AMG Coupling Kit for 200 nm Magnetic Particles AI-LNPCKMP-06.00 INSTRUCTIONS FOR USE Coupling Kit 200 nm Magnetic Particles Antibody Concentration: The concentration range for coupling antibody is 25 - 100 µg/mg particles, with a determined maximal binding capacity up to 100 µg/mg particles. Antibody coupling concentration is best optimised as this can vary depending on the protein used. This product is for Laboratory Use Only Provided Materials AMG Coupling Kits utilise Mix&Go™ technology to stably bind biomolecules of interest to functionalised polymer magnetic particles. Mix&Go allows proteins to bind faster and with more functionality. AMG Coupling Kits provide enhanced loading capacity for the capture of the target molecules and downstream applications use. The particles are provided fully activated with Mix&Go and are ready to use, with general buffer solutions known to work for a majority of applications. AMG Coupling Kits are suitable for a range of magnetic, fluorescent and chemiluminescent immunoassays and purification applications using biomolecules including proteins, peptides, antigens and antibodies. Product Description Catalogue #: A-LNPCKMP-10 (10 Reactions) A-LNPCKMP-30 (30 Reactions) Particle: Concentration: 200 nm, Superparamagnetic 10 mg/mL (1% w/v solids) Kit Storage: Shelf life at 2°C to 8°C is 1 year. Do not expose the AMG Coupling Kit to temperatures exceeding 60°C or below 0°C. Component Activated 200 nm Magnetic Particles Coupling Buffer - Formulation C Blocking Buffer - Formulation B Storage Buffer - Formulation A Additional Materials Required Antibody Pipettes Magnetic separator for tubes (capable to separate 200 nm magnetic particles) Tube rotator Vortex mixer Sonication Bath with fresh water (Min Power 60W) • • • • • • Before Starting Allow all reagents to come to room temperature (20°C to 25°C). Refer to the AMG Coupling Kit process flowchart on page 3. Particle Preparation 1. 2. 3. Safety Precautions 4. Standard precautions exercised when handling laboratory reagents should be adhered to. Refer to the Coupling Kit MSDS for safety precautions. Product Compatibility Assay Compatibility: Particles are compatible with the majority of existing uses and protocols. This allows for easy substitution of the AMG Coupling Kit into your application of choice. Kit Reagent Compatibility: Pre-activated particles are stable under the provided conditions, however the presence of certain materials, at the time of coupling, will interfere with and reduce the coupling efficiency. It is recommended to use the provided Coupling Buffer and reduce the presence of these reagents during coupling as much as practically possible. For information on interfering materials visit the Anteo Technologies website (www.anteotech.com). Always determine optimal conditions for your protein of interest. Antibody Coupling Procedure The following procedure is an example of how to couple antibody to the particles and states only general conditions. Protocols for antibodies or proteins of interest should be optimised to meet individual requirements. Additional information may be found on the Anteo Technologies website (www.anteotech.com). Vortex the stock particles on high for 10 seconds. Sonicate the stock particles for 5 minutes. Aliquot 100 µL (1 mg) of the particle suspension to a 1.5 mL tube. Place the tube on the magnetic separator for up to 5 minutes. Helpful Hint: When separating magnetic particles from supernatant, it is recommended to put the tube containing the particles on the magnetic separator until the supernatant is clear (up to 5 minutes), and carefully remove the supernatant so as not to disturb the particle pellet. Low strength magnets will take longer to form a pellet or may leave residue on the tube. 5. 6. 7. Remove and discard the supernatant from the tube. Remove tube from magnet and add 100 µL of Coupling Buffer to the tube. Resuspend the particles by vortexing on high for 10 seconds. Helpful Hint: Particles may partially aggregate and appear to stick on the tube at this stage. This is the normal process whereby the surface is equilibrating to the Coupling Buffer conditions for subsequent coupling of your protein. 8. 9. Repeat above wash steps 4 - 7 once (2 washes total). Place the tube on the magnetic separator for up to 5 minutes. 10. Remove and discard the supernatant from the tube. 11. Resuspend the particles in 100 µL of Coupling Buffer. By vortexing on high for 10 seconds. Copyright ©2015 Anteo Technologies Ltd. All Rights Reserved A-CMPLNMP-X A-CMPCBC1-X A-CMPBBB1-X A-CMPSBA1-X 1.7 mL low binding microcentrifuge tubes Note: Product contains ProClin® 300 as preservative. Product is not guaranteed DNase, RNase or endotoxin free. The user must determine the suitability of the product for specific uses. www.anteotech.com Page 1 of 3 Catalogue Number Effective Date: 06/05/2015 Review Date: 06/05/2017 AMG Coupling Kit for 200 nm Magnetic Particles AI-LNPCKMP-06.00 Storage and Stability Antibody Coupling Helpful Hint: Particles may aggregate during coupling. This may be part of the normal process whereby the surface during coupling is interacting with your protein of interest. There may be a need for optimisation of the coupling conditions. Particles can be dispersed by 5-minute incubations in a bath sonicator. 12. Prepare 100 µL of antibody at the required final concentration in Coupling Buffer in a fresh 1.5 mL tube. 13. Aspirate the prepared particles. 