CN1410533A - Large brill rhabdo virus toxic strain and its preparation method and application - Google Patents
Large brill rhabdo virus toxic strain and its preparation method and application Download PDFInfo
- Publication number
- CN1410533A CN1410533A CN 02139281 CN02139281A CN1410533A CN 1410533 A CN1410533 A CN 1410533A CN 02139281 CN02139281 CN 02139281 CN 02139281 A CN02139281 A CN 02139281A CN 1410533 A CN1410533 A CN 1410533A
- Authority
- CN
- China
- Prior art keywords
- rhabdovirus
- turbot
- strain
- fish
- cell
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Pending
Links
Images
Landscapes
- Micro-Organisms Or Cultivation Processes Thereof (AREA)
Abstract
A Scophthalmus maximus rahbdovirus (SMRV0207, CCTCC No.202006) is prepared through sampling the liver, kidney, heart and spleen tissues from the scophthalmus maximus in ill, shearing, adding PBS, homogenizing, adding double antibody, freezing, thawing, centrifugal extracting, filtering, inoculating it to CLC 0207 cell, and constant-temp. continuous culture. Its advantages are high reproduction speed, and high reproduction valency up to 10 to the power 8 TCID 50/ml. It can be used to prepare vaccine.
Description
Technical field
The present invention relates to aquatic animal disease cause of disease and separation, vitro culture and authenticate technology, particularly the in-vitro multiplication of sea farming fish virus, detection diagnostic techniques.More specifically relate to a kind of Da Ling Maximus rhabdovirus strain, the preparation method who also relates to a kind of turbot rhabdovirus strain also relates to a kind of biological method simultaneously and is identifying seawater fish rhabdovirus and the sea water fish rhabdovirus purposes in the cell engineering vaccine preparation.
Background technology
(Scophthalmus maximus is the Pleuronectiformes seawater fish of dwelling at the bottom of a kind of cold water that originates in Europe turbour) to Da Ling Maximus, also is local famous sea farming breeding.Because the smooth delicacy of turbot mouthfeel and deliciousness, spur are few, no off-flavors, fin limit and subcutaneous abundant colloid arranged can be compared U.S. with soft-shelled turtle with sea cucumber, be that ideal keeps healthy and beauty food.Turbot personality docility, there is not mutual residual phenomenon, and growth is rapidly, acceptant mixed feed, and the food efficiency of conversion was up to 1: 1, be easy to characteristics such as intensive culture, be subjected to the great attention of international mariculture industry, and the peculiar figure of flatfish is arranged, in water body, can build colourful, the appreciation effect that light butterfly is danced exquisitely becomes the upstart of whole world culture fishery rapidly.China introduced a fine variety the beginning of the nineties, and under the batch production condition, the fry of 5cm was cultured 1 year at present, and body weight can reach 800-1000g.But with the expansion of the scale of breed, the disease of turbot also becomes increasingly conspicuous, especially viral disease [Angulo etc., 1994, the J.Fish Dis.17:163-169 that causes; Breton etc., 1997, J.Fish Dis, 20:145-152], become the restraining factors of turbot aquaculture development.
The turbot virus disease is by the bait throwing in horizontal transmission a bit, as viral nervous necrosis [Breton etc., 1997] and infectious pancreatic necrosis [Mortensen etc., 1995, J World Aqacul.Soci.26:217-219].Some disease directly contacts by water body or with ill fish and propagates.Also have a kind of spherical virus particle, the hemocyte of directtissima turbot causes fish body anoxic [Lamas etc., 1995, J.Fish Dis, 18:425-433] by influencing erythrocytic function.Cultivation density increases, and propagating for the turbot virus disease provides more opportunity.
Known hydrocoles rhabdovirus majority is the strong pathogenic agent of fish, is the pathogenic agent of fish septicemia as viral septicemia virus (VHSV), and they can cause the fatal disease that host animal is serious, and morbidity host mortality ratio in 1 week can reach 100%.Also have barracuda rhabdovirus (pike fry rhabdovirus), snakehead fish rhabdovirus (snakehead rhabdovirus), SVCV (spring viremia of carp), the beautiful fish rhabdovirus of Bluepoint (Rio grande cichlid rhabdovirus) and perch rhabdovirus (perch rhabdovirus) multiple in addition.These rhabdoviruses can both cause fish morbidity and dead, cause heavy economic big loss.Therefore, set up corresponding method, the turbot virus causing disease is separated, especially the fulminant disease that causes of rhabdovirus is identified, can set up corresponding early diagnosis technology, and understand its fashion trend, in conjunction with the corresponding virus vaccines of development, thereby can play effective monitoring and prophylactic effect to its propagation.
