Genome-Wide Inference of Ancestral Recombination Graphs
The unusual and complex correlation structure of population samples of genetic sequences presents a fundamental statistical challenge that pervades nearly all areas of population genetics. Historical recombination events produce an intricate network of intertwined genealogies, which impedes demography inference, the detection of natural selection, association mapping, and other applications. It is possible to capture these complex relationships using a representation called the ancestral recombination graph (ARG), which provides a complete description of coalescence and recombination events in the history of the sample. However, previous methods for ARG inference have not been adequately fast and accurate for practical use with large-scale genomic sequence data. In this article, we introduce a new algorithm for ARG inference that has vastly improved scaling properties. Our algorithm is implemented in a computer program called ARGweaver, which is fast enough to be applied to sequences megabases in length. With the aid of a large computer cluster, ARGweaver can be used to sample full ARGs for entire mammalian genome sequences. We show that ARGweaver performs well in simulation experiments and demonstrate that it can be used to provide new insights about both demographic processes and natural selection when applied to real human genome sequence data.
Published in the journal:
Genome-Wide Inference of Ancestral Recombination Graphs. PLoS Genet 10(5): e32767. doi:10.1371/journal.pgen.1004342
Category:
Research Article
doi:
https://doi.org/10.1371/journal.pgen.1004342
Summary
The unusual and complex correlation structure of population samples of genetic sequences presents a fundamental statistical challenge that pervades nearly all areas of population genetics. Historical recombination events produce an intricate network of intertwined genealogies, which impedes demography inference, the detection of natural selection, association mapping, and other applications. It is possible to capture these complex relationships using a representation called the ancestral recombination graph (ARG), which provides a complete description of coalescence and recombination events in the history of the sample. However, previous methods for ARG inference have not been adequately fast and accurate for practical use with large-scale genomic sequence data. In this article, we introduce a new algorithm for ARG inference that has vastly improved scaling properties. Our algorithm is implemented in a computer program called ARGweaver, which is fast enough to be applied to sequences megabases in length. With the aid of a large computer cluster, ARGweaver can be used to sample full ARGs for entire mammalian genome sequences. We show that ARGweaver performs well in simulation experiments and demonstrate that it can be used to provide new insights about both demographic processes and natural selection when applied to real human genome sequence data.
Introduction
At each genomic position, orthologous DNA sequences drawn from one or more populations are related by a branching structure known as a genealogy [1], [2]. Historical recombination events lead to changes in these genealogies from one genomic position to the next, resulting in a correlation structure that is complex, analytically intractable, and poorly approximated by standard representations of high-dimensional data. Over a period of many decades, these unique features of genetic data have inspired numerous innovative techniques for probabilistic modeling and statistical inference [3]–[9], and, more recently, they have led to a variety of creative approaches that achieve computational tractability by operating on various summaries of the data [10]–[17]. Nevertheless, none of these approaches fully captures the correlation structure of collections of DNA sequences, which inevitably leads to limitations in power, accuracy, and generality in genetic analysis.
In principle, the correlation structure of a collection of colinear orthologous sequences can be fully described by a network known as an ancestral recombination graph (ARG) [18]–[20]. An ARG provides a record of all coalescence and recombination events since the divergence of the sequences under study and specifies a complete genealogy at each genomic position (Figure 1A). In many senses, the ARG is the ideal data structure for population genomic analysis. Indeed, if an accurate ARG could be obtained, many problems of interest today—such as the estimation of recombination rates or ancestral effective population sizes—would become trivial, while many other problems—such as the estimation of population divergence times, rates of gene flow between populations, or the detection of selective sweeps—would be greatly simplified. Various data representations in wide use today, including the site frequency spectrum, principle components, haplotype maps, and identity by descent spectra, can be thought of as low-dimensional summaries of the ARG and are strictly less informative.
An extension of the widely used coalescent framework [1], [2], [9] that includes recombination [21] is regarded as an adequately rich generative process for ARGs in most settings of interest. While simulating an ARG under this model is fairly straightforward, however, using it to reconstruct an ARG from sequence data is notoriously difficult. Furthermore, the data are generally only weakly informative about the ARG, so it is often desirable to regard it as a “nuisance” variable to be integrated out during statistical inference (e.g., [22]). During the past two decades, various attempts have been made to perform explicit inference of ARGs using techniques such as importance sampling [19], [22] (see also [23]) and Markov chain Monte Carlo sampling [24]–[27]. There is also a considerable literature on heuristic or approximate methods for ARG reconstruction in a parsimony framework [28]–[35]. Several of these approaches have shown promise, but they are generally highly computationally intensive and/or limited in accuracy, and they are not suitable for application to large-scale data sets. As a result, explicit ARG inference is rarely used in applied population genomics.
The coalescent-with-recombination is conventionally described as a stochastic process in time [21], but Wiuf and Hein [36] showed that it could be reformulated as a mathematically equivalent process along the genome sequence. Unlike the process in time, this “sequential” process is not Markovian because long-range dependencies are induced by so-called “trapped” sequences (genetic material nonancestral to the sample flanked by ancestral segments). As a result, the full sequential process is complex and computationally expensive to manipulate. Interestingly, however, simulation processes that simply disregard the non-Markovian features of the sequential process produce collections of sequences that are remarkably consistent in most respects with those generated by the full coalescent-with-recombination [37], [38]. In other words, the coalescent-with-recombination is almost Markovian, in the sense that the long-range correlations induced by trapped material are fairly weak and have a minimal impact on the data. The original Markovian approximation to the full process [37] is known as the sequentially Markov coalescent (SMC), and an extension that allows for an additional class of recombinations [38] is known as the SMC'.
In recent years, the SMC has become favorite starting point for approximate methods for ARG inference [39]–[42]. The key insight behind these methods is that, if the continuous state space for the Markov chain (consisting of all possible genealogies) is approximated by a moderately sized finite set—typically by enumerating tree topologies and/or discretizing time—then inference can be performed efficiently using well-known algorithms for hidden Markov models (HMMs). Perhaps the simplest and most elegant example of this approach is the pairwise sequentially Markov coalescent (PSMC) [42], which applies to pairs of homologous chromosomes (typically the two chromosomes in a diploid individual) and is used to reconstruct a profile of effective population sizes over time. In this case, there is only one possible tree topology and one coalescence event to consider at each genomic position, so it is sufficient to discretize time and allow for coalescence within any of possible time slices. Using the resulting -state HMM, it is possible to perform inference integrating over all possible ARGs. A similar HMM-based approach has been used to estimate ancestral effective population sizes and divergence times from individual representatives of a few closely related species [39]–[41]. Because of their dependency on a complete characterization of the SMC state space, however, these methods can only be applied to small numbers of samples. This limits their utility with newly emerging population genomic datasets and leads to reduced power for certain features of interest, such as recent effective population sizes, recombination rates, or local signatures of natural selection.
An alternative modeling approach, with better scaling properties, is the product of approximate conditionals (PAC) or “copying” model of Li and Stephens [43]. The PAC model is motivated primarily by computational tractability and is not based on an explicit evolutionary model. The model generates the th sequence in a collection by concatenating (noisy) copies of fragments of the previous sequences. The source of each copied fragment represents the “closest” (most recently diverged) genome for that segment, and the noise process allows for mutations since the source and destination copies diverged. The PAC framework has been widely used in many applications in statistical genetics, including recombination rate estimation, local ancestry inference, haplotype phasing, and genotype imputation (e.g., [44]–[48]), and it generally offers good performance at minimal computational cost. Recently, Song and colleagues have generalized this framework to make use of conditional sampling distributions (CSDs) based on models closely related to, and in some cases equivalent to, the SMC [49]–[52]. They have demonstrated improved accuracy in conditional likelihood calculations [49], [50] and have shown that their methods can be effective in demographic inference [51], [52]. However, their approach avoids explicit ARG inference and therefore can only be used to characterize properties of the ARG that are directly determined by model parameters (see Discussion).
In this paper, we introduce a new algorithm for ARG inference that combines many of the benefits of the small-sample SMC-based approaches and the large-sample CSD-based methods. Like the PSMC, our algorithm requires no approximations beyond those of the SMC and a discretization of time, but it improves on the PSMC by allowing multiple genome sequences to be considered simultaneously. The key idea of our approach is to sample an ARG of sequences conditional on an ARG of sequences, an operation we call “threading.” Using HMM-based methods, we can efficiently sample new threadings from the exact conditional distribution of interest. By repeatedly removing and re-threading individual sequences, we obtain an efficient Gibbs sampler for ARGs. This basic Gibbs sampler can be improved by including operations that rethread entire subtrees rather than individual sequences. Our implementation of these methods, called ARGweaver, is efficient enough to sample full ARGs on a genome-wide scale for dozens of diploid individuals. Simulation experiments indicate that ARGweaver converges rapidly and is able to recover many properties of the true ARG with good accuracy. In addition, our explicit characterization of the ARG enables us to examine many features not directly described by model parameters, such as local times to most recent common ancestry, allele ages, and gene tree topologies. These quantities, in turn, shed light on both demographic processes and the influence of natural selection across the genome. For example, we demonstrate, by applying ARGweaver to 54 individual human sequences from Complete Genomics, that it provides insight into the sources of reduced nucleotide diversity near functional elements, the contribution of balancing selection to regions containing very old polymorphisms, and the relative influences of direct and indirect selection on allele age. Our ARGweaver software (https://github.com/mdrasmus/argweaver), our sampled ARGs (http://compgen.bscb.cornell.edu/ARGweaver/CG_results), and genome-browser tracks summarizing these ARGs (http://genome-mirror.bscb.cornell.edu; assembly hg19) are all freely available.
Results
The Sequentially Markov Coalescent
The starting point for our model is the Sequentially Markov Coalescent (SMC) introduced by McVean and Cardin [37]. We begin by briefly reviewing the SMC and introducing notation that will be useful below in describing a general discretized version of this model.
The SMC is a stochastic process for generating a sequence of local trees, and corresponding genomic breakpoints , such that each describes the ancestry of a collection of sequences in a nonrecombining genomic interval , and each breakpoint between intervals and corresponds to a recombination event (Figure 1B). The model is continuous in both space and time, with each node in each having a real-valued age in generations ago, and each breakpoint falling in the continuous interval , where is the total length of the genomic segment of interest in nucleotide sites. The intervals are exhaustive and nonoverlapping, with , , and for all . Each is a binary tree with for all leaf nodes . We will use the convention of indexing branches in the trees by their descendant nodes; that is, branch is the branch between node and its parent.
As shown by Wiuf and Hein [36], the correlation structure of the local trees and recombinations under the full coalescent-with-recombination is complex. The SMC approximates this distribution by assuming that is conditionally independent of given , and, similarly, that depends only on and , so that,
where is the effective population size, is the recombination rate, and it is understood that . Thus, the SMC can be viewed as generating a sequence of local trees and corresponding breakpoints by a first-order Markov process. The key to the model is to define the conditional distributions and such that this Markov process closely approximates the coalescent-with-recombination. Briefly, this is accomplished by first sampling the initial tree from the standard coalescent and setting , and then iteratively (i) determining the next breakpoint, , by incrementing by an exponential random variate with rate , where denotes the total branch length of ; (ii) sampling a recombination point uniformly along the branches beneath the root of , where is a branch and is a time along that branch; (iii) dissolving the branch above point ; and (iv) allowing to rejoin the remainder of tree above time by the standard coalescent process, creating a new tree (Figure 1B). As a generative process for an arbitrary number of genomic segments, the SMC can be implemented by simply repeating the iterative process until then setting equal to and equal to .
