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Surveillance and disease control
 approaches for pigs and their
       application to ASF


          Raymond (Bob) Rowland
          College of Veterinary Medicine,
 Kansas State University, Manhattan, Kansas
        July 21, 2011, Nairobi, Kenya
USDA Coordinated Agricultural Project
                        (PRRS CAP)
•   Stakeholder driven (scientists, producers,
    veterinarians)
•   “Out-of-the-box” approaches to infectious
    disease problem solving
•   Conduct activities that are unique and not
    routinely supported by existing mechanisms
•   Activities converge at the control and elimination
    of virus in the field
•   Leverage
Center of Excellence for Emerging and Zoonotic Animal Diseases (CEEZAD)
                                         CD
                                        Richt
                                         AD:
                                       Rowland

   Theme 1: Vaccines
    C: Richt        AC:        Theme 2: Detection
       Garcia-Sastre               C: Lipkin                  Theme 3: Modeling/
                                 AC: R. Hesse                   Epidemiology
           RVFV:
 (Richt/Young/Ksiazek/Flick)      RVFV/FMDV/AIV:                       C: Gray
                               (Lipkin/Palacios/Wilson)   ACs: HabteMariam/Webby/Scoglio
           FMDV:
  (Estes/Rodriguez/ Golde)       Novel Pathogens:
                                    (Lipkin/Briese)                      RVFV:
            AIV:                                               (Linthicum/Habtemariam)
                                    Field Devices:
   (Garcia-Sastre/ Richt)                                                FMDV:
                                 (Higgins/Culbertson/
                                                              (Perez/HabteMariam/Scott)
      Vaccine Platform:            Anderson/Hesse)
                                                                          AIV:
 (Garcia-Sastre/Rowland/Ma/    Translational Partners:         (Stallknecht/Gray/Webby)
         Rodriguez)               (Orion Biosciences         Others (Data collection, GIS,
                                       Inc./INT/                          etc.):
   Translational Partners:     BI-Vetmedica/Akonni Inc,      (Scoglio/Erickson/Anderson/
 (LAH/BI-Vetmedica/Merial/            Synbiotics)                  Schroeder/Damon)
 GenVec Inc./Bioprotection
         Systems)
Center of Excellence for Emerging and Zoonotic Animal Diseases (CEEZAD)
                                                                  Admin. Core with Admin. Core Dir.
                                          CD                        (ACD)/Emergency Response
                                         Richt                    Coordinator and Internal/External
 International Collaborations                                               Committees
                                          AD:
     (Africa, Asia, Europe)                                      National Collaborations with:
                                        Rowland
                                                                        Agriculture Industry
                                                                 Federal, State, and Local Agencies
   Theme 1: Vaccines                                                  Governmental Groups
    C: Richt        AC:         Theme 2: Detection                  Non-governmental groups
       Garcia-Sastre                C: Lipkin                          Theme 3: Modeling/
                                  AC: R. Hesse                           Epidemiology
           RVFV:
 (Richt/Young/Ksiazek/Flick)       RVFV/FMDV/AIV:                                C: Gray
                                (Lipkin/Palacios/Wilson)           ACs: HabteMariam/Webby/Scoglio
           FMDV:
  (Estes/Rodriguez/ Golde)        Novel Pathogens:
                                     (Lipkin/Briese)                               RVFV:
            AIV:                                                         (Linthicum/Habtemariam)
                                     Field Devices:
   (Garcia-Sastre/ Richt)                                                          FMDV:
                                  (Higgins/Culbertson/
                                                                        (Perez/HabteMariam/Scott)
      Vaccine Platform:             Anderson/Hesse)
                                                                                    AIV:
 (Garcia-Sastre/Rowland/Ma/     Translational Partners:                  (Stallknecht/Gray/Webby)
         Rodriguez)                (Orion Biosciences                  Others (Data collection, GIS,
                                        Inc./INT/                                   etc.):
   Translational Partners:      BI-Vetmedica/Akonni Inc,               (Scoglio/Erickson/Anderson/
 (LAH/BI-Vetmedica/Merial/             Synbiotics)                           Schroeder/Damon)
 GenVec Inc./Bioprotection
         Systems)
                                 Overlay: Outreach/
                                 Training/Education        Outreach/Training/Education:
                                 C: Roth; AC: Montelone      (Roth/Stewart/ Montelone)
Elimination vs. Eradication
Eradication
•   Based on laws- legislated
•   Government supported. Indemnify against losses.
•   Draconian. Non-palatable to producers.
Elimination
•   Stakeholder driven- Incentive to maintain profitability.
•   Varied in scope (herd, region).
•   Incorporates education and organization (sociology).
•   Must be “voluntary”, can be chaotic and divisive.
Arteriviruses (order Nidovirales)
Porcine reproductive and respiratory syndrome virus (PRRSV)
                (Type 1 and Type 2 genotypes)
        Lactate dehydrogenase elevating virus (LDV)
                 Equine arteritis virus (EAV)
           Simian hemorrhagic fever virus (SHFV)

