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Diarrhea in Suckling Pigs
Role of Rotavirus
26th Annual Client Appreciation Day
Kent Schwartz
Iowa State University
Veterinary Diagnostic Laboratory
Overview
• History and changes
• Bit of science
• Causes of diarrhea in farrowing
• Role of rotavirus
• Prevention of endemic diarrhea
History
Housing  Nutrition  Genetics
What is “normal”?
Normal is what you are used to…
History
Housing  Nutrition  Genetics
What is “normal”?
Normal is what you are used to…
Continuous improvement requires open minds
 ask “why”?
 willing to learn via analysis
 willing to implement changes
that have demonstrable benefit
History: Infectious Agents of diarrhea
Housing  Nutrition  Genetics
• E. coli 1900
• Salmonella 1900
• TGE 1940
• Clostridium perfringens
type C – 1960’s
• Coccidiosis – 1970’s
• Rotavirus A 1970’s
• PRRSV: 1990
• Clostridium perfringens type A:
2000
• Clostridium difficile 2005
• Rotavirus C 2010
• Rotavirus A, B 2010
• PEDV 2013
• PDCV 2013
• Seneca virus A 2015
• E. coli 1900
• Salmonella 1900
• TGE 1940
• Clostridium perfringens
type C – 1960’s
• Coccidiosis 1970’s
• Rotavirus A 1970’s
History: Infectious Agents of diarrhea
Housing  Nutrition  Genetics
• PRRSV: 1990
• Clostridium perfringens A: 2000
• Clostridium difficile 2005
• Rotavirus C 2010
• Rotavirus A, B 2010
• PEDV 2013
• PDCV 2013
• Seneca virus A 2015
• Cryptosporidia
• Adenovirus
• Next Generation Sequencing
• Microbiome and “biotics”
• More…..
• E. coli 1900
• Salmonella 1900
• TGE 1940
• Clostridium perfringens
type C – 1960’s
• Coccidiosis 1970’s
• Rotavirus A 1970’s
Extreme and constant vigilance 
EXTERNAL BIOSECURITY
The rest are nearly always present
INTERNAL BIOSECURITY
MANAGEMENT
HYGIENE
HERD IMMUNITY
Secret to prevention of endemic diseases?
Some people try to find things in this game
that don’t exist, but football is only two
things – blocking and tackling” (Vince Lombardi)
One of the things young people always ask me about is
what is the secret to success. The secret is there is no
secret. It’s the basics. Blocking and tackling. (Chris Gardner)
Wins come from flawless execution of basics - the
blocking and tackling – every day.
“Science”: Sterile gut experiences “waves” of invaders
Micro-ecology changes and variations are infinite
Ongoing from birth through adult: Metagenomics & Biomes
Birth
Types and numbers of bacteria
CHANGING
Physiology
pH
Anti-trypsin
Enzymes
Microflora
Diets
Age
Immunity
High numbers (billions) of C. perfringens, C. difficile, E. coli within hours
Logbacteriacounts
Time
“Science”: Completely reliant on Passive immunity
• Systemic: Absorbed from COLOSTRUM (absorbed first day)
– Antibody (IgG) mediated immunity
• Systemic bacteria & viruses, toxins of Clostridium
– Immunocytes (cells) that help direct immune response
• cells, cytokines, immunomodulators)
• Mucosal: Continuous via milk ingestion (every 4 hours)
– Antibody (IgA) mediated immunity
• Mucosal pathogens
– Rotaviruses, PEDV, E. coli, TGE
– IgA is gone with weaning (or low milk ingestion / agalactia)
Science: NEONATE Risk factors: Anatomy / Physiology
Small Intestine
• Has longer villi and shorter crypts (7-20x more villus height
• More mature enterocytes more receptors (virus & bacteria)
• Slower to regenerate epithelium / villi (5 days)
Colon not completely functional
• Decreased ability to resorb water & salt or maintain pH balance
Flow: rate? Peristaltic Waves Orderly Motility?
Bacteria
“ Science”: Host physiology AND bacterial physiology
Piglets: high stomach pH, high metabolic rate, limited colon function,
limited regulation of body temperature & gut motility, no trypsin, more…
Bacteria: Dose, maternal immunity, bacteria replication rate, toxin genes
“on” or “off”, more …
RISKS
Chilling and heat stress
Pathogen load in environment
Cross fostering
Compromised passive immunity
The “mathematics” of enteric disease
Severity of disease = DOSE x virulence
Animals’ RESISTANCE
Dose can determine the outcome of infection
Subclinical infection  Disease  Death
DOSE can be controlled – HYGIENE / SANITATION
Internal Biosecurity: Sanitation - Management - Commitment
Severity of disease = dose x VIRULENCE
animal’s resistance
Virulence is difficult to influence with management/nostrums
EXTERNAL BIOSECURITY: A barrier to outside pigs/sources
Do NOT introduce “new” pathogens to a herd
Severity of disease = dose x virulence
Animals’ RESISTANCE
“IMMUNITY”
PASSIVE IMMUNITY
Colostrum contains IgG and Cells – immunomodulation
Colostrum offers systemic immunity; not much mucosal immunity
Milk (Lactogenic) immunity to provide IgA antibody for mucosal (IgA
and IgM) but not systemic immunity; GONE at Weaning
ACTIVE IMMUNITY
Vaccination or infection stimulates antibody and cellular response
What about Animal Science and RISK FACTORS?
Risk Factors influencing piglet resistance to disease
Temperature / chilling / drafts (these are BIG)
Nutritional status and condition of dams
Condition (too fat / too thin)
Ease of farrowing: no hypoxia
Ongoing supply of milk
Genetics, genotype, litter size, milking ability, consumption
Nutrition: quality and quantity of macro- and micro-nutrients
“Herd immunity” – infections consistent across population
Avoid “subpopulations”  all gilts/dams exposed to all potential pathogens
Active immunity via mitigated infection or vaccinations
Good supply of colostrum – litter size – birth weight
Colostrum from immune dams
Acclimation & Vaccination of gilts and sows
Feed-back to gestating dams ???
