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Review

Cytauxzoonosis in North America

by
Mason V. Reichard
1,*,
Tiana L. Sanders
1,
Pabasara Weerarathne
1,
James H. Meinkoth
1,
Craig A. Miller
1,
Ruth C. Scimeca
1 and
Consuelo Almazán
2,*
1
Department of Veterinary Pathobiology, College of Veterinary Medicine, Oklahoma State University, Stillwater, OK 74078, USA
2
Facultad de Ciencias Naturales, Universidad Autónoma de Querétaro, Avenida de las Ciencias S/N, Juriquilla, Querétaro 76230, Mexico
*
Authors to whom correspondence should be addressed.
Pathogens 2021, 10(9), 1170; https://0-doi-org.brum.beds.ac.uk/10.3390/pathogens10091170
Submission received: 6 August 2021 / Revised: 1 September 2021 / Accepted: 3 September 2021 / Published: 10 September 2021
(This article belongs to the Special Issue Ticks and Tick-Borne Pathogens at the Wildlife–Domestic Interface)
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Abstract

:
Cytauxzoonosis is an emerging tick-borne disease of domestic and wild felids produced by infection of Cytauxzoon felis, an apicomplexan protozoan similar to Theileria spp. Transmitted by Amblyomma americanum, lone star tick, and Dermacentor variabilis, American dog tick, infection of C. felis in cats is severe, characterized by depression, lethargy, fever, hemolytic crisis, icterus, and possibly death. Cytauxzoonosis occurs mainly in the southern, south-central, and mid-Atlantic United States in North America, in close association with the distribution and activity of tick vectors. Infection of C. felis, although severe, is no longer considered uniformly fatal, and unless moribund, every attempt to treat cytauxzoonosis cats should be made. Herein we review cytauxzoonosis, including its etiology, affected species, its life cycle and pathogenesis, clinical signs, diagnosis, and epidemiology, emphasizing clinical pathology findings in cats infected with this important emerging tick-borne disease in North and South America.

1. Introduction

Cytauxzoonosis is an emerging tick-borne disease produced by infection of Cytauxzoon felis (Piroplasmorida: Theileriidae), an apicomplexan protozoan that is transmitted by Amblyomma americanum and Dermacentor variabilis ticks to wild and domestic felids. Acute cytauxzoonosis in domestic cats is a severe clinical syndrome characterized by fever, inappetence, lethargy, depression, dehydration, dyspnea, hemolytic crisis, and icterus. Mortality can be high, but cats may also survive infection, and every attempt should be made to treat cats with cytauxzoonosis, especially if diagnosis is made early in the course of disease. If C. felis-infected cats survive acute disease, the cats will become chronic survivors, with only piroplasms present in erythrocytes. Cytauxzoon felis was first reported in four cats from southwestern Missouri that presented with anemia, icterus, dehydration, and fever [1]. Feline infectious anemia was originally suspected before schizonts consistent with Cytauxzoon spp. were noted in liver, lung, spleen, and lymph nodes from the cats at necropsy [1]. Later that same year, two cases of cytauxzoonosis were confirmed in domestic cats from central and southeastern Texas [2]. Cytauxzoon felis was established as the etiologic agent of cytauxzoonosis based on ultrastructural morphology, vertebrate host cell tropism, and mode of replication [3]. Acute cytauxzoonosis in domestic cats is colloquially referred to as bobcat fever, as cats with acute cytauxzoonosis are febrile at presentation and infected bobcats serve as wild animal reservoirs. Infections of C. felis are found primarily in the southern, south-central, and mid-Atlantic United States in North America, and it is likely that C. felis or closely related Cytauxzoon spp. are found in Brazil in South America [4,5,6,7]. This review is focused on the etiologic agent, affected species, life cycle and pathogenesis, clinical signs, diagnosis, and epizootiology of cytauxzoonosis, emphasizing the clinical pathology findings observed in cats infected with this important emerging disease in North America.

2. Etiologic Agent

Cytauxzoon felis is the only known piroplasm of domestic cats in the United States. Yabsley et al. [8] reported an unidentified Babesia sp. in Florida panthers (Puma concolor coryi); however, this unnamed piroplasm has not been identified in domestic cats. Numerous other piroplasms have been found in domestic and wild felids throughout the world [9,10,11], some of which were identified as C. felis. Identification of C. felis infection in domestic and wild cats outside of the Americas should be considered tentative until data can be provided that unequivocally confirm identification. Indeed, the taxonomy and definitive identification criteria for Cytauxzoon spp. are in need of elucidation [10]. Other species of Cytauxzoon in felids include: C. manual in Pallas’ cats (Otocolobus manual) [12], C. europaeus in European wildcats (Felis sylvestris) and Eurasian lynx (Lynx lynx) [11], C. otrantorum in European wildcats [11], and C. banethi in European wildcats [11]. The genus Cytauxzoon was erected in 1948 based on a piroplasm (C. sylvicaprae) found in a duiker (Sylvicapra grimmia) [13]. Cytauxzoon spp. are closely related to Theileria spp. sensu stricto and were differentiated based on vertebrate host leukocyte predilection. Schizogony for Theileria spp. occurs in lymphocytes with multiple fission in erythrocytes, whereas for Cytauxzoon spp., schizogony occurs in histiocytes with binary fission in erythrocytes [13,14]. However, differentiation between Theileria and Cytauxzoon based on vertebrate host leukocyte predilection may be inadequate and in need of reconsideration [15].
Gene sequence analysis of various C. felis isolates from the United States has demonstrated genetic variability across their range. Multiple studies have found genetic variation within internal transcriber spacer regions 1 and 2 (ITS1, ITS2) [16,17,18,19,20]. The ITSa genotype has been one of the most common genotypes reported, and while previously associated with higher survivability and found primarily in Arkansas, more recent evidence found it to occur in acute, fatal, and subclinical cases in domestic cats from Oklahoma, Arkansas, and Missouri [17]. Multiple genotypes have been reported to circulate within both domestic cats and wild felids. Pollard et al. [17] found ITS genotypes that had previously only been reported in wild felids also occuring in domestic cats, demonstrating the adaptivity of C. felis. Several studies have linked C. felis cytochrome b (cytb) genotypes with treatment success in response to administration of atovaquone and azithromycin (see below) [21,22]. However, Hartley et al. [23] reported a mutation in wild-type C. felis cytb methionine (M128). Post-treatment, cytb coded for isoleucine and valine at 2 and 4 months post-treatment despite repeated treatment with a higher dose of atovaquone in combination with azithromycin [23].