• Enveloped
• Positive single-stranded RNA genome (10-15kb)
• During replication, produce a nested set of subgenomic mRNAs
  with a common leader and poly A tail
• Macrophage-tropic
• Persistent infection and severe and fatal disease
PRRS
“Reproductive Failure of Unknown
Etiology”,Kerry K. Keffaber, 1989, AASP
1.    Anorexia during finishing
2.    Transient increase in respiration rates
3.    Temperature increase (102-106)
4.    Mid- to late-term abortions
5.    Delay in return to heat and infertility
6.    Pre-weaning mortality
7.    Respiratory distress
Blue ear disease-Kansas 2006
PRRS is a swine disease cofactor
  Reston ebolavirus (REBOV)
        Philippines 2008

               Co-Infection of pigs with
               REBOV and PHFD PRRSV
PRRSV as a disease cofactor




Days after weaning            Mortality in groups of 200
                            experimentally challenged pigs
Complex surface topology & composition
  Sites for neutralization remain largely unknown
           heterodimer            heterotrimer
                 GP5                     GP3
            M                     GP2            GP4
  viral
envelope

                            2b 5a
    N
                                        Glycosylation sites
 nucleocapsid
 homopolymer
Complex surface topology & composition


        M
                    Minor
   N          GP    Proteins
              5     • GP2
                    • 2b (E)
                    •GP3
                    •GP4
                    •5a



Dockland-Vet Res (2010)154: 86
Genetic diversity
                               (poor heterologous protection)
                                                    Mutations in a single isolate over time
Peptide sequence variability




                                                                     nsp2
Subversion of innate immunity by NSP1
        (inhibition of the Type 1 IFN response)
• Degradation of CREB-binding protein (CBP) in the nucleus, making
  it unable to form a complex with p300 and interferon regulatory
  factor 3 (IRF3; Kim et al., 2010)
• Inhibition of dsRNA-induced IRF3 and IFN promoter activities (Kim
  et al., 2010)
• Interaction with PIAS1 (Yoo unpublished)
• Inhibition NF-kB function (Song et al., 2010)
• Interference of RIG-I signaling (Yoo et al., 2010)
• Inhibit nuclear translocation of STAT1 (Chen et al., 2010)




      nsp1α          nsp1β
Virus properties that relate
                   to control and eradication
•   Complex virion composition and surface topology
•   Subversion of innate and adaptive immunity
•   Capacity to generate a large degree of genetic diversity
    in structural and nonstructural proteins
•   Macrophage tropism (lymphotropism during subclinical
    infection)
•   Capacity to exist as a subclinical infection and cause
    severe disease
•   Delayed and reduced Ab neutralizing activity (no
    heterologous protection)
•   Co-factor with other infections (ASFV and CSFV)
PRRSV Ecology/Epidemiology •               60% herds infected
              Neumann-2003             •   $600 million/yr
  Endemic infection      Acute outbreaks

                                           FAD Threats
                                           •Feral pigs (8 million)
                                           •Backyard farms



