determined the ability of L929R cells, which express both IFNAR and FLP40, to bind labeled ligands. Both IFN-alpha8 and IFN-alpha2 specifically bound to L929R cells (Fig. 3, A and B). Saturation ligand binding could be demonstrated, and Scatchard analysis of the binding data demonstrated the presence of 31,000 ± 5,000 high affinity and 125,640 ± 20,000 low affinity sites/cell (mean ± S.E., n = 2). The K(D) of IFN-alpha8 binding for the high affinity site was 350 pM ± 80 pM (mean ± S.E., n = 2) whereas the K(D) of binding to the low affinity site was 4.5 nM ± 1.0 nM (mean ± S.E., n = 2). The affinity of ligand binding to L929R cells was similar to that observed on Daudi cells(20) .


Figure 3: IFN-alpha8 and -alpha2 binding to L929, L929R(1), L929R(2), and L929R cells. Cell lines were grown to near confluency in 35-mm dishes, and phosphorylated ligand (25-750 pM) was allowed bind to cells for 90 min at 20 °C. Cells were then washed and solubilized, and radioactivity was determined by scintillation counting. Nonspecific binding was determined in the presence of a 100-fold excess of unlabeled IFN. A, binding of IFN-alpha8 was observed in L929R (open circles), but not in L929R(1) (triangles), or L929R(2) (large circles) cells. Nonspecific binding to L929R cells (filled circles) was determined in the presence of a 100-fold excess of unlabeled IFN-alpha8. Inset, Scatchard analysis of IFN-alpha8 binding revealed 31,000 ± 5,000 high affinity and 125,640 ± 20,000 low affinity sites/cell (mean ± S.E., n = 2). The K of IFN-alpha8 binding for the high affinity site was 350 pM ± 80 pM (mean ± S.E., n = 2) whereas the K of binding to the low affinity site was 4.5 nM ± 1.0 nM (mean ± S.E., n = 2). B, binding of IFN-alpha2 was observed in L929R (open circles), but not in L929R(1) (triangles) or L929R(2) (large circles) cells. Nonspecific binding to L929R cells (filled circles) was determined in the presence of a 100-fold excess of unlabeled IFN-alpha8.



Both IFN-alpha8 and IFN-beta1b were able to compete binding of radiolabeled IFN-alpha8 (150 pM) to L929R cells (Fig. 4). Unlabeled IFN-alpha8 exhibited an IC of 500 pM, while unlabeled IFN-beta1b competed for the binding of radiolabeled IFN-alpha8 with an IC of 50 pM. A similar result was observed using Daudi cells (not shown).


Figure 4: Binding of IFN-alpha8 to L929R cells in the presence of unlabeled IFN-alpha8 or human IFN-beta1b. Radiolabeled IFN-alpha8 (150 pM) was allowed to bind to L929R cells in the presence of increasing concentrations of unlabeled IFN-alpha8 (circles) or IFN-beta1b (squares). IFN-beta1b appears to compete for the binding of radiolabeled IFN-alpha8 more efficiently than does IFN-alpha8 itself.



To investigate further the role of IFNAR in the formation of a ligand binding complex, we performed studies using a polyclonal antiserum directed against the extracellular region of IFNAR. This antiserum reacts with IFNAR present on the surface of Daudi, L929R(1) and L929R cells as judged by FACS analysis (not shown). Preincubation of cells with this antiserum inhibited IFN-alpha8 binding to both Daudi and L929R cells by 80-90% (Fig. 5A). A dose-response curve demonstrating the antibody induced inhibition of IFN-alpha8 binding to L929R cells is shown in Fig. 5B. The blocking of ligand binding by the anti-IFNAR antibody supports the suggestion that IFNAR interacts with an additional component(s) which together form a receptor complex that can bind with high affinity either IFN-alpha8, IFN-alpha2, or IFN-beta1b.


