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Herpesviruses of Molluscs
                  Carolyn Friedman
• Herpesvirus infections have been detected in many mollusc
  species in association with mortality outbreaks, including

                    Crassostrea virginica

                          C. gigas
                        Ostrea edulis
                          O. angasi
                         O. chilensis
                    Ruditapes decussatus
                      R. phillipinarum
                      Pecten maximus

                Haliotis diversicolor supertexa
                       Haliotis laevigata
                         Haliotis rubra
Global distribution of OsHV




         OsHV infections
OsHV-1
                                                                 OsHV-1
• Icosahedral DNA virus, replicates in nucleus
  and migrates to cytoplasm (enveloped by
  nuclear membrane)
• OsHV-1 in France has been characterized
  – Virions have been
    purified, described, and sequenced
     • The genome is 207 kb
                                                 From: Davison et al. 2005

  – Sequence comparisons showed that
    OsHV-1 is tenuously related to vertebrate
    herpesviruses
Herpesvirus evolutionary tree



  FISH AND     TERRESTRIAL
  AMPHIBIANS   VERTEBRATES OYSTERS
Oyster herpesviruses (OsHV)
• Mortalities are typically short in duration and can
  reach up to 90% (in larvae) and 40-80% (in seed)
  – Mortalities particularly affect small and/or fast growing
    seed oysters
• Virus also detected in multiple adult species where
  mortality not recorded
• Associated with warm water temperatures and high
  densities of animals
  – 24-25 C needed for virion replication based on lab
    experiments in larvae
  – 24-25 C also associated with field mortalities of seed
    oysters
Possible modes of transmission

• In hatcheries, vertical transmission has been
  suggested
• In the field, at least in Tomales Bay, uninfected
  seed oysters are outplanted each year
  – OsHV has not been detected in any hatcheries or
    nurseries to date in the US
  – Adult bivalves in the bay may have latent infections
• In lab – cannot transmit to stages older than
  larvae
OsHV Transmission in Tomales Bay

           Mortality   Max     Mean     Dection of OsHV
100                                                       30
 90
 80                                                       25
 70                                                       20
 60
 50                                                       15
 40
 30                                                       10
 20                                                       5
 10
  0                                                       0
      5/17- 6/4- 6/17- 7/2- 7/16- 7/30 8/13- 8/28- Cum.
       6/3 6/16 7/1 7/15 7/29 -8/12 8/27 9/9
OsHV Transmission in larvae

                   100
                   90
                   80
                   70
Percent Survival




                   60
                   50
                   40
                   30
                   20
                   10
                    0
                         1      3          5          7   9
                                     Experiment Day
OsHV Diagnostic Methods
                                               4d

• Light microscopy
   – Nuclear hypertrophy and
     chromatin margination
     • Cells of the gills, mantle, and velum
       (not epithelial cells)
     • Signs of viral-induced apoptosis
  – Slight or no inflammatory                  4b

    response around infected cells
  – Changes often described in
    larvae but not juvenile or adult
    oysters
OsHV Diagnostic Methods 2
• In situ hybridization
  – Section through the
    visceral ganglion.
  – Labelled cells
    (arrowheads) and non-
    labelled cells (arrows).
  – The DIG-labelled probe
    reacts strongly within
    the cytoplasm and the
    nucleus of nervous cells
    (bar=10 um).
OsHV Diagnostic Methods 3
• Transmission Electron
  Microscopy (TEM)
  – Presence of spherical to
    polygonal unenveloped
    particles ~80 nm in
    diameter in nucleus of
    infected larvae and spat
  – Enveloped virions ~122
    nm in cytoplasmic
    vesicles, perinuclear
    space & extrcellularly
OsHV Diagnostic Methods 4
OsHV Diagnosis Methods 5
• Multiple conventional and QPCR primer sets have
  been designed to amplify regions of the OsHV-1
  genome
• PCR allows for both diagnosis of OsHV and the
  comparison of possible OsHV variants

        A)
                    UL            X         US
             TRL            IRL       IRS        TRS


        B)
              C              C
                   A GP B
Global distribution of OsHV