                             Vaccines as biosecurity tools
                             • Block introduction (antibody)
                             • Break endemicity (T cells and innate
                             responses)
                             •Prevent or lower shedding
PRRS vaccines
• Modified live virus (MLV) vaccine introduced in 1994-
  suitable for infected herds
• MLV limitations-virus shedding, persistent infection,
  incomplete immune protection, inability to differentiate
  infected from vaccinated animals (DIVA), potential for
  reversion to virulence
• Killed vaccines are not effective
• Acclimation with wild-type virus as an alternative to
  vaccination
Population size matters
                  Natural Termination/Elimination/Extinction
   Small                                                                 SIR
Populations     Susceptible           Infectious           Resistant


                               Continuous Infection
                                                                       SIRS
               Susceptible            Infectious           Resistant


   Large
Populations
              Loss of immunity- appearance of an escape mutant-introduction
                                      of a new virus
Trends (10 year)
• Less government involvement in disease control and
  eradication (government may not indemnify producers)

$20 million spent to support market prices during the
  pandemic SIV outbreak covered 84 minutes of
  production
How much does $20 million buy in research?

• Developing infectious disease models that are predictive
• Implementing regional approaches to PRRSV elimination
PRRS herd control methodologies
•   Syndromics (1990)
•   Test and removal (1992)
•   Vaccination (1994)
•   Depop-repop
•   All in - all out
•   Acclimation with known viruses
•   Herd closure (200 days-virus extinction)
•   Barn filtration (high density areas – expensive!)
Sow Herd Filtration Study
Scott Dee, University of Minnesota
          Pipetsone, MN


                 Attic installation of filter boxes
                       Advances in biosecurity
Regional approach to elimination
• Herd-level strategies generally fail (virus re-enters from and
  unknown source)
• For herd-level control and elimination to be sustainable, the
  effort must be regional
• Sufficient tools, technologies, resources and leadership
  (political will) to initiate and conduct regional scale projects
• Regional efforts will identify gaps in knowledge that future
  research can fill
PRRS CAP regional elimination projects
•Oral fluid analysis for molecular and
     immunological sureveillance
•Risk analysis tools (PADRAP)
•Risk-based testing
       and surveillance
•Point of care testing
    (serology and PCR)
•Sociology
•Economic cost-benefit analysis
•Vaccines
•Host genetics
Minnesota
                     (Bob Morrison, Montse Torremorell)
                           164,000 pigs-83 sites




2004
  Infected
  Unknown    2006
  Free
  Nursery
  Sows
  Finish
                    2010
Technologies to facilitate elimination
•Oral fluid analysis for molecular and
     immunological surveillance
•Risk analysis tools (PADRAP)
•Risk-based testing
       and surveillance
•Point of care testing
    (serology and PCR)
•Sociology
•Economic cost-benefit analysis
•Vaccines
•Host genetics
PRRSV as dual vaccine vector
5’ UTR   Nsp2-fusion protein
                                           2b
                                1b                  3             6
           1a                               2a            4   5       7   pA

                               GFP   GFP                                  pA

                                     2                                    pA
                                M
                                                3   GFP                   pA
                                                    4                     pA
                          N          GP5                                  pA
                                                          5
                                                              M           pA
                                                              N           pA
Advantages of dual vaccine
• Targets PRRSV and cofactor infection
• Insertion of Ag attenuates or inactivates wild-type virus
• Compliance and DIVA markers
• In the case of nsp2, antigen expressed as a fusion
  protein-incorporated in macromolecular complexes
  (replication complexes) or VLP
• PRRSV is resistant to MDA or existing antibody
Analysis of virus and antibodies in Oral Fluids
                                      Jeff Zimmerman, Iowa State

                       Non-invasive and easy to collect
                       Collect daily
                       Population sample
                       Modification of existing tests (PCR and Ab)
                       Sensitivity
Circulation of three infectious agents
             PRRSV, SIV, PCV2




                    Oral fluid testing for routine surveillance
                   of infectious diseases in swine populations
                             Jeff Zimmerman, IA State
Luminex- Microsphere Immunoassay

