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P.C. Chikezie
Abstract: In the present in-vivo study, the capacities of five antimalarial drugs (Fansidar, Halfan, Quinine, Coartem and Chloroquine phosphate) to alter/distort methaemoglobin concentrations of three human erythrocyte genotypes (HbAA, HbAS and HbSS) was investigated. Spectrophotometric method was used to ascertain this erythrocyte parameter. The male participants enrolled for this study were grouped according to their genotypes, pathologic status, (that is, non-malarious and malarious individuals). Determination of erythrocyte methaemoglobin concentration was carried out before (control; t = 0 h) and after (tests; that is, at t = 3, 6 and 18 h) the five (5) antimalarial drugs were administered to various corresponding groups of participants. The results showed that methaemoglobin concentrations of these individuals ranged between 1.45+/-0.13 and 2.50+/- 0.43%; 8.27+/-2.41 and 14.78+/-2.45%, for non-malarious and malarious male individuals respectively. There was no significant difference (p > 0.05) between methaemoglobin concentrations of HbAA and HbAS erythrocyte of non-malarious participants. The doses of the five antimalarial drugs administered to non-malarious individuals did not cause toxic methaemoglobinemia. Under the same experimental conditions, erythrocytes obtained from persons of HbSS genotype exhibited significant (p < 0.05) elevation of methaemoglobin concentration. Relatively high levels of methaemoglobin concentration of parasitized red blood cells decreased in a time dependent manner after administration of the five antimalarial drugs. Therefore, erythrocyte methaemoglobin evaluation is a reliable biochemical marker and rational for diagnostic and therapeutic potential in malaria. Furthermore, moderate increases of erythrocyte methaemoglobin in HbSS individuals served as point of caution when administering these drugs to this category of human subjects.[...] Read More.
Keywords: Antimalarials, erythrocyte, malaria, genotype, methaemoglobin.
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文章
H. Belguith*, S. Fattouch, T. Jridi and J. Ben Hamida
Abstract: Lipase or triacylglycerol acylhydrolase (E.C.3.1.1.3) was purified to homogeneity from rapeseed-germinated cotyledons (Brassica napus L.). The purification scheme involved homogenization, centrifugation, ultracentrifugation and affinity chromatography using polyclonal antibodies raised against porcine pancreatic lipase. The purified rapeseed lipase was homogenous and did not contain contaminating proteins detectable by SDS-PAGE and HPLC analysis. The specific activity of the purified preparation was increased about 1950 times, with an overall yield of 35%. The rapeseed lipase was found to be a cytosoluble, glycosylated and heat-labile serine-hydrolase. It was monomeric with a molecular mass of 38 kDa and a pI of 6.6. The purification method used in the present work is rapid, simple and yields highly purified lipase. It may therefore be applicable in the purification of other uncharacterized plant lipases.[...] Read More.
Keywords: Brassica napus L., immuno-affinity, lipase, purification, triacylglycerol acyl hydrolase.
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文章
S.  Alagendran, K. Rameshkumar, K. Palanivelu, N. Puspha, M. Ranjani, N. Arulmozhi and G. Archunan*
Abstract: The present study was carried out to detect amino acids profile in women saliva in order to establish the qualitative and quantitative differences that might have potential value in detection of ovulation by noninvasive methods. For the collection of sample, the stages of menstrual cycle were decided by the physical and morphological examination of salivary fern pattern. The saliva from various reproductive phases (prepubertal, preovulatory, ovulatory, postovulatory phases and menopause) was collected and analyzed by reverse phase high performance liquid chromatography (HPLC) after precolumn derivitization of amino acids using O-Pthaldehyde (OPA) by means of RP-HPLC amino acid analyzer. Among the various amino acids identified the compounds such as tryptophan, arginine and phenylalanine were comparatively found to be higher during ovulatory phase when compared to that of other phases. The increase in amino acid concentration during ovulatory phase may be due to the circulation of steroid hormones. Thus, the presence of specific amino acids in ovulatory saliva makes the possibility to develop a biomarker for detection of ovulation by noninvasive methods.[...] Read More.
Keywords: Ovulation steroid hormones, O-Pthaladehyde, chromatography, amino acids.
