(Received for publication, April 16, 1997, and in revised form, May 9, 1997)
From the Institute of Biochemistry, University of
Lausanne, BIL Biomedical Research Center, CH-1066 Epalinges,
Switzerland and ¶ Glaxo Institute for Molecular Biology,
CH-1228 Plan-Les-Ouates, Switzerland
The death-inducing receptor Fas is activated when
cross-linked by the type II membrane protein Fas ligand (FasL). When
human soluble FasL (sFasL, containing the extracellular portion) was expressed in human embryo kidney 293 cells, the three
N-linked glycans of each FasL monomer were found to be
essential for efficient secretion. Based on the structure of the
closely related lymphotoxin -tumor necrosis factor receptor I
complex, a molecular model of the FasL homotrimer bound to three Fas
molecules was generated using knowledge-based protein modeling methods.
Point mutations of amino acid residues predicted to affect the
receptor-ligand interaction were introduced at three sites. The F275L
mutant, mimicking the loss of function murine gld mutation,
exhibited a high propensity for aggregation and was unable to bind to
Fas. Mutants P206R, P206D, and P206F displayed reduced cytotoxicity toward Fas-positive cells with a concomitant decrease in the binding affinity for the recombinant Fas-immunoglobulin Fc fusion proteins. Although the cytotoxic activity of mutant Y218D was unaltered, mutant
Y218R was inactive, correlating with the prediction that Tyr-218 of
FasL interacts with a cluster of three basic amino acid side chains of
Fas. Interestingly, mutant Y218F could induce apoptosis in murine, but
not human cells.
The Fas ligand (CD95 ligand) is a 40-kDa type II membrane protein belonging to the tumor necrosis factor (TNF)1 family of proteins (1, 2). This family consists of trimeric ligands that induce defined cellular responses upon binding to their respective receptors. Fas and the other members of the TNF receptor family are type I membrane proteins. They are characterized by the presence of cysteine-rich motives conferring an elongated structure to their extracellular domains (1).
The Fas ligand is one of the major effectors of CD8+ cytotoxic T lymphocytes (3, 4) and natural killer cells (5). It is also involved in the establishment of peripheral tolerance (6), in the activation-induced cell death of lymphocytes (7-10), and in the delimitation of immunoprivileged regions such as the eye and testis (11, 12). Along the lines of this latter feature, cotransplantation of myoblasts engineered to express FasL can protect an islet allograft from rejection (13). The loss of function due to mutations in murine Fas ligand (gld), murine Fas (lpr), human Fas, or human FasL leads to lymphoproliferation, lymphadenopathy, and autoimmune diseases (14-18). Fas-null mice have a similar but more severe phenotype (19).
The Fas-FasL system is implicated in a number of pathogenesis. Abnormally elevated levels of soluble Fas ligand are detected in leukemia/lymphomas of T and natural killer cells, and in an aggressive nasal lymphoma (20, 21). Various tumor cells express FasL, therefore potentially creating their own immunoprivileged sites (22-24). The Fas/Fas ligand system is also involved in the CD4+ T cell deletion observed in human immunodeficiency virus-infected individuals (25-27), in multiple sclerosis (28), and in acute graft-versus-host disease (29, 30).
Membrane-bound Fas ligand can be processed into a soluble form by a
metalloprotease whose inhibitor profile is similar to that of the
protease solubilizing TNF (20, 31-34). The soluble forms of the TNF
family members that have been crystallized so far include TNF
(35),
lymphotoxin
(also known as TNF
) (36), and CD40L (37). They all
share a similar conformation resulting in a compact, pear-shaped
trimeric structure. Other family members (Fas ligand (38), TRAIL (39),
CD30L, CD27L, OX40L, and 4-1BBL) show clear sequence homology at the
amino acid level, and there is little doubt that they are all
trimeric.
In this study, we produce biologically active human soluble Fas ligand (sFasL) and amino acid residues essential for the Fas/FasL interaction are identified. We also demonstrate the importance of extensive N-glycosylation for the efficient secretion of FasL.
