Cloning and expression and immunogenicity of Helicobacter pylori BabA2 gene

Figure 1 BabA₂ DNA fragment amplified by PCR from Helicobacter pylori electrophoresed on 8 g/L agarose gel. Lane 1: Nucleotide marker; Lane 2: PCR products.

Figure 2 Identification of recombinant plasmid by restriction enzyme digestion. Lane 1: Nucleotide marker; Lane 2: PCR products; Lane 3: Recombinant plasmid/Not I; Lane 4: Recombinant plasmid/Not I and Nco I; Lane5: pET22b (+)/Not I.

Figure 3 The 100 g/L SDS-PAGE analysis of fusion protein expressed in BL21 (DE3). Lane 1: Molecular mass marker (67, 94) × 10³; Lane 2: control strain BL21 (pET) before induction; Lane 3: control strain BL21 (pET) after 5-h induction with IPTG; Lane 4: BL21 (pET-BabA) cells before induction; Lane 5: BL21 (pET- BabA) cells after 3-h induction with IPTG; Lane 6: BL21 (pET- BabA) cells after 5-h induction with IPTG; Lane 7: BL21 (pET- BabA) cells periplasm protein after 3-h induction with IPTG; Lane 8: sonicated supernatant of BL21 (pET-BabA) cells after 3-h induction with IPTG; Lane 9: recombinant protein BabA purified.