Hepatotoxins in Small Animals

Wide interindividual differences in clinical signs are observed among affected dogs. This diversity may reflect differences in pharmacogenetics (cytochrome P450 activity, GSH transferase activity) affecting toxin biotransformation or detoxification, the amount and duration of toxin exposure, nutritional status of the patient (poor nutritional support can decreased hepatic GSH concentrations), interactions with other toxic insults, antecedent disease processes or drugs that might induce P450 activity, patient age (younger animals have greater risk), and nutritional and hormonal status. 

With these considerations in mind, clinical signs of canine aflatoxicosis typically include anorexia, lethargy, vomiting and diarrhea, occasional polyuria and polydipsia, and gradual onset jaundice. Initial illness with slow chronic hepatotoxicosis is eventually followed by hematochezia or melena as well as development of an abdominal effusion (modified transudate, rarely hemorrhagic). 

Peripheral edema and abdominal effusion may emerge after IV fluid administration. Severe hepatic synthetic failure and hepatic parenchymal injury (parenchymal collapse) lead to loss of clotting factors, consumptive coagulopathy, and terminal signs of hepatic encephalopathy associated with severe enteric hemorrhage. 

In addition to hepatic synthetic failure, gastrointestinal bleeding may be a coumarin-related effect of aflatoxin as well as portal hypertension, provoking diapedesis of RBCs from capillaries into the enteric lumen. Acquired portosystemic shunts develop in dogs surviving > 4 weeks after onset of clinical signs. In some dogs with severe illness, enteral nutrition is thwarted by severe gastric and enteric atony that fails to respond to prokinetic agents.

Not all dogs die of aflatoxicosis despite demonstration of clinical illness. Resolution of abdominal effusion manifesting 60 days after illness onset was followed by resolution and apparent full recovery in some dogs given supportive care. Preexistent necroinflammatory liver disease may increase vulnerability of some dogs. Conversely, inappetence due to unrelated causes (ie, hypoadrenocorticism associated with anorexia, severe diffuse vacuolar hepatopathy that may have slowed toxin delivery to hepatocytes or altered hepatocyte metabolism, and intestinal malabsorption that deterred toxin absorption) has protected some dogs from fatal toxicity.

Experimentally, pretreatment with phenobarbital increases metabolism of AFB1 to less toxic metabolites with biliary elimination compared to formation of the AFB1 8,9 epoxide adduct. There is no benefit from phenobarbital after toxin exposure.

There are no distinguishing hematologic features; thrombocytopenia often coordinates with development of coagulopathy. Electrolyte status reflects dehydration, losses incurred from vomiting and diarrhea, and third-space fluid sequestration associated with fluid therapy, hypoalbuminemia, and loss of microvascular integrity (suspected to be toxin related). 

While hepatotoxicosis is often heralded by marked increases in ALT and AST and lesser concentrations of ALP and GGT, aflatoxicosis is associated with wide variability in liver enzyme activities. This likely reflects the mode of hepatocyte death associated with aflatoxicosis orchestrated by mitochondrial-initiated apoptotic pathways (programed cell death) rather than necroinflammatory, cytotoxic, or coagulative necrosis. Further relevant to aflatoxicosis is that toxic effects impairing hepatocyte synthetic capabilities also blunt enzyme activity. 

Biochemical features reflecting impaired hepatic synthesis in dogs with aflatoxicosis include:

• development of hypoalbuminemia, hyperbilirubinemia, and hypocholesterolemia

• prolonged prothrombin time (PT) and activated partial thromboplastin time (aPTT) clotting times (factor insufficiency)

• low antithrombin and protein C activity

• hypofibrinogenemia

Coagulopathy likely reflects impaired protein synthesis as well as development of a consumptive coagulopathy with a possibility of released thromboplastic substances from damaged hepatocytes, decreased clearance of activated proteases, and a potential contribution from a suspected coumarin-like effect of aflatoxin. In some dogs the kidneys manifest injury by the presence of granular casts (only observed in animals that die).

While there are clear differences in median values of clinicopathologic parameters between dogs that survive and dogs that do not in large retrospective studies, these observations lack utility for single-patient prognosis. Rather, it is important to sequentially evaluate relative changes in parameters over time, usually over multiple weeks (4–16 weeks) of survival. Positive indicators included increase in cholesterol and albumin concentrations, decline of hyperbilirubinemia, and increased activity of protein C and antithrombin.

