Instructions for Use. Tg Antibody ELISA

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Instructions for Use Tg Antibody ELISA Enzyme Immunoassay for the Quantitative Determination of Autoantibodies to Thyroglobulin (Tg) in Serum and Plasma I V D REF EA618/96 12 x 8 2 8 C DLD Gesellschaft für Diagnostika und medizinische Geräte mbh Adlerhorst 15 22459 Hamburg Germany Tel +49-40-555 87 10 Fax +49-40-555 87 111 Internet: http://www.dld-diagnostika.de E-Mail: contact@dld-diagnostika.de 104/e/1 2016-02-29

Contents 1. Introduction and Principle of the Test Page 3 2. Precautions Page 3 3. Storage and Stability Page 4 4. Contents of the Test Page 4 5. Preparation of Reagents and Samples Page 5 6. Assay Procedure Page 6 7. Calculation of Results Page 7 8. Typical Example Page 7 9. Assay Characteristics Page 9 10. References Page 11 Pipetting Scheme Page 12 Page 2

1. Introduction and Principle of the Test In some diseases of the thyroid, serum autoantibodies against some thyroid antigens are found. The most important antigens are: Thyroglobulin (Tg) Thyroid peroxidase (TPO), formerly known as microsomal antigen TSH-Receptor Measurement of these autoantibodies is of considerable value in the diagnosis of autoimmune thyroid diseases (Hashimoto-thyroiditis, primary myxedema, hyperthyroidism, asymptomatic autoimmune thyroiditis) and the anti-tg-elisa kit provides a convenient method of quantitating Tg autoantibodies in patients' serum or plasma samples. The assay is based on an easy to use and flexible strip well system employing wells coated with highly purified thyroglobulin. Autoantibody binding to the Tg coated wells is detected using Protein A conjugated to alkaline phosphatase as marker and p-nitrophenyl phosphate as substrate. Quantification of unknowns is achieved by comparing the enzymatic activity of unknowns with a response curve prepared by using known standards (NIBSC65/093). The same diluted sample can be used for both anti-tg-elisa and anti- TPO-ELISA. 2. Precautions For in vitro diagnostic use only. Do not eat, drink or smoke where immunodiagnostic materials are being handled. Do not pipet by mouth. Some reagents contain sodium acid as preservative. Avoid skin contact. Wear disposable gloves when handling immunodiagnostic material. Some kit components are made with human sera. All sera used were tested for HIV I/II antibodies and HBsAg and found to be negative. However, because no test method can offer complete assurance that infectious agents are absent, these reagents should be handled as potential biohazardous material. Page 3

3. Storage and Stability Store all reagents at 2-8 C and use before expiry date. Wash Buffer may be stored at 2-8 C after dilution and used within the shelf life of the kit. Unused Tg coated strip wells must always be stored at 2-8 C with desiccant in the self-seal bag provided. 4. Contents of the Test 4.1 MT Strips STRIPS 12 strips 8 wells each, breakable, coated with thyroglobulin. 4.2 Enzyme Conjugate CONJ 1 vial 11 ml, ready for use Contains Protein A conjugated to alkaline phosphatase. 4.3 Standards A - E CAL A CAL E 5 vials 1.0 ml each, ready for use Concentrations (Units are NIBSC 65/093): Standard A B C D E U/ml 0 35 150 1,000 5,000 4.4 Controls 1 and 2 CON 1 & 2 2 vials 0.5 ml, concentrates. Dilute 1:20 with Assay Diluent. For Tg antibody concentration see QC-Certificate. For longer storage (more than 4 weeks) freeze Controls at - 20 C. 4.5 Wash Buffer WASH 1 bottle 125 ml, concentrate. Dilute 10 times with distilled water. 4.6 Assay Diluent DIL 1 bottle 125 ml, ready for use Page 4

4.7 Substrate SUB 1 vial 11 ml pnpp solution, ready for use. 4.8 Stop Solution STOP 1 vial 10.5 ml, ready for use. Contains 0.2 M NaOH; 0.25 M EDTA. Reagents and materials required but not provided: Multi Channel Pipette Variable Pipets ( 0-100 µl and 0-200 µl) Microtiter Plate - Reader Distilled water 5. Preparation of Reagents and Samples Allow reagents and required number of MT Strips to reach room temperature. The volumes listed below are for 96 determinations. Specimens and Controls Dilute patient sera and Controls 1 and 2 with Assay Diluent 1:20, e.g. 50 µl + 950 µl. (Do not dilute the ready for use Standards.) Wash Buffer Dilute the concentrate 10 times with distilled water (e.g. 100 ml concentrate + 900 ml distilled water). Page 5