Notice that, if the sampled recombination points are retained, this process generates not only a sequence of local trees but a complete ARG. In addition, a sampled sequence of local trees, , is sufficient for generation of aligned DNA sequences corresponding to the leaves of the trees (Figure 1C). Augmented in this way, the SMC can be considered a full generative model for ARGs and sequence data.
The Discretized Sequentially Markov Coalescent
We now define an approximation of the SMC that is discrete in both space and time, which we call the Discretized Sequentially Markov Coalescent (DSMC). The DSMC can be viewed as a generalization to multiple genomes of the discretized pairwise sequentially Markov coalescent (PSMC) used by Li and Durbin [42]. It is also closely related to several other recently described discretized Markovian coalescent models [39], [40], [50].
The DSMC assumes that time is partitioned into intervals, whose boundaries are given by a sequence of time points , with , for all (), and equal to a user-specified maximum value. (See Table 1 for a key to the notation used in this paper.) Every coalescence or recombination event is assumed to occur precisely at one of these time points. Various strategies can be used to determine these time points (see, e.g., [50]). In this paper, we simply distribute them uniformly on a logarithmic scale, so that the resolution of the discretization scheme is finest near the leaves of the ARG, where the density of events is expected to be greatest (see Methods). Each local block is assumed to have an integral length measured in base pairs, with all recombinations occurring between adjacent nucleotides. The DSMC approaches the SMC as the number of intervals and the sequence length grow large, for fixed and .
Like the SMC, the DSMC generates an ARG for (haploid) sequences, each containing nucleotides (Figure 1B). In the discrete setting, it is convenient to define local trees and recombination events at the level of individual nucleotide positions. Assuming that denotes a recombination between and , we write , with for positions and . Notice that it is possible in this setting that and . Where a recombination occurs (), we write where is the branch in and is the time point of the recombination. For simplicity and computational efficiency, we assume that at most one recombination occurs between each pair of adjacent sites. Given the sparsity of variant sites in most data sets, this simplification is likely to have, at most, a minor effect during inference (see Discussion).
Like the SMC, the DSMC can additionally be used to generate an alignment of DNA sequences (Figure 1C). We denote such an alignment by , where each represents an alignment column of height . Each can be generated, in the ordinary way, by sampling an ancestral allele from an appropriate background distribution, and then allowing this allele to mutate stochastically along the branches of the corresponding local tree, in a branch-length-dependent manner. We denote the induced conditional probability distribution over alignment columns by , where is the mutation rate. In this work, we assume a Jukes-Cantor model [53] for nucleotide mutations along the branches of the tree, but another mutation model can easily be used instead. Notice that, while the recombinations are required to define the ARG completely, the probability of the sequence data given the ARG depends only on the local trees .
The Threading Problem
In the case of an observed alignment, , and an unobserved ARG, , the DSMC can be viewed as a hidden Markov model (HMM) with a state space given by all possible local trees, transition probabilities given by expressions of the form , and emission probabilities given by the conditional distributions for alignment columns, . The complete data likelihood function of this model—that is, the joint probability of an ARG and a sequence alignment given model parameters —can be expressed as a product of these terms over alignment positions (see Methods for further details):
This HMM formulation is impractical as a framework for direct inference, however, because the set of possible local trees—and hence the state space—grows super-exponentially with . Even with additional assumptions, similar approaches have only been able to accommodate small numbers of sequences [32], [35], [54].
Instead, we use an alternative strategy with better scaling properties. The key idea of our approach is to sample the ancestry of only one sequence at a time, while conditioning on the ancestry of the other sequences. Repeated applications of this “threading” operation form the basis of a Markov chain Monte Carlo sampler that explores the posterior distribution of ARGs. In essence, the threading operation adds one branch to each local tree in a manner that is consistent with the assumed recombination process and the observed data (Figure 2). While conditioning on a given set of local trees introduces a number of technical challenges, the Markovian properties of the DSMC are retained in the threading problem, and it can be solved using standard dynamic programming algorithms for HMMs.
The threading problem can be precisely described as follows. Assume we are given an ARG for sequences, , a corresponding data set , and a set of model parameters Assume further that is consistent with the assumptions of the DSMC (for example, all of its recombination and coalescent events occur at time points in and it contains at most one recombination per position). Finally, assume that we are given an th sequence , of the same length of the others, and let The threading problem is to sample a new ARG from the conditional distribution under the DSMC.
The problem is simplified by recognizing that can be defined by augmenting with the additional recombination and coalescence events required for the th sequence. First, let be represented in terms of its local trees and recombination points: . Now, observe that specifying the new coalescence events in is equivalent to adding one branch to each local tree, for , to obtain a new tree (Figure 2). Let us denote the point at which each of these new branches attaches to the smaller subtree at each genomic position by , where indicates a branch in and indicates the coalescence time along that branch. Thus, the coalescence threading of the th sequence is given by the sequence .
To complete the definition of , we must also specify the precise locations of the additional recombinations associated with the threading—that is, the specific time point at which each branch in a local tree was broken before the branch was allowed to re-coalesce in a new location in tree . Here it is useful to partition the recombinations into those that are given by , denoted , and those new to , which we denote (Figure 3A&B). Each is either null (), meaning that there is no new recombination between and , or defined by , where is a branch in and is the time along that branch at which the recombination occurred. We call the recombination threading of the th sequence. For reasons of efficiency, we take a two-step approach to threading: first, we sample the coalescence threading , and second, we sample the recombination threading conditional on . This separation into two steps allows for a substantially reduced state space during the coalescence threading operation, leading to significant savings in computation. When sampling the coalescence threading (step one), we integrate over the locations of the new recombinations , as in previous work [42], [50]. Sampling the recombination threading (step two) can be accomplished in a straightforward manner independently for each recombination event, by taking advantage of the conditional independence structure of the DSMC model (see Methods for details).
The core problem, then, is to accomplish step one by sampling the coalescence threading from the distribution,
where the notation indicates that random variable is held fixed (“clamped”) at a particular value throughout the procedure. This equation defines a hidden Markov model with a state space given by the possible values of each , transition probabilities given by and emission probabilities given by (Figure 3C). Notice that the location of each new recombination, , is implicitly integrated out in the definition of . Despite some unusual features of this model—for example, it has a heterogeneous state space and normalization structure along the sequence—its Markovian dependency structure is retained, and the problem of drawing a coalescent threading from the desired conditional distribution can be solved exactly by dynamic programming using the stochastic traceback algorithm for HMMs. Additional optimizations allow this step to be completed in time linear in both the number of sequences and the alignment length and quadratic only in the number of time intervals (see Methods for details).
Markov Chain Monte Carlo Sampling
The main value of the threading operation is in its usefulness as a building block for Markov chain Monte Carlo methods for sampling from an approximate posterior distribution over ARGs given the data. We employ three main types of sampling algorithms based on threading, as described below.
Sequential sampling
First, the threading operation can be applied iteratively to a series of orthologous sequences to obtain an ARG of size from sequence data alone. This method works by randomly choosing one sequence and constructing for it a trivial ARG (i.e. every local tree is a single branch). Additional sequences are then threaded into the ARG, one at a time, until an ARG of sequences has been obtained. Notice that an ARG derived in this manner is not a valid sample from the posterior distribution, because each successive (for ) is sampled conditional on only (the first sequences). Nevertheless, the sequential sampling algorithm is an efficient heuristic method for obtaining an initial ARG, which can subsequently be improved by other methods. If desired, this operation can be applied multiple times, possibly with various permutations of the sequences, to obtain multiple initializations of an MCMC sampler. Heuristic methods can also be used to choose a “smart” initial ordering of sequences. For example, one might begin with one representative of each of several populations, to first approximate the overall ARG structure, and subsequently add more representatives of each population.
Gibbs sampling for single sequences
Second, the threading operation can serve as the basis of a Gibbs sampler for full ARGs. Starting with an initial ARG of sequences, individual sequences can be removed, randomly or in round-robin fashion, and rethreaded. Since the threading procedure samples from the conditional distribution , this produces a valid Gibbs sampler for the ARG up to the assumptions of the DSMC. The ergodicity of the Markov chain follows, essentially, from the fact that any tree is reachable from any other by a finite sequence of branch removals and additions (see Text S1 for details).
The main limitation of this method is that it leads to poor mixing when the number of sequences grows large. The essential problem is that rethreading a single sequence is equivalent to resampling the placement of external branches in the local trees, so this method is highly inefficient at rearranging the “deep structure” (internal branches) of the ARG. Furthermore, this mixing problem becomes progressively worse as grows larger. Indeed, as approaches infinity, the single-sequence threading operation reduces to a procedure that selects a sequences of short genealogy “tips” leading to other sequences in the data set, leaving all other aspects of the ARG unchanged; in effect, it approaches the “copying” model of Li and Stephens [43]. As a result, an alternative strategy for ARG sampling is needed for large numbers of sequences.
Subtree sampling
The third sampling strategy addresses the mixing limitations of the single-sequence Gibbs sampler by generalizing the threading operation to accommodate not only individual sequences but subtrees with arbitrary numbers of leaves. As a result, internal branches in the local trees can be resampled and the full ARG can be perturbed, including the deep branches near the roots of the local trees.
In principle, one could address the subtree threading problem by arbitrarily selecting an internal branch for each nonrecombining segment of the ARG and resampling its attachment point to the remainder of the tree, by essentially the same procedure used for the reattachment of external branches in single-sequence threading. The problem is that, because the local trees change along the sequence, it is impossible in general to select a sequence of internal branches whose subtrees are maintained across the entire ARG (this is possible only for external branches). Furthermore, if a poor sequence of internal branches is selected, the attachment points at both ends of each segment will be constrained by the flanking local trees, creating a strong tendency to resample the original attachment points, which would result in poor mixing of the sampler.
To address this problem, we devised a novel method for selecting sequences of subtrees guaranteed to have good continuity properties. Once such a sequence is selected, the subtree threading operation can be accomplished efficiently using the stochastic traceback algorithm, in a similar manner as with single sequences. Our algorithm for selecting sequences of internal branches is fairly technical in nature and a detailed description is left for Text S1. Briefly, to select sequences of subtrees, we use a data structure called a branch graph, which traces the shared ancestry among branches across genomic positions. Using dynamic programming, we are able to identify paths through the branch graph that correspond to sequences of internal branches with good continuity properties. After a sequence of internal branches is identified, the selected branch is removed from each local tree, splitting it into a main tree and a subtree. A new branch is then added above the root of every subtree and allowed to re-coalesce with the corresponding main tree in a manner consistent with the DSMC.
One important limitation of the algorithm is worth noting. As in the single-sequence case, the stochastic traceback algorithm samples from the desired conditional distribution over subtree threadings. However, since the number of ways of removing internal branches depends on the current structure of the ARG, the Hastings ratio is not equal to one in this case, and a more general Metropolis-Hastings algorithm (with rejection of some proposed threadings) is required (see Text S1 for details). In practice, the acceptance rates for proposed threadings are fairly high (∼40% for typical human data), and despite this limitation, Metropolis-Hastings subtree threading considerably improves the mixing properties of the Gibbs sampler for moderately large values of (see below).
