ABSTRACT
O presente estudo investigou os efeitos do chumbo na morfologia branquial, nos hematócritos e nas concentrações plasmáticas de sódio, glicose, lipídeos, proteínas e colesterol de Prochilodus lineatus exposto a duas concentrações subletais de chumbo durante 96 h. Inicialmente, testes agudos (96 h) e estáticos determinaram a CL50 (96 h) de chumbo para P. lineatus em 95 mg Pb.L-1. As concentrações de chumbo utilizadas nos testes subletais foram 24 e 71 mg Pb.L-1, que correspondem a 25% e 75%, respectivamente, da CL50 (96 h). As brânquias de P. lineatus expostos a ambas as concentrações de chumbo apresentaram maior incidência de lesões histopatológicas, como elevação epitelial, hiperplasia e aneurisma lamelar. P. lineatus não apresentou alterações significativas no hematócrito durante a exposição a ambas as concentrações de chumbo. Peixes expostos a 71 mg Pb.L-1 apresentaram decréscimo significativo do Na+ plasmático após 48 h, o que pode estar se refletindo na redução das taxas de influxo desse íon. P. lineatus expostos a ambas as concentrações de chumbo apresentaram resposta clássica ao estresse, como verificado pela hiperglicemia associada ao decréscimo dos lipídeos e proteínas plasmáticas. A magnitude da resposta ao estresse foi dose-dependente. A resposta apresentada na concentração mais baixa representa um processo adaptativo, enquanto na maior concentração caracteriza a exaustão.
Subject(s)
Animals , Adaptation, Physiological , Fishes , Gills , Lead , Dose-Response Relationship, Drug , Fishes , Gills , Lethal Dose 50 , Time Factors , Toxicity Tests, AcuteABSTRACT
Minerals more readily adsorb amino acids with charged R groups than uncharged R groups, so that the incorporation of amino acids with charged R groups into peptides would be more frequent than for amino acids with uncharged R groups. However, 74% of the amino acids in the proteins of modern organisms contain uncharged R groups. Thus, what could have been the mechanisms that produced peptides/proteins with more amino acids with uncharged R groups than precursors with charged R groups? Should we expect the composition of amino acids adsorbed on minerals to be similar to those of present proteins? Was the adsorption of amino acids on minerals important for the origin of life? The lipid world offers an alternative view of origin of life. Liposomes contributed to elongation of peptides as well as select hydrophobic amino acids and peptides. These experiments could be showing the mechanism, which hydrophobic amino acids have been selected. However, liposomes have no influence on the stereoselectivity in the oligomerization of amino acids. In the present paper, several other mechanisms are also discussed that could produce peptides with a greater proportion of amino acids with uncharged R groups.
Subject(s)
Amino Acids/chemistry , Minerals/chemistry , Origin of Life , Adsorption , Earth, Planet , Life , Liposomes/metabolism , Peptide Biosynthesis , Peptides/chemistryABSTRACT
The present study investigated lead effects on gill morphology, hematocrit, blood sodium, glucose, lipids, protein, and cholesterol of Prochilodus lineatus exposed to two sublethal lead concentrations for 96 h. Preliminary series of short-term static toxicity tests were run to determine LC50 (96 h) of lead in P. lineatus, which was 95 mg Pb.L-1. Therefore, lead concentrations tested in the sublethal experiments were 24 and 71 mg Pb.L-1, which correspond to 25% and 75% of the LC50 (96 h), respectively. Gills of P. lineatus exposed to both lead concentrations during 96 h presented a higher occurrence of histopathological lesions such as epithelial lifting, hyperplasia, and lamellar aneurism. P. lineatus did not show significant alterations in hematocrit during exposure to both lead concentrations. Fish exposed to the highest lead concentration showed a significant decrease in Na+ plasma concentration after 48 h, possibly reflecting a sodium influx rate decrease. P. lineatus exposed to both lead concentrations presented a "classical general adaptation syndrome to stress", as hyperglycemia associated with lowered lipids and proteins was reported. Stress-response magnitude was dose-dependent. While the response to the lowest lead concentration might represent adaptation, the highest concentration seems to characterize exhaustion.
Subject(s)
Adaptation, Physiological , Fishes/physiology , Gills/drug effects , Lead/toxicity , Animals , Dose-Response Relationship, Drug , Fishes/blood , Gills/pathology , Lethal Dose 50 , Time Factors , Toxicity Tests, Acute/methodsABSTRACT
A previous study was undertaken to test the reaction of several quinones (p-benzoquinone; 2,5-dichloro and 2,6-dichloro p-benzoquinone; tetrachloro-p-benzoquinone; tetrachloro-o-benzoquinone; 2,5-dichloro-3,6-dihydroxy-p-benzoquinone; benz[a]anthracene-7,12-dione) with bovine serum albumin (BSA). From this study, we have devised a spectrophotometric method for determination of total proteins. The quinone, tetrachloro-p-benzoquinone (p-chloranil), showed the best result. The product of reaction between proteins and p-chloranil absorbed at 360 nm and Beer's law was followed up to 200 mug ml(-1) of BSA. The product of reaction of BSA/p-chloranil was stable for 30 min, after that the absorbance increased 16% and kept stable for 24 h. The p-chloranil method showed a limit of detection (1.25 mug ml(-1)) lower than the biuret method (52.0 mug ml(-1)) or p-benzoquinone (PBQ) method (2.6-4.0 mug ml(-1)). The method was applied to spectrophotometric determination of total proteins in blood plasma; the results were compared with the biuret method that is widely used in clinical analysis.