6. Assay Procedure 6.1 Pipette 50 µl of Standards, diluted Controls and diluted samples into suitable wells of the coated MT Strips. Duplicate determinations are recommended. 6.2 Cover the plate and incubate at room temperature on an ELISA plate shaker (500 shakes per min.) for 15 minutes. 6.3 After the first incubation, invert the plate and briskly shake out the well contents. Fill each well with diluted Wash Buffer dispensed from a laboratory wash bottle, dispenser or pipette. Repeat this procedure 3 times. Remove excess solution by tapping the inverted plate on a paper towel. 6.4 Pipette 100 µl of the Enzyme Conjugate into the wells. 6.5 Cover the plate and incubate at room temperature on an ELISA plate shaker (500 shakes per min.) for 15 minutes. 6.6 Repeat the washing procedure as described in 6.3. 6.7 Pipette 100 µl of Substrate into each well, and incubate for 15 minutes at room temperature in the dark without shaking. 6.8 After this time a yellow-green colour will have developed, and the reaction is stopped by addition of 100 µl of Stop Solution to each well. 6.9 Read the optical density at 405 nm within 30 minutes using a microplate reader blanked preferably against a well containing 100 µl Substrate and 100 µl Stop Solution. Any test sample reading above the highest standard should be further diluted with Assay Diluent and measured again in the test. Page 6

7. Calculation of Results On a semilogarithmic graph paper the concentration of the Standards (x-axis, logarithmic) are plotted against their corresponding optical density (y-axis, linear). Alternatively, the optical density of each Standard and sample can be related to the optical density of the highest standard, expressed as the ratio OD/ODmax, and then plotted on the y-axis. The concentration of the neat samples can be read directly from this standard curve by using their average optical density. The 1:20 predilution of samples and Controls has already been considered in the given concentrations of the Standards. 8. Typical Example Below is listed a typical example of a standard curve with the anti-tg- ELISA. Concentration (U/ml) Mean OD at 405 nm 0 0.024 35 0.069 150 0.231 1,000 1.212 5,000 2.567 Page 7

Typical Standard Curve OD 405 2.6 2.4 2.2 2 1.8 1.6 1.4 1.2 1 0.8 0.6 0.4 0.2 0 100 1,000 10,000 U/ml Page 8

9. Assay Characteristics Assay Cut Off Negative Positive < 65 U/ml 65 U/ml Clinical Specificity Samples from 200 individual healthy blood donors were analysed in the anti-tg ELISA. 190 (95%) were identified as being negative for Tg autoantibodies. Clinical Sensitivity Samples from 66 patients diagnosed with Hashimoto's or Graves' diease were assayed in the anti-tg ELISA. 48 (73%) were identified as being positive for Tg autoantibodies. Lower Detection Limit The zero standard was assayed 20 times and the mean and standard deviation calculated. The lower detection limit at 2 standard deviations was 9.8 U/ml. Intra-Assay Variation (n=25) Inter-Assay Variation (n=20) sample mean U/ml cv (%) 1 61 7.1 2 139 4.6 3 711 2.8 4 1,315 3.3 sample mean U/ml cv (%) 1 56 15.8 2 205 10.9 3 759 7.2 4 1,864 7.3 Page 9

Clinical Accuracy Analysis of sera from patients with autoimmune diseases other than Graves' or Hashimoto's dieases indicated no interference from autoantibodies for 21-OH (n=4). 29% (n=7) of sera positive for antibodies to GAD, 18% (n=17) of sera positive for antibodies to IA-2, 44% (n=9) of sera positive for acetylcholine receptor, 40% (n=5) of sera positive for antibodies to dsdna and 25% (n=28) of sera positive for Rheumatoid Factor were positive for anti-tg Ab in the ELISA. Interference No interference was observed when samples were spiked with the following materials: haemoglobin up to 500 mg/dl, bilirubin up to 20 mg/dl and intralipid up to 3,000 mg/dl. The data quoted in these instructions should be used for guidance only. It is recommended that each laboratory include its own panel of control samples in the assay. Each laboratory should establish its own normal and pathological reference ranges for anti-tg Ab levels. Page 10

10. References B. Rees Smith (2001); Thyroid Autoantibodies Scand J Clin Lab Invest 2001 61 (suppl 235): pp. 45-52. P. Burne et al. (2005); Point of care assays for autoantibodies to thyroid peroxidase and thyroglobulin Thyroid 2005 15: 1005-1010 Page 11

Pipetting Scheme Standards (A to E) 50 µl Controls 1:20 diluted 50 µl Samples 1:20 diluted 50 l 15 minutes incubation at room temperature on an ELISA plate shaker (500 shakes per min.) 3 x washing with Wash Buffer Conjugate 100 µl 15 minutes incubation at room temperature on an ELISA plate shaker (500 shakes per min.) 3 x washing with Wash Buffer Substrate 100 µl 15 minutes incubation at room temperature in the dark without shaking Stop Solution 100 µl Reading of absorbance at 405 nm Page 12