Anaplasma spp. and Ehrlichia spp. are tick-transmitted bacteria that are of significant economic importance as they can infect large and small ruminants and also people. There is little information on anaplasmosis and ehrlichiosis in ruminants in China. 16S rRNA FRET-qPCRs were used to screen convenience whole blood samples from 2,240 domestic ruminants in 12 provinces of China for Anaplasma spp. and Ehrlichia spp. Positive samples were further analyzed with a standard PCR for the gltA. Anaplasma spp. DNA was detected in the sheep (11.7%; 13/111), goats (81.8%; 219/270), cattle (13.2%; 241/1,830), and water buffaloes (6.9%; 2/29). Ehrlichia spp. DNA was detected in sheep (1.8%; 2/111), goats (1.1%; 3/270), and cattle (3.6%; 65/1830) but not in water buffaloes (0/29). Sequencing of gltA PCR products showed that A. marginale, A. ovis, Ehrlichia canis, and Ehrlichia sp. (JX629807) were present in ruminants from China, while the 16S rRNA FRET-qPCR sequence data indicated that there might also be A. platys, A. phagocytophilum, Anaplasma sp. BL126-13 (KJ410243), and Anaplasma sp. JC3-6 (KM227012). Our study shows that domestic ruminants from China are not uncommonly infected with a variety of Anaplasma spp. and Ehrlichia spp.
National Natural Science Foundation of China3127257532472225Priority Academic Program Development of Jiangsu Higher Education Institutions1. Background
Anaplasma spp. and Ehrlichia spp. are tick-transmitted, intracellular Gram-negative bacteria that are important animal and human pathogens. The major Anaplasma species that impact animal and human health are Anaplasma marginale, A. ovis, A. centrale, A. bovis, A. phagocytophilum, and A. platys [1]. The most important of these in ruminants is A. marginale which causes bovine anaplasmosis (formerly gall-sickness) which is associated with fever, anemia, icterus, and often death. The major pathogenic Ehrlichia species are E. canis, E. chaffeensis, E. ewingii, E. muris, and E. ruminantium [2] with the latter causing heartwater in domestic ruminants. This disease is prevalent in Africa, where it causes high mortality (up to 90%) and extensive economic losses [3].
In China, there is little information on the Anaplasma and Ehrlichia species in domestic ruminants. Anaplasma bovis, A. marginale, and A. ovis have been described in various Provinces, including Xinjiang, Gansu, Henan, Yunnan, Hubei, Guizhou, and Zhejiang [1, 4–7]. In addition, A. phagocytophilum has been reported in ruminants (sheep and cattle) in Henan and Xinjiang as well as in dogs and ticks [1, 6–14], and A. platys has been detected in red deer and sika deer from Gansu province [4]. In the case of Ehrlichia spp. in ruminants in China, an unclassified species has been reported in cattle in Tibet [15] and E. canis, a species that infects dogs worldwide, has been reported in sika deer from Gansu [4].
To provide further information on Anaplasma spp. and Ehrlichia spp. infections in domestic ruminants of China, we carried out a PCR survey for the organisms in blood samples from ruminants in 12 provinces of China. Our findings are reported below.
2. Materials and Methods2.1. Blood Samples
This study was reviewed and approved by the Institutional Animal Care and Use Committee of Yangzhou University and animal owners gave written permissions for blood collection.
Between 2007 and 2013, convenience whole blood samples (around 6 mL) from cattle (n=1,830), water buffaloes (n=29), goats (n=270), and sheep (n=111) were collected in 12 provinces/municipalities of China as described before [16, 17] (Table 1). DNA was extracted from the whole blood samples using a standard phenol-chloroform method as described previously [16] and stored at −80°C until PCRs were performed.
Molecular detection of Anaplasma spp. and Ehrlichia spp. in Chinese ruminants.