       Measure Surface
       Tag Florescence            Green laser
                             Host antibody (analyte)
Measure Internal              Antigen
Dye Florescence
                             Red laser




                         Each sphere is coated
                         with a different antigen
                         “multiplexing to assess quantity
                         and quality of immunity”
Microimmunoassay (MIA) Luminex
• Substitute for standard ELISA
• Can detect multiple analytes (antigens)
  including native and denatured proteins,
  peptides
• Interrogate host antibody response
    DIVA
   Targets of neutralizing antibody
    Immunopathogenic responses
• Sensitivity/Specificity
• Multiple variations
• 2010 MAGPIX instrument (magnetic beads)
   LED detection
   Lower cost-instrument and sample prep
   96 well format
   Simple sample prep
Serum IgG and IgM responses (Luminex)
                 PRRSV N protein

                             n=16 pigs
                                              IgG
                   RNA                                        7
       12000
                                                              6
       10000
                                                              5
MFI     8000                                                      Log
                                                              4
        6000
                                                                  PRRSV
                                                              3
        4000
                                                              2
        2000                        IgM                       1
           0                                                  0
               0         5     10       15          20   25
                              Day after infection
Oral fluid PRRSV IgG and IgM responses
        (Luminex, PRRSV protein)
   14000
   12000
   10000
    8000
    6000
    4000
    2000
      0
           1     3    5   7   9   11   13   15   17   19   21   23   25


               IgM- anti-PRRSV N mean for 12 pens
               IgG- anti-PRRSV N mean for 12 pens
Pig movement
    Point-of-care tests

                          Transport
Transport                 Into a region
out of a region




   Transport
   within a region
Host genetics
   PRRS Host Genetics Consortium (PHGC)
    (CoPDs, Bob Rowland and Joan Lunney, ARS)

1. Use genotyping and phenotyping tools to determine if
   there are host genes that control host response to
   infection (resistance vs. susceptibility)
2. Identify relative importance of different protein markers
   that predict outcomes following infection
3. Conduct “ultra-deep” phenotyping to identify gene
   pathways and novel biomarkers related to virus
   replication and disease
Nursery Pig Model
• 200 pigs (2-3 weeks of age) from different sources in
  Canada and the US
• 5-10 pigs set aside as reference pigs
• 15-16 pigs per pen
• A week after arrival pigs challenged with isolate NVSL
  97-7985
• Collect blood at 0, 3, 7, 10, 14, 21, 28, 35, 42 days dpi
  (serum, RNA Tempus tubes)
• Weigh weekly
• Collect tonsils and ears at Day 42
Phenotypic data (deep phenotype)
•   Morbidity and mortality
•   Viremia, qRT-PCR (ABI) log PRRSV RNA templates/rxn
•   Virus Load, area under curve for the 21 days
•   Weight (weekly)
•   Total antibody and virus neutralizing activity (42 dpi)
•   Circulating cytokine levels
•   Transcriptome analysis of whole blood and tonsil
    (ultradeep phenotyping)
“Deep” phenotyping

Weight gain over time      Log PRRSV RNA over time
Viral Load
                         (AUG)
Quantified as area under the curve from day 0 to 21
Subpopulations with unique phenotypic properties

                                  PRRS tolerant




                                   J.P. Steibel
                                   Mich. St. U.
GWAS-Illumina Porcine 60k Beadchip
Genomic Association Model
                                     k
                  y = Xb + ∑ z iα i δ i + ε
                                    i =1
Where y = phenotypic observations for VL or WG
      X = incidence matrix relating fixed effects to phenotypes
      b = vector of fixed effects of experiment(pen) and
           experiment*parity
      zi = vector of genotypes at SNP i , coded 0/1/2
     αi = substitution effect of SNP i
     δi = indicator for whether SNP i was included (δi=1) or
            excluded (δi=0) in the model for a given iteration of the
            Monte Carlo Markov Chain
           The prior probability of δi= 0 was set equal to pi = 0.99
Bayes B analysis
                                                                      pi = 0.99
                                 Viral Load (AUG)                                                          Weight Gain (ADWG)