     OsHV infections   PCR as diagnostic tool
OsHV research in our lab
• Improving survival of seed oysters in the field
• OsHV transmission in larval and seed oysters
   – may include the addition of Vibrio tubiashii in transmission
     experiments
• Comparison of global OsHV variants
• Testing histology blocks from early Tomales Bay
  mortalities as well as imports into TB from other parts
  of the world
• Developed 2 qPCR assays
   – One DNA-based and one RNA-based
OsHV µ-var 1
• In 2008- high mortality rates of 80% to 100% in
  Crassostrea gigas
  – Mainly juvenile oysters from May to September
• 75% positive batches for OsHV-1
  – ?new biotype of OsHV-1?
• Extracts of field affected oysters  induced
  mortalities (80% IM, 40% cohabitation) in spat and
  juvenile oysters
  – qPCR and TEM confirmed viral infection
• 0.1μm filtration or UV inactivated OsHV µvar
OsHV µ-var
• “Both biotypes identified in isolates, OsHV1 and
  OsHV1 μVar*, were virulent and generated
  mortality with the oyster stages used”
• “the first time that such results trial were obtained”
• “Analysis of various target sequences within viral
  genome present in infected batches demonstrated
  the presence of polymorphism”  OsHV1 μVar
  and patented finding


• From Sauvage et al. 2009
Specific questions

Could you tell me what do you do when detect a positive
sample to OsHV-1?

Do you have an estimation about the losses when an
episode of OsHV-1 occurs?

Is there any governmental regulation to avoid dispersion of
OsHV-1?

Do you have a surveillance program for OsHV-1 in oyster
farms or environment?

If yes, how is it?
If we detect a new positive sample (ie in a new
location), we repeat our analysis, add sequence
analysis and in situ hybridization to confirm infection

The losses due to a herpes outbreak in Tomales Bay
can certainly be greater than 90%, at least in patches.

Regarding regulations, OsHV is not on our list of
diseases that California regulates. It probably will be
added next time we make changes, but that will be
more than a year from now. However, we still can use
more broad, open-ended regulations to restrict
movement of infected product or seed.
.
I was hoping to get the OsHV-1 RT PCR assay going in my
lab this summer and we got most of the way there but have
not had time to set up the proper standards yet for
quantification. I hope to be completely setup by next Spring
to conduct regular testing and do some experiments. Also
want to get OsHV uvar testing. So currently there is no
proper surveillance program for OsHV-1 but I expect there
will be by next year. We will examine oysters from the
growing areas listed above as well as from naturalized C.
gigas in numerous southern California harbors and bays.
To my knowledge OsHV has only been detected in Tomales
Bay and Drakes Bay. The growers in these areas will not
send seed to other growing areas. Actually, all of the seed
or larvae that enters the state's growing areas- Carlsbad
Lagoon, Santa Barbara, Morro Bay, Tomales Bay, Drakes
Bay and Humboldt Bay- comes either from Taylor in
Washington    (or   Hawaii),   Coast   in   Washington   (or
Hawaii), Whiskey Creek in Oregon, Hawaiian Shellfish in
Hilo, or from Humboldt Bay to the other growing areas
Abalone herpesvirus disease
• Known affected species - to date, primarily
  observed in
  – Taiwan beginning in 2003, detected 2003-2005
     • both subspecies of Haliotis diversicolor (aquatilis and supertexta)
  – Australia beginning in December 2005/January
    2006
     • Haliotis laevegata
     • H. rubra
     • hybrids of H. laevegata x H. rubra
• Losses typically occur when water temperatures are
  <22C and often range from 16-19C
The first abalone farm infected with herpes-like virus

              Gross observations of ALVD




   •Tank water turbid and frothy (above) from regurgitated food
   particles and mucus in water in Taiwan
   •Rapid onset of mortality in tanks, ponds, or wild populations
   • No visible change in abalone feeding habits prior to onset
Clinical signs: Holiotis diversicolor
                   supertexta
Tank water was turbid and bubbly.