ABSTRACT
A simple, sensitive, and selective method has been developed for determination of cysteine (Cys) or carbocysteine (carboCys) in pharmaceutical products, shampoos and a mixture of amino acids. The results showed the reaction between p-benzoquinone (PBQ) and Cys occurs through the sulfhydryl group. Previous derivatization or extraction is not necessary before the assay is carried out. The method is based on the fact that the product of reaction between PBQ and Cys absorbs at 352 and 500 nm or PBQ and carboCys absorbs at 500 nm. Beer's law is followed in the range 0-40 mug/ml for Cys and 0-150 mug/ml for carboCys. The product of reaction PBQ-Cys is stable for 2 h with absorption bands at 352 and 500 nm. In the presence of amino acids, PBQ is highly selective to Cys. Several substances such as amino acids, urea, salts, and dipeptide did not interfere with the proposed method. A recovery of about 100% is observed for both Cys and carboCys, when the method is applied to determine Cys in a mixture of amino acids resembling blood plasma, shampoo, and pill food as well as carboCys in pharmaceutical products.
ABSTRACT
A microtome for frozen sections was developed using the facilities and equipment avaiable in our country. The requirements for making it were: 1) fast frozen of the tissue; 2) easy hystological procedure; 3) no necessity of long period for preparation of the tissue for histological procedure, and 4) low cost for making. This study shows results obtained by using the microtome for frozen sections of brain of rats
Subject(s)
Animals , Mice , Microtomy , Paraffin EmbeddingABSTRACT
The effects of chemical stimulation of the dorsomedial hypothalamic nucleus (DMH) on blood plasma concentration of glucose, triglycerides, insulin, and free fatty acids (FFA) were investigated in anesthetized adult Wistar rats. Microinjection of 12.5 nmol of norepinephrine into the DMH increased blood plasma concentration of glucose and FFA, decreased triglycerides, and did not change plasma insulin within 5 min; after 20 min, blood glucose and FFA reached control values. Microinjection of epinephrine (12.5 nmol) into the DMH also increased blood plasma glucose concentration and decreased triglycerides after 5 min. These effects are probably mediated by beta-adrenergic mechanisms, because they were prevented by beta-adrenergic antagonist propranolol, but not by alpha-adrenergic antagonist prazosin. Microinjection into the DMH of glutamate, dopamine, or acetylcholine failed to cause any change in those metabolic parameters, corroborating the hypothesis that the DMH is part of a beta-adrenergic pathway involved in short-term modulation of the availability of glucose and FFA.
Subject(s)
Blood Glucose/metabolism , Dorsomedial Hypothalamic Nucleus/physiology , Fatty Acids, Nonesterified/metabolism , Triglycerides/metabolism , Animals , Male , Rats , Rats, Wistar , Stimulation, ChemicalABSTRACT
1. In the present study we have documented the use of the reagent, p-benzoquinone (PBQ) for the spectrophotometric determination of total proteins in blood plasma. 2. Since the products of reaction are stable for several hours at room temperature after the 20-min boiling step, the time at which absorbance is measured is not a critical factor. 3. Common anticoagulants such as EDTA, citrate, or heparin do not interfere with the PBQ method at concentrations used in clinical laboratories. 4. The products of the reaction between PBQ and either plasma (specific absorbance 2.33 x 10(-3) +/- 0.20 x 10(-3) micrograms cm-2) or purified proteins (specific absorbance 2.61 x 10(-3) +/- 0.31 x 10(-3) micrograms cm-2) show an absorption band at 350 nm, which follows Beer's law, and therefore can be used for analytical purposes. 5. The PBQ method has a lower limit of detection (4 micrograms/ml) than that of the biuret method (45 micrograms/ml) for a final reaction mixture of 5.0 and 4.2 ml, respectively.
Subject(s)
Benzoquinones , Blood Proteins/analysis , Spectrophotometry, Ultraviolet/methods , Animals , Anticoagulants/pharmacology , Blood Proteins/drug effects , Dose-Response Relationship, Drug , Drug Interactions , Indicators and Reagents , Male , Rats , Rats, WistarABSTRACT
In the present study we have documented the use of the reagent p-benzoquinone (PBQ) for the spectrophotometric determination of total protein in blood plasma. Since the products of reaction are stable for several hours at room temperature after the 20-min boiling step, the time at which absorbance is measured is not a critical factor. Common anticoagulants such as EDTYA, citrate, or heparin do not interfere with the PBQ method at concentrations used in clinical laboratories. The products of the reaction between PBQ and either plasma (specific absorbance 2.33 x 10-3 ñ 0.20 x 10-3 ug cm -2) or purified proteins (specific absorbance 2.61 x 10-3 ñ 0.31 x 10-3 ug cm-2) show an absorption band at 350 nm, which follows Beer's law, and therefore can be used for analytical purposes. The PBQ method has a lower limit of detection (4 ug/ml) than that of biuret method (45 yg/ml) for a final reaction mixture of 5.0 and 4.2 ml, respectively
