Abstract
Killer-cell immunoglobulin-like receptors (KIRs) are encoded by one of the most polymorphic families in the human genome. KIRs are expressed on natural killer (NK) cells, which have dual roles: (1) in fighting infection and (2) in reproduction, regulating hemochorial placentation. Uniquely among primates, human KIR genes are arranged into two haplotypic combinations: KIR A and KIR B. It has been proposed that KIR A is specialized to fight infection, whilst KIR B evolved to help ensure successful reproduction. Here we demonstrate that a combination of infectious disease selection and reproductive selection can drive the evolution of KIR B-like haplotypes from a KIR A-like founder haplotype. Continued selection to survive and to reproduce maintains a balance between KIR A and KIR B.
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Introduction
Killer-cell immunoglobulin-like receptors (KIRs) are expressed on the surface of natural killer cells (NK cells)—the major effector lymphocytes of innate immunity. Specific KIR genotypes, genes or alleles are associated with differential responses to a variety of infectious diseases (Gao et al. 2010; Hirayasu et al. 2012; Khakoo et al. 2004; Knapp et al. 2010; Martin et al. 2002, 2007; Seich al Basatena et al. 2011). Furthermore, in addition to their role in fighting infection, NK cells are involved in pregnancy. Uterine NK cells (uNK cells) regulate how fetal placental cells remodel the spiral arteries that supply nutrients and oxygen to the developing feto-placental unit. In humans, maternal KIR genotype has been shown to affect the likelihood of severe pregnancy syndromes (Hiby et al. 2004, 2008, 2010; Nakimuli et al. 2015), and birth weight itself (Hiby et al. 2014).
KIRs can be activating or inhibitory. Multiple KIR genes are found in a 150-kb cluster on chromosome 19. Strikingly, all human populations—even those which have experienced extreme bottlenecks (Gendzekhadze et al. 2006)—possess two KIR haplotypes with distinctly different gene contents. The KIR A haplotype has largely fixed gene content, with mostly genes encoding inhibitory KIRs; the KIR B haplotype has a more variable gene content and contains several genes encoding activating KIRs. Other primate species display a high degree of KIR haplotypic diversity, but no equivalent organisation into KIR A and KIR B-like entities (de Groot et al. 2015; Guethlein et al. 2015). Why KIRs should have been segregated in this way in humans, and why KIR A and KIR B are always maintained in every human population, is an evolutionary phenomenon demanding explanation.
One hypothesis that has been proposed is that KIR A haplotypes are specialized to ensure success in fighting infection, and KIR B haplotypes are specialized to ensure success in reproduction (Parham 2005, 2008; Parham and Moffett 2013). This is in keeping with the observation that KIR A homozygous individuals exhibit better clearance of hepatitis C infection (Khakoo et al. 2004), but KIR B homozygous mothers are protected against the potentially fatal pregnancy syndrome pre-eclampsia (Hiby et al. 2004, 2010; Nakimuli et al. 2015). However, population genetic frameworks within which to test whether a combination of such selective pressures can indeed promote the evolution of KIR A and KIR B haplotypes have so far been lacking. Here, we integrate links between KIR genotype, infectious disease and reproduction into a single model. We demonstrate that a combination of infectious disease selection and reproductive selection can drive the evolution of both KIR A—like and KIR B-like haplotypes from a KIR A-like ancestor.
Methods
Many KIRs have been shown to bind directly to class I major histocompatibility complex (MHC) molecules expressed on the surface of other cells. In humans, MHC molecules are known as human leukocyte antigens, or HLAs. For simplicity, we will henceforth consider only KIR/HLA interactions involving HLA-C, the dominant HLA ligand for KIRs which is present in all individuals. HLA-C molecules form two types of KIR ligand, depending on the amino acid residue at position 80. These are known as C1 and C2, and a balance between HLA-C alleles encoding C1 or C2 ligands is observed in all human populations. In order to explore the generation of A and B KIR haplotypes, we simulated a haplotype containing three possible KIR genes (Fig. 1). One gene encodes a KIR that can bind C1 (and is thus equivalent to human KIR2DL2 or KIR2DL3) and two genes encode KIRs that can bind C2 [equivalent to KIR2DL1 or KIR2DS1, and perhaps also KIR2DS5*006 (Nakimuli et al. 2015)]. Mutation rates were incorporated in the model such that (1) genes could switch between encoding activating or inhibitory KIRs; (2) genes could switch between being expressed or pseudogenes, and (3) the strength (magnitude) of the inhibitory or activating signal associated with the encoded KIR could change. In this way, a range of possible three-gene KIR haplotypes could be generated at random within each simulation, of varying degrees of similarity to those seen in human populations.