Variability in clinicopathologic parameters displayed among dogs with confirmed aflatoxicosis (2005 outbreak in North America), irrespective of survival outcome, included increased ALT (83%), AST (79%), ALP (44%), and GGT (44%) activities; hypocholesterolemia (72%); and subnormal protein C (96%) and antithrombin (96%) on initial assessments. Abnormal protein C, antithrombin, and cholesterol preceded development of clinical signs or were detected in dogs presenting only with hyporexia. On sequential testing, abnormalities in protein C, antithrombin, and cholesterol persisted beyond several weeks whereas serum liver enzyme activities remained nonspecific mildly increased or were within reference range in some dogs.

Markedly increased serum liver enzyme activities and overt hyperbilirubinemia (total bilirubin > 2.5 mg/dL, consistent with jaundice) were inconsistent laboratory features of early intoxication. This corroborates with experimental findings in dogs with chronic aflatoxicosis in which hyperbilirubinemia usually developed after ≥ 1 month of toxin exposure.

Ultrasound imaging discloses abnormal hepatic architecture in chronically affected dogs and dogs developing portal hypertension. Hyperechoic parenchyma reconciles with diffuse microvesicular lipid vacuolation of aflatoxicosis with hypoechoic hepatic nodules observed in dogs with regenerative nodules. Anechoic abdominal effusion, a thick edematous gallbladder wall, and large lymph nodes were observed in dogs with portal hypertension.  Occasionally, APSSs were observed (color-flow Doppler ultrasonography) after 4–6 weeks of illness.

Cytologic evaluation of liver aspirates from dogs with aflatoxicosis discloses diffuse microvesicular hepatocyte lipid vacuolation, rare degenerative hepatocytes, and sparse mononuclear infiltrates (lymphocytes, macrophages).

Definitive confirmation of aflatoxicosis is based on histologic changes in liver (see below) and confirmation of toxic levels of aflatoxin in consumed food, circumstantially linked with patient illness. Several samples of food from different areas of a bag of dry food should be analyzed because the toxin can be unevenly distributed.

Attempting to measure aflatoxin B1 in liver is usually unsuccessful due to its exceptionally short half-life (minutes), AFB1 being instantaneously converted to the AFB1-8,9, epoxide and other metabolites. As lapses of several days between tissue sampling and ingestion of contaminated foods are common in clinical patients, the determination of AFB1 or its metabolites is often unrewarding. That said, collection of urine or blood samples in animals still consuming the suspected aflatoxin-contaminated food may reveal presence of the M1 metabolite, M1 having a half-life < 12 hours.

One study analyzing the M1 metabolite in liver from dogs dying of aflatoxicosis confirmed its presence in 7 of 8 samples. However, this complex analytic procedure is not routinely used as a diagnostic test.

Different species vary greatly in their susceptibility to AFB1, with dogs being highly susceptible. While a zero tolerance for aflatoxin is suggested by the Food and Drug Administration for humans, a legal limit of 20 mg/kg (ppb) food is imposed for human and dog foods. For dog food, toxic concentrations > 60 mg/kg (ppb) feed and lethal concentrations of 500–1,000 mg/kg (ppb) food are recognized.

In outbreaks of canine foodborne aflatoxicosis since 2005, the causal source was corn distributed in manufactured foods and in one instance was home-cooked polenta added to a homemade ration. While the thermal stability of aflatoxin B1 is disrupted at 160°C, polenta is made in boiling water (~100°C).

Among these outbreaks, aflatoxin food contamination ranged from 48 to 800 ppb food (2005, US, commercial food) up to 4,946 ppb food (2011, South Africa, commercial food) and 1,640 to 1,770 ppb (2011, southern Brazil, polenta scraps).  Based on experimental work, dogs exposed chronically to 0.05–0.3 mg AFB1/kg of feed over 6–8 weeks demonstrated chronic illness, eventually dying of liver failure and hemorrhagic diathesis with a cirrhotic liver.

