Molecular detection of a novel Ancylostoma sp. by whole mtDNA sequence from pangolin Manis javanica

Ancylostoma species are hematophagous parasites that cause chronic hemorrhage in various animals and humans. Pangolins, also known as scaly anteaters, are mammals that live in soil environments where they are readily exposed to soil-borne parasitic nematodes. However, only a limited number of helminth species have been identified in this animal host so far. Ancylostoma sp. was isolated from a wild pangolin, and the complete mitochondrial (mt) genome of Ancylostoma sp. was obtained by Illumina sequencing of total genomic DNA. The circular complete mt genome that was assembled had a total length of 13,757 bp and comprised 12 protein-coding genes (PCGs), 22 transfer ribosomal RNAs, two ribosomal RNAs (rRNAs), two non-coding regions and one AT-rich region, but lacked the gene coding for ATPase subunit 8 (atp8). The overall AT content of the mt genome of Ancylostoma sp. was 76%, which is similar to that of other nematodes. The PCGs used two start codons (ATT and TTG) and three stop codons (TAA, TAG, and T). The nucleotide identity of the 12 PCGs ranged from 83.1% to 89.7% and had the highest sequence identity with Ancylostoma caninum among species in the Ancylostomatidae family. Also, the pangolin-derived Ancylostoma sp. lacked repeat sequences in the non-coding regions and in the unique sequence of the short non-coding regions, which differentiated it from other Ancylostoma species. In addition, phylogenetic analyses of 18S rRNA and mtDNA sequences revealed that the Ancylostoma sp. was positioned in a separate branch in the subfamily Ancylostomatinae along with other Ancylostoma species. The Ancylostoma sp. isolated from a pangolin in this study was identified as a possible new Ancylostoma species. The identification of this Ancylostoma sp. from pangolin enriches our knowledge of the species in the Ancylostomatidae family and provides information that will lead to a better understanding of the taxonomy, diagnostics, and biology of hookworms.

Morphological and morphometric methods have been used to classify nematodes based on the shape of their mouth, tail and sexual organ, the size of the worm body, eggs and larvae [11,12]. However, these traditional methods for nematode identification have been challenged for a number of reasons. Firstly, some species share similar morphological characteristics; for example, eggs of Necator americanus, Ancylostoma species and Strongylids have similar shapes, and it is not easy to discriminate between closely related species [13]. Traditional identification methods also face some challenges in identifying cryptic species of parasitic nematodes due to their identical morphological features [6]. In addition, nematode collection is also complicated by seasonal fluctuations in the prevalence and intensity of specific species; consequently long-term monitoring is required to collect all nematodes of particular hosts [14]. Another complication is obtaining intact nematodes for morphological identification. Therefore, molecular approaches have been used to discriminate nematodes via nuclear genetic markers and mitochondrial genomes. The mitochondrial (mt) genome has important unique features of maternal inheritance and rapid evolution, but an absence of recombination [15,16]. Hence, mt genomes provide genetic markers for molecular identification, epidemiological and genetic studies, as well as for phylogenetic and population studies [17][18][19][20].
Pangolins, also known as the scaly anteater, are endangered and rare animals that require special protection [21]. These small mammals live in soil environments and can be easily exposed to soil parasitic nematodes. However, only a few helminth parasites have been identified, using egg and adult morphological characteristics, after being isolated from the pangolin gastrointestinal tract; many others are still unknown. A total of 13 parasitic helminths have been reported from pangolins to date. Of these, eight helminth parasites were isolated from the gastrointestinal tract in egg, larvae and adult morphological investigations, including Cylicospirura sp., Leipernema leiperi, Manistrongylus meyeri, Necator americanus, Strongyloides sp., Trichochenia meyeri, Ancylostoma sp. and Gendrespirura sp. [22][23][24][25][26][27]. Until recently, the identification of Ancylostoma species in pangolin was limited to the genus level. In the family Ancylostomatidae, only N. americanus has been identified in pangolin to the species level [28]. However, there is a paucity of molecular data for identifying Ancylostoma species in pangolins. The aims of this study were to obtain a molecular characterization of a novel Ancylostoma sp. originated from a wild pangolin through the sequencing of total DNA using the Illumina sequencing platform (Illumina, Inc., San Diego, CA, USA).

