mircute mirna qpcr Detection Kit (SYBR Green)



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mircute mirna qpcr Detection Kit (SYBR Green) For detection of mirna using real-time RT-PCR (SYBR Green I) www.tiangen.com

QP110302 mircute mirna qpcr Detection Kit (SYBR Green) Kit Contents Cat. no. FP401 Kit Contents FP401 50 μl 50 rxns 2 mircute mirna Premix (with SYBR and ROX) 1.35 ml Reverse Primer (10 μm) 55 μl 50 ROX Reference Dye 250 μl Handbook 1 Storage mircute mirna qpcr Detection Kit should be shipped in dry ice and stored immediately upon receipt at -20 in dark condition. Once used, 2 mircute mirna Premix (with SYBR and ROX) can be stored at 4 for 6 months in dark condition. Reverse Primer (10 µm) should be still stored at -20. Introduction mircute mirna qpcr Detection Kit is designed for mirna real-time PCR by using SYBR Green I. The kit is composed of 2 mircute mirna Premix, 50 ROX Reference Dye and Reverse Primer (10 µm). 2 mircute mirna premix (with SYBR and ROX) was developed specifically for quantitative detection of mirna. The DNA polymerase in this kit is the antibody modified hot-start DNA polymerase, which ensures high specificity, sensitivity and accurate quantitative detection in a wide range combined with the unique buffer. Note: The kit has to be used with mircute mirna First-Strand cdna Synthesis Kit (Cat. no. KR 201) mircute mirna qpcr Detection Kit Handbook 1

Important Notes 1. The kit contains SYBR Green I. Store and prepares PCR reaction in dark condition. 2. Pipet the reaction solution and aliquot with sterile tips and consumable items to avoid contamination. Reagents and Materials Not Supplied 1. RNase-free ddh 2 O 2. Forward primer Design Principles of Forward Prime 1. Follow the most common design principles of primers. 2. Based on mature mirna sequence, change U to T to design forward prime. 3. Tm value of Reverse Primer (10 µm) in the kit is about 65. Ensure that Tm value of forward prime is basically consistent with supplied Reverse Primer (10 µm). 4. If Tm value of the designed forward prime is too low according to principle 2, it is recommended to add several nucleotides (G or C is optional) to 5 -terminal, or add one or several adenines to 3 -terminal. Optionally, modify both 5 terminal and 3 terminal at the same time. 5. If Tm value of the designed forward prime is too high according to principle 2, remove several nucleotides from 5 or 3 terminal. Protocol 1. Thaw 2 mircute mirna Premix and Reverse Primer (10 µm) at room temperature. mircute mirna qpcr Detection Kit Handbook 2

2. Mix the 2 mircute mirna Premix thoroughly by inverting gently. Avoid bubbling in the process and centrifuge gently before use. Note: The performance will decrease unless the reagents are mixed thoroughly. Do not vortex by shaker. 3. Place all the reagents on ice, and prepare the reaction Table A according to Table A. Note: If using PRISM 7000/7300/7700/7900HT, Step one/ Step one plus PCR system from ABI, prepare the reaction according to Table B. Components 2 mircute mirna Premix (with SYBR and ROX) Forward Prime (not supplied) (50 µl) (20 µl) Final Conc. 25 µl 10 µl 1 - - 200 nm Reverse Primer (10 µm) 1 µl 0.4 µl 200 nm mirna first-strand cdna - - - ddh 2 O Up to 50 µl Up to 20 µl Note: Ensure addition of mirna first-strand cdna is less than 1/10 volume of real-time PCR reaction. Dilute the cdna according to actual concentration (Dilution ratio may be 1/10 or 1/100) since high concentration of cdna will lead to non-specific amplification. mircute mirna qpcr Detection Kit Handbook 3

Table B Components 2 mircute mirna Premix (with SYBR and ROX) Forward Prime (not supplied) (50 µl) (20 µl) Final Conc. 25 µl 10 µl 1 - - 200 nm Reverse Primer (10 µm) 1 µl 0.4 µl 200 nm mirna first-strand cdna - - - 50 ROX Reference Dye 4 µl 1.6 µl 5 ddh 2 O Up to 50 µl Up to 20 µl - Note: Ensure addition of mirna first-strand cdna is less than 1/10 volume of real-time PCR reaction. Dilute the cdna according to actual concentration (Dilution ratio may be 1/10 or 1/100) since high concentration of cdna will lead to non-specific amplification. Compatible Real-time Instruments PRISM 7000/7300/7500/7700/7900HT Real-Time PCR System, Step one/ Step one plus PCR System (Applied Biosystems) LightCycler (Rocle) Mx3000P, Mx3005P and Mx 4000 (Stratagene) Mastercycler ep realplex (Eppendorf) Line-Gene (Bioer) Other Real-time instruments Set up the real-time PCR program according to the procedure outlined in the following table. 2 mircute mirna premix (with SYBR and ROX) contains antibody modified DNA polymerase. The DNA polymerase is activated in a mircute mirna qpcr Detection Kit Handbook 4

shorter time than other hot-start Taq DNA polymerases. This shorts the reaction time of real-time PCR significantly. Cycle numbers Temperature Time Comments 1 94 2 min Initial PCR denaturation 40-45 94 20 sec Denaturation 60 34 sec Annealing and extension Ordering Information Reverse Transcription Product Size Cat.no. mircute mirna First-Strand cdna Synthesis Kit 25 rxns 50 rxns KR201-01 KR201-02 mircute mirna qpcr Detection Kit Handbook 5