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. 2018 Mar 25;11(8):1257–1269. doi: 10.1111/eva.12621

Hurdles in the evolutionary epidemiology of Angiostrongylus cantonensis: Pseudogenes, incongruence between taxonomy and DNA sequence variants, and cryptic lineages

Sirilak Dusitsittipon 1,2,, Charles D Criscione 3,†,, Serge Morand 4, Chalit Komalamisra 5, Urusa Thaenkham 1,†,
PMCID: PMC6099809  PMID: 30151038

Abstract

Angiostrongylus cantonensis, the rat lungworm, is a zoonotic pathogen that is one of the leading causes of eosinophilic meningitis worldwide. This parasite is regarded as an emerging pathogen with a global range expansion out of southeastern Asia post‐WWII. To date, molecular systematic/phylogeographic studies on A. cantonensis have mainly used two mitochondrial (mtDNA) markers, cytochrome c oxidase 1 (CO1) and cytochrome b (CYTB), where the focus has largely been descriptive in terms of reporting local patterns of haplotype variants. In order to look for more global evolutionary patterns, we herein provide a collective phylogenetic assessment using the six available whole mtDNA genome samples that have been tagged as A. cantonensis, A. malaysiensis, or A. mackerrasae along with all other GenBank CO1 and CYTB partial sequences that carry these species identifiers. The results reveal three important complications that researchers will need to be aware of, or will need to resolve, prior to conducting future molecular evolutionary studies on A. cantonensis. These three problems are (i) incongruence between taxonomic identifications and mtDNA variants (haplotypes or whole mtDNA genome samples), (ii) the presence of a CYTB mtDNA pseudogene, and (iii) the need to verify A. mackerrasae as a species along with other possible cryptic lineages, of which there is suggestive evidence (i.e., A. cantonensis could be a species complex). We provided a discussion of how these complications are hurdles to our understanding of the global epidemiology of angiostrongyliasis. We call for future studies to be more explicit in morphological traits used for identifications (e.g., provide measurements). Moreover, it will be necessary to repeat prior morphological and life‐history studies while simultaneously using sequence data in order to assess possible associations between critical epidemiological data (e.g., biogeography, virulence/pathology, host species use) and specific lineages.

Keywords: Angiostrongylus cantonensis, Angiostrongylus mackerrasae, Angiostrongylus malaysiensis, cryptic lineages, cytochrome b (CYTB) gene, cytochrome c oxidase 1 (CO1) gene, pseudogene, species complex

1. INTRODUCTION

Angiostrongylus cantonensis, the rat lungworm, is a zoonotic pathogen that is one of the leading causes of eosinophilic meningitis worldwide (Barratt et al., 2016). This parasite is regarded as an emerging pathogen with a global range expansion out of southeastern Asia post‐WWII (Kliks & Palumbo, 1992; Wang, Lai, Zhu, Chen, & Lun, 2008). Despite cases of human infection in many of the areas where A. cantonensis has expanded its range (Wang et al., 2008), there has been little attempt to use molecular evolutionary methods to elucidate the global epidemiology of this important pathogen. Indeed, the use of DNA data only came about in the 2000s. For example, ribosomal DNA sequences were used to assess metastrongylid nematode relationships (Carreno & Nadler, 2003) or to help survey larvae from mollusk intermediate hosts (Fontanilla & Wade, 2008; Qvarnstrom, Sullivan, Bishop, Hollingsworth, & da Silva, 2007; Qvarnstrom et al., 2010), and ~360‐bp region of the cytochrome c oxidase 1 (CO1) gene was used to assess relationships to other species of Angiostrongylus (Eamsobhana et al., 2010). To date, molecular systematic/phylogeographic studies on A. cantonensis have mainly used two mitochondrial (mtDNA) markers, CO1 and cytochrome b (CYTB), where the focus has largely been descriptive in terms of reporting local patterns of haplotype variants (Aghazadeh et al., 2015; Dalton, Fenton, Cleveland, Elsmo, & Yabsley, 2017; Dusitsittipon, Criscione, Morand, Komalamisra, & Thaenkham, 2017; Dusitsittipon, Thaenkham, Watthanakulpanich, Adisakwattana, & Komalamisra, 2015; Eamsobhana, Song, et al., 2017; Eamsobhana, Yong, et al., 2017; Lv et al., 2012; Monte et al., 2012; Moreira et al., 2013; Nakaya et al., 2013; Okano et al., 2014; Rodpai et al., 2016; Simoes et al., 2011; Tokiwa et al., 2012, 2013; Vitta et al., 2016; Yong, Eamsobhana, Song, Prasartvit, & Lim, 2015; Yong, Song, Eamsobhana, Goh, & Lim, 2015; Yong, Song, Eamsobhana, & Lim, 2016).

Comparisons among molecular systematic studies on A. cantonensis would be useful to look for evolutionary patterns that could aid in epidemiological inference (e.g., biogeographic patterns and sources of introductions, host‐associated or disease‐associated lineages). Unfortunately, because studies did not concurrently use the CO1 and CYTB markers, such comparisons are difficult to make. However, the availability of recent whole mitochondrial genome sequences of A. cantonensis, A. malaysiensis, and A. mackerrasae provides a chance to “anchor” CO1 and CYTB clades because the mtDNA does not generally recombine (Ballard & Whitlock, 2004).

In order to look for more global evolutionary patterns, we herein provide a collective phylogenetic assessment using the six available whole mtDNA genome samples that have been tagged as A. cantonensis, A. malaysiensis, or A. mackerrasae along with all other GenBank CO1 and CYTB partial sequences that carry these species identifiers. Our study focuses on these three species due to their morphological and life‐history similarities (Spratt, 2015; details given in the Discussion). Our results reveal three important complications that researchers will need to be aware of, or will need to resolve, prior to conducting future molecular evolutionary studies on A. cantonensis. These three problems are (i) incongruence between taxonomic identifications and mtDNA variants (haplotypes or whole mtDNA genome samples), (ii) the presence of a CYTB mtDNA pseudogene, and (iii) the need to verify A. mackerrasae as a species along with other possible cryptic lineages, of which there is suggestive evidence (i.e., A. cantonensis could be a species complex). We provided a discussion of how these complications are hurdles to our understanding of the global epidemiology of angiostrongyliasis. We call for future studies to be more explicit in morphological traits used for identifications (e.g., provide measurements). Moreover, it will be necessary to repeat prior morphological and life‐history studies while simultaneously using sequence data in order to assess possible associations between critical epidemiological data (e.g., biogeography, virulence/pathology, host species use) and specific lineages.