3. Affected Species

Cytauxzoon felis infects domestic and wild felids. Because of its similarity to Theileria spp. (e.g., T. parva and T. annulata), when C. felis was first identified, investigators were concerned that this parasite produced a severe infection, and fatal disease in cats may also have debilitating effects on production or other pet animals. Kier et al. [24] inoculated 33 different species of domestic, laboratory animal, and wildlife vertebrates with schizonts of C. felis to determine what impact the parasite may have on other animals and whether a laboratory animal model could be developed. The only animals that produced clear evidence of cytauxzoonosis were bobcats (Lynx rufus).

3.1. Domestic Cats

Cases of cytauxzoonosis occur in cats throughout the southcentral, southeastern, and mid-Atlantic United States [25,26]. First reported in domestic cats from southwestern Missouri, cases of C. felis infection have since been reported from Alabama, Arkansas, Florida, Georgia, Illinois, Kentucky, Louisiana, Mississippi, North Carolina, Oklahoma, South Carolina, Tennessee, Texas, and Virginia (Table 1). Historically, infection of C. felis in domestic cats was considered highly fatal, with a very high mortality rate. However, cats surviving cytauxzoonosis were first noted around 2000 [19,25,27,28,29]. More recently, investigators have realized that there is a significant subpopulation of domestic cats that are subclinically infected with C. felis. Out of 902 blood samples of healthy, asymptomatic cats from Arkansas, Missouri, and Oklahoma, Rizzi et al. [30] demonstrated 15.5%, 12.9%, and 3.4%, respectively, were infected with C. felis. Similarly, in a study of 1,104 healthy cats in Kansas and 22 healthy cats in northwest Arkansas, 270 (25.8%) [31] and 4 (18.2%) [32], respectively, were infected with C. felis. Considering that (1) infection of C. felis is no longer considered uniformly fatal, (2) there is a significant subpopulation of domestic cats subclinically infected with C. felis found in close proximity to other domestic cats, and (3) transmission from cats subclinically infected with C. felis to naïve cats with A. americanum has been observed (46,47,50,52,53), it is likely these chronically infected cytauxzoonosis survivor cats are an important domestic reservoir of infection to other domestic cats.

3.2. Bobcats

Bobcats are the wild vertebrate reservoir of C. felis. Fatal infections of C. felis in bobcats have been reported [48,49]. However, the natural mortality rate of cytauxzoonosis in bobcats is not known, and given the high prevalence of C. felis infection in apparently healthy bobcats from enzootic areas (Table 2), the wild felid is considered a normal host for the parasite. Relatively few studies have been conducted to evaluate the occurrence of C. felis in bobcats. Nonetheless, the prevalence of C. felis infection is often high in areas where A. americanum and D. variabilis (see below) are present. Shock and colleagues [50] tested 696 bobcat spleens from 13 different states. The highest prevalence of C. felis in bobcats was reported in Missouri (79.5%), followed by North Carolina (62.5%), Oklahoma (65.0%), South Carolina (57.1%), Kentucky (55.4%), Florida (35.6%), Kansas (30.8%), Georgia (9.1%), and North Dakota (1.7%). Cytauxzoon felis was not detected in bobcats collected from Ohio, West Virginia, California, and Colorado. Birkenheuer et al. [51] surveyed bobcats in both North Carolina (where cytauxzoonosis is enzootic in domestic cats) and Pennsylvania (where cytauxzoonosis is not known to occur in domestic cats). They found bobcats in North Carolina had a significantly higher prevalence (33.0%) than Pennsylvania (7.3%). Shock et al. [50] also found a low prevalence of C. felis infection in bobcats from North Dakota (1.7%) where cytauxzoonosis is not known to occur in domestic cats. In southwestern Illinois, Zieman et al. [52] reported a prevalence of C. felis infection in bobcats of 70.6%. These same authors sequentially sampled five bobcats in their study area for 5 years and noted both that the wild felids were chronically infected with C. felis and that one of the cats became infected with a second strain of C. felis during the study [53]. More studies are needed to ascertain the transmission dynamics of C. felis spillover from bobcats in sylvatic ecosystems to domestic cats in urban settings. Additional surveys should also be conducted in bobcats to monitor changes in areas not previously recognized as enzootic for C. felis and to monitor changes locally in enzootic areas.

3.3. Puma and Florida Panthers

In addition to bobcats, infection of C. felis has been reported in pumas (also known as cougars or mountain lions [Puma concolor]) from North America [8,50,55,56] and South America [6] and Florida panthers (Puma concolor coryi; a subspecies of P. concolor distinguished for conservation efforts) from Florida [8,56,57]. Rotstein et al. [56] sampled pumas translocated from Texas to Florida as well as wild Florida panthers to estimate the impact of cytauxzoonosis on wild felids. In total they sampled 91 wild felids, finding that 11 out of 28 (39%) pumas and 22 out of 63 (35%) Florida panthers were infected with C. felis. While there were significant differences in blood parameters measured between the translocated pumas and the Florida panthers, the authors reported that biological differences in the blood values were not likely, as hematologic parameters measured were within expected ranges for healthy animals [56]. In addition, Rotstein et al. [56] noted the pumas translocated from Texas became infected with C. felis in Florida, as hemoparasites were not detected prior to arriving in Florida. It is probable that Puma spp. throughout North and South America are natural hosts for C. felis in enzootic areas; however, this hypothesis has yet to be tested.