                      Healthy vs. moribund abalone
AHLVD: Gross observations
• Affected abalone with clinical signs varying from
  none to
  – Stiff pedal muscle with darkened lateral mantle
  – Increased mucus production reported in many
    cases
  – And may present swollen, prolapsed mouth with
    everted radula in some cases (noted in Australian
    abalone species)
  – Mortalities typically observed within 3 days of onset
    of clinical signs, and dead abalone may remain
    adhered to substrata
  – Losses often complete within 9-14d
AHLVD: Gross Signs Australia
AHLVD in Australia




Infected farm (above) and healthy farm (right)
AHLVD: Histology 1
• Light microscopic observations
  – The main pathological change is ganglioneuritis
    with lesions prominent in cerebral and pedal
    ganglia
  – Lesions characterized by nerve tissue necrosis
    accompanied by hemocytosis in some nerve
    tissue
    • In nerves under mucosa of esophagus and intestine
  – No Cowdry type A inclusions were observed
  – However neuronal cells may contain marginated
    chromatin
AHLVD: Histology 2
 (Australia + Taiwan)
Normal vs GNV Nerves
AHLVD: TEM 1
• Transmission electron microscopic (TEM)
  observations
  – Spherical, enveloped virus (~100nm) with
    icosahedral (hexagonal) nucleocapid and dense
    core
  – Naked virions observed in nucleus and particles
    with smooth envelope in cytoplasm
  – Negative-contrast electron microscopy also reveals
    hexagonal particles with single, smooth envelope
    (~100nm)
AHLVD: TEM 2




Australia

                   Taiwan
AHLV: experimental transmission
                        Cumulative mortality in abalone

              100


               80

                                                                     Co-habitation
% mortality




               60                                                    Fresh virus injected
                                                                     Frozen virus injected

               40                                                    DMEM injected
                                                                     Untreated

               20


                0
                    1      2          3          4           5   6
                               Days post-exposure to virus
AHLV: experimental transmission 2
                        Cumulative mortality in abalone exposed to virus
                                        infected water

              100


              80                                                              Co-habitation
                                                                              100% water
% mortality




              60                                                              10% water
                                                                              1% water
              40                                                              0.01% water
                                                                              0.001% water

              20                                                              Untreated control



               0
                    1    3   5   7   9   11   13   15     17   19   21   23
                                     Days post-exposure
AHLV: Summary
• Rapid onset of mortalities occur with these disease
  leading to high levels of mortality
• Transmission experiments indicate virus is highly
  pathogenic
• AHLV spread rapidly in both Taiwan and Australia
  including human caused (spread in farms and
  processing plants) and nature (water movement)
• Molecular methods will help us better understand the
  similarities between the virus in Taiwan and Australia
  as well as earlier reports in China
Treatment and Control of Viruses
• No treatment available
• Strict Farm and processing plant hygiene
  (mainly abalone)
• Health examination prior to importation and
  quarantine to assess sub-clinical infections

• How do you think this should be done?

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7 viral diseases of molluscs 2012 for baja symposium 1

