By
From the Department of Molecular and Cell Biology and Cancer Research Laboratory, 489 Life Sciences Addition, University of California at Berkeley, Berkeley, California 94720
The Ly49 natural killer (NK) cell receptors are class I MHC-specific inhibitory receptors that are distributed to overlapping NK cell subsets. The formation of the Ly49 receptor repertoire was examined with transgenic mice that express Ly49A in all NK cells. In MHC class I-deficient mice, the Ly49A transgene did not prevent expression of endogenous Ly49 genes. However, in H-2d mice that express a Ly49A ligand, the transgene caused clear alterations in the endogenous Ly49 repertoire. The frequency of NK cells expressing another H-2d-specific receptor, Ly49G2+, was substantially reduced. Reduced numbers of cells expressing endogenous Ly49A was suggested by reduced endogenous Ly49A mRNA levels. These results support the existence of an MHC-dependent education process that limits the number of NK cells that coexpress multiple self-specific Ly49 receptors. Ligand-dependent downregulation of Ly49 cell surface levels was also examined. Cell-surface downregulation occurred even when the transgene was expressed at low levels. The results demonstrate that downregulation of Ly49A cell surface levels is a posttranscriptional event, and argue against a model in which Ly49 receptors are calibrated to specific cell surface levels depending on the available class I ligands.
NK cells recognize a variety of target cells, including
tumor cells, cells infected with some viruses or bacteria, and some normal cells. A critical determinant of target
cell recognition by NK cells is the MHC class I expression
pattern of the target cell. NK cells are equipped with receptors that display specificity for allelic variants of MHC
class I molecules. In the human, these receptors have been
identified as a family of proteins with homology to immunoglobulins (1). In the mouse, the class I-specific receptors are encoded by at least nine closely related genes which encode C type lectin-like Ly49 receptors (Ly49A-I) (5).
The expression of Ly49 receptors is restricted to NK cells
and a small subset of T cells (5). Monoclonal antibodies
have been generated against the Ly49A, Ly49G2, and
Ly49C/I receptors. Each of these antibodies defines a subpopulation of 20-50% of total NK cells. Coexpression of
two or more receptors is quite common, as many NK cells
can be costained with two or even all three antibodies (7,
9). The common coexpression of two or more receptors results in a complex Ly49 repertoire, despite the relatively small number of receptors.
The specificities of some Ly49 receptors have been investigated. The Ly49A receptor is specific for Dd and Dk
class I molecules (13). The Ly49G2+ subset is inhibited by
target cells expressing Dd or Ld (10). The SW-5E6 mAb was
originally thought to specifically define the Ly49C receptor
(7, 11). However, recent evidence indicates that in B6
mice, SW-5E6 binds to both Ly49C and Ly49I (16). Based
on cell binding studies, Ly49C binds to both H-2b and H-2d
class I molecules, and Ly49I may bind to neither (16).
The distribution of Ly49 receptors to distinct, albeit
overlapping, NK cell subsets has important biological consequences. In normal H-2b mice, where ~20% of NK cells
express Ly49A, lysis of H-2d target cells is accomplished by
Ly49A Little is known concerning the mechanisms that impose
subset-specific expression of Ly49 receptors. We recently
reported that most NK cells in Ly49A heterozygous mice
that express the Ly49A gene express only one or the other
Ly49A allele (9). Monoallelic expression of Ly49 genes can
be accounted for by a number of different models. Ly49
gene expression may be regulated by a feedback mechanism wherein the expression of Ly49A from one allele prevents expression of the other Ly49A allele. Such a mechanism could have evolved to prevent the coexpression of
two allelic Ly49 receptors with distinct specificities. Indeed, Ly49 genes exhibit allelic sequence polymorphism
(9, 16). However, it is difficult to understand why coexpression of both alleles at the same locus would be prevented in NK cells, when coexpression of different Ly49
genes in the same cell is quite frequent. An alternative explanation of monoallelic expression of Ly49 genes is that it
reflects the outcome of a more general process that distributes the expression of Ly49 receptors to different NK cells.
It was proposed that a process governing receptor expression imparts a specific probability of stable activation to
each Ly49 allele in individual NK cells (9, 19). Most Ly49A+ NK cells would thus express only one or the other
Ly49A allele; a smaller number would simultaneously express both alleles.