3.4. Other Wild and Exotic Felids

Fatal cases of cytauxzoonosis have been reported from a captive Bengal tiger (Panthera tigris) at a zoo in Germany (14 months after importation of three bobcats from North America to the facility) [58], a captive-reared white tiger (Panthera tigris) in northern Florida [59], and captive-reared lions (Panthera leo) in Brazil [5]. Subclinical infections of C. felis have been reported in four captive tigers (P. tigris) in northwest Arkansas [60], six captive ocelots (Leopardus pardalis) in Brazil [6], and jaguars (Panthera onca) in Brazil [6,7]. Similar to bobcats and Puma spp., other wild felids native to North and South America are likely natural hosts for C. felis in enzootic areas.

4. Life Cycle and Pathogenesis

The life cycle of C. felis occurs in two phases, one inside its tick vector (sexual) and the second inside the feline vertebrate host (asexual). Cats become infected with the transfer of C. felis sporozoites while an infected tick is feeding. Perinatal transmission of C. felis has been hypothesized but has not been demonstrated [61]. Ticks that have been experimentally demonstrated to transmit C. felis to cats include A. americanum adults [62,63,64,65], A. americanum nymphs [66], and D. variabilis adults [49,67]. Amblyomma americanum adults infected with C. felis need to be attached for a minimum of 36 to 48 h for cats to become infected [68,69]. Ingestion of C. felis-infected A. americanum adults is not a route of transmission to cats [69]. Inside the cat, sporozoites enter mononuclear cells, where they transform and undergo schizogony. During schizogony, the C. felis-infected host cell is transformed into a schizont (Figure 1) that can be found attached to the endothelium or within the lumina of veins and venules of all organs and tissues and within the interstitium of other tissues (e.g., spleen, lymph nodes) [70]. Schizonts are initially small in diameter (15 to 20 µm) and few until about day 12 post-infection. By day 19 post-infection, schizonts are larger (80 to 250 µm) and more numerous [70]. Schizogonous replication of C. felis results in distention and enlargement of the host cell schizont. Often referred to as megaschizonts, these cells can act like thrombi and occlude vessels. Vascular occlusion is a hallmark of acute cytauxzoonosis and is exhibited to some degree in all cases [71], resulting in multi-organ failure. Clinical signs of cytauxzoonosis begin 11–14 days after infected ticks begin feeding [62,63] and are considered a direct result of the C. felis schizogony process.
The schizogonous cycle of C. felis is considered limited [49], and this observation is supported in that schizonts are not found in cats that survive acute cytauxzoonosis [19,27,28,29,30,31]. Nevertheless, schizogony results in the formation of uninucleated merozoites that rupture from the schizonts, some of which are taken up by erythrocytes and become piroplasms (Figure 2). Piroplasms reproduce asexually within red blood cells through merogony, although many of the details of C. felis piroplasm multiplication and development are unknown and assumed from related Theileria spp. [72] At some point, C. felis piroplasms undergo gamogony, forming gametocytes in red blood cells, which at this time cannot be morphologically differentiated from merozoites. The gametocyte are what must be ingested by A. americanum or D. variabilis for the life cycle to continue. Once inside a tick, gametocytes metamorphose to gametes within the gut. Fertilization of piroplasm gametes results in the formation of a zygote that penetrates the peritrophic matrix and immediately invades the epithelial cells of the tick gut [72]. Inside the epithelial cells, the piroplasm zygote undergoes a meiotic division to form motile kinetes; once released in to hemolymph, they invade type II and III salivary glands [72]. In the salivary glands, they enlarge and transform into a sporont and then a sporoblast that is multinucleated [72]. Formation of the sporoblast is associated with hypertrophy of infected salivary glands for C. felis and other closely related piroplasms [72]. Sporogony occurs asynchronously, providing a continuous release of sporozoites into tick saliva and to the feline hosts while infected ticks are feeding [72].
Initial attempts at transmitting C. felis through ticks were unsuccessful [73] (as reported in [3]). However, Blouin et al. [67] successfully transmitted C. felis by acquisition-feeding D. variabilis nymphs on an infected bobcat that was splenectomized, and then transmission-feeding the adult ticks (Figure 3) on two splenectomized domestic cats. Blouin et al. [49] subsequently confirmed the ability of D. variabilis to transmit C. felis by acquisition-feeding D. variabilis nymphs on another splenectomized bobcat and transmission-feeding the adult ticks on two spleen-intact bobcats. Reichard et al. [63] acquisition-fed nymphs of A. americanum, D. variabilis, Ixodes scapularis, and Rhipicephalus sanguineus on a naturally infected, C. felis survivor domestic cat. Once the nymphs had fed to repletion, they were molted to adults, and then ticks of each species were transmission-fed on individual cats. The cat infested with A. americanum adults (Figure 3) was the only one that became infected with C. felis. Reichard et al. [62] confirmed the ability of A. americanum to act as a vector for C. felis by acquisition-feeding nymphs of A. americanum and D. variabilis simultaneously on a subclinically infected C. felis survivor cat and subsequently transmission-feeding adults of each tick species on four domestic cats. All four of the A. americanum transmission-fed cats became infected with C. felis, whereas none of the D. variabilis-fed cats became infected. Allen et al. [66] acquisition-fed A. americanum and D. variabilis larvae on a parasitemic cytauxzoonosis survivor cat and then transmission-fed nymphs of those ticks on each of three cats. Only the three cats infected with A. americanum nymphs (Figure 3) became infected with C. felis.
Surveys on the occurrence and prevalence of C. felis in ticks are limited (Table 3). Bondy et al. [74] amplified DNA of C. felis in partially engorged A. americanum nymphs recovered from a cat that died of acute cytauxzoonosis. Reichard et al. [62] reported minimum infection rates of C. felis in unengorged A. americanum females at 1.5%, A. americanum males at 0.5%, and A. americanum nymphs at 0.8%, and no infections in D. variabilis females and males from north-central Oklahoma. Shock et al. [75] tested ticks from Georgia, Kentucky, Pennsylvania, Tennessee, and Texas for C. felis infection, and detected C. felis only in D. variabilis from Tennessee and Georgia. Infection of C. felis in A. americanum was not detected from those states (Table 3). Zieman et al. [52] collected A. americanum and D. variabilis from an enzootic area where 70.4% of bobcats were infected with C. felis. They found 15.4% of A. americanum and 15.8% of D. variabilis were infected with C. felis in southern Illinois [52].
Amblyomma americanum is considered the primary vector of C. felis in the United States due to the overlap in distribution and abundance of lone star ticks in the southern Unites States with that of cytauxzoonosis cases [51], corresponding seasonal activity of A. americanum and occurrence of clinical cases in domestic cats [47], and host preference of lone star ticks compared to American dog ticks and the likelihood of those ticks feeding on cats [76,77]. Additionally, the three studies that have been performed comparing the competency of A. americanum and D. variabilis in the transmission of C. felis to domestic cats [62,63,66] demonstrated transmission only with lone star ticks. Nevertheless, it is evident that D. variabilis can be involved in the transmission of C. felis, as it has been demonstrated experimentally [49,67], C. felis has been found in questing American dog ticks [52,75], and C. felis has been found in bobcats outside the range of lone star ticks but in areas where American dog ticks occur [51,75]. Considerably more research needs to be performed to determine the transmission dynamics of C. felis to domestic cats and the vector competence of A. americanum, D. variabilis, and possibly other ticks throughout the ranges of the parasites. As we are currently appreciating considerable change in our comprehension in the distribution of D. variabilis [78] and expansion in the range of A. americanum [79,80], it will become ever more important to understand the transmission dynamics, the role of these tick vectors (and possibly others), and the risk of cytauxzoonosis to cats in areas not currently recognized as enzootic.
It is still unknown what ticks transmit C. felis or the C. felis-like organism(s) in South America. Amblyomma cajennense were found in the habitat of captive lions that died of cytauxzoonosis in Rio de Janeiro [5]. However, these ticks could not be definitively linked to transmission, as no C. felis were found in hemolymph nor histological sections of the ticks. Currently, 44 species of hard ticks are recognized in Brazil: 30 species of Amblyomma, 1 species of Dermacentor, 3 species of Haemaphysalis, 8 species of Ixodes, and 2 species of Rhipicephalus [81].
Pathogenesis of cytauxzoonosis is largely attributed to schizogony of C. felis in histiocytes. These cells accumulate in the veins and sinusoids of many tissues [25]. In severe cases, schizonts of C. felis may occlude the lumen (Figure 4) of these vessels [70]. Thrombosis of affected vessels is common, and histological changes consistent with ischemia are seen in many tissues, including the brain and heart [82]. The lungs, spleen, and liver are usually the most severely affected organs, but most any parenchymatous organs can be involved [25]. Evaluation of the pulmonary histopathology of 148 C. felis infections from Oklahoma showed moderate interstitial pneumonia, mild alveolar macrophage involvement, mild intra-alveolar hemorrhage, and moderate to severe vascular occlusion, with pulmonary edema common [71]. A histopathology review of eight cases of C. felis infection from Georgia showed the presence of intravascular schizont-laden macrophages in leptomeningeal and parenchymal arterioles and venules, along with occlusion of small capillaries throughout the gray and white matter and choroid plexus [83].