  • 1. Herpesviruses of Molluscs Carolyn Friedman • Herpesvirus infections have been detected in many mollusc species in association with mortality outbreaks, including Crassostrea virginica C. gigas Ostrea edulis O. angasi O. chilensis Ruditapes decussatus R. phillipinarum Pecten maximus Haliotis diversicolor supertexa Haliotis laevigata Haliotis rubra
  • 2. Global distribution of OsHV OsHV infections
  • 3. OsHV-1 OsHV-1 • Icosahedral DNA virus, replicates in nucleus and migrates to cytoplasm (enveloped by nuclear membrane) • OsHV-1 in France has been characterized – Virions have been purified, described, and sequenced • The genome is 207 kb From: Davison et al. 2005 – Sequence comparisons showed that OsHV-1 is tenuously related to vertebrate herpesviruses
  • 4. Herpesvirus evolutionary tree FISH AND TERRESTRIAL AMPHIBIANS VERTEBRATES OYSTERS
  • 5. Oyster herpesviruses (OsHV) • Mortalities are typically short in duration and can reach up to 90% (in larvae) and 40-80% (in seed) – Mortalities particularly affect small and/or fast growing seed oysters • Virus also detected in multiple adult species where mortality not recorded • Associated with warm water temperatures and high densities of animals – 24-25 C needed for virion replication based on lab experiments in larvae – 24-25 C also associated with field mortalities of seed oysters
  • 6. Possible modes of transmission • In hatcheries, vertical transmission has been suggested • In the field, at least in Tomales Bay, uninfected seed oysters are outplanted each year – OsHV has not been detected in any hatcheries or nurseries to date in the US – Adult bivalves in the bay may have latent infections • In lab – cannot transmit to stages older than larvae
  • 7. OsHV Transmission in Tomales Bay Mortality Max Mean Dection of OsHV 100 30 90 80 25 70 20 60 50 15 40 30 10 20 5 10 0 0 5/17- 6/4- 6/17- 7/2- 7/16- 7/30 8/13- 8/28- Cum. 6/3 6/16 7/1 7/15 7/29 -8/12 8/27 9/9
  • 8. OsHV Transmission in larvae 100 90 80 70 Percent Survival 60 50 40 30 20 10 0 1 3 5 7 9 Experiment Day
  • 9. OsHV Diagnostic Methods 4d • Light microscopy – Nuclear hypertrophy and chromatin margination • Cells of the gills, mantle, and velum (not epithelial cells) • Signs of viral-induced apoptosis – Slight or no inflammatory 4b response around infected cells – Changes often described in larvae but not juvenile or adult oysters
  • 10. OsHV Diagnostic Methods 2 • In situ hybridization – Section through the visceral ganglion. – Labelled cells (arrowheads) and non- labelled cells (arrows). – The DIG-labelled probe reacts strongly within the cytoplasm and the nucleus of nervous cells (bar=10 um).
  • 11. OsHV Diagnostic Methods 3 • Transmission Electron Microscopy (TEM) – Presence of spherical to polygonal unenveloped particles ~80 nm in diameter in nucleus of infected larvae and spat – Enveloped virions ~122 nm in cytoplasmic vesicles, perinuclear space & extrcellularly
  • 13. OsHV Diagnosis Methods 5 • Multiple conventional and QPCR primer sets have been designed to amplify regions of the OsHV-1 genome • PCR allows for both diagnosis of OsHV and the comparison of possible OsHV variants A) UL X US TRL IRL IRS TRS B) C C A GP B
  • 14. Global distribution of OsHV OsHV infections PCR as diagnostic tool
  • 15. OsHV research in our lab • Improving survival of seed oysters in the field • OsHV transmission in larval and seed oysters – may include the addition of Vibrio tubiashii in transmission experiments • Comparison of global OsHV variants • Testing histology blocks from early Tomales Bay mortalities as well as imports into TB from other parts of the world • Developed 2 qPCR assays – One DNA-based and one RNA-based
  • 16. OsHV µ-var 1 • In 2008- high mortality rates of 80% to 100% in Crassostrea gigas – Mainly juvenile oysters from May to September • 75% positive batches for OsHV-1 – ?new biotype of OsHV-1? • Extracts of field affected oysters  induced mortalities (80% IM, 40% cohabitation) in spat and juvenile oysters – qPCR and TEM confirmed viral infection • 0.1μm filtration or UV inactivated OsHV µvar
  • 17. OsHV µ-var • “Both biotypes identified in isolates, OsHV1 and OsHV1 μVar*, were virulent and generated mortality with the oyster stages used” • “the first time that such results trial were obtained” • “Analysis of various target sequences within viral genome present in infected batches demonstrated the presence of polymorphism”  OsHV1 μVar and patented finding • From Sauvage et al. 2009
  • 18. Specific questions Could you tell me what do you do when detect a positive sample to OsHV-1? Do you have an estimation about the losses when an episode of OsHV-1 occurs? Is there any governmental regulation to avoid dispersion of OsHV-1? Do you have a surveillance program for OsHV-1 in oyster farms or environment? If yes, how is it?
