Cytotoxic effect of oxaloacetate on a human hepatic carcinoma cell line HepG2 through apoptosis and ROS accumulation

Aim Oxaloacetate （OA） is one of the intermediates in the Krebs cycle. In addition to its role in the metabolism of energy production, OA may have other effects on the cell. We report in the present study that OA could have a cell type dependent cytoto^ic effect on the human hepatic carcinoma cell line HepG2 through induction of apoptosis and ROS accumulation. In our study, OA decreased the viability and colony formation of HepG2 cell and induced cell death. Caspase-3 activity was increased, pro-apoptotic protein Bax was up-regulated, and anti-ap- optotic protein Bcl-2 was clown-regulated in OA-treated HepG2 cells indicating that apoptosis through the intrinsic pathway was involved in the death of the cell. The level of reactive oxygen species （ROS） in OA-treated HepG2 cells was increased. Anti-oxidant N-acetylcysteine （NAC） and glutathione （GSH） prevented the viability of the cell induced by OA from decrease but could not alleviate the enhanced level of apoptotic Bax/Bcl-2 mRNA expres- sion ratio, which suggests that the OA-induced apoptosis of HepG2 cell is not driven by oxidative damage and at least two distinct mechanisms, one mediated by ROS and one involving apoptosis, lead to the cytotoxic effect of OA on HepG2 cells. These studies expand the biological functional repertoire of OA and provide a mechanism by which hepatocellular carcinoma may be targeted by OA to kill the cancer cells.

Establishment of 6VS Telocentric Lines of Haynaldia villosa Resistant to Powdery Mildew Induced by Immature Embryo Culture

The line of T240-6 was selected from 32 SC 2 lines of immature embryo culture of T240 (common wheat (Triticum aestivum L.)× Wheat-Haynaldia villosa (L.) Schur. 6D/6V substitution line) through powdery mildew characterization, glutamate oxaloacetate transaminase (GOT) enzyme and gliadin (Gli) analyses and in situ hybridization. All of the individual plants resistant to powdery mildew lacked the locus of GOT at 6VL arm (GOT-V 2) and had gliadin locus at 6VS arm (Gli-V 2) of Haynaldia villosa. All the plants resistant to powdery mildew had one or two telocentric chromosomes that did not pair with wheat chromosomes but paired between themselves. T240-6 was identified as a telocentric line through in situ hybridization.

Effects of Purified Indian Cattle Tick Rhipicephalus microplus Saliva Toxins on Various Enzymes in Blood Serum, Liver and Muscles of Albino Mice

In the present investigation, in vivo effects of purified ticks’ saliva toxin were evaluated on the level of certain important cellular metabolic enzymes i.e. acid phosphatase (ACP), alkaline phosphatase (ALP), glutamate pyruvate transaminase, glutamate oxaloacetate transaminase and lactic dehydrogenase. For this purpose, sub-lethal doses, 40% and 80% of 24 h LD50 purified saliva toxins of Rhipicephalus microplus (Canestrini, 1888) were injected subcutaneously in the albino mice. In treated mice saliva toxins targeted membrane-bound enzymes i.e. serum acid phosphatase and alkaline phosphatase, its level was increased from 118.30% to 163.63% at the 6th hr in comparison to the control. Besides this, the levels of serum glutamate pyruvate transaminase (GPT) and glutamate oxaloacetate transaminase (GOT) and lactic dehydrogenase (LDH) also increased up to 161.11% (at 6th hr), 148.27 (at 8th hr) and 125.45% (at 6th hr) respectively in comparison to control. An increase in the level of LDH showed insufficient oxygen supply, massive disintegration of cells and leakage of the enzyme into the circulation. It clearly indicated the toxic effects of saliva toxins on the membrane of blood cells, hepatocytes and myocardial muscle cell functions in albino mice. On the other hand activity of acetyl cholinesterase was reduced by 65.51% at the 6th hr of the saliva toxin injection in comparison to the control. This inhibition of acetyl cholinesterase activity caused the accumulation of acetylcholine molecules at the synaptic junctions and led to prolonged activation of acetylcholine receptors. It caused permanent stimulation of nerves and muscle cells that may result in muscular paralysis and finally death of the animal.

