How To Get Rid Of Small Dna Fragments



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AxyPrep TM Mag FragmentSelect-I Protocol (Fragment Size Selection for Illumina Genome Analyzer and Life Technologies SoLiD) Introduction The AxyPrep Mag FragmentSelect-I purification kit utilizes a unique paramagnetic bead technology for quick high-throughput DNA size selection for the Illumina and Life Technologies next generation sequencing platforms. DNA of diverse fragment sizes differentially binds to beads, in response to the AxyPrep FragmentSelect-I concentration. The higher the concentration of AxyPrep Mag FragmentSelect-I, the smaller size DNA fragments bound to beads. AxyPrep Mag FragmentSelect-I consists of two major stages. The first stage is to determine the optimal AxyPrep Mag FragmentSelect-I ratio to DNA sample ratio for target DNA size selection. The second stage utilizes the determined AxyPrep Mag FragmentSelect-I ratio for isolation of target DNA fragment size. There are two different ways to isolate target DNA using the FragmentSelect-I kits. If the goal is to remove smaller DNA fragments a one step process is available. However, if the goal is to remove both the larger or smaller DNA fragments a two step process is recommended. The protocol consists of: Binding larger DNA to the paramagnetic beads, Binding the target DNA off beads, Targeting DNA recovery, o Performing ethanol washes to remove impurities o A final elution step to recover only the targeted DNA fragment. DNA fragment sizes larger or smaller than the target size is mostly removed during the binding and washing-off steps. The purified DNA product is essentially free of contaminants. The binding of DNA to magnetic beads is based on the amount of AxyPrep FragmentSelect-I added into DNA solution. The more AxyPrep Mag FragmentSelect-I is added; the smaller size DNA can be isolated. Depending on the amount of the AxyPrep Mag FragmentSelect-I added, DNA fragment ranging from 300 bp 1000 bp can be isolated from a population of page 1

DNA fragments. AxyPrep Mag FragmentSelect-I can be used in the following applications: PCR Sequencing (Sanger and Next Generation) Cloning Process Overview A- One-step process to remove smaller DNA fragments: 1. Add AxyPrep Mag FragmentSelect-I to the DNA solution for larger fragments to bind to the magnetic beads (decreasing the amount of AxyPrep Mag FragmentSelect-I produces less precipitation power that allows the binding of larger size DNA). DNA fragments less than the target size remains in solution. 2. Use a magnetic plate, the Axygen IMAG, to separate the smaller DNA (in solution) from the target fragments (bound to the beads). 4. Remove and discard the supernatant. 5. While the magnetic beads are retained on the magnet wash the beads twice with 80% ethanol to remove salt and contaminants. 6. Elute target size DNA from magnetic beads and transfer to a new plate. B- Two-step process to isolate larger or smaller DNA fragments: 1. Add AxyPrep Mag FragmentSelect-I into DNA solution to allow binding of large size DNA onto magnetic beads (this step removes DNA larger than target DNA). 2. Separate beads from clear supernatant. 3. Add additional beads to the supernatant in step 3 to facilitate binding of the target DNA onto the magnetic beads. 4. Wash beads twice with 80% ethanol to remove salt and contaminants. 5. Elute target DNA. Specifications The AxyPrep Mag FragmentSelect-I kit can be performed in a tube and 96-well formats. The following table illustrates the number of reactions an AxyPrep FragmentSelect-I kit can purify depending on the volume of DNA solution page 2