5. Clinical Signs

Infection of C. felis in domestic cats is severe. Cats present with fever (Figure 5), inappetence, lethargy, depression, dehydration, dyspnea, hemolytic crisis, and possibly icterus (Figure 6). Before 2000, cytauxzoonosis was considered a uniformly fatal disease. However, that is no longer the case, and a considerable number of cats have been documented to survive acute cytauxzoonosis [19,25,26,27,28,29,30,31,32]. Additionally, current treatment strategies (see below) improve the likelihood of survival to discharge by a factor of over 7 [84]. Unless a cat infected with C. felis is moribund at presentation, every attempt should be made to treat and recover the cat. Cats become febrile approximately 11–14 days after being bitten by a C. felis-infected tick. A typical case of cytauxzoonosis as seen at presentation with CBC and chemistry panel is provided in Table S1.
Cats displaying signs of cytauxzoonosis will likely have a low white blood cell count (leukopenia), characterized by low neutrophils with a left shift and toxic change. Cats will be thrombocytopenic and possibly anemic. Upon examination of blood smears, piroplasms of C. felis may not be present during acute disease or if cats are being treated with the recommended therapy (see below). Cats initially have a non-regenerative anemia, but if they survive, schizogonous replication of C. felis they will become regenerative at some point. The anemia is attributable to both hemolysis (not increase in bilirubin) and bone marrow suppression. Large granular lymphocytes may be normal or increased. However, if large granular lymphocytes are present in leukopenic or neutropenic cats, the index of suspicion for C. felis infection is high. Cats that survive acute cytauxzoonosis become persistently infected [84] and are considered life-long carriers of C. felis.
The current recommended treatment for cytauxzoonosis includes a combination of atovaquone (15 mg/kg PO q8H) and azithromycin (10 mg/kg PO q24h) [84]. Use of diminazene diaceturate was hypothesized to clear C. felis subclinically infected carrier cats, but this treatment was not effective, and adverse side effects were common [85]. Administration of atovaquone and azithromycin therapy combined with aggressive supportive and nursing care [26] resulted in a 60% survival rate, and treated cats were 7.2 times more likely to survive to discharge [84]. Recommended supportive care measures to consider, depending on specifics of the case, include judicious intravenous crystalloid fluid therapy, heparin to prevent disseminated intravascular coagulation, analgesic therapy, antiemetics, red blood cell transfusion, fresh or frozen plasma, oxygen supplementation, therapeutic thoracocentesis, and nutritional support [26]. Interestingly, administration of antipyretic agents may be contraindicated but deserves further evaluation [26].
Bioinformatic analysis of the C. felis genome has been used to predict a candidate vaccine for cytauxzoonosis [86]. However, a vaccine for cytauxzoonosis has not yet become commercially available. Disease prevention currently relies on administration of acaricides to cats to control tick feeding. Two products, approved for use on cats in the United States, have demonstrated efficacy for blocking the transmission of C. felis to cats by preventing or interrupting feeding of infected A. americanum: Seresto (imidacloprid and flumethrin collar) [65] and Revolution Plus (selamectin and sarolaner topical solution) [64].

