Maternally-derived neutralizing antibodies reduce vaccine efficacy against porcine reproductive and respiratory syndrome virus infection

被引:21
|
作者
Renson, Patricia [1 ,4 ,5 ]
Fablet, Christelle [2 ,5 ]
Andraud, Mathieu [2 ,5 ]
Normand, Valerie [6 ]
Lebret, Arnaud [6 ]
Paboeuf, Frederic [3 ,5 ]
Rose, Nicolas [2 ,5 ]
Bourry, Olivier [1 ,5 ]
机构
[1] Agence Natl Securite Sanitaire Alimentat Environm, Unite Virol Immunol Porcines, BP 53, F-22440 Ploufragan, France
[2] Anses, Unite Epidemiol, BP 53, F-22440 Ploufragan, France
[3] Anses, Serv Prod Pores Assainis & Expt, BP 53, F-22440 Ploufragan, France
[4] UGPVB, 104 Rue Eugene Pottier, F-35065 Rennes, France
[5] Univ Bretagne Loire, 1 Pl Paul Ricoeur,CS 54417, F-35044 Rennes, France
[6] ZA Goheleve, Grp Vet Chene Vert Conseil, Porc Spect, F-56920 Noyal Pontivy, France
关键词
PRRS virus; Modified live virus vaccine; Maternally derived antibody; Neutralizing antibody; IFNa; Interference; MODIFIED-LIVE VACCINE; IMMUNE-RESPONSES; FARM; TRANSMISSION; PERFORMANCE; PROTECTION; PIGLETS; DISEASE; INNATE; STRAIN;
D O I
10.1016/j.vaccine.2019.06.045
中图分类号
R392 [医学免疫学]; Q939.91 [免疫学];
学科分类号
100102 ;
摘要
Modified live virus (MLV) vaccines are commonly used to reduce the impact of porcine reproductive and respiratory syndrome (PRRS) but limited efficacy is achieved in field conditions. Here, we evaluated the impact of maternally-derived neutralizing antibodies (MDNAs) on vaccine efficacy after PRRS virus (PRRSV) challenge. Piglets with low (A-) or high (A+) MDNA levels derived from a commercial pig herd were moved to experimental facilities to be vaccinated (V+) or not (V-) with a PRRSV-1 MLV vaccine at 3 weeks of age (woa). Because of unexpectedly low vaccine detection in A-V+ piglets post-vaccination (pv), all V+ piglets received a second vaccination at 4 woa. Five weeks (W5) pv, piglets were inoculated with a PRRSV-1 field strain to evaluate vaccine protection, and were mingled 24 h later with non-inoculated piglets of similar immune status to assess viral transmission. Vaccine strain was detected at W2 pv in 69% and 6% of A-V+ and A+V+ piglets, and at W5 pv in 50% and 25% of A-V+ and A+V+ piglets, respectively. At W5 pv, 94% of A-V+ and 44% of A+V+ piglets seroconverted, with a significant IFNg response induction in the A-V+ group only. After challenge, compared to the V- inoculated group, viremia was 100-fold lower at 10 days post-infection in A-V+ whereas viremia was not significantly reduced in A+V+ piglets. A lower transmission rate was estimated for the A-V+ group: 0.15 [0.07-0.29] versus 0.44 [0.18-1.76] and 0.32 [0.14-0.68] for the A+V+ and V- groups, respectively. Investigations about the low vaccine strain detection after the first vaccination suggested a relationship between IFNa levels and vaccine strain detection in A-V+ piglets. We showed that MDNAs impair vaccine efficacy against PRRSV both in inoculated and contact piglets, probably by reducing vaccine replication. IFNa may also interfere with PRRSV vaccination. These new data could help improving vaccination protocols. (C) 2019 Elsevier Ltd. All rights reserved.
引用
收藏
页码:4318 / 4324
页数:7
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