Materials
The anti-flag M2 monoclonal antibody and the anti-flag M2 antibody coupled to agarose were purchased from Integra Biosciences (Wallisellen, Switzerland). Protein A-Sepharose was purchased from Pharmacia (Uppsala, Sweden). Tunicamycin and Protein A were obtained from Sigma (Buchs, Switzerland). Peptide N-glycanase F was purchased from New England Biolabs (Schwalbach, Germany). The PCR-2 TA cloning vector and PCR-3 mammalian expression vector were obtained from InvitroGen (NV Leek, the Netherlands). Cell culture media and antibiotics were obtained from Life Sciences (Basel, Switzerland). The non-radioactive cell proliferation assay was purchased from Promega (Wallisellen, Switzerland). The fusion protein muFas-Fc was kindly provided by Dr. C. A. Smith (Immunex, Seattle, WA).
Cells
Murine B lymphoma A20 cells were grown into DMEM containing 5% heat-inactivated fetal calf serum (FCS) and the human T lymphoblastoma Jurkat cell line was grown in RPMI supplemented with 10% FCS. Human embryonic kidney 293 cells (ATCC CRL 1573) were cultured in DMEM:nutrient mix F-12 (1:1) supplemented with 2% FCS. Human embryonic kidney 293 cells stably transfected with the large T antigen of SV40 (293T cells, kindly provided by Dr. M. E. Peters, German Cancer Research Center, Heidelberg, Germany) were grown in DMEM supplemented with 10% FCS. All media contained antibiotics (penicillin and streptomycin at 5 µg/ml each and neomycin at 10 µg/ml).
Expression Vectors for the Recombinant sFasL and the Soluble Human Fas-Human Immunoglobulin Fc Chimera
sFasLA DNA fragment coding for the signal peptide of
hemaglutinin, including 6 bases of its 5-untranslated sequence (40),
the flag epitope (41), a linker (GPGQVQLQ), and the PstI,
SalI, XhoI, and BamHI restriction
sites, was cloned between the HindIII and BamHI
sites of a modified PCR-3 vector in which nucleotides 720-769 had been
deleted. This plasmid was called pHAflag-038. The full-length cDNA
of human Fas ligand was amplified by PCR from the cDNA of activated
peripheral blood lymphocytes (oligonucleotides: 5
-CCTCTACAGGACTGAGAAGAAG-3
and 5
-CAACATTCTCGGTGCCTGTAAC-3
), and
cloned into PCR-2 TA cloning vector. This plasmid was used as PCR
template for the amplification of a portion of the extracellular domain
of the FasL (amino acids 139-281) with suitable restriction sites
added at each end. The resulting PstI/EcoRI
fragment was inserted into pHAflag-038, in frame with the flag
sequence.
For each point mutation, a set of complementary oligonucleotides
containing the target mutation was used. In the first round of the PCR,
two products were produced with pHAflag-FasL as template using:
(a) the forward oligonucleotide and Sp6 primer, and
(b) the reverse oligonucleotide and T7 primer. Purified PCR
products, containing the 3 and 5
portions of FasL, respectively, were mixed and allowed to undergo three cycles of PCR before amplification with T7 and Sp6 primers. The PstI/EcoRI fragment
of the resulting PCR product was cloned into pHAflag-038.
The extracellular domain of hFas (GenBank X63717,
nucleotides 24 to 510, the A of ATG being nucleotide 1) with 5
HindIII and 3
SmaI sites was amplified by PCR
from a full-length cDNA clone (kindly provided by Prof. P. H. Krammer, German Cancer Research Center, Heidelberg). The
HindIII-SmaI fragment was cloned between the
HindIII and EcoRV sites of a modified PCR-III
vector containing an added SalI site after the existing
EcoRV site. A SalI/NotI cDNA
cassette encoding the hinge, CH2, and CH3 domains (amino acid residues
231-447) of human IgG1 (42) was cloned in frame at the 3
end of the
extracellular domain of Fas. Both strands of each construct were
checked by sequencing.
Expression of sFasL and hFas-Fc
Plasmids were either expressed transiently in 293T cells or stably in 293 cells. Plasmids (10 µg) were transfected by the calcium phosphate method (3 × 105 cells/28-cm2 plate) in HEPES buffer (43). After transfection, cells were grown for 48-72 h in serum-free Opti-MEM medium, and supernatants were harvested. Stably transfected 293 cells were obtained by selection in 800 µg/ml G418 (70% active) for 2 weeks and cloned at that stage. Supernatants of stably transfected clones were harvested after 10-12 days in culture and screened by Western blotting or receptor binding ELISA (see below) for expression levels.