Figure 5: Inhibition of IFN-alpha8 binding to Daudi and L929R cells using a polyclonal antibody recognizing IFNAR. A, IFN-alpha8 (250 pM) binding to 10^6 L929R cells/ml and 10^6 Daudi cells/ml was performed in the presence of a polyclonal antiserum (1:100 dilution, solid bars) directed against IFNAR. The antiserum inhibited the binding of phosphorylated IFN-alpha8 to L929R cells (L929R) and Daudi cells. Values shown are the mean for three experimental points ± S.E. Preimmune serum (1:100 dilution, open bars) did not inhibit ligand binding to Daudi or L929R cells. Percent of control binding of IFN-alpha8 is equal to the amount of IFN-alpha8 bound in the absence of antisera. B, dose-response curve for the antibody induced inhibition of IFN-alpha8 (250 pM) binding to L929R cells. Data represent the mean of two experimental points (S.E. ± 10%). Antisera concentration is represented as the log of the dilution.



The data presented here indicate that IFNAR and FLP40 cooperate to form a high affinity ligand binding site for type I IFNs. Previous examples of other cytokine receptors, such as interleukin receptors, suggests this class of cell surface receptors form multicomponent complexes(5, 6, 21) . Such a receptor complex is thought to bring together proteins which act to form a high affinity ligand binding complex. Once this occurs, cytosolic protein kinases (e.g. Jak, Tyk2) are activated and phosphorylate specific tyrosines located within the cytoplasmic C-terminal region of the receptor(22, 23) . The potential interaction between various proteins forming such a receptor have been suggested in structural models for the type I IFN receptor(24, 25) . In line with other known cytokine families, it is likely that the human type I IFN receptor is comprised of multiple protein subunits and that the interaction of these subunits is a prerequisite for ligand binding or signaling. We have tested this hypothesis by first demonstrating that murine cell lines L929R(1) and L929R(2), which stably express either IFNAR or FLP40, respectively, do not specifically bind IFN-alpha8 or IFN-alpha2 at levels detectable by saturation binding. However, when we attempted to establish ligand binding by producing an additional cell line, L929R, expressing both IFNAR and FLP40, we observed specific binding of IFN-alpha8 and IFN-alpha2 to this cell. There are several findings that suggest the possibility that other proteins may be involved in the specific binding of some type I IFNs. First, our finding that IFN-beta1b appears to be more efficient in competition binding than IFN-alpha8 (Fig. 4). Second, the recent description(26, 27) and our finding (28) of a IFN-beta-specific IFNAR-associated surface protein. It appears likely that although IFNAR does not bind ligand with high affinity, it is capable of interacting with other receptor components. Such an interaction between IFNAR and ligand is further suggested by the observation that IFNAR can become phosphorylated in a ligand-dependent manner by both IFN-alpha and IFN-beta.

One final issue to be addressed is that of biological response in our L929R cells. To address this, we are currently investigating the functional response of L929R cells to various human type I IFNs in order to correlate ligand binding with biological activity.

Understanding the process by which these components interact with each other will help to shed some light on the mechanism by which IFNAR and FLP40 form a ligand binding site on L929R cells. Such studies can serve as a starting point for identifying the protein components of the human type I IFN receptor. Studying the mechanism in which receptor proteins assemble to form a multicomponent type I IFN receptor complex in different cells will yield valuable insights into early events of type I IFN signaling in addition to helping define tissue-specific IFN responses.


FOOTNOTES

*
The costs of publication of this article were defrayed in part by the payment of page charges. This article must therefore by hereby marked ``advertisement'' in accordance with 18 U.S.C. Section 1734 solely to indicate this fact.

§
To whom correspondence should be addressed: Dept. of Biochemistry and Biophysics, Berlex Biosciences, 15049 San Pablo Ave., Richmond, CA 94804-0099. Tel. 510-669-4043; Fax: 510-669-4246; ed_croze@berlex.com.

(^1)
The abbreviations used are: IFN, human interferon; IFN-beta1b, human interferon beta in which cysteine 17 has been replaced with a serine; IFNAR, human interferon alpha receptor; FLP40, full-length P40; FACS, fluorescence activated cell sorter; PCR, polymerase chain reaction; kb, kilobase(s).


ACKNOWLEDGEMENTS

We thank Dr. Trey White for performing polymerase chain reaction (PCR) and Joanne Cordova for help in preparing the manuscript.

Note Added in Proof-A paper appeared after the submission of this Communication (29) in which a somewhat similar result in murine NIH 3T3 cells was observed. In agreement with our results, co-expression of IFNAR and FLP40 in murine NIH 3T3 cells generated a high affinity ligand binding site.


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