Background
Acanthamoeba species are widely distributed in the environment: their habitats include soil, freshwater, seawater, dust, and putrilage. Some
Acanthamoeba species can cause keratitis, granulomatous amoebic encephalitis (GAE), pulmonary infections, cutaneous lesions, rhinosinusitis, osteomyelitis, or diffuse inflammation [
1‐
3].
Acanthamoeba keratitis can lead to scarring of the cornea, resulting in a permanent visual impairment or complete blindness. GAE is a central nervous system disease that usually occurs in immunocompromised patients, such as those with acquired immune deficiency syndrome, systemic lupus erythematosus, and transplanted organ, or those undergoing chemotherapy for cancer. Nonetheless, several cases of GAE and skin infection due to
Acanthamoeba spp. have been reported in immunocompetent individuals [
4‐
8].
Eye infections have been reported to be caused by
Acanthamoeba castellanii,
Acanthamoeba polyphaga,
Acanthamoeba rhysodes,
Acanthamoeba culbertsoni,
Acanthamoeba lugdunensis,
Acanthamoeba griffini,
Acanthamoeba hatchetti,
Acanthamoeba quina,
Acanthamoeba lenticulata, and
Acanthamoeba triangularis. Central nervous system diseases have been caused by
A. castellanii,
A. culbertsoni,
Acanthamoeba astronyxis,
A. rhysodes,
Acanthamoeba healyi, and
A. lenticulata [
6,
9‐
13].
There have been few reports of
Acanthamoeba spp. isolated from environmental samples in China [
14]. In this study, we report the molecular biological characterization of four strains of
Acanthamoeba (CJY/S1, CJY/S2, CJY/S3, and CJY/W1) isolated from soil and tap water in China. We identified these species by using mitochondrial DNA restriction fragment length polymorphism (mtDNA RFLP) analysis and 18S rDNA sequence alignment. We found that the three strains isolated from the soil belonged to the morphological group II and had genotypes T4 and T5, whereas the strain isolated from tap water belonged to the morphological group II and had genotype T16.
Methods
Isolation and cultivation of Acanthamoeba
Samples of soil and tap water were collected in Yanji, China. The samples were loaded onto 1.5% agar plates covered with heat-inactivated (60 °C for 1 h) Escherichia coli (American Type Culture Collection, ATCC 25922, free of plasmid). The plates were incubated at 25 °C, and growth of Acanthamoeba was observed under an inverted microscope on a daily basis for 1 week. Each cyst isolated with a glass capillary was inoculated on a new agar plate and incubated for 1 week. For axenization, a piece of agar (1 cm × 1 cm) covered with cysts was treated with 0.1 N HCl for 24 h, washed three times with sterile water, placed in peptone yeast glucose medium (10 g proteose peptone, 10 g yeast extract, 10 mL of 50% glucose, 10 mL of 0.5 M Na2HPO4, and 10 mL of 0.5 M K2HPO4 in 970 mL of sterile water), and incubated at 25 °C for 3 weeks. When most of the amoebae reached trophozoite stage, they were harvested and washed three times with phosphate-buffered saline.
Morphological examination
A cyst formed on the monoxenic plate was picked with a sterilized inoculating loop and transferred to a glass slide with a drop of sterile distilled water. The slide was then covered with a coverslip. Fifty cysts per plate were observed and measured under a Nomarski (differential interference contrast) microscope (Olympus, Japan).
Analysis of 18S rDNA sequences
Genomic DNA was extracted using phenol/chloroform method. The 18S rRNA gene was amplified using the following primers by Xuan et al. [
13]: forward, 5′-CCGAATTCGTCGACAACCTGGTTGATCCTGCCAGT-3′; reverse, 5′-GGATCCAAGCTTGATCCTTCTGCAGGTTCACCTAC-3′. The amplified products were resolved by electrophoresis, recovered from the gel, and ligated into a T/A cloning vector (pGEM-T Easy Vector System I, Promega, USA) for subsequent transformation of
E. coli. Positive clones were picked, and recombinant plasmid DNA was extracted using the Wizard® Plus Minipreps DNA Purification System (Promega, USA). Plasmids with inserts of the correct size were identified by
EcoRI digestion and sequenced. The obtained final 18S ribosomal DNA (rDNA) sequences of the
Acanthamoeba strains were deposited in GenBank (accession nos. KY827389–KY827392). The sequences were then compared with those of other
Acanthamoeba sequences in GenBank using the Basic Local Alignment Search Tool (BLAST) search engine. Clustal X and GeneDoc were used for pairwise alignment and calculation of percent sequence dissimilarity. Phylogenetic analyses were performed, and the phylogenetic tree was drawn using the neighbor-joining (NJ) method with MEGA3 [
15]. The reference strains of
Acanthamoeba and the GenBank accession numbers of the 18S rDNA sequences used in this study are as follows:
A. castellanii CDC:0981:V006 (T1), U07400;
Acanthamoeba palestinensis (T2), U07411;
A. griffini H37 (T3), S81337;
A. castellanii Neff (T4), U07416;
A. lenticulata E18-2 (T5), U94735;
A. palestinensis 2802 (T6), AF019063;
A. astronyxis R&H (T7), AF019064;
Acanthamoeba tubiashi OC-15C (T8), AF019065;
Acanthamoeba comandoni Pussard (T9), AF019066;
A. culbertsoni A-1 (T10), AF019067;
A. hatchetti BH-2 (T11), AF019068;
A. healyi OC-3A (T12), AF019070;
Acanthamoeba sp. UWC9 (T13), AF132134;
Acanthamoeba sp. PN13 (T14), AF333609;
Acanthamoeba jacobsi ATCC 30732 (T15), AY262360;
Acanthamoeba sp. U/H-C1 (T16), AY026245;
Acanthamoeba sp. E1a (T17), GU808277;
Acanthamoeba byersi CDC:V621 (T18), KC822464;
Acanthamoeba micheli BRO-2 (T19), KP711387; and
Acanthamoeba sp. OSU 04-020 (T20), DQ451161.