Severity of disease = dose x virulence
Animals’ RESISTANCE
Concept: Many enteric swine “pathogens” are ENDEMIC
“Potential
Pathogens”
“immunity, nutrition, genetics”
“facilities, management”
“infectious diseases”
Dose x Virulence
Most agents of diarrhea are ENDEMIC 
We can find them with “tests”
 Why is disease being expressed?
INSULT
Age (days)
Mortality0-4 5-8 8-wean
Agalactia x x x can be high
E. coli x x can be high
Clostridium perfringens A x x low
Clostridium perfringens C high
Clostridium. difficile x low
Rotavirus A x x low
Rotavirus B x low
Rotavirus C x x low
PEDV / TGEV x x x high
Porcine deltacoronavirus x x variable
Isospora (coccidia) x x low
PRRSV x x x variable
Salmonella x variable
BIAS: We can find a “bug” but often it is risk factors that allow disease expression
“find something
infectious”
Assign
blame
Bias AND
Diagnosis: Causation or correlation?
(Confirming bias or objective analysis?)
Collect Information
Diagnostic testing
DIAGNOSTIC ACCURACY
Does it “make sense”?
Treatment, Control
Identify Opportunities
Continuous Improvement
Achieving an ACCURATE DIAGNOSIS IS A PROCESS
Think, Analyze, Research
Refine
Repeat
process
Case definition and epidemiology
Information to gather BEFORE making a “diagnosis”
• OBJECTIVE:
– Clinical signs
– Epidemiology
– Timeline
• SUBJECTIVE
– Farm History
– Area history
“Assessing sick piglets
and diarrhea”
Sow problem?
Milk flow?
Sow condition?
Feeding & Water?
Piglet problem?
Clinical signs
Lesions
Laboratory tests
Management problem?
Hygiene
Environment
Process compliance
Cross fostering
Look – Ask – Verify – Think
Necropsy: acutely affected vs moribund pig?
Full
Stomach
White streaks
(Chyle - milkfat)
Subgross examination: Villi
Materials:
• Freshly euthanized pig
• Glass tube (red stopper blood tube)
• Water
Procedure:
• Immediately place 1 cm section of small
intestine in tube
• Add water
• Gently swirl and wait for 1 minute
• Examine directly or with magnifying glass
Interpretation:
• Length: duodenum>jejunum>ileum
• Age: villi get shorter with age
<5 days like photos
Do your own comparisons
10% formalin Refrigerated Test types Agents
Cecal-colon
contents
NO 3-10 ml PCR, ELISA,
isolation
TGE, rotavirus,
Cdiff toxin
Small intestine 6-8 one-inch
segments/lesions
6” ileum
6” jejunum
Histo, IHC,
isolation,
impression
smear, PCR
E. coli, CptA,
CptC, Salmonella,
Isospora
Colon Cross-section of
several loops
Remainder of
colon intact
Histo, isolation C.difficile, AEEC,
Salmonella
Other affected
organs
½” slice Golf ball size Depends Multiple
BAL (lung) NO 1-5 ml (or pieces) PCR PRRSV
Specimens: Select the right pigs!!
3 Acutely Affected Pigs:
Colon Contents
Colon fresh and fixed
Ileum fresh and fixed
Jejunum fresh and fixed
Pool BALs or lung (R/O PRRSV)
Enterotoxigenic E coli: Diagnosis
E. coli (secretory diarrhea)
• Observations:
– Watery diarrhea
– Villi intact
– Chyle in lymphatics
– Bacterial adherence
• Frequently detected
• Frequently blamed
• Is it primary or potentiated
by risk factors?
E. coli Genotyping
Animal ID Gene Result
A, 107 EAST1 (toxin) Positive
LT(toxin) Positive
STa(toxin) Positive
STb(toxin) Positive
Stx1 (toxin) Negative
Stx2 (toxin) Negative
Stx2e(toxin) Negative
F18(pilus) Negative
F41(pilus) Negative
K88(pilus) Positive
K99(pilus) Negative
987P(pilus) Negative
AIDA (adhesin) Negative
EAEA (adhesin) Negative
PAA (adhesin) Positive
E. Coli will always be detected … but is it important?
Histopathology
Virulence-related disease: genotyping
Clostridium perfringens Type C
Disease fairly limited to defined geographical locations
Midwest USA: once common, now uncommon
Quite dramatic when it occurs
Coccidiosis – Isospora suis
- ~5 days through post-weaning
Dose-related disease
Prevention is preferred!
Facility – Hygiene
Internal biosecurity
0
10
20
30
40
50
60
70
80
90
Number of cases of COCCIDIOSIS in suckling piglets
ISU VDL
Control of Isosporosis: Example of dose and hygiene
Must eliminate “sticky” oocysts (also bacteria, viruses)
Bugs “build up” from previous litters – transmit by people
Change flooring – no concrete or wood
All-in/all-out management
SANITATION –
• Soak, soap, degreaser
• Eliminate films
• Appropriate disinfectants
MANAGEMENT
• Mats and mat management
• Cross-fostering pigs
• Hands, boots, fomites, carts, utensils Blocking and tackling of
hygiene
management
environment
Clostridium difficile
Necrotizing typhlocolitis in humans, horses, piglets
Opportunist with severe consequences
in medicated humans and horses
Common (normal) flora in swine:
• MOST (>95%) of herds are colonized
• MOST piglets are colonized by 2 days
Increased frequency of “disease diagnosis”
• Little evidence for “antibiotic induced”
Colon important for absorbing water and
determines feces consistency
Clostridium perfringens type A
• Clostridium perfringens type A is common = ubiquitous
– Environment
– In gut from D0 (high - 108 populations by 12 hr) through adult
• CptA: There are no consistent experimental models using
biologically achievable inoculum to critically evaluate
pathogenesis, treatment and control in enteric disease
Type Alpha Beta Epsilon Iota
A + - (beta2) - -
B + + + -
C + + - -
D + - + -
E + - - +
PED/TGE: segmental or entire small intestine
Isospora: Lower small intestine
E. coli: mid to lower small intestine
Clostridium: upper small intestine
Rotavirus: segmental but mid to lower small intestine
C. difficile: colon
Swine Coronaviruses associated with diarrhea
Transmissible GastroEnteritis - TGEV
Porcine Epidemic Diarrhea - PEDV
Deltacoronavirus - PDCoV
Swine Rotaviruses
Rotaviruses Group A
Rotaviruses Group B
Rotaviruses Group C
No cross-protection between groups
Villi are covered with infected
epithelial cells stained brown
Crypt epithelium is spared and will
be the source of new cell growth
Just 36 hours post-infection in a neonatal piglet:
• Villi are gone  damage done / gut compromised
• Only a few brown-staining cells remain
diagnosis only from ACUTELY affected)
• Millions to billions of virus particles have been shed into the environment
• Tipping point is reached  cows are out of the barn!!
