Baculoviruses are arthropodian pathogens, infecting lepidoptera, hymenoptera, diptera, and decapoda hosts. Baculovirus infects most commonly in the larvae of moths. In 1983, baculovirus was first used to express exogenous proteins. From then on, this technique has been widely used in vaccination, drug discovery and recombinant protein production. Increasing protein yields of baculovirus expression vector system (BEVS) has long been an important goal. Previously, our laboratory have used the mutagen, BrdU, to induce random mutation to the vABhcmEpL baculovirus, and identified a clone C4 virus with a delayed cell lysis phenotype after infecting Sf21 insect cell. C4 virus also expresses higher levels of EGFP than does parental virus vABhcmEpL. The purpose of my experiment is to characterize the C4 virus, focusing on protein expression and virus production. According to current experimental results, I found that C4 could express EGFP for longer time and produce higher virus titer than vABhcmEpL in the eight-day time course experiment. In addition, I utilized NGS to analysis genome of C4 in order to find out the responsive gene(s) to these phenotypes. The NGS result showed that there are 73 mutants different from vABhcmEpL. Comparing the results with cosmid transfection tests done by previous study, I discovered that mutant ORF52 may be responsible for the delay cell lysis phenotype of C4 virus. Therefore, I constructed recombinant baculoviruses based on ORF52 of wild type and compared the phenotype with C4. The result show that vC4-ORF52 induced cell lysis earlier than vC4. Therefore, the mutant ORF52 of vC4 is proved to be the gene results in the phenotype of delayed cell lysis. On the other hand, I also took advantage of C4 to better express the hemagglutinin of influenza virus. The results showed that C4 is not only resulted delayed cell lysis but also produced more virus particles and engineered HA protein than the BEVS derived from commercial vector system of BaculoGold.