Whatever the mechanisms that generate clonal diversity
of Ly49 receptor expression in NK cells, it is likely that
they are coordinated with "education" processes that adapt
NK cells to the MHC environment in which they develop.
Indeed, the results of functional experiments suggest that
the NK cell population is adapted to the MHC molecules
of the host (20). It was postulated that the education
process ensures that each NK cell expresses at least one inhibitory receptor specific for at least one self-MHC class I
allele, to avoid autoimmunity. Consistent with this hypothesis, cultured Ly49A+ NK cells isolated from H-2b mice
were tolerant of H-2b lymphoblast target cells, whereas
Ly49A+ NK cells from H-2d mice efficiently lysed H-2b
target cells (25, 26). Both populations of NK cells lysed class I-deficient lymphoblasts equivalently, indicating that
the Ly49A+ cells from H-2b mice were not simply anergic.
Furthermore, antibody fragments specific for Ly49A did
not restore lysis of H-2b target cells by Ly49A+ NK cells
from H-2b mice, suggesting that inhibition was not mediated through Ly49A, and therefore that these NK cells expressed additional, H-2b-specific receptors compared to the
Ly49A+ NK cells from H-2d mice (26). Consequently, although definitive evidence has not yet been obtained, it
seems that each functional NK cell expresses at least one
self class I-specific Ly49 receptor.
In addition to the functional evidence discussed above,
we have reported that expression of MHC class I molecules
affects the frequencies of Ly49-defined subsets. NK cells
that matured in an environment of low MHC class I expression in MHC class I molecules affect not only the frequencies of
cells expressing specific Ly49 receptors, but also the cell surface levels of Ly49 receptors. Studies performed with Ly49A
(13, 25) and Ly49G2 (12) indicated that these receptors are
expressed at lower cell surface levels in the presence of their
inhibitory MHC ligand compared to its absence. This finding led to the suggestion that a developmental process calibrates the expression level of the inhibitory receptor to the
respective MHC environment, allowing NK cells to detect
small alterations in the levels of self-class I molecules (25).
The hypothesis that an education process limits the
numbers of cells that express multiple self-specific Ly49 receptors leads to the prediction that expression of a Ly49A
transgene in all NK cells of H-2d mice will result in a reduced frequency of cells expressing endogenous receptors
of the same specificity. Here we have tested this hypothesis. Expression of an Ly49A transgene causes a reduction in the
usage of a second H-2d-specific Ly49 receptor in H-2d
mice, but not in class I-deficient mice, strongly supporting the existence of an education process that limits Ly49 receptor coexpression. Furthermore, we used the transgenic
mice to test the hypothesis that monoallelic expression of
Ly49A genes is the result of a mechanism wherein the
mere presence of Ly49A protein expressed from one allele
prevents expression of the other Ly49A allele. It was observed that the ubiquitously expressed Ly49A transgene did
not prevent expression of the endogenous Ly49A gene in class
I-deficient mice, arguing against this model. The transgenic mice also provide a means to investigate the mechanisms that underlie the reduction of Ly49A levels observed
in mice that express Ly49 ligands. The results indicate that
the ligand-induced reduction in Ly49A levels is largely determined by a posttranscriptional process, and that downregulation is observed, even when the levels of transgeneencoded Ly49A are low to begin with. These results argue
against a model in which Ly49A levels are adjusted to a specific level depending on ligand binding.
Mice.
B10.D2/oSnJ were purchased from the Jackson Labs
(Bar Harbor, ME) or the National Cancer Institute (Frederick,
MD). C57BL/6J (B6) mice were bred in the animal facility of the
University of California (Berkeley, CA). Class I MHC-deficient
(B6 Generation and Analysis of Ly49A Transgenic Mice.
The generation of Ly49A transgenic mice is described in detail elsewhere
(18). In brief, a Ly49A cDNA clone was isolated from the C57/
BL6 (B6)-derived thymoma EL-4 using reverse transcriptase PCR with Ly49A-specific primers (9). The Ly49A cDNA clone
was subcloned into the class I promoter expression cassette (27) and injected into fertilized (B6 × CBA/J)F2 eggs to generate
transgenic mice.
