AccuPrep GMO DNA Extraction Kit Cat. No.: K-3031

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AccuPrep GMO DNA Extraction Kit Cat. No.: K-3031 V109C3

Safety Warnings and Precautions. For research use only. It is not recommended to diagnose disease in humans or animals. DO NOT use to humans or animals. Wear gloves when you are handling irritant or harmful reagents. Warranty and Liability All BIONEER products are tested under extensive Quality Control procedures. BIONEER guarantees the quality under the warranty period. Any problems should be reported immediately. Liability is conditional upon the customer providing full details of the problem to BIONEER. Once the problem occurs, customer must report to BIONEER within 30 days. Quality Management System ISO 9001 Certified Every aspect of our quality management system from product development, production to quality assurance and supplier qualification meets the world-class standards. QC Testing Each lot of BIONEER s product is carefully tested in the quality control team. Trademarks AccuPrep is trademark of Bioneer Corporation. Copyright 2002 by Bioneer Corporation. All rights reserved V109C3

CONTENTS Ⅰ. INTRODUCTION... 3 II. KIT COMPONENTS... 4 III. REQUIRED REAGENTS AND EQUIPMENT... 5 IV. BEFORE YOU BEGIN... 5 V. EXPERIMENTAL PROTOCOL... 6 VI. PROBLEM SOLVING... 8 VII. SUPPLEMENT... 11 VIII. REFERENCES... 12 IX. PRODUCT INFORMATION... 12

AccuPrep GMO DNA Extraction Kit Technical Manual Ⅰ. Introduction The AccuPrep GMO DNA Extraction Kit is designed for quick and convenient extraction of up to 5 g of DNA from 100 mg of beans or corn. In the presence of chaotropic salt, DNA binds to glass fibers fixed in a column. Proteins and other contaminants are removed during washing steps, and the DNA is isolated and eluted in the final elution step. The process does not require the use of organic solvents or ethanol precipitation step; therefore, it is ideal for safe and convenient extraction DNA from a variety of botanical sources such as beans and corns. Advantages: 1. DNA can be prepared more promptly and conveniently. 2. Other cellular components besides nucleic acids, such as protein, nucleases, and other contaminants or inhibitors are completely eliminated, improving the efficiency and reproducibility of PCR. 3. As no precipitation or organic solvent is used, damage to DNA is minimized. 4. Prepared DNA can be used in a variety of applications. 3

II. Kit Components The product can perform 100 purifications, and will maintain performance capability for at least a year. K-3031 AccuPrep GMO DNA Extraction Kit Reagents Proteinase K, lyophilized 25 mg x 2 One vial of 25 mg lyophilized proteinase K. Dissolve in 1.25 ml of nuclease-free water. Dissolved proteinase K is stable for up to 1 month when stored at 4. Storage at -20 is recommended to prolong the activity, but repeated freezing and thawing should be avoided. Lysis buffer (L) 50 ml Mix L buffer thoroughly by shaking before use. L buffer is stable for 2 year when stored at room temperature. Binding buffer (B) 50 ml Mix B buffer thoroughly by shaking before use. B buffer is stable for 2 year when stored at room temperature. * NOTE: Do not add Proteinase K directly to Binding buffer. Washing Buffer (W1) 40 ml W1 buffer is supplied as a concentrate. Before using for the first time, add 30 ml of absolute ethanol. W1 buffer is stable for 2 year when stored closed at room temperature. Washing Buffer (W2) 20 ml W2 buffer is supplied as a concentrate. Before the first use, add 80 ml of absolute ethanol. W2 buffer is stable for 2 year when stored closed at room temperature. Elution Buffer (EL) 25 ml 10 mm Tris-HCl(pH8.5). Store at room temperature. Columns and tubes DNA-binding column tubes 100 ea 2 ml tubes for filtration 100 ea 1.5 ml tubes for elution 100 ea 4