2. MATERIALS AND METHODS

2.1. Assembly of CYTB and CO1 datasets

Available in GenBank, there are five mitochondrial genomes identified as either A. cantonensis (NC_013065 = GQ398121, Lv et al., 2012; AP017672, BioProject: PRJEB493; KT186242, Yong, Song, et al., 2015; KT947978, Yong et al., 2016) or A. malaysiensis (KT947979 = NC_030332; Yong et al., 2016). A whole mtDNA genome identified as A. mackerrasae was discussed in Aghazadeh et al. (2015), but where the actual sequence was obtained from the appendix of the thesis by Aghazadeh (2015). We refer to these six samples as the mtDNA genome reference samples. Sample information, for example, geographic location, and host species, of the six reference samples was obtained from the original publications or available information on GenBank and is included in Tables S1 and S2.

As prior studies on A. cantonensis do not include both CO1 and CYTB, a primary goal was to determine the correspondence between CO1 and CYTB clades that have been identified in prior work. Because the mtDNA does not generally recombine (Ballard & Whitlock, 2004), we used the CYTB and CO1 sequences from the above six mtDNA genome reference samples to anchor CYTB or CO1 haplotypes obtained from previous studies. From GenBank, we assembled all available CYTB or CO1 sequences that have been tagged as A. cantonensis, A. malaysiensis, or A. mackerrasae and that have associated publications. Tables S1 and S2 also contain the sample information for all these additional sequences obtained from GenBank. For outgroups, we used CYTB and CO1 sequences from the mtDNA genome samples of A. costaricensis (NC013067, AP017675, and KR827449) and A. vasorum (NC_018602).

Alignments were conducted with ClustalW in BioEdit (Hall, 1999) along with manual corrections made by eye. In aligning sequences, a haplotype from a particular study may have been subsumed (i.e., there was an identical match in the overlapping region) by a longer sequence from another study. In such cases, we only used the longer sequence in the phylogenetic analyses. The matching GenBank haplotypes are indicated in Tables S1 and S2.

The CYTB alignment consisted of approximately 852 nucleotides. Primers that amplify this region of CYTB are described in Dusitsittipon et al. (2017) (also, see below). Due to the presence of indels in a CYTB pseudogene (see Results), the CYTB alignment was based on amino acid translation (translation table 5, the invertebrate mtDNA code, on GenBank) of the mtDNA sequences. Subsequent nucleotide alignments (after back translation) were then kept in codon reading frame to facilitate downstream molecular evolution analyses. The CYTB dataset contained 38 unique in‐group haplotypes (including pseudogene haplotypes; see Results) and three outgroup sequences. Table S3 contains the CYTB alignment in fasta format.

Because many of the available CO1 sequences were short (e.g., ~300 bases), information with regard to the relationships among the six mtDNA genome reference samples would be lost if we trimmed the alignment to match the shortest sequence. As our primary interest was in assessing CO1 haplotype relationships with respect to the six mtDNA genome reference samples, the CO1 alignment retained the full‐length sequences of reference samples. The resulting gapped sites (i.e., sites that flank the overlapping region) in such an alignment are treated as missing data in a maximum‐likelihood phylogenetic analysis. We note that there were two CO1 sequences (MF000735 and MF000736) from Dalton et al. (2017) that did not overlap with the region of CO1 that has predominately been used in studies of A. cantonensis. As a result, the phylogenetic positions of the CO1 haplotypes of Dalton et al. (2017) should only be interpreted with respect to the six reference sequences and not the remaining CO1 haplotypes. The topology of the CO1 tree remains the same even if the sequences of Dalton et al. (2017) are excluded (results not shown). The CO1 dataset contained 41 unique in‐group haplotypes and four outgroup sequences. Table S4 contains the CO1 alignment in fasta format. Tables S1 and S2 contain information on the references from which CO1 or CYTB haplotypes originated as well as matching haplotypes, naming conventions, and sample identifiers used in the original papers.

2.2. Phylogenetic analyses

Phylogenetic analyses were conducted in MEGA6 software (Tamura, Stecher, Peterson, Filipski, & Kumar, 2013) after using the maximum‐likelihood model selection (with the “use all sites' option”) to determine the evolutionary substitution model. To confirm that both the CO1 and CYTB haplotypes from the six reference samples provided the same phylogenetic signal, we first conducted maximum‐likelihood analyses using the TN93 + G and HKY + G models, respectively. For heuristic purposes and to determine whether the two mtDNA markers provided similar information, we calculated pairwise p‐distance between the six reference samples and tested for a correlation between the CO1 and CYTB pairwise p‐distances using a Mantel test. For the complete CO1 and CYTB datasets, maximum‐likelihood analyses with the GTR + G and HKY + G models, respectively, were used for phylogenetic reconstruction. One thousand bootstraps were used to assess nodal support. In our prior study (Dusitsittipon et al., 2017), we found strong associations between nine nuclear microsatellite clusters and CYTB mtDNA clades. We follow the naming conventions of the clusters and clades identified in Dusitsittipon et al. (2017) to facilitate discussion in linking to CO1 clades.

In general, we linked CO1 and CYTB clades based on the phylogenetic positions of the reference samples. However, bootstrap support was expected to be low in the complete CO1 dataset because of the presence of many short sequences (e.g., ~300 bases). As a result, it is important to recognize that the positions of the short CO1 haplotypes are subject to change pending acquisition of new sequence data. Also, for the latter reason, we used a conservative approach where a link in the CO1 phylogeny was made only back to the node that contained the most recent common ancestor of a reference sequence unless a clade had >90% bootstrap support. There were two exceptions to this rule where we used the relative phylogenetic positions of clades; we consider these exceptions to be hypothesized clades (see Results).

