en تخصصي Special پژوهشي Original article <div style="border-bottom:solid windowtext 1.0pt; border-top:solid windowtext 1.0pt; border-left:none; border-right:none; padding:1.0pt 0in 1.0pt 0in"><span style="font-size:12pt"><span style="unicode-bidi:embed"><span new="" roman="" style="font-family:" times=""><b><span style="font-size:11.0pt">Background and Aims: </span></b><span style="font-size:10.5pt">Selecting appropriate antigens, suitable delivery vehicles and proper immune adjuvants are important items in vaccine designing. According to the previous studies, Carcinoembryonic </span><span style="font-size:11.0pt">antigen (CEA) and Adenoviral vector are considered as proper antigen and reliable delivery vehicle for cancer vaccines, respectively. Directing antigens to DCs with antibody single-chain fragment variable (scFv) against to DEC-205 (scDEC) can play the role of adjuvant. The aim of this study was to produce a construct encoding CEA targeted to DCs by scDEC in Adenovirus vector platform.</span></span></span></span><br> <span style="font-size:12pt"><span style="unicode-bidi:embed"><span new="" roman="" style="font-family:" times=""><b><span style="font-size:11.0pt">Materials and Methods: </span></b><span style="font-size:11.0pt">scDEC were cloned into p-track-CEA-GFP. Linearized p-track-scDEC-CEA-GFP and pAdenoVator ∆E1/E3 were co-transformed into BJ5183 cells. Resulting pAd scDEC-CEA-GFP was transfected into HEK293 cells to produce Adenoviruses (Ad scDEC-CEA-GFP). The presence of scDEC-CEA gene in the recombinant virus and expression of CEA protein was detected by PCR and electrochemiluminescence tests, respectively. Flow cytometry tests were used to confirm the attachment of scDEC-CEA protein to DCs. Adenovirus infectivity in cells other than HEK293 was confirmed by transduction of Ad scDEC-CEA-GFP into L929 cells.</span></span></span></span><br> <span style="font-size:12pt"><span style="unicode-bidi:embed"><span new="" roman="" style="font-family:" times=""><b><span style="font-size:11.0pt">Results:</span></b><span style="font-size:11.0pt"> PCR test showed the presence of scDEC-CEA gene in adenovirus genome. Electrochemilu-minescence and flow cytometry analysis confirmed expression of CEA protein and attachment of scDEC-CEA protein to DCs, respectively. GFP expression in L929 cells indicated Ad scDEC-CEA-GFP could effectively infect cells other than HEK293.</span></span></span></span><br> <span style="font-size:12pt"><span style="unicode-bidi:embed"><span new="" roman="" style="font-family:" times=""><b><span style="font-size:11.0pt">Conclusion: </span></b><span style="font-size:11.0pt">As construction of a suitable construct for immunotherapy is a major goal of many research groups, the Ad scDEC-CEA-GFP engineered in this study, which properly targets DCs, can be applied in future in vivo cancer immunotherapy investigations in mice.</span><span style="font-size:11.0pt"></span></span></span></span></div> Cancer immunotherapy, CEA, DEC205, Adenoviral vector 15 22 http://journal.isv.org.ir/browse.php?a_code=A-10-318-1&slc_lang=en&sid=1 Nazila Hajiahmadi n.hajiahmadi@modares.ac.ir 10031947532846007530 10031947532846007530 No Department of Virology, Faculty of Medical Sciences, Tarbiat Modares University, Tehran, Iran. Seyed Mohammad Moazzeni moazzeni@modares.com 10031947532846007531 10031947532846007531 No Department of Immonulogy, Faculty of Medical Sciences, Tarbiat Modares University, Tehran, Iran. Taravat Bamdad Bamdad_t@modares.ac.ir 10031947532846007532 10031947532846007532 Yes Department of Virology, Faculty of Medical Sciences, Tarbiat Modares University, Tehran, Iran.