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SSIV_First_Strand_Synthesis_System_UG.pdf

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Pub. no. MAN0013442 Rev. B.0 SuperScript™ IV First-Strand Synthesis System Protocol outline A. Anneal primer to RNA B. Assemble reaction mix C. Add reaction mix to annealed RNA RT reaction setup Use the measurements below to prepare your RT reaction, or enter your own parameters in the column provided. Component 20-µL rxn Custom Final Conc. DEPC-treated water to 20 µL to µL N/A 5× SSIV Buffer 4.0 µL µL 1× 10 mM dNTP mix (10 mM each) 1.0 µL µL 0.5 mM each 100 mM DTT 1.0 µL µL 5 mM Ribonuclease Inhibitor (40 U/µL) 1.0 µL µL 2.0 U/µL 50 µM Oligo d(T)20 primer, or 50 ng/μL random hexamers, or 2 µM gene-specific primer 1.0 µL 1.0 µL 1.0 µL µL 2.5 µM 2.5 ng/μL 0.1 µM Template RNA* varies µL < 5 μg total RNA or < 500 ng mRNA * 10 pg–5 µg total RNA or 10 pg–500 ng mRNA RT protocol Go to page 2 for instructions on preparing and running your RT experiment. Optimization strategies and troubleshooting Refer to the pop-ups below for guidelines to optimize and troubleshoot your RT reaction. RNA Sample Prep RT Guidelines Troubleshooting Limited Warranty, Disclaimer, and Licensing Information Package contents Catalog Number 18091050 18091200 Size 50 reactions 200 reactions Kit Contents Storage conditions Store at –20°C (non-frost-free) Required materials ∤ ∤ Template: RNA ∤ ∤ Optional: 2 μM gene-specific primers Timing ∤ ∤ Preparation time: 10 minutes ∤ ∤ Run time: 20 minutes Selection guides Go online to view related products. PCR Enzymes and Master Mixes RT Enzymes and Kits Real-Time PCR Instruments Real-Time PCR Master Mixes PCR Thermal Cyclers Product description For first strand cDNA synthesis using total RNA or poly(A)+-selected RNA primed with oligo(dT), random primers, or a gene-specific primer. Important guidelines Pre-warm the 5× SSIV Buffer to room temperature before use. Vortex and briefly centrifuge the buffer prior to preparing the reverse transcription reaction mix. Online resources Visit our product page for additional information and protocols. For support, visit www.thermofisher/support. For Research Use Only. Not for use in diagnostic procedures. Print Options
For support, visit www.thermofisher.com/support. SuperScript™ IV First-Strand Synthesis System User Guide -2- 6 SuperScript™ IV First-Strand cDNA Synthesis Reaction The example procedure below shows appropriate volumes for a single 20-µL reverse transcription reaction. For multiple reactions, prepare a master mix of components common to all reactions to minimize pipetting error, then dispense appropriate volumes into each reaction tube prior to adding annealed template RNA and primers. Steps Procedure Procedure details 1 Anneal primer to template RNA a. Combine the following components in a PCR reaction tube. Note: Consider the volumes for all components listed in steps 1 and 2 to determine the correct amount of water required to reach your final reaction volume. Component Volume 50 µM Oligo d(T)20 primer, 50 ng/μL random hexamers, or 2 µM gene-specific reverse primer 1 µL 10 mM dNTP mix (10 mM each) 1 µL Template RNA (10 pg–5 µg total RNA or 10 pg–500 ng mRNA) up to 11 µL DEPC-treated water to 13 µL b. Mix and briefly centrifuge the components. c. Heat the RNA-primer mix at 65°C for 5 minutes, and then incubate on ice for at least 1 minute. 2 Prepare RT reaction mix a. Vortex and briefly centrifuge the 5× SSIV Buffer. b. Combine the following components in a reaction tube. Component Volume 5× SSIV Buffer 4 µL 100 mM DTT 1 µL Ribonuclease Inhibitor 1 µL SuperScript™ IV Reverse Transcriptase (200 U/μL) 1 µL c. Cap the tube, mix, and then briefly centrifuge the contents. 