Parasite collection
Guangzhou customs confiscated two pangolins from poachers and placed them in the Guangzhou Zoo, Guangdong Province, China. No information on the origin and species of the pangolins was available. One pangolin suffered severe trauma and a purulent infection of the forelimb and ultimately died due to complicated infections. During the post-mortem examination, a total of 15 adult parasites were collected from the duodenum of the naturally infected pangolin. The parasites were washed completely in phosphate-buffered saline, preserved in 70% ethanol and frozen for further identification. Prior to examination under a microscrope, the worms were cleaned with lactophenol and mounted in glycerine. We examined several frozen worms to obtain a complete description of their morphological features under dissecting microscopes (magnifications: 10-40×) and light microscopes (magnifications: 40-100×), but it was difficult to obtain precise morphological features.

DNA extraction and whole-genome amplification
Total genomic DNA was extracted from a single adult worm using the Wizard ® SV Genomic DNA Purification System (Promega, Guangzhou, China) according to the manufacturer's instructions and then stored at − 20 °C until use. Complete genomic DNA was amplified using a whole genome amplification kit (REPLI-g ® Midi Kit; Qiagen, Hilden, Germany). All procedures were performed according to the manufacturer's instructions. The amplified DNA was sequenced with an Illumina Novaseq 6000 sequencing platform using a 150-bp paired-end technique (Illumina, Inc.). Approximately 12 Gb of sequence data had a quality score (Q-score) ≥ 20.

PCR amplification and DNA sequencing
The 18S ribosomal ribonucleic acid (rRNA) gene was amplified from the total extracted DNA of the observed worm using DreamTaq DNA Polymerase with the primers NC18S (AAA GAT TAA GCC ATGCA) and NC5B (GCA GGT TCA CCT ACA GAT ) [29]. The amplification procedure was: 95 °C for 5 min; followed by 35 cycles of 95 °C for 30 s, 54 °C for 30 s, 71 °C for 75 min and 72 °C for 5 min. The amplified fragments were visualized and verified by electrophoresis in a 1.5% agar gel (Sangon Biotech Co., Ltd. Shanghai, China) with staining (0.2 mg/ml ethidium bromide). The PCR fragments were sequenced by Sanger sequencing (Sangon Biotech Co.).

Assembly of the complete mt genome of pangolin and worm
The raw data was mapped to the pangolin genome and then filtered using Samtools (v1. 7) to remove the host gene sequences [30]. The filtered data were assembled into contigs and scaffolds using SPAdes (v3.14.1) [31]. Contigs were aligned into the nucleotide (nt) database using BLAST+ (v2.11.0) [32]. We extracted contigs that contained worm mt genomes with a sequencing depth > 100 and a length > 150 bp. Finally, eight contigs were randomly chosen as a seed sequence, and each seed sequence was assembled using Novoplasty (v.4.2) to reconstruct the complete mt genome of the worm [33].
To determine host identity, the filtered host data were also assembled into contigs and scaffolds using SPAdes, and all the mitochondrial contigs were aligned to the nt database using BLAST+ (v2.11.0). We identified the pangolin mtDNA by comparing it with the known mtDNA of pangolin species available in GenBank.

Gene annotation and sequence analysis
Gene annotation of the assembled mt genome was conducted using MITOS and Geseq (https:// chlor obox. mpimp-golm. mpg. de/ geseq. html) [34]. The Mitos webserver was employed to predict protein-coding genes (PCGs) and non-coding regions (NCRs) of parasitic nematodes using the genetic code of invertebrate mtDNA (http:// mitos. bioinf. uni-leipz ig. de) [35]. Initiation and termination codons were identified using the Expasy translation tool (https:// web. expasy. org/ trans late/) [36]. The secondary structures of transfer RNA (tRNA) were predicted and shown by MiTFi and the webserver FoRNA on Mitos [37]. Both rRNA genes (small and large ribosomal subunits [rrnS and rrnL, respectively]) were identified by MiTFi. The codon usage of amino acids for PCGs was determined by the sequence manipulation suite [38]. The complete mt genome was visualized by the MTviz (http:// pacosy. infor matik. uni-leipz ig. de/ mtviz/). A comparison of the nucleotide identity (%) of the observed worm mt genome with 13 closely related species of the Ancylostomatidae family was conducted using Clustal Omega [39].