 Extraordinary efforts required to regain control
PEDV and TGEV: Don’t get them!!
EXTERNAL Biosecurityhave and follow protocols)
• Biosecurity protocols: review, strict, tighten, update
– People, supplies, feed, food, etc.
• Limit traffic: people and equipment
• Clean and disinfect incoming: anything
• Enforce downtime
• Disposal of dead stock
• Animal isolation, monitoring and surveillance: diagnostic tests
• Shower, clothing and boots: thorough / change
– Truck and trailer biosecurity
• Loading and unloading procedures
• Crew and driver protocols
• Truck wash procedures
• Manure disposal biosecurity
• Swine transportation
• Verify implementation!
http://www.aasv.org/aasv%20website/Resources/Diseases/PED/PEDVBiosecurity.pdf
Vaccination???
PEDV booster of previously positive sows
Not for “priming” – only after exposure
Rotaviruses cannot be eliminated
• Non-enveloped: very resistant in environment (it’s everywhere!)
• Can cause severe atrophic enteritis just like TGEV/PEDV
• 6 structural proteins (VP)
– VP4
• 26 antigenic P genotypes with 7 P serotypes
• cleaved to VP5+VP8 for infectivity
– VP6: most abundant
– VP7: 15 G genotypes are antigenic with 10 G serotypes
• 6 non-structural proteins (NSP)
– NSP4 may be hypersecretory (like E. coli)
• Structure
– Outer layers: VP7, VP4
– Inner layer: VP6
– Core: VP1, VP2, VP3
• VP6 determines antigenically distinct serogroups 1-7
• Antibody to VP6, VP7, NSP2, NSP4.
– 3 serogroups (A, B, C) and multiple serotypes
are not cross-protective
– “influenza of the gut”
0.00%
10.00%
20.00%
30.00%
40.00%
50.00%
60.00%
2007 2008 2009 2010 2011 2012 2013
Rotavirus Detection: IHC (group A only) prior to 2009
PCR started in 2009  now usually positive for rotavirus
%B & C
%C only
%B only
%A
NOTE: IHC detects rotavirus A  PCR detects rotaviruses A, B and C.
Impact of PCR test sensitivity on “frequency of diagnosis”
Age Distribution versus Serotype
29%
25%
39%
7%
Group A only (N = 479)
< 1 week
1-3 weeks
3- 6 weeks
> 6 weeks
22%
16%
31%
31%
Group B only (163)
< 1 week
1-3 weeks
3- 6 weeks
> 6 weeks
56%
10%
25%
9%
Group C only (N = 521)
< 1 week
1-3 weeks
3- 6 weeks
> 6 weeks
PCR Positive Cases by Month
No seasonal effect
84%
73%
85%88%
81%
89%
79%81%83%
72%72%
80%
0%
10%
20%
30%
40%
50%
60%
70%
80%
90%
100%
% Positive
% Positive
Cases tested in year 2012 (N = 1696)
Diagnosis: Rotavirus
• Experimentally, all serogroups cause similar disease in suckling pigs
• DX = clinical signs + detection + microscopic lesions + rule out others
– Gross and microscopic lesions are not specific
– Lesions segmental  look at multiple (>6) sections
– PCR Ct value (lower is more virus) depend on stage of disease
Sample ACUTELY affected piglets
Sacrifice of 2-3 typical pigs better than simple fecal PCR
• Specific Laboratory Tests
– IHC: Serogroup A
– PCR: Serogroups A, B & C
– Histopathology: compatible lesions
• No serology test available or helpful
Risk Factors / Noninfectious contributors
• Hygiene (ALL OUT with sanitation / disinfection) impacts DOSE
• Environment impacts RESISTANCE
• Chilling (wet, drafts, temperature, heat lamps, mats)
• Mat management; disinfection and timely removal
• Management impacts DOSE and RESISTANCE
– Sow factors: genetics, nutrition
– People and farm culture: teams with pride and engagement
– Farrowing processes and procedures
– Colostrum management
• Immunity impacts RESISTANCE
– Proper acclimation
– Influencing maternal immunity / dam immune status
– Acclimation
– Vaccination?
Vaccination???
PEDV booster of previously positive sows
Not for “priming” – only after exposure
Where are the data for rotaviruses?
Rotavirus: Controlling “Flare-ups”
Double down on basics
Blocking and tackling operate in PEDV mode
Farrowing room processes and procedures / McRebel
Optimize piglet acquisition of colostrum and milk
Manage chilling, drafts, hygienic practices
Can we increase dam immunity?
Acclimation: expose incoming gilts to “prime” their immune
system to resident viruses and bacteria
Vaccine?
Booster maybe?
Lots of effort & Lots of “technology”:
Commercial, autogenous, subunit and otherwise
NO GOOD DATA (vs human vaccines)
What about “feed-back”?
Evolution of concepts: Can feedback help?
• Protect the offspring from disease via IgA and/or IgG and/or CMI
– Passive mucosal immunity – may prevent disease
• Prototypes: TGE, PED and E. coli
• Best IgA response if boostered 10-14 days prefarrow
– Passive systemic immunity – may delay infections
• Systemic disease that are IgG / CMI mediated (Clostridium toxins)
• Best IgG response if boostered 4-5 weeks prefarrow
• Protect the unborn fetus during gestation
– Active systemic immunity prevents viremia in dam
• Protect unborn fetuses
• Prototype: porcine parvovirus
• PRRSV, perhaps other “SMEDI” or unknowns
“Assumptions
– Prototype: PRRSV … but may not be via “Feedback”
– Extrapolations start to get fuzzy
– BTY: Feedback and controlled exposure are NOT the same as vaccination
What do we really know about
feedback to gestating dams?