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Shohda A. EL-Maraghy, Sherine M. Rizk and Maha M. El-Sawalhi*
Abstract: The present study was undertaken to evaluate the possible ameliorating effect of crocin and curcumin on certain biochemical alterations associated with iron overload-induced liver injury in rats. 5 groups of rats were used, a normal control group received daily i.p. injections of saline and 4 groups received daily i.p. injections of ferric nitrilotriacetate (FeNTA) for 8 successive days, the dose of iron was increased during the experimental period (from 6 to 15 mg Fe/kg). The first iron overloaded group kept without further treatment and served as a positive control group. The second iron overloaded group received daily i.p injections of crocin (200 mg/kg) in saline. The 3rd and the 4th iron overloaded groups received orally either 0.5% carboxy methyl cellulose (CMC) or curcumin (100 mg/kg) in CMC respectively. Treatment started 3 days before and concurrently with iron administration for 8 days. Results revealed that iron- induced liver injury was reflected by significant changes in the liver function indices, hyperammonemia and reduced serum urea level. A significant deposition of iron in liver was associated with enhanced oxidative and nitrosative stress status. Moreover, iron overloaded rats exhibited significant alterations in liver energy metabolism together with diminished ureogenesis and a decline in dimethylarginine dimethylaminohydrolase activity. Supplementation with either crocin or curcumin ameliorated most of the biochemical changes induced by iron overload in rat liver. A function that may be beneficial for populations at risk for iron overload.[...] Read More.
Keywords: Iron overload, liver, rat, oxidative stress, energy metabolism, ureogenesis, crocin, curcumin.
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Saeed Nazifi*, Mahdi Saeb, Hasan Baghshani and Saeedeh Saeb
Abstract: Transportation causes stress in livestock that may alter numerous physiological variables with a negative impact on production and health. The objective of the current study was to investigate the effects of road transport on oxidative stress biomarkers in camels. Ten Iranian dromedary camels were selected and subjected to a journey of approximately 300 km in a truck by road in August 2008. Blood samples were collected immediately before loading at 8:30 A.M., after 1 h transportation, at 9:30 A.M., and at the end of the journey after unloading at 1:30 PM. Final blood sample was taken 24 h after arrival. Plasma concentrations of malondialdehyde and a-tocopherol, erythrocyte superoxide dismutase and whole blood glutathione peroxidase activities were measured using validated methods. The mean concentration of MDA (1.87 ± 0.26 nmol/mL) and glutathione peroxidase activity (297.86 ± 25.68 U/g Hb) in basal pre-transport conditions show significant increase 24 h after arrival. The mean concentration of a-tocopherol (5.22 ± 0.74 mol/L) and superoxide dismutase activity (1742.5 ± 74.36 U/g Hb) in basal pre- transport conditions had no significant change during and after transportation. Results suggest that transport stress causes an oxidative challenge in dromedary camels and represent novel biomarkers for stress-associated disease susceptibility and welfare assessment. However, further research efforts should be directed towards understanding the role of particular antioxidants and oxidants on the stressful conditions.[...] Read More.
Keywords: Dromedary camel, road transportation, oxidative status, malondialdehyde, a-tocopherol, glutathione peroxidase, superoxide dismutase.
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C. Egwim Evans and O. Adenomon Monday
Abstract: Alpha amylase yield in sprouting Maize, Acha, Rice and Sorghum were studied for 180 h. The result was analyzed using 2nd order polynomial model. The result showed that the rate of - amylase secretion with growth period is significantly high (p < 0.05) and the R2 for each ranged from 67 - 90%, while the R2 for sprouting vigour ranged within 99% for all the cereals studied. The prediction for amylase activity from sprouting vigour was significant (p < 0.05) for all the cereals studied, the R2 for all the cereals ranged between 63 - 91%. The results conclude that a-amylase and malt quality can be predicted in sprouting cereals from the growth vigour.[...] Read More.
Keywords: Cereals, amylase, growth vigour, model.
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H. O. T. Iyawe* and A. O. Onigbinde
Abstract: This work aimed at examining the effect of malaria parasites and ascorbic treatments in mice. The relevance of this research derives from the desire to understand the role of ascorbic acid in malaria infection. In this study design, three groups of ten mice each categorized as non-parasitized-non-treated (control), parasitized-non-treated (PnT) and parasitized ascorbic acid treated (P+asT) were used. Results collected and analyzed using adequate statistical software revealed that parasitism in mice had significant (p < 0.05) increases in erythrocyte fragility, total and indirect bilirubin, total protein and globulin but decreased (p < 0.05) mice packed cell volume (PCV). Plasma malondialdehyde (MDA) significantly (p < 0.05) increased while superoxide dismutase (SOD) and catalase (CAT) decreased (p < 0.05). Liver SOD and CAT as well as kidney MDA of parasitized non treated mice were observed to increase (p < 0.05) following Plasmodium berghei infection. Ascorbic acid treatment of parasitized mice was observed to reverse the effects of P. berghei in mice. The findings suggest ascorbic acid to be critical in the management of malaria parasite infection.[...] Read More.
