Abstract
Background
Giardia duodenalis is a flagellated parasite that causes diarrhea in humans and other animals. Although G. duodenalis is found in companion animals worldwide, information regarding the prevalence and genetic characteristics of G. duodenalis in pet chipmunks in China is limited. The present study therefore aimed to investigate the prevalence and genotypes of G. duodenalis in pet chipmunks in Sichuan province, southwestern China, as well as to assess zoonotic potential of revealed assemblages.
Results
A total of 279 fecal samples were collected from pet chipmunks in seven pet shops and one breeding facility in Sichuan province, southwestern China. The prevalence of G. duodenalis was 8.6% (24/279), as determined by nested PCR detection of the beta giardin (bg) gene. Giardia duodenalis assemblages and subtypes were determined using multilocus genotyping of the bg, triosephosphate isomerase (tpi), and glutamate dehydrogenase (gdh) loci. Two assemblages were identified: potentially zoonotic assemblage A (54.2%, 13/24) and rodent-specific assemblage G (45.8%, 11/24). A total of 24, 17 and 17 sequences of the bg, gdh and tpi loci, respectively, were successfully obtained, which formed four, four and three subtypes, respectively. Moreover, four assemblage A (MLGs A1-A4) and three assemblage G (MLGs G1-G3) multilocus genotypes were identified.
Conclusions
To our knowledge, this is the first study that investigated G. duodenalis in pet chipmunks in China. Detection of assemblage A in pet chipmunks and in previous studies in humans suggests a possible role of chipmunks as a reservoir for human giardiasis in Sichuan Province, China.
Electronic supplementary material
The online version of this article (10.1186/s13071-018-2790-z) contains supplementary material, which is available to authorized users.
Keywords: Giardia duodenalis, Chipmunk, Assemblage, Multilocus genotype
Background
Giardia duodenalis is a common enteric parasite that infects a broad spectrum of vertebrate hosts, including humans, livestock, companion animals and wildlife worldwide [1]. Usually, humans and animals become infected with G. duodenalis via fecal-oral route by ingesting infective stage cysts in contaminated food or water [2]. Clinical manifestations vary depending upon the immunological status of the host [3]. In immunocompetent individuals, G. duodenalis causes self-limiting diarrhea and malabsorption, whereas in infants, elderly persons, and individuals with deficient immune system, it also can cause chronic or life-threatening diarrhea and weight loss [4, 5].
Molecular studies have demonstrated that G. duodenalis comprises at least eight genetically distinct assemblages (A-H) [6]. Assemblages A and B, considered zoonotic genotypes, can infect humans and a wide range of mammalian hosts, whereas the remaining assemblages (C-H) seem to be host-specific [7]. Assemblages C and D mainly infect dogs, assemblage E livestock, assemblage F cats, assemblage G rodents, and assemblage H marine mammals [8, 9]. So far, assemblages A and B have been determined as predominant genetic sub-populations of Giardia in pet rodents in countries such as Spain, Italy, Australia, Belgium and China [10–12]. In addition, assemblages C, G, and E have been also occasionally identified in pet rodents [12, 13].
In China, epidemiological data about Giardia prevalence have been reported in domestic dogs and cats (assemblages C and D) [14], raccoon dogs (assemblages C and D) [15], cattle (A, B, and E) [16], horses (assemblages A and B) [17], sheep, goats (assemblages A, B and E) [18, 19], pet chinchillas (assemblages A and B) [11], as well as in humans (assemblages A and B) [20]. Recently, chipmunks (Eutamias asiaticus) have become popular in China as companion animals. As such, they have been commercially bred in significant numbers in many breeding facilities. However, information regarding G. duodenalis infection in pet chipmunks in China is rare, and the zoonotic potential of this parasite in chipmunks remains unknown. Therefore, the purpose of this study was to identify the prevalence and assemblages of G. duodenalis in pet chipmunks and to determine the genetic characteristics of G. duodenalis-positive samples.