Phylogenetic analysis of 18S rRNA and PCGs of mt genome of worm
We obtained 18S rRNA sequences of 14 nematodes from the NCBI database and used these and the amplified 18S rRNA of the worm to construct a phylogenetic tree (Additional file 1: Table S1). The maximum likelihood (ML) method was performed to evaluate the phylogenetic tree, and the ML tree was made with the TPM3 + G4 model using RAxML-ng (v. 1.0.2) [40]. ML bootstrap > 70% was considered to be strong support [41].
We obtained nucleotide sequences of 12 PCGs from the mt genome of the worm isolated from the pangolin. We also downloaded the complete mt genome sequences of 13 species in the Ancylostomatidae family and 4 species in the Chabertiidae family (outgroup) from NCBI GenBank and aligned these for sequence comparison (Additional file 1: Table S2). A phylogenic tree was reconstructed with RAxML-ng (v. 1.0.2) and a ML method was used with the GTR+G+I model.

Identification of pangolin species
To identify the pangolin species implicated in this case, we obtained the mt genome of the animal, with a total length of 16,574 bp, from Illumina sequencing data. This mtDNA showed the highest sequence identity (99.50%) and coverage (99.0%) with Manis javanica (Malayan pangolin) available from GenBank (accession number: MG196302.1).

Observation on the worm
The worms were isolated from the wild pangolin's duodenum and frozen immediately in 75% ethanol for further identification. The worms were round and tapered at both ends. However, it was challenging to observe precise morphological features due to frozen state of the worms. Therefore, we performed molecular characterization using total genomic DNA by Illumina sequencing.

Primary identification of worm by molecular markers
The amplified 18S rDNA sequence of the worm was 1681 bp and was deposited in GenBank databases under accession number: MZ681936.1. It showed 99.88% sequence identity with the 18S rDNA sequence of A. caninum from GenBank (accession number: AJ920347.2). Phylogenetic analysis of 18S rRNA sequences showed that the amplified 18S rDNA sequence of the worm clustered with Ancylostoma duodenale, A. caninum and N. americanus in the family of Ancylostomatidae (Fig. 1). This worm was relatively closer to Ancylostoma species than N. americanus. Thus, we proposed that this worm might be closely related to Ancylostoma species in the Ancylostomatidae family.

Features, gene organization and composition of the mt genome
For further identification of this worm, we obtained 12 Gb of raw data with 80,271,718 reads from the complete genomic DNA of the worm using Illumina sequencing. The assembled sequence showed that the complete mt genome of the worm was 13,757 bp; this sequence was deposited in GenBank with accession number MZ665481.1. The mt genome of this worm was a circular DNA molecule and contained 36 genes, comprising 12 PCGs, 22 tRNA genes (2 coding for leucine and 2 coding for serine), two rRNA genes, two NCRs (a long non-coding region [LNCR] and a short noncoding region [SNCR]) and an AT-rich region. Interestingly, the ATPase subunit 8 gene (atp8) was missing from the mt genome (Fig. 2). Twelve PCGs of this worm were transcribed in the same direction. In general, the overall base composition of the mt genome of this worm was: A = 27%, T = 49%, C = 7% and G = 17%, with an entire AT content of 76%, which was greatly inclined towards A and T bases. The AT-and GCskews of the worm's mt genome were determined to be: AT-skew (A−T)/(A+T) = − 0.26; GC-skew (G−C)/ (G+C) = 0.41; Additional file 1: Table S3).

PCGs and codon usage
The total length of the 12 PCGs was 10,283 bp, which accounts for 74.7% of the entire mt genome of the worm. These PCGs ranged in size from 234 bp of NADH dehydrogenase subunit 4L (nad4L) to 1578 bp of cytochrome c oxidase subunit I (cox1). The overall base composition of the PCGs in the worm mt genome was: A = 25%, T = 50%, C = 7% and G = 18%, with AT skew = − 0.32 and GC skew = 0.42, which was largely biased towards the A and T bases. The most favored nucleotide was the T base, but the C base was the least favored in PCGs of the worm. The nad4L gene had the highest AT content (81%) among the 12 PCGs, while cox1 had the lowest AT content (68%) (Additional file 1: Table S3). All of the ATskew values of the 12 PCGs were negative, and all of the GC-skew values were positive.
The PCGs of the worm contained a total of 3417 amino acids. Two different types of codons (ATT and TTG) were used as start codons, while three different  (Table 1). ATT was used as a start codon in 10 genes, namely cox1, cox2, nad3, nad5, nad6, nad4L, nad1, atp6, cob and cox3, while TTG was used as a start codon in the nad2 and nad4 genes. TAA was used as a stop codon in seven genes: cox1, cox2, nad6, nad4L, nad1, cytochrome b (cob) and nad4. TAG was used as a stop codon in three genes, including nad3, atp6 and nad2; moreover, an incomplete codon (T) was used in the genes nad5 and cox3 for transcription termination. Thus, in 12 PCGs, ATT and TAA were the most frequently used start and stop codons, respectively. Phenylalanine (TTT: 13.0%) was the most repeatedly employed amino acid in the mt genome of the worm, followed by leucine (TTA: 8.6%) and isoleucine (ATT: 7.0%). However, some transcription codons were absent, such as CGC and CGG coding for arginine and CTC coding for leucine (Table 2).

