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rat anti �C human interleukin 1�˰׽���-1��il-1��ø��ԇ���У�elisa kit�� collect sample �C secretion package size: 96 determinations catalogue no.: qrct �C 322101eia \ utl storage: 2 - 8 ��c i. introduction producing of il-1 cell the il-1 is main to be produced by cell;in addition and almost allly there is cell, such as the t that b cell, nk the cell, outside educate cell, horniness cell, tree cell, star polygon cell, fiber cell, neutral grain cell, inside skin the cell and smooth muscle cell can all produce the il-1. although its amino acids is in proper order to only reach 26% of , however the il-1 cell of similar to il-1 the �� is with the affinity that same to join together in �� surface suffer, and develop the same biology function.the il-1 suffers the il-1 the r to almost exsits in all have the cell the il-1 r of the surface, each cell the number and does not wait, little then several ten( such as the t cell), much and then several thousand.special function that il-1 although not extensive used for the body research, its make it have the foreground of the person in the clinical application aspect to immune system.moreover, because of the il-1 too the various and pathologic process of the and machine, therefore study the il-1 repress the thing may also have the actual meaning.now already the gram outs the il-1 suffer the anti- the il-1 for activity for, that material can outside inside closing the il-1, is first kind than ideal to close the factor. ii. reagents materials provided with the kits : 􀂄 coated microtitration strips 96 wells. 􀂄 standard 0, 25, 50, 100, 250, 500 pg/ml, 1 ml/vial, lyophilized. 1 set. 􀂄 enzyme conjugate solution, 6 ml. 􀂄 chromogen solution a, 6 ml. 􀂄 chromogen solution b, 6 ml. 􀂄 stopping solution (1n hcl), 6 ml. 􀂄 wash concentrate,50 ml( x 20). materials required but not provided : 􀁺 precision pipettes: 0.10, 0.20, and 1.0 ml. 􀁺 disposable pipette tips. 􀁺 distilled water. 􀁺 vortex mixer or equivalent. 􀁺 absorbent paper or paper towels. 􀁺 microtiter plate shaker 􀁺 graph paper. 􀁺 a microtiter plate reader with a bandwidth of 10nm or less and an optical density range of 0-2 od or greater at 450 nm . - page 1- for informational use only ▪ do not use for performing assay ▪ refer to most current package in-sert accompanying testkit rat anti �C human interleukin 1 collect sample �C secretion package size: 96 determinations catalogue no.: qrct �C 322101eia \ utl storage: 2 - 8 ��c iii. storage of test kit and instrumentation unopened test kits should be stored at 2-8��c upon receipt and the microtiter plate should be kept in a sealed bag with desiccants to minimize exposure to damp air. opened test kits will remain stable until the expiration date shown, provided it is stored as described above. a microtiter plate reader with a bandwidth of 10nm or less and an optical density range of 0-2 od or greater at 450nm wavelength is acceptable for use in absorbance measurement. iv. assay procedure 1. secure the desired number of coated wells in the holder. 2. dispense 100 ��l of standards and specimens into appropriate wells. 3. dispense 50 ��l of enzyme conjugate reagent into each well. gently mix for 15 seconds. 4. incubate at 18-25 ��c for 90 minutes. 5. remove the incubation mixture by emptying plate contents into a suitable waste container. 6. rinse and empty the microtiter wells 5 times with distilled or deionized water. (mix 50ml of washing buffer 20x with 950ml of distilled water.) 7. strike the wells sharply onto absorbent paper to remove residual water dr-oplets. 8. dispense 50 ��l of color a and color b reagent into each well. gently mix for 5 seconds. 9. incubate at 18-25 ��c for 15 minutes. 10. stop the reaction by adding 50 ��l of stop solution to each well. 11. gently mix for 30 seconds. it is important to make sure that all the blue color changes to yellow color completely. 12. using a microtiter plate reader, read the optical density at 450 nm within 30 minute. v. important notes the wash procedure is critical. insufficient washing will result in poor precision and falsely elevated absorbance readings. it is recommended that if manual pipetting is used, no more than 32 wells be used for each assay run, since pipetting of all standards, specimens and controls should be completed within 3 minutes. a full plate of 96 wells may be used if automated pipetting is available. duplication of all standards and specimens, although not required, is recommended. vi. example of standard curve calculate the average absorbance values (a450) for each set of reference standards, control, and samples. construct a standard curve by plotting the mean absorbance obtained for each reference standard against its concentration on linear graph paper, with absorbance on the vertical (y) axis - page 2- for informational use only ▪ do not use for performing assay ▪ refer to most current package in-sert accompanying testkit rat anti �C human interleukin 1 collect sample �C secretion package size: 96 determinations catalogue no.: qrct �C 322101eia \ utl storage: 2 - 8 ��c and concentration on the horizontal (x) axis.using the mean absorbance value for each sample, determine the corresponding concentration of in from the standard curve. results of a typical standard run with optical density readings at 450nm shown in the y axis against concentrations shown in the x axis. this standard curve is for the purpose of illustration only, and should not be used to calculate unknowns. each user should obtain his or her own data and standard curve. vii. calculation of results the minimum detectable concentration of il1 in this assay is estimated to be 1.0pg/ml. viii. limitations of the procedure reliable and reproducible results will be obtained when the assay procedure is carried out with a complete understanding of the package in-sert instructions and with adherence to good laboratory practice. the wash procedure is critical. insufficient washing will result in poor precision and falsely elevated absorbance readings. the results obtained from the use of this kit should be used only as an adjunct to other diagnostic procedures and information available to the physician. - page 3-

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