NK cells (17). Expression of Ly49A in all NK cells
from a transgene prevented H-2b mice from rejecting H-2d
bone marrow grafts in vivo, and from lysing H-2d tumor
target cells in vitro (18), presumably because each NK cell
was inhibited when it encountered Dd-expressing cells.
Thus, the restriction of inhibitory Ly49 receptor expression
to subsets of NK cells is a necessary condition to observe
allo-aggression in the NK cell compartment. By the same reasoning, subset-specific expression of Ly49 receptors is
likely to be necessary for NK cells to attack self cells that
have extinguished expression of some, but not all, class I
molecules as a consequence of infection or mutation.
2m
/
mice included a higher frequency of
cells expressing two or three different Ly49 receptors than
did NK cells from normal
2m+ mice (12). Moreover, it
was observed that NK cells expressing multiple H-2d-specific Ly49 receptors were significantly less frequent in H-2d
mice that express the corresponding inhibitory MHC
ligand, than in H-2b mice (12). These observations suggested that an education process dependent on class I MHC
limits the number of different Ly49 receptors expressed by
individual NK cells.
2m
) mice were established by backcrossing (129/Sv × B6)F1
2m
mice to B6 mice five times and intercrossing.
2m
/
mice to generate
2m-deficient Ly49A transgenics. In
the experiments shown here, all mice used were hemizygous for
the Ly49A transgene, had been backcrossed three times to the
B6/B10 background, the MHC haplotypes were H-2b/b, H-2b/d,
H-2d/d, or
2m
/
, as indicated, and the NK complex on chromosome 6 was always homozygous of B6 origin.
Flow Cytometry.
Spleen cell suspensions from individual mice
were passed over nylon wool columns and nonadherent cells (5 × 105) were stained with PE-labeled goat anti-mouse IgG (Southern Biotechnology Assoc., Birmingham, AL). Free binding sites
were saturated with mouse IgG. Cells were further stained with
PE-conjugated anti-CD3 (PharMingen, San Diego, CA) and biotinylated PK136 (anti-NK1.1). After washing, the cells were incubated with a mixture of streptavidin-Tricolor (CALTAG, San
Francisco, CA) plus FITC-labeled JR9-318 (JR9; anti-Ly49A), SW5E6 (anti-Ly49C), or 4D11 (anti-Ly49G2). In general, 5 × 104-105 events were analyzed on a flow cytometer (EPICS XL;
Coulter Corp., Hialeah, FL). Expression of Ly49 receptors on
NK cells was assessed by gating on NK1.1+CD3 Ig
cells.
Graphics were generated using the WindMDi software (John Trotter, Salk Institute, La Jolla, CA).
Ribonuclease Protection Assay.
The 3 portion of Ly49A cDNA
(position 783-1162, reference 30), most of which is not included
in the Ly49A transgene construct (903-1162), and an NK1.1
(NKR-P1C) fragment (207-620, clone No. 40, reference 31),
were obtained by PCR from B6 A-LAK cDNA using the following Ly49A- and NKRP1-specific PCR primers, respectively: Ly49A, 804 sense: GGAAATACAATATAAGAGATGGG; 1143 antisense: CAAATAAAACAGATTCGTCC; NKR-P1 (NKRP1A and C), 207 sense: ACACAGGTTGGCTCTGAAGC, and
(NKR-P1B and C), 680 antisense: ACTTTRTCTCCTRAGATGGWG.
We have generated transgenic mice expressing a Ly49A cDNA of B6 origin, driven by the class I promoter and the immunoglobulin enhancer. A previous analysis of an H-2b transgenic
line (line No. 2) with a high (>15) transgene copy number
demonstrated that the transgenic Ly49A receptor was expressed on the surface of essentially all NK cells, T cells,
and B cells, and the level of expression was similar to that
of normal NK cells (Fig. 1, Table 1; reference 18). Transgene expression conferred Dd-specific inhibitory function to
NK cells, as tested in vitro or in vivo (18). In a second
lower copy transgenic line (line No. 12), the level of
Ly49A expression on the surface of most of the NK cells
from H-2b mice was ~30% of the normal level (Fig. 1, Table 1), whereas some NK cells, presumably those expressing endogenous Ly49, continued to express high levels of
Ly49A (Fig. 1).
