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Avian Influenza Vaccination
Plan of Talk
 Introduction
Ideal Avian Influenza Vaccine
1. Prepared from low pathogenic strain.
2. Able to grow well in eggs, to ensure enough antigen in the
vaccine product.
3. Well matched antigenically with the prevalent viruses.
Limitation of Protection
1. Best protection is in experimental studies with SPF chickens.
2. Field protection is less than in laboratory.
3. Poor quality vaccines.
4. Improper storage and handling of vaccines.
5. Reduced vaccine dose, or number of doses used per bird and
length of immunity is important.
6. Improper vaccination technique.
7. Inability to vaccinate 100% of poultry population.
8. Species of birds like ducks and geese are more difficult to get
good immune response.
Environmental Factors That Impact
Success
1. Immunological competence of birds, control of IBDV and CAV.
2. Presence of maternal antibodies
– For broilers research supports 2 dose regime to provide
the best protection throughout the production cycle.
– For single dose vaccination, a full dose of vaccine at 7-10
days maybe the best option at the moment.
3. Virus load in environment, high environmental load may
require Increasing number of vaccinations.
Cont. …
4. HPAI breaks in vaccinated flocks may need minimum of 2
doses and boost every 6 months to optimize protection.
5. Changing virus (drift), periodic testing of emerging field
against vaccines every 2 years.
Important Factors For Vaccine Efficacy
Vaccine Quality
1. HA (antigen) content in vaccine, measured by
hemagglutinating activity.
2. Quality of inactivation.
3. Oil emulsion adjuvant.
4. Vaccine stability.
5. Demonstrated quality control by vaccine manufacturers.
Currently Used Vaccines
 Current vaccines against avian influenza (AI) virus infections
are primarily based on classical inactivated whole-virus
preparations.
Cont. …
 Although administration of these vaccines can protect poultry
from clinical disease, sterile immunity is not achieved under
field conditions, allowing for undetected virus spread and
evolution under immune cover.
 Therefore, there is an urgent need for a robust and reliable
system of differentiation between infected and vaccinated
animals.
Cont. …
Avian influenza (AI) viruses (AIV) are classified into highly
pathogenic and low pathogenicity AIV, depending on the severity
of disease in affected species, whereas;
1. Low pathogenicity AIV (LPAIV) are ubiquitous, and
represent part of the wild bird ecosystem, particularly in
water birds.
2. Highly pathogenic AIV (HPAIV) are primarily found as
causative agents of outbreaks of fowl plague in poultry.
AIV Outbreaks
 Although HPAIV outbreaks have occasionally occurred
worldwide, they have, until recently, been restricted in
geographic spread to the regional or, at most, national level.
Cont. …
 Endemicity of HPAIV in poultry, as observed in several
countries in Southeast Asia and Africa, as well as scattered
outbreaks in domestic poultry in numerous other countries.
 Prompted mass vaccination campaigns using commercially
available vaccines and also led to increased efforts to develop
novel vaccines with improved characteristics.
Cont. …
The first lines of defense against AI are:
1. Surveillance
2. Biosecurity
3. Restrictions on movement
4. Rapid and reliable diagnosis
5. Elimination of AI infected poultry
6. Vaccination can be an additional measure in a
comprehensive control strategy.
Avian Influenza Vaccines
 Vaccinating poultry not only enables the protection of
chickens from clinical signs and death following challenge with
HPAIV, but also reduces virus shedding.
 More importantly, it can prevent the spread of the notifiable
LPAIV H5 and H7, both of which can spontaneously mutate
into highly pathogenic forms, sometimes with only a single
nucleotide alteration.
Inactivated AI Whole-virus Vaccines
 Historically, AIV strains used for inactivated vaccines have
generally been based on LPAIV obtained from field outbreaks.
– The use of HPAIV for this purpose is limited, since this
would require high-level biocontainment manufacturing
facilities.
 Virus preparations are inactivated with beta-propiolactone
(EU) or formaldehyde (USA) and administered intramuscularly
in an oil emulsion mixture.
Cont. …
Homologous vaccines
 Homologous means: containing the same HA subtype as the
field virus but a same NA subtype, as the field virus.
 The disadvantage of this is that these vaccines do not allow
the detection of infection in vaccinated flocks (DIVA:
differentiation between infected and vaccinated animals).
Cont. …
Heterologous vaccines
 Heterologous means: containing the same HA subtype as the
field virus but a different NA subtype, as the field virus.
 The advantage of using heterologous vaccines, allows a DIVA
approach by differentiating NA-specific serum antibodies.
