Fish necropsy & Sample collection for TiLV diagnosis · Slide B: Fish Necropsy 1. Preparation of...

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Fish necropsy & Sample collection for TiLV diagnosis 1 Session 2 Ha Thanh Dong 1,2 1 King Mongkut’s University of Technology Thonburi, 2 Fish Health Platform, Centex Shrimp (Mahidol University/BIOTEC),Thailand.

Transcript of Fish necropsy & Sample collection for TiLV diagnosis · Slide B: Fish Necropsy 1. Preparation of...

Page 1: Fish necropsy & Sample collection for TiLV diagnosis · Slide B: Fish Necropsy 1. Preparation of scissor, forceps, tray, tissue paper for dissection 2. Terminate the fish by an overdose

Fish necropsy & Sample collection

for TiLV diagnosis

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Session 2

Ha Thanh Dong1,2

1King Mongkut’s University of Technology Thonburi, 2Fish Health

Platform, Centex Shrimp (Mahidol University/BIOTEC),Thailand.

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Objectives

• To be able to understand

❖What are target tissues of TiLV?

❖How to necropsy and collect samples?

❖How to preserve tissues for histology?

❖How to preserve tissues for PCR?

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What are target tissues of TiLV?

• Liver

• Kidney

• Spleen

• Brain

• Gills

• Muscle

• Blood

• Mucus

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What is the best

tissue for

histopathology and PCR diagnosis?

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How to necropsy and collect samples?

Record basic information

Collect fish samples

Collect samples for TiLV diagnosis

(non-destructive & destructive)

Preserve samples for histology & PCR

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What need to be recorded?

• General information of fish farm

• Fish species, sizes, source

• Environmental parameters

• Disease history

• Clinical signs (both external and internal),

abnormal behaviors (plus pictures, video)

• Mortality rate

• Others

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Sample collection

Non-Destructive sampling• Feces

• Gill filaments

• Blood

• Mucus

• Fins

• Liver biopsy

Destructive sampling

• Whole fish (for small fish such as fry, fingerlings)

• Some parts of the body (liver, spleen, kidney, gills, etc.)

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Non-destructive sampling(Broodstock or ornamental fish)

Cut 2-3 filaments or

collect mucus using a cotton swab

Blood collection

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Destructive sampling for TiLV diagnosis

Small fish

(< 2 g)

Preserve whole

fish (Slide A)

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Large fish

Necropsy (Slide B)

Liver, Kidney, Brain

Preserve (Slide C)

Note: Liver, kidney and brain are recommended organs for

TiLV diagnosis. However, other organs such as gills, spleen, muscle, mucus, etc. maybe possible for diagnosis as well.

Page 9: Fish necropsy & Sample collection for TiLV diagnosis · Slide B: Fish Necropsy 1. Preparation of scissor, forceps, tray, tissue paper for dissection 2. Terminate the fish by an overdose

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Open fish belly before preserving

Slide A: Preservation

Small fish < 2 g (open fish belly if possible)

For PCR or histology

Page 10: Fish necropsy & Sample collection for TiLV diagnosis · Slide B: Fish Necropsy 1. Preparation of scissor, forceps, tray, tissue paper for dissection 2. Terminate the fish by an overdose

Slide B: Fish Necropsy

1. Preparation of scissor, forceps, tray,

tissue paper for dissection

2. Terminate the fish by an overdose

of clove oil (≥100 ppm) or ice

3. Disinfect the fish body surface with

alcohol 70%

4. Dissect the fish (see picture below)

5. Collect target tissues for different

purpose (histology, molecular

analysis, TEM or virus isolation)

add clove oil into water

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Slide B: Fish Necropsy

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Slide B: Fish Necropsy

How to dissect a fish?

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Slide B: Fish Necropsy

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How to dissect a fish?

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Slide B: Fish Necropsy

Clinically healthy tilapia

Where are target tissues for TiLV?

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head kidney

heartliver spleen

posterior kidney

trunk kidney

intestine

gills

Slide B: Fish Necropsy

How to collect kidney?

Clinically sick tilapia

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head kidney

spleenheart Liver(TiLV target)

Kidney

Slide B: Fish Necropsy

How to collect brain?

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gills

Clinically sick tilapia

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Slide C: Preservation

Purpose Procedures

Histology • Fix in 10% neutral buffered formalin for

24h (sample: fixative, 1:10 (v/v)), then

change to alcohol 70% for long-termpreservation

Molecular analysis

(PCR, RT-PCR, qPCR)• Alcohol 95% (sample: fixative, 1:10

(v/v))

• Trizol or RNA later (sample: fixative,

1:10 (v/v))• Fresh sample, frozen sample

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head kidney

liver

spleen

gill

posterior kidney

heart

Slide C: Preservation

• For histology, all organs can be

preserved in the same tube/

bottle

• For PCR, preserve individually

or pool together

• Size of tissue: ~1 x 1 cm

Samples in alcohol 95% for PCRSamples in 10% NBF

for histology

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Frozen

Slide C: Preservation

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• Frozen samples can be used for

PCR or viral isolation

• Deep frozen (-80 oC) is

recommended if you aims for viral

isolation

• -20 or -40 oC is sometimes

acceptable if no -80 oC refrigerator

available

• Deep frozen is useful for

retrospective study

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Paraffin blocks

Slide C: Preservation

• Paraffin blocks can be preserved for many years for

histology and ISH

• Useful for retrospective study

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10% neutral buffered formalin (NBF)

Sodium phosphate, monobasic 4.0 gm

Sodium phosphate, dibasic 6.5 gm

Formaldehyde, 37-40% 100.0 ml

Distilled water 900.0 ml

Mix well

Label and date.

Sample preservation for histology

• Sample : NBF ratio 1:10 (v/v), keep at room temp.

• After 24 h, change to alcohol 70% ratio 1:10 (v/v) for long-

term preservation, keep at room temp.

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What should be avoided• Dead fish → post mortem change

• Dissection takes too long time → autolysis

• Contamination

• Physical destruction of tissue → not good for histology

• Tissue pieces are too big

• Fixative is not enough

• Sample in formalin 10% for too long → not good for ISH

22good size for preservation

1 cmNot enough fixative

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Example

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Normal liver(standard preparation)

Poor fixing/post mortem change

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Discussion

Question: If an unexplained mortality occurs

in fish farm, how to preserve samples for

later diagnosis/investigation?

Answer:

1……………..

2……………..

3……………..

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Thank you for your attention!

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