Peptide N-Glycanase F Digestion of sFasL
293 cells (2 × 105) transiently transfected with sFasL and their corresponding supernatants (20 × concentrated, 15 µl) were heated in 20 µl of 0.5% SDS, 1% 2-mercaptoethanol for 3 min at 95 °C. Samples were cooled and supplemented with 10% Nonidet P-40 (2 µl) and 0.5 M sodium phosphate, pH 7.5 (2 µl). Peptide N-glycanase F (125 units/µl, 1 µl) was added (or omitted in controls), and samples were incubated for 3 h at 37 °C prior to analysis by Western blotting.
Purification of sFasL and hFas-Fc
Supernatants of stably transfected cells were filtered using a 0.22-µm membrane and loaded as 40-ml aliquots onto 1-ml columns of anti-flag M2 agarose (for sFasL) or Protein A-Sepharose (for hFas-Fc) equilibrated in PBS. The columns were washed with 10 ml of PBS and eluted with 2.5 ml of 50 mM citric acid. The eluate was neutralized with 1 M Tris base, concentrated, and exchanged into PBS using Centriprep-30 concentrators. Protein concentration was determined by the bicinchoninic acid method (Pierce) using bovine serum albumin as the standard, and the purity of the samples was assessed by SDS-PAGE and Coomassie Blue staining.
SDS-PAGE and Western Blotting
SDS-PAGE and Western blotting were performed on 12% mini gels according to previously published methods (44, 45). Blots were incubated with anti-flag M2 monoclonal antibodies (5 µg/ml, 0.02% NaN3, in blocking buffer: PBS, 0.5% Tween 20, 4% skim milk), followed by rabbit anti-mouse immunoglobulins coupled to horseradish peroxidase (diluted 1:2000 in blocking buffer). Peroxidase activity was detected by enhanced chemiluminescence.
Inhibition of N-Glycosylation with Tunicamycin
Tunicamycin was stored at 70 °C at a concentration of 1 mg/ml in 10 mM Tris-HCl, pH 9. Stably transfected cells
secreting sFasL were grown for 10 days in the presence of 1, 100, or
1000 ng/ml tunicamycin. Cells and supernatants were harvested and
analyzed by Western blotting.
Cytotoxic Assay
A20 or Jurkat cells (100 µl, 50,000 cells, in 96-well plates) were incubated at 37 °C in the presence of sFasL at the indicated concentrations and 1 µg/ml M2 monoclonal antibody. In some experiments, hFas-Fc or muFas-Fc was added at the indicated concentrations in the presence of 1 µg/ml Protein A. Four to 8 h after the addition of FasL, 20 µl of a solution containing 2 mg/ml 3-(4,5-dimethylthiazol-2-yl)-5-(3-carboxymethoxyphenyl)-2-(4-sulfophenyl)-2H-tetrazolium, inner salt (MTS) reagent (Promega) and 50 µg/ml phenazine methosulfate was added to the cells. Following color development (2-4 h), absorbance at 490 nm was taken with an ELISA reader.
In Vitro Fas-FasL Binding Assay
96-well ELISA plates (Nunc Maxisorp) were coated with either hFas-Fc or muFas-Fc (1 µg/ml in PBS, 100 µl, 2 h, 37 °C). The following incubation and washing steps were performed: (a) saturation in block buffer (PBS, 5% FCS, 300 µl, 1 h, 37 °C), (b) three washes (PBS, 0.05% Tween-20), (c) incubation with sFasL (10-1000 ng/ml in PBS containing 50 µg/ml bovine serum albumin, 100 µl, 1 h, 37 °C), (d) three washes, (e) incubation with M2 monoclonal antibody (1 µg/ml in block buffer, 100 µl, 37 °C, 30 min), (f) three washes, (g) incubation with rabbit anti-mouse IgG coupled to peroxidase (1/1000 dilution in block buffer, 100 µl, 30 min, 37 °C), (h) three washes, (i) detection (0.3 mg/ml o-phenylenediamine hydrochloride, 0.01% H2O2 in 50 mM citric acid, 100 mM Na2HPO4, 200 µl, as necessary (1-5 min), 25 °C), and (j) termination (2 N HCl, 50 µl). Absorbance was taken at 490 nm with an ELISA reader.
