Standard cDNA libraries
Service Procedure
Step 1: Selection of RNA and vector
- Provide us with cells, tissue or RNA. If you wish to use commercially available RNA as a source for your library, please indicate this to us and we will purchase the RNA for you.
- Choose the appropriate library vector
Step 2: Library construction
- If you provide tissue or cells, we will isolate total or polyA+ RNA from it (please see guidelines).
- We perform a stringent quality control on the RNA using Experion lab-on-chip equipment
- 1st strand cDNA is generated by reverse transcription
- The 1st strand cDNA is size-selected and split into two size pools to optimize representation of big and small fragments
- 2nd strand cDNA is generated separately on both size pools
- The two size pools are quality checked using Experion lab-on-chip equipment
- The two size pools are separately ligated into the library vector
Step 3: Quality control
- A test amplification is carried out two optimize amplification parameters
- Quality control is performed. Only cDNA libraries which pass the following criteria are amplified:
- Greater than 2x106 independent clones
- More than 85% plasmids containing inserts
- Average insert size at least 1.3 kb
Step 4: Amplification
- The final library is amplified in E. coli
- Primary stocks are generated
- Plasmid DNA is isolated
Step 5: Delivery of the following reagents and data
- Library quality control sheet
- At least 500 µg of purified library plasmid - ready to screen!
- Primary glycerol stocks for later amplification of the library
Ordering information
S03 | Custom cDNA library construction |