|
Previous studies in normal mice have demonstrated that
the cell surface levels of Ly49A, on NK cells are lower in
mice that express the Dd ligand for Ly49A, than in H-2b or
2m
/
mice (12, 13, 25). Here we determined the effects
of MHC genes on the cell surface levels of the transgeneencoded Ly49A receptor. We transferred the transgenes
onto different MHC backgrounds by backcrossing to B6,
B10.D2, or B6-
2m
/
strains. Irrespective of their MHC
background, transgenic mice and their nontransgenic littermates were found to contain comparable numbers of NK
cells per spleen (data not shown), indicating that expression
of the Ly49A transgene did not prevent NK cell development, even in the presence of the inhibitory H-2d ligand of
Ly49A. In Ly49A transgenic line No. 2 mice, Ly49A cell surface levels on all NK cells were reduced by a factor of
two- to threefold in H-2d mice, compared to the levels in
H-2b or
2m
/
mice (Fig. 1, Table 1). Although Ly49A
transgenic line No. 12 mice had generally lower levels of
Ly49A cell surface expression than did line No. 2 mice, H-2d
expression (in H-2b/d mice) nevertheless also caused a two-
to threefold reduction in Ly49A levels compared to levels
in H-2b mice (Fig. 1, Table 1).
The magnitudes of these effects were similar to the magnitude of the reduction observed for the endogenous Ly49A in nontransgenic mice (Fig. 1, Table 1). The results indicate that Ly49A expression driven by the class I promoter cassette is subject to ligand-mediated downregulation, and therefore, that receptor downregulation does not require the Ly49A gene regulatory elements. The fact that the low cell surface level of the transgene-encoded Ly49A in H-2b line No. 12 mice is reduced even further by H-2d expression indicates that the levels are reduced from the level in the absence of ligand, rather than being adjusted to a specific level determined by the MHC ligand.
The Ly49A Transgene Does Not Inhibit Expression of Endogenous Ly49 Receptors inThe expression of a
TCR- transgene in mice prevents the expression of endogenous TCR-
genes, even in mice that do not provide a selecting MHC ligand for the transgenic receptor. To ascertain whether Ly49A transgene expression inhibits expression of endogenous Ly49 genes, we determined whether
the transgene influenced the frequencies of NK cells expressing receptors reacting with the SW5E6 mAb (Ly49C/I)
and 4D11 (Ly49G2) mAbs. In
2m-deficient mice, the
Ly49A transgene (line No. 2) had no detectable effect on
the frequencies of SW5E6+ or 4D11+ NK cells (Fig. 2, Table 2), nor did the transgene cause alterations in the staining intensities observed with these mAbs (Table 1). Thus,
the Ly49A transgene did not appreciably inhibit endogenous Ly49G2 or Ly49C/I expression in class I-deficient
mice.
|
The frequency of cells expressing the endogenous Ly49A
gene could not be determined by flow cytometry because
all Ly49A antibodies react with the B6 Ly49A protein
used as the transgene. However, the transgenic and endogenous Ly49A mRNAs contained distinct 3 untranslated
regions, allowing us to determine the levels of endogenous Ly49A mRNA with the ribonuclease protection assay (33).
When an internal control probe is used, this assay is one of
the most quantitative assays for determining mRNA levels
(33). The use of a large excess of probe makes the assay linear with respect to mRNA levels. A probe was designed
that spanned the 3
end of the coding region and part of
the 3
untranslated region of the Ly49A mRNA, a region
not included in the transgene construct. A probe for the
NKR-P1C mRNA served as an internal control to which
the Ly49A signal was normalized. NKR-P1C encodes the
NK1.1 antigen, which is expressed by all NK cells in the
mouse strains used here (34). Representative data are
shown in Fig. 3, and the results from three experiments are
summarized in Table 3.
In 2m-deficient and H-2b mice, the Ly49A transgene
did not appreciably inhibit expression of the endogenous
Ly49A mRNA (Fig. 3, Table 3). These findings indicate
that the mere presence of the transgene-encoded Ly49A
protein in the cell does not prevent expression of the endogenous Ly49A gene. Monoallelic Ly49A gene expression in
normal mice must therefore be explained by a distinct mechanism. As will be elaborated below, the transgene did
influence endogenous Ly49A gene expression in H-2d mice.