The median lethal dose (LD₅₀) of AFB1 for dogs is 0.5–1.5 mg AFB1/kg with death occurring within 3 days; the LD₅₀ of AFB1 for cats is reported as 0.3–0.6 mg/kg. It is rare to encounter aflatoxicosis in pet cats, likely because of their carnivore dietary formulations.

Histopathologic features consistent with aflatoxicosis are not pathognomonic for this cause of hepatic injury; rather, they reflect a pattern observed in hepatotoxicosis targeting nucleoprotein integrity, gene transcriptional responses, mitochondrial function, and oxidative damage. The magnitude of liver enzyme activity does not reconcile with the severity of hepatocellular injury observed in clinical patients with aflatoxicosis. This phenomenon was also described in dogs sequentially monitored with chronic experimental aflatoxicosis.

A consistent histologic feature is microvesicular hepatocyte lipid vacuolation, initially with a centrilobular tropism that becomes panlobular. Additional features include canalicular bile plugs reflecting hepatocyte canalicular membrane injury, areas of parenchymal collapse (hepatocyte degeneration, initially centrilobular), with moderate to marked Kupffer cell and macrophages accumulation of lipofuscin (pigment reflecting oxidized membrane debris) and iron (released from the hemoprotein cytochrome P450 with hepatocyte death). 

Depending on chronicity, variable ductular reaction (cholangiocyte proliferation) and bile duct hyperplasia reflect regeneration of viable progenitor cells and interference with bile flow imposed by tissue injury/remodeling. Variable mixed lymphocyte and macrophage infiltrates in central and portal regions reflect nonspecific reactions to cell injury and response to cytokine elaboration by activated macrophages. Aflatoxin B1 has been shown experimentally to provoke macrophage activation, thereby increasing inflammatory cytokine expression. In the later stage of injury, nodular hyperplasia and dissecting fibrosis are evident.

Necrotic hepatocytes are rarely observed. Rather, apoptotic hepatocytes with condensed cytoplasm with nonfragmented pyknotic nuclei without adjacent inflammatory infiltrates are observed. Hepatocyte death in aflatoxicosis coordinates with downregulation of antioxidant enzymes (catalase and GSH peroxidase) that are typically upregulated in a necroinflammatory process or oxidative cause of cell death, and upregulation of genes involved with death receptor-initiated apoptosis (associated with mitochondrial injury).

Despite intensive supportive care including judicious administration of fluids, potassium, water-soluble vitamins vitamin K, blood component therapy, N-acetylcysteine (NAC) constant-rate infusion every 8 hours, oral SAMe in dogs that could tolerate oral medications, oral vitamin E supplements, control of gastric acidity and esophageal reflux, and antimicrobial coverage, mortality rate among dogs with inappetence, vomiting, and evidence of synthetic failure was approximately 65%.

Lower mortality rate was observed in dogs without or with only minor clinical illness, despite evidence of liver injury and modest hemostatic abnormalities. When confronted with an outbreak of suspected aflatoxicosis, determination of cholesterol concentrations and measurement of protein C and antithrombin activities, looking for subnormal values, can be used to incriminate exposure. These parameters appear to function as biomarkers of aflatoxin-suppressed synthetic function.

Liver enzymes and total bilirubin concentrations cannot be relied upon to accurately identify these dogs. Dogs with suspected exposure should be treated with removal of the suspected toxin-laden food, administration of hepatoprotectants (IV NAC recommended early) combined with oral bioavailable SAMe and vitamin E, and parenteral vitamin K administration every few days. Blood component therapy is reserved for animals with spontaneous bleeding.

Sequential surveillance of cholesterol, albumin, protein C, antithrombin, and if jaundiced, total bilirubin allows prediction of recovery over several weeks. These animals are given hospitalized care for only a few days until it is clear they are not destabilizing. No treatment can accelerate recovery. Recovery occurs if there are enough hepatocytes with replicatory and synthetic capabilities.

Clinical evidence of A phalloides syndrome is not obvious until extensive liver or renal injury has occurred; this ranges from hours to several days after exposure. Four phases of amanitin toxicosis are characterized:

1. The initial latent phase lasts for up to 12 hours.

2. The gastrointestinal phase develops ~6–24 hours after toxin ingestion, persisting up to 36 hours. Clinical signs include abrupt onset of nausea, vomiting and diarrhea (often bloody), abdominal pain, and hematuria. Dehydration, electrolyte disequilibrium, and hypoglycemia may develop. Immediate gastrointestinal signs may reflect phallotoxins also present in toxigenic mushrooms.