Gel Permeation Chromatography
sFasL samples (5 µg in 100 µl) were mixed with the internal standards catalase and ovalbumin, then loaded onto a Superdex-200 HR10/30 column, and the proteins were eluted in PBS at 0.5 ml/min. Fractions (0.25 ml) were analyzed using the receptor binding ELISA (using 5 µl of fractions for active ligands), and Western blotting was carried out after trichloroacetic acid precipitation of the entire fraction. The column was calibrated with standard proteins: thyroglobulin (669 kDa), ferritin (440 kDa), catalase (232 kDa), aldolase (158 kDa), bovine serum albumin (67 kDa), ovalbumin (43 kDa), chymotrypsinogen A (25 kDa), and ribonuclease A (13.7 kDa).
Protein Modeling
Molecular models for both Fas and FasL were generated using
knowledge-based protein modeling methods as implemented in the Swiss-Model server (46, 47). A molecular model for FasL was built using
the known tridimensional structures of both TNF (48) and lymphotoxin
(TNF
) (49) (Protein Data Bank entries 1TNF and 1TNR chains A, B,
and C) (50). The known structure of the 55-kDa tumor necrosis factor
receptor (51) was used to produce a molecular model for Fas. In both
cases, the modeling procedure was started by submitting the respective
protein sequences to Swiss-Model via the First Approach Mode. The
resulting models were then used to correct the automated multiple
sequence alignments generated by the server in several loop regions.
These corrected alignments were resubmitted to Swiss-Model through the
Optimize Mode. The resulting models were structurally sound, and did
not show obvious sequence or structure inconsistencies (51) according to three-dimensional/one-dimensional profiles (52) and ProsaII (53).
The quaternary structure of the Fas-FasL complex was generated using
the x-ray structure of the human lymphotoxin
-TNF receptor I complex
(54). Three copies of the ligand model and three copies of the receptor
model were superimposed onto the corresponding subunits of the
experimental structure. The hexameric protein complex was further
refined by 200 cycles of energy minimization with CHARMM (53). The
three N-glycosylation sites are located at Asn-184, Asn-250,
and Asn-260 in the FasL model. A short branched N-linked
glycan structure
(GlcnAc
1-4Man
1-6[Man
1-3]Man
1-4GlcNAc
1 -4GlcNAc)
was extracted from Brookhaven Protein Data Bank entry 9API, and was
linked to the respective asparagines using interactive graphics.
A plasmid encoding the signal peptide
of hemaglutinin, in frame with a flag epitope and the COOH-terminal
portion of the extracellular domain of human Fas ligand (amino acids
139-281), was transfected into the human embryonic kidney 293 cell
line. Secreted sFasL was affinity-purified using immobilized anti-flag
antibodies. The theoretical molecular mass of the encoded recombinant
protein is 18.2 kDa. Purified sFasL migrated as a doublet on SDS-PAGE with deduced molecular masses of 29 and 25.5 kDa (Fig.
1A). Taken together with previous data (55),
this heterogeneity and the discrepancy between predicted and observed
molecular masses suggest that carbohydrates are present on the sFasL.
Indeed, sFasL present in both cell extracts and cell supernatants could
be digested with peptide N-glycanase F to a single band with
the predicted molecular mass of 18 kDa (Fig. 1B), indicating
that the various species of sFasL differed by their degree of
N-glycosylation. This result was confirmed when cells were
treated with the N-glycosylation inhibitor tunicamycin; a
dose-dependent accumulation of cellular, unglycosylated
18-kDa sFasL was observed with concomitant loss of sFasL secretion
(Fig. 1C). A total of four evenly spaced bands of sFasL
could be detected, which probably correspond to the unglycosylated, mono-, di-, and tri-N-glycosylated sFasL monomers. Thus, all
three potential N-glycosylation sites of human FasL
(Asn-184, Asn-250, and Asn-260) appear to be used. Interestingly,
secreted sFasL is consistently found in its highly glycosylated form,
even at intermediate tunicamycin concentrations where unglycosylated
sFasL is by far the predominant cellular species (Fig. 1C).
This strongly suggests that N-linked oligosaccharides are
required for efficient secretion of sFasL.
We next generated a molecular model of the FasL-Fas complex (Fig.
2) using knowledge-based protein modeling methods and
the known tridimensional structures of lymphotoxin (TNF
) and the 55-kDa tumor necrosis factor receptor (49). It can be seen that the
N-linked oligosaccharides are concentrated on the lateral edge of each FasL monomer, leaving vertical clefts, which would allow
the receptor to reach the interaction site of the ligand.
