Troponin Test Card Troponin I-1221.
SD BIOLINE Troponin I quick test is a fast immuno-chromatographic measure for the subjective identification of heart troponin I(cTnI) in human serum, plasma or entire blood as a guide in the determination of myocardial dead tissue in trauma center, basic consideration, place of-care, and clinic settings.
• Time to Therapy Reduced
• Length of Stay in ER Reduced
• Patient Satisfaction Increased
• Cost of Care Reduced
• Example : Serum, plasma or entire blood (80 μl)
• Test result : 15 minutes
• Remove level : 0.5 ng/ml
• Timeframe of realistic usability and capacity temperature: two years at 1-30 °C
• Execution: Sensitivity – 96.9 %, Specificity – 97.3 % (versus Quantitative measure)
Human Troponin I, Cardiac Muscle (TNNI3) ELISA Kit
Human Troponin I, Cardiac Muscle (TNNI3) ELISA Kit is an ELISA Kit for the in vitro quantitative estimation of Human Troponin I, Cardiac Muscle (TNNI3) fixations in serum, plasma and other organic liquids.
Troponin I, heart muscle is a protein that in people is encoded by the TNNI3 quality. It is a tissue-explicit subtype of troponin I, which thusly is a piece of the troponin complex. The TNNI3 quality encoding heart troponin I (cTnI) is situated at 19q13.4 in the human chromosomal genome. Human cTnI is a 24 kDa protein comprising of 210 amino acids with isoelectric point (pI) of 9.87. cTnI is only communicated in grown-up heart muscle.
The solidness of the not set in stone by the pace of action misfortune. The misfortune rate is under 5% inside the termination date under proper capacity conditions. To limit execution changes, activity methods and lab conditions ought to be completely controlled. It is likewise unequivocally recommended that the entire measure is performed by a similar client all through.
Serum, plasma and other natural liquids.
Examine Principle This unit depends on sandwich compound connected immuno-sorbent measure innovation. A neutralizer is pre-covered onto a 96-well plate. Norms, test tests, and biotin-formed reagent are added to the wells and hatched. The HRP-formed reagent is then added, and the entire plate is brooded. Unbound forms are eliminated utilizing wash support at each stage. TMB substrate is utilized to measure the HRP enzymatic response. After TMB substrate is added, just wells that contain adequate TNNI3 will create a blue hued item, which then changes to yellow subsequent to adding the acidic stop arrangement. The power of the yellow tone is corresponding to the TNNI3 sum bound on the plate. The Optical Density (OD) is estimated spectrophotometrically at 450 nm in a microplate peruser, from which the convergence of TNNI3 can be determined.
Pack Components
The pack parts recorded are for reference as it were. The item manual might vary marginally. The item ought to be utilized as expressed on the item manual included and conveyed along with the item.
- Pre-covered 96-Well Microplate
- Standard
- Standard Diluent Buffer
- Wash Buffer
- Recognition Reagent A
- Discovery Reagent B
- Diluent A
- Diluent B
- TMB Substrate
- Stop Solution
- Plate Sealer
Reagent Preparation
This strategy is accommodated reference as it were. The item manual might vary somewhat. The item ought to be utilized as expressed on the item manual included and conveyed along with the item.
1) Standard: Prepare the norm with the suggested volume of Standard Diluent Buffer, to make the standard arrangement. Then, at that point, utilize the Standard Diluent cradle to complete sequential weakenings of the standard arrangement, as trained in the Protocol.
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2) Wash Buffer: Dilute the concentrated Wash Buffer with refined water, as taught in the Protocol.
3) Detection Reagent Preparation: Calculate the complete volume of working arrangement required. Weaken Detection Reagent An and Detection Reagent B with Diluent An and Diluent B, separately, at 1:100.