ARGweaver Program and Visualization
We implemented these sampling strategies in a computer program called ARGweaver, that “weaves” together an ARG by repeated applications of the threading operation. The program has subroutines for threading of both individual sequences and subtrees. Options allow it to be run as a Gibbs sampler with single-sequence threading or a general Metropolis-Hastings sampler with subtree threading. In either case, sequential sampling is used to obtain an initial ARG. Options to the program specify the number of sampling iterations and the frequency with which samples are recorded. The program is written in a combination of C++ and Python and is reasonably well optimized. For example, it requires about 1 second to sample a threading of a single 1 Mb sequence in an ARG of 20 sequences with 20 time steps. Our source code is freely available via GitHub (https://github.com/mdrasmus/argweaver).
To summarize and visualize samples from the posterior distribution over ARGs, we use two main strategies. First, we summarize the sampled ARGs in terms of the time to most recent common ancestor (TMRCA) and total branch length at each position along the genome. We also consider the estimated age of the derived alleles at polymorphic sites, which we obtain by mapping the mutation to a branch in the local tree and calculating the average time for that branch (see Methods). We compute posterior mean and 95% credible intervals for each of these statistics per genomic position, and create genome browser tracks that allow these values to be visualized together with other genomic annotations.
Second, we developed a novel visualization device for ARGs called a “leaf trace.” A leaf trace contains a line for each haploid sequence in an analyzed data set. These lines are ordered according to the local genealogy at each position in the genome, and the spacing between adjacent lines is proportional to their TMRCAs (Figure S2). The lines are parallel in nonrecombining segments of the genome, and change in order or spacing where recombinations occur. As a result, several features of interest are immediately evident from a leaf trace. For example, recombination hot spots show up as regions with dense clusters of vertical lines, whereas recombination cold spots are indicated by long blocks of parallel lines.
Simulation Study
Effects of discretization and convergence of sampler
Before turning to inference, we performed a series of preliminary experiments to verify that our discretization strategy allowed for an adequate fit to the data and that ARGweaver converged to a plausible posterior distribution for realistic simulated data sets. Briefly, we found that the DSMC produces similar numbers of recombination counts and segregating sites as the coalescent-with-recombination and SMC, when generating data under various recombination rates and effective population sizes (see Text S1 and Supplementary Figure S1). With small numbers of sequences, the Gibbs sampler based on the single-sequence threading operation appeared to converge rapidly, according to both the log likelihood of the sampled ARG and the inferred numbers of recombination events. When the number of sequences grew larger than about 6–8 (depending on the specific details of the simulation), the Gibbs sampling strategy was no longer adequate. However, the subtree threading operation and Metropolis-Hastings sampler appeared to address this problem effectively, allowing the number of sequences to be pushed to 20 or more. With 20 sequences 1 Mb in length, the sampler converges within about 500 sampling iterations, which takes about 20 minutes on a typical desktop computer (Supplementary Figure S3).
Recovery of global ARG features
Next, we systematically assessed the ability of ARGweaver to recover several features of interest from simulated ARGs over a range of plausible ratios of mutation to recombination rates (see Methods for simulation parameters). In these experiments, we considered three “global” features of the ARG: (i) the log joint probability of the ARG and the data (log of equation 2), (ii) the total number of recombinations, and (iii) the total branch length of the ARG. We define the total branch length of the ARG to be the sum of the total branch lengths of the local trees at all sites (in generations), a quantity proportional to the expected number of mutations in the history of the sample. We applied ARGweaver to each simulated data set with 500 burn-in iterations, followed by 1000 sampling iterations, with every tenth sample retained (100 samples total).
We found that ARGweaver was able to recover the features of interest with fairly high accuracy at all parameter settings (Figure 4A and Supplementary Figure S4). In addition, the variance of our estimates is generally fairly low, but does show a clear reduction as increases from 1 to 6, corresponding to an increase in the phylogenetic information per nonrecombining segment. Most current estimates of average rates would place the true value of for human populations between 1 and 2 [55]–[57], but the concentration of recombination events in hot spots implies that the ratio should be considerably more favorable for our methods across most of the genome. Notably, we do observe a slight tendency to under-estimate the number of recombinations, particularly at low values of . This underestimation is paired with an over-estimation of the joint probability (left column), suggesting that it reflects model misspecification of the DSMC. It is possible that this bias could be improved by the use of the SMC' rather than the SMC, or by a finer-grained discretization scheme (see Discussion).
Recovery of local ARG features
An advantage of explicitly sampling full ARGs is that it enables inferences about local features of the ARG that are not directly determined by model parameters. Using the same simulated data and inference procedure as in the previous section, we evaluated the performance of ARGweaver in estimating three representative quantities along the genome sequence: (i) time to most recent common ancestry (TMRCA), (ii) recombination rate, and (iii) allele age. We estimated each quantity using an approximate posterior expected value, computed by averaging across sampled ARGs. With 20 sequences, we found that ARGweaver was able to recover the TMRCA with fairly high accuracy and resolution (Figure 4B). The quality of the estimates degrades somewhat at lower values of the ratio but remains quite good even with (Supplementary Figure S5). We found that our power for recombination rates was weak with only 20 sequences, but with 100 sequences the reconstructed ARGs clearly displayed elevated rates of recombination in simulated hotspots compared with the flanking regions (Supplementary Figure S6). Estimates of allele ages appeared to be unbiased, with good concordance between true and estimated values, although the variance in the estimates was fairly high (Supplementary Figure S7, left column). Notably, the ARG-based estimates of allele age appear to be considerably better than estimates based on allele frequency alone (Supplementary Figure S7, right column). Together, these results suggest that, even with modest numbers of sequences, the distributions of ARGs inferred by our methods may be informative about loci under natural selection, local recombination rates, and other local features of evolutionary history.
Accuracy of local tree topologies
In our next experiment, we evaluated the accuracy of ARGweaver in inferring the topology of the local trees, again using the same simulated data. The local trees are a more complex feature of the ARG but are of particular interest for applications such as genotype imputation and association mapping. For comparison, we also inferred local trees using the heuristic Margarita program [34], which is, to our knowledge, the only other published ARG-inference method that can be applied at this scale. In addition, we applied an unpublished method, called treesim (http://niallcardin.com/treesim/index.html), that samples genealogies using heuristic extensions of the Monte Carlo methods of Fearnhead and Donnelly [22]. To compare these programs, we identified 100 evenly spaced locations in our simulated data sets, and extracted the local trees reconstructed by all three methods at these positions. We found that ARGweaver produced more accurate local tree topologies than both Margarita and treesim across most values of , except for the case of , where treesim performed slightly better (Supplementary Figure S8). The improvements were most pronounced at high values, where topological information is greatest. In addition, the absolute accuracy of the trees inferred by ARGweaver was fairly high, given the sparseness of informative sites in these data sets. For example, at , more than 80% of predicted branches were correct and Maximum Agreement Subtree (MAST) percentages approached 75%, and even in the challenging case of , over 60% of branches were correct and MAST percentages exceeded 50%. These results indicate that the sampler is effectively pooling information from many sites across the multiple alignment in making inferences about local tree topologies.
Finally, we evaluated the accuracy of ARGweaver's assessment of the uncertainty about the local trees given the data. We grouped individual branches into bins according to their estimated posterior probabilities (i.e., the fraction of sampled local trees in which each branch is found), and compared these values with the relative frequencies with which the same branches were observed in the true trees. We found that the predicted and actual probabilities of correctness were closely correlated, indicating that ARGweaver is accurately measuring the uncertainty associated with the local trees (Supplementary Figure S9). By contrast, the heuristic Margarita sampler shows a clear tendency to overestimate the confidence associated with branches in the local trees, often by 10–20%. This comparison is not entirely fair, because the authors of Margarita do not claim that it samples from the posterior distribution, but it nevertheless highlights an important advantage of the Bayesian approach. Notably, the unpublished treesim program performed remarkably well on this test.
Analysis of Real Data
Having demonstrated that ARGweaver was able to recover many features of simulated ARGs with reasonable accuracy, we turned to an analysis of real human genome sequences. For this analysis we chose to focus on sequences for 54 unrelated individuals from the “69 genomes” data set from Complete Genomics (http://www.completegenomics.com/public-data/69-Genomes) [58]. The 54 genome sequences were computationally phased using SHAPEIT v2 [59] and were filtered in various ways to minimize the influence from alignment and genotype-calling errors. They were partitioned into ∼2-Mb blocks and ARGweaver was applied to these blocks in parallel using the Extreme Science and Engineering Discovery Environment (XSEDE). For this analysis, we assumed generations, , and , implying . We allowed for variation across loci in mutation and recombination rates. For each ∼2-Mb block, we collected samples for 2,000 iterations of the sampler and retained every tenth sample, after an appropriate burn-in (see Methods for complete details). The entire procedure took ∼36 hours for each of the 1,376 2-Mb blocks, or 5.7 CPU-years of total compute time. The sampled ARGs were summarized by UCSC Genome Browser tracks describing site-specific times to most recent common ancestry (TMRCA), total branch length, allele ages, leaf traces, and other features across the human genome. These tracks are publicly available from our local mirror of the UCSC Genome Browser (http://genome-mirror.bscb.cornell.edu, assembly hg19).
Distortions in the ARG due to natural selection
While our prior distribution over ARGs is based on the neutral coalescent, we were interested in exploring whether natural selection produces a sufficiently strong signal in the data to create detectable distortions in the ARG near functional elements. We began by examining the estimated posterior expected values of the TMRCA around known protein-coding genes, focusing on fourfold degenerate (4d) sites within coding exons and noncoding sites flanking exons. For comparison with our ARG-based measures, we also computed a simple measure of nucleotide diversity, . Both and the ARG-based TMRCA behave in a qualitatively similar manner near genes, achieving minimal values in coding exons and gradually increasing with distance from exon boundaries (Figure 5A). These observations are consistent with several recent studies indicating reduced neutral diversity near both coding and noncoding functional elements, which has been attributed to indirect effects from selection at linked sites [60]–[64]. However, it has been difficult to distinguish between two alternative modes of selection both predicted to have similar influences on patterns of neutral diversity: “background selection” (BGS) associated with negative or purifying selection at linked sites [65]–[68], and “hitchhiking” (HH) (selective sweeps) associated with linked mutations under positive selection [69]. In principle, explicit ARG inference could help to resolve this controversy, because BGS and HH lead to different predictions for the structure of genealogies (e.g., [70], [71]).
To examine these questions further, we computed the same statistics for 255 putative partial selective sweeps identified in CEU populations and 271 partial sweeps identified in YRI populations based on the integrated extended haplotype homozygosity statistic (iHS) [72]. As expected, the sweep regions were broadly similar to the protein-coding genes in terms of nucleotide diversity (Figure 5B). However, unlike the protein-coding genes, the sweep regions displayed no clear depression in TMRCA. One possible way of understanding this observation is that, while sweeps tend to be enriched overall for recent coalescence events (as indicated by the reductions in ), the oldest coalescence events are relatively unaffected by selective sweeps, perhaps because some lineages tend to “escape” each sweep, leading to near-neutral patterns of coalescence near the roots of genealogies (where the contribution to the TMRCA is greatest). This may be particularly true for the partial sweeps identified by the iHS method, but a similar phenomenon should occur in flanking regions of the causal mutations for complete sweeps. BGS, by contrast, is expected to affect both the total branch length and TMRCA approximately equally, by effectively reducing the time scale of the coalescence process, but to have a minimal influence on the relative intervals between coalescence events.