The Ly49A transgenic mice allowed us to test the hypothesis that education processes limit the frequencies of cells coexpressing two or more self-specific Ly49 receptors. Thus, the hypothesis predicts that the Ly49A transgene, in H-2d mice, should cause a reduced frequency of cells expressing endogenous, H-2d-specific receptors, such as Ly49G2 and endogenous Ly49A.
In accord with this prediction, the percentage of NK
cells expressing the H-2d-specific Ly49G2 receptor (detected with 4D11 mAb) was reduced from 50.7% in nontransgenic H-2d littermates to 18.5% in H-2d line No. 2 Ly49A transgenic mice, a 2.7-fold reduction (Fig. 2, Table
2). A similar but slightly smaller effect was observed in the
second transgenic line, line No. 12, where the frequency of
Ly49G2+ cells was reduced from 45% in nontransgenic H-2d+
(H-2b/d) littermates to 22.3% in transgenic H-2b/d mice
(Fig. 2, Table 2). It is of interest that this reduction in line
No. 12 mice occurred, despite the significantly lower levels
of transgene expression compared to line No. 2 mice. Both effects were highly reproducible and significant (P <0.001).
The similar effects observed in two transgenic lines represent strong evidence that the effects are due to MHC genes
rather than to other genes the mice might have inherited
from the transgenic founder mice despite multiple backcrosses. These results strongly support the hypothesis that
an education process limits the number of cells coexpressing Ly49G2 and Ly49A in H-2d mice compared to H-2b
or 2m
/
mice. Much smaller, albeit statistically significant,
reductions in the frequency of SW5E6+ NK cells were also
observed in H-2d mice of both transgenic lines (Table 2).
Although these reductions are of dubious significance, they
may occur because one of the two receptors reactive with
the SW5E6 mAb, Ly49C, reportedly binds to H-2d class I
molecules, whereas the other does not (16).
Surprisingly, in H-2b mice, which are normally thought
not to express a Ly49A ligand (17, 25, 26), marginal, but statistically significant, reductions in the percentages of Ly49G2+
cells were apparent in both Ly49A transgenic lines (Table 2). These reductions were only of 15-25%, and therefore of
dubious significance. Because the percentage of Ly49G2+
cells was not significantly affected by the transgene in
2m
/
transgenic mice, the data suggest that the effect in
H-2b mice may be due to an H-2b-encoded class I molecule(s). Although Ly49A is not thought to react with H-2b
class I molecules, the data raise the possibility that a weak interaction may occur. This interaction may be too weak
to detect in functional experiments, yet, nevertheless, exert
an effect in a developmental step, analogous to some T cell
receptor-ligand interactions.
The hypothesized education process predicts that the
Ly49A transgenes in H-2d mice should cause reduced usage, not only of Ly49G2, but also of endogenous Ly49A.
Although we were unable to measure the frequency of cells
expressing endogenous Ly49A in the transgenic mice by flow cytometry, we were able to determine the level of endogenous Ly49A mRNA with the use of the RNase protection assay. Considering first the results from nontransgenic
mice, we observed that the average relative Ly49A mRNA
level in H-2d mice (76 ± 13) was slightly lower than the
level in H-2b mice (92 ± 31), which was slightly lower that
the level in 2m
/
mice (100 ± 8) (Table 3). These small
differences could all be accounted for by a reduced frequency of Ly49A+ cells observed in nontransgenic H-2d
mice compared to non-transgenic H-2b and
2m
/
mice
(see Table 3). Thus, the level of Ly49A mRNA per
Ly49A+ cell was unaffected by MHC expression. Therefore,
the reduced cell-surface expression of Ly49A observed in
nontransgenic H-2d mice (13; Table 1) was not accompanied by reduced Ly49A mRNA levels per Ly49A+ cell,
supporting the contention that H-2d-induced downregulation of Ly49A levels in normal mice is a posttranscriptional event. This observation is of interest in itself, and serves as an aid to interpretation of the transgenic data.