Proceedings, AASV and SDC
Robbins and Byers: Field Study
1. No statistical differences in outcome over 1 year period
2. Feedback can contain agents that are unexpected
Arruda: Controlled Study
No differences measured in colostrum, sows
or piglet diarrhea after feedback of feces
containing Clostridium spp, E. coli, and rotaviruses
Feedback: understanding pathogenesis, mechanisms
and virulence factors
Moeser AJ, Blikslager AT: J Am Vet Med Assoc 231: 56-
• Fimbria, Pili, Adhesins: Attachment is common 1st step
F18, K88, …. MANY and not just for E. coli
• Viruses and coccidia cause individual cell necrosis
• Pathogenicity islands (code for nanomachine-like proteins) for invasion
• Toxins:
Exotoxins: Clostridia, E. coli
Mediators and modulators: permeability and altered cellular machinery
• Stimulate inflammation
Helpful?
Overzealous?
What is the mechanism
for immunity for
the target agent?
Agents: 4000 in “microbiome” PLUS “Diseases of Swine”
Variation in strains, virulence, cross-protection
Bacteria:
• Actinobacillus sp / type
• Bordetella
• Brachyspira
• Brucella
• Clostridium
• Erysipelothrix
• E. coli: toxins, pili, other
• Haemophilus
• Lawsonia
• Lepto
• Mycobacterium
• Mycoplasma
• Pasteurella multocida A/D
• Salmonella
• Staphylococcus
• Streptococcus
Viruses:
• Coronaviruses (TGE, PDCV, PEDV,
PRCV)
• Enteroviruses (Teschovirus)
• Influenza
• PCMV
• Porcine pestiviruses (CSF, swine pesti)
• Porcine parvoviruses
• Porcine circoviruses
• PRRSV
• PRV
• Rotavirus
• Senecavirus
• Swine poxvirus
• Transboundary: numerous
– Paramyxovirus: Blue-eye, Nipah, Menangle
– Japanese B
• FEED BACK: Objectives?  ENHANCE HERD IMMUNITY
– “Priming” mode  First exposure to a specific strain of pathogen
• Sow Farms: assure uniform first exposure (PEDV)
• Gilt acclimation  PEDV, PRRSV, parvoviruses and MORE
– “Boostering” mode  rotavirus, E. coli, Clostridium sp.
• Boostering previously exposed animals requires HIGH Dose
• Can feedback spread bugs or increase persistence????
– Is that a good thing or bad thing?
• Clostridium perfringens type C or type A or C. difficile?
• Rotaviruses, PRRSV and PCV2
• Erysipelas, Brachyspira, Salmonella, Lawsonia, toxigenic E. coli
• Parasites: Isospora, nematodes
What are some obstacles to
“boostering immunity” via re-infection?
• “Hypo-responsive” to feed matrix / microbiome / diet antigens
• Physiologic: Stomach pH, digestion
• Epithelium
• Innate resistance mechanisms, including
– Mucus flux
– Tight Junctions
– Antimicrobial peptides (kill zone)
– Inflammatory response
• Adaptive immunity – antibody and CMI
– Systemic
– Mucosal
Slight perturbations may not “booster” immunity
– Happens locally
– No need to call in all the “reinforcements”
WHAT and WHEN to feed back?
• For Rotavirus ( enteric viruses, bacteria, piglet scours)
– Feces from acute piglets, 10-14 days prior to farrowing
– Source?
• Feces, wipes, processing carts, anything with poop
• Macerated gut tissue from dead pigs
• Feces/content from intentionally infected pigs??
– Colostrum deprived and sow milk deprived
– Harvest feces and intestines from 1-2 day old pigs
– Easily 1000x more virus particles/unit (Ct 25 15)
• Disclaimer: no published, peer-reviewed research!!
• To protect unborn piglets (congenital tremors, PPV, SMEDI)
– Entrails (guts/viscera/mummies) given prior to breeding
– Eviscerate and macerate (garbage disposal or meat grinder)
IF doing feedback, suggestions are:
1. What is your stated objective? booster IgA to control rotavirus
2. DOSE is important
– High dose better than multiple doses for “booster”
– One dose done right probably better than multiple doses
(Antigenic mass / agent replication sufficient to induce response)
3. TIMING is probably important
– 10-14 days for IgA booster (to control scours)
– 5 weeks for IgG booster (to increase antibody for systemic
diseases or toxins of Clostridium, influenza, IAV, erysipelas)
4. Define and refine the process and procedures
– What are the risks?
– What material to use? Feces/intestines?
– Dilute with cold saline and use immediately or refrigerate < 3 days
– Can retain for future use (for a while) by freezing
5. Be tidy – spend time cleaning
Controlling endemic scour flare-ups
If it’s not TGE or PED, fall back to basics
Go into “PED elimination mode” in farrowing rooms
Develop a checklist / McRebel
 Gilt acclimation (truly acclimated)
 Sow condition, colostrum management, attended farrowings
 Sow farrowing processes and procedures
 Farrowing hygiene between groups and throughout suckling phase
 Stop cross-fostering
 Stop transmitting feces (boots, hands, fomites, carts, etc.)
 Scrupulous hygiene  It is an OB ward!!!
Attempt to develop good herd immunity
 Gilt acclimation, controlled exposure, vaccination, feedback
 Feedback to gestating dams
 Assess risk factors
 Establish a process
 Reinforce basic concepts
 One big dose more important than lots of little doses
Risk Factors potentiate endemic pathogens
Confirmation bias in
making decisions?
Thank you!
ADDED COMMENTS
Does diagnosis matter?
Endemic flareups…
specific interventions?
We can control some level of disease just by management
Hygiene, sanitation, not spreading it, etc
All interventions work better if
Sows are healthy and well fed
Facilities are clean
People are not spreading infectious agents between litters/rooms
People not tranfering disease by moveing pigs or holding them back to
Infect younger pigs
Sometimes it is useful to know the specific agent, particularly if
There are specific interventions!!!

