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Protocol (50 prep) - Norgen Biotek Corp.

1. directly processed Please check the product and proceed to the appropriate section for your i Plasma Serum cfc DNA Purification Section 1 Plasma Serum cfc DNA Purification Micro Kit Product 55500 Note The procedure outlined below is for 200 uL inputs of Plasma Serum If processing a sample volume lower than 200 uL Plasma Serum simply bring the volume of your samples up to 200 uL using 1X PBS and proceed as outlined below 1 Place 200 uL of plasma serum sample in a 2 mL tube provided by the user Add 6 uL Proteinase K and mix well by vortexing for 10 seconds then incubate at 55 C for 10 minutes 2 After incubation add 600 uL of Binding Buffer B and mix well by vortexing for 10 seconds 3 Transfer 400 uL of the mixture from Step 2 into a Micro Spin column assembled with one of the provided collection tubes Centrifuge for 2 minutes at 3 300 x g 6 000 RPM Discard the flowthrough and reassemble the spin column with its collection tube 4 Repeat Step 3 to transfer the remaining mixture into the Micro Spin column 5 Apply 600 uL of Wash Solution A to the column and centrifuge for 1 minute at 3 300 x g 6 000 RPM Discard the flowthrough and reassemble the spin column with its collection tube 6 Repeat Step 5 one more time for a total of two washes 7 Spin the column empty for 2 minutes at 13 000 x g 14 000 RPM Discard the collection tube 8 Transfer the spin column to a fresh 1 7 mL Elution tube Apply 25 50 uL
2. standard DNA using a small DNA amplicon such as the 5S rRNA housekeeping gene Common DNA Quantification Methods 1 2100 Bioanalyzer DNA Quantification kits DNA1000Kit DNA 7500 Kit DNA 12000 Kit High Sensitivity DNA Kit 25 1000 bp 100 7500 bp 100 12000 bp 50 7000 bp 20 CV 20 CV 25 CV 20 CV 0 5 50 ng L 0 5 50ng pL 0 5 50 ng pL 5 500 pg pL 2 NanoDrop 2000 gt Detection Limit 2 ng ul dsDNA 3 Quant iT Pico Green dsDNA Assay Kit gt Detection Limit 25 pg mL 4 qPCR DNA Standard Curve generated by Norgen Standard Curve Log Starting Quantity O Standard X Unknown SYBR E 296 1 R 2 0 890 Sjope 1 673 y int 32 707 Frequently Asked Questions 1 What if a variable speed centrifuge is not available and the speed differs from the recommended e A fixed speed centrifuge can be used however reduced yields may be observed 2 At what temperature should I centrifuge my samples e All centrifugation steps are performed at room temperature Centrifugation at 4 C will not adversely affect kit performance 3 What if added more or less of the specified reagents volume e Adding more or less than the specified volumes may reduce both the quality and the quantity of the purified DNA Eluting your DNA in high volumes will increase the yield but will lower the concentration Eluting in small volumes will increase the concentration but will lower the overall yield 4 What If I forgot t
3. 3430 Schmon Parkway Thorold ON Canada L2V 4Y6 Phone 866 667 4362 e 905 227 8848 Fax 905 227 1061 Email techsupport norgenbiotek com NORGEN BIOTEK wie CORPORATION gn x Plasma Serum Cell Free Circulating DNA Purification Kits Product Insert Product 55500 55100 55600 55800 Introduction It has been suggested recently that Plasma Serum cell free circulating DNA cfc DNA can be utilized as a biomarker CFC DNA has the potential to provide biomarkers for certain cancers and disease states as well as fetal DNA in maternal blood Currently significant advancements are being made in utilizing cfc DNA as biomarkers for the early diagnosis prognosis and monitoring of therapy for several cancer types and autoimmune diseases Cell free mitochondrial DNA cfmtDNA is also under investigation for its clinical significance This cfc DNA is usually present as short fragments of less than 1000 bp In addition cell free fetal DNA has been widely used as a non invasive method for prenatal diagnosis including early identification of fetal sex genetic studies for families at high risk for inherited genetic disorders screening for Rhesus factor screening for aneuploidy and identification of preeclampsia Norgen s Plasma Serum Cell Free Circulating DNA Purification Kits provide fast reliable and simple procedures for isolating cell free circulating DNA cfc DNA from various amounts of plasma serum ranging from 10 uL up to 10 mL where