Analysis of the transgenic line No. 2 mice revealed that
Ly49A transgene expression in H-2d mice resulted in a two-
to threefold reduced level of endogenous Ly49A mRNA in
the NK cell population compared to nontransgenic H-2d
littermates (Fig. 3, Table 3). This reduction was reproducible and significant (P <0.01). As previously noted, the
transgene had little effect in 2m
/
mice, nor did it have a
significant effect in H-2b mice (Fig. 3, Table 3). Therefore,
the reduction of endogenous Ly49A levels was dependent
on both the transgene and H-2d expression.
The level of endogenous Ly49A mRNA in the population should correlate with the frequency of cells expressing endogenous Ly49A, as long as the amount of endogenous Ly49A mRNA per expressing cell remains roughly constant. As noted above, the level of Ly49A mRNA per Ly49A+ cell in nontransgenic mice was unaffected by H-2d expression (Table 3). Since there is no apparent reason why the endogenous mRNA levels per cell should be downregulated by receptor-ligand engagement in transgenic mice, but not normal mice, we favor the interpretation that the reduced endogenous Ly49A levels in H-2d transgenic mice reflects a reduced frequency of cells expressing endogenous Ly49A. These data suggest that the transgene, in H-2d mice, results in a significant reduction in the proportion of cells expressing not only Ly49G2, but also endogenous Ly49A.
The cell surface
levels of Ly49 receptors are downregulated in mice that express the corresponding class I MHC ligands of the receptor (13, 25). It was proposed that receptor downregulation reflects a mechanism that calibrates Ly49 levels to the particular class I molecules expressed in the host (25). Our results demonstrate that Ly49A cell surface levels are regulated by a posttranscriptional event. First, despite the
significant differences in Ly49A cell surface staining, the
level of Ly49A mRNA per Ly49A+ NK cell was the same
in nontransgenic H-2d mice, where surface expression is
low, as in nontransgenic H-2b or 2m
/
mice, where surface expression is high (Fig. 3). Second, the H-2d-induced
downregulation of cell surface Ly49A expression was observed, even with a Ly49A transgene that was regulated by
regulatory elements from a class I MHC gene and an immunoglobulin heavy chain gene (Fig. 1, Table 1). It should
also be noted that the transgene does not contain the 3
untranslated sequences found in the endogenous Ly49A transcript; 3
untranslated sequences often serve as target sequences for regulation of transcript turnover rates (35). Considering that Ly49 receptor levels are downregulated in
H-2d mice independently of the mRNA levels, the most
likely explanation for the phenomenon would appear to be
ligand-induced receptor modulation. We have not, however, ruled out the possibilities that receptor signaling at the
cell surface causes inhibition of receptor protein biosynthesis from the mRNA, or prevents trafficking of the receptor
to the cell surface. Previous evidence argues against the
possibility that downregulation is due to an intracellular interaction of Ly49A with Dd (36).
The receptor calibration model seems to imply that receptor levels are calibrated to some specific absolute level dependent upon the available class I molecules, to maximize sensitivity of the system to changes in class I levels. In light of this model, it is of interest that ligand-induced downregulation occurred even in the case of the Ly49A No. 12 transgenic line. In this line, transgene expression was generally lower than endogenous Ly49A expression, presumably due to the low transgene copy number and/or the integration site of the transgene. In H-2b line No. 12 mice, the level of transgene-encoded Ly49A receptors was as low as the levels directed by the endogenous Ly49A gene or transgene No. 2 Ly49A receptors in H-2d mice. In H-2b/d line No. 12 mice, the levels were reduced further. Since class I MHC levels did not change in the different transgenic lines, it cannot be said that the Ly49A receptor levels are set to a specific level dependent upon the interaction with MHC. These observations argue against the notion that receptor levels are calibrated to maximize sensitivity to changes in class I MHC levels (25). Rather, the results suggest that the presence of the ligand results in reduced levels of surface expression from the levels that pertain in the absence of the ligand. The altered Ly49A levels may nevertheless influence the functional class I specificity of the NK cell as has been previously proposed (25).