Extraction of mtDNA and RFLP analysis
mtDNA of
Acanthamoeba isolates was extracted using the method described by Yagita and Endo [
16]. Briefly, amoebae were harvested and washed in cold phosphate-buffered saline, treated with TEG buffer (25 mM Tris–HCl, 10 mM ethylenediaminetetraacetic acid (EDTA), 50 mM glucose, pH 8.0), lysed with a fresh solution of 1% sodium dodecyl sulfate in 0.2 N NaOH and potassium acetate buffer, and left on ice for 30 min. mtDNA was then extracted with a phenol/chloroform mixture (1:1) and recovered by the precipitation with cold absolute ethanol in the presence of sodium acetate. The extracted mtDNA was then digested with
EcoRI at 37 °C. The digested mtDNA was electrophoresed in 0.7% agarose gel and stained with ethidium bromide. The mtDNA RFLP patterns were observed and photographed.
Discussion
There are many species of free-living amoebae. Some, such as
Acanthamoeba spp.,
Naegleria spp.,
Hartmannella spp., or
Balamuthia mandrillaris, are opportunists that can cause infections in humans and animals [
18,
19].
Naegleria and
Acanthamoeba species have been identified as causes of serious human infections. Some species of
Acanthamoeba can cause amoebic keratitis, particularly in contact lens wearers and immunocompromised individuals experiencing subacute or chronic central nervous system infections [
20,
21].
Eighteen species of
Acanthamoeba have been classified into three groups according to the shape and size of cysts. Species in group I are nonpathogenic except
A. astronyxis,
A. byersi and
A. comandoni [
22,
23]. Most of the pathogenic
Acanthamoeba species belong to group II. Species in group III, such as
A. culbertsoni,
A. healyi, and
A. lenticulata, often cause infections of the brain. The cyst morphology of the four isolates characterized in this study resembled that of various species within morphological group II. However, the classification of
Acanthamoeba spp. based on morphological characteristics has proven to be unreliable. The morphology of
Acanthamoeba spp. may change depending on culture conditions. Furthermore, different
Acanthamoeba species in the same group can have similar morphology, and
Acanthamoeba cysts of two species may show only transient differences, thereby causing difficulties in the identification of the species.
Lass et al. reported partial sequences of T4 strains in environmental samples in China recently [
14], which is different from our data which is full of 18S sequences of four distinct genotypes of isolated strains. At present, sequence analysis of genomic DNA is considered the method of choice for identifying species of
Acanthamoeba. Sequence analysis of 18S rRNA genes is frequently used.
Based on the nucleotide sequence of 18S rDNA,
Acanthamoeba was initially clustered into 12 genotypes, from T1 to T12 [
12,
24]. Recently, new genotypes of
Acanthamoeba have been identified [
25‐
29]. Five genotypes of
Acanthamoeba are associated with keratitis: T4 is the primary genotype and T3 is the secondary genotype, whereas
Acanthamoeba species of the remaining genotypes (T5, T6, and T2) are considered to be rare causes of this disease. Gast [
28] reported that sequence differences among 15 strains of
Acanthamoeba within genotype T4 were in the range of 0–4%, whereas sequence differences among genotypes were 6–12%.
In this study, the full-length 18S rRNA genes from the
Acanthamoeba sp. strains CJY/S1, CJY/S2, CJY/S3, and CJY/W1, isolated from soil and tap water of Yanji, China, were determined to be 2255, 2252, 2292, and 2252 bp, respectively. These lengths are close to the range of 2300–2700 bp reported by Stothard et al. [
12]. The 18S rDNA sequences of the
Acanthamoeba sp. strains CJY/S1, CJY/S2, CJY/S3, and CJY/W1 were compared with those of reference strains of genotypes T1–T20, which were obtained from GenBank by using BLAST searches. Pairwise alignment and calculation of the percent sequence dissimilarity using Clustal X and GeneDoc showed that
Acanthamoeba sp. strains CJY/S1 and CJY/S2 had genotype T4, which encompasses the majority of clinical and environmental isolates of
Acanthamoeba. In a phylogenetic tree based on the 18S rDNA sequence,
Acanthamoeba CJY/S3 strain was positioned close to genotype T5 species and was related to
A. lenticulata. The
Acanthamoeba sp. strains CJY/S1 and CJY/S2 showed extremely similar mtDNA RFLP patterns.
Acanthamoeba sp. CJY/W1 had genotype T16 and was closely related to
Acanthamoeba sp. U/H-C1 (99%) and
Acanthamoeba sp. UWC9 (95%) [
30].
Acanthamoeba sp. CJY/W1, isolated from tap water, had a mtDNA RFLP pattern different from those of the
Acanthamoeba sp. strains CJY/S1, CJY/S2, and CJY/S3, which were isolated from soil.
Recent studies have shown that A. castellanii (genotype T4) and A. lenticulata (genotype T5) can infect the cornea and central nervous system in humans, but there are insufficient reports pertaining to strains of genotype T16. Further research is required to determine whether the Acanthamoeba sp. strains CJY/S1, CJY/S2, CJY/S3, and CJY/W1 isolated by us from environmental samples could be pathogenic to humans and animals.
Conclusions
Strains CJY/S1 and CJY/S2, isolated from soil, had similar mtDNA RFLP patterns, whereas strain CJY/W1, isolated from tap water, displayed a different pattern. To the best of our knowledge, this is the first report on the identification of genotypes T4, T5, and T16 from environmental sources in Yanji, China.