Methods
Specimen collection
From March 2016 to April 2017, 279 fecal specimens were collected from chipmunks in seven pet shops and one breeding facility located in Sichuan province, southwestern China (Additional file 1: Table S1). Chipmunks were bred in individual cages. Fecal samples were collected from the bottom of the each cage, immediately placed into individual 30 ml sterile containers, and taken to the laboratory in a cooler with ice packs within 24 h. At sampling time, the age, sex, and health condition were recorded. All chipmunks whose fecal samples were examined were in apparently good health at the time of sampling.
DNA extraction and PCR amplification
All fecal specimens were washed three times by centrifugation at 1500× g for 10 min with distilled water. Genomic DNA was extracted from approximately 200 mg of each processed fecal specimen using an E.Z.N.A.R® Stool DNA kit (Omega Biotek Inc., Norcross, GA, USA) according to the manufacturer’s instructions. Extracted DNA was stored at -20 °C until molecular analysis.
Giardia duodenalis prevalence and assemblages were first determined by nested PCR amplification of approximately 550 bp fragment of the beta giardin (bg) gene. Furthermore, bg-positive specimens were also analyzed by PCR amplification of the glutamate dehydrogenase (gdh) and triosephosphate isomerase (tpi) genes. PCR amplification primers and annealing temperatures in this study (Table 1) were as previously reported [21]. PCR products were visualized by electrophoresis in 1.5% agarose containing ethidium bromide.
Table 1.
Gene | Primer | Sequence (5'-3') | Annealing temperature (°C) | Fragment length (bp) | Reference |
---|---|---|---|---|---|
bg | F1 | AAGCCCGACGACCTCACCCGCAGTGC | 65 | 530 | [21] |
R1 | GAGGCCGCCCTGGATCTTCGAGACGAC | ||||
F2 | GAGGCCGCCCTGGATCTTCGAGACGAC | 65 | |||
R2 | CATAACGACGCCATCGCGGCTCTCAGGAA | ||||
tpi | F1 | AAATIATGCCTGCTCGTCG | 50 | 530 | [21] |
R1 | CAAACCTTITCCGCAAACC | ||||
F2 | CCCTTCATCGGIGGTAACTT | 50 | |||
R2 | GTGGCCACCACICCCGTGCC | ||||
gdh | F1 | TTCCGTRTYCAGTACAACTC | 50 | 511 | [21] |
R1 | ACCTCGTTCTGRGTGGCGCA | ||||
F2 | ATGACYGAGCTYCAGAGGCACGT | 50 | |||
R2 | GTGGCGCARGGCATGATGCA |
Sequence and phylogenetic analyses
All amplified products were sent to Life Technologies (Guangzhou, China) for sequencing on an ABI 3730 DNA Analyzer (Applied Biosystems, Foster City, CA, USA) using the BigDye® Terminator v3.1 cycle sequencing kit. Nucleotide sequence accuracy was confirmed by sequencing two separate PCR products. Assemblages and subtypes were identified by aligning nucleotide sequences with known reference tpi, gdh and bg gene sequences of G. duodenalis available in GenBank using BLAST (http://www.ncbi.nlm.nih.gov/BLAST/).
A phylogenetic analysis was performed by constructing a neighbor-joining tree using Mega 6 software [12], based on the evolutionary distances calculated by a Kimura 2-parameter model. The reliability of these trees was assessed using bootstrap analysis with 1000 replicates.
Results and discussion
The present study identified 24 (8.6%, 95% CI: 0.053–0.119%) fecal samples that were G. duodenalis-positive by PCR analysis of the bg gene. In China, the prevalence of giardiasis varies from 1.9% [22] to 27.1% [11] in pets by PCRs. In Heilongjiang Province, the rates of infection with G. duodenalis in pet cats and dogs were 1.9 and 4.5%, respectively [22]. In Guangzhou, 11% of fecal samples form pet dogs were positive for G. duodenalis [23]. The prevalence of G. duodenalis in pet dogs in Henan Province was 12.4% [14]. In Niaoning Province, the infection rate of G. duodenalis in farm dogs was 13.2% [24]. In Shanghai, Hualiu et al. [25] reported that G. duodenalis was found in 26.67 and 9.26% of samples from pets and zoo animals, respectively. The infection rate of G. duodenalis in pet chinchillas was 27.1% in four different cities in China [11]. The variability of G. duodenalis prevalence in China may be explained by the differences in geographical location, climate, age and gender of the animals, management system, and the diagnostic method.