rRNA and tRNA genes
The worm had two rRNAs, including a large subunit (rrnL) of 967 bp and a small subunit (rrnS) of 698 bp.
The rrnL was situated between trnH and nad3, while rrnS was found between trnE and trnS2. The position of rRNA in Ancylostoma sp. was similar to that found in other Ancylostoma species but distinct from that found in Trichinella spiralis (class Adenophorea) [43]. The rrnL of the worm was longer than the rrnL of 13 species in the Ancylostomatidae family, which ranged from 957 bp (Uncinaria sanguinis) to 963 bp (A. caninum) ( Table 3). In addition, sequence identity of rrnL and rrnS in the observed worm was higher with species in the subfamily Ancylostomatinae than with species in the subfamily Bunostominae. The highest sequence identity of rrnL of the worm was 89.6% with Ancylostoma tubaeforme compared to other species in the Ancylostomatidae family, and rrnS had the highest sequence identity of 94% with Ancylostoma ceylanicum (Table 3). The length of the 22 tRNAs ranged from 53 bp (trnS1) to 63 bp (trnS2 and trnK). The total length of the 22 tRNAs of the worm was 1239 bp with an A+T content of 80%; consequently, most codons were composed of A+T bases relative to G+C bases. Apart from serine (CUN and UUR) and leucine (AGR and UGN), there was a one-to-one binding between codon and anticodon for all other tRNAs. With the exception of trnS1 and trnS2, all tRNA secondary structures of the mt genome of Ancylostoma sp. had the DHU arm and DHU loop, which were similar to those of most nematodes, including Toxocara canis, Ascaris suum, A. tubaeforme, Onchocerca volvulus and Anisakis simplex [44][45][46][47][48]. Only trnI, trnK, trnS1 and trnS2 had a pseudouridine (TΨC) arm. Other tRNAs lacked a pseudouridine (TΨC) arm and changed into a TV replacement loop. Moreover, an undeveloped form of the TΨC loop was only found in trnK; a typical TΨC loop was detected in trnM but it lacked TΨC arm (Additional file 1: Fig. S1).

NCR and AT-rich regions
The LNCR of the worm was located between nad4 and cox1 with a length of 106 bp, whereas the SNCR was found between nad3 and nad5 with a length of 100. The entire base composition of the NCRs was as follows: A = 41%, G = 10%, C = 4%, T = 45%, AT = 86% and GC = 14%. The NCRs of this worm lacked repeat sequences, unlike other Ancylostoma species, including A. caninum, A. ceylanicum, A. tubaeforme and A. duodenale. LNCR sequence identity of the worm was   [49]. Nonetheless, the SNCR of the worm had low identity with a few species in the family Ancylostomatidae, while there was no sequence identity with many species in the family of Ancylostomatidae (Table 3). Thus, the SNCR was the unique region in the mt genome of the worm based on nucleotide identity ( Table 3). The AT-rich region was situated between trnA and trnP in the mt genome of the worm. The size of ATrich region of the worm (261 bp) lay within range 173 bp (N. americanus) and 333 bp (A. duodenale and B. phlebotomum) ( Table 3). The AT-rich region had 90% A+T content and comprised a poly-A stretch, poly-T stretch and microsatellites (such as an TA or TA repeat). The AT-rich region of the worm had a sequence identity of 73.2-80.8% with that of species in the subfamily Ancylostomatinae, and 50.6-60.0% sequence identify with some species in the subfamily Bunostominae. The AT-rich region of the worm had no sequence identity with that of N. americanus in the subfamily Bunostominae (Table 3). Thus, the sequence of the AT-rich region showed that this worm was more closely related to species in the subfamily Ancylostomatinae than to species in the subfamily Bunostominae.