Animal species
Subspecies/breed
Province
City
Anaplasma positivity
Ehrlichia positivity
Positive/total, %
Positive/total, %
Cattle (n=1,830)
Bos p. taurus
Holsteins
Anhui
Bengbu
3/109, 2.8%
1/109, 0.9%
Wannan
Anhui
Wuhu
17/17, 100.0%
14/17, 82.4%
Holsteins
Beijing
Sanyuan
0/107, 0.0%
0/107, 0.0%
Holsteins
Jiangsu
Yancheng
1/395, 0.3%
2/395, 0.5%
Holsteins
Jiangsu
Yangzhou
0/269, 0.0%
1/269, 0.4%
Holsteins
Heilongjiang
Qiqihar
1/111, 0.9%
0/111, 0.0%
Simmentals
Inner Mongolia
Chifeng
0/132, 0.0%
0/132, 0.0%
Luxi
Shandong
Jining
3/42, 7.1%
0/42, 0.0%
Bohaiblack
Shandong
Binzhou
1/33, 3.0%
0/33, 0.0%
Holsteins
Shanghai
Shanghai
0/255, 0.0%
0/255, 0.0%
Holsteins
Tianjin
Tianjin
0/94, 0.0%
0/94, 0.0%
Cattle (n=1,830)
Bos p. indicus
Minnan
Fujian
Putian
17/24, 70.8%
2/24, 8.3%
Leiqiong
Hainan
Haikou
74/74, 100.0%
15/74, 20.3%
Yunling
Yunnan
Kunming
124/168, 73.8%
30/168, 17.9%
Water buffalo (n=29)
Haizi
Jiangsu
Yancheng
2/29, 6.9%
0/29, 0.0%
Goats (n=270)
Yangtze River Delta White
Jiangsu
Yangzhou
119/172, 69.2%
3/172, 1.7%
Xinjiang
Xinjiang
Urumqi
10/98, 10.2%
0/98, 0.0%
Sheep (n=111)
Sishui Fur
Inner Mongolia
Xilingol
0/72, 0.0%
1/72, 1.4%
Wuranke
Shandong
Jining
13/39, 33.3%
1/39, 2.6%
2.2. FRET-qPCR
As described previously, FRET-qPCRs for the 16S rRNA of Anaplasma spp. [18] and Ehrlichia spp. [19], and the mammalian HMBS gene [20] as an endogenous internal control, were performed on a Roche Light-Cycler 480-II PCR Instrument. Positive PCR products were verified by gel electrophoresis and sequenced using forward and antisense primers (BGI, Shanghai, China). Negative controls consisting of sterile molecular grade water were used to detect cross-contamination during DNA extraction and PCR processing.
2.3. Standard PCR for the Citrate Synthase Gene (gltA)
To further characterize the Anaplasma and Ehrlichia species detected above, we carried out standard PCRs for the citrate synthase gene (gltA) of Anaplasma spp. as described previously [21] and for Ehrlichia spp. with primers designed for the study (forward primer: GGTTTATGGTGCTTTTCCTAGTGTTGA; reverse primer: TTACAGATTTCTCAGGAGTATATGCCTCC). The PCR products we obtained were verified by gel electrophoresis and sequenced (BGI, Shanghai, China).
2.4. DNA Sequence Data Analysis
Compilation and assembly of the multiple sequences generated from each template were performed using the Vector NTI. Sequence alignment was performed with Align (Vector NTI).
3. Results
The mammalian HMBS gene endogenous internal control was positive for all samples, indicating that DNA extraction had been successful.
3.1. Anaplasma spp. DNA in Ruminants
Overall, 17.2% (385/2240) of the ruminants from 8 of the 12 provinces studied (Table 1 and Figure 1) were positive for the 16S rRNA of Anaplasma spp. with copy numbers ranging from 50 to 52,000/mL blood (median 1,720 copies/mL blood). Goats were most frequently positive (81.1%; 219/270), followed by cattle (13.2%; 241/1,830), sheep (11.7%; 13/111), and water buffaloes (6.9%; 2/29).
Detection of Anaplasma spp. and Ehrlichia spp. in ruminants from 12 provinces of China. Blood samples of ruminants (2,240) were collected from twelve provinces (in bisque) of China. The prevalence is shown for Anaplasma spp. (red) and Ehrlichia spp. (blue).
