The last mutant rYJ-CL-1-59 contained a single amino acid mutatio

The last mutant rYJ-CL-1-59 contained a single amino acid mutation of arginine for alanine at position 59 (R59A) in the capsid protein of PCV2b/YJ. The IPMA reactivity between each antibody and PK-15 cells transfected with each PCV2 construct is indicated next to each construct. The IPMA reactivity

of the constructs in transfected PK-15 cells was demonstrated by PCV2-positive serum and mAb 8E4. +: Positive; -: Negative. In vitro transfection Plasmids were excised by SalI digestion to produce SalI fragments that contained the complete genomic sequence. The purified SalI fragments were self-ligated for 30 min at 16°C, using T4 DNA ligase (Takara, Dalian, China), and subsequently transfected into PK-15 cells (80-90% confluency) in each well of a 24-well plate, using Lipofectamine 2000 (Invitrogen) according to the manufacturer’s selleck products mTOR inhibitor instructions. Mock-transfected PK-15 cells were regarded as the negative control. After incubation for 6 h at 37°C, 400 μl RPMI 1640 containing 10% FBS was added to each well and incubated at 37°C with 5% CO2. At 48 h post transfection, the cells were tested in the IPMA with PCV2-positive serum and mAb 8E4. Results Generation

and characterization of mAb against PCV2 capsid protein One stable hybridoma secreting PCV2 mAb was generated and designated as 8E4. The isotype of the mAb was identified with the Mouse MonoAb-ID Kit (HRP). It was determined that the isotype and light chain of 8E4 was IgG2a and λ type, respectively. The reactivity of mAb 8E4 with PCV2a/LG strain purified by ultracentrifugation was determined by western blot analysis (Figure 2). MAb 6F10 (positive control) gave a strong and specific reaction with the 28-kDa capsid protein of PCV2. However, mAb 8E4 did not give a positive www.selleck.co.jp/products/Rapamycin.html reaction. No reaction was observed with the culture supernatant of SP2/0 cells, used as a negative control. Figure 2 Analysis of immunoreactivity of mAb by western

blot analysis. Purified virions of the PCV2a/LG strain were separated by SDS-PAGE, transferred to nitrocellulose membranes, and incubated with mAb. Lane M: protein molecular weight markers; lane 1: mAb 8E4; lane 2: mAb 6F10 as a positive control; lane 3: SP2/0 supernatant as a negative control. Reactivity of mAb 8E4 with different PCV2 strains The IPMA was used to examine the reactivity of mAb 8E4 with six different PCV2 strains and recPCV1/G. The PCV2-positive serum stained all the PCV2 strains (Figure 3a, odd numbers), whereas the PCV1-positive serum stained the recPCV1/G antigen. MAb 8E4 stained PCV2a/LG, PCV2a/CL and PCV2a/JF2 antigens, and did not stain PCV2b/SH, PCV2b/YJ, PCV2b/JF antigens (Figure 3a, even numbers) or the recPCV1/G antigen. Figure 3 Reactivity of six PCV2 isolates with mAb 8E4 by the IPMA, serum neutralization assay and capture ELISA.

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