III. Required Reagents and Equipment 1. Absolute ethanol 2. Absolute isopropanol 3. Table-top microcentrifuge 10,000 x g (13,000 rpm) 4. Incubator or thermal block. IV. Before You Begin Before you proceed, check the followings. 1. Did you dissolve proteinase K in 1.25 ml of nuclease-free water? 2. Did you add adequate amount of absolute ethanol to washing buffer 1 (W1) and washing buffer 2 (W2)? 3. Before starting a extraction process warm the Elution buffer (EL) to 60 The Binding buffer contains irritant chaotropic salt. Take appropriate laboratory safety precaution, and wear gloves when handling. If everything is prepared, you can proceed. 5

V. Experimental Protocol 1. Extracting DNA from beans 1) Grind 50-100 mg of beans to fine powder. Put the powder and 400 ul of Lysis Buffer (L) in a 1.5 ml microcentrifuge tube. Powdered beans are efficient for lysis.. 2) Add 20 ul of Proteinase K, mix, and incubate for 10 minutes at 60. You should observe the formation of aggregates. 3) After the bean powder has been lysed for 10 minutes, briefly spin down, add 400 ul of Binding buffer (B), and mix well. 4) Incubate for 10 minutes at 60. 5) After 10 minutes, centrifuge the tube at 12,000 rpm for 5 minutes, then transfer the supernatant to a new tube. 6) Add 100 ul of isopropanol, lightly vortex for about 5 seconds, and then spin down for 10 seconds to get the liquid clinging to the walls and lid of the tube. 7) Fit the binding column into the 2ml tube and transfer the liquid into the binding column. Be cautious not to get the lid wet. 8) Carefully close lid and centrifuge for 1 minute at 8,000 rpm. If the liquid is left on the column, not completely passing the column following centrifugation, centrifuge again until the liquid has completely passed. 6

9) Following THE centrifugation, transfer the binding column to a new 2 ml tube. 10) Add 500 ul of washing buffer 1 (W1) to the column, without the sides getting wet; close the lid, and centrifuge for 1minute at 8,000 rpm. 11) Carefully open the binding column and pour the solution in 2 ml tube to garbage bottle. 12) Add 500 ul of Washing buffer 2 (W2), without the sides getting wet; close the lid, and centrifuge for 1 minute at 8,000 rpm. 13) Spin down once more at 13,000 rpm for 1 minute to completely remove ethanol. Check that there is no droplet hanging at the bottom of the binding column. Residual Washing buffer 2 (W2) left in the binding column can hinder the following steps. Transfer the binding column to a 1.5 ml collection tube, add 200 ul of Elution Buffer, and react for 1 minute to allow the buffer to permeate the column. Longer reaction time will increase the product yield. You can add less Elution Buffer, for example, 50 ul or 100 ul, for a higher concentration of DNA, but the total yield will be reduced. You can also increase yield by heating the Elution Buffer to about 70 before adding to the column. 14) Elute by spinning down at 8,000 rpm for 1 minute. About 180 ul of eluate can be recovered after using 200 ul of Elution buffer. For maximum yield, you can repeat the elution step. The eluted DNA solution can be directly used, or stored at 4 or 20 for longer storage periods. 7

VI. Problems Solving 1. Yield or purity of DNA is low. 1) The kit may have been stored under non-optimal conditions. Store kit at 15-25 at all times upon arrival. 2) Buffers or other reagents may have been exposed to conditions that reduced their effectiveness. Store all buffers at 15-25 C. Close all reagent bottles tightly after use, in order to preserve ph, stability, and to avoid contamination. After constitution of any lyophilized reagent, separate into aliquots and store each aliquot at either 2 ~ 8 or -15 ~ - 25 (as indicated in the manual). 3) Ethanol may not have been added to the Washing Buffers. Add absolute ethanol to all Wash Buffers before using. After adding ethanol, mix the Wash Buffer well and store at 15 ~ 25. Always mark the Wash Buffer vial to indicate whether ethanol has been added or not. 4) Reagents and samples may not have been completely mixed. Always mix the sample tube thoroughly after adding each reagent. 2. There is a low recovery of DNA following elution. You may not have used the optimal reagent for DNA elution. An alkaline ph is required for optimal elution. 8