The genetic diversity of G. duodenalis-positive samples was observed by sequencing the bg, tpi and gdh genes. A total of 24, 17 and 17 sequences were obtained for the three gene loci, respectively (Table 2). Analysis of the bg gene identified 13 sequences as belonging to assemblage A (9 subtype AI and 4 subtype AI-1) and 11 to assemblage G (7 subtype GI and 4 subtype GII). The subtype AI sequence (MF671918) was identical to the known assemblage AI sequences: accession no. KR051224 (from tortoise in China) and accession no. GQ329671 (from human in Sweden [26]). The subtype AI-1 sequence (MF671917) had one single nucleotide polymorphism (SNP) when compared to sequence KR051224 (Table 3). The subtype GI sequence (MF671919) was identical to sequence EU769221 (from Rattus norvegicus in Sweden), whereas the subtype GII sequence had two SNPs (at position 97 G/A, and at position 325 A/C) in comparison with sequence EU769221. Among 17 samples positive for the tpi gene, 13 sequences were identified as assemblage A (5 subtype AI and 8 subtype AV) and 4 were identified as assemblage G (2 subtype GI and 2 subtype GII). The genetic characterization is presented in Table 3. Subtype GII sequence (MF671913) was identical to sequence EU781013 (from Rattus norvegicus in Sweden), whereas subtype GI sequence had one SNP (at position 184 C/T) in comparison with sequence EU781013. Out of 17 samples positive for the gdh gene, 10 sequences were identified as belonging to assemblage A (7 subtype AI and 3 novel subtypes AI-1) and 7 were identified as belonging to assemblage G. The novel subtype AI-1 sequence had not been reported previously; it had 5 SNPs when compared with sequence KR075940 (from sheep in China [27]) (Table 3). Assemblage G sequence was identical to sequence AY178748 (from mouse in Australia). The phylogenetic trees based on bg, gdh and tpi are presented in Additional file 2: Figure S1.
Table 2.
Chipmunk ID | Assemblage | GenBank ID | MLG type (n) | ||
---|---|---|---|---|---|
bg | tpi | gdh | |||
CD26, CD27 | GI | GI | G | MF671919, MF671914, MF671912 | MLG G1 (2) |
CD28 | GI | GII | G | MF671919, MF671913, MF671912 | MLG G2 (1) |
CD79 | GII | GII | G | MF671920, MF671913, MF671912 | MLG G3 (1) |
CD29, CD34, CD69 | AI | AV | AI-1 | MF671918, MF671915, MF671910 | MLG A1 (3) |
CD60, CD119 | AI | AI | AI | MF671918, MF671916, MF671911 | MLG A2 (2) |
CD61, CD96, CD124, CD144 | AI-1 | AV | AI | MF671917, MF671915, MF671911 | MLG A3 (4) |
CD64 | AI | AV | AI | MF671918, MF671915, MF671911 | MLG A4 (1) |
CD74, CD92, CD186 | AI | AI | Neg | MF671918, MF671916, – | – |
CD81, CD203, CD211 | GII | Neg | Neg | MF671920, –, – | – |
CD22, CD44, CD102 | GI | Neg | G | MF671919, –, MF671912 | – |
CD23 | GI | Neg | Neg | MF671919, –, – | – |
Abbreviations: Neg no genotype determined; – GenBank accession numbers not available
Table 3.