4. 5600 Cat 55800 Sample Type Plasma Serum Plasma Serum Plasma Serum Plasma Serum Anti lant for Plasma EDTA Citrate EDTA Citrate or EDTA Citrate EDTA Citrate coagulant fo or Heparin Heparin or Heparin or Heparin Sample Volume Range 10 to 200 uL 200 to 500 uL 1to4mL 5 to 10 mL Minimum Elution Volume 25 uL 50 uL 50 uL 50 uL Maximum Elution Volume 50 uL 100 uL 100 uL 100 uL Time ta Complete 10 15 20 minutes 15 20 minutes 40 45 minutes 40 45 minutes Purifications Size of DNA Purified 2 50 bp Average Yields Variable depending on specimen Please check page 7 for Average Plasma Serum Yields and Common DNA Quantification Methods Customer Supplied Reagents and Equipment e Benchtop microcentrifuge e Micropipettors e 15 mL and or 50 mL tubes e 96 100 ethanol Storage Conditions and Product Stability All buffers should be kept tightly sealed and stored at room temperature 15 25 C for up to 2 years without showing any reduction in performance Norgen s Plasma Serum Cell Free Circulating DNA Purification Kits contain ready to use Proteinase K solution which is dissolved in a specially prepared storage buffer The Proteinase K is stable for up to 2 5 years after delivery when stored at room temperature To prolong the lifetime of Proteinase K storage at 2 8 C is recommended Quality Control In accordance with Norgen s Quality Management System each lot of Norgen s Plasma Serum Cell Free Circulating DNA Purifica
5. disposable tubes etc It is recommended that gloves are changed frequently to avoid contamination gt Ensure that all solutions are at room temperature prior to use and that no precipitates have formed If necessary warm the solutions and mix well until the solutions become clear again gt Prepare a working concentration of the Wash Solution A by adding 42 mL of 96 100 ethanol provided by the user to the supplied bottle containing the concentrated Wash Solution A This will give a final volume of 60 mL The label on the bottle has a box that may be checked to indicate that the ethanol has been added gt Ensure that samples have not undergone more than one freeze thaw cycle as this may lead to DNA degradation gt Preheat an incubator or heating block to 55 C gt Always vortex the Proteinase K before use gt This kit is suitable for the isolation of DNA from fresh or frozen serum or plasma prepared from blood collected on Heparin EDTA or citrate gt If any of the solutions do not go through the Spin Columns within the specified centrifugation time spin for an additional 1 2 minutes until the solution completely passes through the column Do NOT exceed the centrifugation speed as this may affect DNA yield gt Frozen plasma or serum samples should be centrifuged for 2 minutes at 400 x g 2 000 RPM before processing Only clear supernatant should be processed as column clogging may be encountered if frozen samples are
6. econds 2 Transfer up to 14 mL of the mixture from Step 1 into a Maxi Spin column assembled with one of the provided collection tubes Centrifuge for 2 minutes at 1 000 x g 2 200 RPM Discard the flowthrough and reassemble the spin column with its collection tube Note Make sure that lid of the tubes is not tightly closed Repeat Step 2 to transfer the remaining mixture from Step 1 into the Maxi Spin column 4 Transfer the Maxi Spin column to a fresh 50 mL tube not provided Apply 0 5 mL of Elution Buffer B to the column and let stand at room temperature for 2 minutes Centrifuge for 2 minutes at 500 x g 1 600 RPM 5 Apply an additional 1 mL of Elution Buffer B to the column and let stand at room temperature for 3 minutes Centrifuge for 3 minutes at 500 x g 1 600 RPM 6 To the elution from Step 5 add 115 uL of Proteinase K and mix well by vortexing for 10 seconds then incubate the mixture at 55 C for 35 minutes 7 After incubation add 1 5 mL of Binding Buffer B to the mixture and mix well by vortexing for 10 seconds 8 Transfer 800 uL of the mixture from Step 7 into a Mini Spin column assembled with one of the provided collection tubes Centrifuge for 2 minutes at 3 300 x g 6 000 RPM Discard the flowthrough and reassemble the spin column with its collection tube 9 Repeat Step 8 three more times to transfer the remaining mixture into the Mini Spin column 10 Apply 600 uL of Wash Solution A to the column and ce