AxyPrep FragmentSelect-I Kits AxyPrep Mag FragmentSelect-I Products AxyPrep Mag FragmentSelect-I - 5 ml AxyPrep Mag FragmentSelect-I - 50 ml AxyPrep Mag FragmentSelect-I - 250 ml P/N Mag-FRAG-I-5 Mag-FRAG-I-50 Mag-FRAG-I-250 DNA Reaction Volume (96 well, L) Mag-FRAG-I-5 (# reactions) Mag-FRAG-I-50 (# reactions) 100 18 175 875 50 35 350 1750 Materials supplied in the Kit: - AxyPrep Mag FragmentSelect-I paramagnetic bead Solution - Store at 4 C upon arrival (do NOT freeze) for up to 12 months Mag-FRAG-I-250 (# reactions) - Mix the reagent well at room temperature to completely resuspend beads prior to use. The solution should appear homogenous. Materials supplied by the User: Consumables & Hardware: Recommended Name Model 96-well PCR reaction plate 384-well PCR reaction plate 96-well round/ flat bottom microtiter plate. Plate selection depends on the PCR reaction volume 96-well cycling plate Recommended Vendor and P/N Corning, Inc., www.corning.com # 3797, 96 well round bottom # 3591, 96 well flat bottom # 3957, 0.5 ml v bottom 96 # 3365, 360 l round 96 # 3364, 360 l flat 96 # 3371, 96 clear pro Axygen, PCR-96-FS-C, PCR-96M2-HS-C, www.axygen.com 384 well cycling plate Axygen, PCR-384M2-C, www.axygen.com PCR Plate Seals Easy Peel Heat Sealing Foil Axygen, MF-111, www.axygen.com Liquid handling robotics Compatible with open platform robotics Multichannel hand pipette AxyPet Single, 8 and 12 Multichannel Contact Axygen Biosciences Technical support for compatible AxyPrep Mag methods and accessories for automation Handheld Magnetic Separation Devices Selection Guide: The handheld magnetic devices have been optimized for different AxyPrep Mag protocols. These magnets address different volumes for tubes and plate types. page 3

Protocol Manufacturer Part number Plate description 0.5 ml Self Standing Screw cap Axygen SCT-050-SS-C tube AxyPrep Mag Kits 1.5 ml Self Standing Screw cap Axygen SCT-150-SS-C tube 2.0 ml Self Standing Screw cap Axygen SCT-200-SS-C tube Plate Material Part Number IMAG-12T Protocol Manufacturer Part number Plate description AxyPrep Mag PCR Clean -up AxyPrep FragmentSelect-I AxyPrep FragmentSelect-R AxyPrep Mag DyeClean AxyPrep Mag DNA Normalizer AxyPrep Mag Blood gdna AxyMag FFPE (DNA-RNA- mirna) AxyPrep Mag Plasmid Kit AxyPrep Mag Tissue gdna Plate Material Corning 3364 96 flat 360 l Corning 3591 96 flat bottom Polystyrene Corning 3365 96 round 360 l Corning 3371 96 clear pro round Corning 3797 96 round bottom Polystyrene Corning 3957 96 v bottom 0.5 ml Axygen PCR-96-FS-C 96 PCR full skirt Axygen PCR-96M2-HS-C 96 PCR half skirt Corning 3959 96 round bottom 1 ml Corning 3961 96 round bottom 2 ml Part Number IMAG-96P Reagents: Reagents Application 100% ethanol Binding reagent 70% ethanol Washing solvent 10 mm Tris-HCl, ph=8.0 reagent grade water DNA elution 10 mm Tris-HCl ph 8.0, 1 mm EDTA page 4