  • 19. If we detect a new positive sample (ie in a new location), we repeat our analysis, add sequence analysis and in situ hybridization to confirm infection The losses due to a herpes outbreak in Tomales Bay can certainly be greater than 90%, at least in patches. Regarding regulations, OsHV is not on our list of diseases that California regulates. It probably will be added next time we make changes, but that will be more than a year from now. However, we still can use more broad, open-ended regulations to restrict movement of infected product or seed.
  • 20. . I was hoping to get the OsHV-1 RT PCR assay going in my lab this summer and we got most of the way there but have not had time to set up the proper standards yet for quantification. I hope to be completely setup by next Spring to conduct regular testing and do some experiments. Also want to get OsHV uvar testing. So currently there is no proper surveillance program for OsHV-1 but I expect there will be by next year. We will examine oysters from the growing areas listed above as well as from naturalized C. gigas in numerous southern California harbors and bays.
  • 21. To my knowledge OsHV has only been detected in Tomales Bay and Drakes Bay. The growers in these areas will not send seed to other growing areas. Actually, all of the seed or larvae that enters the state's growing areas- Carlsbad Lagoon, Santa Barbara, Morro Bay, Tomales Bay, Drakes Bay and Humboldt Bay- comes either from Taylor in Washington (or Hawaii), Coast in Washington (or Hawaii), Whiskey Creek in Oregon, Hawaiian Shellfish in Hilo, or from Humboldt Bay to the other growing areas
  • 22. Abalone herpesvirus disease • Known affected species - to date, primarily observed in – Taiwan beginning in 2003, detected 2003-2005 • both subspecies of Haliotis diversicolor (aquatilis and supertexta) – Australia beginning in December 2005/January 2006 • Haliotis laevegata • H. rubra • hybrids of H. laevegata x H. rubra • Losses typically occur when water temperatures are <22C and often range from 16-19C
  • 23. The first abalone farm infected with herpes-like virus Gross observations of ALVD •Tank water turbid and frothy (above) from regurgitated food particles and mucus in water in Taiwan •Rapid onset of mortality in tanks, ponds, or wild populations • No visible change in abalone feeding habits prior to onset
  • 24. Clinical signs: Holiotis diversicolor supertexta Tank water was turbid and bubbly. Healthy vs. moribund abalone
  • 25. AHLVD: Gross observations • Affected abalone with clinical signs varying from none to – Stiff pedal muscle with darkened lateral mantle – Increased mucus production reported in many cases – And may present swollen, prolapsed mouth with everted radula in some cases (noted in Australian abalone species) – Mortalities typically observed within 3 days of onset of clinical signs, and dead abalone may remain adhered to substrata – Losses often complete within 9-14d
  • 26. AHLVD: Gross Signs Australia
  • 27. AHLVD in Australia Infected farm (above) and healthy farm (right)
  • 28. AHLVD: Histology 1 • Light microscopic observations – The main pathological change is ganglioneuritis with lesions prominent in cerebral and pedal ganglia – Lesions characterized by nerve tissue necrosis accompanied by hemocytosis in some nerve tissue • In nerves under mucosa of esophagus and intestine – No Cowdry type A inclusions were observed – However neuronal cells may contain marginated chromatin
  • 29. AHLVD: Histology 2 (Australia + Taiwan)
  • 30. Normal vs GNV Nerves
  • 31. AHLVD: TEM 1 • Transmission electron microscopic (TEM) observations – Spherical, enveloped virus (~100nm) with icosahedral (hexagonal) nucleocapid and dense core – Naked virions observed in nucleus and particles with smooth envelope in cytoplasm – Negative-contrast electron microscopy also reveals hexagonal particles with single, smooth envelope (~100nm)
  • 33. AHLV: experimental transmission Cumulative mortality in abalone 100 80 Co-habitation % mortality 60 Fresh virus injected Frozen virus injected 40 DMEM injected Untreated 20 0 1 2 3 4 5 6 Days post-exposure to virus
  • 34. AHLV: experimental transmission 2 Cumulative mortality in abalone exposed to virus infected water 100 80 Co-habitation 100% water % mortality 60 10% water 1% water 40 0.01% water 0.001% water 20 Untreated control 0 1 3 5 7 9 11 13 15 17 19 21 23 Days post-exposure
  • 35. AHLV: Summary • Rapid onset of mortalities occur with these disease leading to high levels of mortality • Transmission experiments indicate virus is highly pathogenic • AHLV spread rapidly in both Taiwan and Australia including human caused (spread in farms and processing plants) and nature (water movement) • Molecular methods will help us better understand the similarities between the virus in Taiwan and Australia as well as earlier reports in China
  • 36. Treatment and Control of Viruses • No treatment available • Strict Farm and processing plant hygiene (mainly abalone) • Health examination prior to importation and quarantine to assess sub-clinical infections • How do you think this should be done?