Formato de Reporte de atención prehospitalaria - Equipo Multidisciplinario de Atención Prehospitalaria.Full description
Full description
mbu ifaDeskripsi lengkap
Assay ManagementDescripción completa
Post LabFull description
Descripción: ASSAY
Full description
Descripción completa
Assay of Sodium BicarbonateFull description
Enzyme-Linked Immunosorbent Assay (ELISA) adalah suatu teknik biokimia yang terutama digunakan dalam bidang imunologi untuk mendeteksi kehadiran antibodi atau antigen dalam suatu sampel.Full description
Mayank Tandon, Thirumeignanam, D. and Dr. S.N. Rai. Ferric Reducing Antioxidant Power (FRAP) Assay. Dairy Cattle Nutrition Division, N.D.R.I., Karnal, India.
ESTIMATION OF TOTAL ANTIOXIDANT ACTIVITY Total antioxidant activity is measured by ferric reducing antioxidant power (FRAP) assay of Benzie and Strain (1999). FRAP assay uses antioxidants as reductants in a redox-linked colorimetric method, employing an easily reduced oxidant system present in stoichiometric excess. Principle At low pH, reduction of ferric tripyridyl triazine (Fe III TPTZ) complex to ferrous form (which has an intense blue colour) can be monitored by measuring the change in absorption at 593nm. The reaction is non specific, in that any half reaction that has lower redox potential, under reaction conditions, than that of ferric ferrous half reaction, will drive the ferrous (Fe III to Fe II) ion formation. The change in absorbance is therefore, directly related to the combined or “total” reducing power of the electron donating antioxidants present in the reaction mixture. Reagents FRAP Reagent a) Acetate buffer 300 mM pH 3.6: Weigh 3.1g sodium acetate trihydrate and add 16 ml of glacial acetic acid and make the volume to 1 L with distilled water. b) TPTZ (2, 4, 6-tripyridyl-s- triazine) (M.W. 312.34) 10 mM in 40mM HCl (M.W. 36.46) c) FeCl3. 6H2O (M.W. 270.30) 20 mM The working FRAP reagent was prepared by mixing a b & c in the ratio of 10:1:1 at the time of use. Standard: Ascorbic Acid (M.W. 176.13) 1000 µ M Procedure Sample (100 µl) (Plasma/ Milk/ Urine/ Feed Extract etc.) is mixed with 3 ml of working FRAP reagent and absorbance (593 nm) is measured at 0 minute after vortexing. Thereafter, samples are placed at 370C in water bath and absorption is again measured
FRAP Assay
1
after 4 minutes. Ascorbic acid standards (100µM-1000µM) were processed in the same way. Solutions Blank Sample (Plasma/ -- --
Standard -- --
Test 100 μl
Milk/ Urine/ Feed Extract etc.) Standard (Ascorbic acid) Working FRAP
-- --
100 μl
-- --
3000 μl
3000 μl
3000 μl
Solution -
Mix well
-
Blank the analyzer/ spectrophotometer with Blank
-
Measure the OD of Standard and Test at zero minute and again after four minutes at 593 nm.
Calculation: Results were calculated as follows. FRAP value of Sample (µM) = (Change in absorbance of sample from 0 to 4 minute /
Change in absorbance of standard
from 0 to 4 minute) X FRAP value of standard (1000 µM) Note: FRAP value of Ascobic acid is 2.
Reference: Benzie, F.F. and Strain, J.J. 1999. Ferric Reducing/ Antioxidant Power Assay: Direct Measure of Total antioxidant Activity of Biological Fluids and Modified Version for Simultaneous Measurement of Total Antioxidant Power and Ascorbic Acid Concentration. Methods in enzymology. vol. 299:15-23.