2.3. Pseudogene analyses

In our prior study (Dusitsittipon et al., 2017), we described how the CYTB primer pairs Cytb‐F, 5′‐TGAATAGACAGAATTTTAAGAG‐3′ and Cytb‐R, 5′‐ATCAACTTAACATTACAGAAAC‐3′ of Dusitsittipon et al. (2015) would fail in some samples or produce sequences that translated with premature stop codons (henceforth referred to as untranslatable haplotypes). Upon the design of new primers Cytb‐F3 5′‐ATGTTATCTTGATAAGGTAGAG‐3′ and Cytb‐R2 5′‐AACCTAAATTCAATATACATACTAT‐3′ (see Dusitsittipon et al., 2017), we were able to obtain translatable sequences from specimens that previously failed or produced untranslatable haplotypes. Specimen sampling and sequencing protocols are explained in detail in Dusitsittipon et al. (2017). Here, we note that untranslatable haplotypes were obtained from 41 individuals (Table S1 gives the individual identifiers and locations of samples) using Cytb‐F and Cytb‐R. From 30 of these 41 individuals, we also obtained the real CYTB sequence using Cytb‐F3 and Cytb‐R2 (Table 1).

Table 1.

Samples from which both the pseudogene and CYTB gene were obtained (n = 30)

Sample ID Provinces Coordinates Pseudogene haplotype CYTB haplotype
BKK 6, 7
BKK 9 		Bangkok 13°45′0″N 100°31′1.20″E H22
H24 		H14
H14
LB 19–21 Lop Buri 14°51ʹ21ʺN 100°59ʹ24ʺE H24 H14
PCK 2, 5
PCK 7, 		Prachuap Khiri Khan 12°23ʹ42ʺN 99°55ʹ0ʺE H22
H22 		H13
H16
CTI 1, 2, 16 Chanthaburi 12°36′3″N 102°16′14″E H14 H14
CMI 3 Chiang Mai 18°47′43″N 98°59′55″E H22 H18
NWT 7
NWT 9 		Narathiwat 6°25′N 101°49′E H22
H25 		H16
H19
NKI 1–3, 6, 7
NKI 10 		Nong Khai 17°52′5″N 102°44′40″E H26
H26 		H19
H20
PNA 2, 4 Phang Nga 8°27′52″N 98°31′54″E H22 H14
RNG 1–5, 7 Ranong 9°57′43″N 98°38′20″E H24 H14
KKN 6 Khon Kaen 16°26′N 102°50′E H25 H19
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GenBank accession numbers are MG516589MG516592 for H22‐H25, respectively. Sample CMI 4 had H23 (Table S4), but we did not obtain the corresponding CYTB haplotype from this sample.

As pseudogenes are genes that have lost function, selection pressures, especially purifying, will be relaxed and the pseudogenes may accumulate indels resulting in frameshifts and possible premature stop codons. Also, substitution rates will become equal among codon positions; that is, the ratio of nonsynonymous to synonymous substitution rates (dN/dS = ω) will approach 1 (Bensasson, Zhang, Hartl, & Hewitt, 2001; Wertheim, Murrell, Smith, Kosakovsky Pond, & Scheffler, 2015). We used amino acid translated sequences to guide alignment between the CYTB of the six reference mtDNA samples and the untranslatable haplotypes, that is, candidate pseudogene haplotypes. Manual corrections to nucleotide alignments were made by eye. We inspected the alignment for indels that would cause frameshifts and premature stop codons.

We then tested for elevated ω and relaxed selection in the hypothesized pseudogene lineage. PAML v4.9d (Yang, 2007) via the PAMLX v1.3.1 GUI interface (Xu & Yang, 2013) was used to run codeml. The CYTB alignment file was the same as for the phylogenetic analysis above (Table S3). Gapped sites (i.e., ambiguous codons) are ignored in the analyses. A likelihood ratio test of branch models was used to determine whether there was elevated ω on the hypothesized pseudogene lineage. The null model (M0) of one ω ratio for all branches was compared to an alternative model of two ω ratios: one for the hypothesized pseudogene (foreground branches) and one for the remaining branches (background branches). Likelihood ratio tests 1 and 2 described in Zhang, Nielsen, and Yang (2005) were used to determine whether the elevated ω was due to relaxed selection as opposed to positive selection (e.g., see Pavlova et al., 2017). In both tests, branch‐site Model A is the alternative hypothesis. Branch‐site Model A model assumes four site classes: sites under purifying selection (0 < ω0 < 1); sites under neutrality (ω1 = 1); sites under positive selection ω2 > 1 in the foreground lineage but under purifying selection (0 < ω0 < 1) in background lineages; and sites under positive selection ω2 > 1 in the foreground lineage but under neutrality (ω1 = 1) in background lineages. Test 1 uses as a null the sites model M1a, which assumes two site classes for all branches: 0 < ω0 < 1 and ω1 = 1. Rejection of the null in Test 1 has good power to detect relaxed selection, but has a high false‐positive rate for positive selection (Zhang et al., 2005). Test 2 compares branch‐site Model A to a null where branch‐site Model A has ω2 = 1 in foreground branches. Test 2 has an appropriate type I error when testing for positive selection (Zhang et al., 2005). Thus, a significant Test 1 along with failure to reject in Test 2 would provide support for relaxed selection.

3. RESULTS

3.1. Phylogenetic analyses

CO1 and CYTB phylogenetic trees based on the six mtDNA genome reference samples were identical in topology (data not shown) and matched their relationships observed in the results based on the complete CO1 and CYTB datasets (Figures 1 and 2). There is a significant and very high correlation in CO1 and CYTB pairwise p‐distances of the six reference samples (= .99; < .001; Table 2). Thus, as would be expected if there was no recombination, the two mtDNA genes show the same phylogenetic signal and are appropriate to use as anchors for the CYTB and CO1 haplotypes observed in previous studies.

Figure 1.