3. The hypoglycemic phase reflects glycogen utilization in the face of hepatic synthetic failure (impaired gluconeogenesis) and can lead to death if euglycemia is not achieved with IV fluid supplementation.

4. The final hepatorenal phase reflects severe progressive hepatic necrosis and is characterized by development of jaundice and clinicopathologic markers of escalating liver failure, worsening coagulopathy, and emergence of hepatic encephalopathy and renal failure.

Notably, dogs ingesting large amounts of amanitin may die without developing classic phased progression.

Presumptive diagnosis of amanitin hepatotoxicity is usually based on circumstantial association of observed mushroom ingestion, clinical signs, biochemical features, and histologic liver lesions. However, definitive detection of alpha-amanitin in serum, urine, gastric contents, suspect mushrooms, liver, or kidneys can be done by select veterinary toxicology laboratories. The Meixner test for rapid amatoxin detection does not provide definitive identification and can be misleading.

Serum, urine, and tissue sections from animals dying from suspected amanitin toxicosis should be frozen if subsequent definitive testing is desired. Serum and urine samples should be saved as early in the illness prodrome as possible because with time the circulating toxin diminishes. In dogs an LD₅₀ of 0.11 mg/kg alpha-amanitin had been determined.

Experimental alpha-amanitin hepatotoxicity in dogs given 0.09 mg/kg, PO, once (study done to evaluate utility of IV silibinin over 30 years ago), provides details regarding canine amanitin toxicity. No clinical signs were manifest for 16 hours. Thereafter, vomiting and bloody diarrhea commenced, peaking at ~48 hours. 

Survivors improved rapidly after ~60 hours. Extreme increases in ALT (~180× baseline), AST (50× baseline), and lesser increases in ALP (6× baseline), GGT (2× baseline), and bilirubin (6× baseline) developed by 48 hours. Within this time frame, marked prolongation of the prothrombin clotting time was also documented. Dogs that died of amanitin toxicosis became azotemic (increased BUN and creatinine concentrations) and developed enteric bleeding and terminal hepatic encephalopathy between 35 and 54 hours. 

Hyperammonemia reflects decreased hepatic ammonia detoxification due to FHF and may be provoked by renal azotemia and enteric hemorrhage. While the magnitude of documented transaminase activity is extreme, it is possible that these are somewhat limited by severe hepatic synthetic failure. With onset of synthetic failure, hypoglycemia, hypoalbuminemia, and hypocholesterolemia simultaneously emerge.

Dogs surviving experimental amatoxin toxicosis had normalization of clinicopathologic abnormalities by 192 hours. Despite attempts to normalize alpha-amanitin dosing among studied dogs, 4 of 12 died. This may reflect variable distribution of toxin within the mushroom extract or individual variation in toxin tolerance. 

Bleeding diathesis is an important complication of amanitin hepatotoxicity that requires administration of fresh frozen plasma. Simple vitamin K administration cannot arrest this process. Hepatic synthetic failure provokes coagulopathy due to loss of pro- and anticoagulant proteins, altered activity of fibrinolytic proteases, and release of tissue thromboplastin from hepatic necrosis. Consumptive coagulopathy escalates bleeding complications and causes the appearance of schistocytes in the early phase of tissue injury. Bleeding complications and development of disseminated intravascular coagulation (DIC) complicate tolerance of liver injury and contribute to multiorgan failure in lethal amanitin hepatotoxicity.  

While nephrotoxicity is common, it is far less critical than hepatotoxicity. Renal azotemia secondary to acute tubular necrosis is associated with active urine sediment characterized by the appearance of numerous hyaline and granular casts. Rarely, an acquired Fanconi renal tubular acidosis also develops.

In acute lethal toxicity, the liver is swollen, may have a friable texture and mottled red and yellow pallor, and may display subcapsular hemorrhage. The yellow pallor reflects diffuse lipid vacuolation of residual hepatocytes.