Cont. …
Vaccines containing Al/chicken/Mexico/232/94/CPA strain (LPAI):
1. FLU-KEM vaccine (CEVA-Mexico)
2. Optimune AI (Ceva-Biomune)
3. Nobilis Influenza H5 (Intervet)
4. Valvac AI (Boehringer)
Live AI Vaccines
Owing to this potential danger, the application of live virus
vaccines based on low pathogenic viruses of the H5 and H7
subtype is not recommended, moreover, it is prohibited.
Live Attenuated Vaccines
Cold-adapted attenuated influenza
vaccines have been developed for
humans and equines.
Cont. …
 The use of attenuated live
vaccines (especially of the H5 and
H7 subtypes) in poultry is not
recommended by the World
Organization for Animal Health or
the Food and Agriculture
Organization of the United
Nations (FAO
 They may potentially mutate into
HPAIV by reassortment or
mutation of the HA cleavage site.
Reverse Genetics
Since the advent of reverse genetics for influenza virus and the
development of entirely plasmid-based reverse genetic systems
to rescue recombinant influenza virus, without the need for
helper virus, the generation of recombinant influenza viruses,
according to the respective epidemiological situation, has now
become possible
Cont. …
The use of plasmid-based reverse genetics allows the safe and
efficient generation of attenuated high-growth reassortant
viruses, which derive the genes encoding the envelope proteins
HA and/or NA from circulating influenza A viruses and the
internal genes from vaccine donor strains, such as influenza A
Puerto Rico/8/34 (PR8) (H1N1) or A/WSN 33 (H1N1).
Cont. …
To avoid the requirement for high-level biocontainment facilities,
and to obtain high virus yields in ECE, the polybasic cleavage site
of HPAIV H5 has been altered by deletion and/or mutation of
basic amino acids, resulting in proteins specifying a monobasic
cleavage site characteristic for LPAIV.
Cont. …
 The resulting viruses were used as inactivated oil emulsion AI
vaccines to immunize chickens, ducks and geese.
 They provided effective protection from clinical disease and a
significant reduction of virus shedding after challenge.
Vector Vaccines
 Influenza viruses possess a limited number of immunogenic
proteins, including the envelope glycoproteins HA and NA,
matrix proteins M1 and M2, nucleoprotein NP and non-
structural protein NS1.
 Of these, HA has been demonstrated to be the most relevant
for inducing neutralizing antibodies.
Cont. …
 Different chicken viruses have been used as vectors for the
expression of AIV proteins.
 They include attenuated strains of DNA viruses, such as fowl
pox (FP) virus and infectious laryngotracheitis (ILT) virus, as
well as RNA viruses, such as NDV.
Cont. …
Replication-competent vector vaccines
 Attenuated but replication-competent viruses are probably
the most economic vaccines since;
– They combine the immunogenic properties of protein and DNA
vaccines.
– They are efficacious even at low doses (they can proliferate inside the
vaccinated bird)
Cont. …
 Over the last few decades, many virus genomes have become
accessible to reverse genetics and DNA manipulation
technology, and directed deletion of virulence genes and
insertion of foreign genes, has become feasible.
Vector Vaccines
Poxviruses
 Poxviruses were among the first viral vectors used for the
expression of heterologous proteins.
 The considerable size of the FPV genome, of nearly 300
kilobase pairs, allowed not only insertions of single genes but
also the simultaneous insertion of several genes, encoding,
for example, HA and NA, or HA and NP.
Cont. …
 Avian influenza virus genes were inserted into the genomes of
attenuated FP virus (FPV), which were already in use as live-
virus vaccines against FP in chickens and turkeys.
 Non-essential regions of the FPV genome, such as the
thymidine kinase gene locus, were used as insertion sites and
the foreign proteins were expressed under the control of
strong poxvirus promoters, for instance, the vaccinia virus H6
promoter.
Cont. …
 Single vaccinations with approximately 10 log 5 infectious
units of H5 or H7 expressing FPV recombinants protected
chickens and ducks against lethal challenge infections with
homologous or heterologous AIV of the corresponding
subtypes.
 However, like other AIV vaccines, HA-expressing FPV did not
confer sterile immunity, as demonstrated by the re-isolation
of HPAIV challenge virus from tracheal and cloacal swabs.
Cont. …
 Avian influenza virus vaccines based on fowl pox can be
produced economically on the chorioallantois membrane of
chicken embryos or in primary chicken cell cultures, and can
be administered to one-day-old chickens.
 However, to obtain optimal protection, individual
subcutaneous vaccination (the wing web method) is
recommended.