Comparison of the worm mt genome with that of species in the family Ancylostomatidae
Total sequences of the worm mt genome had higher identities of 86.8-87.3% with those of related species in the subfamily Ancylostomatinae than with those in the subfamily Bunostominae (Table 3). Moreover, the entire mt genome of the worm had the highest sequence identity of 87.3% with A. caninum compared to other Ancylostomatidae species (Table 3). The relatively low sequence identity was noted with the Bunostomum species, Uncinaria sanguinis, and N. americanus, with sequence identity ranging from 80.8% to 83.7%. In PCGs, the most conserved gene across the subfamily Ancylostomatinae was nad4L, with a sequence identity of 89.7-92.8%, whereas nad6 was the least conserved gene with 80.0-83.6% sequence identity ( Table 3). The 12 PCGs of the collected worm also had the highest sequence identity (83.1-91.0%) with A. caninum compared with other species from the subfamilies Ancylostomatinae and Bunostominae. These results suggest that the reported worm is an undescribed Ancylostoma sp. and genetically related closer to A. caninum than to other Ancylostoma species.

PCGs of the mt genome based on phylogenetic analysis
The PCG sequences of the collected Ancylostoma sp., 12 species from the Ancylostomatidae family and 4 species from the Chabertiidae family (outgroup) were used to reconstruct the phylogenetic tree (Fig. 3). Accordingly, Ancylostoma sp. was grouped into the family Ancylostomatidae, separate from the species of the Chabertiidae family. In the Ancylostomatinae subfamily, Ancylostoma sp. was grouped with A. ceylanicum, A. caninum, A. tubaeforme and A. duodenale, while N. americanus and two Bunostomum species (Bunostomum phlebotumum and Bunostomum trignocephalum) were grouped in the Bunostominae subfamily (Fig. 3). Thus, the worm had a closer relationship with A. ceylanicum, A. caninum, A. tubaeforme and A. duodenale than to species in the subfamily Bunostominae. Phylogenetic analyses of the PCGs showed that Ancylostoma sp. clustered with other Ancylostoma species in the Ancylostomatinae subfamily. Sequence identity showed that the Ancylostoma sp. from the pangolin was distinct from known species of the genus Ancylostoma. Thus, the Ancylostoma analyzed herein may represent a novel species in the genus Ancylostoma.