Histologic features are dominated by massive centrilobular to panlobular coagulative and hemorrhagic necrosis with loss of sinusoidal architecture. Rare residual viable hepatocytes abut normal-appearing portal elements; these hepatocytes demonstrate microvesicular lipid vacuolation and vacuolar degeneration. Centrilobular and subcapsular congestion and hemorrhage are usually obvious. There are limited inflammatory infiltrates.

There is no internationally accepted protocol for treatment of amanitin hepatotoxicity in humans; an IV form of silibinin is the preferred intervention. With acute presentation, decontamination is critical. Unfortunately, many poisoned dogs are not presented until after onset of clinical signs, such that gastric lavage is likely too late. After evacuating the stomach (self-induced vomiting, therapeutically initiated vomiting, or possible gastric lavage), activated charcoal (with sorbitol if there is no diarrhea) is used absorb the remaining toxin. This may also interrupt the enterohepatic circulation of amanitin. Oral and rectal administration routes may be used. 

There are no data supporting utility of cholestyramine for capture of amatoxin. Concurrently, critical supportive care includes the following:

• IV fluid therapy

• electrolyte adjustments

• maintenance of euglycemia with supplemental IV glucose

• blood component therapy (usually fresh frozen plasma) to address complicating coagulopathy

• antioxidants (IV N-acetylcysteine, oral bioavailable SAMe)

• combinations of drugs thought to compete with amanitin OATP transport into hepatocytes and that block its enterohepatic circulation (high-dose penicillin G and IV silibinin; see below)

Adequate fluid therapy may be renal protective because amanitin is easily filtered via glomeruli; this toxin does not undergo renal tubular reabsorption.

Patient survival depends on the extent of hepatic injury, ability of surviving hepatocytes to regenerate, and management of systemic complications secondary to acute hepatic failure. In humans, liver transplantation is the salvage therapy for amanitin-induced FHF. Extracorporeal elimination (hemodialysis, hemoperfusion, or plasmapheresis) for removal of circulating amatoxin is thought to have limited value because amatoxins are only detected in plasma at the early phase of toxicosis and only for a short period of time. Newer extracorporeal techniques involving fractionated plasma separation and adsorption systems scavenge both protein-bound and water-soluble moieties and have shown benefit in humans with preclinical toxicity.

Specific measures aimed at limiting amanitin cellular uptake are predicated on the basis of experimental data from canine studies and observational deductions derived from human patients with Amanita hepatotoxicity. These include use of high-dose penicillin G or benzylpenicillin and high-dose IV silibinin to competitively block amanitin OATP transport. In humans, penicillin is dosed at 1,000,000 U/kg on day 1, 500,000 U/kg on days 2 and 3, and then discontinued. While there are multiple reports demonstrating circumstantial benefit, there is no consensus regarding efficacy of this treatment. In dogs, penicillin G given at a dose of 1,000 mg/kg, IV, every 5 hours after toxin ingestion appreciably decreased hepatic amanitin accumulation.

Silibinin, a flavonolignan derived from seeds of the milk thistle fruit, represents a mixture of two diastereomers, silibinin A and silibinin B.  Mechanistically, silibinin competitively inhibits OATP amanitin transport into hepatocytes and during its subsequent enterohepatic circulation. Silibinin also affords benefit via suppression of TNF-alpha released from damaged tissues (thought to contribute to live injury) and via its antioxidant properties. IV silibinin is a bioavailable microcrystalline hydrosoluble ester of silibinin (with succinic anhydride); intravenous administration allows high-dose delivery not attainable by oral silibinin containing products. This product is not licensed for sale in the US and is acquired under a compassionate use assignment or from a European distributor.

The human protocol for amanitin toxicosis is to provide IV silibinin at 5 mg/kg during the first hour of presentation, followed by 20 mg/kg/d as a constant-rate infusion for 3 days. Alternatively, 20–50 mg/kg/d, IV, is continued for 3 to 4 days. There is no recommended limit on duration of silibinin administration because there are no recognized adverse effects. Studies in dogs with amanitin hepatotoxicosis suggest similar safety.

In early canine studies, IV silymarin administered at 50 mg/kg at 5 hours after amatoxin ingestion, repeated at 30 mg/kg at 24 hours, afforded hepatoprotection. In humans, IV silibinin administered up to 48 hours after amanitin ingestion also appears to prevent severe liver damage.