TWO-STEP PROCEDURE WITH DNA AXYPREP FRAGMENTSELECT- I TARGET FRAGMENT SIZE: 500bp Procedure For 96-well Plate: 1. Add 65 l of room temperature AxyPrep FragmentSelect-I to 50 l of the DNA solution (DNA target size is 500 bp). Then Pipette-mix five times to obtain a homogenous solution and incubate at room temperature for 5 minutes. During this time the fragment sizes greater than 500bp will bind to the beads, while smaller DNA fragments will remain in solution. NOTE: To obtain a fragment size of 500 bp the ratio of AxyPrep FragmentSelect-I to DNA solution is 1.3X. If a DNA volume other than 50 l is used, adjust the AxyPrep FragmentSelect-I volume accordingly to maintain the ratio. NOTE: Prior to adding the AxyPrep FragmentSelect-I to the DNA solution briefly vortex the paramagnetic beads. 2. After the five minute incubation in step 1, place the plate on an Axygen IMAG to separate the paramagnetic beads from the solution containing the target DNA. Incubate at room temperature for 1 minute or until solution clears. 3. Transfer the supernatant to a fresh plate. 4. Add 10ul of FragmentSelct-I to the supernatant from step 3 and gently pipette-mix five times. Incubate at room temperature for 5 minutes 5. Place the 96-well plate on the Axygen IMAG for 2 minutes to allow for separation or until the solution is clear. NOTE: Target DNA is bound to beads. 6. Remove the cleared supernatant and discard. 7. While the plate is on the magnet, wash the beads with 200 l of 80% ethanol by carefully pipetting up/down five times. Discard the ethanol after the wash. NOTE: While washing the paramagnetic beads pipette the ethanol on the opposite side of the beads so as NOT to disturb the beads. 8. Repeat Step 6 and 7. 9. Remove 80% ethanol after the final wash and let the beads dry for 5 minutes at room temperature. NOTE: A longer drying time may be necessary to remove any residual ethanol that may page 5

interfere with downstream applications. However, be careful not to over dry the beads (e.g. placing the beads at 37 C) because this will inhibit DNA recovery. 10. Remove the plate from the magnet and resuspend beads in 20 l of molecular biograde water to elute the target DNA. 11. Place the plate on the magnet to separate the beads from solution and incubate for 1 minute or until solution becomes clear. 12. Transfer the clear DNA solution to a fresh plate. 13. Examine the DNA size distribution and concentration with Bioanalyzer. NOTE: To recover DNA fragments smaller than 500bp such as 300bp, use 1.6X for the initial bind. ONE-STEP SIZE SELECTION PROCEDURE WITH DNA AXYPREP FRAGMENTSELECT- I 1. Add 70 l of room temperature AxyPrep FragmentSelect-I to 50 l of the DNA solution (DNA target size is > 500 bp). Then Pipette-mix five times to obtain a homogenous solution and incubate at room temperature for 5 minutes. During this time the fragment sizes larger than 500 bp will bind to the beads, while DNA fragments 500 bp and smaller will remain in solution. NOTE: To obtain a fragment size of 500 bp the ratio of AxyPrep FragmentSelect-I to DNA solution is 1.4X. If a DNA volume other than 50 l is used, adjust the AxyPrep FragmentSelect-I volume accordingly to maintain the ratio. NOTE: Prior to adding the AxyPrep FragmentSelect-I to the DNA solution briefly vortex the paramagnetic beads. 2. After the incubation in step 1, place the plate on the Axygen IMAG for 2 minutes or until solution clears to separate the paramagnetic beads from the solution. 3. Remove the cleared supernatant and discard. 4. While the plate is on the magnet wash the beads with 200 l of 80% ethanol by pipetting ethanol five times. NOTE: While washing the paramagnetic beads pipette the ethanol on the opposite side of the beads so as NOT to disturb the beads. 5. Repeat Steps 3 4 once. 6. Completely remove 80% ethanol after the final wash and let the beads dry for 5 page 6

minutes at room temperature. NOTE: A longer drying time may be necessary to remove any residual ethanol that may interfere with downstream applications. However, be careful not to over dry the beads (e.g. placing the beads at 37 C) because this will inhibit DNA recovery. 7. Remove the plate from the magnet and resuspend beads in 20 l of molecular biograde water to elute the target DNA. 8. Place the plate on the magnet and incubate for 1 minute or until solution becomes clear to separate the beads from solution. 9. Transfer the clear DNA solution to a fresh plate. 10. Examine the DNA size distribution and concentration with Bioanalyzer. Please contact Axygen Biosciences for sales support at: axgsales@corning.com and for technical support at: axgsupport@corning.com * The PCR process is covered by patents owned by Roche Molecular Systems, Inc., and F. Hoffman-La Roche, Ltd. All trademarks are property of their respective owners. page 7

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