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A IMPROVED SMART METHOD TO CONSTRUCTION FULL-LENGTH cDNA LIBRARY FOR LARGE CLONES

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ã€Authorã€‘ Dong Zhimin~(1,2) Li Yinghui~2 Zhang Baoshi~1 Guan Rongxia~2 Chang Ruzhen~2 Qiu Lijuan~2(1.College of Agronomy,Shenyang Agricultural University,Shenyang 110161;2.National Key Facility of Crop Gene Resources and Genetic Improvement,Key Laboratory of Crop Germplasm & Biotechnology(MOA)/ Institute of CropSciences,Chinese Academy of Agricultural Sciences,Beijing 100081)

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ã€Abstractã€‘ It is difficult to obtain large clones among the SMART library due to PCR amplification impairing the proportion of large clones.According to this,SMART method was improved based on the primary SMART method.The soybean leaves cDNAs were separated into three parts based on the size distribution of amplified dscDNA by agarose gel size fractionation.Each of three parts was ligated respectively to vector and transformed to Ecoli.The sub-library contain about 1.0Ã—10~6 clones.The recombination ratio was nearly 99% and full-length ratio was 53.6% which was correspondence with that of primary SMART library.The inserts size ranged between 0.5kb to 3.5kb and the size of largest inserts was about 1.5kb larger than that of primary SMART method.The improved SMART method increased obviously the large clone proportion among the library which was in favor of soybean fuctional genomics research.æ›´å¤š è¿˜åŽŸ