<p>It has been previously disclosed that DNA segments can be made in massively parallel chemical synthesis operations on a common substrate followed by release of the segments from the substrate and assembly of the segments into target DNA molecules. Here it is taught that if the DNA primary constructs are sufficiently long and properly designed, that the copy numbers of the primary constructs can be multiplied as needed by a PCR process using as a template regions at the ends of the primary constructs. The end regions, called flanking regions, can also be designed so that they may be cleaved easily from the amplification products. The target double-stranded DNA can then be assembled from the cleaved fragments. Hundreds of thousands of oligonucleotides can be synthesized and assembled into many different individual genes by this process in a relatively quick and efficient process.</p>
申请公布号
EP1759019(B1)
申请公布日期
2010.07.21
申请号
EP20050785221
申请日期
2005.06.08
申请人
WISCONSIN ALUMNI RESEARCH FOUNDATION
发明人
SUSSMAN, MICHAEL, R.;RICHMOND, KATHRYN, E.;RODESCH, MATT, J.