In an attempt to distinguish further between BGS and HH, we introduced a statistic called the relative TMRCA halflife (RTH), defined as the ratio between the time to most recent common ancestry for the first 50% of chromosomes and the full TMRCA. The RTH captures the degree to which coalescence events are skewed toward the recent past, in a manner that does not depend on the overall rate of coalescence. Thus, the RTH should be relatively insensitive to BGS, but sensitive to HH if, as proposed above, sweeps tend to affect many but not all lineages (see Supplementary Figure S10). In the European populations, the statistic showed a pronounced valley near selective sweeps (Figure 5B), as expected, but it was much more constant across genic regions (Figure 5A). Its behavior was similar in the African populations, except that it showed somewhat more variability near genes, yet in an opposite pattern from the sweeps (Supplementary Figure S11). Overall, these results suggest that, while the total rate of coalescence differs substantially across genic regions, the relative depths of middle and extreme coalescence events do not, on average, consistent with the predictions of a model in which BGS dominates in genes [60], [62], [64]. The sharply contrasting patterns for the iHS-identified sweeps suggest that partial sweeps of this kind make at most a minor contribution to the reduced diversity near protein-coding exons. Nevertheless, these observations do not rule out the possibility that alternative modes of hitchhiking for which iHS has low power—such as recurrent hard or soft sweeps—might make a non-negligible contribution to patterns of variation near human protein-coding genes (see Discussion).
Genomic regions with extremely ancient most recent common ancestry
The previous section showed that genomic regions with reduced TMRCAs are often associated with purifying selection. To see whether the opposite signal was also of interest, we computed the posterior expected TMRCA in 10-kb blocks across the human genome and examined the regions displaying the oldest shared ancestry. Not surprisingly, four of the top twenty 10-kb blocks by TMRCA fall in the human leukocyte antigen (HLA) region on chromosome 6 (see Table 2). It has been known for decades that the HLA region exhibits extraordinary levels of genetic diversity, which is believed to be maintained by some type of balancing selection (overdominance or frequency-dependent selection) associated with the immunity-related functions of the HLA system [73]–[75]. The four HLA-related high-TMRCA blocks include three regions near HLA-F and one region between HLA-A and HLA-J (Supplementary Figure S12). All four high-TMRCA regions exhibit more than 12 polymorphisms per kilobase of unfiltered sequence, 8–10 times the expected neutral rate after normalizing for local mutation rates (as detailed in Table 2; see also Supplementary Figure S13). The estimated TMRCAs for these regions range from ∼340,000–380,000 generations, or ∼8.5–9.5 My (assuming 25-year generations).
Among these high-TMRCA blocks were two additional regions that displayed extraordinary levels of mutation-rate-normalized nucleotide diversity. The first of these, in a gene desert near the telomere of the long arm of chromosome 4, exhibits the deepest expected TMRCA in the genome, at >600,000 generations (15 My), and has >30 times the neutral polymorphism rate (Table 2). The second region is the PRIM2 gene on chromosome 6, which contributes the 4th and 7th highest TMRCA blocks in the genome, exhibiting polymorphism rates 28.0 and 12.8 times the neutral expectation, respectively. Both of these regions were identified as extreme outliers in a recent study of coincident SNPs in humans and chimpanzees, and it was argued that the PRIM2 gene was a likely target of balancing selection [76]. On closer inspection, however, we found that both regions were flagged by Complete Genomics as having “hypervariable” or “invariant” read depth across individuals, suggesting that the elevated SNP rates in our data are likely artifacts of copy number variation (CNV) at loci unduplicated in the reference genome. (Leffler et al. recently reached a similar conclusion about PRIM2 [77].) Despite that these flags were associated with only ∼5% of genomic positions, they indicated that five of our top six regions were likely CNVs (Table 2). Thus, for all subsequent analyses reported in this paper and for our publicly available browser tracks, we filtered out all regions labeled as invariant or hypervariable.
Once these extreme outliers were excluded, several loci of interest remained. In addition to the four HLA loci, these included (#5 in Table 2) an apparent cis-regulatory region downstream of the KCNE4 gene, which encodes a potassium voltage-gated channel (Supplementary Figure S14); (#9) an intronic interval in BCAR3, a gene involved in the development of anti-estrogen resistance in breast cancer (Supplementary Figure S15); (#16) an apparent regulatory region upstream of TULP4, a tubby-like protein that may be involved in ubiquitination and proteasomal degradation with a possible association with cleft lip (Supplementary Figure S16); and (#18) an intronic region in CRHR1, which encodes a GPCR that binds corticotropin releasing hormones, has roles in in stress, reproduction, immunity, and obesity, and is associated with alcohol abuse, asthma, and depression. Notably, all of these are predominantly noncoding regions that include multiple ChIP-seq-supported transcription factor binding sites. The estimated TMRCAs of these regions range from 335,000–450,000 generations (8.4–11.3 My), suggesting genetic variation in these loci considerably predates the human/chimpanzee divergence.
Segregating haplotypes shared between humans and chimpanzees
To explore the connection between extreme TMRCAs and balancing selection further, we examined 125 loci recently identified as having segregating haplotypes that are shared between humans and chimpanzees [77]. These loci are expected to be enriched for ancient polymorphisms maintained by balancing selection, although some may reflect independent occurrences of the same mutation in both species. We compared these putative balancing selection loci with neutral sequences having the same length distribution (see Methods), and found that their ARGweaver-estimated TMRCAs were clearly shifted toward higher values, with a mean value nearly twice as large as that of the neutral sequences (Supplementary Figure S17). In addition, the putative balancing selection loci that do not contain polymorphisms in CpG dinucleotides—which are less likely to have experienced parallel mutations—had slightly higher TMRCAs than the group as a whole.
If these loci are sorted by their estimated TMRCAs, several loci that were highlighted by Leffler et al. [77] for having more than two pairs of shared SNPs in high LD appear near the top of the list (Table 3). For example, the haplotype between the FREM3 and GYPE genes (#11 in Table 3; Supplementary Figure S18) contains shared SNPs in almost perfect LD with several expression quantitative trait loci (eQTLs) for GYPE, a close paralog of a gene (GYPA) that encodes a receptor for Plasmodium falciparum and may be under balancing selection. Another haplotype (#3) contains shared SNPs in significant LD with an eQTL for MTRR, a gene implicated in the regulation of folate metabolism, including one SNP that is also segregating in gorillas. In a third case (#18), the shared SNPs occur in a likely enhancer in an intron of IGFBP7, a gene that plays a role in innate immunity, among other functions. Another example is a locus near the ST3GAL1 gene (#7) that contains only one pair of shared SNPs but was suggested by a phylogenetic analysis to have an ancient origin [77]. Notably, all of these shared haplotypes fall outside of coding regions and several show signs of regulatory activity based on functional genomic data [77]. Their expected TMRCAs range from roughly 150,000 to 250,000 generations, or 3.8–6.3 My. Thus, the ARGweaver estimates of age are reasonably consistent with the hypothesis that these hapolotypes predate the human/chimpanzee divergence (estimated at 3.7–6.6 Mya [57]), an observation that is especially notable given that our analysis does not make direct use of data from chimpanzees.
By contrast, the loci near the bottom of the list (with the shortest TMRCAs) appear to be much less convincing. For example, the bottom 20 have expected ages of only 25,000–50,000 generations (0.65–1.3 My), suggesting that they actually post-date the human/chimpanzee divergence by millions of years. In addition, many of these regions appear hundreds of kilobases from the nearest gene, and they typically do not overlap regions with strong functional or comparative genomic evidence of regulatory potential. Indeed, if our ARG-based estimates of the TMRCA are interpreted literally, a majority of the 125 segregating haplotypes may post-date the human/chimpanzee divergence, which current estimates would place at ≥150,000 generations ago (see Supplementary Figure S17). This observation is in general agreement with rough calculations by Leffler et al. suggesting that the false discovery rate for ancient balancing selection in this set could be as high as 75% [77]. Thus, it appears that our ARG-based methods may be useful in distinguishing true ancestral polymorphisms from shared haplotypes that occur by chance due to homoplasy.
Natural selection and allele age
Next we examined the ARG-based expected ages of derived alleles at polymorphic sites in various annotation classes. Classical theory predicts that both deleterious and advantageous alleles will not only have skewed population frequencies but will also tend to be younger than neutral alleles at the same frequency, because directional selection will tend to accelerate a new mutation's path to fixation or loss [78]. This idea has recently been used to characterize selection in the human genome based on a haplotype-based summary statistic that serves as a proxy for allele age [79]. We computed ARG-based estimates of allele age in putatively neutral regions (Neut), fourfold degenerate sites in coding regions (4d), conserved noncoding sequences (CNS), missense coding mutations predicted by PolyPhen-2 to be “benign” (PPh:Benign), “possibly damaging” (PPh:PosDam), or “probably damaging” (PPh:ProbDam), and coding or noncoding mutations classified by the ClinVar database (http://www.ncbi.nlm.nih.gov/clinvar) as “nonpathogenic” (categories 1–3; CV:NonPath) or “pathogenic” (categories 4 & 5; CV:Path) based on direct supporting evidence of phenotypic effects. We found, indeed, that the Neut mutations were significantly older, on average, than all other classes (Figure 6A). In addition, among the missense coding mutations, PPh:Benign mutations were the oldest, PPh:PosDam were significantly younger, and PPh:ProbDam mutations were the youngest. Similarly, mutations in the CV:NonPath class were significantly older than those in the CV:Path class. Interestingly, the 4d mutations showed substantially lower average ages (by >30%) than the Neut mutations. We attribute this reduction primarily to the effects of selection from linked sites (see [60]), although direct selection from mRNA secondary structure and exonic regulatory elements may also contribute to it.
In part, these differences in age simply reflect differences in the site frequency spectrum (SFS) across classes of mutations. For example, missense mutations are well known to be enriched for low-frequency derived alleles, which will tend to be younger, on average, than higher-frequency derived alleles. To account for the influence of allele frequency, we further grouped the sites in each annotation class by derived allele frequency and compared the average allele ages within each group (Figure 6B). As expected, the estimated ages increase with the derived allele frequency across all annotation classes. In addition, within each class we continue to observe approximately the expected rank-order in allele ages, with Neutral mutations being the oldest, 4d, PPh:Benign, CNS, and CV:NonPath mutations coming next, followed by PPh:PosDam, PPh:ProbDam, and CV:Path mutations. This analysis demonstrates that ARGweaver is able to obtain information about natural selection from allele ages beyond what can be obtained from the SFS alone.
Another way of viewing these results is to consider the reduction in allele age relative to the neutral expectation within each frequency group, across annotation classes (Supplementary Figure S19). As expected, these reductions are larger at higher allele frequencies, where sojourn times will tend to be longer. However, from this representation it is also clear that the reductions in age increase with frequency much more rapidly for the mutations under strong, direct selection than for the mutations at which selection from linked sites is expected to dominate. For example, at very low derived allele frequencies (singletons), the reduction in age of 4d mutations is roughly equal to that at PPh:PosDam mutations, whereas at higher derived allele frequencies the damaging mutations exhibit reductions in age 2–3 times larger. The reason for this observation is probably that the reduction in age for the nearly neutral sites is largely a consequence of reductions in the local effective population size due to selection at linked sites, while the reductions at sites under direct selection are driven by the influence of selection on sojourn times (see Supplementary Figure S19 for a detailed discussion). Consistent with this interpretation, CNS mutations show less reduction in age than 4d and PPh:Benign mutations at low frequencies, and more reduction at high frequencies, suggesting that CNS mutations are influenced less by selection at linked sites and more by direct selection.