3 Combine annealed RNA and RT reaction mix Add RT reaction mix to the annealed RNA. 4 Incubate reactions a. If using random hexamer, incubate the combined reaction mixture at 23°C for 10 minutes, and then proceed to step b. If using oligo d(T)20 or gene-specific primer, directly proceed to step b. b. Incubate the combined reaction mixture at 50–55°C for 10 minutes. c. Inactivate the reaction by incubating it at 80°C for 10 minutes. 5 Optional: Remove RNA Note: Amplification of some PCR targets (>1 kb) may require removal of RNA. To remove RNA, add 1 µL E. coli RNase H, and incubate 37°C for 20 minutes. PCR amplification Use your RT reaction immediately for PCR amplification or store it at–20°C. Note: As a recommended starting point for PCR, reverse transcription reaction (cDNA) should compose 10% of the total reaction volume
For support, visit www.thermofisher.com/support. SuperScript™ IV First-Strand Synthesis System User Guide -3- SuperScript™ IV Control Reactions - cDNA synthesis reaction Follow the procedure below to perform the cDNA synthesis step of the SuperScript™ IV RT-PCR control reactions. Steps Procedure Procedure details 1 Anneal primer to template RNA a. Prepare two tubes for annealing primer to template RNA. In each tube, combine the following: Component Volume 50 µM Oligo d(T)20 primer 1 µL 10 mM dNTP mix (10 mM each) 1 µL 10 ng/μL total HeLa RNA (10 ng total) 1 µL DEPC-treated water 10 µL b. Mix and briefly centrifuge the components. c. Heat the RNA-primer mix at 65°C for 5 minutes, and then incubate on ice for at least 1 minute. 2 Prepare RT reaction mix a. Vortex and briefly centrifuge the 5× SSIV Buffer. b. Prepare two reactions. In each reaction tube, combine the following: Component Volume 5× SSIV Buffer 4 µL 100 mM DTT 1 µL Ribonuclease Inhibitor 1 µL SuperScript™ IV Reverse Transcriptase (positive control) or DEPC-treated water (no RT control) 1 µL c. Cap the tube, mix, and then briefly centrifuge the contents. 3 Combine annealed RNA and RT reaction mix Add RT reaction mix to the annealed RNA. 4 Incubate reactions a. Incubate the combined reaction mixture at 50°C for 10 minutes. b. Inactivate the reaction by incubating it at 80°C for 10 minutes. 5 Remove RNA a. Add 1 µL E. coli RNase H and incubate 37°C for 20 minutes. b. Proceed to PCR amplification (page 4)
For support, visit www.thermofisher.com/support. SuperScript™ IV First-Strand Synthesis System User Guide -4- 20 August 2015 SuperScript™ IV Control Reactions - PCR amplification Follow the procedure below to perform the PCR amplification step of the SuperScript™ IV RT-PCR control reactions. Steps Procedure Procedure details 1 Assemble PCR amplification mix a. Prepare two reactions. In each tube, combine the following: Component Volume DEPC-treated water 37.8 µL 10× High Fidelity PCR Buffer 5 μL 50 mM MgSO4 2 μL 10 mM dNTP mix (10 mM each) 1 μL Control sense primer (10 µM) (5’-GCTCGTCGTCGACAACGGCTC-3’) 1 μL Control antisense primer (10 µM) (5’-CAAACATGATCTGGGTCATCTTCTC-3’) 1 μL cDNA from positive control reaction (step 5, page 3) or DEPC-treated water for no RT control 2 μL Platinum™ Taq DNA Polymerase High Fidelity (5 U/µL) 0.2 μL b. Mix gently by pipetting up and down and briefly centrifuge the components. 2 Incubate reactions in a thermal cycler a. Place reaction mixture in preheated (94°C) thermal cycler. b. Perform PCR amplification using the following cycling parameters: Step Temperature Time Initial denaturation 94°C 2 minutes 35 PCR cycles Denature 94°C 15 seconds Anneal 55°C 30 seconds Extend 68°C 1 minute Hold 4°C hold 3 Analyze with gel electrophoresis Analyze 10 µL of each reaction using agarose gel electrophoresis and ethidium bromide staining. A 353-bp band should be visible for the positive control reaction with RT. For the no RT control reaction, the same band should be ≤ 50% in intensity when compared to the positive control.