Figure 1

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Maximum‐likelihood phylogenetic tree of the complete mtDNA CYTB dataset (Tables S1 and S3). The six reference mtDNA samples are indicated by circles. Clade I is anchored by three reference mtDNA samples originally identified as Angiostrongylus cantonensis (NC_013065, AP017672, and KT947978) and the sample identified as A. mackerrasae. Clade I is referred to as A. cantonensis (see main text for justification). Clade II is anchored by KT947979 (originally identified as A. malaysiensis; Yong et al., 2016) and KT186242 (originally identified as A. cantonensis, Yong, Song, et al., 2015). Clade II is referred to as A. malaysiensis (see main text for justification). Clade III represents a CYTB pseudogene lineage within specimens that fall in Clade II. Outgroups include A. vasorum (NC_018602), and A. costaricensis (NC_013067, and AP017675). Subclade designations (discussed in main text) that link the CYTB clades to CO1 clades are denoted by different colors. Numbers at nodes indicated bootstrap support (only nodes with >50% support or that are of particular interest are shown)

Figure 2.

Figure 2

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Maximum‐likelihood phylogenetic tree of the complete mtDNA CO1 dataset (Tables S2 and S4). The six reference mtDNA samples are indicated by circles. Clade I is anchored by three reference mtDNA samples originally identified as Angiostrongylus cantonensis (NC_013065, AP017672, and KT947978) and the sample identified as A. mackerrasae. Clade I is referred to as A. cantonensis (see main text for justification). Clade II is anchored by KT947979 (originally identified as A. malaysiensis; Yong et al., 2016) and KT186242 (originally identified as A. cantonensis, Yong, Song, et al., 2015). Clade II is referred to as A. malaysiensis (see main text for justification). Outgroups include A. vasorum (NC_018602 and NC_013067) and A. costaricensis (AP017675 and KR827449). Subclade designations (discussed in main text) that link the CO1 clades to CYTB clades are denoted by different colors. Numbers at nodes indicated bootstrap support (only nodes with >50% support or that are of particular interest are shown)

Table 2.

Pairwise p‐distance between the six mtDNA reference samples. CO1 is above the diagonal and CYTB is below

AP017672 Aghazadeh KT947978 NC013065 KT947979 KT186242
AP017672 0.009 0.018 0.041 0.090 0.090
Aghazadeh 0.006 0.019 0.041 0.090 0.090
KT947978 0.014 0.014 0.038 0.091 0.091
NC013065 0.036 0.038 0.036 0.086 0.086
KT947979 0.110 0.108 0.109 0.117 0.001
KT186242 0.112 0.110 0.111 0.119 0.002
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At the broadest level, two divergent clades are observed in the both the CO1 and CYTB datasets (Figures 1 and 2). Clade I is anchored by three reference mtDNA samples originally identified as A. cantonensis (NC_013065, AP017672, and KT947978) and the sample identified as A. mackerrasae, which is very closely related to AP017672. Clade II is anchored by KT947979 (originally identified as A. malaysiensis; Yong et al., 2016) and KT186242 (originally identified as A. cantonensis, Yong, Song, et al., 2015). A third clade, Clade III, was also identified in the CYTB dataset. Evidence is provided below that shows Clade III represents a CYTB pseudogene lineage within specimens that fall in Clade II.

Comparing the CO1 and CYTB phylogenetic trees, the reference samples enabled the linking of four subclades and relative phylogenetic positions provided hypothesized links between two additional subclades. Within Clade I, Subclade I.1 is anchored by the reference KT947978 (=CYTB Haplotype 6 of Dusitsittipon et al., 2017; red clade in Figures 1 and 2). Subclade I.2 was anchored by both AP017672 and the mtDNA genome sample of A. mackerrasae (orange clade in Figures 1 and 2). The reference NC_013065 linked Subclade I.4 (pink clade in Figures 1 and 2). Subclades I.3 and I.5 (aqua and black clades, respectively, in Figures 1 and 2) are the hypothesized clades based on relative phylogenetic positions; however, additional reference samples (i.e., samples from which both CO1 and CYTB have been obtained) are needed to verify these links. Within Clade II, the Subclade II.1 (light green clade in Figures 1 and 2) is anchored by the reference samples KT186242 and KT947979 (=CYTB Haplotype 14 of Dusitsittipon et al., 2017).

Generally, the subclade designations have strong bootstrap support (>90%) in the CYTB phylogeny (Figure 1). In contrast, bootstrap support for subclades is often low in the CO1 phylogeny (Figure 2) because many haplotypes are short (e.g., <500 nucleotides). As a result of our conservative approach, several CO1 haplotypes that were sister to Subclades I.1 or I.2 were not included in these subclades (Figure 2). Likewise, no additional linking was made in Clade II due to a lack of additional reference sequences and the low phylogenetic resolution among the CO1 or CYTB haplotypes in this clade. We also note that in Subclade II.1, a few haplotypes (KY439008, KY439011, KY439012) are short (~300 nucleotides), but show large divergence (i.e., long branches; Figure 2); hence, their inclusion in this clade should be considered tentative.

3.2. Pseudogene analyses

From prior studies (Dusitsittipon et al., 2015, 2017), the primers Cytb‐F and Cytb‐R produced sequences with uninterrupted amino acid translations (i.e., no premature stop codons) for specimens that only fall out in Clade I (Figure 1). In the current study, these same primers yielded five haplotypes (H22–H26) with interrupted amino acid CYTB translations from 41 specimens collected from various locations across Thailand (Table S1). Upon using primers Cytb‐F3 and Cytb‐R2, we obtained CYTB sequences with uninterrupted amino acid translations from 30 of these 41 specimens (Table 1). Hence, both translatable and untranslatable haplotypes were obtained from the same individuals. The translatable haplotypes (from primers Cytb‐F3 and Cytb‐R2) from all 30 of these individuals fall in Clade II (Table 1, Figure 1).

