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Stepwise haplotype analysis: Are LD patterns repeatable?
Human Genomics volume 2, Article number: 376 (2006)
Abstract
A variety of techniques exist to describe and depict patterns of pairwise linkage disequilibrium (LD). In the current paper, a new log-linear framework is proposed for the summarisation of local interactions among single nucleotide polymorphisms (SNPs). Our approach provides a straightforward means of capturing the diversity of higher-order LD relationships for small numbers of loci by investigating inter-marker interactions. Our method was applied to a dataset of 76 SNP markers spanning a genomic interval of length 2.8 megabases. The analysis of three short sub-regions is described in detail here. Model and graphical representations of contiguous markers in medium to high LD are presented. In the regions studied, evidence for sub-structure was detected, supporting the view that the genomic reality is complex. Interestingly, a critical evaluation of the method by bootstrapping showed that while some LD relationships were captured in a highly repeatable fashion, the majority were not. Large numbers of small interactions, both direct and indirect, mean that many models can adequately summarise the data at hand. Our results suggest that repeatability should be further investigated in the application of LD-based approaches.
Introduction
The abundance of single nucleotide polymorphisms (SNPs) and the limited power, in some situations, of single-locus analysis has led to increased use of haplotype-inference methods such as Clark's algorithm, [1] the Expectation-Maximisation (EM) algorithm [2] and iterative-sampling algorithms to resolve phase ambiguity by both coalescent and non-coalescent models [3, 4].
Recent studies [5–9] have shown that the human genome can be viewed in terms of haplotype blocks, given by discrete regions of high linkage disequilibrium (LD), and separated by shorter regions of low LD. Haplotype block identification has been conducted via evaluation of measures of LD, such as Lewontin's D', as well as by methods of directly assessing evidence of recombination [10]. The corollary of the block concept was that a small proportion of the SNPs, the 'haplotype -tagging' SNPs, should be sufficient to capture the majority of the haplotype structure contained in blocks genome-wide [11]. More recently, Bayesian graphical modeling has been applied to describe more complex patterns of relationship, for example among loci that are proximal but non-adjacent [12].
We introduce a novel application of log-linear modelling, to describe higher-order interactions among SNPs. The log-linear step is embedded within the EM algorithm in order correctly to model phase. Previously, log-linear models have been used to form the basis of Bayesian priors in resolving phase and to model different levels of LD with known phase [13, 14]. We show that the log-linear model may be used to describe discrete islands of LD, [15] as well as smaller conditionally independent sub-fragments of high LD. We test the repeatability of our findings by bootstrapping and find instances of complex LD for which model repeatability is low.
Materials and methods
The methods described below were applied to a dataset consisting of a random sample of 150 Caucasian controls from the Prevention of REStenosis with Tranilast and its Outcomes (PRESTO) study [16, 17]. Appropriate consent was obtained and these samples were genotyped across 76 SNPs spanning approximately 2.8 megabases (Mb), within and around the UGT1A1 gene. These data and their analyses are described in detail elsewhere [18].
EM log-linear approach
Our method takes as its basis the EM algorithm [2]. In summary, log-linear modelling is used in the E-step to update haplotype frequencies, while the likelihood of the data, given the model, is maximised in the M-step. The process proceeds iteratively.
More formally, [3] given a sample of n diploid individuals from a population, let G = (G 1 , ..., G n ) denote the known genotypes, let H = (H 1 , ..., H n ) denote the unknown corresponding haplotype pairs and let F = (F 1 , ..., F m ) be the unknown population haplotype frequencies. The algorithm starts under random assignment of genotypes. The M-step of the EM algorithm then finds the set of haplotype frequencies, F, which maximises the following likelihood:
Under Hardy-Weinberg equilibrium, the genotype probabilities can be partitioned into the product of haplotype probabilities:
where Ω i is the set of all (ordered) haplotype pairs consistent with the multilocus genotype G i .