When we sequenced the positive 16S rRNA FRET-qPCRs, we obtained clean sequencing data for 38 of the samples from cattle (23) and goats (15) (Table 2). The sequences in the cattle were most commonly identical to those of A. phagocytophilum (12/23; 52%) and A. marginale (10/23; 44%) with positive animals in 4 and 2 of the 9 provinces studied, respectively. Representative sequences were deposited in GenBank for A. phagocytophilum (KX279691) and A. marginale (KX279690). The one other Anaplasma sp. found was in a Wannan cow from Anhui which had a 16S RNA sequence identical to that of a poorly characterized Anaplasma sp. BL126-13 (KJ410243). We also found evidence for this organism in three goats from Jiangsu. Other Anaplasma spp. we detected in goats were A. ovis (KX279688) in Xinjiang (2), A. platys (KX279689) in Jiangsu (2), and a poorly characterized Anaplasma sp. (KM227012) in Jiangsu (5). The 16S rRNA sequences we deposited in GenBank (KX279683; KX279685) are identical to those of Anaplasma sp. (KM227012) and Anaplasma BL126-13 (KJ410243), respectively.
Source of Anaplasma and Ehrlichia spp. identified in this study based on 16S rRNA and gltA gene sequences.
Organism
Species
16S RNA
Species
gltA
GenBank #
Numbers
Animal
City, province
GenBank #
Numbers
Animal
City, province
Anaplasma spp.
A. marginale
KX279690
10
Cattle
Binzhou, Shandong (1)
A. marginale
KX506005
1
Cattle
Kunming, Yunnan
Kunming, Yunnan (9)
A. platys
KX279689
2
Goat
Yangzhou, Jiangsu
A. phagocytophilum
KX279691
15
Cattle
Bengbu, Anhui (2)
Haikou, Hainan (5)
Kunming, Yunnan (4)
Wuhu, Anhui (1)
Goat
Yangzhou, Jiangsu (3)
A. ovis
KX279688
2
Goat
Urumqi, Xinjiang (2)
A. ovis
KX506006
1
Goat
Urumqi, Xinjiang
Anaplasma sp.
KX279685
4
Cattle
Wuhu, Anhui (1)
Goat
Yangzhou, Jiangsu (3)
Anaplasma sp.
KX279683
5
Goat
Yangzhou, Jiangsu (5)
Ehrlichia spp.
Ehrlichia sp.
KX279682
14
Sheep
Inner Mongolia (1)
Cattle
Yunnan, Kunming (10)
Ehrlichia sp.
KX506007
5
Cattle
Yunnan, Kunming
Goat
Yangzhou, Jiangsu (3)
E. canis
KX506008
1
Goat
Yangzhou, Jiangsu
Since there is limited polymorphism in the 16S rRNA FRET-qPCR sequences of different ruminant Anaplasma spp. (Figure 2), to enable more definitive species differentiation we carried out a PCR and sequencing of the more polymorphic gltA on 20% of the 16S rRNA positive samples with the highest copy numbers (range of 610 to 52,000/mL blood; median 2,300). Only two samples provided clean sequencing data with one (16S rRNA FRET-qPCR copy number 52,000/mL blood) from a bovine in Yunnan having 100% identity with A. marginale (0/620 mismatches with CP006847.1) and the other (16S rRNA FRET-qPCR copy number 47,700 copies/mL blood) from a goat in Xinjiang having 99.7% identity with A. ovis (1/438 mismatches with KJ410284.1). The gltA sequence of A. marginale we identified was deposited in GenBank under the accession number KX506005 and that of A. ovis as KX506006. The 16S rRNA sequences for Anaplasma spp. from ruminants in this study are compared with those of other representing Anaplasma spp. (Figure 3).
Alignment of the sequences obtained with the 16S rRNA FRET-qPCR we used in our study and those of Anaplasma spp. in GenBank. “.” denotes the identical nucleotide sequence to that of A. bovis. Organisms with GenBank accession numbers identified in the study are in red.
Phylogenetic comparison of Anaplasma spp. from ruminants in this study. The 16S rRNA sequences (in red font and accession number) are compared with those of other representing Anaplasma spp. (in black font and accession number). Branch lengths are measured in nucleotide substitutions and numbers show branching percentages in bootstrap replicate. Scale bar represents the percent sequence diversity.
3.2. Ehrlichia spp. DNA in Ruminants
A total of 70 animals (70/2,240, 3.1%) were positive for DNA of Ehrlichia spp. in our 16S rRNA FRET-qPCR with copy numbers varying from 50 to 42,900/mL blood (median 5,100). Cattle were most frequently positive (3.6%, 65/1,830) followed by goats (1.1%, 3/270) and sheep (1.8%, 2/111). None of the water buffaloes (29) were positive. We found Ehrlichia sp. positive animals in over half (7/12) the provinces we studied with the highest prevalence in Wuhu (82.4%, 14/17) of Anhui province and lower prevalence in the tropical provinces in the south of China, mainly Hainan (20.3%, 15/74), Yunnan (17.9%, 30/168), and Fujian (8.3%, 2/24). No positive animals were detected from the more northern provinces of Beijing, Shanghai, Heilongjiang, and Tianjin (Table 1; Figure 1).