We also highlight that the Cytb‐F and Cytb‐R primers were used in a study by Yong, Eamsobhana, Song, et al. (2015) for samples they identified as A. cantonensis and A. malaysiensis. However, upon downloading from GenBank, it was observed that all of Yong, Eamsobhana, Song, et al. (2015) sequences labeled as A. malaysiensis were marked as “unverified” on GenBank (Table S1). Indeed, straight translation (i.e., no gaps in the alignment are inserted) of these sequences revealed premature stop codons. One haplotype we observed, H24, was the same as their AMM_1TAK sample (GenBank # KP732098) (Figure 1, Table S1). Aligning these “unverified” sequences with our own samples showed eight different untranslatable haplotypes. After alignment of these eight to the reference mtDNA samples, the untranslatable haplotypes had four common regions with deletions of six, one, one, and two nucleotides in length. It is after the first two deletion regions that there is a frameshift that leads to several premature stop codons in translation of the ungapped haplotypes. These eight haplotypes are largely distinguished from one another by unique single indels or a few single nucleotide polymorphisms (Table S3). The phylogenetic analyses showed that all eight of the untranslatable haplotypes fall into a single clade, Clade III, which is sister to Clade I (Figure 1). Note that because the maximum‐likelihood analysis treats gaps as missing data, some unique untranslatable haplotypes appear identical in the phylogenetic tree as their only differences are indels (Figure 1).

The branch test with two ω ratios (ωbackground = 0.015, ωforeground = 0.534, lnL = −3,033) was significantly favored over the M0 model of a single ratio (ω = 0.019, lnL = −3,037) for all branches (χ2 = 8, df = 1, = .005). Hence, the hypothesized pseudogene branches show elevated ω. There was no difference in the branch‐site Model A (lnL = −3,025) and Model A with ω2 = 1 (lnL = −3,025), that is, ω2 was estimated to be 1 in Model A (Test 2, χ2 = 0, df = 1, = 1). However, Test 1 was significant were Model A was favored over M1a (lnL = −3,031; χ2 = 12, df = 2, = .002). The results of Test 1 and Test 2 are consistent with relaxed selection on the hypothesized pseudogene lineage.

4. DISCUSSION

4.1. Incongruence between taxonomic identifications and mtDNA lineages

In Dusitsittipon et al. (2017), we observed two divergent CYTB clades (>11% p‐distance) among wild‐caught larval samples originally identified as A. cantonensis (based on morphology of adult worms from experimentally infected rats). At the time of our study, we had used two mtDNA genome samples as references in our phylogenetic analyses because they were identified in their respective publications as A. cantonensis. These were NC_013065 (Lv et al., 2012) and KT186242 (Yong, Eamsobhana, Lim, et al., 2015; Yong, Song, et al., 2015), both of which originated from laboratory‐maintained isolates in China or Thailand, respectively. Clade I contained NC_013065 and Clade II had KT186242. Moreover, we observed these two mtDNA clades were completely congruent with two genetically distant clusters that were based on 12 nuclear microsatellite loci (Dusitsittipon et al., 2017). As the mtDNA and microsatellites came from the same individuals, the complete non‐random association between mtDNA clades and microsatellite clusters provided conclusive evidence that these two clades represented distinct species (Dusitsittipon et al., 2017). In the current study after adding additional CYTB haplotypes along with four more mtDNA reference samples, these two CYTB clades remained clearly defined (Figure 1). Furthermore, these two clades, anchored by the six reference mtDNA samples, are clearly observed in the CO1 phylogeny (Figure 2).

While the current molecular data show clear evidence of two species as reflected by the two clades (Figures 1 and 2), there are evident incongruences between taxonomic identifications of samples and mtDNA clades when comparing the CYTB and CO1 phylogenies. With the exception of the A. mackerrasae reference (discussed below), all haplotypes (CYTB or CO1) that fall in Clade I originated from samples originally identified as A. cantonensis (Tables S1 and S2). In contrast, samples that fall in Clade II were identified as either A. cantonensis or A. malaysiensis.

In the CO1 phylogeny, several haplotypes from wild‐collected larval samples that were identified as A. cantonensis in Vitta et al. (2016) fall into Clade II (Table S2, Figure 2). Vitta et al. (2016) also used KT186242 as a CO1 reference in their phylogeny. Haplotypes from Rodpai et al. (2016), also from wild‐caught larval samples, fell into Clade II. Rodpai et al. (2016) referred to their samples as A. malaysiensis in conjunction with the finding of two diverged CO1 clades that corresponded to two 18S ribosomal DNA (rDNA) clades that had prior species‐designated reference sequences (see below). Eamsobhana, Yong, et al. (2017) identified adult, wild‐caught samples as A. malaysiensis, and their samples also fall in Clade II (Table S2; Figure 2).

Notably, we highlight that the reference sequence KT186242 (Yong, Song, et al., 2015) was based on the whole‐genome sequence of a Thai laboratory isolate identified as A. cantonensis in Yong, Eamsobhana, Lim, et al. (2015). The same group in the subsequent year (Yong et al., 2016) published the mtDNA genome of a wild‐caught adult sample from Malaysia that they identified as A. malaysiensis (KT947979). Yong et al. (2016) and Eamsobhana, Yong, et al. (2017) do not compare KT947979 to KT186242. We note that these two mtDNA genomes, which carry different species names in GenBank, fall in Clade II (Figures 1 and 2) and are extremely similar at the CO1 and CYTB (<0.2% p‐distance, Table 2).

Selective inclusion/exclusion of haplotypes among studies along with possible misidentifications due to similar morphologies of A. malaysiensis and A. cantonensis (discussed below) have likely led to these incongruences between taxonomy of samples and phylogenetic relationships of their respective haplotypes. Based on the fact that all samples for CYTB and CO1 in Clade I have been identified as A. cantonensis and that Eamsobhana, Yong, et al. (2017) identified wild‐caught adult worms a priori as A. malaysiensis, we henceforth refer to Clade I as A. cantonensis and Clade II as A. malaysiensis.

Further support for assigning these species names to these clades comes from Rodpai et al. (2016) in which they obtained both CO1 and 18S rDNA sequences from the same individuals. Rodpai et al. (2016) found complete congruence between two CO1 clades and two 18S clades where the two 18S clades had prior reference sequences designating them as A. cantonensis (GenBank AY295804; Carreno & Nadler, 2003) or A. malaysiensis (GenBank EF514914; Fontanilla & Wade, 2008). To facilitate future studies, we provided Tables S5 and S6, which provide sample information linking 18S haplotypes and CO1 haplotypes as well as the alignment of the unique 18S haplotypes of A. malaysiensis and A. cantonensis in fasta format. We also note that the nuclear 18S clades of Rodpai et al. (2016) are completely congruent with the two main diverged microsatellite clusters observed in Dusitsittipon et al. (2017), thereby reinforcing the species delimitation of clades I and II. Of special note, because KT186242 (Yong, Song, et al., 2015) would now be classified as being from A. malaysiensis, then the genome sequence in Yong, Eamsobhana, Lim, et al. (2015) also needs to be reclassified as coming from A. malaysiensis and not A. cantonensis.