Diploid combinations of KIR haplotypes and HLA genotypes (HLA-C1 homozygous; HLA-C2 homozygous and HLA-C1/C2 heterozygous) were used to define individuals in an individual-based model. Every generation, all individuals had to survive infectious disease challenge, where their probability of success was linked to their KIR/HLA genotype (further details in the following sections). Survivors were then randomly sampled with replacement to be the parents of the next generation, such that a maximum of K pregnancies took place. The success of each simulated pregnancy was determined by the combination of maternal KIR and fetal HLA genotype (further details in the following sections), and only surviving offspring could contribute to the next generation. The individual-based process of first surviving infection and then reproducing was iterated over T generations in each simulation. With each birth, came fixed probabilities of the aforementioned KIR mutations or recombination (see Table 1).
Infectious disease selection
We included two types of infectious disease selection in our simulations:
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1.
Selection from HLA-evading pathogens. Individuals heterozygous for HLA-C1 and HLA-C2 whose genome encoded at least one expressed inhibitory KIR specific to each of C1 and C2 were assumed to have an advantage against pathogens which exploit particular forms of HLA-evasion. This advantage is captured by parameter θ (see Table 1).
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2.
Selection from pathogens for which the degree to which NK cells are activated or inhibited is important. We generated, for each individual in the model, a normal distribution of possible NK cell activation states derived from their KIR/HLA genotype. In this way, the various KIR/HLA interactions possible for a specific individual (i.e. the different types and magnitudes of signals associated with those interactions) could combine to generate a single phenotype (see Electronic supplementary material (ESM) Methods for further details We defined a range of optimum NK cell activation states to survive infection (x L < x < x H). The per generation probability of a given individual dying from this type of infection was then given by \( \upmu \left(1-{A}_{x_L\le x\le {x}_H}\right) \), where \( {A}_{x_L\le x\le {x}_H} \) is the proportion of that individual’s NK cell distribution that fell within the optimum range.
The biological justifications for these assumptions were as follows:
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1.
Certain viruses down-regulate MHC molecules and/or express decoy MHC molecules as a means of immune evasion. In humans, inhibitory KIRs help NK cells to combat such viruses by detecting a lack of HLA (‘missing self’). When HLAs are present, inhibitory KIRs for which those HLAs are ligands prevent NK cell killing. If such inhibitory signals are lost, the NK cell kills the abnormal cell. In keeping with evolutionary simulations that suggest the presence of multiple possible inhibitory KIR-HLA ligand pairs is advantageous against a cytomegalovirus-like pathogen (Carrillo-Bustamante et al. 2014), we have assumed that HLA C1/C2 heterozygotes who express inhibitory KIRs that can recognise both C1 and C2, and thus have the maximum possible number of KIR-HLA ligand pairs protected by a missing-self mechanism in our model, are protected against extra mortality from pathogens capable of this or similar forms of HLA-evasion.
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2.
KIRs differ in the relative inhibitory or activating effects they have on NK cells (Moesta et al. 2008), and the strength of this inhibition or activation seems to affect the possibility of mortality. For both hepatitis C and hepatitis B, the genotype associated with the weakest possible inhibitory interaction involving HLA-C (homozygosity for KIR2DL3 and HLA-C1) offers an increased chance of clearing the infection (Gao et al. 2010; Khakoo et al. 2004; Knapp et al. 2010). Conversely, genotypes which encode certain highly inhibitory KIRs and their known HLA ligands are associated with delayed progression to AIDS (Martin et al. 2007). Activating KIRs are also directly implicated in improved responses: the activating receptor KIR3DS1 together with its putative ligand HLA-Bw4 is associated with a delayed progression to AIDS (Martin et al. 2002) and reduced susceptibility to opportunistic infections in individuals with HIV (Qi et al. 2006).