Discussion
Several decades have passed since investigators first worked out the general statistical characteristics of population samples of genetic markers in the presence of recombination [21], [80]–[83]. Nevertheless, solutions to the problem of explicitly characterizing this structure in the general case of multiple markers and multiple sequences—that is, of making direct inferences about the ancestral recombination graph (ARG) [19], [20]—have been elusive. Recent investigations have led to important progress on this problem based on the Sequentially Markov Coalescent (SMC) [17], [37]–[42], but existing methods are still either restricted to small numbers of sequences or require severe approximations. In this paper, we introduce a method that is faithful to the SMC yet has much better scaling properties than previous methods. These properties depend on a novel “threading” operation that can be performed in a highly efficient manner using hidden Markov modeling techniques. Inference does require the use of Markov chain Monte Carlo (MCMC) sampling, which has certain costs, but we have shown that the sampler mixes fairly well and converges rapidly, particularly if the threading operation is generalized from single sequences to subtrees. Our methods allow explicit statistical inference of ARGs on the scale of complete mammalian genomes for the first time. Furthermore, the sampling of ARGs from their posterior distribution has the important advantage of allowing estimation of any ARG-derived quantity, such as times to most recent common ancestry, allele ages, or regions of identity by descent.
Despite our different starting point, our methods are similar in several respects to the conditional sampling distribution (CSD)-based methods of Song and colleagues [49]–[52]. Both approaches consider a conditional distribution for the th sequence given the previous sequences, and in both cases a discretized SMC is exploited for efficiency of inference. However, the CSD-based methods consider the marginal distribution of the th sequence only given the other sequences and never explicitly reconstruct an ARG, while ours considers the joint distribution of an ARG of size and the th sequence, given an ARG of size and the previous sequences. In a sense, we have employed a “data augmentation” strategy by explicitly representing full ARGs in our inference procedure. The main cost of this strategy is that it requires Markov chain Monte Carlo methods for inference, rather than allowing direct likelihood calculations and maximum-likelihood parameter estimation. The main benefit is that it provides an approximate posterior distribution over complete ARGs and many derived quantities, including times to most recent common ancestry, allele ages, and distributions of coalescence times. By contrast, the CSD-based methods provide information about only those properties of the ARG that are directly described by the model parameters. We view these two approaches as complementary and expect that they will have somewhat different strengths and weaknesses, depending on the application in question.
Our explicit characterization of genealogies can be exploited to characterize the influence of natural selection across the genome, as shown in our analysis of the Complete Genomics data set. In particular, we see clear evidence of an enrichment for ancient TMRCAs in regions of known and predicted balancing selection, reduced TMRCAs near protein-coding genes and selective sweeps, and reduced allele ages in sites experiencing both direct selection and selection at closely linked sites. Interestingly, the genealogical view appears to have the potential to shed light on the difficult problem of distinguishing between background selection and hitchhiking. Our initial attempt at addressing this problem relies on a genealogy-based summary statistics, the relative TMRCA halflife (RTH), that does appear to distinguish effectively between protein-coding genes and partial selective sweeps identified by iHS. However, more work will be needed to determine how well this approach generalizes to other types of hitchhiking (e.g., complete sweeps, soft sweeps, recurrent sweeps) and whether additional genealogical information can be used to characterize the mode of selection more precisely. Additional work is also needed to determine whether our ARG-based allele-age estimator—which is highly informative in bulk statistical comparisons but has high variance at individual sites—can be used to improve functional and evolutionary characterizations of particular genomic loci. A related challenge is to see whether our genome-wide ARG samples can be used to improve methods for association/LD mapping (see [34], [84]–[88]).
In addition to natural selection, our methods for ARG inference have the potential to shed light on historical demographic processes, an area of particular interest in the recent literature [16], [17], [51], [52], [89]. To explore the usefulness of ARGweaver in demography inference, we attempted to infer a population phylogeny with admixture edges for the 11 human populations represented in the Complete Genomics data set, based on the genealogies sampled under our naive (panmictic) prior distribution. We extracted 2,304 widely spaced loci from our inferred ARGs, obtained a consensus tree at each locus, and reduced this tree to a subtree with one randomly selected chromosome for each of the 11 populations (see Text S1 for details). We then analyzed these 11-leaf trees with the PhyloNet program [90], [91], which finds a population tree that minimizes the number of “deep coalescences” required for reconciliation with a given set of local trees, allowing for both incomplete lineage sorting and hybridization (admixture) events between groups. PhyloNet recovered the expected phylogeny for these populations in the absence of hybridization and generally detected complex patterns of gene flow where they are believed to have occurred, but it had difficulty reconstructing the precise relatinonships among source and admixed populations (Supplementary Figure S20). These experiments suggested that the posterior distribution of ARGs does appear to contain useful information about population structure even when a noninformative prior distribution is used, but that additional work will be needed to fully exploit the use of ARG inference in demographic analysis.
An alternative strategy would be to extend our methods to incorporate a full phylogenetic demographic model, such as the one used by G-PhoCS [92], thereby generalizing this fully Bayesian method to a setting in which recombination is allowed and complete genome sequences are considered. Importantly, the use of the complete ARG would allow information about demographic history from both patterns of mutation and patterns of linkage disequilibrium to be naturally integrated (see [92]). However, as with CSD-based methods [51], [52], an extension to a full, parametric multi-population model for application on a genome-wide scale would be technically challenging. In our case, it would require the ability to sample “threadings” consistent with the constraints of a population model (e.g., with no coalescent events between genetically isolated populations) and exploration of a full collection of population parameters, which would likely lead to slow convergence and long running times. Nevertheless, a version of this joint inference strategy may be feasible with appropriate heuristics and approximations. Our methods may also be useful for a wide variety of related applications, including local ancestry inference [47], [93], [94], haplotype phasing/genotype imputation [46], [48], [95], [96], and recombination rate estimation [22], [97].
Our initial implementation of ARGweaver relies on several simplying assumptions that appear to have minimal impact on performance with (real or simulated) human sequence data, but may produce limitations in other settings. Following Li and Durbin [42], we compute probabilities of recombination between discrete genomic positions under the assumptions of the continuous-space SMC [37]. When recombination rates are low, the discrete and continuous models are nearly identical, but the differences between them can become significant when recombination rates are higher [98]. Similarly, our assumption of at most one recombination event per site and our use of the SMC rather than the improved [38] may lead to biases in cases of higher recombination rates, larger numbers of sequences, or more divergent sequences. In addition, our heuristic approach of accommodating zero-length branches by randomly sampling among “active” branches for coalescence and recombination events (see Methods) may lead to biases when the discretization scheme is coarse relative to evolutionary events of interest. Finally, we currently assume haploid genome sequences as input, which, in most cases of current interest, requires computational phasing as a pre-processing step. Phasing errors may lead to over-estimation of recombination and mutation rates and associated biases, because the sampler will tend to compensate for them with additional recombination and/or mutation events. In principle, most of these limitations can be addressed within our framework. For example, it should be fairly straightforward to extend ARGweaver to use the SMC' and Hobolth and Jensen's finite-loci transition density. In addition, we believe it is possible to enable the program to work directly with unphased data and integrate over all possible phasings (see, e.g., [92], [99]).
The ability to perform explicit ARG inference on the scale of complete genomes opens up a wide range of possible applications, but the long running times required for these analyses and the unwieldy data structures they produce (numerous samples of ARGs) are potential barriers to practical usefulness. In our initial work, we have attempted to address this problem by precomputing ARGs for a highly informative public data set and releasing both our complete ARGs and various summary statistics as browser tracks for use by other groups. We have also developed a simple web interface that allows users to retrieve local trees and several useful summary statistics for specified genomic intervals, populations, and individuals (http://compgen.bscb.cornell.edu/ARGweaver/CG_results). In future work, it may be possible to improve data access by providing more sophisticated tools for data retrieval and visualization. For example, sampled ARGs could be stored in a database in a manner that allowed researchers to efficiently extract features such as regions of IBD or recombination maps for designated subsets of samples. A related possibility would be to support on-the-fly threading of user-specified query sequences into precomputed ARGs. This operation would be analogous to local ancestry inference [47], [93], [94], but would reveal not only the population sources of query sequence segments, but also additional information about recombination events, coalescence times, approximate mutation ages, and other features. The same operation could be used to allow our sampling methods to scale to thousands of genomes: one could infer ARGs for, say, 100 genomes, then simply thread in hundreds more, without full MCMC sampling. In general, we believe that posterior samples of ARGs will be a rich resource for genetic analysis, but additional work is needed on data storage and query interfaces for these samples to become practically useful to large numbers of genomic researchers.
Methods
Discretized Sequentially Markov Coalescent
Discretization scheme and notation
The Discretized Sequentially Markov Coalescent (DSMC) assumes that all coalescence and recombination events occur at discrete time points, , with (the present time) and equal to a user-specified maximum value. These time points are defined in units of generations before the present time. We evenly distribute these time points on a logarithmic scale, so that the discretization scheme has finer resolution near the leaves of the ARG, where more events are expected to occur. Specifically, we define (for ) to be , where
Here, is the maximum time and is a tuning parameter that, when increased, causes the time points to become more densely clustered near the leaves of the ARG. Notice that and . In this work, we have assumed generations and . We denote the length of time interval as . The DSMC process is defined such that it approaches the continuous SMC as a limit as and each , with sufficiently large that the probability of a coalescence event older than is close to zero.
It is useful to specify “midpoints” between time points (on a log scale), to facilitate rounding of continuous-valued times to the nearest discrete time point. We define the midpoint between times and (for ) as . We can alternatively refer to the midpoint between times and as (for ), noting that . Coalescence events that occur between and are “rounded” to time point . We found that it was less critical to round recombination events to the nearest time point, so they are simply rounded to the next most recent time point (see below). We denote the lengths of the half intervals between and , and between and , as and , respectively.
Because all coalescence events must occur at the designated time points, the collection of branches is fixed for each interval between time points and . Given a local tree that is consistent with the DSMC, we denote the set of branches in time interval as . The size of this set, , is of particular interest, and is abbreviated (with clear from context). In addition, it is often of interest to consider the branch sets for a tree from which a branch has been removed. We denote such a tree by and abbreviate the number of branches in interval as (again, with clear from context).
One consequence of discretizing time is that the DSMC will tend to generate ARGs that contain many branches of length zero (corresponding to polytomies in the local trees), which will have zero probability of recombination, coalesce, or mutation events. In effect, the rounding procedure will tend to shrink short branches to zero, which may lead to distortions in data generation and inference. We address this problem heuristically, by defining the DSMC to first sample the times of recombination and coalescence events, and then randomly select a branch from all of those “active” at the sampled time point. We define the set of active branches at a time point , for a local tree , to be those branches in that start, end, or pass through . This set is denoted and its size is abbreviated as . As above, we use to indicate the active branches at excluding branch . Simulations indicate that this heuristic solution to the problem of zero-length branches works fairly well in practice (see Figure S1).