6. Diagnosis

Definitive diagnosis of cytauxzoonosis is based on observation of C. felis in infected tissue or by detecting parasites through a molecular-based method, typically PCR. The most widely used but least-sensitive method for diagnosing C. felis infection is microscopic observation of Wright–Giemsa stained thin-blood smears for piroplasms of C. felis in erythrocytes (Figure 2). Piroplasms of C. felis are piriform (i.e., pear-shaped) but can also be found in ring, oval, or anaplasmoid forms, occurring as singles, pairs, or possibly tetrads (i.e., maltese crosses), and measure 0.3–0.7 µm up to 1.0–2.2 µm in diameter or 0.8–1.0 µm in width by 1.5–2.0 µm in length depending on morphological form [70]. Clinical signs of cytauxzoonosis may precede the presence of C. felis piroplasms in erythrocytes by several days or more [26]. Cats that survive acute cytauxzoonosis will develop a low-level parasitemia in ≤1% of erythrocytes. While definitive evidence has not been provided, cats that survive cytauxzoonosis are considered life-long carriers of C. felis and can be reservoirs of infection if not provided with effective tick prevention. Schizonts of C. felis precede the production of piroplasms in erythrocytes and can be observed in fine needle aspirates of infected organs (e.g., spleen, lymph nodes), histopathology, or impression smears. Schizonts range from 15–20 µm in diameter early in the course of infection up to 80–250 µm in diameter as disease progresses (Figure 1) [70]. As cats become more ill and the size of schizonts increases, so does the number of schizonts, which leads to vascular occlusion. Despite substantial pulmonary pathology due to C. felis infection, pathognomonic lesions of acute cytauxzoonosis are not evident on thoracic radiographs [87].
Polymerase chain reactions using primers that amplify specific genetic segments of C. felis (Table 4) are the most widely used molecular methods employed for diagnosing C. felis infection. These molecular methods are considerably more sensitive and specific compared to light microscopy but are more time-consuming and costly. A patient-side assay that can aid veterinary practitioners in diagnosis cytauxzoonosis would be considerably advantageous and would allow initiation of treatment early in the course of disease. Different genetic targets used for C. felis diagnosis include 18S rRNA [19,63,74,88], internal transcribed spacer 1 (ITS1) [19], ITS 2 [19,28,63], cytochrome b (cytb) [89], and cytochrome c oxidase subunit III (cox3) [89,90]. Of the PCR methods available, digital droplet PCR (ddPCR) is the most sensitive assay, detecting as little as 0.175 copies/µL, and can provide an absolute quantification of parasite load over time while requiring only a small quantity of DNA (as little as 0.0000231 ng DNA/reaction) [90]. Other sensitive quantitative PCR methods are nested-PCR targeting 18S rRNA [63,74] and real-time PCR targeting ITS2 region [63]. In addition to these molecular methods, in situ hybridization has been used to visualize and confirm the C. felis in tissue samples [91].

7. Epizootiology

Presentation of cytauxzoonosis cases to veterinary clinics follows a bimodal pattern that is related to the seasonal activity of ticks [47]. Tick activity is dependent on environmental factors such as temperature range, precipitation, and humidity [92]. Peak activity of adult and nymphal A. americanum occurs from April to June and August to September, respectively [47,50], but may differ across geographical regions. Other environmental factors such as low-density residential areas, wooded habitat, and proximity to natural or unmanaged areas [47] pose a higher risk of C. felis infection to domestic cats. Not only do these environmental factors suit the tick vectors, but wooded habitats and edge habitats also provide suitable conditions for bobcats [47]. However, the bimodal pattern of clinical cases correspond with seasonal fluctuations of infected tick vectors more than activity of bobcats [47], indicating that clinicians should be aware of the seasonal activity of tick vectors in their area to best guide their client prevention, treatment, and control protocols.
In addition to environmental risk factors, age, sex, and lifestyle may influence the risk of cytauxzoonosis to domestic cats. More clinical cases have been diagnosed in young cats from 1–4 years of age [44,93]. There are several possible explanations of why young cats may contribute to higher clinical cases. Young cats may have a greater drive to explore territory, risking exposure to tick vectors; clients may bring in younger cats with acute illness more often than older cats, in whom illness may be contributed to by old age; and older cats that have recovered from previous infection with C. felis may be asymptomatic carriers [93]. Multiple studies have found that young, male cats were over-represented when diagnosing acute cytauxzoonosis as well [44,93]. Cats that spend most of their lives outdoors have a significantly higher risk of becoming infected with C. felis due to tick exposure. A study in Kansas found 29.6% of feral cats were positive for C. felis compared to 25.4% of owned cats and 21.8% of rescue cats [93]. These feral cats spent their entire lives outdoors, greatly increasing their risk of tick exposure.
Initially, infection of C. felis was considered almost 100% fatal. In fact, many practitioners would euthanize upon a definitive cytauxzoonosis diagnosis. However, several studies conducted in disparate geographical areas have documented the presence of subclinical, chronically C. felis-infected domestic cats [27,28,29,30]. Prior to the realization that domestic cats were surviving infection, bobcats were considered the only vertebrate reservoir. With free-roaming and feral domestic cats being found in closer proximity to client-owned domestic cats, and knowing that tick transmission can occur from a subclinically infected carrier domestic cat to a naïve domestic cat [62,63,64,65,66,69], it is likely that C. felis-infected subclinical carrier domestic cats with access to the outdoors are domestic vertebrate reservoirs, along with infected bobcats being wild vertebrate reservoirs.