The E-step of the algorithm, used here, then estimates the population haplotype frequencies F by using the log-linear model and not the traditional counting method. Investigation of the saturated log-linear model, however, in which all loci and interactions are represented, is challenging due to the necessarily high number of parameters. Therefore, a stepwise approach of fitting intermediate models has been used. These intermediate models contain more parameters than a model of complete linkage equilibrium (LE) but fewer parameters than the saturated model [19, 20]. In the current paper, we show how such models provide the framework for quantifying the patterns of LD.
Notation
Notation for the remainder of the paper will focus on the composition of the log-linear model, as it is this that is of interest in describing patterns of SNP interaction. The variable corresponding to the ith SNP is given by l i and models are specified by using the Wilkinson and Rogers notation, where the SNP variables are combined by '+' to denote independence, and '*' to denote interaction [21]. For example, l 1 +l 2 denotes independence between the first and second SNP and l 3 * l 4 denotes interaction between the 3rd and 4th.
Forward stepwise algorithm
We propose a forward stepwise approach to determining a parsimonious model of LD. Starting with a model of complete LE, higher-order LD terms are added sequentially to the model until a parsimonious model is found. This procedure has been implemented as the command swblock within STATA [22] and is available using the ssc command. A likelihood ratio test (LRT) was used to measure the strength of LD or inter-SNP interaction, although other test statistics are possible. The LRT was performed using hapipf, a command [20] implemented in STATA [22].
More formally, the algorithm examines a region of n SNPs. In order to preserve efficiency of the EM algorithm, fewer than ten SNPs is practical. The first step is to estimate the log-likelihood under the base model of LE l1 + l2 + ... + ln. Then, every pairwise SNP interaction term is added to this model and the LRT, comparing the new model with the base model is re-evaluated. The most significant interaction term is then added to the base model, this becomes the new base model and the process repeats. A nominal p-value of 0.05 was initially chosen to compare new models with the base model; however, other thresholds of p = 0.01 and p = 0.001 were also investigated. Once no more pairwise interactions are significant, the algorithm proceeds to the next order of interaction terms, and so on. This approach accommodates the fact that pairwise interactions can occur over greater distances than contiguous pairs and that LD does not decay monotonically with distance. At each step, the number of degrees of freedom is minimised in the sequence of LRTs, and the algorithm continues until the highest interaction term is evaluated.
Application to LD structure
Certain LD features have been helpfully described in a review by Wall and Pritchard, [23] who established three criteria, derived using pairwise LD, for assessing haplotype blocks. They introduced concepts of 'holes' and 'overlapping blocks' in regions of high LD, and these concepts are applicable to more general evaluations of complex LD structure. As described below, these concepts can be presented in terms of log-linear models.
Holes arise when the outermost SNPs are not in strong LD with an SNP or multiple SNPs that lie in between. To translate this to a log-linear framework, consider a triplet of markers parameterised as l l , l 2 and l 3 . If l 1 and l 3 show high LD, but intervening pairs (l 1 , l 2 and l 2 , l 3 ) do not show high LD, as can happen with low frequency SNPs, then this situation may be described by the model l 1 *l 3 +l 2 .
This representation can be extended to a fourth SNP, l 4 , in a similar fashion. Continuing the example of a hole at SNP2 (variable l 2 ), one model describing the interactions would be l 1 *l 3 *l 4 +l 2 . Alternatively, if the three-way interaction is not needed, then another suitable model might be l 1 *l 3 +l 3 *l 4 +l 1 *l 4 +l 2 , where, again, SNP2 (l 2 ) is independent of the other three SNPs.
Also defined by Wall and Pritchard, [23] another feature of certain regions is the presence of SNPs that are assignable to more than one region of high LD. In the simplest case of four SNPs (l 1 -l 4 ), two overlapping sets of relationships might be specified as l 1 *l 2 *l 3 +l 2 *l 3 *l 4 . In this model, SNP1 and SNP4 are conditionally independent, given SNP2 and SNP3. In reality, there may be a combination of holes and overlapping regions. The method may be easily generalised.