Reproductive selection
We generated, for every pregnancy that occurred within each simulation, a normal distribution of uterine NK (uNK) cell activation states, based on the inhibition/activation signal strengths of the KIRs encoded in the mother’s genome that could interact with the HLA-C supplied by the father (see ESM Methods for full details). Both excessive inhibition of uNK cells and excessive activation of uNK cells can be risky. The probability of the failure of a pregnancy due to excessive inhibition of uNK cells was \( p.{A}_{y\le {y}_T} \) where p = the maximum mortality rate and \( {A}_{y\le {y}_T} \) = the proportion of the uNK cell response equal to or below the critical value y T . The probability of the failure of a pregnancy due to excessive activation of uNK cells was \( q.{A}_{y_U\le y} \) where q = the maximum risk and \( {A}_{y_U\le y} \) = the proportion of the uNK cell response equal to or above the critical value y U . In both cases, we assumed that the failure of a pregnancy led to the deaths of both mother and infant.
The biological justifications for these assumptions were as follows:
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uNK cells associate closely with the developing trophoblast (Moffett-King 2002). KIRs expressed on uNK cells bind to HLA-C molecules expressed by invading trophoblast cells, and the interaction between fetal HLA-C and maternal KIR genotype has been shown to influence pregnancy outcome (reviewed in Moffett and Colucci 2015). Excessive inhibition of uNK cells is a risk factor for pregnancy disorders where placentation is poor, e.g. pre-eclampsia, fetal growth restriction and recurrent miscarriage (Hiby et al. 2004, 2008, 2010, 2014; Nakimuli et al. 2015). At the other extreme, greater activation of uNK cells is positively correlated with higher birth weights (Hiby et al. 2014). Paternally derived C2 expressed by the trophoblast seems to be particularly associated with these effects, hence our use of paternal HLA-C only to define such risks in the model. It seems that the degree of activation or inhibition of uNK cells upon their interaction with fetal trophoblast cells has a direct effect on the effectiveness of placentation; most likely on the level of blood supplied through remodelled spiral arteries in the uterine wall (reviewed in Moffett and Colucci 2015).
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The importance of these observations becomes apparent when we consider the obstetric dilemma: an evolutionary challenge unique to modern humans. Bipedalism places physical restrictions on the structure of the pelvis, but encephalization (increasing brain size) demands that babies be born with heads as large as possible. Childbirth for Homo sapiens is therefore an exceptionally dangerous process for both mother and baby, owing to the extremely tight fit of the head of the fetus through the birth canal (Wittman and Wall 2007). Given that, as we have just discussed, the greater the level of activation of uNK cells, the greater the birth weight, the obstetric dilemma is likely to generate intense selective pressures on KIRs.
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In our model, we assume that both excessive inhibition and excessive activation of uNK cells are capable of killing women and fetuses during pregnancy. Pre-eclampsia, which is clearly linked to uNK cell inhibition, can lead to fatal eclampsia. Obstructed labour, particularly common in humans for the reasons just outlined, is associated with higher birth weights and therefore likely to be linked to excessive activation of uNK cells. Obstructed labour, too, can kill both mother and fetus, or can leave the mother with major injuries, hence our assumption that both extremes of uNK cell inhibition and activation have the potential to be extremely disadvantageous.
Choice of parameter values
For computational feasibility we set the maximum number of births per generation (i.e. the maximum population size), K = 1000. In terms of the probability of a mutation arising in the population at all, a mutation rate of 1 × 10−5 in a population of 1000 individuals is equivalent to a mutation rate of 1 × 10−7 in a population of 100,000 individuals. Given the relatively small population size in our simulations, for the scenarios presented in the main text we have used relatively high mutation rates—which made it possible for a wider range of potential KIR haplotypes to emerge and compete with one another. In the ESM Results, we show that our overall results do not depend on the specific mutation or recombination rates applied, provided rates are not so low that no mutations can emerge in our simulated populations (Fig. S1).
