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[Construction of cDNA library of Magnaporthe grisea with magnetic bead].

作者信息

Feng Xu, Xiaoli Wu, Dewen Qiu

机构信息

College of Life Science, Yangtze University, Jingzhou 434025, China.

出版信息

Wei Sheng Wu Xue Bao. 2008 Jun;48(6):806-10.

PMID:18720847
Abstract

OBJECTIVE

We constructed cDNA library of Magnaporthe grisea. The good quality cDNA library could facilitate finding proteinaceous elicitors of M. grisea, and elucidating the mechanisms of the M. grisea--rice interaction.

METHODS

The Oligo(dT) combined with the magnetic bead was used to extract mRNA from total RNA of Magnaporthe grisea and as primers to synthesize the first-strand cDNA. Terminal transferase introduced PolyA into 3'terminal of the first cDNA strand, then the PolyA was used for amplifying the second-strand cDNA. Restriction enzyme and adapter were avoided in this research, which could solve technical limitation of the traditional method. Because all reactions were done in one centrifuge tube, this process could reduce the risk of cDNA loss and cross-contamination. The primers designed in this research could clone the amplified cDNAs into expression vector in a desirable orientation.

RESULTS

The cDNA library constructed had a high titer of 8.9 x 10(6) cfu/mL, and contained a total clones of 8.9 x 10(7) cfu, with an average inserts size of about 1380 bp.

CONCLUSION

Constructing cDNA library with magnetic bead was a highly efficient method using only small amount of experimental materials within a short period.

摘要

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