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FMD sampling and laboratory
diagnosis
UTC-1
David Paton, Eoin Ryan, Kees Van Maanen,
Nick Lyons, Jenny Maud, Etienne Chevanne
Uninfected
Live Virus
by virus isolation
in cell cultures
Viral Proteins by LFD or double
antibody sandwich ELISA
Viral Nucleic Acid
by RT-PCR
Anti-FMD antibodies can be
detected in serum by ELISA or
VNT
FMD Virus infected Recovered (or vaccinated)
Lesion, swab, probang or
clotted blood samples
Virus or viral
components can be
detected
Clotted blood samples
(saliva)
Anti-viral antibodies can
be detected
1-4 days
10-30 minutes (LFD)
4 hours (ELISA)
Around 4 hours 5-18 hours (ELISA)
2-3 days (VNT)
Probang
samples
Principals of FMD Diagnosis
1 Rapid confirmation
of clinical signs
FMD diagnostic windows
2 Pre-clinical surveillance
Virus in blood
Antibody
response
3 Sero-surveillance
for FMDV exposed animals
DAYS
QUANTITY
14654321 87 ● ● ● ●
Source: WRLFMD, Pirbright
Clinical
lesions
virus in
lesions
Vesicular epithelium and fluid !! Sample of Choice !!
Always collect if present
The richest source of FMD virus
Highly desired from primary cases
Suitable for all virus detection tests
Blood
Always collect, whether or not vesicles present
Detection of virus in viraemic animals (Clotted or EDTA anticoagulated blood).
Detection of antibodies in recovering/immune animals (Clotted blood).
Oral/nasal swabs
Virus persists longer here than in blood (e.g. 4-5 day old lesions)
Detection of virus by RT-PCR or VI. Also differential diagnosis.
Top Priority Samples
Other Samples
Oropharyngeal fluid (probang)
>1 month virus persistence in ~50% infected ruminants (carriers).
Low levels of virus detected by RT-PCR or VI
Cardiac muscle in myocarditis cases
Rich source of virus
Detection by all tests – RT-PCR, Ag ELISA, VI
Milk
Variable amount of virus or antibody
Detection by RT-PCR and by serology
Air or environmental samples
Low levels of often inactivated virus
Detection by RT-PCR.
Sampling cases with lesions
Collect: Vesicular epithelium +/- fluid and blood, always!
Heart muscle (myocarditis cases)
Herd-level: Samples from at least 5 animals with obvious lesions should
be sufficient to confirm a diagnosis
– For tissues
At least 2 cm2 of epithelium from unruptured or freshly ruptured vesicles –
fingernail sized amount
Transport medium - equal amounts of glycerine and 0.04 M phosphate
buffer pH 7.2-7.6
– For vesicular fluids (very hard to get!)
Into a plain tube
Herd-level: For diagnosis, select at least 10 animals, prioritizing those
with suspicious clinical signs or epidemiological links
-- Fever, depression, lameness, milk drop, healed lesions --
Collect clotted or EDTA blood samples
to obtain serum to detect viraemia or antibodies
Oronasal swabs and/or probangs (ruminants only)
may be of value, laboratory capacity for processing?
Sampling cases with no/old vesicular lesions
Sheep
Calf
Cow
Packaging of samples for shipment to the lab
Collect samples in leak-proof, shatter-proof containers and label indelibly;
Disinfect outside of containers, surround with absorbent material and
place in secondary container;
Surround with cool packs and place with submission form in insulated box;
Address outer package and add contents description and hazard warning
Inform laboratory
Probang technique
Restrain animal and measure probang against side of head to
calculate distance to throat,
Insert probang over tongue into the oropharynx, avoiding teeth,
Move back and fourth 4-6 times to collect fluid from the soft
palate area,
Withdraw the probang cup with the head held up. Discard the
sample if it contains rumen material (pH=5).
Cattle: tip the fluid into a tube containing 2-3 ml of neutral pH
0.08M PBS.
Sheep/goats: insert probang head into a wide-necked tube
containing 2-3 ml of neutral pH 0.08M PBS and agitate.