4.2. CYTB pseudogene

We found strong evidence for a CYTB pseudogene within individuals that are in the A. malaysiensis clade. First, from 30 individuals (Table 1), we obtained both an untranslatable haplotype that resides in Clade III and a translatable haplotype that falls in Clade II (Figure 1). Second, the untranslatable haplotypes show the classic signs of a pseudogenized gene in having indels, which caused frameshifts and thus, downstream premature stop codons. The four shared deletion regions (Table S3) in all eight haplotypes of Clade III suggest the deletions happened in the ancestral haplotype of this clade. Third, molecular evolution analyses supported relaxed selection with elevated ω on the pseudogene lineage.

Incorrect phylogenetic inferences can be drawn if the pseudogene is treated as an ortholog to the real mtDNA genes (Ballard & Whitlock, 2004). Yong, Eamsobhana, Song, et al. (2015) used the Cytb‐F and Cytb‐R primers on samples identified as A. malaysiensis and recovered untranslatable haplotypes. As shown in our analyses, these haplotypes of Yong, Eamsobhana, Song, et al. (2015) fall into Clade III, that is, the pseudogene clade. Fortunately, no phylogenetic inferences were grossly misrepresented as A. malaysiensis is still sister to A. cantonensis using the orthologous CO1 or CYTB genes (Figures 1 and 2). Nonetheless, appropriate genetic distance comparisons would need to be made between clades I and II and not clades I and III (e.g., Rodpai et al., 2016; Yong, Eamsobhana, Song, et al., 2015).

4.3. Need to verify cryptic lineages and A. mackerrasae as species

Another interesting pattern obtained by collectively analyzing the CO1 and CYTB data is that the sample mtDNA genome from A. mackerrasae (Aghazadeh et al., 2015) is nested within samples that have been identified as A. cantonensis (Subclade I.2, Figures 1 and 2). In particular, the A. mackerrasae sample is very closely related to and less than 1% divergent (p‐distance) at the CO1 and CYTB (Table 2) from AP017672 (Figures 1 and 2), an unpublished GenBank entry that was part of the 50 Helminth Genomes Project (BioProject: PPRJEB493). AP017672 was identified as A. cantonensis from Taiwan with no other information given.

Recently Song, Yong, and Eamsobhana (2017) compared the whole mtDNA of A. mackerrasae (Aghazadeh, 2015) to KT947978 (Thailand isolate of A. cantonensis, Yong et al., 2016) and to NC_013065 (China isolate of A. cantonensis, Lv et al., 2012). They found across all protein coding genes the following pairwise p‐distances: A. mackerrasaeKT947978 = 1.73%, A. mackerrasaeNC_013065 = 3.7%, KT947978NC_013065 = 3.52%. These overall distances are reflected in the average of the CO1 and CYTB p‐distances given in Table 2. Because of the genetic similarity, they concluded “…that A. mackerrasae may be conspecific with A. cantonensis (Song et al., 2017). It remains to be resolved whether A. mackerrasae is conspecific with A. cantonensis or undergoing incipient speciation.” We agree with their argument and in general suggest concordance in multiple markers be used in species delimitation especially when mtDNA divergence is low (Janzen et al., 2017).

Our prior study showed concordant patterns between nuclear microsatellite markers and CYTB lineages (Dusitsittipon et al., 2017). Affiliations between the subclades designated herein, and these microsatellite clusters are given in Table 3. The non‐random associations between mtDNA haplotypes and nuclear clusters, along with p‐distances upwards of 6% between some CYTB haplotypes (e.g., between Subclades I.1 and I.5) within Clade I, are strong suggestive evidence of cryptic species within what is regarded as the single species A. cantonensis (Dusitsittipon et al., 2017). For example, from the Nan province of Thailand, Dusitsittipon et al. (2017) found two CYTB haplotypes (H7 and H9; Subclades I.2 and I.3, respectively) each of which corresponded to distinct microsatellite clusters (clusters 6 and 5, respectively). Thus, in sympatry, strong mtDNA–nuclear marker associations remain intact. As another example, CYTB haplotypes 13, 14, 16, 17 (Subclade II.1; Figure 1) are found only in samples that belong to microsatellite Cluster 8, but yet this cluster is dispersed across seven provinces in Thailand (Dusitsittipon et al., 2017). The maintenance of mtDNA–nuclear marker associations within sympatry and across geography indicates reproductive isolation. Hence, we hypothesize that A. cantonensis may in fact be a recently diverged species complex wherein the five subclades in Clade I may reflect different species.

Table 3.

Subclade affiliations to microsatellite clusters from Dusitsittipon et al. (2017), country locations, and host species. Affiliations were made from sample information (Tables S1 and S2) from either the CO1 or CYTB haplotypes that fall within the respective clade. (L = laboratory‐maintained, W = wild‐collected, U = unknown origin. If no superscript is given, then it was wild‐collected.)

Subclade I.1 I.2 I.3, hypothesized I.4 I.5, hypothesized II.1
Microsatellite cluster 1–3 6 5 No data 4 8
Countries ThailandL,W TaiwanU
ThailandL,W
Australia
Japan
United States, mainland
Brazil 		Thailand ChinaL,W
United States, HawaiiL
Japan
Taiwan
Myanmar 		Thailand
ChinaL,W
Japan
Brazil 		ThailandL,W
Malaysia
Taiwan
Mollusc hosts Achatina fulica
Cryptozona siamensis 		Achatina fulica Achatina fulica Achatina fulica
Limax marginatus 		Achatina fulica Achatina fulica
Cryptozona siamensis
Mammal hosts Rattus rattus
Rattus exulans
Bandicota indica 		Rattus norvegicus
Rattus fuscipes
Rattus rattus
Bandicota indica
Diplothrix legata
Dasypus novemcinctu
Didelphis virginiana 		Rattus rattus Rattus norvegicus
Rattus rattus 		Rattus norvegicus
Rattus rattus 		Rattus rattus diardii
Rattus rattus
Rattus norvegicus
Bandicota savilei
Rattus losea
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Due to low phylogenetic resolution in the CYTB of Clade II and due to a lack of additional reference sequences (i.e., samples from which both CO1 and CYTB have been obtained), it is not possible to link to the microsatellite clusters 7 and 9 of Dusitsittipon et al. (2017).