                                        SSC 4             SSC X
Proportion of Genetic Variance




                                                                          Proportion of Genetic Variance
                                                                                                                  SSC 4


                                                                                                                               SSC 17




                                 5-SNP window ordered by chromosome                                         5-SNP window ordered by chromosome
Jack Dekkers and Nick Boddicker
Integrated approach (no single solution)

•   Good vaccines
•   Good diagnostics
•   Good understanding of ecology epidemiology
•   Good surveillance approaches
•   Good understanding of social psychology
•   Good pig
Researchable Issues
• Role of PRRSV as a cofactor in ASF pathogenesis and
  ecology
• Development of tools for the study of ASF in BSL-2
  (pseudotyped virus system)
• Multiplex serological assays (Luminex) for investigating
  ASFV immune response and cofactors
• Novel surveillance approaches (oral fluids)
• Risk assessment and biosecurity
• Role of host genes in ASF disease susceptibility,
  resistance and persistence
• Transcriptome analysis to investigate virus-host
  interactions during acute and subclinical infection
• Education

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Surveillance and disease control approaches for pigs and their application to ASF

  • 1. Surveillance and disease control approaches for pigs and their application to ASF Raymond (Bob) Rowland College of Veterinary Medicine, Kansas State University, Manhattan, Kansas July 21, 2011, Nairobi, Kenya
  • 2.
  • 3. USDA Coordinated Agricultural Project (PRRS CAP) • Stakeholder driven (scientists, producers, veterinarians) • “Out-of-the-box” approaches to infectious disease problem solving • Conduct activities that are unique and not routinely supported by existing mechanisms • Activities converge at the control and elimination of virus in the field • Leverage
  • 4. Center of Excellence for Emerging and Zoonotic Animal Diseases (CEEZAD) CD Richt AD: Rowland Theme 1: Vaccines C: Richt AC: Theme 2: Detection Garcia-Sastre C: Lipkin Theme 3: Modeling/ AC: R. Hesse Epidemiology RVFV: (Richt/Young/Ksiazek/Flick) RVFV/FMDV/AIV: C: Gray (Lipkin/Palacios/Wilson) ACs: HabteMariam/Webby/Scoglio FMDV: (Estes/Rodriguez/ Golde) Novel Pathogens: (Lipkin/Briese) RVFV: AIV: (Linthicum/Habtemariam) Field Devices: (Garcia-Sastre/ Richt) FMDV: (Higgins/Culbertson/ (Perez/HabteMariam/Scott) Vaccine Platform: Anderson/Hesse) AIV: (Garcia-Sastre/Rowland/Ma/ Translational Partners: (Stallknecht/Gray/Webby) Rodriguez) (Orion Biosciences Others (Data collection, GIS, Inc./INT/ etc.): Translational Partners: BI-Vetmedica/Akonni Inc, (Scoglio/Erickson/Anderson/ (LAH/BI-Vetmedica/Merial/ Synbiotics) Schroeder/Damon) GenVec Inc./Bioprotection Systems)
  • 5. Center of Excellence for Emerging and Zoonotic Animal Diseases (CEEZAD) Admin. Core with Admin. Core Dir. CD (ACD)/Emergency Response Richt Coordinator and Internal/External International Collaborations Committees AD: (Africa, Asia, Europe) National Collaborations with: Rowland Agriculture Industry Federal, State, and Local Agencies Theme 1: Vaccines Governmental Groups C: Richt AC: Theme 2: Detection Non-governmental groups Garcia-Sastre C: Lipkin Theme 3: Modeling/ AC: R. Hesse Epidemiology RVFV: (Richt/Young/Ksiazek/Flick) RVFV/FMDV/AIV: C: Gray (Lipkin/Palacios/Wilson) ACs: HabteMariam/Webby/Scoglio FMDV: (Estes/Rodriguez/ Golde) Novel Pathogens: (Lipkin/Briese) RVFV: AIV: (Linthicum/Habtemariam) Field Devices: (Garcia-Sastre/ Richt) FMDV: (Higgins/Culbertson/ (Perez/HabteMariam/Scott) Vaccine Platform: Anderson/Hesse) AIV: (Garcia-Sastre/Rowland/Ma/ Translational Partners: (Stallknecht/Gray/Webby) Rodriguez) (Orion Biosciences Others (Data collection, GIS, Inc./INT/ etc.): Translational Partners: BI-Vetmedica/Akonni Inc, (Scoglio/Erickson/Anderson/ (LAH/BI-Vetmedica/Merial/ Synbiotics) Schroeder/Damon) GenVec Inc./Bioprotection Systems) Overlay: Outreach/ Training/Education Outreach/Training/Education: C: Roth; AC: Montelone (Roth/Stewart/ Montelone)