Parameters p, q, μ and θ generate different types and strengths of selective pressure. As such, the absolute values of each parameter are less important than their relative values. We seek to define which selective pressures are vital in order to obtain a balance between KIR-A and KIR-B, not to claim that specific values for each parameter have applied throughout human history.
p is the maximum per-pregnancy probability of pregnancy failure and maternal death associated with insufficiently activated uNK cells. Present-day rates of pre-eclampsia, a proxy which will substantially underestimate parameter p because p only applies to the most at risk genotypes, are 6.2 to 10.2 % in American populations (Nakimuli et al. 2014). q is the maximum per-pregnancy probability of pregnancy failure and maternal death associated with excessively activated uNK cells. Present-day rates of obstructed labour, a proxy which will likewise underestimate parameter q, are between 3 and 6 % (Dolea and AbouZahr 2003). Given the uncertainty in the historical effects of pre-eclampsia and obstructed labour on human survival, and to make sure that we explored a wide range of possibilities, in our sensitivity analyses we tested values of p and q between 0 and 0.4 (see ESM Results and Fig. S2).
θ is the selection pressure from pathogens for which having two types of HLA-C KIR ligand, both protected by a missing-self mechanism, is an advantage. As a shorthand, we refer to these as HLA-evading pathogens. μ is the selection pressure from pathogens for which the degree to which NK cells are activated or inhibited affects the survival of the host. In each generation of the model, θ and μ define the maximum probability of dying from either type of infectious disease before reproducing, i.e. the probability of dying for the most at risk genotypes. Importantly, these parameters do not represent the case fatality rates of specific pathogens: rather the overall probability of dying from a particular sort of infectious disease during childhood. We know from human history that specific pathogens come and go. Smallpox, for example, is a relatively recent burden that was only a significant cause of mortality within the last several hundred generations; falciparum malaria, similarly, seems to only have emerged within the last ten thousand years. We can, however, be confident that infectious diseases have plagued modern humans for as long as we have existed. Parameters θ and μ allow our model to ask which types of relationship between infectious diseases, KIRs and HLAs (if any) are most likely to generate a balance between KIR A and KIR B haplotypes. Just as for parameters p and q, in our sensitivity analyses we allowed parameters θ and μ to take values between 0 and 0.4, to capture a wide range of possible selection scenarios.
Results
Selection from HLA-evading pathogens alongside reproductive selection is essential to generate A and B like KIR haplotypes
Our closest evolutionary relatives, chimpanzees, possess both C1 and C2, but lack an obvious KIR A/B haplotypic structure. Human KIR A haplotypes have more in common with chimpanzee KIR haplotypes than human KIR B. We thus began each simulation with balanced frequencies of C1 and C2 encoding HLA alleles and the population fixed for a KIR A-like haplotype (Fig. 1). We sought to identify the conditions under which a KIR B-like haplotype emerged alongside the evolving KIR A haplotype, and the two were still maintained together at the end of a 15,000 generation simulation. Figure 2 illustrates the time course of one of our simulations displaying this behaviour of interest.
We found that a balanced scenario (such as illustrated in Fig. 2), where KIR A-like and KIR B-like haplotypes and C1 and C2 are all present after 15,000 generations, was impossible to obtain without assuming some degree of selection from HLA-evading pathogens (Fig. S2, parameter θ). Without such selection, either C1 or C2 was likely to be lost from the population over the thousands of generations simulated, and without a diversity of HLA ligands there was no reason to maintain a specific KIR haplotypic structure. So long as selection from HLA-evading pathogens was present (θ > 0.1), the inclusion of at least a low level of reproductive selection whereby excessive inhibition of uNK cells can cause mortality, made a balanced scenario possible (Fig. S2 and Fig. 3a, first graph).
Selection from pathogens for which strongly inhibited NK cells are advantageous increases the probability of obtaining a balance between KIR A and KIR B
We found that scenarios where KIR A and KIR B coexisted were obtained most frequently when we included not only reproductive selection and selection from HLA-evading pathogens, but also selection from pathogens for which strongly inhibited NK cells were particularly advantageous (Fig. 3a, second graph). Without selection in favour of strongly inhibited NK cells, the highest probability of the balanced scenario for any single set of parameters in Fig. 3 was 14.7 %; including such selection, the highest probability of obtaining a balanced scenario rose to 39.4 %. If strongly inhibitory KIRs are advantageous against certain pathogens, and therefore maintained in the population, certain pregnancies will experience excessive inhibition of NK cells, and suffer associated mortalities (i.e. eclampsia). This in turn generates a selection pressure for haplotypes containing activating KIRs, and makes the evolution of KIR A and KIR B more likely.