7. enaturants Check the compatibility of your Elution Buffer with the intended use 10 Do I need to do an RNase treatment for my DNA Elution e Norgen s Plasma Serum Cell Free Circulating DNA Purification Mini Kit doesn t co purify plasma serum circulating RNA along with circulating DNA therefore an RNase step is not required 11 Why are the A260 280 ratio and the A260 230 ratio of the purified DNA low e Most of the Plasma Serum Cell Free Circulating DNA is present in short fragments The low A260 280 ratio and the low A260 230 ratio will not affect any downstream applications Technical Assistance NORGEN s Technical Service Department is staffed by experienced scientists with extensive practical and theoretical expertise in sample and assay technologies and the use of NORGEN products If you have any questions or experience any difficulties regarding Norgen s Plasma Serum Cell Free Circulating DNA Purification Kits or NORGEN products in general please do not hesitate to contact us NORGEN customers are a valuable source of information regarding advanced or specialized uses of our products This information is helpful to other scientists as well as to the researchers at NORGEN We therefore encourage you to contact us if you have any suggestions about product performance or new applications and techniques For technical assistance and more information please contact our Technical Support Team between the hours of 8 30 and 5 30 Eastern Standa
8. hould be taken when working with plasma or serum Important Notes gt All centrifugation steps are performed at room temperature gt Ensure that centrifuge tubes used are capable of withstanding the centrifugal forces required gt The spin columns provided with Norgen s Plasma Serum Cell Free Circulating DNA Purification Kits are optimized to be used with benchtop centrifuges and not to be used on a vacuum apparatus gt Most standard benchtop microcentrifuges will accommodate Norgen s Micro and Mini Spin Columns gt Most standard swinging bucket centrifuges will accommodate Norgen s Midi and Maxi Spin Columns Do not use a fixed angle rotor gt Norgen s Midi and Maxi Spin Columns are centrifuged in 15 mL and 50 mL centrifuge tubes respectively gt Centrifuging Norgen s spin columns at a speed higher than recommended in the procedure may affect DNA yield gt Centrifuging Norgen s spin columns at a speed lower than recommended in the procedure will not affect DNA yield However centrifugation at a lower speed may require longer time for the solutions to pass through the spin column gt When placing Norgen s Midi and Maxi Spin Columns into the swinging bucket centrifuge make sure that lids of the tubes are not tightly closed Tightly closed lids may cause back pressure which may cause column clogging or disintegration gt Clean disposable gloves should be worn at all times when handling reagents samples pipettes
9. ing Buffer B and mix well by vortexing for 10 seconds 2 Transfer up to 5 5 mL of the mixture from Step 1 into a Midi Spin Column assembled with one of the provided collection tubes Centrifuge for 3 minutes at 1 000 x g 2 200 RPM Discard the flowthrough and reassemble the spin column with its collection tube Note Make sure that lid of the tubes is not tightly closed Repeat Step 2 to transfer the remaining mixture from Step 1 into the Midi Spin column 4 Transfer the Midi Spin column to a fresh 15 mL tube not provided Apply 0 25 mL of Elution Buffer B to the column and let stand at room temperature for 2 minutes Centrifuge for 2 minutes at 500 x g 1 600 RPM 5 Apply an additional 1 mL of Elution Buffer B to the column and let stand at room temperature for 3 minutes Centrifuge for 3 minutes at 500 x g 1 600 RPM 6 To the elution from Step 5 add 47 uL of Proteinase K and mix well by vortexing for 10 seconds then incubate the mixture at 55 C for 25 minutes 7 After incubation add 1 25 mL of Binding Buffer B to the mixture and mix well by vortexing for 10 seconds 8 Transfer 700 uL of the mixture from Step 7 into a Mini Spin column assembled with one of the provided collection tubes Centrifuge for 2 minutes at 3 300 x g 6 000 RPM Discard the flowthrough and reassemble the spin column with its collection tube 9 Repeat Step 8 three more times to transfer the remaining mixture into the Mini Spin column 10 A