Investigating the repeatability of derived models
Regression approaches are better suited to hypothesis generation than to inference, due to the large number of models evaluated, but repeatability is of importance when assessing the utility of these methods. Data from 150 controls were available for study. To investigate the repeatability of our models, this control set was subjected to bootstrapping. In other words, the following process was carried out 12 times: 150 samples were selected with replacement from the entire control set and model fitting applied. In this way, 12 models were derived for each genomic interval.
In the first round of analysis, a threshold of p = 0.05 was used in the stepwise regression to select parameters for inclusion in the model. Acknowledging that this threshold may be considered generous in the context of the large number of tests being applied, the whole analysis was repeated using thresholds of p = 0.01 and p = 0.001. Again, model repeatability was assessed.
Results
All pairwise R2 statistics for the 76 SNPs were produced using STATA [22] and the pwld command (available from http://www-gene.cimr.cam.ac.uk/clayton). Figure 1 displays estimates of all of the pairwise statistics. The diagonal cells are shown as white, as the program does not calculate R2 values for these. Elsewhere, increasingly high R2 is denoted by increasingly dark grey shading. A few areas had very high R2 values, given by the black squares. Three regions were selected for model fitting. They were chosen by eye, based upon Figure 1, as having different characteristics, and while they do not provide a comprehensive evaluation of the region, they provide an interesting insight into the question of repeatability. The three are boxed in Figure 1, and resultant models are shown graphically in Figures 2, 3, 4, 5. These subsequent graphs were constructed using the command gipf within STATA, installed using the command ssc. In these graphs, each node represents a SNP and an edge represents a significant pairwise relationship. Three-way relationships are given by solid bold lines and four-way interactions are given by broken bold lines.
Forward stepwise analysis of SNP1-SNP5
For the group SNP1-SNP5, the LD plot (Figure 1) suggested a simple pattern of uniformly high LD. When model fitting was applied, however, more complex models were derived. Figure 2 shows 12 graphs that represent the series of models derived from bootstrapping. Some features, such as the l 2 *l 3 and l 1 *l 4 pairwise relationships, were captured in every model; however, relationships among SNPs 3-5 were captured in three different ways. The variability of these 12 simple graphs and of the models they denote is interesting, given the apparently uniform 'block' of LD seen in Figure 1. This may, however, be attributed to the fact that a small percentage of overall variability can be explained in a number of ways. Importantly, the overall conclusion from this regional analysis -- that all markers are strongly inter-related -- is not affected by the nuances in the models selected. When the threshold for parameter inclusion in stepwise model fitting was decreased from p = 0.05 to p = 0.01 and p = 0.001 (results not shown), the models derived were almost identical. The only change was the loss of the l 4 *l 5 parameter in two of the bootstrap samples at p = 0.01, and from three of the samples at p = 0.001.
Forward stepwise analysis of SNP36-SNP41
This group of markers was selected because they mark the join between two apparent regions of high LD (Figure 1). The models derived from this more complex region are shown in Figure 3. In this more complex example, model repeatability was lower. The strong block-like relationship among markers SNP38 - SNP41 was clearly visible as a tangle of graphical relationships in each bootstrap sample, but the exact positioning of edges tended to vary. Lowering the threshold for parameter inclusion from p = 0.05 to p = 0.01 led to the loss of edges in every bootstrap sample (Figure 4). At this lower threshold, the two regions of high LD (SNP36 -SNP37 and SNP38 -SNP41) became more visibly distinct. Few model changes were observed as the threshold was lowered from p = 0.01 to p = 0.001 (results not shown).
Forward stepwise analysis of SNP44-SNP49
Lastly, for SNP44 - SNP49, the LD plot (Figure 1) suggests a complex set of interrelationships. The parsimonious models for the 12 bootstrap samples are given in Figure 5. The large number of edges suggests that this is an area of high haplotype diversity and this interval provides the most striking example of lack of repeatability in model fitting. Only two features were captured in all models. These were a three-way interaction (SNP46, SNP47, SNP48) and a two-way interaction (SNP44, SNP45). Other features were variously described. This is a clear example where overall variability of relationship can be explained in a model in a number of ways.