Effect of Purified Paper Wasp Ropalidia marginata Venom Toxin Enzyme Activity in Blood Serum, Liver, and Gastrocnemius Muscle of Albino Mice

In the present, investigation effects of sub-lethal dose of purified paper wasp Ropalidia marginata venom toxins were evaluated on important metabolic enzymes i.e. ALP ACP, GPT, GOT, LDH, and AchE enzyme activity in serum, liver, and gastrocnemius muscles of albino mice. Alkaline phosphatase was found to be increased up to 119.9% at the 6th hr of the toxin injection in comparison to control. This elevation may be due to cytolysis. Maximum increase i.e., 153.33% level of glutamate pyruvate transaminase (GPT) was found at 6 hrs of 40% of 24-h LD50 treatment while it was found to be 151.1% at 6 hrs of 24 hr 80% of LD50, venom injection. A significant elevation was observed in LDH activity in serum, liver, and muscles, while the activity of AchE was decreased in serum, liver, and gastrocnemius muscles of albino mice after injecting the sub-lethal dose of Ropalidia marginata venom. This increase in the activity of LDH produces liver damage, massive disintegration and necrosis of hepatic cells. This elevation in LDH level led to a significant increase in the glucose catabolism and elevated oxidative stress in muscle and liver cells. It also displays insufficient oxygen supply and consequently leads to cell death. In experimental animals, venom toxin treatment decreased AchE level, and animals showed muscular paralysis. When mice were treated with 40% and 80% of 24-h LD50 of purified venom caused a significant (p < 0.05) elevation in the level of ACP, GOT, GPT, and LDH while the reduction in ALP and AChE level. Present study will be useful in the development of prototypes for study of pharmacological and therapeutic effects of various venom toxins. For this purpose structure activity relationship of enzyme and venom toxin, its due interaction to various metabolic enzymes and receptors must be explored.

Functional analysis of OAT gene in Aspergillus Niger

Mitochondrial oxaloacetate transporter protein encoded by OAT gene transports oxaloacetate from cytoplasm into mitochondria. To investigate the primary effects of OAT gene on relative metabolism in Aspergillus niger, a oat-deleted mutant was derived from wild-type A. niger ATCC1015 using the double-crossover chromosome replacement technique. Then batch fermentation was performed to evaluate the mutant. Compared with the wild type, the mutant showed lower organic acids production, with the experimental data that the production of pyruvate and 2-ketoglutarate decreased by 31.6% and 35.7%, respectively, and by contrast, the mutant showed higher glycerol formation. The results suggest that OAT gene plays significant roles on metabolism in A. niger.

人类常用止痛剂布洛芬(Ibuprofen)及乙酰胺酚(Acetaminophen)对多齿新米虾(Neocaridina denticulate)的影响

近年来许多研究指出,人类长期使用的药物如抗生素或止痛剂等医疗药品,无法经由污水处理厂而完全分解消失,当这些药物进入环境中时将可能具有生物毒性,并对生态环境系统造成冲击。为了解人类常用止痛剂—布洛芬(ibuprofen, IBU)及乙酰胺酚(acetaminophen, ACE)残留于水体后对水生生物可能的影响。本研究应用多齿新米虾(Neocaridina denticulate,后简称米虾)进行0.1、1和5 mg/L的IBU及ACE不同浓度的曝露。并于曝露后1、4及7天,并测定米虾体内解毒酵素的活性(monooxygenase, Mon)及glutathione-S-transferase, GST)与肝胰脏受损指标(glutamic oxaloacetic transaminase, GOT)及(glutamic pyruvic transaminase, GPT)。试验结果显示,米虾曝露IBU及ACE后1,4及7天,各处理组间Mon活性并无明显高于对照组(37.8 ± 9.1 ΔA650mm/30 min/mg),GST活性在曝露5 mg/L的IBU及ACE处理组中有明显上升的趋势;5 mg/L IBU处理组在7天时GOT及GPT有上升的情况,代表IBU可能米虾的肝胰脏造成影响。综合实验结果,止痛剂IBU及ACE等药物于水体中残留时,不但会诱发米虾的解毒机制,甚至可能造成肝胰脏的发炎的现象。初步结果显示,止痛剂IBU及ACE等药物残留于水体中确实会对水生生物生理上的影响,此等问题势必会成为环境生态重要议题之一。