Two of the three glycosylation sites of the FasL have counterparts in
other family members. Residue Asn-260 of FasL is also found at the
corresponding position in lymphotoxin , CD27L, and CD40L, whereas
residue Asn-250 of FasL corresponds to a site in CD30L. In some TNF
family members, N-glycosylation appears to be important for
the biological activity of the protein. For example, FasL, which can be
expressed in a variety of eukaryotic systems (20, 56, 57), forms
inactive inclusion bodies when expressed in
bacteria.2 The extensively glycosylated
CD30L (four putative N-glycosylation sites) is also best
produced in a recombinant form in eukaryotic systems (57). Glycosylated
recombinant CD40L is readily expressed at the surface of eukaryotic
cells, but transport to the cell surface is blocked in the presence of
the N-glycosylation inhibitor tunicamycin (57). In contrast,
TNF
(58) and lymphotoxin
(59) can be produced in a soluble,
non-glycosylated and active form in prokaryotic expression systems.
When these two latter ligands are expressed in eukaryotic systems,
N-glycosylation can result in minor effects such as a
10-fold decrease in specific activity of TNF
(60) or the masking of
epitopes recognized by neutralizing antibodies for lymphotoxin
(61). This supports the conclusion that N-glycosylation can
be important for the efficient secretion of FasL and other glycosylated
ligands of this family.
The
availability of an efficient system for the production of recombinant
sFasL allowed us to test the validity of the structural model of the
Fas-FasL by generating a number of mutants (Fig. 3). A
well characterized spontaneous mutation (F273L) in murine FasL, called
gld, abolishes FasL activity and results in a phenotype of
generalized lymphoproliferative disease (15). The mutant F275L was
engineered to test whether an analogous mutation would also inactivate
human FasL (Fig. 3A). The yield of F275L sFasL secretion was
low compared with wild type sFasL, but its molecular weight suggested
that it was completely N-glycosylated (Fig.
4A, lane F275L). The F275L
mutation had a severe effect on the cytotoxic activity of sFasL, which
was reduced by more than 5 orders of magnitude compared with wild type
(Fig. 4B). These results raised the question of whether the
F275L mutant was properly folded and trimerized. Therefore wild type
and mutated FasL were analyzed by gel permeation chromatography. Wild
type FasL eluted as a defined peak with an apparent molecular mass of
79 kDa (corresponding to a 2.7-mer), whereas the F275L mutant eluted
broadly throughout the profile (Fig. 5). It is
conceivable that this mutation, occurring at the hydrophobic interface
of two monomers (62), prevents correct association of otherwise
properly folded monomers leading to uncontrolled association and
impairment of binding to Fas. Interestingly, FasL is normally expressed
at the surface of activated T-lymphocytes from gld mice
(62), raising the question of whether the structural impact of the
gld mutation is less severe in the murine protein as
compared with human FasL.
Amino Acid Residues Pro-206 and Tyr-218 of FasL Are Important for the Interaction with Fas
Due to their predicted close proximity
to the receptor (Fig. 6), amino acids Pro-206 and
Tyr-218 were chosen for mutagenesis. The mutants P206F, P206D, and
P206R were secreted and glycosylated (Fig. 4A), and were
between 100-fold (for P206F) and 500-fold (for P206D) less active than
wild type FasL (Fig. 4B). The binding of the FasL to Fas was
determined in vitro with a Fas-FasL interaction ELISA. In
this assay, recombinant FasL is captured by chimeric Fas-Fc coated on
plastic, and the interaction is detected by antibody binding to the
flag epitope present at the NH2 terminus of the sFasL (Fig.
7). The binding affinity was strong for wild type FasL,
weak yet significant for the Pro-206 mutants, and equal to background
for the F275L "gld" mutant, correlating with their respective potency to induce apoptosis in target cells. These results
suggest that the Pro-206 residue of the FasL is directly involved in
the Fas-FasL interaction, although we cannot formally exclude that the
observed phenotype is the result of the structural impact of the
mutation on FasL.
Tyr-218 is located in a loop between -strands D and E of the FasL
(Figs. 3B and 6). This residue is conserved among a number of ligands, including all known death-inducing ligands (Fig.