Summary of the invention
The object of the present invention is to provide a kind of turbot rhabdovirus strain, turbot rhabdovirus strain is at CLC
0207High efficiently multiplying in the cell, propagation is tired and can be reached 10
8TCID
50/ ml.
Another object of the present invention also relates to a kind of preparation method who prepares turbot rhabdovirus strain, this method is simple, and can be external a large amount of amplification flounder rhabdoviruses, and the fish body infection experiment condition that has solved turbot virus is difficult to control, the cost height, the problem of poor repeatability.
The invention still further relates to the application of a kind of turbot rhabdovirus strain in biological method evaluation seawater fish rhabdovirus.
The invention still further relates to the application of a kind of turbot rhabdovirus strain in kinds of fish Rhabdovirus detection accurately and effectively and diagnosis.
The invention still further relates to the application of a kind of turbot rhabdovirus strain in the preparation of sea water fish rhabdovirus cell engineering vaccine.
In order to achieve the above object, the present invention is by the following technical solutions:
From the Da Ling Maximus that suffers from fatal disease, be separated to a strain rhabdovirus, be called turbot rhabdovirus (Scophthalmus maximus rahbdovirus, SMRV
0207), CCTCC NO:V202006 proves that through the inoculation experiments to multiple fish cell this virus can cause that host cell produces the cracking performance pathology.This is the wider kinds of fish Rhabdovirus cause of disease of a kind of host range.Virus disease with other animal is the same, does not still have medicine so far and can effectively control them, have only by virus vaccines carry out immunity by way of, just for the prevention virus disease, keep the turbot healthy aquaculture to show hope.
The illness of ill turbot is to have occurred many vesicles and blutpunkte on body surface, skin, and liver has the irregular piebald of the depth, the nephridial tissue erosion, and body surface diseases occurs 24 hours, and sick fish will be dead.Get the organization material of disease fish, be prepared into tissue homogenate, be inoculated in the sensitive cells, carry out the separation and Culture of virus; Or the organization material of getting the disease fish directly with glutaraldehyde fixing after, the preparation ultrathin section(ing) is used for electron microscopic observation.
To SMRV
0207Infect CLC
0207The ultrathin section(ing) of cell carries out electron microscopic observation, show consistently with viewed situation in ill turbot cell, turbot rhabdovirus morphological specificity is: it is that 110-150 * 40-60nm, form are the rhabdoviruses of an end tip, the other end tack that a lot of sizes are arranged in the cell.
As material, vitro culture and evaluation have been carried out with ill or dying big water chestnut Maximus tissue from different aspects to wherein rhabdovirus.Comprise:
After A, ill turbot tissue preparation become homogenate, infect different fish cells, clear and definite CLC
0207Cell is to SMRV
0207Sensitivity can produce the pathology spot behind the virus inoculation, and SMRV
0207Virus strain is at CLC
0207Propagation in the cell is tired and can be reached 10
8TCID
50/ ml.
The directly fixing fresh sick fish tissue sample of B carries out ultramicroscopic view and examines after ultrathin section(ing), dyeing, size, the form of clear and definite virus and cause the ultra micro pathological change of host cell.
Description of drawings
Fig. 1, turbot rhabdovirus SMRV
0207The ultra micro form, showing a large amount of sizes among the figure is that 110-150 * 40-60nm, form are the rhabdoviruses of an end tip, the other end tack.x30000
Fig. 2, (A), normal CLC
0207Cell and (B), infect SMRV
0207, and the CLC of pathology appears
0207The cell Photomicrograph.x40
Fig. 3, SMRV
0207Infect CLC
0207Cavity appears in the electromicroscopic photograph of cell in the cells infected.x4000
Embodiment
Vessel equipment, substratum, the reagent of the cell cultures that is useful on and virus amplification all require in advance to keep aseptic through processing such as autoclaving or filtration sterilizations.The compound method of part common agents is as follows:
Phosphate buffered saline buffer (PBS, no Ca
++, Mg
++):
NaCl 8.00g
KCl 0.20g
Na
2HPO
4 2.31g
KH
2PO
4 0.31g
Be dissolved in the 500ml distilled water, add 5ml 0.4% phenol red liquid, add distilled water to 1000ml after stirring.10 pounds of sterilizations in 15 minutes are standby.