Figures 3b and c compare the frequencies of KIR AA genotypes and HLA-C2 observed in human populations worldwide with the model’s output for two sets of parameters where a balanced scenario is likely. Although neither of the parameter combinations shown produce a negative correlation as strong as that observed in human data, our model can certainly produce frequency combinations within a plausible range.
Different types of infectious disease selection cannot substitute for the combination of infectious disease selection and reproductive selection
Figure 4 illustrates the contrasting selective forces acting within our model in greater detail. Each of the vertical grey lines in the figure illustrates the range of inhibitory/activating behaviours exhibited by functional C2 interacting KIRs in a single simulated population after 15,000 generations of evolution. As shown in panel 4a, a combination of selection from reproduction and infectious disease encourages wider ranges of KIR-C2 interactions, from the inhibitory (negative values on the y-axis) to the activating (positive values on the y-axis) to coexist. It is in the regions of parameter space which allow such a wide range of KIR-C2 interactions that KIR A and KIR B haplotypes can emerge. If selection from infectious disease becomes too high (the far right hand side of panel 4a), the range of evolved KIR-C2 interactions narrows to match that which is best adapted to survive infection.
In panel 4b, we have applied no reproductive costs, but each individual in the population must survive challenge with pathogens for which strongly inhibited NK cells are optimal, and pathogens for which the optimal range of NK cell inhibition/activation is the same as that previously optimal for reproduction. Each simulation ends up with a set of possible KIR-C2 interactions that match one or other of the optimum ranges but we see none with a range of KIR-C2 interactions spanning both. This result suggests that it is difficult to create a balance between KIR A and KIR B using infectious disease selection alone—but there are many other factors, such as variable selection from different types of pathogens at different stages in human history, that we have not yet considered in our framework.
Discussion
Specific examples of trade-offs between the capacity to either survive in the long term or maximise reproductive success in the short term are rare; although one excellent recent example is a negative association between antibody responsiveness and reproductive success observed in Soay sheep (Graham et al. 2010). A growing collection of studies suggests that KIR genes may be pivotal to a reproductive/immunological trade-off in humans (Hiby et al. 2014; Khakoo and Jamil 2011; Parham and Moffett 2013). The results presented here strongly suggest that present-day population genetic patterns exhibited by KIR haplotypes do indeed result from competing pressures to survive infection or to reproduce successfully.
Our model identifies a combination of reproductive selection and selection from HLA-evading pathogens as critical in allowing KIR A and B to emerge, but also shows that including an infection survival advantage for individuals with strongly inhibited NK cells makes a balance between A and B, alongside HLA alleles encoding C1 and C2 ligands, more likely. An infection advantage associated with strongly inhibited NK cells may follow from a process of ‘education’ or ‘licencing’ during NK cell development: specifically if stronger inhibitory signals during NK cell development set up the capacity for greater activation of NK cells during infection, as has been proposed for certain HLA-B/KIR3DL1 combinations in HIV patients (Martin et al. 2007). Alternatively, relatively strong inhibition of NK cells may help avoid immunopathologies associated with an over-reactive immune response. A recent observation in keeping with this hypothesis is that the relatively weakly inhibitory combination of KIR2DL3 and C1 is a risk factor for cerebral malaria, and the activating combination of KIR2DS1 and C2 may be a risk factor for non-cerebral severe malaria (Hirayasu et al. 2012). No infectious disease has yet been reported for which the specific combination of alleles encoding highly inhibitory KIR2DL1 receptors and their C2 ligands is of particular benefit. However, given the importance of such an effect in driving the evolution of KIR A and KIR B within our model, we predict that such a relationship should exist for at least some of the infectious diseases with which humans have coexisted for thousands of generations: e.g. malaria or similar pathogens which cause mortality prior to reproduction and are able to persist in non-urban social groups.
