Hi, I'm trying to transform E. coli DH10Bac cells with a pFB-Lic-Bse vector containing my gene of interest. 48 h after transformation, I get some white colony on LB-Km-Tet-Gent-Xgal-IPTG, but when I do the PCR using the M13 for and rev primers I obtain only the band relative to the bacmid alone. My recombinant plasmid (insert+pFB-Lic-Bse) is more than 10,000 bp in length. Is it possible that the recombinant plasmid is too large to enter the DH10BAc cells? If this is the case, what would you suggest? Do I have to prolong the transformation or use more DNA?
Thank you everyone!