Two anti-(penicillin, Streptomycin sulphate) solution
With 10
6Unit penicillin G and 10
6μ g Streptomycin sulphate is dissolved in the tri-distilled water of 100ml sterilization, makes every ml penicillin 10
4Unit, Streptomycin sulphate 10
4μ g.
The TC119 substratum
To purchase next TC199 substratum pulvis, the amount that by specification requires adds with fresh tri-distilled water dilution, fully the dissolving back adds serum (10% new-born calf serum), two anti-, and adds the light sodium solution of carbonic acid and regulate pH to 7.2-7.4, use the tri-distilled water constant volume again after, filter packing through filter.
The operation steps of virus inoculation and amplification:
After the liver of ill turbot, kidney, the heart, spleen tissue taken out, the PBS that shreds, adds 1-2 times of volume carried out homogenate, adds two anti-again, put refrigerator-20 ℃ freezing spending the night, take out next day treat that it melts after, with 1000-2000 rev/min speed centrifugal 10 minutes, obtain SMRV
0207The virus crude extract.With the SMRV for preparing
0207The virus crude extract is inoculated into the CLC that has grown up to individual layer respectively after filtering
0207In the cell.Be provided with the contrast of corresponding normal cell simultaneously, and to put temperature be to continue to cultivate in 20 ℃ the constant incubator.Utilize opticmicroscope, regularly observe having inoculated viral active somatic cell, and make comparisons with corresponding normal cell.
Behind the virus inoculation 12-24 hour, under inverted microscope, can see: at fine and close originally CLC
0207In the cell monolayer, the pathology spot successively occurred, beginning is the dispersive small amounts of cells formed little cavity that comes off, and the cavity increases (Fig. 2) gradually.To at this moment the section got, SMRV
0207The electron microscopic sample of cells infected preparation is observed, and show that the mandarin fish rhabdovirus breeds in a large number in host cell, and tangible pathology (Fig. 3) has appearred in cell.The cell that does not come off as yet in the cell monolayer forms netted subsequently.
Claims (6)
1, a kind of turbot rhabdovirus strain is characterized in that big water chestnut rhabdovirus strain Scophthalmus maximusrahbdovirus, SMRV
0207, CCTCC NO:V202006.
2, a kind of turbot rhabdovirus strain according to claim 1 is characterized in that Da Ling Maximus rhabdovirus is: size is the rhabdovirus of an end tip, the other end tack for 110-150 * 40-60nm, form.
3, a kind of preparation method who realizes the described a kind of turbot rhabdovirus strain of claim 1, after it is characterized in that the liver of ill turbot, kidney, the heart, spleen tissue taken out, the PBS that shreds, adds 1-2 times of volume carries out homogenate, add two anti-again, it is ℃ freezing to put refrigerator-20, after take out melting, with 1000-2000 rev/min speed centrifugal 10 minutes, obtain SMRV
0207The virus crude extract is with SMRV
0207The virus crude extract is inoculated into the CLC that has grown up to individual layer respectively after filtering
0207In the cell, temperature is to continue in 20 ℃ the constant incubator to cultivate.
4, the application of the described a kind of turbot rhabdovirus strain of claim 1 in biological method evaluation seawater fish rhabdovirus.
5, the application of the described a kind of turbot rhabdovirus strain of claim 1 in kinds of fish Rhabdovirus detects and diagnoses.
6, the application of the described a kind of turbot rhabdovirus strain of claim 1 in the preparation of sea water fish rhabdovirus cell engineering vaccine.