Discussion
Ancylostoma species are one of the most prevalent soiltransmitted helminths, affecting both domestic and wild animals, as well as humans. In this study, we identified a novel Ancylostoma sp. that originated from a Sunda pangolin (Manis javanica) by analysis of the mt genome using Illumina sequencing of total DNA.
The complete mt genome of Ancylostoma sp. was 13,757 bp, which is longer than that of A. caninum (13,717 bp) [50], A. tubaeforme (13,730 bp) [48], A. ceylanicum (13,660 bp) [51], A. duodenale (13,721 bp), U. sanguinis (13,753 bp) [52], and N. americanus (13,606 bp), respectively [53], but shorter than that of B. phlebotomum (13,790 bp) [50]. This difference in mt genome length is due to the longer NCR and rRNA sequences of A. caninum in comparison to those of other Ancylostomatidae species. Thus, differences in mt genome size may be a useful indicator to increase our understanding of mtDNA mutation, mitochondrial genetics and evolutionary biology. The 12 PCGs of Ancylostoma sp. were transcribed in the same direction as those of class Secernentea nematodes of hookworms (A. duodenale and N. americanus) and other species (Ascaris suum and Onchocerca volvulus) [45,49]. The direction of transcription in the mtDNA of Secernentea nematodes is conserved. The mt genome organization and gene arrangement of Ancylostoma sp. were similar with those of N. americanus and A. duodenale, with the exception of the position of rrnL and rrnS, which were located between trnH and nad3, and trnE and trnS2, respectively [49]. However, the gene arrangement and organization of Ancylostoma sp. were identical with those of A. tubaeforme, A. caninum and B. phlebotomum [48,50]. The cox1 gene in Ancylostoma sp. was the longest gene among the 12 PCGs, similar to the situation in A. tubaeforme [48]; conversely, nad5 was the longest gene in A. ceylanicum, A. doudenale and N. americanus [48,49,53]. Nad4L was the shortest region of the PCGs in Ancylostoma sp., which is consistent with observations in other hookworms [48,50]. The overall base composition of PCGs in Ancylostoma sp. was inclined towards AT bases. All PCGs from different nematodes have a higher AT base selection that maintains the stability of gene structure through decreasing gene mutation [54]. Thus, the length of mtDNA and PCGs of Ancylostoma sp. was slightly different from that of known Ancylostoma species. A complete mt genome sequence of Ancylostoma species can be used as a genetic marker for molecular investigation and diagnosis of members of the family Ancylostomatidae. Moreover, the entire mt genome data of Ancylostoma sp. would contribute to a further understanding of the pangolin helminth fauna.
ATT is the most common start codon found in hookworms, followed by TTG. Likewise, Ancylostoma sp. used ATT and TTG as start codons, similar to A. ceylanicum and A. duodenale [49,51]. Nonetheless, A. tubaeforme and A. caninum utilize GTG as additional start codons [48,50]. This variation in codon usage in the different genes of parasite species arises from various factors, but mainly from compositional constraints and translational selection [55]. It is noteworthy that the start codons of nad5 and nad6 in Ancylostoma species were remarkably different from other those of PCGs [8]. With the exception of A. ceylanicum, the nad5 gene of this Ancylostoma sp. and other Ancylostoma species uses ATT as a start codon. Similarly, the nad6 gene of Ancylostoma sp. utilized ATT as a start codon, consistent with A. ceylanicum but distinct from A. tubaeforme and A. caninum, both of which use GTG codons [48,50]. Ancylostoma sp. utilized three codons (TAA, TAG and T) as stop codons, but A. caninum, A. tubaeforme and A. doudenale use additional TA codons [48][49][50]. The translation termination in the cox3 and nad5 genes of Ancylostoma sp. used an incomplete codon of T, which is similar to that of cox3 and nad5 genes in A. ceylanicum and N. americanus [51,53]. It is believed that post-transcriptional polyadenylation has been shown to complete codons by adding A's to incomplete stop codons, resulting in TAA [56].
The majority of codons were composed of A and T bases, contributing to the high AT content of the entire mt genome of Ancylostoma sp. Nucleotide bias significantly impacts codon usage and amino acid composition. For example, it has been reported that mutational bias at the nucleotide level can alter codon usage and amino acid content [57,58]. The length of the rrnL gene of Ancylostoma sp. was 967 bp, which is longer than that of other known species of hookworm by 4 bp (A. caninum, B. phlebotumum), 7 bp (A. ceylanicum), 9 bp (A. tubaeforme and N. americanus) and 11 bp (A. doudenale) [48][49][50]. The rrnS gene of Ancylostoma sp. (698 bp) was slightly longer than that of other hookworm species, with the exception of N. americanus (699 bp) [49]. Thus, the difference in the entire mt genome size of Ancylostoma sp. from other known hookworm species is also due to longer rRNA sizes.
Ancylostoma sp. had an AT-rich region with a length of 261 bp and maximum A+T content of 90%. The placement of the AT-rich region of Ancylostoma sp. was between trnA and trnP, which is consistent with all hookworms [10,48,51]. Although the function of the AT-rich region has not yet been explored, it is believed to be the epicenter for the the initiation of gene replication and transcription [15]. The SNCR in Ancylostoma sp. was larger than that of other hookworms in the families Ancylostomatinae and Bunostominae [10,[49][50][51]. However, the position of the SNCR in the mt genome was identical to that of other Ancylostoma species [50,53]. The LNCR in Ancylostoma sp. (106 bp) was larger than that in most hookworm species, with the exception of A. tubaeforme (107 bp) and B. phlebotomum (108 bp) [48,50]. Previous studies showed that the NCR contained repeat sequences of TTTTA in A. caninum and A. ceylanicum; TAT ATT TAGT in A. tubaeforme; and TTTG in A. doudenale [48]. However, none of these repeat sequences were found in the NCR of Ancylostoma sp. Thus, the NCR of Ancylostoma sp. is an important region that differentiates this species from other Ancylostoma species.
Phylogenetic analyses of 18S rRNA and the complete mt genome showed that the Ancylostoma sp. clustered with A. ceylanicum, A. caninum, A. tubaeforme and A. duodenale in the subfamily Ancylostomatinae. However, some differences in the size of the mt genome, codon usage in PCGs, NCR sequences and tRNA secondary structures of the Ancylostoma sp. mt genome were helpful to differentiate it from other Ancylostoma species. Based on these results, we believe that this is a novel Ancylostoma species in the family Ancylostomatidae.

Conclusions
We characterized the complete mt genome of an Ancylostoma sp. isolated from the Sunda pangolin (Manis javanica) by Illumina sequencing of total DNA. Amplified 18S rRNA and mt genome data identified this Ancylostoma sp. as a novel species in the Ancylostomatidae family. The identification of this novel mtDNA sequence enriches our knowledge of mt genomes in the Ancylostomatidae family.