Supplementary Materials

The following are available online at https://0-www-mdpi-com.brum.beds.ac.uk/article/10.3390/pathogens10091170/s1. Table S1: Results of complete blood count (CBC), and serum chemistry profile (SCP) obtained from a typical case of acute cytauxzoonosis in a cat presented to a veterinary clinic in an enzootic region.

Author Contributions

Conceptualization, M.V.R. and C.A.; investigation, all; resources, all; original draft preparation, all; writing, reviewing, and editing, all. All authors have read and agreed to the published version of the manuscript.

Funding

This research received no specific funding.

Institutional Review Board Statement

Not applicable.

Informed Consent Statement

Not applicable.

Acknowledgments

Megan Lineberry, National Center for Veterinary Parasitology, is acknowledged for providing tick images.

Conflicts of Interest

The authors declare no conflict of interest.

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Figure 1. A schizont of Cytauxzoon felis from a stained impression smear of infected tissue. Schizonts range from 15–20 µm in diameter early in the course of infection up to 80–250 µm in diameter as disease progresses. As the disease progresses, the size and number of schizonts increases, leading to vascular occlusion.
Figure 1. A schizont of Cytauxzoon felis from a stained impression smear of infected tissue. Schizonts range from 15–20 µm in diameter early in the course of infection up to 80–250 µm in diameter as disease progresses. As the disease progresses, the size and number of schizonts increases, leading to vascular occlusion.
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Figure 2. Piroplasms of Cytauxzoon felis in a stained thin-blood smear from an infected cat. Piroplasms of C. felis are morphologically variable but are generally pear-shaped, oval, ring-shaped, or anaplasmoid (arrows). They can occur singly, in pairs, or possibly in tetrads. Individual piroplasms measure 0.3–0.7 µm up to 1.0–2.2 µm in diameter or 0.8–1.0 µm in width by 1.5–2.0 µm in length depending on morphological form.
Figure 2. Piroplasms of Cytauxzoon felis in a stained thin-blood smear from an infected cat. Piroplasms of C. felis are morphologically variable but are generally pear-shaped, oval, ring-shaped, or anaplasmoid (arrows). They can occur singly, in pairs, or possibly in tetrads. Individual piroplasms measure 0.3–0.7 µm up to 1.0–2.2 µm in diameter or 0.8–1.0 µm in width by 1.5–2.0 µm in length depending on morphological form.
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Figure 3. Ticks that have been experimentally demonstrated to act as vector for Cytauxzoon felis by feeding infected ticks on domestic cats or bobcats include: (A) Amblyomma americanum female, (B) A. americanum male, (C) A. americanum nymph, (D) Dermacentor variabilis female, (E) D. variabilis male. Images courtesy of Megan Lineberry, National Center for Veterinary Parasitology. All images 1.6× magnification.
Figure 3. Ticks that have been experimentally demonstrated to act as vector for Cytauxzoon felis by feeding infected ticks on domestic cats or bobcats include: (A) Amblyomma americanum female, (B) A. americanum male, (C) A. americanum nymph, (D) Dermacentor variabilis female, (E) D. variabilis male. Images courtesy of Megan Lineberry, National Center for Veterinary Parasitology. All images 1.6× magnification.
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Figure 4. Pulmonary vessels (outlined with chevrons) occluded by schizonts of Cytauxzoon felis. As schizonts replicate, they become larger and more numerous in the veins and sinusoids of many tissues. If infection is severe, vessels in any parenchymatous organ may contain schizonts.
Figure 4. Pulmonary vessels (outlined with chevrons) occluded by schizonts of Cytauxzoon felis. As schizonts replicate, they become larger and more numerous in the veins and sinusoids of many tissues. If infection is severe, vessels in any parenchymatous organ may contain schizonts.
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Figure 5. Temperature profile of two cats (A and B) with cytauxzoonosis compared to a control cat (C) that was not infected. Onset of cytauxzoonosis typically begins 11–14 days after being bitten by a C. felis-infected tick. Fever can peak around 40.6–41.1 °C (105.0–106.0 °F). Once cats begin to recover, they can become hypothermic before the temperature returns to normal or they become moribund.
Figure 5. Temperature profile of two cats (A and B) with cytauxzoonosis compared to a control cat (C) that was not infected. Onset of cytauxzoonosis typically begins 11–14 days after being bitten by a C. felis-infected tick. Fever can peak around 40.6–41.1 °C (105.0–106.0 °F). Once cats begin to recover, they can become hypothermic before the temperature returns to normal or they become moribund.