Transgenic Ly49 Gene Expression Does Not Prevent Endogenous Ly49 Gene Expression.Allelic exclusion of TCR-
and Ig heavy chain genes is accomplished by feedback inhibition, wherein expression of the protein product of one
allele of the gene prevents activation of the other allele. For
example, expression of TCR-
transgenes prevents activation of the corresponding endogenous genes, even when
the transgenic mice do not express the MHC ligand of the
transgenic receptor. In contrast, the Ly49A transgene had
no significant effect on expression of the endogenous Ly49A
genes in
2m
/
mice. Nor did the transgene affect the
frequencies of cells expressing other Ly49 receptors in
2m
/
mice. The results argue strongly against a model in
which Ly49A gene expression is inhibited by the mere
presence of Ly49A protein in the cell, independent of the
presence of a corresponding class I ligand. Therefore, monoallelic Ly49A gene expression must have another explanation. In light of this, the issue arises of whether monoallelic
Ly49A gene expression should be called "allelic exclusion," as we have previously called it. It should be noted that an
"unregulated" model was once prominently proposed to
account for allelic exclusion of immunoglobulin genes,
suggesting that the term does not imply a specific mechanism (37). Furthermore, it remains possible that regulation
of the extent of monoallelic gene expression occurs in mice
that express the corresponding MHC ligand (see below). In
any case, this issue is primarily a semantic one.
As we have proposed elsewhere, one possibility to account for monoallelic Ly49 gene expression is that during NK cell development, Ly49 genes are chosen for expression by a stochastic process (12, 19). If different Ly49 genes, and different alleles of the same Ly49 gene, are activated independently and with a relatively low probability, most cells would activate only one of the two alleles at a given Ly49 locus. This model would also account for the fact that NK cells commonly coexpress two or more different Ly49 receptors. This mechanism would ensure that different cells express different combinations of Ly49 receptors, and thus would serve to generate clonal diversity. A repertoire generated in this way might then be modified by an MHC-dependent education process.
MHC-dependent Education Process.The Ly49A transgenic
mice provided the opportunity to test the hypothesis that
an education process limits the number of NK cells that coexpress multiple self-specific Ly49 receptors. This hypothesis was based on analysis of the repertoire in nontransgenic mice, which revealed that coexpression of two H-2d-specific Ly49 receptors, Ly49A and Ly49G2, occurred less frequently in H-2d mice than in mice that do not express H-2d
(12). The finding that Ly49A transgene expression in all NK cells caused a specific reduction in the frequency of Ly49G2+
NK cells in H-2d mice, and to a much smaller extent in
H-2b mice, but not in 2m
/
mice (Fig. 2) fulfills a major
prediction of this model. The observation that the low expressing (line No. 12) and high expressing (line No. 2)
transgenic lines exhibited a comparable reduction in Ly49G2+
cells in H-2d+ mice suggests that the Ly49A-Dd interaction
is sufficiently strong that even low Ly49A surface expression can cause these alterations in the repertoire. The comparable results with two transgenic lines also demonstrates that the results were a consequence of the transgene, rather
than of other genes coincidentally inherited from the transgenic founders.
The hypothesis that an education process limits coexpression of multiple self-specific receptors also predicts that
endogenous Ly49A gene usage should be less frequent in
the Ly49A transgenic mice. The finding that the H-2d
transgenic NK cells contained less endogenous Ly49A mRNA
than nontransgenic mice or than transgenic H-2b and
2m
/
mice (Table 3) is consistent with the hypothesis.
The reduction in endogenous Ly49A mRNA among NK
cells in H-2d transgenic mice could reflect a reduction in
the amount of mRNA per expressing cell, rather than a reduction in the frequency of expressing cells. However, the
finding that H-2d expression does not affect the level of
Ly49A mRNA per Ly49A+ cell in nontransgenic mice
(Fig. 3) argues against a ligand-dependent mechanism that
reduces the mRNA levels in each expressing cell. Therefore, although not definitive, the results are most consistent with the interpretation that NK cells expressing endogenous Ly49A are less frequent in transgenic H-2d mice.
The effects of transgene expression on endogenous Ly49G2 and Ly49A gene usage strongly suggest that an education process disfavors NK cells that express multiple self class I-specific Ly49 genes or alleles. Why should the education process disfavor NK cells that coexpress multiple self-class I-specific Ly49 receptors? Previous analysis of NK cells that coexpress two Ly49 receptors suggests that each Ly49 receptor can independently inhibit NK cell lysis (10, 38). If each NK cell expressed all self-class I-specific receptors, the NK cell population would be unable to attack potential target cells that have extinguished expression of some, but not all, self-class I molecules. We propose that by imposing a limit on the coexpression of self-class I-specific receptors, the education process greatly enhances the discriminatory capacity of the NK cell population for self-class I molecules.