Keywords: Plasmodium berghei, ascorbic acid, antioxidants, erythrocyte fragility, oxidative stress.
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Suzana Makpol*, Nur Nadia Mohd Arifin, Zahariah Ismail, Chua Kien Hui, Yasmin Anum Mohd Yusof and Wan Zurinah Wan Ngah
Abstract: Melanin is the pigment that determines skin color. Melanin synthesis is catalysed by the enzyme tyrosinase and is controlled by TYR, TYRP1 and TYRP2 genes. The objective of this study was to evaluate the anti pigmentation property of palm tocotrienol rich fraction by determining melanin synthesis and expression of genes involved in its regulation in skin melanocytes. Palm tocotrienol rich fraction (TRF) which contains 75% a-tocotrienol and 25% tocopherol was used to inhibit melanin synthesis which was determined by determining melanin level and tyrosinase enzyme activity. Expression of TYR, TYRP1 and TYRP2 genes was determined by quantitative real time reverse transcriptase polymerase chain reaction (real time RT-PCR). Primary culture of skin melanocytes was divided into two groups; untreated control and cells that were treated with 500 µg/ml tocotrienol rich fraction for 24 h. Our results showed that there was a reduction in tyrosinase activity and melanin content in melanocytes treated with tocotrienol rich fraction compared to control (p < 0.05). Expression of TYRP2 gene in melanocytes treated with tocotrienol rich fraction was also decreased (p < 0.05) compared to control. In conclusion, palm tocotrienol rich fraction has an anti pigmentation property that inhibit melanin synthesis by inhibiting tyrosinase activity and down regulating TYRP2 gene expression.[...] Read More.
Keywords: Melanin synthesis, gene expression, tocotrienol rich fraction, skin melanocytes.
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Soria Baouz, Anne Woisard, Lila Chenoune, Gustave Aguié, Gérard Keith, Jean-Marie Schmitter, Jean-Pierre Le Caer and Codjo Hountondji*
Abstract: Periodate-oxidized tRNA (tRNAox), the 2’,3’-dialdehyde derivative of tRNA, was used as a zero-length active site-directed affinity labeling reagent, to covalently label proteins at the peptidyl transferase center (PTC), the catalytic site of the large ribosomal subunit. When human 80S or Escherichia coli 70S ribosomes were reacted separately with tRNAox positioned at the P-site, in the presence of an appropriate 12 mer mRNA, a set of two tRNAox- labeled ribosomal proteins was observed. These proteins referred to in this work as rPox1 and rPox2 exhibited comparable physico-chemical properties including apparent molecular weights. In the case of human 80S ribosome, the protein present in the major labeled tRNA- rPox1 covalent complex was identified as the 60S ribosomal protein L36a-like (RPL36AL) by mass spectrometry. The molecular weight of the minor labeled tRNA-rPox2 covalent complex was estimated from the data of the 1-D SDS-PAGE, and a deduced molecular weight of 34,000+  2,000 Da for the ribosomal protein referred to as rPox2 designated protein RPL5 as the candidate minor labeled protein of human 80S ribosome. Search for candidate ribosomal proteins for the tRNAox-labeled proteins rPox1 and rPox2 of 70S ribosome from E. coli designated RPL2 (M.W. 29,860 Da), the largest eubacterial rP as the tRNAox-labeled protein corresponding to the minor labeled human RPL5, and RPL15 (M.W. 14,980 Da) or RPL16 (M.W. 15,281 Da) as corresponding to the major labeled human RPL36AL.[...] Read More.
Keywords: Human 80S or E. coli 70S ribosomes, peptidyl transferase center, human RPL36AL, RPL5/P-site or A-site tRNA, periodate-oxidized tRNA.
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M. Ahanjan, M. P. Raghavendra , and K. A. Raveesha*
Abstract: Aqueous and methanol extracts of Parrotia persica leaves were assayed for antifungal activity against phytopathogenic Fusarium oxysporum and human pathogenic Candida albicans by poisoned food technique. Both the aqueous and methanol extracts demonstrated significant antifungal activity. Further fractionation of methanol extract guided by antifungal activity resulted in the isolation of an active principle and it is identified as phenolic compound. The structure of the active principle was elucidated by mass spectroscopy, 1H NMR and 13C NMR spectroscopy. These results revealed that the compound is 6-(ethoxymethyl)-tetrahydro-2H-pyran-2, 3, 4, 5-tetraol compound with 1- isopropyl-4-methoxybenzene, the compound was found responsible for antifungal activity against both F. oxysporum and C. albicans.[...] Read More.
Keywords: Parrotia persica, phenolic compound, antifungal activity.
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