Recombination process
As in the standard SMC, recombinations are assumed to occur according to a Poisson process with rate , where is the total branch length of local tree and is the average number of recombinations/generation/site. Once a recombination occurs, the ordinary SMC process places the recombination uniformly along the branches of . The analogous operation of sampling a recombination branch and time point, , in the DSMC is accomplished by first sampling a time point in proportion to the total branch length present during time interval , then randomly selecting one of the branches active at that time point. Consistent with the assumptions of the SMC, the recombination point cannot occur above the time point associated with the root of tree , which we denote . Thus, the sampling distribution for a recombination point on a local tree is given by,
where is a constant that explicitly normalizes the distribution over time points . The special case for the time point at the root of the tree, , is required because the SMC does not allow recombinations to occur beyond this point, so the effective number of active branches is only two at this time point, despite that will have a value of three. The number of branches in the interval above the root, , is necessarily one, so this term can be omitted in this case.
This sampling distribution effectively rounds the times of recombination events downward to the next most recent time point. However, a strict policy of downward rounding, together with a prohibition again recombination events above the root node, would make it impossible to sample recombination events at time point , which turns out to have undesirable effects in inference (it makes some trees unreachable by the threading operation). Therefore, when sampling time points, we use the heuristic approach of imagining that recombinations can also occur in the time interval immediately above the root and assigning these events to the time point . This has the effect of redistributing some of the probability mass from later time points to the root, without altering the overall rate at which recombinations occur (). For this reason, the normalizing constant differs slightly from the total branch length ; in particular, . It would be slightly more elegant to allow upward as well as downward rounding of times for recombinations, as we do with coalescence events (see below), but as long as the time discretization is not too coarse these differences are of minor importance, and the approach we have used seems to be adequate.
Re-coalescence process
Once a recombination point is sampled, the selected branch is removed from time points and older, and allowed to re-coalesce to the remainder of the tree, in a manner analogous to the SMC. Because we explicitly prohibit multiple recombinations between adjacent positions, the local tree must be reachable from by a single “subtree pruning and regrafting” (SPR) operation corresponding to the recombination, i.e., an operation that cuts a branch of the tree at the recombination point and re-attaches it (and any descendant nodes) to the remainder of the tree. Thus, we can write,
where is a function that returns the new tree produced by an SPR operation on that cuts branch at time and re-attaches it to branch at time , and is a joint conditional distribution over re-coalescence branches and time points.
The main challenge is therefore to define the discrete re-coalescence distribution, , for (as required by the SMC). There are two distinct cases to consider: and . When , the unattached branch must first fail to re-coalesce during the interval between and , and then must re-coalesce between and (because all such re-coalescence events will be rounded to ). By contrast, when , the branch must simply re-coalesce between () and (because the re-coalescence time is strictly bounded by the recombination time).
In all cases, the instantaneous rate of re-coalescence in each interval () is given by , in the standard manner for the coalescent. (Note that we use rather than , because we are concerned with the coalescence rate to the remainder of the tree, excluding branch . We also assume a diploid species throughout, so the total number of chromosomes per locus is .) The probability that a lineage starting at a time coalesces before is given by the cumulative distribution function for exponentially distributed waiting times,
and the probability of coalescence during a sequences of intervals, is given by,
Similarly, the probabilities of coalescence during the half intervals before and after time point are given, respectively, by,
Thus, the distribution of re-coalescence times for the case of is given by,
The probability of re-coalescence for the case of is simply,
Finally, the requirement for re-coalescence by the maximum time, , is enforced by explicitly normalizing the distribution:
Once the coalescence time point is chosen, a lineage is uniformly chosen from the active lineages in at that time point, similar to the process for recombination events. Thus, , and equation 6 can be rewritten as,
where is given by equations 10–12.
Initial local tree
The DSMC begins by generating an initial local tree, , using a discretized version of the coalescent process. This process can be decomposed into two steps: (1) the generation of a sequence of branch counts, for time points , and (2) sampling of a topology consistent with these branch counts. The probability of an observed initial tree can therefore be calculated as,
where is a vector of effective population sizes, . The branch count for time 0 is constrained to be equal to the number of samples, , and the branch count for time is required to be one, (see below).
Since the coalescent process is Markovian in time, the distribution for the vector of branch counts can be factored by time intervals,
with degenerate first and last terms, and .
The conditional distributions of the form , for , have been derived previously as [100],
Hidden Markov Model
Hidden Markov model for full threading problem
As noted in the Results section, the complete data likelihood function under the DSMC is given by equation 2. If the full ARG is regarded as a latent variable, this equation defines a hidden Markov model with a state space given by all possible pairs , transition probabilities given by expressions of the form and emission probabilities given by (see Figure 3A). The transition probabilities can be computed using equations 5 and 13, and the emission probabilities can be computed using Felsenstein's pruning algorithm. This model can be viewed as an instance of the “phylo-HMMs” that have been widely used in comparative genomics [101]. As discussed in the Results section, however, unless the number of sequences is very small, the state space of this HMM will be too large to allow it to be used directly for inference.
Instead, we constrain the inference problem by fixing the ARG for the first sequences, , and sampling from the conditional distribution . Using the notation and , we define , where is a vector of coalescence points such that indicates a coalescence of the th sequence to branch and time point of local tree , and , where is a vector of recombination points such that indicates a recombination at branch and time point of local tree between positions and . (Note that is undefined.) Thus, we can sample from the desired conditional distribution by sampling from . We refer to a sample from this distribution as a threading of the th sequence through the ARG (see Figure 3B). For now, we will consider a complete threading , but in later sections we will describe our two-step process for sampling, first, the coalescent threading , and second, the recombination threading given .
Note that the restriction to one recombination event per position implies that wherever , and that wherever . This restriction is not strictly required but it simplifies the description of new recombination events , and in the setting of interest here it comes with little cost (see Discussion).
It turns out to be more convenient to work with the joint distribution (the complete data likelihood) than with the conditional distribution . However, to emphasize that the variables and are held fixed (“clamped”) at pre-specified values throughout the threading operation, we denote them as and , and refer to the distribution of interest as . (Notice that the data are also clamped, as usual for HMMs.) When , , and are clamped,
Thus, samples of drawn in proportion to the unnormalized density will be valid samples from the desired conditional distribution. In general, any clamped joint density function, , can be viewed as an unnormalized version of a corresponding conditional density function, , but sometimes the joint density is more convenient to manipulate.
We can now write the density function for the (unnormalized) sampling distribution for a threading as,
where all terms are computable using previously described expressions, as for equation 2.
Notice that this threading HMM has the same conditional independence structure as the HMM for the full DSMC (equation 2, Figure 3), but its state space is now defined by sets of possible pairs rather than the set of possible pairs, making it far more tractable for inference.
Reduced model for coalescent threading
The state space can be reduced further by proceeding in two steps. First, we sample a coalescent threading from the marginal distribution . Then we sample a recombination threading, , from the conditional distribution . Notice that the data need not be considered when sampling the recombination threading, because is conditionally independent of given , , and .
The marginal distribution can be computed efficiently by changing the order of products and sums in the usual way for HMMs:
This equation defines an HMM with a state space given by the possible values of only, the size of which is bounded by , where is the number of sequences and is the number of time intervals (see Figure 3C).
While this model has the conditional independence structure of a standard HMM, the state space is heterogeneous along the sequence, because the set of possible coalescent points at each position depends on the local tree, . (The full threading HMM described above also has this property.) If we denote the state space at position as , the transition probabilities between states in position and states in position are defined by a transition matrix where and index the states of and , respectively, and can be computed as,
using equations 5 and 13. The emission probability for alignment column in state in is denoted and can be computed using Felsenstein's pruning algorithm, as in all cases above. The initial state probabilities for the HMM are given by for and can be computed using equations 14–16.
Notice that, unlike with a standard, locally normalized HMM, it is not true in this model that . Furthermore, for two positions and , it is not true in general that , because of differences across positions in the local trees and recombination points . Similarly, it is not true that . Thus, this model is not only globally unnormalized, but it also has a heterogeneous local normalization structure across positions. Importantly, this heterogeneity stems directly from differences in the and and is inherent in the threading problem—that is, it is not possible to express the desired conditional distribution, , directly in terms of a locally normalized hidden Markov model (one in which all transition probabilities and all emission probabilities sum to one at each position in the sequence). For this reason, we find it most convenient to work with the unnormalized clamped joint distribution.
Stochastic traceback
Despite the unusual features of the HMM described in the previous section, it still permits the use of standard dynamic programming algorithms to integrate over all coalescent threadings (the forward or backward algorithms), obtain a most likely threading (the Viterbi algorithm), compute marginal posterior distributions for each (forward-backward algorithm), and sample threadings in proportion to their conditional probability [102], [103]. These algorithms depend only on the linear conditional independence structure of the model (and, equivalently, on its factorization into local transition and emission probabilities) and on the use of nonnegative potential functions, both properties that are maintained in this model.
We are primarily interested in a dynamic programming algorithm for sampling from the posterior distribution over HMM paths that is sometimes referred to as the stochastic traceback algorithm [103]–[105]. In our case, each application of this algorithm is guaranteed to sample a coalescent threading in proportion to the density , and equivalently, in proportion to the desired conditional distribution.
The stochastic traceback algorithm consists of a deterministic forward pass and a stochastic backward pass. The forward pass is identical to the forward algorithm. In our notation, the algorithm recursively fills out a matrix , , . Each represents the probability of a prefix of the data joint with a constraint on the state path at position . Here, , where the notation indicates the subsequence . After an initialization of , for , the algorithm proceeds iteratively for from 2 to and sets each value (for ) equal to,
Note that the heterogeneity of the state space along the sequence implies that portions of the matrix are left undefined.
In the backward pass, the algorithm samples a sequence one element at a time, starting with and working backward to . First, is simply sampled in proportion to . Then, for from down to 1, each is sampled conditional on in proportion to,
The limiting step of the algorithm is the forward pass, which in general requires time, where is the size of the state space, . However, in our case the structure of the matrices can be exploited to reduce the running time to (see Text S1).
It can be shown by induction on suffixes of that this procedure will correctly sample from the target distribution, . Briefly, in the base case, the suffix is by construction sampled from the density , which is proportional to the desired conditional distribution, . For the inductive case, assume has been sampled from . The procedure of sampling from given is equivalent to sampling from,
where the last step is possible because is conditionally independent of , , , and given . Thus, the algorithm will correctly sample from for all such that .
Sampling a recombination threading
The final step in the threading operation is to sample a recombination threading conditional on a coalescent threading and the clamped parameters. This step is greatly simplified by the fact that the individual values are conditionally independent of one another given the variables and the clamped and variables (see Figure 3B). Consequently, each can be sampled separately from the distribution,
where the variables are now clamped along with the and variables. Notice that the distribution on the RHS is the same one considered in equations 19 & 20. The normalizing constant for this distribution, for clamped values and , is given by the transition probability .
Notice that this distribution is implicitly degenerate in the case in which , owing to the limitation of at most one recombination event per position. In particular, if , then , hence . At the same time, notice that, if , a new recombination is still possible () even if and , because a branch could be broken by a recombination event but then re-coalesce at precisely its original position in the local tree.
When , the efficiency of sampling from this distribution can be improved by noting that most possible values still have zero probability. Let represent the set of values having nonzero probability for given values of , , and , where denotes the branch being threaded. There are two cases to consider, a main case and a special case. We will denote the corresponding subsets of values and , with . Recall that and , where and are branches in and , respectively, and and are time points from the set . In the main case, the recombination occurs on the new branch . Here, the recombination time must be at least as recent as both the old and new re-coalescence times, and . Thus, . Notice that .