  • 6. Elimination vs. Eradication Eradication • Based on laws- legislated • Government supported. Indemnify against losses. • Draconian. Non-palatable to producers. Elimination • Stakeholder driven- Incentive to maintain profitability. • Varied in scope (herd, region). • Incorporates education and organization (sociology). • Must be “voluntary”, can be chaotic and divisive.
  • 7. Arteriviruses (order Nidovirales) Porcine reproductive and respiratory syndrome virus (PRRSV) (Type 1 and Type 2 genotypes) Lactate dehydrogenase elevating virus (LDV) Equine arteritis virus (EAV) Simian hemorrhagic fever virus (SHFV) • Enveloped • Positive single-stranded RNA genome (10-15kb) • During replication, produce a nested set of subgenomic mRNAs with a common leader and poly A tail • Macrophage-tropic • Persistent infection and severe and fatal disease
  • 8. PRRS “Reproductive Failure of Unknown Etiology”,Kerry K. Keffaber, 1989, AASP 1. Anorexia during finishing 2. Transient increase in respiration rates 3. Temperature increase (102-106) 4. Mid- to late-term abortions 5. Delay in return to heat and infertility 6. Pre-weaning mortality 7. Respiratory distress
  • 10. PRRS is a swine disease cofactor Reston ebolavirus (REBOV) Philippines 2008 Co-Infection of pigs with REBOV and PHFD PRRSV
  • 11. PRRSV as a disease cofactor Days after weaning Mortality in groups of 200 experimentally challenged pigs
  • 12. Complex surface topology & composition Sites for neutralization remain largely unknown heterodimer heterotrimer GP5 GP3 M GP2 GP4 viral envelope 2b 5a N Glycosylation sites nucleocapsid homopolymer
  • 13. Complex surface topology & composition M Minor N GP Proteins 5 • GP2 • 2b (E) •GP3 •GP4 •5a Dockland-Vet Res (2010)154: 86
  • 14. Genetic diversity (poor heterologous protection) Mutations in a single isolate over time Peptide sequence variability nsp2
  • 15. Subversion of innate immunity by NSP1 (inhibition of the Type 1 IFN response) • Degradation of CREB-binding protein (CBP) in the nucleus, making it unable to form a complex with p300 and interferon regulatory factor 3 (IRF3; Kim et al., 2010) • Inhibition of dsRNA-induced IRF3 and IFN promoter activities (Kim et al., 2010) • Interaction with PIAS1 (Yoo unpublished) • Inhibition NF-kB function (Song et al., 2010) • Interference of RIG-I signaling (Yoo et al., 2010) • Inhibit nuclear translocation of STAT1 (Chen et al., 2010) nsp1α nsp1β
  • 16. Virus properties that relate to control and eradication • Complex virion composition and surface topology • Subversion of innate and adaptive immunity • Capacity to generate a large degree of genetic diversity in structural and nonstructural proteins • Macrophage tropism (lymphotropism during subclinical infection) • Capacity to exist as a subclinical infection and cause severe disease • Delayed and reduced Ab neutralizing activity (no heterologous protection) • Co-factor with other infections (ASFV and CSFV)
  • 17. PRRSV Ecology/Epidemiology • 60% herds infected Neumann-2003 • $600 million/yr Endemic infection Acute outbreaks FAD Threats •Feral pigs (8 million) •Backyard farms Vaccines as biosecurity tools • Block introduction (antibody) • Break endemicity (T cells and innate responses) •Prevent or lower shedding