Cont. …
Since the natural host range of FPV is largely limited to chickens,
to what extent FPV vector vaccines could be suitable for other
species threatened by HPAIV remains to be evaluated in detail.
Cont. …
Although HA-expressing FPV induced specific immune responses
in cats, the protection of immunized turkeys was significantly
less pronounced than that of chickens.
Cont. …
Furthermore, it has been shown that, in chickens that had
previously been immunized against FP, replication of HA-FPV was
inhibited, and only insufficient protection against AIV ensued.
Vector Vaccines
Herpes viruses
 Like poxviruses, herpes viruses possess large, double stranded
DNA genomes that contain numerous genes which are not
needed for virus replication in cultured cells, and which could
be deleted or replaced by foreign DNA sequences.
Vector Vaccines
ILT Viruses
 The ILT virus (ILTV) recombinants, which had been attenuated
by deletion of the non-essential deoxyuridine triphosphatase
(UL50) or UL0 genes, were used for insertion of the coding
sequences of HA subtypes H5 and H7, or NA subtype N1 at
the corresponding loci.
Cont. …
 A single ocular immunization of chickens with 10 log 4 to 10
log 5 plaque forming units of HA-expressing ILTV-
recombinants reliably protected the animals from clinical
symptoms after challenge with lethal doses of homologous
HPAIV.
 However, the death of the animals was delayed, but not
prevented, by immunization with NA-expressing ILTV,
although AIV-specific antibody responses were induced.
Cont. …
 The efficacy of HA-expressing ILTV could be further enhanced
by coadministration with an NA-expressing recombinant,
which parallels the results obtained with other AIV vaccines.
Cont. …
 One limitation of ILTV-based vector vaccines results from the
narrow host range of this virus, which is almost restricted to
chickens, and which barely replicates in other avian species,
such as turkeys.
 In these species, AIV vaccines based on other viral vectors
would be preferable.
 One candidate might be the apathogenic herpesvirus of
turkeys (HVT), which has been used as a live vaccine against
Marek’s disease, and further developed as a vector expressing
immunogenic proteins of NDV and infectious bursal disease
virus.
Cont. …
Furthermore, HVT-based vaccines are suitable for in ovo
vaccination of chickens.

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Avian Influenza Vaccination

  • 2. Plan of Talk  Introduction
  • 3. Ideal Avian Influenza Vaccine 1. Prepared from low pathogenic strain. 2. Able to grow well in eggs, to ensure enough antigen in the vaccine product. 3. Well matched antigenically with the prevalent viruses.
  • 4. Limitation of Protection 1. Best protection is in experimental studies with SPF chickens. 2. Field protection is less than in laboratory. 3. Poor quality vaccines. 4. Improper storage and handling of vaccines. 5. Reduced vaccine dose, or number of doses used per bird and length of immunity is important. 6. Improper vaccination technique. 7. Inability to vaccinate 100% of poultry population. 8. Species of birds like ducks and geese are more difficult to get good immune response.
  • 5. Environmental Factors That Impact Success 1. Immunological competence of birds, control of IBDV and CAV. 2. Presence of maternal antibodies – For broilers research supports 2 dose regime to provide the best protection throughout the production cycle. – For single dose vaccination, a full dose of vaccine at 7-10 days maybe the best option at the moment. 3. Virus load in environment, high environmental load may require Increasing number of vaccinations.
  • 6. Cont. … 4. HPAI breaks in vaccinated flocks may need minimum of 2 doses and boost every 6 months to optimize protection. 5. Changing virus (drift), periodic testing of emerging field against vaccines every 2 years.
  • 7. Important Factors For Vaccine Efficacy Vaccine Quality 1. HA (antigen) content in vaccine, measured by hemagglutinating activity. 2. Quality of inactivation. 3. Oil emulsion adjuvant. 4. Vaccine stability. 5. Demonstrated quality control by vaccine manufacturers.
  • 8. Currently Used Vaccines  Current vaccines against avian influenza (AI) virus infections are primarily based on classical inactivated whole-virus preparations.
  • 9. Cont. …  Although administration of these vaccines can protect poultry from clinical disease, sterile immunity is not achieved under field conditions, allowing for undetected virus spread and evolution under immune cover.  Therefore, there is an urgent need for a robust and reliable system of differentiation between infected and vaccinated animals.
  • 10. Cont. … Avian influenza (AI) viruses (AIV) are classified into highly pathogenic and low pathogenicity AIV, depending on the severity of disease in affected species, whereas; 1. Low pathogenicity AIV (LPAIV) are ubiquitous, and represent part of the wild bird ecosystem, particularly in water birds. 2. Highly pathogenic AIV (HPAIV) are primarily found as causative agents of outbreaks of fowl plague in poultry.