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Dr. Kent Schwartz - Understanding Rotavirus

  • 1. Diarrhea in Suckling Pigs Role of Rotavirus 26th Annual Client Appreciation Day Kent Schwartz Iowa State University Veterinary Diagnostic Laboratory
  • 2. Overview • History and changes • Bit of science • Causes of diarrhea in farrowing • Role of rotavirus • Prevention of endemic diarrhea
  • 3. History Housing  Nutrition  Genetics What is “normal”? Normal is what you are used to…
  • 4. History Housing  Nutrition  Genetics What is “normal”? Normal is what you are used to… Continuous improvement requires open minds  ask “why”?  willing to learn via analysis  willing to implement changes that have demonstrable benefit
  • 5. History: Infectious Agents of diarrhea Housing  Nutrition  Genetics • E. coli 1900 • Salmonella 1900 • TGE 1940 • Clostridium perfringens type C – 1960’s • Coccidiosis – 1970’s • Rotavirus A 1970’s
  • 6. • PRRSV: 1990 • Clostridium perfringens type A: 2000 • Clostridium difficile 2005 • Rotavirus C 2010 • Rotavirus A, B 2010 • PEDV 2013 • PDCV 2013 • Seneca virus A 2015 • E. coli 1900 • Salmonella 1900 • TGE 1940 • Clostridium perfringens type C – 1960’s • Coccidiosis 1970’s • Rotavirus A 1970’s History: Infectious Agents of diarrhea Housing  Nutrition  Genetics
  • 7. • PRRSV: 1990 • Clostridium perfringens A: 2000 • Clostridium difficile 2005 • Rotavirus C 2010 • Rotavirus A, B 2010 • PEDV 2013 • PDCV 2013 • Seneca virus A 2015 • Cryptosporidia • Adenovirus • Next Generation Sequencing • Microbiome and “biotics” • More….. • E. coli 1900 • Salmonella 1900 • TGE 1940 • Clostridium perfringens type C – 1960’s • Coccidiosis 1970’s • Rotavirus A 1970’s Extreme and constant vigilance  EXTERNAL BIOSECURITY The rest are nearly always present INTERNAL BIOSECURITY MANAGEMENT HYGIENE HERD IMMUNITY
  • 8. Secret to prevention of endemic diseases? Some people try to find things in this game that don’t exist, but football is only two things – blocking and tackling” (Vince Lombardi) One of the things young people always ask me about is what is the secret to success. The secret is there is no secret. It’s the basics. Blocking and tackling. (Chris Gardner) Wins come from flawless execution of basics - the blocking and tackling – every day.
  • 9. “Science”: Sterile gut experiences “waves” of invaders Micro-ecology changes and variations are infinite Ongoing from birth through adult: Metagenomics & Biomes Birth Types and numbers of bacteria CHANGING Physiology pH Anti-trypsin Enzymes Microflora Diets Age Immunity High numbers (billions) of C. perfringens, C. difficile, E. coli within hours Logbacteriacounts Time
  • 10. “Science”: Completely reliant on Passive immunity • Systemic: Absorbed from COLOSTRUM (absorbed first day) – Antibody (IgG) mediated immunity • Systemic bacteria & viruses, toxins of Clostridium – Immunocytes (cells) that help direct immune response • cells, cytokines, immunomodulators) • Mucosal: Continuous via milk ingestion (every 4 hours) – Antibody (IgA) mediated immunity • Mucosal pathogens – Rotaviruses, PEDV, E. coli, TGE – IgA is gone with weaning (or low milk ingestion / agalactia)
  • 11. Science: NEONATE Risk factors: Anatomy / Physiology Small Intestine • Has longer villi and shorter crypts (7-20x more villus height • More mature enterocytes more receptors (virus & bacteria) • Slower to regenerate epithelium / villi (5 days) Colon not completely functional • Decreased ability to resorb water & salt or maintain pH balance
  • 12. Flow: rate? Peristaltic Waves Orderly Motility? Bacteria “ Science”: Host physiology AND bacterial physiology Piglets: high stomach pH, high metabolic rate, limited colon function, limited regulation of body temperature & gut motility, no trypsin, more… Bacteria: Dose, maternal immunity, bacteria replication rate, toxin genes “on” or “off”, more … RISKS Chilling and heat stress Pathogen load in environment Cross fostering Compromised passive immunity
  • 13. The “mathematics” of enteric disease Severity of disease = DOSE x virulence Animals’ RESISTANCE Dose can determine the outcome of infection Subclinical infection  Disease  Death DOSE can be controlled – HYGIENE / SANITATION Internal Biosecurity: Sanitation - Management - Commitment
  • 14. Severity of disease = dose x VIRULENCE animal’s resistance Virulence is difficult to influence with management/nostrums EXTERNAL BIOSECURITY: A barrier to outside pigs/sources Do NOT introduce “new” pathogens to a herd
  • 15. Severity of disease = dose x virulence Animals’ RESISTANCE “IMMUNITY” PASSIVE IMMUNITY Colostrum contains IgG and Cells – immunomodulation Colostrum offers systemic immunity; not much mucosal immunity Milk (Lactogenic) immunity to provide IgA antibody for mucosal (IgA and IgM) but not systemic immunity; GONE at Weaning ACTIVE IMMUNITY Vaccination or infection stimulates antibody and cellular response What about Animal Science and RISK FACTORS?