3B). This is a remarkable feature, as loop residues are
normally highly variable between family members. Moreover, this
tyrosine residue is known to be essential for lymphotoxin
(TNF
)
and TNF
binding to TNF-receptor I (49, 59, 63).
Surprisingly, the Y218D mutant and the wild type FasL have similar
abilities to kill both murine and human target cells (Fig. 4B) and to bind to recombinant Fas of both species (Fig.
7B). This is, however, in sharp contrast with the Y218R
mutant, which is 4 orders of magnitude less active than wild type FasL
on murine cells, and which displays impaired binding to Fas (Figs.
4B and 7B). This latter mutant is, however, very
similar to wild type FasL by other criteria such as secretion
efficiency, glycosylation, and size as determined by gel permeation
chromatography (Fig. 4A and data not shown). The region of
Fas interacting with Tyr-218 is rich in basic amino acid residues (Fig.
8). The phenol group of the tyrosine is therefore likely
to form hydrogen bonds with Fas, and could even exist as phenolate in
this environment to form a salt bridge with Fas. In this context,
changing the Tyr residue for a negatively charged Asp residue can be
considered as a conservative mutation. In contrast, mutation of the Tyr
residue for a positively charged Arg residue (Y218R) will not only
disrupt the existing interactions but will add a detrimental
electrostatic repulsion leading to the observed greatly impaired
cytotoxic phenotype.
It has been shown recently that the amino acid residue Arg-86 (but not Lys-78) of Fas is essential for ligand binding (64). Taken together with our results, this suggests that a strong interaction takes place between Tyr-218 of FasL and Arg-86 of Fas (Fig. 8).
The Y218F sFasL Mutant Specifically Interacts with Murine but Not Human FasThe effect of the Y218F mutation on sFasL should be
intermediate between that seen for the Y218D and Y218R mutations
described above, since the positive interaction of the phenol group of
Tyr-218 with Fas should be lost without generating additional
repulsion. As expected from this model, the Y218F mutant of FasL
displays intermediate cytotoxic activity (Fig. 4B).
Interestingly, the cytotoxic effect of this mutant is markedly
dependent upon the species from which the receptor derives, which is in
contrast with the documented complete cross-reactivity between wild
type human and murine FasL and Fas (38). The Y218F mutant is relatively potent at killing murine target cells and is apparently inactive on
human target cells (Fig. 4B). This species specificity is
also evident at the level of recombinant Fas binding (Fig. 7). This suggests that the binding of the sFasL to murine Fas relies on more
frequent, or more stable interactions than to human Fas. Destroying the
Tyr-218 interaction site is therefore less detrimental for murine Fas
binding activity than for human Fas. A list of Fas residues, which are
likely to be involved in FasL binding but which are different between
both species, is given in Table I. This difference in
activity between murine and human Fas was not due to the presence of an
Asp-74 in murine Fas instead of a Ser-83 in human Fas (Table I and data
not shown). Similar effects of specificity restriction have been
observed in TNF, where point mutations induced marked specificity
for either TNF-R1 or TNF-R2 (58).
|
If the Y218F sFasL mutant is species-specific, it should be able to
exert its cytotoxic effect on murine target cells even in the presence
of an excess of soluble recombinant human Fas, but should be inhibited
by recombinant murine Fas. In contrast, wild type sFasL should be
inhibited by recombinant Fas from both species. To confirm this point,
murine target cells were exposed to a lethal dose of either wild type
or Y218F sFasL, in the presence of increasing amounts of recombinant
human or murine Fas-Fc fusion proteins (Fig. 9). As
predicted, Y218F sFasL was inhibited by murine Fas-Fc but left
practically unaffected by human Fas-Fc. In contrast, wild type sFasL
was inhibited by both fusion proteins (Fig. 9). This experiment
demonstrates the strong (however not absolute) species specificity of
Y218F sFasL toward murine Fas.
In summary, we have found that the N-glycosylation of sFasL is required for its solubility, and we describe a method for its production and purification. The availability of sFasL (and its inhibitor Fas-Fc) will prove useful to study a variety of systems in which Fas and FasL are implicated. In addition, the model that we presented here allowed us to successfully design mutations affecting the binding of FasL to Fas, and should therefore facilitate the design of specific inhibitors of Fas-FasL inhibitors.
We are grateful to Dr. D. Rimoldi for providing us with human activated PBL cDNA and to S. Belli for careful reading of the manuscript.