Abstract
The construction of full-length cDNA libraries allows researchers to study gene expression and protein interactions and undertake gene discovery. Recent improvements allow the construction of high-quality cDNA libraries, with small amounts of mRNA. In parallel, these improvements allow for the incorporation of adapters into the cDNA, both at the 5′ and 3′ end of the cDNA. The 3′ adapter is attached to the oligo-dT primer that is used by the reverse transcriptase, whereas the 5′ adapter is incorporated by the template switching properties of the MMLV reverse transcriptase. This allows directional cloning and eliminates inefficient steps like adapter ligation, phosphorylation, and methylation. Another important step in the construction of high-quality cDNA libraries is the normalization. The difference in the levels of expression between genes might be several orders of magnitude. Therefore, it is essential that the cDNA library is normalized. With a recently discovered enzyme, duplex-specific nuclease, it is possible to normalize the cDNA library, based on the fact that more abundant molecules are more likely to reanneal after denaturation compared to rare molecules.
This is a preview of subscription content, log in via an institution to check access.
Access this chapter
Tax calculation will be finalised at checkout
Purchases are for personal use only
References
Carninci P, Kvam C, Kitamura A et al (1996) High-efficiency full-length cDNA cloning by biotinylated CAP trapper. Genomics 37:327–336
Zhu YY, Machleder EM, Chenchik A et al (2001) Reverse transcriptase template switching: a SMART approach for full-length cDNA library construction. Biotechniques 30:892–897
Young DD, Anderson M (1985) Quantitative analysis of solution hybridization. In: Hames BD, Higgins SJ (eds) Nucleic acids hybridisation: a practical approach. IRL Press, Oxford, pp 47–71
Zhulidov PA, Bogdanova EA, Shcheglov AS et al (2004) Simple cDNA normalization using kamchatka crab duplex-specific nuclease. Nucleic Acids Res 32:e37. doi:10.1093/nar/gnh031
Shagin DA, Rebrikov DV, Kozhemyako VB et al (2002) A novel method for SNP detection using a new duplex-specific nuclease from crab hepatopancreas. Genome Res 12:1935–1942
Bogdanova EA, Barsova EV, Shagina IA et al (2011) Normalization of full-length-enriched cDNA. Methods Mol Biol 729:85–98
Bogdanova EA, Shagina IA, Mudrik E et al (2009) DSN depletion is a simple method to remove selected transcripts from cDNA populations. Mol Biotechnol 41:247–253
Clontech (2009) Make your own “Mate&Plate" library system user manual. PT2085-1.
Carninci P, Nishiyama Y, Westover A et al (1998) Thermostabilization and thermoactivation of thermolabile enzymes by trehalose and its application for the synthesis of full length cDNA. Proc Natl Acad Sci U S A 95:520–524
Author information
Authors and Affiliations
Editor information
Editors and Affiliations
Rights and permissions
Copyright information
© 2014 Springer Science+Business Media New York
About this protocol
Cite this protocol
Kooiker, M., Xue, GP. (2014). cDNA Library Preparation. In: Henry, R., Furtado, A. (eds) Cereal Genomics. Methods in Molecular Biology, vol 1099. Humana Press, Totowa, NJ. https://doi.org/10.1007/978-1-62703-715-0_5
Download citation
DOI: https://doi.org/10.1007/978-1-62703-715-0_5
Published:
Publisher Name: Humana Press, Totowa, NJ
Print ISBN: 978-1-62703-714-3
Online ISBN: 978-1-62703-715-0
eBook Packages: Springer Protocols