Returning to discussion of the A. mackerrasae sample, we draw particular attention to CYTB Haplotype 7, which was reported within Nakhon Si Thammarat and Nan, Thailand (Dusitsittipon et al., 2017). Haplotype 7 is very closely related to the A. mackerrasae sample (differs by 2 of 852 bp; Subclade I.2; Figure 1). CYTB Haplotype 7 was restricted to individuals that were in microsatellite Cluster 6 and no other haplotype was found in this cluster (= 15; Dusitsittipon et al., 2017). Again, as there was 100% concordance between nuclear and mtDNA data, this is suggestive evidence in support of A. mackerrasae as a distinct species. Nevertheless, additional multilocus data are needed to confirm whether there are independent evolutionary units (i.e., distinct species) within Clade I. For example, based on the collective analyses we conducted herein, we would predict that if A. mackerrasae is indeed a distinct species, then samples of morphologically identified A. mackerrasae from Australia would have a microsatellite profile that would cluster them with Cluster 6.

4.4. Evolutionary epidemiological inferences: gaps in linking the phylogenetic data to the life history and morphology

First, we highlight two caveats in linking the CYTB and CO1 subclades. (i) We are assuming that there is no effective recombination in the mtDNA. Mitochondrial recombination, which has been documented in a few animal species (Ladoukakis & Zouros, 2017), would preclude anchoring the two phylogenies. However, as noted in our results, congruent CYTB and CO1 topologies and pairwise p‐distances among the six mtDNA reference samples suggest recombination was not present in appreciable amounts. (ii) The many small CO1 haplotypes led to low bootstrap support for many of the subclades in the CO1 tree. Hence, the subclade links we made should be regarded as tentative hypotheses that need to be tested with additional data. Our goal was to begin making sense of the available sequence data in relation to the biology of rat lungworms; thus, the subclade designations were necessary to facilitate discussion and address future avenues of study. Below we relate our phylogenetic results to what is known for the life histories, morphology, and geographic distributions of A. cantonensis, A. malaysiensis, and A. mackerrasae. Admittedly, we probably indicate more gaps than links to the phylogenetic data, but by calling attention to these gaps, we hope to highlight critical areas for future study. We only briefly summarize some key traits below. For a more extensive discussion of the life histories of these three species, we refer readers to an excellent review by Spratt (2015).

Angiostrongylus cantonensis, A. malaysiensis, and A. mackerrasae have similar adult morphologies. These three species are largely distinguished by the adult male spicule lengths and separation or length of bursal rays (Bhaibulaya, 1968, 1979; Bhaibulaya & Cross, 1971; Chen, 1935). Bursal ray separation and length are very subtle and A. malaysiensis and A. cantonensis overlap in the range of spicule lengths with A. cantonensis being larger on average. Angiostrongylus mackerrasae has the smallest spicule length and does not overlap the other two (Bhaibulaya, 1979). Likewise, the larvae have very subtle morphological differences (Bhaibulaya, 1975). In part, these subtle differences or overlap in traits has likely lead to some of the taxonomic–mtDNA clade incongruences we noted above. Therefore, we call on future studies to be explicit in key traits such as spicule length.

Also, A. cantonensis, A. malaysiensis, and A. mackerrasae have been described as having similar life histories. They all infect the pulmonary arteries and right ventricle of various rodents. However, differences in developmental rates and pathological affects in primates have been reported (Bhaibulaya, 1979; Cross, 1979). In particular, Cross (1979) describes how experimental infections of monkeys with various geographic isolates of A. cantonensis (morphologically identified) resulted in greater pathological effects and death than compared to infections with A. malaysiensis or A. mackerrasae (monkeys survived infections with the latter species). In experimental infections of rats, Cross (1979) recovered a statistically lower percentage of adults of A. malaysiensis compared to A. cantonensis.

We are aware of only two studies that have looked at morphology and/or life history in relation to mtDNA isolates. Monte et al. (2014) examined the morphology of laboratory‐maintained worms that had the CO1 ac8 (Subclade I.2, Figure 2) and CO1 ac9 (Subclade I.5, Figure 2) haplotypes. Interestingly, CO1 ac8 is closely related to the A. mackerrasae sample. They reported significant differences in the spicule length (mm): 1.29 for worms with ac8 and 1.23 for those with ac9. However, both of these means fall in the range of A. cantonensis (1–1.46) and out of the range for A. mackerrasae (0.4–0.56) (Bhaibulaya, 1979). Future studies are needed to determine whether spicule length (and other traits) is affected by environmental background (e.g., intermediate or definitive host species). Monte et al. (2012) also report greater larval output with infections of CO1 ac9. In Lee et al. (2014), morphology and pathogenicity were examined between two CO1 mtDNA isolates, Pingtung (P) and Hualien (H), identified as A. cantonensis from Taiwan. There is difficulty in interpreting their sequence data (see Table S2). Nonetheless, they reported significantly lower recovery of adult worms from rats for the H isolate compared to the P isolate and smaller female body size in the H isolate. Lee et al. (2014) also reported greater pathogenicity and survival in rats infected with the P isolate. They indicated no differences in male body size, bursal number, bursal shape, or spicule morphology (though sizes not given).

In some other interesting life‐history studies, cross‐breeding experiments by Bhaibulaya (1974) and Cross and Bhaibulaya (1974) have shown that viable F1 hybrids could be generated between A. cantonensis × A. mackerrasae and A. cantonensis × A. malaysiensis, respectively. However, while the F1 females appeared to produce eggs (which we take to mean oocytes), the F1 males did not produce spermatozoa. In agreement, with the results of the latter cross, Dusitsittipon et al. (2017) found an F1 hybrid between Clade I (A. cantonensis) and Clade II (A. malaysiensis), using microsatellite markers. The mtDNA–nuclear concordance for clades I and II indicates there is little to no backcrossing of F1 hybrids, which is in agreement F1 sterility found by Cross and Bhaibulaya (1974).