10. ly fluids including plasma or serum Cell free circulating DNA yield varies depending on a number of factors including age sex diet exercise and most importantly the health status of the donor Below is a list of the most common DNA quantification methods as well as the limit of detection for each of these methods Unfortunately none _of these methods can be used reliably for measuring the concentration of DNA purified from plasma or serum unless large plasma serum volumes have been processed This would only be applicable if plasma serum contains the maximum amount of DNA that can fit within the specification range of these quantification tools It should be noted that the specifications outlined below are based on measuring a pure dsDNA which will not be the case for the DNA purified from plasma or serum Plasma Serum DNA is short fragmented DNA which is usually present in less than 1000 bp Purified plasma serum DNA usually contains traces of proteins which will interfere with most quantification methods leading to the overestimation of the purified DNA concentration Therefore purified DNA contaminated with more proteins will be presented at a higher concentration as compared to DNA purified with less protein contaminants which in this case will depend on the method used for plasma serum DNA purification The only reliable method that can assess the quality and the relative quantity of the purified plasma serum DNA is qPCR amplification of a
11. nsfer the remaining mixture into the Mini Spin column 5 Apply 600 uL of Wash Solution A to the column and centrifuge for 1 minute at 3 300 x g 6 000 RPM Discard the flowthrough and reassemble the spin column with its collection tube 6 Repeat Step 5 one more time for a total of two washes 7 Spin the column empty for 2 minutes at 13 000 x g 14 000 RPM Discard the collection tube 8 Transfer the spin column to a fresh 1 7 mL Elution tube Apply 50 uL of Elution Buffer B to the column and let stand at room temperature for 2 minutes Centrifuge for 1 minute at 400 x g 2 000 RPM followed by 2 minutes at 5 800 x g 8 000 RPM 9 For maximum recovery transfer the eluted buffer back to the column and let stand at room temperature for 2 minutes Centrifuge for 1 minute at 400 x g 2 000 RPM followed by 2 minutes at 5 800 x g 8 000 RPM gt Plasma Serum DNA is ready for the downstream application of your choice For an explanation of expected yields and recommendations for quantification of the DNA please refer to Appendix A Section 3 Plasma Serum cfc DNA Purification Midi Kit Product 55600 Note The procedure outlined below is for processing 1 mL to 4 mL inputs of Plasma Serum If the sample volume is lower than 4 mL Plasma Serum simply bring the volume of your sample up to 4 mL using 1X PBS and proceed as outlined below 1 Place 4 mL of plasma serum sample in a 15 mL tube provided by the user Add 7 mL of Bind
12. ntrifuge for 1 minute at 3 300 x g 6 000 RPM Discard the flowthrough and reassemble the spin column with its collection tube 11 Repeat Step 10 one more time for a total of two washes 12 Spin the column empty for 2 minutes at 13 000 x g 14 000 RPM Discard the collection tube 13 Transfer the spin column to a fresh 1 7 mL Elution tube Apply 50 uL of Elution Buffer B to the column and let stand at room temperature for 2 minutes Centrifuge for 1 minute at 400 x g 2 000 RPM followed by 2 minutes at 5 800 x g 8 000 RPM 14 For maximum recovery transfer the eluted buffer back to the column and let stand at room temperature for 2 minutes Centrifuge for 1 minute at 400 x g 2 000 RPM followed by 2 