  • 16. Risk Factors influencing piglet resistance to disease Temperature / chilling / drafts (these are BIG) Nutritional status and condition of dams Condition (too fat / too thin) Ease of farrowing: no hypoxia Ongoing supply of milk Genetics, genotype, litter size, milking ability, consumption Nutrition: quality and quantity of macro- and micro-nutrients “Herd immunity” – infections consistent across population Avoid “subpopulations”  all gilts/dams exposed to all potential pathogens Active immunity via mitigated infection or vaccinations Good supply of colostrum – litter size – birth weight Colostrum from immune dams Acclimation & Vaccination of gilts and sows Feed-back to gestating dams ??? Severity of disease = dose x virulence Animals’ RESISTANCE
  • 17. Concept: Many enteric swine “pathogens” are ENDEMIC “Potential Pathogens” “immunity, nutrition, genetics” “facilities, management” “infectious diseases” Dose x Virulence
  • 18. Most agents of diarrhea are ENDEMIC  We can find them with “tests”  Why is disease being expressed? INSULT Age (days) Mortality0-4 5-8 8-wean Agalactia x x x can be high E. coli x x can be high Clostridium perfringens A x x low Clostridium perfringens C high Clostridium. difficile x low Rotavirus A x x low Rotavirus B x low Rotavirus C x x low PEDV / TGEV x x x high Porcine deltacoronavirus x x variable Isospora (coccidia) x x low PRRSV x x x variable Salmonella x variable
  • 19. BIAS: We can find a “bug” but often it is risk factors that allow disease expression “find something infectious” Assign blame Bias AND
  • 20. Diagnosis: Causation or correlation? (Confirming bias or objective analysis?)
  • 21. Collect Information Diagnostic testing DIAGNOSTIC ACCURACY Does it “make sense”? Treatment, Control Identify Opportunities Continuous Improvement Achieving an ACCURATE DIAGNOSIS IS A PROCESS Think, Analyze, Research Refine Repeat process
  • 22. Case definition and epidemiology Information to gather BEFORE making a “diagnosis” • OBJECTIVE: – Clinical signs – Epidemiology – Timeline • SUBJECTIVE – Farm History – Area history
  • 23. “Assessing sick piglets and diarrhea” Sow problem? Milk flow? Sow condition? Feeding & Water? Piglet problem? Clinical signs Lesions Laboratory tests Management problem? Hygiene Environment Process compliance Cross fostering Look – Ask – Verify – Think
  • 24. Necropsy: acutely affected vs moribund pig? Full Stomach White streaks (Chyle - milkfat)
  • 25. Subgross examination: Villi Materials: • Freshly euthanized pig • Glass tube (red stopper blood tube) • Water Procedure: • Immediately place 1 cm section of small intestine in tube • Add water • Gently swirl and wait for 1 minute • Examine directly or with magnifying glass Interpretation: • Length: duodenum>jejunum>ileum • Age: villi get shorter with age <5 days like photos Do your own comparisons
  • 26. 10% formalin Refrigerated Test types Agents Cecal-colon contents NO 3-10 ml PCR, ELISA, isolation TGE, rotavirus, Cdiff toxin Small intestine 6-8 one-inch segments/lesions 6” ileum 6” jejunum Histo, IHC, isolation, impression smear, PCR E. coli, CptA, CptC, Salmonella, Isospora Colon Cross-section of several loops Remainder of colon intact Histo, isolation C.difficile, AEEC, Salmonella Other affected organs ½” slice Golf ball size Depends Multiple BAL (lung) NO 1-5 ml (or pieces) PCR PRRSV Specimens: Select the right pigs!! 3 Acutely Affected Pigs: Colon Contents Colon fresh and fixed Ileum fresh and fixed Jejunum fresh and fixed Pool BALs or lung (R/O PRRSV)
  • 27. Enterotoxigenic E coli: Diagnosis E. coli (secretory diarrhea) • Observations: – Watery diarrhea – Villi intact – Chyle in lymphatics – Bacterial adherence • Frequently detected • Frequently blamed • Is it primary or potentiated by risk factors?
  • 28. E. coli Genotyping Animal ID Gene Result A, 107 EAST1 (toxin) Positive LT(toxin) Positive STa(toxin) Positive STb(toxin) Positive Stx1 (toxin) Negative Stx2 (toxin) Negative Stx2e(toxin) Negative F18(pilus) Negative F41(pilus) Negative K88(pilus) Positive K99(pilus) Negative 987P(pilus) Negative AIDA (adhesin) Negative EAEA (adhesin) Negative PAA (adhesin) Positive E. Coli will always be detected … but is it important? Histopathology Virulence-related disease: genotyping
  • 29. Clostridium perfringens Type C Disease fairly limited to defined geographical locations Midwest USA: once common, now uncommon Quite dramatic when it occurs
  • 30. Coccidiosis – Isospora suis - ~5 days through post-weaning Dose-related disease Prevention is preferred!
  • 31. Facility – Hygiene Internal biosecurity 0 10 20 30 40 50 60 70 80 90 Number of cases of COCCIDIOSIS in suckling piglets ISU VDL
  • 32. Control of Isosporosis: Example of dose and hygiene Must eliminate “sticky” oocysts (also bacteria, viruses) Bugs “build up” from previous litters – transmit by people Change flooring – no concrete or wood All-in/all-out management SANITATION – • Soak, soap, degreaser • Eliminate films • Appropriate disinfectants MANAGEMENT • Mats and mat management • Cross-fostering pigs • Hands, boots, fomites, carts, utensils Blocking and tackling of hygiene management environment
  • 33. Clostridium difficile Necrotizing typhlocolitis in humans, horses, piglets Opportunist with severe consequences in medicated humans and horses Common (normal) flora in swine: • MOST (>95%) of herds are colonized • MOST piglets are colonized by 2 days Increased frequency of “disease diagnosis” • Little evidence for “antibiotic induced” Colon important for absorbing water and determines feces consistency
  • 34. Clostridium perfringens type A • Clostridium perfringens type A is common = ubiquitous – Environment – In gut from D0 (high - 108 populations by 12 hr) through adult • CptA: There are no consistent experimental models using biologically achievable inoculum to critically evaluate pathogenesis, treatment and control in enteric disease Type Alpha Beta Epsilon Iota A + - (beta2) - - B + + + - C + + - - D + - + - E + - - +
  • 35. PED/TGE: segmental or entire small intestine Isospora: Lower small intestine E. coli: mid to lower small intestine Clostridium: upper small intestine Rotavirus: segmental but mid to lower small intestine C. difficile: colon
  • 36. Swine Coronaviruses associated with diarrhea Transmissible GastroEnteritis - TGEV Porcine Epidemic Diarrhea - PEDV Deltacoronavirus - PDCoV Swine Rotaviruses Rotaviruses Group A Rotaviruses Group B Rotaviruses Group C No cross-protection between groups