  • 18. PRRS vaccines • Modified live virus (MLV) vaccine introduced in 1994- suitable for infected herds • MLV limitations-virus shedding, persistent infection, incomplete immune protection, inability to differentiate infected from vaccinated animals (DIVA), potential for reversion to virulence • Killed vaccines are not effective • Acclimation with wild-type virus as an alternative to vaccination
  • 19. Population size matters Natural Termination/Elimination/Extinction Small SIR Populations Susceptible Infectious Resistant Continuous Infection SIRS Susceptible Infectious Resistant Large Populations Loss of immunity- appearance of an escape mutant-introduction of a new virus
  • 20. Trends (10 year) • Less government involvement in disease control and eradication (government may not indemnify producers) $20 million spent to support market prices during the pandemic SIV outbreak covered 84 minutes of production How much does $20 million buy in research? • Developing infectious disease models that are predictive • Implementing regional approaches to PRRSV elimination
  • 21. PRRS herd control methodologies • Syndromics (1990) • Test and removal (1992) • Vaccination (1994) • Depop-repop • All in - all out • Acclimation with known viruses • Herd closure (200 days-virus extinction) • Barn filtration (high density areas – expensive!)
  • 22. Sow Herd Filtration Study Scott Dee, University of Minnesota Pipetsone, MN Attic installation of filter boxes Advances in biosecurity
  • 23. Regional approach to elimination • Herd-level strategies generally fail (virus re-enters from and unknown source) • For herd-level control and elimination to be sustainable, the effort must be regional • Sufficient tools, technologies, resources and leadership (political will) to initiate and conduct regional scale projects • Regional efforts will identify gaps in knowledge that future research can fill
  • 24. PRRS CAP regional elimination projects •Oral fluid analysis for molecular and immunological sureveillance •Risk analysis tools (PADRAP) •Risk-based testing and surveillance •Point of care testing (serology and PCR) •Sociology •Economic cost-benefit analysis •Vaccines •Host genetics
  • 25. Minnesota (Bob Morrison, Montse Torremorell) 164,000 pigs-83 sites 2004 Infected Unknown 2006 Free Nursery Sows Finish 2010
  • 26. Technologies to facilitate elimination •Oral fluid analysis for molecular and immunological surveillance •Risk analysis tools (PADRAP) •Risk-based testing and surveillance •Point of care testing (serology and PCR) •Sociology •Economic cost-benefit analysis •Vaccines •Host genetics
  • 27. PRRSV as dual vaccine vector 5’ UTR Nsp2-fusion protein 2b 1b 3 6 1a 2a 4 5 7 pA GFP GFP pA 2 pA M 3 GFP pA 4 pA N GP5 pA 5 M pA N pA
  • 28. Advantages of dual vaccine • Targets PRRSV and cofactor infection • Insertion of Ag attenuates or inactivates wild-type virus • Compliance and DIVA markers • In the case of nsp2, antigen expressed as a fusion protein-incorporated in macromolecular complexes (replication complexes) or VLP • PRRSV is resistant to MDA or existing antibody
  • 29. Analysis of virus and antibodies in Oral Fluids Jeff Zimmerman, Iowa State Non-invasive and easy to collect Collect daily Population sample Modification of existing tests (PCR and Ab) Sensitivity
  • 30. Circulation of three infectious agents PRRSV, SIV, PCV2 Oral fluid testing for routine surveillance of infectious diseases in swine populations Jeff Zimmerman, IA State
  • 31. Luminex- Microsphere Immunoassay Measure Surface Tag Florescence Green laser Host antibody (analyte) Measure Internal Antigen Dye Florescence Red laser Each sphere is coated with a different antigen “multiplexing to assess quantity and quality of immunity”
  • 32.