Standard PCR and sequencing of the gltA were performed on samples positive in the FRET-qPCR for 16S rRNA with higher copy numbers, namely, those between 14,400 and 42,900/mL blood (median 16,700). Useable gltA sequences were obtained for six of the animals studied (copy numbers 33,100 to 42,900/mL blood, mean 37,600) showing five, all cattle from Yunnan, to be infected with an Ehrlichia sp. having an identical sequence (563/563; 100%) to that of a new species closely related to E. canis and found in Rhipicephalus microplus in the Czech republic (JX629807) [22]. The remaining animal, a goat from Jiangsu, was found to be infected with E. canis having a sequence almost identical (549/563; 98%) to that of E. canis (Oklahoma strain; AF304143) [23] and a strain found in a dog in Thailand (KJ459920) [24].
The gltA sequence of E. canis we identified was deposited in GenBank under the accession number KX506008 and that of a representative of the Ehrlichia sp. (JX629807) as KX506006. The gltA sequences for Ehrlichia spp. from ruminants in this study are compared with those of other representing Ehrlichia spp. (Figure 4).
Phylogenetic comparison of Ehrlichia spp. from ruminants in this study. The gltA sequences (in red font and accession number) are compared with those of other representing Ehrlichia spp. (in black font and accession number). Branch lengths are measured in nucleotide substitutions and numbers show branching percentages in bootstrap replicate. Scale bar represents the percent sequence diversity.
4. Discussion
Our results are consistent with other PCR studies from China [1, 6–10, 12, 13] showing that domestic ruminants from the country are infected with a range of Anaplasma and Ehrlichia spp. Differences in the prevalence of animals on the farms we studied were most likely due to differing husbandry practices and tick exposure, with dairy animals and water buffaloes raised intensively having the lowest levels of positivity. Also, although our sample numbers were small, our results indicate that ruminants are generally more commonly infected with Anaplasma and Ehrlichia spp. in the more southern provinces (Yunnan and Hainan) and along the seaboard (Fujian, Anhui, and Jiangsu) where there are more tropical conditions and tick vectors are expected to be more prevalent. Lower prevalence was found in the cooler northern provinces (Heilongjiang, Beijing, Inner Mongolia, and Xinjiang).
Although we obtained relatively large numbers of animals positive by FRET-qPCR for the 16S rRNA of Anaplasma spp., we were only able to amplify a small number of these with the gltA primers. We presume this was because of low parasitemia in affected animals and different numbers of target sequences for the PCRs [25], since we could only amplify the gltA from animals with high copy numbers in the 16S rRNA FRET-qPCR. It might also, however, have been because of different sensitivities of the PCRs we used as has been described before with molecular detection of different genes in Anaplasma spp. [10, 25, 26].
The one Anaplasma we definitively identified with the gltA PCR was A. marginale which is the agent of bovine anaplasmosis, a very common disease of cattle around the world in tropical and subtropical countries [27]. Infections are mainly transmitted by Rhipicephalus microplus and although most infections are subclinical, there can be fever and severe anemia resulting in production losses from decreased milk production and abortion. Studies in China have shown that the organism can be found in Rhipicephalus (Boophilus) microplus [28] and also that the organism might be transmitted by Hyalomma asiaticum [5]. The organism appears to be widespread in domestic ruminants in China and it has been reported to be a relatively common infection of cattle in southern and northern China [5, 15, 29, 30].
The other Anaplasma we definitively identified, A. ovis, has also been reported previously in China in goats (15%) from central and southern China [1] and in sheep and goats (41%) in Henan and Xinjiang [6, 7]. This organism is the agent of ovine anaplasmosis which can be transmitted by Dermacentor nuttalli, Hyalomma asiaticum kozlovi, and Rhipicephalus pumilio in China where infections mostly result in subclinical anemia in indigenous animals [31]. Recently, the organism has been shown to infect humans [32] as has a closely related organism in China, putatively named “Anaplasma capra” [33].