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SSIV_First_Strand_Synthesis_System_UG.pdf

  • 1. Pub. no. MAN0013442 Rev. B.0 SuperScript™ IV First-Strand Synthesis System Protocol outline A. Anneal primer to RNA B. Assemble reaction mix C. Add reaction mix to annealed RNA RT reaction setup Use the measurements below to prepare your RT reaction, or enter your own parameters in the column provided. Component 20-µL rxn Custom Final Conc. DEPC-treated water to 20 µL to µL N/A 5× SSIV Buffer 4.0 µL µL 1× 10 mM dNTP mix (10 mM each) 1.0 µL µL 0.5 mM each 100 mM DTT 1.0 µL µL 5 mM Ribonuclease Inhibitor (40 U/µL) 1.0 µL µL 2.0 U/µL 50 µM Oligo d(T)20 primer, or 50 ng/μL random hexamers, or 2 µM gene-specific primer 1.0 µL 1.0 µL 1.0 µL µL 2.5 µM 2.5 ng/μL 0.1 µM Template RNA* varies µL < 5 μg total RNA or < 500 ng mRNA * 10 pg–5 µg total RNA or 10 pg–500 ng mRNA RT protocol Go to page 2 for instructions on preparing and running your RT experiment. Optimization strategies and troubleshooting Refer to the pop-ups below for guidelines to optimize and troubleshoot your RT reaction. RNA Sample Prep RT Guidelines Troubleshooting Limited Warranty, Disclaimer, and Licensing Information Package contents Catalog Number 18091050 18091200 Size 50 reactions 200 reactions Kit Contents Storage conditions Store at –20°C (non-frost-free) Required materials ∤ ∤ Template: RNA ∤ ∤ Optional: 2 μM gene-specific primers Timing ∤ ∤ Preparation time: 10 minutes ∤ ∤ Run time: 20 minutes Selection guides Go online to view related products. PCR Enzymes and Master Mixes RT Enzymes and Kits Real-Time PCR Instruments Real-Time PCR Master Mixes PCR Thermal Cyclers Product description For first strand cDNA synthesis using total RNA or poly(A)+-selected RNA primed with oligo(dT), random primers, or a gene-specific primer. Important guidelines Pre-warm the 5× SSIV Buffer to room temperature before use. Vortex and briefly centrifuge the buffer prior to preparing the reverse transcription reaction mix. Online resources Visit our product page for additional information and protocols. For support, visit www.thermofisher/support. For Research Use Only. Not for use in diagnostic procedures. Print Options
  • 2. For support, visit www.thermofisher.com/support. SuperScript™ IV First-Strand Synthesis System User Guide -2- 6 SuperScript™ IV First-Strand cDNA Synthesis Reaction The example procedure below shows appropriate volumes for a single 20-µL reverse transcription reaction. For multiple reactions, prepare a master mix of components common to all reactions to minimize pipetting error, then dispense appropriate volumes into each reaction tube prior to adding annealed template RNA and primers. Steps Procedure Procedure details 1 Anneal primer to template RNA a. Combine the following components in a PCR reaction tube. Note: Consider the volumes for all components listed in steps 1 and 2 to determine the correct amount of water required to reach your final reaction volume. Component Volume 50 µM Oligo d(T)20 primer, 50 ng/μL random hexamers, or 2 µM gene-specific reverse primer 1 µL 10 mM dNTP mix (10 mM each) 1 µL Template RNA (10 pg–5 µg total RNA or 10 pg–500 ng mRNA) up to 11 µL DEPC-treated water to 13 µL b. Mix and briefly centrifuge the components. c. Heat the RNA-primer mix at 65°C for 5 minutes, and then incubate on ice for at least 1 minute. 2 Prepare RT reaction mix a. Vortex and briefly centrifuge the 5× SSIV Buffer. b. Combine the following components in a reaction tube. Component Volume 5× SSIV Buffer 4 µL 100 mM DTT 1 µL Ribonuclease Inhibitor 1 µL SuperScript™ IV Reverse Transcriptase (200 U/μL) 1 µL c. Cap the tube, mix, and then briefly centrifuge the contents. 