minutes at 5 800 x g 8 000 RPM gt Plasma Serum DNA is ready for the downstream application of your choice For an explanation of expected yields and recommendations for quantification of the DNA please refer to Appendix A Appendix A Cell Free Circulating DNA Yield Plasma Serum Cell free circulating DNA cfc DNA is normally found in very low amounts 1 100 pg L therefore measuring cfc DNA concentration using common DNA quantification methods is very difficult and challenging Typical yields of cfc DNA vary significantly from sample to sample Variability is also observed between samples collected from the same donor at different times during the day and therefore there is no absolute yield for cfc DNA purified from bodi
13. o do a dry spin before my final elution step e Your purified DNA will be contaminated with the Wash Solution A This may reduce the quality of your purified DNA and will interfere with your downstream applications 5 Can I perform a second elution e Yes but it is recommended that the 2 elution be in a smaller volume 50 of 1 Elution It is also recommended to perform the 2 elution into a separate elution tube to avoid diluting the 1 elution 6 What if my incubation temperature varied from the specified 55 C e The incubation temperature can be in the range of 55 C 60 C If the temperature is outside of that range the activity of the Proteinase K will be reduced This will result in a reduction in your DNA yields 7 What if my incubation time varied from what is specified in the product manual e Varying the incubation time will result in a reduction in your DNA yields 8 Why do my samples show very low DNA yield e Plasma Serum samples contain very little cfc DNA This varies from individual to individual In order to increase the yield the amount of Plasma Serum input could be increased 9 Why does my purified cfc DNA not perform well in downstream applications e lf a different Elution Buffer was used other than the one provided in the kit the buffer should be checked for any components that may interfere with the application Common components that are known to interfere are high salts including EDTA detergents and other d
14. of Elution Buffer B to the column and let stand at room temperature for 2 minutes Centrifuge for 1 minute at 400 x g 2 000 RPM followed by 2 minutes at 5 800 x g 8 000 RPM 9 For maximum recovery transfer the eluted buffer back to the column and let stand at room temperature for 2 minutes Centrifuge for 1 minute at 400 x g 2 000 RPM followed by 2 minutes at 5 800 x g 8 000 RPM gt Plasma Serum DNA is ready for the downstream application of your choice For an explanation of expected yields and recommendations for quantification of the DNA please refer to Appendix A Section 2 Plasma Serum cfc DNA Purification Mini Kit Product 55100 Note The procedure outlined below is for processing 200 uL to 500 uL inputs of Plasma Serum If the sample volume is lower than 500 pL Plasma Serum simply bring the volume of your sample up to 500 uL using 1X PBS and proceed as outlined below 1 Place 500 uL of plasma serum sample in a 2 mL tube provided by the user Add 12 uL Proteinase K and mix well by vortexing for 10 seconds then incubate at 55 C for 10 minutes 2 After incubation add 1000 uL of Binding Buffer B and mix well by vortexing for 10 seconds 3 Transfer 800 uL of the mixture from Step 2 into a Mini Spin column assembled with one of the provided collection tubes Centrifuge for 2 minutes at 3 300 x g 6 000 RPM Discard the flowthrough and reassemble the spin column with its collection tube 4 Repeat Step 3 to tra