Although we were not able to use gltA sequencing to definitively identify most of the Anaplasma spp. we detected with our 16S rRNA FRET-qPCR, we could confirm the accuracy of the qPCR in detecting A. marginale and A. ovis. Anaplasma marginale was one of the most common Anaplasma species we detected with the 16S rRNA FRET-qPCR along with A. phagocytophilum which has also already been described in China where it appears to be common in ruminants [7, 11, 12, 34]. Anaplasma phagocytophilum is the agent of tick-borne fever of ruminants and is transmitted by Dermacentor silvarum, Haemaphysalis concinna, H. longicornis, and Ixodes persulcatus in China [35, 36]. The organism is now known to infect a wide variety of domestic and wild animals and is the agent of human granulocytic anaplasmosis [27].
Other Anaplasma spp. we appear to have identified based on their 16S rRNA sequences include A. platys, the agent of infectious canine cyclic thrombocytopenia [3], which has been described in dogs in Asia [24, 37] and in sika deer, goats, and cattle in China [4, 19]. The remaining two Anaplasma spp. we appear to have found are as yet only poorly characterized with Anaplasma sp. (KM227012) first reported in Procapra gutturosa, the Mongolian gazelle, in China and appear to be most closely related to A. ovis and A. centrale [38]. Anaplasma sp. BL126-13 (KJ410243) has only been identified in a Hyalomma asiaticum from Xinjiang [39]. As we found that these poorly characterized organisms seem to occur relatively commonly, especially in goats, it would seem appropriate that they should be studied further as they could be important pathogens.
A number of Ehrlichia spp. have been described in China, E. chaffeensis, E. canis, E. platys, E. ewingii (granulocytic ehrlichial agent), and also a novel species closely related to E. chaffeensis and A. marginale [14, 15, 33, 40]. The most important Ehrlichia species infecting ruminants, E. ruminantium, is restricted to Africa and some Caribbean islands [19] and has not been reported in China. Of the other Ehrlichia known to infect ruminants (summarized in Zhang et al., 2015 [19]), we only found evidence of infection with E. canis in the domestic ruminants we studied in China. Although E. canis is best known as a very common dog pathogen around the world, infections have also been described in people [41] and in cats [42], and there is thus growing evidence that E. canis has a wider host range than previously thought [2, 19, 43]. Our finding of E. canis and closely related organisms in a goat and cattle in China further supports this evidence and is consistent with the findings of a study showing that E. canis or very closely related organisms are present in domestic ruminants in the Caribbean [19] and also a study showing that E. canis occurs in sika deer in China [4]. Further studies are underway in our laboratory to determine the pathogenicity of E. canis in domestic ruminants.
In summary, we found DNA of Anaplasma spp. and Ehrlichia spp. relatively common in the blood of the goats (81.1% and 1.1%, resp.), cattle (13.7% and 3.6%, resp.), sheep (11.7% and 1.8%, resp.), and water buffaloes (6.9% and 0%, resp.) we studied from China. Further, our data from 12 provinces show that a wide range of Anaplasma spp. and Ehrlichia spp. occur in ruminants in China and further larger scale studies are indicated to determine more accurate prevalence data for these agents and their impact on health and production. The low copy numbers we commonly found indicate that chronic infections are common and this did not enable us to obtain reliable multigene sequence data from most samples. It would appear best, then, for future studies on the presence of Anaplasma and Ehrlichia spp. to rather be conducted on organisms cultured from infected animals. Ticks should also be considered for such studies as they generally contain relatively high numbers of Anaplasma and Ehrlichia spp. (2,530 to 970,000/positive tick) [25].
Competing Interests
The authors declare that they have no competing interests.
Authors’ Contributions
Chengming Wang, Haixiang Qiu, Jilei Zhang, and Patrick John Kelly designed the study. Haixiang Qiu, Jilei Zhang, Qinghua Luo, Yi Yang, Yongjiang Mao, Zhangping Yang, Jing Li, and Hongzhuan Wu performed the experiment. Chengming Wang, Haixiang Qiu, Jilei Zhang, and Patrick John Kelly wrote the manuscript. All authors read and approved the final manuscript.
Acknowledgments
This project was supported by the National Natural Science Foundation of China (Grants 31272575 and 32472225) and by the Priority Academic Program Development of Jiangsu Higher Education Institutions.
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