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Figure 6. Cats that developed cytauxzoonosis from infection with Cytauxzoon felis. (A) Depression and lethargy are the first clinical signs owners notice with cats infected with C. felis. This cat would be dehydrated and febrile at presentation. (B) Cats severely affected by cytauxzoonosis can become anemic and icteric, the degree of which can be highly variable among C. felis infected cats.
Figure 6. Cats that developed cytauxzoonosis from infection with Cytauxzoon felis. (A) Depression and lethargy are the first clinical signs owners notice with cats infected with C. felis. This cat would be dehydrated and febrile at presentation. (B) Cats severely affected by cytauxzoonosis can become anemic and icteric, the degree of which can be highly variable among C. felis infected cats.
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Table
Table 1. Reports and surveys of domestic cats for Cytauxzoon felis infection in North America.
Table 1. Reports and surveys of domestic cats for Cytauxzoon felis infection in North America.
StateNo. of Cats TestedNo. of Cats InfectedPrevalence; 95% Confidence IntervalSample PeriodSample TypeTest MethodReference
AlabamaNANANANANANA[33]
ArkansasNANANANANANA[34]
NA18NA1997–1998bloodmicroscopy and PCR for 18S[29]
NA3NANAbloodmicroscopy and PCR for ITS 1&2[28]
NA57NA2005–2007bloodmicroscopy and PCR for ITS 1&2[18]
431841.9%; 28.4–56.7%NAbloodmicroscopy and PCR for ITS 1&2[19]
NA12NA1998–2011blood or other tissuemicroscopy[35]
1612515.5%; 10.7–22.0%2008–2012bloodPCR for18S[30]
22418.2%; 6.7–39.1%2020–2021bloodPCR for cox3[32]
Florida49410.2%; <0.1–1.3%1999–2000bloodPCR for18S[27]
GeorgiaNANANANANANA[34]
NA9NANAblood or other tissuemicroscopy[36]
NA31NA2005–2007bloodmicroscopy and PCR for ITS 1&2[18]
46919.6%; 10.4–33.4%NAbloodmicroscopy and PCR for ITS 1&2[19]
Illinois5953612NA2003–2012blood and spleenmicroscopy and PCR for ITS 1&2[37]
IndianaNANANANANANA[38]
Iowa29200.0%; 0.0–1.3%2012–2014bloodPCR for18S[39]
KansasNA1NANAlung and livermicroscopy[40]
110427025.8%; 22.0–27.1%2018–2019bloodPCR: cox3[31]
KentuckyNA1NANAbrain, heart, lung, intestine, spleen, lymph node, and kidneymicroscopy[41]
NA56NA2001–2011blood or other tissuemicroscopy[42]
LouisianaNA1NANAblood and other tissuemicroscopy[43]
MississippiNANANANANANA[33]
MissouriNA4NA1973–1975liver, lung, spleen, and lymph nodesmicroscopy[1]
NA68NA1998–2011blood or other tissuemicroscopy[35]
62812.9%; 6.4–23.7%2008–2012bloodPCR for18S[30]
North CarolinaNA28NA1998–2004blood or other tissuemicroscopy[44]
39200.0%; 0.0–1.2%1999–2000BloodPCR for18S[27]
OklahomaNA2NA1984blood or other tissuemicroscopy[45]
NA8NA1985–1992blood or other tissuemicroscopy[46]
NA18NA1997–1998bloodmicroscopy and PCR for 18S[29]
NA232NA1995–2006blood or other tissuemicroscopy[47]
NA130NA1998–2011blood or other tissuemicroscopy[35]
679233.4%; 2.2–5.1%2008–2012bloodPCR for18S[30]
38030.79%; 0.2–2.4%2012–2014bloodPCR for18S[39]
South CarolinaNA3NA1998–2004blood or other tissuemicroscopy[44]
Tennessee7511.3%; <0.1–7.9%2006bloodPCR for18S[27]
TexasNA2NANAtissuemicroscopy[2]
VirginiaNA3NA1998–2004blood or other tissuemicroscopy[44]
NA, not assessed.
Table
Table 2. Reports and surveys of bobcats (Lynx rufus) for Cytauxzoon felis infection in North America.
Table 2. Reports and surveys of bobcats (Lynx rufus) for Cytauxzoon felis infection in North America.
StateNo. of Bobcats TestedNo. of Bobcats InfectedPrevalence; 95% Confidence IntervalSampling PeriodSample TestedTest MethodReference
Arkansas6NANANAspleenreal-time PCR for 18S; PCR for ITS1 and ITS2[19]
California2600.0%; 0.0–15.2%1999–2010blood or spleennested PCR for ITS1[50]
Colorado6700.0%; 0.0–6.5%1999–2010blood or spleennested PCR for ITS1[50]
Florida451635.6%; 23.2–50.2%1999–2010blood or spleennested PCR for ITS1[50]
54NANANAspleenreal-time PCR for 18S; PCR for ITS1 and ITS2[19]
Georgia143139.1%; 5.3–15.1%1999–2010blood or spleennested PCR for ITS1[50]
73NANANAspleenreal-time PCR for 18S; PCR for ITS1 and ITS2[19]
Illinois1258870.4%; 61.9–77.7%2003–2015blood or spleennested PCR for 18S[52]
Kansas391230.8%; 18.5–46.5%1999–2010blood or spleennested PCR for ITS1[50]
11NA2000 microscopy[48]
Kentucky744155.4%; 44.1–66.2%1999–2010blood or spleennested PCR for ITS1[50]
Missouri393179.5%; 64.2–89.5%1999–2010blood or spleennested PCR for ITS1[50]
North Carolina301033.3%; 19.3–51.3%2004, 2005, 2006bloodPCR for18S[51]
8562.5%; 30.4–86.5%1999–2010blood or spleennested PCR for ITS1[50]
