Abstract
Human papillomaviruses (HPVs) are responsible for about 25% of cancer cases worldwide. HPV-16 E7 antigen is a tumor-associated antigen (TAA) commonly expressed in HPV-induced tumors; however, it has low immunogenicity. The interaction of 4-1BBL with its receptor induces pleiotropic effects on innate, adaptive, and regulatory immunity and, if fused to TAAs in DNA vaccines, can improve the antitumor response; however, there is low transfection and antitumor efficiency. Oncolytic virotherapy is promising for antitumor gene therapy as it can be selectively replicated in tumor cells, inducing cell lysis, and furthermore, tumor cell debris can be taken in by immune cells to potentiate antitumor responses. In this study, we expressed the immunomodulatory molecule SA-4-1BBL fused to E7 on an oncolytic adenovirus (OAd) system. In vitro infection of TC-1 tumor cells and NIH-3T3 non-tumor cells with SA/E7/4-1BBL OAd demonstrated that only tumor cells are selectively destroyed. Moreover, protein expression is targeted to the endoplasmic reticulum in both cell lines when a signal peptide (SP) is added. Finally, in an HPV-induced cancer murine model, the therapeutic oncolytic activity of OAd can be detected, and this can be improved when fused to E7 and SP.
Highlights
Introduction iationsCancer ranks among the leading causes of mortality with approximately 8 million deaths worldwide registered in 2015 [1], predominately in low and medium socioeconomic countries
It has been reported that some mouse cells are semi-permissive to OAd infection; can lyse tuToincrease prove that oncolytic adenovirus (OAd) expressing can lyse mor cells, we proposed infecting the tumor cell lineSP/SA/E7/4-1BBL
After we showed that OAd is capable of infecting NIH/3T3 non-tumor cells and expressing the signal peptide (SP)/SA/E7/4-1BBL protein, we evaluated whether cell viability was affected
Summary
The oncolytic adenovirus (OAd) used in this study was synthesized by O.D.260 Inc. (Boise, ID, USA). The oncolytic adenovirus (OAd) used in this study was synthesized by O.D.260. This OAd has a 24-bp deletion in the E1A conserved region 2 (CR2), a 1222-bp-long BglII-MfeI deletion in the E3 region, in which the E3 ADP, RIDα, RIDβ, and 14.7K genes are preserved, a hybrid Ad5/3 fiber, and a CMV-(SP)-SA-E7-4-1BBL-SV40. PA expression cassette inserted between the fiber gene and the E4 region
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