Design of endonuclease restriction sites into primers for PCR cloning
نویسنده
چکیده
I present a software system PCRCLNG that facilitates the design of endonuclease restriction sites into the 5'-end of PCR primers. The product amplified using these primers can be directly cloned into vectors. The program estimates the annealing temperature for each primer and selects the primer pairs with comparable annealing temperature. Finally the software determines whether the PCR product can be cloned into the vector to generate in-frame gene fusion.
منابع مشابه
Efficient cloning of PCR generated DNA containing terminal restriction endonuclease recognition sites.
DNA generated by the polymerase chain reaction (PCR) (1) containing terminal restriction endonuclease recognition sites to permit cloning usually relies on the use of unphosphorylated primers incorporating a restriction endonuclease recognition site of choice plus 3 —4 extra 5' bases flanking that site. Various sites (Notl, Xhol and Xbal (2), for example) incorporated into the termini of PCR pr...
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ورودعنوان ژورنال:
- Bioinformatics
دوره 18 12 شماره
صفحات -
تاریخ انتشار 2002