在线翻译

Large-scale analyses of insertion sites have been per-formed by high-throughput modification of GW strategies. By means of the thermal asymmetric inter-laced PCR (TAIL-PCR) and suppression PCR GW methods more than 42 000 insertion sites of the Tos17 retro-transposon in the rice genome were analyzed [107]. An automated TAIL-PCR approach was developed [96] for analysis of the collection of insertional mutants of Ac⁄ Dsand Ac transposons in two cultivars of rice. The DLA GW strategy associated with pyrosequencing allowed the identification of about 965 000 sequences flanking the highly active maize mutator ( Mu) transpo-son [60]. These analyses allowed the development of specific insertional mutant databases. In the case of Arabidopsis thaliana the ATIDB database (http://atid-b.or g) was e s tablished [ 110], which also contains information for T-DNA mutants. For rice 更多：https://www.bmcx.com/ , the OryGenesDB database (http://orygenesdb.cirad.fr/) was developed[111].