14. Add the particles to the antibody solution. 15. Vortex on high for 10 seconds, and sonicate for 5 minutes. This results in 200 µL total volume, and particles are at 5 mg/mL. 16. Incubate for 60 minutes at room temperature on a tube rotator, keeping the particles in suspension. Blocking Blocking is recommended for all particles, particularly those that are not fully coupled with protein; and/or for particles that are to be used in downstream applications where complex mixtures are used. Blocking should be assessed depending on the end use and if non-specific binding is encountered. 17. Vortex particles for 30 seconds. Helpful Hint: Sonicate the particles for 5 minutes if aggregation is observed. 18. Add 20 µL of the Blocking Buffer to the tube. 19. Incubate for 60 minutes at room temperature on a tube rotator. Particle Storage 20. Vortex particles for 30 seconds. 21. Place the tube on the magnetic separator for up to 5 minutes. 22. Remove and discard the supernatant from the tube. 23. Remove tube from magnet and add 200 µL of Storage Buffer to the tube. 24. Resuspend the particles by vortexing on high for 10 seconds. 25. Repeat above wash steps 20 - 24 once (2 washes total). 26. Place the tube on the magnetic separator for up to 5 minutes. 27. Remove and discard the supernatant from the tube. 28. Remove tube from magnet and add 100 µL of Storage Buffer to the tube. 29. Resuspend the particles by vortexing on high for 10 seconds. 30. Sonicate particles for 5 minutes. 31. Repeat above steps 29 - 30 once (2 sonication steps total). 32. The particles are stably coupled with protein and ready for use at a final concentration of 10 mg/mL. Particles may be used immediately or stored at 2°C to 8ºC. Helpful Hint: The unopened product should be stored at 2°C to 8°C. Remaining materials should be retained in the supplied container and sealed for future use. Product Information Observed reproducibility of particles in this kit, with intra- and inter-assay protein loading with mouse IgG is <15% CV. Activated particles have been quantified using mouse IgG binding capacity titration (refer to Table 1). The monodispersity of particles refers to the level of aggregation. As particles aggregate, the Polydispersity Index (PdI) increases. Activated particles are assessed by Zetasizer to determine the level of dispersion of the particles (refer to Table 1). Table 1. Activated particles Binding Capacity (mouse IgG, µg/mg particle) Monodispersity (Polydispersity Index, PdI) > 50 < 0.3 Technical Support For questions regarding this product or for technical support please refer to our website or contact us via one of the following methods: Anteo Technologies Pty Ltd Unit 4, 26 Brandl Street Eight Mile Plains QLD 4113 Australia Phone: +61 7 3219 0085 Fax: +61 7 3219 0553 Email: support@anteotech.com www.anteotech.com Other Mix&Go™ Scientific Products For further information on other Mix&Go products please refer to our website: www.anteotech.com All Anteo Products are sold as general purpose reagents for general laboratory and research uses only. Anteo Products are not intended for diagnostic and/or therapeutic purposes and no Anteo Product may be administered to humans. Anteo does not make any representation or warranty that Anteo Products comply with all laws and regulations that may be applicable to Customer’s use of any Anteo Product. Anteo warrants that Anteo Products will conform to the specifications set forth on the applicable Anteo Product Certificate of Analysis (“Anteo’s Limited Warranty”). The Certificate of Analysis may be obtained by contacting Anteo. Anteo’s Limited Warranty is wholly conditioned on the proper use of Anteo Products in the applications for which they are intended, and Anteo makes no warranty (express, implied or statutory) for Anteo Products that are modified; subjected to accident, misuse, neglect, unauthorized repair or improper tampering, testing or storage; and/or used or handled contrary to Anteo’s instructions as set forth on the Anteo Product label and/or in this insert. Unless otherwise expressly provided in this document or in these Terms and Conditions of Sale, Anteo disclaims all warranties, conditions and guarantees, whether written, express, implied, statutory or otherwise, including but not limited to, the implied warranties or guarantees of merchantability and fitness for particular purpose. . ® ProClin 300 is a registered trademark of Rohn and Haas Company. If the particles have been stored, they should be resuspended prior to use (step 29 - 30). www.anteotech.com Page 2 of 3 Copyright ©2015 Anteo Technologies Ltd. All Rights Reserved Effective Date: 06/05/2015 Review Date: 06/05/2017 AMG Coupling Kit for 200 nm Magnetic Particles AI-LNPCKMP-06.00 AMG COUPLING KIT PROCESS FLOWCHART Step 1-3: Prepare and dispense activated particles Step 4-11: Wash particles into Coupling Buffer Step 12: Dilute antibody in Coupling Buffer Step 13-14: Add particles to diluted antibody solution Step 16: Incubate 60 minutes at room temperature Step 17-18: Add Blocking Buffer to particle antibody solution Step 19: Incubate 60 minutes at room temperature Step 20-31: Wash particles into Storage Buffer ✓ www.anteotech.com Page 3 of 3 Step 32: Antibody coupled particles are ready for use Copyright ©2015 Anteo Technologies Ltd. All Rights Reserved Effective Date: 06/05/2015 Review Date: 06/05/2017
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