  • 37. Villi are covered with infected epithelial cells stained brown Crypt epithelium is spared and will be the source of new cell growth
  • 38. Just 36 hours post-infection in a neonatal piglet: • Villi are gone  damage done / gut compromised • Only a few brown-staining cells remain diagnosis only from ACUTELY affected) • Millions to billions of virus particles have been shed into the environment • Tipping point is reached  cows are out of the barn!!  Extraordinary efforts required to regain control
  • 39. PEDV and TGEV: Don’t get them!! EXTERNAL Biosecurityhave and follow protocols) • Biosecurity protocols: review, strict, tighten, update – People, supplies, feed, food, etc. • Limit traffic: people and equipment • Clean and disinfect incoming: anything • Enforce downtime • Disposal of dead stock • Animal isolation, monitoring and surveillance: diagnostic tests • Shower, clothing and boots: thorough / change – Truck and trailer biosecurity • Loading and unloading procedures • Crew and driver protocols • Truck wash procedures • Manure disposal biosecurity • Swine transportation • Verify implementation! http://www.aasv.org/aasv%20website/Resources/Diseases/PED/PEDVBiosecurity.pdf Vaccination??? PEDV booster of previously positive sows Not for “priming” – only after exposure
  • 40. Rotaviruses cannot be eliminated • Non-enveloped: very resistant in environment (it’s everywhere!) • Can cause severe atrophic enteritis just like TGEV/PEDV • 6 structural proteins (VP) – VP4 • 26 antigenic P genotypes with 7 P serotypes • cleaved to VP5+VP8 for infectivity – VP6: most abundant – VP7: 15 G genotypes are antigenic with 10 G serotypes • 6 non-structural proteins (NSP) – NSP4 may be hypersecretory (like E. coli) • Structure – Outer layers: VP7, VP4 – Inner layer: VP6 – Core: VP1, VP2, VP3 • VP6 determines antigenically distinct serogroups 1-7 • Antibody to VP6, VP7, NSP2, NSP4. – 3 serogroups (A, B, C) and multiple serotypes are not cross-protective – “influenza of the gut”
  • 41. 0.00% 10.00% 20.00% 30.00% 40.00% 50.00% 60.00% 2007 2008 2009 2010 2011 2012 2013 Rotavirus Detection: IHC (group A only) prior to 2009 PCR started in 2009  now usually positive for rotavirus %B & C %C only %B only %A NOTE: IHC detects rotavirus A  PCR detects rotaviruses A, B and C. Impact of PCR test sensitivity on “frequency of diagnosis”
  • 42. Age Distribution versus Serotype 29% 25% 39% 7% Group A only (N = 479) < 1 week 1-3 weeks 3- 6 weeks > 6 weeks 22% 16% 31% 31% Group B only (163) < 1 week 1-3 weeks 3- 6 weeks > 6 weeks 56% 10% 25% 9% Group C only (N = 521) < 1 week 1-3 weeks 3- 6 weeks > 6 weeks
  • 43. PCR Positive Cases by Month No seasonal effect 84% 73% 85%88% 81% 89% 79%81%83% 72%72% 80% 0% 10% 20% 30% 40% 50% 60% 70% 80% 90% 100% % Positive % Positive Cases tested in year 2012 (N = 1696)
  • 44. Diagnosis: Rotavirus • Experimentally, all serogroups cause similar disease in suckling pigs • DX = clinical signs + detection + microscopic lesions + rule out others – Gross and microscopic lesions are not specific – Lesions segmental  look at multiple (>6) sections – PCR Ct value (lower is more virus) depend on stage of disease Sample ACUTELY affected piglets Sacrifice of 2-3 typical pigs better than simple fecal PCR • Specific Laboratory Tests – IHC: Serogroup A – PCR: Serogroups A, B & C – Histopathology: compatible lesions • No serology test available or helpful
  • 45. Risk Factors / Noninfectious contributors • Hygiene (ALL OUT with sanitation / disinfection) impacts DOSE • Environment impacts RESISTANCE • Chilling (wet, drafts, temperature, heat lamps, mats) • Mat management; disinfection and timely removal • Management impacts DOSE and RESISTANCE – Sow factors: genetics, nutrition – People and farm culture: teams with pride and engagement – Farrowing processes and procedures – Colostrum management • Immunity impacts RESISTANCE – Proper acclimation – Influencing maternal immunity / dam immune status – Acclimation – Vaccination? Vaccination??? PEDV booster of previously positive sows Not for “priming” – only after exposure Where are the data for rotaviruses?
  • 46. Rotavirus: Controlling “Flare-ups” Double down on basics Blocking and tackling operate in PEDV mode Farrowing room processes and procedures / McRebel Optimize piglet acquisition of colostrum and milk Manage chilling, drafts, hygienic practices Can we increase dam immunity? Acclimation: expose incoming gilts to “prime” their immune system to resident viruses and bacteria Vaccine? Booster maybe? Lots of effort & Lots of “technology”: Commercial, autogenous, subunit and otherwise NO GOOD DATA (vs human vaccines) What about “feed-back”?
  • 47. Evolution of concepts: Can feedback help? • Protect the offspring from disease via IgA and/or IgG and/or CMI – Passive mucosal immunity – may prevent disease • Prototypes: TGE, PED and E. coli • Best IgA response if boostered 10-14 days prefarrow – Passive systemic immunity – may delay infections • Systemic disease that are IgG / CMI mediated (Clostridium toxins) • Best IgG response if boostered 4-5 weeks prefarrow • Protect the unborn fetus during gestation – Active systemic immunity prevents viremia in dam • Protect unborn fetuses • Prototype: porcine parvovirus • PRRSV, perhaps other “SMEDI” or unknowns “Assumptions – Prototype: PRRSV … but may not be via “Feedback” – Extrapolations start to get fuzzy – BTY: Feedback and controlled exposure are NOT the same as vaccination
  • 48. What do we really know about feedback to gestating dams? Proceedings, AASV and SDC Robbins and Byers: Field Study 1. No statistical differences in outcome over 1 year period 2. Feedback can contain agents that are unexpected Arruda: Controlled Study No differences measured in colostrum, sows or piglet diarrhea after feedback of feces containing Clostridium spp, E. coli, and rotaviruses
  • 49. Feedback: understanding pathogenesis, mechanisms and virulence factors Moeser AJ, Blikslager AT: J Am Vet Med Assoc 231: 56- • Fimbria, Pili, Adhesins: Attachment is common 1st step F18, K88, …. MANY and not just for E. coli • Viruses and coccidia cause individual cell necrosis • Pathogenicity islands (code for nanomachine-like proteins) for invasion • Toxins: Exotoxins: Clostridia, E. coli Mediators and modulators: permeability and altered cellular machinery • Stimulate inflammation Helpful? Overzealous? What is the mechanism for immunity for the target agent?