Rapid-onset lethargy, anorexia, and vomiting follow within 1–2 hours of toxin ingestion, with abrupt development of jaundice in dogs challenged by severe MC-LR exposure. With severe toxicity, continued inappetence and vomiting, escalating jaundice, and development of coagulopathy (surface hemorrhages, epistaxis, hematemesis, melena) ensue. However, exposure to sublethal levels of MC-LR may initially pass unnoticed without clinical signs or biochemical abnormalities.

Dogs with single high-dose MC-LR exposure develop extreme increases in hepatic transaminase activity (ie, ALT and AST, 80–200× reference limits), with modest increases in ALP activity (~1.5–2.0× reference limits) and marked hyperbilirubinemia (7.0–12× reference limits) within 24 hours. Liver enzymes escalate over several days with fold increases in transaminases far exceeding those of ALP. Hyperbilirubinemia also worsens. In severe acute toxicity, lethal fulminant liver failure is associated with coagulopathy, hypocholesterolemia, hyperammonemia, and hepatic encephalopathy. 

Recovery is possible in severely impacted dogs given supportive care (IV fluids, vitamin K, blood component therapy, antioxidants, and cholestyramine). Complete resolution of enzyme activity and hyperbilirubinemia may take up to several months in survivors. Exposure to sublethal levels of MC-LR may pass unnoticed without alarming increases in liver enzymes or hyperbilirubinemia.

In acute severe lethal MC-LH hepatotoxicity, the liver appears swollen with rounded margins and has a dark red color due to the severe centrilobular hemorrhagic necrosis. Jaundiced tissues and surface hemorrhages are common in dogs with FHF. Animals with chronic sublethal MC-LR may have no overt changes.

Acute severe MC-LH hepatotoxicity leads to massive centrilobular and midzonal hepatocyte hemorrhagic necrosis with congestion in areas of parenchymal collapse. Few remaining viable hepatocytes abut portal tracts. Retained viable hepatocytes have poorly defined cell-to-cell attachments and display mild microvesicular lipid vacuolation. Based on studies in rodents, chronic low-dose MC-LH exposure leads to centrilobular microvesicular lipid vacuolation, loss of centrilobular sinusoidal organization, and abnormal nuclear chromatin clumping without evidence of apoptotic or necrotic cell injury. These changes are completely reversible within several months after removal of chronic low-dose MC-LH exposure.

Supportive care as described for FHF is indicated for dogs with severe acute MC-LH hepatotoxicity. Because oxidant injury is an early pathomechanism, IV N-acetylcysteine is advised. Oral bioavailable SAMe (20 mg/kg, PO, every 24 hours) and water-soluble vitamin E (10 U/kg, PO, every 24 hours) are given when the animal can tolerate enteral medications, and phosphatidylcholine (25–50 mg/kg, PO, every 24 hours) is advised to support membrane recovery and stabilization. 

Because MC-LR undergoes enterohepatic circulation and has been shown to bind with cholestyramine, this binding resin should be used to remove recycling toxin. As there appears to be site-specific binding in the ileum, if oral cholestyramine is not possible because of vomiting, administration by high rectal installation is advised. High-dose IV silymarin has also been shown to be beneficial; this form of silymarin is commonly available in Europe but not in the US.

Clinical signs vary in respect to the lag time between toxin ingestion and initial presentation. In acutely intoxicated dogs (< 24 hours), signs commonly include vomiting and in declining frequency, diarrhea, hyporexia, lethargy, ptyalism, polydipsia, neurologic signs (ataxia, confusion, somnolence, obtundation, head pressing, rare seizures), GI bleeding (melena or hematochezia), and muscle tremors. During acute presentation, physical examination may be within normal limits. Within 24–48 hours, findings may include dehydration, jaundice (< 30% initially, progresses over time), abdominal discomfort, and abdominal effusion (< 15% initially, may develop over time).

Although clinical signs may manifest within 4 hours of cycad ingestion, biochemical defects are often delayed for up to 72 hours. Initial ALT and AST activities may be within reference limits (within 24 hours) but then become mild to modestly increased. Increases in ALP activity lag behind trends in transaminases and are usually more modest unless there is progressive injury with tissue remodeling and biliary hyperplasia (ductular reaction). Variably, hypoalbuminemia, hyperbilirubinemia, hypoglycemia, and hypocholesterolemia may manifest.