15. pply 600 uL of Wash Solution A to the column and centrifuge for 1 minute at 3 300 x g 6 000 RPM Discard the flowthrough and reassemble the spin column with its collection tube 11 Repeat Step 10 one more time for a total of two washes 12 Spin the column empty for 2 minutes at 13 000 x g 14 000 RPM Discard the collection tube 13 Transfer the spin column to a fresh 1 7 mL Elution tube Apply 50 uL of Elution Buffer B to the column and let stand at room temperature for 2 minutes Centrifuge for 1 minute at 400 x g 2 000 RPM followed by 2 minutes at 5 800 x g 8 000 RPM 14 For maximum recovery transfer the eluted buffer back to the column and let stand at room temperature for 2 minutes Centrifuge for 1 minute at 400 x g 2 000 RPM followed by 2 minutes at 5 800 x g 8 000 RPM gt Plasma Serum DNA is ready for the downstream application of your choice For an explanation of expected yields and recommendations for quantification of the DNA please refer to Appendix A Section 4 Plasma Serum cfc DNA Purification Maxi Kit Product 55800 Note The procedure outlined below is for processing 5 mL to 10 mL inputs of Plasma Serum If the sample volume is lower than 10 mL Plasma Serum simply bring the volume of your sample up to 10 mL using 1X PBS and proceed as outlined below 1 Place 10 mL of plasma serum sample in a 50 mL tube provided by the user Add 17 5 mL of Binding Buffer B and mix well by vortexing for 10 s
16. rd Time at 905 227 8848 or Toll Free at 1 866 667 4362 or call one of the NORGEN local distributors www norgenbiotek com or through email at techsupport norgenbiotek com 3430 Schmon Parkway Thorold ON Canada L2V 4Y6 Phone 905 227 8848 Fax 905 227 1061 Toll Free in North America 1 866 667 4362 2015 Norgen Biotek Corp PI55500 2 M14
17. tion Kits is tested against predetermined specifications to ensure consistent product quality Product Use Limitations Norgen s Plasma Serum Cell Free Circulating DNA Purification Kits is designed for research purposes only It is not intended for diagnostic use Product Warranty and Satisfaction Guarantee NORGEN BIOTEK CORPORATION guarantees the performance of all products in the manner described in our product manual The customer must determine the suitability of the product for its particular use Safety Information Ensure that a suitable lab coat disposable gloves and protective goggles are worn when working with chemicals For more information please consult the appropriate Material Safety Data Sheets MSDSs These are available as PDF files online at www norgenbiotek com Binding Buffer B contains guanidine hydrochloride GnHCI and should be handled with care GnHCl forms highly reactive compounds when combined with bleach thus care must be taken to properly dispose of any of these solutions If liquid containing this buffer is spilt clean with suitable laboratory detergent and water If the spilt liquid contains potentially infectious agents clean the affected area first with laboratory detergent and water and then with 1 v v sodium hypochlorite Plasma or serum of all human and animal subjects is considered potentially infectious All necessary precautions recommended by the appropriate authorities in the country of use s
18. various kit formats address different plasma serum input volumes Purification is based on spin column chromatography that uses Norgen s proprietary resin separation matrix The kits are designed to isolate all sizes of cfc DNA from either fresh or frozen plasma serum samples Moreover these kits allow the user to elute the purified cfc DNA into a flexible elution volume ranging from 25 uL to 50 uL The purified plasma serum cfc DNA is eluted in an Elution Buffer that is compatible with all downstream applications including PCR qPCR methylation sensitive PCR and Southern Blot analysis microarrays and NGS Kit Descriptions and Components Micro Kit Mini Kit Midi Kit Maxi Kit Cat 55500 Cat 55100 Cat 55600 Cat 55800 Number of Preps 50 preps 50 preps 20 preps 10 preps Binding Buffer B 40 mL beatae 2x 85 mL ree ra 1 Proteinase K 0 3 mL 0 6 mL 1 mL 1 2 mL Wash Solution A 18 mL 18 mL 18 mL 18 mL Elution Buffer B 8 mL 8 mL 30 mL 30 mL Micro Spin Columns 50 Mini Spin Columns 50 20 10 Midi Spin Column 20 Maxi Spin Column 10 Collection Tubes 50 50 20 10 Elution tubes 1 7 mL 50 50 20 10 Product Insert 1 1 1 1 These kits are suitable for the isolation of cfc DNA from fresh or frozen serum plasma prepared from blood collected on either Heparin EDTA or Citrate Kits Specifications Micro Kit Mini Kit Midi Kit Maxi Kit Cat 55500 Cat 55100 Cat 5

Protocol (50 prep) - Norgen Biotek Corp.

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