It is important to note that our model does not require that the best response to all pathogens involves strongly inhibited NK cells. It has been shown that KIR B is associated with higher IFN-γ release from NK cells upon stimulation with mycobacteria in vitro (Portevin et al. 2012), and multiple studies of KIR genes in tuberculosis patients suggest that greater NK cell inhibition is a risk factor for the disease (Braun et al. 2013; Mahfouz et al. 2011; Méndez et al. 2006; Shahsavar et al. 2012) [although not every tuberculosis study has found an effect (Tajik et al. 2012)]. It seems plausible that for some diseases, a swift inflammatory response that eliminates infection is best, whereas for other infections, the costs to the host of immunopathological damage are too high, and a less inflammatory response that nonetheless keeps the pathogen under control is preferable.
Our model assumes that when responding to any specific challenge, an individual with a narrow range of possible NK cell behaviours that is entirely optimised for that challenge will do better than an individual with a wider range of possible NK cell behaviours. However, the individual with narrow NK cell responses will, of course, perform badly against any challenge that requires NK cell responses outside of its range. Different ranges of optimum NK cell behaviours could derive from selection to survive infection and selection to reproduce, or could derive from infectious disease selection alone, if—as we have just noted—different ranges of NK cells responses are appropriate to different pathogens.
In Fig. 4, we explored whether KIR A and B haplotypes had to derive from a trade-off between surviving infection and reproducing or could be driven by competing pathogen selection pressures. Our results so far suggest that reproductive selection per se is important in the emergence of KIR A and B. In the presence of pathogen selection alone, a population is more likely to evolve a strategy where all genotypes are equally good at responding to one type of pathogen challenge, even if that means being equally poor at responding to others (Fig. 4b). It may be that the re-association of different HLA-C genotypes with the mother’s existing KIR genotype that is an integral part of the reproductive process is vital to encourage the persistence of diverse KIR haplotypes. This reassortment means that a KIR which happens to end up in a genotype for which the HLA-C ligands present made it relatively unfit, will later have the chance to encounter HLA-C ligands that render it relatively fit (or vice versa). Such a process seems inherently likely to encourage greater KIR diversity—and on one level the persistence of KIR A and B haplotypes in all human populations can be thought of as the persistence of a balance between diverse (activating and inhibitory) KIRs in all human populations.
We have focused on the effect of the KIR/ HLA interaction on NK cells. KIRs are, however, also expressed on a subset of T cells. It has been shown that the presence of KIR2DL2 tends to magnify either protective or detrimental effects of certain HLA alleles against viral infection (Seich al Basatena et al. 2011). The HLA alleles in question are not ones with which KIR2DL2 is likely to interact directly, and the authors suggest that the mechanism underlying their observations may involve KIR2DL2 increasing the lifespan of certain memory T cells. If T cells restricted by either advantageous or disadvantageous HLAs survive for longer in patients, their respective effects should both tend to be enhanced. Other inhibitory KIRs may have similar effects on the survival of T cells, and future models including more diverse HLAs could investigate the evolutionary significance of such a mechanism.
Recent computational studies have demonstrated that viral expression of decoy HLA class I molecules promotes KIR allelic diversity, and a combination of both activating and inhibitory KIRs should offer the maximum level of protection against such viruses (Carrillo-Bustamante et al. 2013, 2014). It seems likely, therefore, that selection from pathogens is responsible for the evolution of multiple KIRs, and multiple KIR/HLA interactions, in the first instance. However, the human-specific organisation of the KIR locus into A and B haplotypes calls for further explanation. As we have illustrated here, such organisation may well reflect selection from both infectious disease and reproductive processes.
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Acknowledgments
This research was supported by a Sir Henry Wellcome Postdoctoral Fellowship (WT096063MA) held by B.S.P and a Merton College Junior Research Fellowship held by B.S.P. SG was funded by a Royal Society Wolfson Research Fellowship and an ERC Advanced Investigator Grant (DIVERSITY).
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Penman, B.S., Moffett, A., Chazara, O. et al. Reproduction, infection and killer-cell immunoglobulin-like receptor haplotype evolution. Immunogenetics 68, 755–764 (2016). https://doi.org/10.1007/s00251-016-0935-9
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DOI: https://doi.org/10.1007/s00251-016-0935-9