The special case occurs when the recombination occurs not on the new branch, , but instead on , the branch to which re-coalesces at position . A recombination on branch , below the point at which joins it, followed by a re-coalescence of to (meaning that ) will produce a signature exactly like the symmetric case of a recombination on followed by a re-coalescence to (Supplementary Figure S21), so this scenario must also be considered. This case can only occur when and in the interval of time between the start of branch and . Recombinations on other branches need not be considered, because the existence of such a recombination would imply that , contrary to our assumption. Hence,
where is the time point of the child node of branch . As with , .
By enumerating the elements of , it is possible to sample each in time. The same approach can be used to enable calculation of the values (equation 20) in time.
Data Preparation
Simulated data
Except where noted otherwise, simulations were performed under the full coalescent-with-recombination model [21]. After generation of local trees, sequence alignments were generated using a finite-sites Jukes-Cantor model [53]. All simulations were performed using custom computer programs. Our standard simulation scheme involved the generation of of twenty 1-Mb sequences, assuming an effective population size of N = 10,000, a mutation rate of mutations/site/generation, and mutation-to-recombination rate ratios of (i.e., recombination rates of events/site/generation). One hundred replicate data sets were generated for each choice of . Alternative parameter values were used in certain cases, as noted in the text and figure captions.
Real data
Information about human polymorphisms came from the “69 Genomes” data set from Complete Genomics (CG) (http://www.completegenomics.com/public-data/69-Genomes). For each individual considered, we recorded the diploid genotype call reported for each position in the hg19 (Genome Reference Consortium Human Build 37) reference genome using CG's ‘masterVar’ files. We considered both “SNPs” and “length-preserving substitutions” in the masterVar file, and also noted positions where CG could not confidently assign a genotype. All other positions were assumed to be homozygous for the allele reported in the reference genome.
Borrowing from our previous work on demography inference [92], we applied several filters to these data to reduce the impact of technical errors from alignment, sequencing, genotype inference, and genome assembly. These filters include simple repeats, recent segmental duplications, and transposable elements. We phased the data using SHAPEIT v2 [59], guided by the pedigree information describing the relationships among the 69 individuals. After phasing, we removed the child in each trio, as well as all but the four grandparents in the 17-member CEU pedigree, leaving 54 unrelated individuals in our data set. From this set, we further filtered all CpG sites, sites with more than two observed alleles, and sites at which CG did not call a genotype in any of the 54 individuals. All genomic positions excluded by our filters were treated as missing data by ARGweaver, meaning that the program integrated over all possible nucleotides at these positions (as in [92]).
In order to account for region-specific variation in recombination and mutation rates, we used the HapMap phase II recombination map [106] and a mutation rate map estimated from alignments of several primate genomes, including chimpanzee (panTro2), orangutan (ponAbe2), and rhesus Macaque (rheMac2) [107]. Mutation rates were scaled to have an average of mutations/generation/site and were averaged over 100 kb non-overlapping windows. This value was obtained by assuming a genome-wide average of mutations/generation/site, and observing a reduction in nucleotide diversity when the CpG filter was applied.
Calls of hypervariable and invariant regions were obtained from the CG FTP site (ftp://ftp2.completegenomics.com). Copy number variant calls for each individual were obtained from a file named cnvDetailsDiploidBeta, which was extracted from an ASM-VAR-files tar archive.
Data Analysis
To sample ARGs genome-wide, we split each sequence alignment into non-overlapping segments of 2 Mb, flanked on each side by 100 kb of overlapping sequence. We chose a core set of 12 individuals (24 haplotypes) randomly such that each major population group was represented. We then used ARGweaver to sample ARGs for these genomes, assuming a population size of time steps, and a maximum time of generations. Our prior estimate of was based on an empirical estimate of from the CG sequence data, and an assumption of mutations per site per generation for non-CpG sites (see previous section). This initial step involved 500 sampling iterations, consisting of 100 initial iterations under an infinite sites assumption, and 400 iterations with the full finite sites model. The final sample from this initial step was used as a starting point for threading in the remaining genomes. Once these were threaded, we applied ARGweaver with infinite sites for 100 iterations, followed by 2400 iterations with the finite sites model. Samples were recorded every 10 iterations for the final 2000 iterations, for a total of 200 samples. For our genome-wide analyses, we integrated the separate 2.2 Mb analyses by setting a switchpoint at the middle of each overlapping 100 kb segment, in order to minimize boundary effects at the analyzed sites.
To compute the neutral CDFs in Figure S17, we used a set of putatively neutral regions obtained by removing all GENCODE (v15) genes plus 1000 bp flank on either side of each exon, as well as all mammalian phastCons elements plus 100 bp of flanking sequence. From the remaining portion of the genome, we sampled 1000 sets of 69 regions with the same distribution of lengths as the non-CpG regions identified by [77].
To estimate the allele age at each polymorphic site, we considered all local genealogies sampled at that position, discarding any sampled genealogies that required more than one mutation to explain the observed data. In addition, we required that all of the retained genealogies implied the same derived allele, excluding positions that violated this condition from our analysis. For the remaining cases, we estimated the allele age for each sample as the average age of the branch on which the mutation leading to the derived allele was assumed to occur by parsimony, and averaged this value across samples.
Supporting Information
Zdroje
1. Hein J, Schierup M, Wiuf C (2005) Gene genealogies, variation and evolution: a primer in coalescent theory. Oxford: Oxford University Press.
2. Wakeley J (2009) Coalescent theory: an introduction. Greenwood Village: Roberts & Co. Publishers.
3. Fisher RA (1930) The Genetical Theory of Natural Selection. Oxford: Oxford University Press.
4. WrightS (1931) Evolution in Mendelian Populations. Genetics 16: 97–159.
5. KimuraM (1962) On the probability of fixation of mutant genes in a population. Genetics 47: 713–719.
6. FelsensteinJ (1973) Maximum-likelihood and minimum-step methods for estimating evolutionary trees from data on discrete characters. Syst Zool 22: 240–249.
7. FelsensteinJ (1981) Evolutionary trees from DNA sequences: a maximum likelihood approach. J Mol Evol 17: 368–376.
8. MenozziP, PiazzaA, Cavalli-SforzaL (1978) Synthetic maps of human gene frequencies in Europeans. Science 201: 786–792.
9. KingmanJ (1982) The coalescent. Stoch Process Appl 13: 235–248.
10. SawyerSA, HartlDL (1992) Population genetics of polymorphism and divergence. Genetics 132: 1161–1176.
11. VoightBF, AdamsAM, FrisseLA, QianY, HudsonRR, et al. (2005) Interrogating multiple aspects of variation in a full resequencing data set to infer human population size changes. Proc Natl Acad Sci USA 102: 18508–18513.
12. KeightleyPD, Eyre-WalkerA (2007) Joint inference of the distribution of fitness effects of deleterious mutations and population demography based on nucleotide polymorphism frequencies. Genetics 177: 2251–2261.
13. BoykoAR, WilliamsonSH, IndapAR, DegenhardtJD, HernandezRD, et al. (2008) Assessing the evolutionary impact of amino acid mutations in the human genome. PLoS Genet 4: e1000083.
14. LawsonDJ, HellenthalG, MyersS, FalushD (2012) Inference of population structure using dense haplotype data. PLoS Genet 8: e1002453.
15. PalamaraPF, LenczT, DarvasiA, Pe'erI (2012) Length distributions of identity by descent reveal fine-scale demographic history. Am J Hum Genet 91: 809–822.
16. RalphP, CoopG (2013) The geography of recent genetic ancestry across Europe. PLoS Biol 11: e1001555.
17. HarrisK, NielsenR (2013) Inferring demographic history from a spectrum of shared haplotype lengths. PLoS Genet 9: e1003521.
18. Hudson RR (1991) Gene genealogies and the coalescent process. In: Futuyma D, Antonovics J, editors. Oxford Surveys in Evolutionary Biology, volume 7. pp. 1–44.
19. GriffithsRC, MarjoramP (1996) Ancestral inference from samples of DNA sequences with recombination. J Comput Biol 3: 479–502.
20. Griffiths R, Marjoram P (1997) An ancestral recombination graph. In: Donnelly P, Tavaré S, editors, Progress in Population Genetics and Human Evolution. Springer Verlag. pp. 257–270.
21. HudsonRR (1983) Properties of a neutral allele model with intragenic recombination. Theor Popul Biol 23: 183–201.
22. FearnheadP, DonnellyP (2001) Estimating recombination rates from population genetic data. Genetics 159: 1299–1318.
23. StephensM, DonnellyP (2000) Inference in molecular population genetics. Journal of the Royal Statistical Society Series B (Statistical Methodology) 62: 605–655.
24. KuhnerMK, YamatoJ, FelsensteinJ (2000) Maximum likelihood estimation of recombination rates from population data. Genetics 156: 1393–1401.
25. NielsenR (2000) Estimation of population parameters and recombination rates from single nucleotide polymorphisms. Genetics 154: 931–942.
26. KuhnerMK (2006) LAMARC 2.0: maximum likelihood and Bayesian estimation of population parameters. Bioinformatics 22: 768–770.
27. O'FallonBD (2013) ACG: rapid inference of population history from recombining nucleotide sequences. BMC Bioinformatics 14: 40.
28. HeinJ (1990) Reconstructing evolution of sequences subject to recombination using parsimony. Math Biosci 98: 185–200.
29. HeinJ (1993) A heuristic method to reconstruct the history of sequences subject to recombination. J Mol Evol 36: 396–405.
30. KececiogluJ, GusfieldD (1998) Reconstructing a history of recombinations from a set of sequences. Discrete Applied Mathematics 88: 239–260.
31. WangL, ZhangK, ZhangL (2001) Perfect phylogenetic networks with recombination. J Comput Biol 8: 69–78.
32. SongYS, HeinJ (2005) Constructing minimal ancestral recombination graphs. J Comput Biol 12: 147–169.
33. SongYS, WuY, GusfieldD (2005) Efficient computation of close lower and upper bounds on the minimum number of recombinations in biological sequence evolution. Bioinformatics 21 Suppl 1: i413–422.
34. MinichielloMJ, DurbinR (2006) Mapping trait loci by use of inferred ancestral recombination graphs. Am J Hum Genet 79: 910–922.
35. WuY (2009) New methods for inference of local tree topologies with recombinant SNP sequences in populations. IEEE/ACM Trans Comput Biol Bioinform 8: 182–193.
36. WiufC, HeinJ (1999) Recombination as a point process along sequences. Theor Popul Biol 55: 248–259.
37. McVeanGAT, CardinNJ (2005) Approximating the coalescent with recombination. Philos Trans R Soc Lond B Biol Sci 360: 1387–1393.
38. MarjoramP, WallJD (2006) Fast “coalescent” simulation. BMC Genet 7: 16.
39. HobolthA, ChristensenOF, MailundT, SchierupMH (2007) Genomic relationships and speciation times of human, chimpanzee, and gorilla inferred from a coalescent hidden Markov model. PLoS Genet 3: e7.
40. MailundT, DutheilJY, HobolthA, LunterG, SchierupMH (2011) Estimating divergence time and ancestral effective population size of Bornean and Sumatran orangutan subspecies using a coalescent hidden Markov model. PLoS Genet 7: e1001319.
41. MailundT, HalagerAE, WestergaardM, DutheilJY, MunchK, et al. (2012) A new isolation with migration model along complete genomes infers very different divergence processes among closely related great ape species. PLoS Genet 8: e1003125.
42. LiH, DurbinR (2011) Inference of human population history from individual whole-genome sequences. Nature 475: 493–496.