  • 50. Agents: 4000 in “microbiome” PLUS “Diseases of Swine” Variation in strains, virulence, cross-protection Bacteria: • Actinobacillus sp / type • Bordetella • Brachyspira • Brucella • Clostridium • Erysipelothrix • E. coli: toxins, pili, other • Haemophilus • Lawsonia • Lepto • Mycobacterium • Mycoplasma • Pasteurella multocida A/D • Salmonella • Staphylococcus • Streptococcus Viruses: • Coronaviruses (TGE, PDCV, PEDV, PRCV) • Enteroviruses (Teschovirus) • Influenza • PCMV • Porcine pestiviruses (CSF, swine pesti) • Porcine parvoviruses • Porcine circoviruses • PRRSV • PRV • Rotavirus • Senecavirus • Swine poxvirus • Transboundary: numerous – Paramyxovirus: Blue-eye, Nipah, Menangle – Japanese B
  • 51. • FEED BACK: Objectives?  ENHANCE HERD IMMUNITY – “Priming” mode  First exposure to a specific strain of pathogen • Sow Farms: assure uniform first exposure (PEDV) • Gilt acclimation  PEDV, PRRSV, parvoviruses and MORE – “Boostering” mode  rotavirus, E. coli, Clostridium sp. • Boostering previously exposed animals requires HIGH Dose • Can feedback spread bugs or increase persistence???? – Is that a good thing or bad thing? • Clostridium perfringens type C or type A or C. difficile? • Rotaviruses, PRRSV and PCV2 • Erysipelas, Brachyspira, Salmonella, Lawsonia, toxigenic E. coli • Parasites: Isospora, nematodes
  • 52. What are some obstacles to “boostering immunity” via re-infection? • “Hypo-responsive” to feed matrix / microbiome / diet antigens • Physiologic: Stomach pH, digestion • Epithelium • Innate resistance mechanisms, including – Mucus flux – Tight Junctions – Antimicrobial peptides (kill zone) – Inflammatory response • Adaptive immunity – antibody and CMI – Systemic – Mucosal Slight perturbations may not “booster” immunity – Happens locally – No need to call in all the “reinforcements”
  • 53. WHAT and WHEN to feed back? • For Rotavirus ( enteric viruses, bacteria, piglet scours) – Feces from acute piglets, 10-14 days prior to farrowing – Source? • Feces, wipes, processing carts, anything with poop • Macerated gut tissue from dead pigs • Feces/content from intentionally infected pigs?? – Colostrum deprived and sow milk deprived – Harvest feces and intestines from 1-2 day old pigs – Easily 1000x more virus particles/unit (Ct 25 15) • Disclaimer: no published, peer-reviewed research!! • To protect unborn piglets (congenital tremors, PPV, SMEDI) – Entrails (guts/viscera/mummies) given prior to breeding – Eviscerate and macerate (garbage disposal or meat grinder)
  • 54. IF doing feedback, suggestions are: 1. What is your stated objective? booster IgA to control rotavirus 2. DOSE is important – High dose better than multiple doses for “booster” – One dose done right probably better than multiple doses (Antigenic mass / agent replication sufficient to induce response) 3. TIMING is probably important – 10-14 days for IgA booster (to control scours) – 5 weeks for IgG booster (to increase antibody for systemic diseases or toxins of Clostridium, influenza, IAV, erysipelas) 4. Define and refine the process and procedures – What are the risks? – What material to use? Feces/intestines? – Dilute with cold saline and use immediately or refrigerate < 3 days – Can retain for future use (for a while) by freezing 5. Be tidy – spend time cleaning
  • 55. Controlling endemic scour flare-ups If it’s not TGE or PED, fall back to basics Go into “PED elimination mode” in farrowing rooms Develop a checklist / McRebel  Gilt acclimation (truly acclimated)  Sow condition, colostrum management, attended farrowings  Sow farrowing processes and procedures  Farrowing hygiene between groups and throughout suckling phase  Stop cross-fostering  Stop transmitting feces (boots, hands, fomites, carts, etc.)  Scrupulous hygiene  It is an OB ward!!! Attempt to develop good herd immunity  Gilt acclimation, controlled exposure, vaccination, feedback  Feedback to gestating dams  Assess risk factors  Establish a process  Reinforce basic concepts  One big dose more important than lots of little doses
  • 56. Risk Factors potentiate endemic pathogens
  • 57. Confirmation bias in making decisions? Thank you!
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  • 60. ADDED COMMENTS Does diagnosis matter? Endemic flareups… specific interventions? We can control some level of disease just by management Hygiene, sanitation, not spreading it, etc All interventions work better if Sows are healthy and well fed Facilities are clean People are not spreading infectious agents between litters/rooms People not tranfering disease by moveing pigs or holding them back to Infect younger pigs Sometimes it is useful to know the specific agent, particularly if There are specific interventions!!!

Editor's Notes

  1. You have seen this before Epidemic Endemic
  2. Objective: observations, check list, numbers, dates, timeline, parities Subjective: lots of biases….prior history, neighboring farms, what others are talking about
  3. WHAT DOES GENOTYPING TELL YOU???? ANTIBIOTIC SENSITIVITY is NOT PREDICTIVE OF PATHOGENIC POTENTIAL
  4. Other than a few months in here (Feb, Oct, Nov), most of the months have a higher percentage of positive cases (in the mid 80s), compared to the previous years.