Wash probang thoroughly between animals: 3 bucket system
WATER
4% NA2CO3
or 0.2% CITRIC ACID
WATER
Field diagnosis of FMD (pen-side)
Lateral-flow devices
(LFDs)
Sensitivity ~80%
Rapid confirmation
of positives
Able to confirm
negatives
T-COR 8 PCR machine in action
(real-time amplification of the target DNA
is displayed on the screen)
Molecular assays
(RT-PCR, LAMP)
Sensitivity>95%
Sample preparation for Ag-LFD
SVANODIP® FMDV-Ag Test: Test Procedure
Reading results after 10 minutes
No line in the ”T” position
indicates a NEGATIVE test result
A line in the
”C” position
indicates a
valid test
A line in the ”T” position
indicates a POSITIVE test result
After field testing,
the LFD can be sent
to the lab for RT-PCR
Y
Y
Y
Y
Y
Y
Y
Y
Y
Y
Y
Y
Y
Y
Y
Y
Absorbent
pad
Release
pad Blue-coloured latex beads
coated with FMDV-specific Ab
Clinical sample
Containing FMDV
FLOW FLOW
Rapid (<10 mins) confirmation of FMD in the field (simple, stable, robust, no need of cold chain,
suited for field conditions)
Recognises all 7 FMDV serotypes
Similar assay performance (sensitivity) to lab-based Ag-ELISA
Only for vesicular epithelium or fluid
Lateral Flow Device (LFD)
• Investigating suspect cases of FMD and quantifying
the prevalence of FMDV infection
• Substantiating freedom from infection at population
or individual animal level (often for trade)
• Evaluating population immunity (post vaccination
monitoring) and vaccine matching
FMD Serology: applications
FMD Serology: SP/NSP tests and the DIVA principle
NSPs
Infection with
live virus
SP antibodies
- Serotype-specific
- Correlate to
protection
NSP antibodies
- Pan-serotype reactive
- Used for DIVA testing
Viral non-structural
proteins (NSP)
Inactivated purified
virus (structural
proteins, SP)
Live virus
KEY TO FIGUREVaccination with
purified vaccine
Vaccinated
- infected
NSPs
Vaccine virus
preparation
Purification
FMD serological tests detect antibodies directed at
either:
• FMD viral structural proteins (SP) that are variable and make
up the capsid or shell of virus particles e.g. SP ELISAs or VNT
or
• FMD viral non-structural proteins (NSP) that are conserved
and involved in intracellular virus replication e.g. NSP ELISAs
Types of FMD Serology
O A C Asia 1 SAT 1 SAT 2 SAT 3
anti-SP Antibodies serotype-specific
Seven different assays, one for each FMD virus type
anti-NSP antibodies identical for 7 serotypes
O / A / C / Asia 1 / SAT 1 / SAT 2 / SAT 3
NSP tests  A unique assay for all FMD virus types
Both can be used to detect animals that have been infected
with FMDV but their markedly different specificities will influence
the choice of which one to use in particular situations
• Only an NSP test can
– detect antibodies to any FMDV serotype
– differentiate antibodies due to infection from those due to
vaccination
• Only an SP test can
– measure protective immunity
– identify the serotype (more difficult in endemic settings)
Differences in Use of SP and NSP tests
What samples would you take?
FMD suspect case in Gharbaya,
Egypt, March 2012
What samples should I have
taken?
What results would you
expect?
Thanks for your attention
Questions on sampling and diagnostic?

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Laboratory diagnosis and sampling Uganda Training Course

  • 1. FMD sampling and laboratory diagnosis UTC-1 David Paton, Eoin Ryan, Kees Van Maanen, Nick Lyons, Jenny Maud, Etienne Chevanne
  • 2. Uninfected Live Virus by virus isolation in cell cultures Viral Proteins by LFD or double antibody sandwich ELISA Viral Nucleic Acid by RT-PCR Anti-FMD antibodies can be detected in serum by ELISA or VNT FMD Virus infected Recovered (or vaccinated) Lesion, swab, probang or clotted blood samples Virus or viral components can be detected Clotted blood samples (saliva) Anti-viral antibodies can be detected 1-4 days 10-30 minutes (LFD) 4 hours (ELISA) Around 4 hours 5-18 hours (ELISA) 2-3 days (VNT) Probang samples Principals of FMD Diagnosis
  • 3. 1 Rapid confirmation of clinical signs FMD diagnostic windows 2 Pre-clinical surveillance Virus in blood Antibody response 3 Sero-surveillance for FMDV exposed animals DAYS QUANTITY 14654321 87 ● ● ● ● Source: WRLFMD, Pirbright Clinical lesions virus in lesions
  • 4. Vesicular epithelium and fluid !! Sample of Choice !! Always collect if present The richest source of FMD virus Highly desired from primary cases Suitable for all virus detection tests Blood Always collect, whether or not vesicles present Detection of virus in viraemic animals (Clotted or EDTA anticoagulated blood). Detection of antibodies in recovering/immune animals (Clotted blood). Oral/nasal swabs Virus persists longer here than in blood (e.g. 4-5 day old lesions) Detection of virus by RT-PCR or VI. Also differential diagnosis. Top Priority Samples
  • 5. Other Samples Oropharyngeal fluid (probang) >1 month virus persistence in ~50% infected ruminants (carriers). Low levels of virus detected by RT-PCR or VI Cardiac muscle in myocarditis cases Rich source of virus Detection by all tests – RT-PCR, Ag ELISA, VI Milk Variable amount of virus or antibody Detection by RT-PCR and by serology Air or environmental samples Low levels of often inactivated virus Detection by RT-PCR.