Priority Applications (2)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN 02139281 CN1410533A (en) | 2002-11-14 | 2002-11-14 | Large brill rhabdo virus toxic strain and its preparation method and application |
| CN 200310116250 CN1239697C (en) | 2002-11-14 | 2003-11-13 | Large brill rhabdo virus toxic strain and its preparation method and application |
Applications Claiming Priority (1)
| Application Number | Priority Date | Filing Date | Title |
|---|---|---|---|
| CN 02139281 CN1410533A (en) | 2002-11-14 | 2002-11-14 | Large brill rhabdo virus toxic strain and its preparation method and application |
Publications (1)
| Publication Number | Publication Date |
|---|---|
| CN1410533A true CN1410533A (en) | 2003-04-16 |
Family
ID=4750001
Family Applications (1)
| Application Number | Title | Priority Date | Filing Date |
|---|---|---|---|
| CN 02139281 Pending CN1410533A (en) | 2002-11-14 | 2002-11-14 | Large brill rhabdo virus toxic strain and its preparation method and application |
Country Status (1)
| Country | Link |
|---|---|
| CN (1) | CN1410533A (en) |
Cited By (2)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN102154176A (en) * | 2011-01-25 | 2011-08-17 | 国家***第一海洋研究所 | Turbot pathogenic strain and inactivated vaccine for ascites disease |
| CN108251384A (en) * | 2017-12-13 | 2018-07-06 | 中国水产科学研究院珠江水产研究所 | One plant of kinds of fish Rhabdovirus attenuated vaccine strain |
-
2002
- 2002-11-14 CN CN 02139281 patent/CN1410533A/en active Pending
Cited By (4)
| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| CN102154176A (en) * | 2011-01-25 | 2011-08-17 | 国家***第一海洋研究所 | Turbot pathogenic strain and inactivated vaccine for ascites disease |
| CN102154176B (en) * | 2011-01-25 | 2012-07-04 | 国家***第一海洋研究所 | Turbot pathogenic strain and inactivated vaccine for ascites disease |
| CN108251384A (en) * | 2017-12-13 | 2018-07-06 | 中国水产科学研究院珠江水产研究所 | One plant of kinds of fish Rhabdovirus attenuated vaccine strain |
| CN108251384B (en) * | 2017-12-13 | 2021-06-15 | 中国水产科学研究院珠江水产研究所 | Fish rhabdovirus attenuated vaccine strain |
Similar Documents
| Publication | Publication Date | Title |
|---|---|---|
| Smith | Insect virology | |
| CN101491228A (en) | Sea no-nucleus pearl incubation method | |
| CN113832035B (en) | Method for inducing aschersonia oligosporus to produce predatory organs by using extracellular vesicles secreted by caenorhabditis elegans | |
| Wagge | Amoebocytes | |
| CN110283777B (en) | Continuous culture method for prawn cells | |
| CN110684709B (en) | Haliotis discus hannai cell culture medium and cell line construction method | |
| CN109971700B (en) | Culture method of primary gill cells of takifugu obscurus | |
| CN1410533A (en) | Large brill rhabdo virus toxic strain and its preparation method and application | |
| Sung et al. | Effect of lipopolysaccharide on in vitro phagocytosis by hemocytes from giant freshwater prawn (Macrobrachium rosenbergii) | |
| Smyth | Cestoda | |
| Meyer | The" bacterial symbiosis" in the concretion deposits of certain operculate land mollusks of the families Cyclostomatidae and Annulariidae | |
| CN1239697C (en) | Large brill rhabdo virus toxic strain and its preparation method and application | |
| CN110713969A (en) | Blue crab blood cell grouping culture method | |
| CN110684718B (en) | Method for efficiently separating and culturing primary hepatocytes of fugu obscurus | |
| Elston et al. | Isolation and in vitro characteristics of chinook salmon (Oncorhynchus tshawytscha) rosette agent | |
| CN1410535A (en) | Mandarin fish rhabdo virus toxic strain, its preparation method and application | |
| CN109792972B (en) | In-vitro culture method for cysticercus cellulosae | |
| Bbockelman et al. | Rhabditis maupasi: occurrence in food snails and cultivation | |
| CN112795484A (en) | Method for extracting and separating exosome of cryptocaryon irritans of marine parasitic ciliates and application of exosome | |
| CN1239696C (en) | Lefteye flounder lymph tumour virus toxic strain, its preparation method and application | |
| Parvez et al. | Studies on the ontogenic development of a high-valued tropical sea urchin, tripneustes gratilla (Linnaeus, 1758) for seed production and commercial aquaculture | |
| Howitt | The cultivation of Endamoeba gingivalis (Gros) | |
| Liwen et al. | Long-term in-vitro culture and subculture of the hemocytes of swimming crab Portunus trituberculatus | |
| Newport et al. | Miracidia infective for snails derived from eggs laid by adult Schistosoma mansoni in vitro | |
| CN1322119C (en) | Mandarin fish rhabdo virus toxic strain, its preparation method and application |
Legal Events
| Date | Code | Title | Description |
|---|---|---|---|
| C06 | Publication | ||
| PB01 | Publication | ||
| C10 | Entry into substantive examination | ||
| SE01 | Entry into force of request for substantive examination | ||
| C02 | Deemed withdrawal of patent application after publication (patent law 2001) | ||
| WD01 | Invention patent application deemed withdrawn after publication |