Impairments of glucose metabolism i

Impairments of glucose metabolism in liver. There are many studies investigating the effects of OP on liver metabolism. Fenthion induced hepatic glycogenolysis76. Exposure to fenitrothion elevated glycogen phosphorylase (GP) activity leading to a reduction in hepatic glycogen content.14,77 The same effect was reported following a 48-hour exposure to carbofuran.78 Subchronic exposure to malathion, enhanced hepatic gluconeogenesis and glycogenolysis, via stimulation of GP and phosphoenolpyruvate carboxykinase (PEPCK); whereas diazinon increased hepatic PEPCK.79-81 Dichlorvos reduced the activity of hepatic GK and liver glycogen content while hepatic GK mRNA levels were increased.65 In other studies, malathion lowered hepatic protein and lipid contents associated with stimulated gluconeogenesis, and increased hexokinase (HK) activity. In contrary to the above studies, malathion decreased hepatic GP activity with a rise in the hepatic glycogen rate (hepatomegaly).43,82,83 Acute exposure to acephate increased liver glycogen content and activities of gluconeogenesis enzymes, glucose-6-phosphatase (G6P), and tyrosine aminotransferase in the liver.36 Lactate dehydrogenase (LDH), a key enzyme in glycolysis, was elevated but succinic dehydrogenase (SDH) and ATPase activities that contribute to production of mitochondrial ATP were depleted in the liver post exposure to quinalphos.84 Moreover, an increase in LDH or a reduction in SDH activity in the livers and brains of exposed subjects to sublethal concentrations of sevin were reported.85 During exposure to fenitrothion, liver and bloodlactate levels increased; however, the protein content decreased.39 The increase of liver and muscle LDH reflects a possible improvement in tissue glycolytic capacity. In signaling cascade level, diazinon up-regulated adenyle cyclase activity, which is a response to stimulants acting on beta-adrenergic, glucagon, or G-protein receptors.86
Hepatic injury. Histochemical alteration in the liver can affect metabolism of carbohydrates, lipids, and particularly proteins. Sublethal doses of carbaryl and phorate increased alkaline phosphatase (ALP) and bilirubin.40 Chlorpyrifos and deltamethrin caused liver damage.87 Exposure to methidathion phosphorodithioic acid S-[(5-methoxy-2-oxo-1,3,4-thiadiazol3(2H)-yl)methyl] O,O-dimethyl ester (MD) induced histopathological changes, including recruited mononuclear cells in all portal areas, sinusoidal dilatation, and focal microvesicular steatosis and hydropic degenerations in parenchymal tissues.88,89 In addition, methylparathion increased liver weight.90 Leptophos, chlorpyrifos, and diazinon inhibited glutamic oxaloacetic transaminase (GOT), glutamic pyruvic transaminase (GPT), gamma-glutamyl transferase (GGT), and LDH.91 Two-bButenoic acid-3-(diethoxyphosphinothioyl) methyl ester (RPR-II) increased plasma GPT and GOT activities, but decreased these values in the liver. Meanwhile, it elevated plasma acid phosphatase (AcP) and ALP and reduced hepatic AcP and ALP levels.92 Finally, dimethoate increased serum urea, total bilirubin, GOT, GPT, and amylase.38,93
Impairments of protein metabolism. OP are known to alter serum levels of amino acids.94,95 For instance, carbofuran decreased liver and muscle total protein. Isofenphos-treated myeloid blast cells showed an increase in lactate production and a decrease in glucose oxidation and the synthesis of glutamate, palmitate, and stearate from glucose.96 It is suggested that pesticides reduce tissue protein content because of glucose production in gluconeogenesis process and also because of inhibition of protein synthesis.
protein expression as a protective mechanism104 reveal muscle injury in response to OP. On the other hand, muscle fasciculation after release of ACh made an extra energy demand that stimulates gluconeogenesis. Therefore, the protein and glycogen stores decreased. Accumulation of lipids inside the muscle occurred following exposure to isofenphos105 probably due to downregulation of metabolic activity in fat tissues.
Lipid metabolism impairments and obesities. The association between OC and homeostatic model assessment-insulin resistance (HOMA-IR) tended to strengthen as waist circumference increased. OC and nondioxin-like PCB can elevate triacylglycerol and fasting glucose that along with obesity can increase the risk of type 2 diabetes.21,106 Diacylglycerol metabolism is the probable target for chlorpyrifos oxon, and in chronic exposure, chlorpyrifos caused an increase in rat body weight via increasing adipose tissue.107,108 Parathion exposure increased weight gain and evoked signs of a prediabetic state, with elevation in fasting serum glucose and impaired fat metabolism.109 Chronic exposure to sublethal doses of dimethoate markedly increased cholesterol levels, whereas DDT lowered blood cholesterol and fatty acids.38,63,110 Ronnel downregulated the metabolic activity in adipose tissue.100 In addition, accumulation of fatty acids in