  • 11. AIV Outbreaks  Although HPAIV outbreaks have occasionally occurred worldwide, they have, until recently, been restricted in geographic spread to the regional or, at most, national level.
  • 12. Cont. …  Endemicity of HPAIV in poultry, as observed in several countries in Southeast Asia and Africa, as well as scattered outbreaks in domestic poultry in numerous other countries.  Prompted mass vaccination campaigns using commercially available vaccines and also led to increased efforts to develop novel vaccines with improved characteristics.
  • 13. Cont. … The first lines of defense against AI are: 1. Surveillance 2. Biosecurity 3. Restrictions on movement 4. Rapid and reliable diagnosis 5. Elimination of AI infected poultry 6. Vaccination can be an additional measure in a comprehensive control strategy.
  • 14. Avian Influenza Vaccines  Vaccinating poultry not only enables the protection of chickens from clinical signs and death following challenge with HPAIV, but also reduces virus shedding.  More importantly, it can prevent the spread of the notifiable LPAIV H5 and H7, both of which can spontaneously mutate into highly pathogenic forms, sometimes with only a single nucleotide alteration.
  • 15. Inactivated AI Whole-virus Vaccines  Historically, AIV strains used for inactivated vaccines have generally been based on LPAIV obtained from field outbreaks. – The use of HPAIV for this purpose is limited, since this would require high-level biocontainment manufacturing facilities.  Virus preparations are inactivated with beta-propiolactone (EU) or formaldehyde (USA) and administered intramuscularly in an oil emulsion mixture.
  • 16. Cont. … Homologous vaccines  Homologous means: containing the same HA subtype as the field virus but a same NA subtype, as the field virus.  The disadvantage of this is that these vaccines do not allow the detection of infection in vaccinated flocks (DIVA: differentiation between infected and vaccinated animals).
  • 17. Cont. … Heterologous vaccines  Heterologous means: containing the same HA subtype as the field virus but a different NA subtype, as the field virus.  The advantage of using heterologous vaccines, allows a DIVA approach by differentiating NA-specific serum antibodies.
  • 18. Cont. … Vaccines containing Al/chicken/Mexico/232/94/CPA strain (LPAI): 1. FLU-KEM vaccine (CEVA-Mexico) 2. Optimune AI (Ceva-Biomune) 3. Nobilis Influenza H5 (Intervet) 4. Valvac AI (Boehringer)
  • 19. Live AI Vaccines Owing to this potential danger, the application of live virus vaccines based on low pathogenic viruses of the H5 and H7 subtype is not recommended, moreover, it is prohibited.
  • 20. Live Attenuated Vaccines Cold-adapted attenuated influenza vaccines have been developed for humans and equines.
  • 21. Cont. …  The use of attenuated live vaccines (especially of the H5 and H7 subtypes) in poultry is not recommended by the World Organization for Animal Health or the Food and Agriculture Organization of the United Nations (FAO  They may potentially mutate into HPAIV by reassortment or mutation of the HA cleavage site.
  • 22. Reverse Genetics Since the advent of reverse genetics for influenza virus and the development of entirely plasmid-based reverse genetic systems to rescue recombinant influenza virus, without the need for helper virus, the generation of recombinant influenza viruses, according to the respective epidemiological situation, has now become possible
  • 23. Cont. … The use of plasmid-based reverse genetics allows the safe and efficient generation of attenuated high-growth reassortant viruses, which derive the genes encoding the envelope proteins HA and/or NA from circulating influenza A viruses and the internal genes from vaccine donor strains, such as influenza A Puerto Rico/8/34 (PR8) (H1N1) or A/WSN 33 (H1N1).
  • 24. Cont. … To avoid the requirement for high-level biocontainment facilities, and to obtain high virus yields in ECE, the polybasic cleavage site of HPAIV H5 has been altered by deletion and/or mutation of basic amino acids, resulting in proteins specifying a monobasic cleavage site characteristic for LPAIV.
  • 25. Cont. …  The resulting viruses were used as inactivated oil emulsion AI vaccines to immunize chickens, ducks and geese.  They provided effective protection from clinical disease and a significant reduction of virus shedding after challenge.
  • 26. Vector Vaccines  Influenza viruses possess a limited number of immunogenic proteins, including the envelope glycoproteins HA and NA, matrix proteins M1 and M2, nucleoprotein NP and non- structural protein NS1.  Of these, HA has been demonstrated to be the most relevant for inducing neutralizing antibodies.