43. LiN, StephensM (2003) Modeling linkage disequilibrium and identifying recombination hotspots using single-nucleotide polymorphism data. Genetics 165: 2213–2233.
44. StephensM, ScheetP (2005) Accounting for decay of linkage disequilibrium in haplotype inference and missing-data imputation. Am J Hum Genet 76: 449–462.
45. MarchiniJ, HowieB, MyersS, McVeanG, DonnellyP (2007) A new multipoint method for genome-wide association studies by imputation of genotypes. Nat Genet 39: 906–913.
46. HowieBN, DonnellyP, MarchiniJ (2009) A flexible and accurate genotype imputation method for the next generation of genome-wide association studies. PLoS Genet 5: e1000529.
47. PriceAL, TandonA, PattersonN, BarnesKC, RafaelsN, et al. (2009) Sensitive detection of chromosomal segments of distinct ancestry in admixed populations. PLoS Genet 5: e1000519.
48. LiY, WillerCJ, DingJ, ScheetP, AbecasisGR (2010) MaCH: using sequence and genotype data to estimate haplotypes and unobserved genotypes. Genet Epidemiol 34: 816–834.
49. PaulJS, SongYS (2010) A principled approach to deriving approximate conditional sampling distributions in population genetics models with recombination. Genetics 186: 321–338.
50. PaulJS, SteinrückenM, SongYS (2011) An accurate sequentially Markov conditional sampling distribution for the coalescent with recombination. Genetics 187: 1115–1128.
51. SheehanS, HarrisK, SongYS (2013) Estimating variable effective population sizes from multiple genomes: a sequentially Markov conditional sampling distribution approach. Genetics 194: 647–662.
52. SteinruckenM, PaulJS, SongYS (2013) A sequentially Markov conditional sampling distribution for structured populations with migration and recombination. Theor Popul Biol 87: 51–61.
53. Jukes TH, Cantor CR (1969) Evolution of protein molecules. In: Munro H, editor, Mammalian Protein Metabolism, New York: Academic Press. pp. 21–132.
54. HusmeierD, WrightF (2001) Detection of recombination in DNA multiple alignments with hidden Markov models. J Comput Biol 8: 401–427.
55. KongA, GudbjartssonDF, SainzJ, JonsdottirGM, GudjonssonSA, et al. (2002) A high-resolution recombination map of the human genome. Nat Genet 31: 241–247.
56. KongA, FriggeML, MassonG, BesenbacherS, SulemP, et al. (2012) Rate of de novo mutations and the importance of father's age to disease risk. Nature 488: 471–475.
57. SunJX, HelgasonA, MassonG, EbenesersdottirSS, LiH, et al. (2012) A direct characterization of human mutation based on microsatellites. Nat Genet 44: 1161–1165.
58. DrmanacR, SparksAB, CallowMJ, HalpernAL, BurnsNL, et al. (2010) Human genome sequencing using unchained base reads on self-assembling dna nanoarrays. Science 327: 78–81.
59. DelaneauO, ZaguryJF, MarchiniJ (2013) Improved whole-chromosome phasing for disease and population genetic studies. Nat Methods 10: 5–6.
60. McVickerG, GordonD, DavisC, GreenP (2009) Widespread genomic signatures of natural selection in hominid evolution. PLoS Genet 5: e1000471.
61. CaiJJ, MacphersonJM, SellaG, PetrovDA (2009) Pervasive hitchhiking at coding and regulatory sites in humans. PLoS Genet 5: e1000336.
62. HernandezRD, KelleyJL, ElyashivE, MeltonSC, AutonA, et al. (2011) Classic selective sweeps were rare in recent human evolution. Science 331: 920–924.
63. GottipatiS, ArbizaL, SiepelA, ClarkAG, KeinanA (2011) Analyses of X-linked and autosomal genetic variation in population-scale whole genome sequencing. Nat Genet 43: 741–743.
64. LohmuellerKE, AlbrechtsenA, LiY, KimSY, KorneliussenT, et al. (2011) Natural selection affects multiple aspects of genetic variation at putatively neutral sites across the human genome. PLoS Genet 7: e1002326.
65. CharlesworthB, MorganMT, CharlesworthD (1993) The effect of deleterious mutations on neutral molecular variation. Genetics 134: 1289–1303.
66. HudsonRR, KaplanNL (1995) Deleterious background selection with recombination. Genetics 141: 1605–1617.
67. NordborgM, CharlesworthB, CharlesworthD (1996) The effect of recombination on background selection. Genet Res 67: 159–174.
68. CharlesworthB (2012) The effects of deleterious mutations on evolution at linked sites. Genetics 190: 5–22.
69. Maynard SmithJ, HaighJ (1974) The hitch-hiking effect of a favourable gene. Genet Res 23: 23–35.
70. BartonNH (1998) The effect of hitch-hiking on neutral genealogies. Genet Res 72: 123–133.
71. WalczakAM, NicolaisenLE, PlotkinJB, DesaiMM (2012) The structure of genealogies in the presence of purifying selection: a fitness-class coalescent. Genetics 190: 753–779.
72. VoightBF, KudaravalliS, WenX, PritchardJK (2006) A map of recent positive selection in the human genome. PLoS Biol 4: e72.
73. HughesAL, NeiM (1988) Pattern of nucleotide substitution at major histocompatibility complex class I loci reveals overdominant selection. Nature 335: 167–170.
74. ApaniusV, PennD, SlevPR, RuffLR, PottsWK (1997) The nature of selection on the major histocompatibility complex. Crit Rev Immunol 17: 179–224.
75. HughesAL, YeagerM (1998) Natural selection at major histocompatibility complex loci of vertebrates. Annu Rev Genet 32: 415–435.
76. HodgkinsonA, Eyre-WalkerA (2010) The genomic distribution and local context of coincident SNPs in human and chimpanzee. Genome Biol Evol 2: 547–557.
77. LefflerEM, ZiyueG, PfeiferS, SegurelL, AutonA, et al. (2013) Multiple instances of ancient balancing selection shared between humans and chimpanzees. Science 339: 1578–1582.
78. MaruyamaT (1974) The age of a rare mutant gene in a large population. Am J Hum Genet 26: 669–673.
79. KiezunA, PulitSL, FrancioliLC, van DijkF, SwertzM, et al. (2013) Deleterious alleles in the human genome are on average younger than neutral alleles of the same frequency. PLoS Genet 9: e1003301.
80. HillWG, RobertsonA (1966) The effect of linkage on limits to artificial selection. Genet Res 8: 269–294.
81. KarlinS, McGregorJ (1968) Rates and probabilities of fixation for two locus random mating finite populations without selection. Genetics 58: 141–159.
82. StrobeckC, MorganK (1978) The effect of intragenic recombination on the number of alleles in a finite population. Genetics 88: 829–844.
83. GriffithsRC (1981) Neutral two-locus multiple allele models with recombination. Theor Popul Biol 19: 169–186.
84. RannalaB, ReeveJP (2001) High-resolution multipoint linkage-disequilibrium mapping in the context of a human genome sequence. Am J Hum Genet 69: 159–178.
85. LarribeF, LessardS, SchorkNJ (2002) Gene mapping via the ancestral recombination graph. Theor Popul Biol 62: 215–229.
86. ZollnerS, PritchardJK (2005) Coalescent-based association mapping and fine mapping of complex trait loci. Genetics 169: 1071–1092.
87. WuY (2008) Association mapping of complex diseases with ancestral recombination graphs: models and efficient algorithms. J Comput Biol 15: 667–684.
88. BesenbacherS, MailundT, SchierupMH (2009) Local phylogeny mapping of quantitative traits: higher accuracy and better ranking than single-marker association in genomewide scans. Genetics 181: 747–753.
89. Prado-MartinezJ, SudmantPH, KiddJM, LiH, KelleyJL, et al. (2013) Great ape genetic diversity and population history. Nature 499: 471–475.
90. ThanC, NakhlehL (2009) Species tree inference by minimizing deep coalescences. PLoS Comput Biol 5: e1000501.
91. YuY, BarnettRM, NakhlehL (2013) Parsimonious inference of hybridization in the presence of incomplete lineage sorting. Syst Biol 62: 738–751.
92. GronauI, HubiszMJ, GulkoB, DankoCG, SiepelA (2011) Bayesian inference of ancient human demography from individual genome sequences. Nature Genetics 43: 1031–1034.
93. TangH, CoramM, WangP, ZhuX, RischN (2006) Reconstructing genetic ancestry blocks in admixed individuals. Am J Hum Genet 79: 1–12.
94. SankararamanS, SridharS, KimmelG, HalperinE (2008) Estimating local ancestry in admixed populations. Am J Hum Genet 82: 290–303.
95. ScheetP, StephensM (2006) A fast and flexible statistical model for large-scale population genotype data: applications to inferring missing genotypes and haplotypic phase. Am J Hum Genet 78: 629–644.
96. BrowningSR, BrowningBL (2007) Rapid and accurate haplotype phasing and missing-data inference for whole-genome association studies by use of localized haplotype clustering. Am J Hum Genet 81: 1084–1097.
97. McVeanGA, MyersSR, HuntS, DeloukasP, BentleyDR, et al. (2004) The fine-scale structure of recombination rate variation in the human genome. Science 304: 581–584.
98. HobolthA, JensenJL (2014) Markovian approximation to the finite loci coalescent with recombination along multiple sequences. Theor Popul Biol 2014: S0040–5809 doi:10.1016/j.tpb.2014.01.002
99. WuY, GusfieldD (2007) Efficient computation of minimum recombination with genotypes (not haplotypes). Journal of Bioinformatics and Computational Biology 181–200.
100. TavareS (1984) Line-of-descent and genealogical processes, and their applications in population genetics models. Theor Popul Biol 26: 119–164.
101. Siepel A, Haussler D (2005) Phylogenetic hidden Markov models. In: Nielsen R, editor, Statistical Methods in Molecular Evolution, New York: Springer. pp. 325–351.
102. RabinerLR (1989) A tutorial on hidden Markov models and selected applications in speech recognition. Proceedings of the IEEE 77: 257–286.
103. Durbin R, Eddy S, Krogh A, Mitchison G (1998) Biological Sequence Analysis: Probabilistic Models of Proteins and Nucleic Acids. Cambridge, UK: Cambridge University Press.
104. CawleySL, PachterL (2003) HMM sampling and applications to gene finding and alternative splicing. Bioinformatics 19 Suppl 2: II36–II41.
105. ZhuJ, LiuJS, LawrenceCE (1998) Bayesian adaptive sequence alignment algorithms. Bioinformatics 14: 25–39.
106. International HapMap Consortium (2007) FrazerKA, BallingerDG, CoxDR, HindsDA, et al. (2007) A second generation human haplotype map of over 3.1 million snps. Nature 449: 851–861.
107. GronauI, ArbizaL, MohammedJ, SiepelA (2013) Inference of natural selection from interspersed genomic elements based on polymorphism and divergence. Mol Biol Evol 30: 1159–1171.
108. RobinsonDF, FouldsLR (1981) Comparison of phylogenetic trees. Mathematical Biosciences 53: 131–147.
109. ArbizaL, GronauI, AksoyBA, HubiszMJ, GulkoB, et al. (2013) Genome-wide inference of natural selection on human transcription factor binding sites. Nat Genet 45: 723–729.
Štítky
Genetika Reprodukčná medicínaČlánok vyšiel v časopise
PLOS Genetics
2014 Číslo 5
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