3 Combine annealed RNA and RT reaction mix Add RT reaction mix to the annealed RNA. 4 Incubate reactions a. If using random hexamer, incubate the combined reaction mixture at 23°C for 10 minutes, and then proceed to step b. If using oligo d(T)20 or gene-specific primer, directly proceed to step b. b. Incubate the combined reaction mixture at 50–55°C for 10 minutes. c. Inactivate the reaction by incubating it at 80°C for 10 minutes. 5 Optional: Remove RNA Note: Amplification of some PCR targets (>1 kb) may require removal of RNA. To remove RNA, add 1 µL E. coli RNase H, and incubate 37°C for 20 minutes. PCR amplification Use your RT reaction immediately for PCR amplification or store it at–20°C. Note: As a recommended starting point for PCR, reverse transcription reaction (cDNA) should compose 10% of the total reaction volume
  • 3. For support, visit www.thermofisher.com/support. SuperScript™ IV First-Strand Synthesis System User Guide -3- SuperScript™ IV Control Reactions - cDNA synthesis reaction Follow the procedure below to perform the cDNA synthesis step of the SuperScript™ IV RT-PCR control reactions. Steps Procedure Procedure details 1 Anneal primer to template RNA a. Prepare two tubes for annealing primer to template RNA. In each tube, combine the following: Component Volume 50 µM Oligo d(T)20 primer 1 µL 10 mM dNTP mix (10 mM each) 1 µL 10 ng/μL total HeLa RNA (10 ng total) 1 µL DEPC-treated water 10 µL b. Mix and briefly centrifuge the components. c. Heat the RNA-primer mix at 65°C for 5 minutes, and then incubate on ice for at least 1 minute. 2 Prepare RT reaction mix a. Vortex and briefly centrifuge the 5× SSIV Buffer. b. Prepare two reactions. In each reaction tube, combine the following: Component Volume 5× SSIV Buffer 4 µL 100 mM DTT 1 µL Ribonuclease Inhibitor 1 µL SuperScript™ IV Reverse Transcriptase (positive control) or DEPC-treated water (no RT control) 1 µL c. Cap the tube, mix, and then briefly centrifuge the contents. 3 Combine annealed RNA and RT reaction mix Add RT reaction mix to the annealed RNA. 4 Incubate reactions a. Incubate the combined reaction mixture at 50°C for 10 minutes. b. Inactivate the reaction by incubating it at 80°C for 10 minutes. 5 Remove RNA a. Add 1 µL E. coli RNase H and incubate 37°C for 20 minutes. b. Proceed to PCR amplification (page 4)
  • 4. For support, visit www.thermofisher.com/support. SuperScript™ IV First-Strand Synthesis System User Guide -4- 20 August 2015 SuperScript™ IV Control Reactions - PCR amplification Follow the procedure below to perform the PCR amplification step of the SuperScript™ IV RT-PCR control reactions. Steps Procedure Procedure details 1 Assemble PCR amplification mix a. Prepare two reactions. In each tube, combine the following: Component Volume DEPC-treated water 37.8 µL 10× High Fidelity PCR Buffer 5 μL 50 mM MgSO4 2 μL 10 mM dNTP mix (10 mM each) 1 μL Control sense primer (10 µM) (5’-GCTCGTCGTCGACAACGGCTC-3’) 1 μL Control antisense primer (10 µM) (5’-CAAACATGATCTGGGTCATCTTCTC-3’) 1 μL cDNA from positive control reaction (step 5, page 3) or DEPC-treated water for no RT control 2 μL Platinum™ Taq DNA Polymerase High Fidelity (5 U/µL) 0.2 μL b. Mix gently by pipetting up and down and briefly centrifuge the components. 2 Incubate reactions in a thermal cycler a. Place reaction mixture in preheated (94°C) thermal cycler. b. Perform PCR amplification using the following cycling parameters: Step Temperature Time Initial denaturation 94°C 2 minutes 35 PCR cycles Denature 94°C 15 seconds Anneal 55°C 30 seconds Extend 68°C 1 minute Hold 4°C hold 3 Analyze with gel electrophoresis Analyze 10 µL of each reaction using agarose gel electrophoresis and ethidium bromide staining. A 353-bp band should be visible for the positive control reaction with RT. For the no RT control reaction, the same band should be ≤ 50% in intensity when compared to the positive control.