We have previously proposed two models of NK cell education that address how MHC class I expression may shape the Ly49 receptor repertoire (12, 19). In a selection model, the stochastic activation of receptor alleles in different cells during an initial stage of NK cell development, generates clonal diversity. This step is followed by MHCdependent selection steps that favor the most "useful" NK cells. It was proposed that one such selection step would ensure that each NK cell expresses at least one self-class I-specific inhibitory receptor, thus preventing autoimmunity. To account for the findings reported here and previously (12), it must also be argued that the selection process includes a step in which cells expressing multiple self-class I-specific receptors are selected against. This process could account for the effects of the transgene observed in this study (39).
Alternatively, a sequential receptor activation model suggests that Ly49 receptor genes may undergo a stage of stochastic activation where different receptors are successively and cumulatively displayed on the cell surface; when the cell eventually expresses a sufficient number of self-class I-specific receptors to achieve a defined threshold of Ly49 receptor signal, the Ly49 gene activation mechanism is disabled, fixing the Ly49 receptor pattern of the cell (12). This model predicts that the formation of NK cells expressing excess self-class I-specific receptors will not occur. Such a mechanism would result in a decreased frequency of NK cells expressing specific pairs of self-specific Ly49 receptors, consistent with our data (39).
Can these models be distinguished? One possible difference in the predictions of the two models concerns the effects of the transgene on non-self-specific receptors (39). The selection model predicts that the transgene should only affect usage of other self-specific receptors, and not the usage of non-self-specific receptors. In contrast, the sequential receptor activation model would seem to predict that early expression of Ly49A on all NK cells in H-2d mice will result in decreased usage of any other receptor, whether it be self or non-self specific. This is because early expression of Ly49A should result in an earlier termination of new receptor expression. The data presented herein demonstrates that in H-2d mice, the transgene exerted a larger effect on Ly49G2 usage than on Ly49C/I receptor usage detected with the SW-5E6 mAb (Table 2). Although Ly49C is thought to bind to H-2d class I molecules, Ly49I reportedly does not (40). Thus, these data might seem to refute the sequential model. However, the predictions of the sequential model would need to be modified if there turns out to be a defined order in which different Ly49 receptors are expressed during development. Moreover, the precise functional specificities of Ly49C and Ly49I are still under investigation. Therefore, we believe that it is premature to arrive at a conclusion on this point based on the available data.
The results reported here clearly demonstrate that a class I-dependent NK cell education process occurs. However, they do not yet discriminate between the selection and sequential receptor activation models, and other models that might be envisaged to explain NK cell education. The production of new reagents that detect each of the Ly49 receptors, and a thorough knowledge of the specificity and expression patterns of each of the receptors, should facilitate this endeavor. Furthermore, elucidation of the molecular mechanisms that activate Ly49 genes in different NK cells, of considerable interest in itself, may also suggest approaches to generate mice that express a more limited Ly49 repertoire. Such mice would represent useful tools for analysis of NK cell development.
Address correspondence to David H. Raulet, 485 LSA, Department of Molecular and Cell Biology, University of California, Berkeley, Berkeley, CA 94720-3200. The present address of W. Held is Ludwig Institute For Cancer Research, Lausanne Branch, Ch. des Boveresses 155, 1066 Epalinges, Switzerland.
Received for publication 21 January 1997 and in revised form 3 April 1997.
W. Held was supported by a fellowship from the Swiss National Science foundation. This work was supported by National Institutes of Health grants RO1-AI35021 and RO1-AI39642 to D.H. Raulet.We thank Dragana Cado for production of the transgenic mice, Peter Schow for expert assistance with flow cytometry, Joonsoo Kang for advice on the RNase protection assays, Rana Orangi for technical assistance, and Vinay Kumar, Jacques Roland, and John Ortaldo for providing the SW5E6, JR9-318, and 4D11 hybridomas, respectively. We thank Cetus Corporation for the gift of recombinant IL-2. We also thank Ellen Robey, Russell Vance, Jeff Dorfman, Joonsoo Kang, Thomas Hanke, and Jens Zerrahn for their comments on the manuscript.
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