North Dakota17231.7%; 0.4–5.2%1999–2010blood or spleennested PCR for ITS1[50]
Pennsylvania6957.3%; 2.8–16.2%2002bloodPCR for 18S[51]
Ohio1900.0%; 0.0–19.8%1999–2010bloodnested PCR for ITS1[50]
Oklahoma10NANA1982–1984blood, liver, spleen, lung, or lymph nodesmicroscopy[49]
201365.0%; 43.2–82.01999–2010blood or spleennested PCR for ITS1[50]
261350.0%; 32.1–67.9%~1982bloodmicroscopy[54]
South Carolina7457.1%; 25.0–84.3%1999–2010blood or spleennested PCR for ITS1[50]
West Virginia3700.0%; 0.0–11.2%1999–2010blood or spleennested PCR for ITS1[50]
Table
Table 3. Reports and surveys of ticks for Cytauxzoon felis infection in North America.
Table 3. Reports and surveys of ticks for Cytauxzoon felis infection in North America.
StateTick SpeciesTick Life StageNo. of Ticks or Tick Pools TestedNo. of Ticks or Tick Pools InfectedPrevalence or Minimum Infection Rate (95% Confidence Interval)Reference
GeorgiaAmblyomma americanumNR *34000.0% (0.0–1.4%)[75]
Dermacentor variabilisNR12510.8% (<0.1–4.8%)
Amblyomma maculatumNR1600.0% (0.0–22.7%)
Ixodes scapularisNR300.0% (0.0–61.8%)
Amblyomma spp.NR200.0% (0.0–71.0%)
IllinoisA. americanumfemale57814.0% (7.0–25.6%)[52]
male601016.7% (9.1–28.3%)
D. variabilisfemale511019.6% (10.8–32.6%)
male50612.0% (5.3–24.1%)
KentuckyA. americanumNR6100.0% (0.0–7.1%)[75]
D. variabilisNR4200.0% (0.0–10.0%)
MissouriA. americanumadult21000.0% (0.0–2.2%)[74]
nymph163 †18.8% (5.8–43.8%) †
D. variabilisadult7900.0% (0.0–5.6%)
Rhipicephalus sanguineusadult3500.0% (0.0–11.8%)
OklahomaA. americanumfemale4931.9% (1.5–17.2%)[62]
male4610.7% (<0.1–12.4%)
nymph8030.9% (0.8–10.9%)
D. variabilisfemale2300.0% (0.0–16.9%)
male2800.0% (0.0–14.3%)
PennsylvaniaIxodes scapularisNR100.0% (0.0–83.3%)[75]
TennesseeA. americanumNR18400.0% (0.0–2.5%)[75]
D. variabilisNR44281.8% (0.9–3.6%)
TexasA. americanumNR15800.0% (0.0–2.9%)[75]
D. variabilisNR9300.0% (0.0–4.8%)
Amblyomma cajennenseNR9900.0% (0.0–4.5%)
Amblyomma spp.NR6400.0% (0.0–6.8%)
Ixodes woodiNR100.0% (0.0–83.3%)
* NR: Not reported. † Ticks were recovered off a Cytauxzoon felis infected cat and cannot ascertain if ticks were infected or if they tested positive because of host blood.
Table
Table 4. Summary of molecular methods used for diagnosing Cytauxzoon felis in infected tissues.
Table 4. Summary of molecular methods used for diagnosing Cytauxzoon felis in infected tissues.
Method *Host SampleGene TargetAmplicon LengthPrimersReference
PCRBlood, other tissues18S284 bpF: 5′-GCGAATCGCATTGCTTTATGCT-3′
R: 5′-CAATTGATACTCCGGAAAGAG-3′		[88]
PCRBlood, other tissuescytb1203 bpF: 5′-AGGATACAGGGCTATAACCAAC-3′
R: 5′-GTACTCTGGCTATGTCAATTTCTAC-3′		[22]
PCRBlood, other tissuesITS2, partial 5.8S and 28S431 bpF: 5′-TGAACGTATTAGACACACCACCT-3′
R: 5′-TCCTCCCGCTTCACTCGCCG-3′		[28]
PCRBlood, other tissues18S82 bpF: 5′-TGC ATC ATT TAT ATT CCT TAA TCG-3′
R: 5′-CAA TCT GGA TAA TCA TAC CGA AA-3′		[19]
PCRBlood, other tissuesITS1651 bp (domestic cats)F: 5′-CGA TCG AGT GAT CCG GTG AAT TA-3′
R: 5′-GCT GCG TCC TTC ATC GAT GTG-3′		[19]
PCRBlood, other tissues746 bp (bobcats)F: 5′-CGA TCG AGT GAT CCG GTG AAT TA-3′
R: 5′-GGA GTA CCA CAT GCA AGC AG-3′
PCRBlood, other tissuesITS2475 bpF: 5′-AGC GAA TTG CGA TAA GCA TT 3′
R: 5′-TCA GCC GTT ACT AGG AGA-3′		[19]
PCRBlood, other tissues18SPrimary—700 bpF: 5′-ACCTGGTTGATCCTGCCAGTAGTCATATGCTTG-3′
R5′-TCACCAGAAAAAGCCACAAC-3′		[74]
Nested—289 bpF: 5′-TCGCATTGCTTTATGCTGGCGATG-3′
R: 5′-GCCCTCCAATTGATACTCCGGAAA-3′		[63]
ddPCRBlood, other tissuescox3118 bpF: 5′-CTACACTCTTTACACGTTTGTG -3′
R: 5′-AGGAGTATACTGGCATTTCG -3′		[90]
ISHFormalin-fixed, paraffin-embedded tissues16S-like600 bpF: 5′-CATGTCTTAGTATAAGCTTTTATACAGAA-3′
R: 5′-AACGCTGCGGAAGCGAGATTAATGACAAGGCAG-3′		[91]
* Abbreviations, PCR: polymerase chain reaction; ddPCR: droplet digital PCR; ISH: in situ hybridization.
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Reichard, M.V.; Sanders, T.L.; Weerarathne, P.; Meinkoth, J.H.; Miller, C.A.; Scimeca, R.C.; Almazán, C. Cytauxzoonosis in North America. Pathogens 2021, 10, 1170. https://0-doi-org.brum.beds.ac.uk/10.3390/pathogens10091170

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Reichard MV, Sanders TL, Weerarathne P, Meinkoth JH, Miller CA, Scimeca RC, Almazán C. Cytauxzoonosis in North America. Pathogens. 2021; 10(9):1170. https://0-doi-org.brum.beds.ac.uk/10.3390/pathogens10091170

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Reichard, Mason V., Tiana L. Sanders, Pabasara Weerarathne, James H. Meinkoth, Craig A. Miller, Ruth C. Scimeca, and Consuelo Almazán. 2021. "Cytauxzoonosis in North America" Pathogens 10, no. 9: 1170. https://0-doi-org.brum.beds.ac.uk/10.3390/pathogens10091170

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