Discussion
This study investigated the performance of stepwise log-linear modelling in the evaluation of LD in three genomic loci. Bootstrapping of the data demonstrated that although certain LD features were consistently captured by this approach, derived models were generally not repeatable. Furthermore, altering the significance threshold for inclusion of parameters in the stepwise analysis did not materially change our models. It is noteworthy that sample size may be a consideration. Repeating the bootstrap analyses with a smaller sample size (n = 75) led to models with a greater number of higher-order interactions (results not shown). With a sample size of n = 150, these same relationships tended to manifest as two-way interactions in the model. Clearly, the allele frequency distribution of the markers available must be a major component of the patterns derived, and while it is not appropriate to extrapolate our findings to all genomic regions and/or all methodologies, these findings do raise interesting questions of repeatability. LD-based inference is widely used, both for exploratory analysis and for the efficient selection of markers for genotyping.
Model complexity and/or lack of repeatability should come as no real surprise. LD mapping exploits historical recombination events to narrow candidate regions for disease genes; however, the pattern of LD is also influenced by mutation and other stochastic factors which create associations between markers that do not have a simple relationship with distance. Our models shed no light on the 'source' of any complexity; they merely support its existence. Greater repeatability of inferred LD has been observed at comparatively low resolution, when a close relationship is maintained between recombination and LD patterns [6]. Our models reflect the more stochastic picture seen at comparatively high resolution.
Other investigators have presented methods of modelling non-adjacent SNP interactions. Thomas and Camp [12] derived Bayesian graphical models using a tailored Metropolis - Hastings approach. Earlier evaluations of partial LD models have also been made. One group commented on the exceeding complication arising from the inclusion of higher-order interactions [24]. Model complexity is indeed an outcome of applying this method to a large genomic region. In terms of applicability, our approach is limited to a relatively small number of SNPs -- fewer than ten -- and thus it is restricted to small genomic regions. For most current-day situations, it would be impractical to apply stepwise log-linear modelling for the purposes of tag selection. The great wealth of marker data available now from the HapMap and other sources, combined with the ever-decreasing cost of genotyping, make it an unlikely avenue to pursue. For small candidate gene studies, however, it would be possible to use a log-linear approach to identify 'sensible' models to test in the analysis of a subsequent replication study, thereby reducing the burden of multiple testing. Such models would include an additional parameter pertaining to the disease locus but would be derived in exactly the same way. It is hoped that the visual immediacy of this approach will aid hypothesis generation and serve as a useful addition to a fine-mapping tool kit that already includes coalescent modelling, [25] for example.
It is now generally agreed that the genome is not simply composed of discrete haplotype blocks of uniformly high LD; indeed, our models support a more complex reality. Nevertheless, LD has an important role to play in designing efficient marker sets for genetic study. Resources such as the HapMap lessen the need for marker validation and provide a means of allowing the selection of informative markers for genotyping. Our bootstrap results show that LD-based inference can be sample dependent, even within an ethnic group. Therefore, in utilising such data, it may be beneficial to investigate the repeatability of one's chosen methodology and, if appropriate, to allow greater redundancy in marker selection.
References
Clark AG: Inference of haplotypes from PCR-amplified samples of diploid populations. Mol Biol Evol. 1990, 7: 111-122.
Excoffier L, Slatkin M: Maximum-likelihood estimation of molecular haplotype frequencies in a diploid population. Mol Biol Evol. 1995, 12: 921-927.
Stephens M, Smith NJ, Donnelly P: A new statistical method for haplotype reconstruction from population data. Am J Hum Genet. 2001, 68: 978-989. 10.1086/319501.
Niu T, Qin ZS, Xu X, et al: Bayesian haplotype inference for multiple linked single-nucleotide polymorphisms. Am J Hum Genet. 2002, 70: 157-169. 10.1086/338446.
Daly MJ, Rioux JD, Schaffner SF, et al: High-resolution haplotype structure in the human genome. Nat Genet. 2001, 29: 229-232. 10.1038/ng1001-229.
Jeffreys AJ, Kauppi L, Neumann R: Intensely punctuate meiotic recombination in the class II region of the major histocompatibility complex. Nat Genet. 2001, 29: 217-222. 10.1038/ng1001-217.