  • 33. Microimmunoassay (MIA) Luminex • Substitute for standard ELISA • Can detect multiple analytes (antigens) including native and denatured proteins, peptides • Interrogate host antibody response DIVA Targets of neutralizing antibody Immunopathogenic responses • Sensitivity/Specificity • Multiple variations • 2010 MAGPIX instrument (magnetic beads) LED detection Lower cost-instrument and sample prep 96 well format Simple sample prep
  • 34. Serum IgG and IgM responses (Luminex) PRRSV N protein n=16 pigs IgG RNA 7 12000 6 10000 5 MFI 8000 Log 4 6000 PRRSV 3 4000 2 2000 IgM 1 0 0 0 5 10 15 20 25 Day after infection
  • 35. Oral fluid PRRSV IgG and IgM responses (Luminex, PRRSV protein) 14000 12000 10000 8000 6000 4000 2000 0 1 3 5 7 9 11 13 15 17 19 21 23 25 IgM- anti-PRRSV N mean for 12 pens IgG- anti-PRRSV N mean for 12 pens
  • 36. Pig movement Point-of-care tests Transport Transport Into a region out of a region Transport within a region
  • 37. Host genetics PRRS Host Genetics Consortium (PHGC) (CoPDs, Bob Rowland and Joan Lunney, ARS) 1. Use genotyping and phenotyping tools to determine if there are host genes that control host response to infection (resistance vs. susceptibility) 2. Identify relative importance of different protein markers that predict outcomes following infection 3. Conduct “ultra-deep” phenotyping to identify gene pathways and novel biomarkers related to virus replication and disease
  • 38. Nursery Pig Model • 200 pigs (2-3 weeks of age) from different sources in Canada and the US • 5-10 pigs set aside as reference pigs • 15-16 pigs per pen • A week after arrival pigs challenged with isolate NVSL 97-7985 • Collect blood at 0, 3, 7, 10, 14, 21, 28, 35, 42 days dpi (serum, RNA Tempus tubes) • Weigh weekly • Collect tonsils and ears at Day 42
  • 39. Phenotypic data (deep phenotype) • Morbidity and mortality • Viremia, qRT-PCR (ABI) log PRRSV RNA templates/rxn • Virus Load, area under curve for the 21 days • Weight (weekly) • Total antibody and virus neutralizing activity (42 dpi) • Circulating cytokine levels • Transcriptome analysis of whole blood and tonsil (ultradeep phenotyping)
  • 40. “Deep” phenotyping Weight gain over time Log PRRSV RNA over time
  • 41. Viral Load (AUG) Quantified as area under the curve from day 0 to 21
  • 42. Subpopulations with unique phenotypic properties PRRS tolerant J.P. Steibel Mich. St. U.
  • 44. Genomic Association Model k y = Xb + ∑ z iα i δ i + ε i =1 Where y = phenotypic observations for VL or WG X = incidence matrix relating fixed effects to phenotypes b = vector of fixed effects of experiment(pen) and experiment*parity zi = vector of genotypes at SNP i , coded 0/1/2 αi = substitution effect of SNP i δi = indicator for whether SNP i was included (δi=1) or excluded (δi=0) in the model for a given iteration of the Monte Carlo Markov Chain The prior probability of δi= 0 was set equal to pi = 0.99
  • 45. Bayes B analysis pi = 0.99 Viral Load (AUG) Weight Gain (ADWG) SSC 4 SSC X Proportion of Genetic Variance Proportion of Genetic Variance SSC 4 SSC 17 5-SNP window ordered by chromosome 5-SNP window ordered by chromosome
  • 46. Jack Dekkers and Nick Boddicker
  • 47. Integrated approach (no single solution) • Good vaccines • Good diagnostics • Good understanding of ecology epidemiology • Good surveillance approaches • Good understanding of social psychology • Good pig
  • 48. Researchable Issues • Role of PRRSV as a cofactor in ASF pathogenesis and ecology • Development of tools for the study of ASF in BSL-2 (pseudotyped virus system) • Multiplex serological assays (Luminex) for investigating ASFV immune response and cofactors • Novel surveillance approaches (oral fluids) • Risk assessment and biosecurity • Role of host genes in ASF disease susceptibility, resistance and persistence • Transcriptome analysis to investigate virus-host interactions during acute and subclinical infection • Education