Do not use water to elute DNA. Use the Elution Buffer included in the kit. 3. There is an incomplete or no restriction enzyme cleavage of DNA extracted from the kit. Glass fibers, which can be coeluted along with the DNA, may inhibit enzyme reactions After the final elution step has been completed, remove column filter from tube containing the eluted sample and spin the sample tube for 1 minute at maximum speed. Glass fibers may be visible at the bottom of the tube. Transfer the supernatant into a new tube, without disturbing the glass fibers at the bottom of the original tube. 4. The absorbency (A 260 ) reading of product is too high. Glass fibers which can coelute with nucleic acid, can scatter light, resulting in a higher absorbency reading. See the method above for removal of glass fibers. 5. There is a low yield of DNA. 1) Proteinase K may not have been completely solubilized. Follow the steps to completely solubilize the lyophilized Proteinase K: 1. Pipette 2.5mL of double distilled water into the glass vial containing lyophilized Proteinase K. 2. Close and invert the vial until all the lyophilizate is dissolved. 3. Separate the reconstituted enzymes into aliquots, mark each one, and store them at 15 to -25 C. *Note : Proteinase K reconstituted this way is stable for 12 months when stored properly. 2) The lysis may have been incomplete. Mix sample 9

immediately after adding Proteinase K. Always mix the lysate thoroughly with isopropanol before adding the sample to the column filter tube. 6. There is a low yield from tissue. Proteinase K digestion may have been incomplete. Be sure to slice the tissue into small pieces before the digestion and lysis steps. There are two ways to increase the incubation time: 1. Incubate tissue overnight with Proteinase K. 2. Incubate with Proteinase K for 3 ~ 4 hr, then add a fresh aliquot of Proteinase K (30 µl) and incubate for another 1 ~ 2 hr. 7. DNA from tissue samples is degraded. There may have been nuclease activity in the unlysed tissue. Tissue should be stored frozen (-20 C) after harvest until the lysis procedure starts. Use only small pieces of tissue (20-40 mg) when homogenizing the tissue sample. 8. The final eluent from blood is still slightly colored. You may not have washed adequately. Wash the filter tube until the flowthrough is colorless. Repeat the purification protocol by mixing 200 µl of eluent with 400 µl of Binding Buffer, then 100 µl of isopropanol. 9. There is a white precipitate in Buffer L or Buffer B. A white precipitate may form in Buffer L or Buffer B after prolonged storage at low temperature. 10

Any precipitate in L Buffer or B Buffer must be dissolved by incubating the buffer at 70 C. The precipitate causes no malfunction, however, dissolving the precipitate at high temperatures will not improve yield and quality of the purified nucleic acids. VII. Supplement 1. Typical Results The yield and purity of genomic DNA vary depending on the samples. The table below shows experimental results. Sample Amounts Yield (µg) Soybean 100mg 2 ~ 5 Maize 100mg 1 ~ 4 Potato 100mg 1 ~ 4 2. Purification yield You can extract about 5 g of DNA from 200 l eluent (25 ng/ l), with an A 260/A 280 ratio of 1.7 ~ 1.9 of a 100 mg of Soybean sample. 11

VIII. References 1. Boom, R. et al. (1990), J Clin. Microbiol., 28, 495-503 2. Carter, M.J. and Milton, I.D. (1993) Nucleic Acids Res., 21, 1044 3. Melzak, K. A. et al. (1996), J Colloid and Interface Sci., 181, 635-644 4. Taylor,R. G., Walker, D. C. and Mclnnes, R. R. (1993) Nucleic Acids Res., 21, 1577-1678 5. Sambrook, J., Fritsch, E.F. and Maniatis, T. (1989) MolecuLar Cloning 2nd. ed. IX. Product information Product Content Cat. No. AccuPrep GMO DNA 100 Purifications K-3031 Extraction Kit 12

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