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. 2012 May;20(3):320-5.
doi: 10.4062/biomolther.2012.20.3.320.

Expression of recombinant rotavirus proteins harboring antigenic epitopes of the hepatitis a virus polyprotein in insect cells

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Expression of recombinant rotavirus proteins harboring antigenic epitopes of the hepatitis a virus polyprotein in insect cells

Van Thai Than et al. Biomol Ther (Seoul). 2012 May.

Abstract

Rotavirus and hepatitis A virus (HAV) spread by the fecal-oral route and infections are important in public health, especially in developing countries. Here, two antigenic epitopes of the HAV polyprotein, domain 2 (D2) and domain 3 (D3), were recombined with rotavirus VP7, generating D2/VP7 and D3/VP7, cloned in a baculovirus expression system, and expressed in Spodoptera frugiperda 9 (Sf9) insect cells. All were highly expressed, with peak expression 2 days post-infection. Western blotting and ELISA revealed that two chimeric proteins were antigenic, but only D2/VP7 was immunogenic and elicited neutralizing antibody responses against rotavirus and HAV by neutralization assay, implicating D2/VP7 as a multivalent subunit-vaccine Candidate for preventing both rotavirus and HAV infections.

Keywords: Hepatitis A virus; Recombinant chimera protein; Rotavirus.

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Figures

Fig. 1.
Fig. 1.. (A) Schematic representation of the two recombinant rotavirus proteins carrying antigenic epitopes of the HAV polyprotein. Recombinant gene cassettes were recombined in frame with a short peptide linker of Leu-Glu-Pro-Gly (LEPG). DNA regions of the vector plasmid are indicated by the filled circles (Օ ). (B) Expression of two recombinant rotavirus proteins using a baculovirus expression system in Sf9 cells. Whole cell lysates of infected Sf9 cells with individual recombinant baculoviruses were resolved by 10% SDS-PAGE. (C) Western blot analysis was performed using anti-V5 antibody and HRP-conjugated goat ani-mouse antibody.
Fig. 2.
Fig. 2.. Kinetics of recombinant baculovirus production of D2/VP7. Cells were harvested every 24 hrs during the experimental period of 10 days after the initial viral infection. Aliquots of infected Sf9 cells were clarified by low-speed centrifugation, lysed with RIPA buffer, and analyzed by Western blot. Lanes 1-10: Cells from 1 to 10 days post-infection.
Fig. 3.
Fig. 3.. Western blot analyses using anti-sera from either (A) rotavirus-infected rabbits or (B) HAV-infected human patients. The Western XP marker (Invitrogen, USA) is shown at the left. Numbers (21, 22 and 23) are patient serum numbers.
Fig. 4.
Fig. 4.. Production of the rotavirus-specific antibodies after experimental immunization of D2/VP7 against rabbits. Rabbit serum antibody response to rotavirus Wa strain was examined using ELISA. Rabbit serum antibody response to rotavirus Wa strain (A) and hepatitis a HM175 strain (B) was examined using ELISA (see Materials and Methods). The sera were serially diluted from 1:10 to 1:640 and analyzed at 492 nm. Negative rabbit serum (♦); Immunized rabbit serum (■); Rabbit serum against rotavirus Wa or goat anti HAV HM175 (▲). OD values are indicated at the right.

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