  • 6. Sampling cases with lesions Collect: Vesicular epithelium +/- fluid and blood, always! Heart muscle (myocarditis cases) Herd-level: Samples from at least 5 animals with obvious lesions should be sufficient to confirm a diagnosis – For tissues At least 2 cm2 of epithelium from unruptured or freshly ruptured vesicles – fingernail sized amount Transport medium - equal amounts of glycerine and 0.04 M phosphate buffer pH 7.2-7.6 – For vesicular fluids (very hard to get!) Into a plain tube
  • 7. Herd-level: For diagnosis, select at least 10 animals, prioritizing those with suspicious clinical signs or epidemiological links -- Fever, depression, lameness, milk drop, healed lesions -- Collect clotted or EDTA blood samples to obtain serum to detect viraemia or antibodies Oronasal swabs and/or probangs (ruminants only) may be of value, laboratory capacity for processing? Sampling cases with no/old vesicular lesions Sheep Calf Cow
  • 8. Packaging of samples for shipment to the lab Collect samples in leak-proof, shatter-proof containers and label indelibly; Disinfect outside of containers, surround with absorbent material and place in secondary container; Surround with cool packs and place with submission form in insulated box; Address outer package and add contents description and hazard warning Inform laboratory
  • 9. Probang technique Restrain animal and measure probang against side of head to calculate distance to throat, Insert probang over tongue into the oropharynx, avoiding teeth, Move back and fourth 4-6 times to collect fluid from the soft palate area, Withdraw the probang cup with the head held up. Discard the sample if it contains rumen material (pH=5). Cattle: tip the fluid into a tube containing 2-3 ml of neutral pH 0.08M PBS. Sheep/goats: insert probang head into a wide-necked tube containing 2-3 ml of neutral pH 0.08M PBS and agitate. Wash probang thoroughly between animals: 3 bucket system WATER 4% NA2CO3 or 0.2% CITRIC ACID WATER
  • 10. Field diagnosis of FMD (pen-side) Lateral-flow devices (LFDs) Sensitivity ~80% Rapid confirmation of positives Able to confirm negatives T-COR 8 PCR machine in action (real-time amplification of the target DNA is displayed on the screen) Molecular assays (RT-PCR, LAMP) Sensitivity>95%
  • 12. SVANODIP® FMDV-Ag Test: Test Procedure Reading results after 10 minutes No line in the ”T” position indicates a NEGATIVE test result A line in the ”C” position indicates a valid test A line in the ”T” position indicates a POSITIVE test result After field testing, the LFD can be sent to the lab for RT-PCR
  • 13. Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Y Absorbent pad Release pad Blue-coloured latex beads coated with FMDV-specific Ab Clinical sample Containing FMDV FLOW FLOW Rapid (<10 mins) confirmation of FMD in the field (simple, stable, robust, no need of cold chain, suited for field conditions) Recognises all 7 FMDV serotypes Similar assay performance (sensitivity) to lab-based Ag-ELISA Only for vesicular epithelium or fluid Lateral Flow Device (LFD)
  • 14. • Investigating suspect cases of FMD and quantifying the prevalence of FMDV infection • Substantiating freedom from infection at population or individual animal level (often for trade) • Evaluating population immunity (post vaccination monitoring) and vaccine matching FMD Serology: applications
  • 15. FMD Serology: SP/NSP tests and the DIVA principle NSPs Infection with live virus SP antibodies - Serotype-specific - Correlate to protection NSP antibodies - Pan-serotype reactive - Used for DIVA testing Viral non-structural proteins (NSP) Inactivated purified virus (structural proteins, SP) Live virus KEY TO FIGUREVaccination with purified vaccine Vaccinated - infected NSPs Vaccine virus preparation Purification
  • 16. FMD serological tests detect antibodies directed at either: • FMD viral structural proteins (SP) that are variable and make up the capsid or shell of virus particles e.g. SP ELISAs or VNT or • FMD viral non-structural proteins (NSP) that are conserved and involved in intracellular virus replication e.g. NSP ELISAs Types of FMD Serology
  • 17. O A C Asia 1 SAT 1 SAT 2 SAT 3 anti-SP Antibodies serotype-specific Seven different assays, one for each FMD virus type anti-NSP antibodies identical for 7 serotypes O / A / C / Asia 1 / SAT 1 / SAT 2 / SAT 3 NSP tests  A unique assay for all FMD virus types
  • 18. Both can be used to detect animals that have been infected with FMDV but their markedly different specificities will influence the choice of which one to use in particular situations • Only an NSP test can – detect antibodies to any FMDV serotype – differentiate antibodies due to infection from those due to vaccination • Only an SP test can – measure protective immunity – identify the serotype (more difficult in endemic settings) Differences in Use of SP and NSP tests
  • 19. What samples would you take? FMD suspect case in Gharbaya, Egypt, March 2012 What samples should I have taken? What results would you expect?
  • 20. Thanks for your attention Questions on sampling and diagnostic?