  • 27. Cont. …  Different chicken viruses have been used as vectors for the expression of AIV proteins.  They include attenuated strains of DNA viruses, such as fowl pox (FP) virus and infectious laryngotracheitis (ILT) virus, as well as RNA viruses, such as NDV.
  • 28. Cont. … Replication-competent vector vaccines  Attenuated but replication-competent viruses are probably the most economic vaccines since; – They combine the immunogenic properties of protein and DNA vaccines. – They are efficacious even at low doses (they can proliferate inside the vaccinated bird)
  • 29. Cont. …  Over the last few decades, many virus genomes have become accessible to reverse genetics and DNA manipulation technology, and directed deletion of virulence genes and insertion of foreign genes, has become feasible.
  • 30. Vector Vaccines Poxviruses  Poxviruses were among the first viral vectors used for the expression of heterologous proteins.  The considerable size of the FPV genome, of nearly 300 kilobase pairs, allowed not only insertions of single genes but also the simultaneous insertion of several genes, encoding, for example, HA and NA, or HA and NP.
  • 31. Cont. …  Avian influenza virus genes were inserted into the genomes of attenuated FP virus (FPV), which were already in use as live- virus vaccines against FP in chickens and turkeys.  Non-essential regions of the FPV genome, such as the thymidine kinase gene locus, were used as insertion sites and the foreign proteins were expressed under the control of strong poxvirus promoters, for instance, the vaccinia virus H6 promoter.
  • 32. Cont. …  Single vaccinations with approximately 10 log 5 infectious units of H5 or H7 expressing FPV recombinants protected chickens and ducks against lethal challenge infections with homologous or heterologous AIV of the corresponding subtypes.  However, like other AIV vaccines, HA-expressing FPV did not confer sterile immunity, as demonstrated by the re-isolation of HPAIV challenge virus from tracheal and cloacal swabs.
  • 33. Cont. …  Avian influenza virus vaccines based on fowl pox can be produced economically on the chorioallantois membrane of chicken embryos or in primary chicken cell cultures, and can be administered to one-day-old chickens.  However, to obtain optimal protection, individual subcutaneous vaccination (the wing web method) is recommended.
  • 34. Cont. … Since the natural host range of FPV is largely limited to chickens, to what extent FPV vector vaccines could be suitable for other species threatened by HPAIV remains to be evaluated in detail.
  • 35. Cont. … Although HA-expressing FPV induced specific immune responses in cats, the protection of immunized turkeys was significantly less pronounced than that of chickens.
  • 36. Cont. … Furthermore, it has been shown that, in chickens that had previously been immunized against FP, replication of HA-FPV was inhibited, and only insufficient protection against AIV ensued.
  • 37. Vector Vaccines Herpes viruses  Like poxviruses, herpes viruses possess large, double stranded DNA genomes that contain numerous genes which are not needed for virus replication in cultured cells, and which could be deleted or replaced by foreign DNA sequences.
  • 38. Vector Vaccines ILT Viruses  The ILT virus (ILTV) recombinants, which had been attenuated by deletion of the non-essential deoxyuridine triphosphatase (UL50) or UL0 genes, were used for insertion of the coding sequences of HA subtypes H5 and H7, or NA subtype N1 at the corresponding loci.
  • 39. Cont. …  A single ocular immunization of chickens with 10 log 4 to 10 log 5 plaque forming units of HA-expressing ILTV- recombinants reliably protected the animals from clinical symptoms after challenge with lethal doses of homologous HPAIV.  However, the death of the animals was delayed, but not prevented, by immunization with NA-expressing ILTV, although AIV-specific antibody responses were induced.
  • 40. Cont. …  The efficacy of HA-expressing ILTV could be further enhanced by coadministration with an NA-expressing recombinant, which parallels the results obtained with other AIV vaccines.
  • 41. Cont. …  One limitation of ILTV-based vector vaccines results from the narrow host range of this virus, which is almost restricted to chickens, and which barely replicates in other avian species, such as turkeys.  In these species, AIV vaccines based on other viral vectors would be preferable.  One candidate might be the apathogenic herpesvirus of turkeys (HVT), which has been used as a live vaccine against Marek’s disease, and further developed as a vector expressing immunogenic proteins of NDV and infectious bursal disease virus.
  • 42. Cont. … Furthermore, HVT-based vaccines are suitable for in ovo vaccination of chickens.

Hinweis der Redaktion

  1. Endemicity توطن
  2. biocontainment احتواء بيولوجي
  3. advent ظهور