Patil N, Berno AJ, Hinds DA, et al: Blocks of limited haplotype diversity revealed by high resolution scanning of human chromosome 21. Science. 2001, 294: 1719-1723. 10.1126/science.1065573.
Gabriel SB, Schaffner SF, Nguyen H, et al: The structure of haplotype blocks in the human genome. Science. 2002, 296: 2225-2229. 10.1126/science.1069424.
Twells RCJ, Mein CA, Phillips MS, et al: Haplotype structure, LD blocks, and uneven recombination within the LRP5 gene. Genome Res. 2003, 13: 845-855. 10.1101/gr.563703.
Schwartz R, Halldorsson BV, Bafna V, et al: Robustness of inference of haploype block structure. J Comp Biol. 2003, 10: 13-19. 10.1089/106652703763255642.
Johnson GCL, Esposito L, Barratt BJ, et al: Haplotype tagging for the identification of common disease genes. Nat Genet. 2001, 29: 233-237. 10.1038/ng1001-233.
Thomas A, Camp NJ: Graphical modeling of the joint distribution of alleles at associated loci. Am J Hum Genet. 2004, 74: 1088-1101. 10.1086/421249.
Morris A, Pedder A, Ayres K: Linkage disequilibrium assessment via log-linear modeling of SNP haplotype frequencies. Genet Epidemiol. 2003, 25: 106-114. 10.1002/gepi.10254.
Huttley GA, Wilson SR: Testing for concordant equilibria between population samples. Genetics. 2000, 156: 2127-2135.
Goldstein DB: Islands of linkage disequilibrium. Nat Genet. 2001, 29: 109-111. 10.1038/ng1001-109.
Holmes D, Fitzgerald P, Goldberg S, et al: The PRESTO (Prevention of restenosis with tranilast and its outcomes) protocol: A double-blind, placebo-controlled trial. Am Heart J. 2000, 139: 23-31.
Danoff TM, Campbell DA, McCarthy LC, et al: A Gilbert's syndrome UGT1A1 variant confers susceptibility to tranilast-induced hyperbilirubinemia. Pharmacogenomics J. 2004, 4: 49-53. 10.1038/sj.tpj.6500221.
Xu CF, Lewis KF, Yeo AJ, et al: Identification of pharmacogenetic effect by linkage disequilibrium mapping. Pharmacogenomics J. 2004, 4: 374-378. 10.1038/sj.tpj.6500268.
Chiano MN, Clayton DG: Fine genetic mapping using haplotype analysis and the missing data problem. Ann Hum Genet. 1998, 62: 55-60.
Mander AP: Haplotype analysis in population-based association studies. Stata Journal. 2001, 1: 58-75.
Wilkinson G, Rogers C: Symbolic description of factorial models for analysis of variance. Appl Stat. 1973, 22: 392-399. 10.2307/2346786.
StataCorp: Stata Statistical Software: Release 70. 2001, StataCorp LP, College Station TX
Wall JD, Pritchard JK: Assessing the performance of the haplotype block model of linkage disequilibrium. Am J Hum Genet. 2003, 73: 502-515. 10.1086/378099.
McPeek MS, Strahs A: Assessment of linkage disequilibrium by the decay of haplotype sharing, with application to fine-scale genetic mapping. Am J Hum Genet. 1999, 65: 858-875. 10.1086/302537.
Morris AP, Whittaker JC, Balding DJ: Fine-scale mapping of disease loci via shattered coalescent modelling of genealogies. Am J Hum Genet. 2002, 70: 686-707. 10.1086/339271.
Acknowledgements
The authors would like to thank members of the Statistics and Programming Department, and members of the Discovery and Pipeline Genetics Department at GlaxoSmithKline, for helpful discussions and input, particularly Karen Lewis and Chun-Fang Xu, for sharing the data described here.
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Mander, A.P., Bansal, A. Stepwise haplotype analysis: Are LD patterns repeatable?. Hum Genomics 2, 376 (2006). https://doi.org/10.1186/1479-7364-2-6-376
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DOI: https://doi.org/10.1186/1479-7364-2-6-376