Subtype | GenBank ID | Gene | Nucleotide at position | |||||
---|---|---|---|---|---|---|---|---|
74 | 248 | 275 | 287 | 443 | 469 | |||
AI (Ref.) | KR051224 | bg | A | A | C | A | A | T |
AI | MF671918 | bg | A | A | C | A | A | T |
AI-1 | MF671917 | bg | A | A | C | C | A | T |
AI (Ref.) | EU014517 | tpi | C | A | A | A | C | G |
AI | MF671916 | tpi | C | A | A | A | C | G |
AV (Ref.) | KP780973 | tpi | C | T | C | G | A | T |
AV | MF671915 | tpi | C | T | C | G | A | T |
AI (Ref.) | KR075940 | gdh | C | T | G | G | C | A |
AI | MF671911 | gdh | C | T | G | G | C | A |
AI-1 | MF671910 | gdh | T | C | A | G | T | C |
In the present study, assemblage A sequences were more prevalent than assemblage G sequences, and no mixed assemblage A and G infections were detected. This result is consistent with data from previous studies in pets in China and Mexico [24, 28]. Thus far, assemblages A-C, E and G have been identified in rodents worldwide, and nearly all tested samples contained at least either assemblage A or B [12, 13]. Subtyping assemblage A sequences at different loci has revealed three sub-assemblages: AI, AII, and AIII. In China, sub-assemblage AI has been detected in a variety of hosts, including humans, cattle, goat, sheep, dogs, cats and pigs [7]. Sub-assemblage AII has also been identified in humans in China. Cross-species transmission of G. duodenalis assemblage AI in Mexico and in Brazil has been recently reported [28, 29]. This finding suggests that chipmunks infected with assemblage AI were probably the source of human giardiasis due to frequent contact of the two species in that specific area. However, the generalization of this proposal requires systematic, molecular epidemiological investigations in humans and animals in other geographical areas. Recently, the multilocus genotype (MLG) model has been widely used to better understand the characteristics of G. duodenalis in different hosts and to assess its zoonotic potential [30, 31]. In this study, 14 samples were successfully sequenced at all three gene loci, and were characterized as four assemblage A MLGs and three different assemblage G MLGs (Table 2).
Conclusions
In the present study, for the first time, we described the rates of infection with G. duodenalis of pet chipmunks in Sichuan province of southwestern China and demonstrated the prevalence of assemblages A and G. On the basis of the multilocus sequence analysis, four assemblage A MLGs and three assemblage G MLGs were identified. Because assemblage A G. duodenalis is known to be zoonotic and has been identified in humans in China, pet chipmunks infected with assemblage A constitute a potential zoonotic risk to humans.
Additional files
Acknowledgements
We would like to thank Qicheng Xiao and Rui Tu for collecting samples.
Funding
The study was supported financially by the National Science and Technology Department “13th five-year” Special Subproject of China (No. 2016YFD0501009) and the Chengdu Giant Panda Breeding Research Foundation (CPF2015-09; CPF2015-07).
Availability of data and materials
Representatives of all the nucleotide sequences generated in this study have been deposited in GenBank under the accession numbers MF671910-MF671920.
Abbreviations
- bg
β-giardin
- tpi
Triosephosphate isomerase
- gdh
Glutamate dehydrogenase
- MLGs
Multilocus genotype
- SNP
Single nucleotide polymorphism
Authors’ contributions
GP and LD conceived and designed the experiments. RL, HL, YC, ZZ1 (Ziyao Zhou) and LY collected samples. Experiments were performed by LD, WW, HF, LL and ZZ2 (Zhijun Zhong), and the data were analyzed by LD, HF and SC. The manuscript was written by LD. All authors read and approved the final manuscript.
Ethics approval
The present study protocol was reviewed and approved by the Research Ethics Committee and the Animal Ethical Committee of Sichuan Agricultural University. Permission was obtained from the shop owners before the fecal specimens were collected.
Consent for publication
Not applicable.
Competing interests
The authors declare that they have no competing interests.
Publisher’s Note
Springer Nature remains neutral with regard to jurisdictional claims in published maps and institutional affiliations.
Footnotes
Electronic supplementary material
The online version of this article (10.1186/s13071-018-2790-z) contains supplementary material, which is available to authorized users.
Contributor Information
Lei Deng, Email: cdl931023@163.com.
Run Luo, Email: 824312202@qq.com.
Haifeng Liu, Email: 121699596@qq.com.
Ziyao Zhou, Email: 83954903@qq.com.
Lingyu Li, Email: 1905759345@qq.com.
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Wuyou Wang, Email: 1119872251@qq.com.
Hualin Fu, Email: fuhl2005@sohu.com.
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Guangneng Peng, Email: pgn.sicau@163.com.
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Associated Data
This section collects any data citations, data availability statements, or supplementary materials included in this article.
Supplementary Materials
Data Availability Statement
Representatives of all the nucleotide sequences generated in this study have been deposited in GenBank under the accession numbers MF671910-MF671920.