Difference between revisions of "5' RACE"

Revision as of 14:49, 4 December 2012

5' RACE Kit (Version 2.0 from Invitrogen; http://products.invitrogen.com/ivgn/product/18374058)
Double distilled water
Absolute ethanol
Total RNA, 1-5 ug
Gene Specific Primers (see Designing Primers for 5' RACE )

Copied from the manufacturer's protcol here

Resuspend gene specific primers to 1 uM
Prepare and chill wash buffer by adding 18 mL water, 21 mL ethanol and 1 mL wash buffer concentrate into a glass bottle. Place at 4C
Prepare and chill 70% ethanol by adding 35 mL ethanol to 15 mL water in a glass bottle. Place at 4C
Place binding solution at room temperature.
Warm some sterile water to 65C

Incubate at 70C for 10 min to denature RNA using the PCR Program 5' RACE 70C
Place on ice for 1 min
Add the following in order:

Incubate 1 min at 42C using the PCR program 5' RACE First Strand, which covers the next three steps
Add 1 uL SuperScript II RT
Incubate 50 min at 42C
Incubate 15min at 70C
Remove and add 1uL RNAse H, mix thoroughly
Incubate 30min at 37c using the PCR Program 5' RACE RNAse H. Can freeze at -20 or continue to cDNA Purification

Add 120 uL binding solution to the first strand reaction.
Transfer reaction to a SNAP column provided.
Spin at 13K for 20s.
Remove the cartridge and transfer flow through to a new microcentrifuge tube. Save until cDNA recovery is confirmed.
Add 400 uL cold wash buffer to the spin cartridge, replaced in microcentrifuge tube.
Spin at 13K for 20s.
Repeat wash three more times.
Wash the cartridge twice with 400 uL cold 70C
After second wash, centrifuge 1 min at 13K to removed residual ethanol.
Transfer cartridge into a clean recovery tube. Add 50 uL of preheated water.
Spin at 13K for 20s.

To a new tube add the following:
1. 6.5uL DEPC Treated water.
2. 5uL 5X tailing buffer.
3. 2.5uL 2mM dCTP.
4. 10 uL Purified cDNA.
Incubate at 94C for 2-3 min. This and the next two steps are in the PCR program 5' RACE TdT.
Add 1 uL TdT, mix and incubate 10 min at 37C.
Heat inactivate at 65C for 10min.

@@ Line 15: / Line 15: @@
 * Prepare and chill wash buffer by adding 18 mL water, 21 mL ethanol and 1 mL wash buffer concentrate into a glass bottle.  Place at 4C
 * Prepare and chill 70% ethanol by adding 35 mL ethanol to 15 mL water in a glass bottle.  Place at 4C
+* Place binding solution at room temperature.
+* Warm some sterile water to 65C
 ===First Strand Synthesis===
@@ Line 47: / Line 49: @@
 ===cDNA Purification===
+# Add 120 uL binding solution to the first strand reaction.
+# Transfer reaction to a SNAP column provided.
+# Spin at 13K for 20s.
+# Remove the cartridge and transfer flow through to a new microcentrifuge tube.  Save until cDNA recovery is confirmed.
+# Add 400 uL cold wash buffer to the spin cartridge, replaced in microcentrifuge tube.
+# Spin at 13K for 20s.
+# Repeat wash '''three''' more times.
+# Wash the cartridge twice with 400 uL cold 70C
+# After second wash, centrifuge 1 min at 13K to removed residual ethanol.
+# Transfer cartridge into a clean recovery tube.  Add 50 uL of preheated water.
+# Spin at 13K for 20s.
+===TdT Tailing of cDNA===
+# To a new tube add the following:
+## 6.5uL DEPC Treated water.
+## 5uL 5X tailing buffer.
+## 2.5uL 2mM dCTP.
+## 10 uL Purified cDNA.
+# Incubate at 94C for 2-3 min.  This and the next two steps are in the PCR program '''5' RACE TdT'''.
+# Add 1 uL TdT, mix and incubate 10 min at 37C.
+# Heat inactivate at 65C for 10min.