Table 3 indicates both host (intermediate and definitive) and geographic locations from which clades have been recorded. Some caution is advised in interpreting these reports as sampling is not equal among studies. Also, the molecular‐based identifications are based on the mtDNA results in Figures 1 and 2. There are rDNA‐based surveys. However, we do not cover the rDNA‐based surveys here as the lack of variation in the rDNA precludes assignment to the subclade level. Despite these limitations, some results confirm past morphological‐based surveys and some interesting patterns have also emerged. For example, although originally described from Malaysia, there are morphological‐based reports of A. malaysiensis in Thailand (Spratt, 2015). In particular, a mixed infection of A. cantonensis and A. malaysiensis has been reported from rats in Bangkok, Thailand (Bhaibulaya & Techasoponmani, 1972). These morphological reports are now confirmed with the molecular‐based studies of Rodpai et al. (2016) and Dusitsittipon et al. (2017), wherein in the latter study, sympatric populations of A. cantonensis and A. malaysiensis were found in Thailand. In addition to the locations reported for Subclade II.1 (Thailand, Malaysia, Taiwan), other countries where the mtDNA data indicate the occurrence of A. malaysiensis include Myanmar and Laos (Tables S1 and S2). Thus, there are no mtDNA‐based identifications of A. malaysiensis outside South‐East Asia.

In contrast, mtDNA‐identified samples of A. cantonensis, Clade I, have not only been found throughout South‐East Asia, but also in Japan, Brazil, and the continental United States. Subclades I.1 and I.3 have only been reported from Thailand. Subclade I.4 is largely restricted to South‐East Asia and Japan. The Hawai'i report (GenBank KP721454 in Figure 1) in this subclade is from a Thailand laboratory‐maintained isolate by way of a Japan laboratory‐maintained isolate (Table S1). The other Hawai'i reports, CO1 haplotypes ac5b and ac5 (sister to Subclade I.2; Figure 2), are also based on laboratory‐maintained isolates in Japan or Thailand (Table S2). As the Hawai'i isolates are not in the same subclades, it appears that there may be more than one type of Hawai'i laboratory isolate. The most globally distributed subclades are I.2 and I.5. Subclade I.2 is interesting in that it contains the A. mackerrasae sample, which is the sole sample from Australia. Intriguingly, the larval samples from Dalton et al. (2017) (GenBank MF000735 and MF000736, Figure 2) that were reported from wildlife in the continental United States are closely related to A. mackerrasae (Figure 2). Thus, if Subclade I.2 represents A. mackerrasae, then caution is advised in interpreting past global reports of A. cantonensis as it is clear that Subclade I.2 has also been introduced to the Americas (Table 3).

5. SUMMARY

Our study represents an initial attempt to consolidate the available mtDNA data to link the findings of past studies. Assimilating the available mtDNA has highlighted three critical factors that investigators need to be aware of or resolve in future studies on the evolutionary epidemiology of A. cantonensis. First, there are incongruences between species identifications and mtDNA variants. We provided a resolution to this problem above and Tables [Link], [Link], [Link], [Link] to aid future studies. Second, we presented strong evidence of a CYTB pseudogene. The primers we designed should enable avoidance of this pseudogene. Third, current mtDNA–nuclear concordant patterns strongly hint at the presence of several cryptic species within Clade I and Clade II (Dusitsittipon et al., 2017). More multilocus‐based studies are needed to assess species delimitations and to test the validity of A. mackerrasae.

Eosinophilic meningitis has only been attributed to A. cantonensis (Barratt et al., 2016), and Spratt (2015) indicates there has not been unequivocal evidence to show that A. mackerrasae or A. malaysiensis are zoonotics. However, as discussed above, morphological identifications of these species are difficult due to their similarities. Thus, experiments are needed to determine trait distributions within clades (or subclades) and where possible, definitively link morphological traits to the molecular‐based phylogenetic lineages. In addition, current molecular diagnostic tools rely on rDNA (Qvarnstrom et al., 2010), which does not have as much variation as mtDNA. The geographic affiliations of subclades given in Table 3 suggest global distributions could be limited to just some subclades. Finer genetic marker resolution is needed because existing studies suggest variation in life history or pathogenicity among lineages (Lee et al., 2014; Monte et al., 2012). More studies are necessary to determine whether mtDNA subclades (possibly representing a species complex) are associated with life‐history, infectivity, or pathogenicity traits. Such studies will provide a clearer picture of the evolutionary epidemiology of A. cantonensis and closely related species as well as enable molecular diagnostics when examining outbreaks or varying pathologies.

CONFLICT OF INTEREST

None declared.

Supporting information

 

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ACKNOWLEDGEMENTS

This work was supported by Agricultural Research Development Agency (CRP5705020410), and Development and Promotion of Science and Technology Talents Project (DPST; Royal Government of Thailand scholarship). We thank our colleagues in Criscione Lab (Isabel Caballero, Emily Kasl, and Andrew Sakla) at the Department of Biology, Texas A&M University, TX, USA, for providing helpful suggestions and technical support, particularly for the microsatellite work. We also thank the Department of Helminthology, Faculty of Tropical Medicine, Mahidol University, Thailand, for technical support, particularly for part of the DNA analysis.

Data for this study are available at: Newly generated pseudogene haplotypes are deposited in GenBank (MG516589–MG516592). All data, including explicit alignment files and matching haplotype information with associated GenBank accession numbers, are included in the supplemental files.

Dusitsittipon S, Criscione CD, Morand S, Komalamisra C, Thaenkham U. Hurdles in the evolutionary epidemiology of Angiostrongylus cantonensis: Pseudogenes, incongruence between taxonomy and DNA sequence variants, and cryptic lineages. Evol Appl. 2018;11:1257–1269. 10.1111/eva.12621

Contributor Information

Charles D. Criscione, Email: ccriscione@bio.tamu.edu

Urusa Thaenkham, Email: urusa.tha@mahidol.ac.th.

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