Prognosis is not possible based on simple first inspection of test results. Rather, case outcome is more related to sequential trends in test results over the first several weeks, then monitored biweekly. Coagulopathies often manifest several days after acute presentation but also may appear after several weeks.

Abdominal radiographs are often within normal limits, with the exception of decreased detail attributed to abdominal effusion. Abdominal ultrasonography may be within normal limits or disclose normal to small liver size (small liver with chronic toxicity), altered parenchymal echogenicity (hyperechoic to hypoechoic), abdominal effusion, a thick gallbladder wall consistent with lymphedema, and intestinal atony.

In dogs dying from acute MAMA hepatotoxicosis, gross appearance of the liver may show scattered red foci (reflecting centrilobular necrosis and congestion) or show pallor (reflecting severe anemia rather than lipid vacuolation). At necropsy, all tissues are typically jaundiced, with numerous surface hemorrhages, evidence of enteric bleeding (melena or hematochezia), and abdominal effusion. In dogs dying from chronic MAMA toxicity, the liver is small and nodular with APSSs and ascites. Jaundice, visceral hemorrhages, and enteric bleeding are also evident. 

Histologic features of acute toxicosis (0–2 days) include prominent centrilobular to midzonal hepatocyte and sinusoidal degeneration/necrosis, with severe regional congestion, parenchymal collapse, and reactive neutrophilic infiltrates. Conspicuous expansion of the space of Disse and damaged sinusoidal endothelium (fenestra widening) distort sinusoidal organization and are associated with loss of intercellular adhesions. Modest microvesicular lipid vacuolation develops in periportal hepatocytes.

Numerous hepatocellular cytologic aberrations are also observed, including cell individuation (detachment from reticulin scaffolding and intercellular tight junctions); loss of polyhedral hepatocyte shape; marked hepatocyte anisocytosis and anisokaryosis; appearance of megalohepatocytes and cells with marked karyomegaly; clumped nuclear chromatin; prominent large, dense, and sometimes vacuolated nucleoli; and mitotic derangements generating polynucleated cells. Variable canalicular cholestasis also be observed.

Retrospective reports of dogs experiencing cycad toxicosis describe recoveries of 34% (n = 60, with suspected cycad toxicity, poison control data) and in dogs with confirmed cycad toxicosis 50% (n = 34) and 64% (n = 14). Two clinical phases of cycad toxicosis are recognized in dogs:

1. an acute phase characterized by gastrointestinal and neurologic signs, with evidence of a modest hepatic insult (based on finding normal or mildly increased liver enzyme activity and lack of hyperbilirubinemia)

2. a latent phase characterized by increasing liver enzyme activity, jaundice, and progressive synthetic failure, with development of sinusoidal hypertension causing portal hypertension and abdominal effusion

In some dogs acute toxicosis is seemingly managed successfully only to discover serious latent hepatotoxicity weeks to months later (ammonium biurate crystalluria, acquired portosystemic shunting, and severe hepatic parenchymal remodeling). Thus, it is important to explain to an owner this possibility. 

Initial decontamination is usually achieved via patient vomiting. If not, vomiting should be initiated if safe (see treatment for fulminant hepatic failure). Cleansing enemas followed by an activated charcoal enema should also be considered if plant material remains within the GI tract. Activated charcoal should be administered after vomiting ceases to be productive. If substantial gastric debris is noted on abdominal ultrasonography, endoscopy can be used to assist in decontamination.

Administration of activated charcoal was strongly associated with survival in one study. There is anecdotal observation that cholestyramine may accelerate recovery from MAMA toxicity. However, there is no information regarding enterohepatic circulation of this toxin. Otherwise, supportive care is used to judiciously adjust hydration and electrolyte status, provide water-soluble vitamins and antioxidant support (ie, NAC given IV, bioavailable SAMe if oral medications can be used), water-soluble vitamin E (10 U/kg, PO), antibiotics to protect against translocating opportunistic bacteria, and blood component therapy as needed. Treatment of hepatic encephalopathy may also be needed.