Veterinary composition of marine algae and andrographis sp extracts, which can be used to treat infe

专利摘要:
Veterinary composition comprising an extract of seaweed containing at least 5% fucoidians and an Andrographis sp plant extract containing at least 5% of andrographolide, which is useful in the control and prevention of infections produced by intracellular microorganisms in fishes.
公开号:DK201770757A1
申请号:DKP201770757
申请日:2017-10-06
公开日:2017-10-23
发明作者:Paula Miranda Campos；Claudio Rabuco Jeraldino
申请人:Maqui New Life S A；
IPC主号:

专利说明:

VETERINARY COMPOSITION OF MARINE ALGAE AND ANDROGRAPHIS SR EXTRACTS, WHICH CAN BE USED TO TREAT INFECTIONS IN FISH
FIELD OF INVENTION
The present invention is directed to a veterinary composition comprising seaweeds extract with a content of at least 5% of fucoids and an extract of Andrographis sp with a content of at least 5% of andrographoid, which is useful in the control and prevention of infections produced by intraceliular microorganisms in fishes.
BACKGROUND OF THE INVENTION
It has been known that the aquatic environment in which grows and cultivates fishes, favors the emergence of diseases. Many measures have been taken to control or prevent these diseases, and until now the vaccination is one of the tools more widely used for the control of bacterial diseases in fishes. This due to vaccinations shows some advantages that start from their good effectiveness in preventing and correcting infections to their low impact in the environment and in public health, allowing the obtaining of a clean product. In general, this can happen with antibiotics, and among its adverse effects can be mentioned: development of the bacterial resistance; accumulation of antibiotics in the muscle of the fish; contamination of aquatic environments among others.
Nevertheless, the vaccination has disadvantages like it requires a big manipulation of the fishes, so its practice requires being careful not to stress the fishes and doing a little bit effective the vaccination or cause mortality, also adverse effects can be shown like the existence of adherences that can lead to mortality and decrease in rates of fishes growing. In general, the diseases increase under stress conditions, and certainly, in the intensive production systems used for fish farming, those conditions are always present. We should not forget that aquaculture is the fastest growing sector in food production, being one of the major economic activities of this century and with important projections of being the main source of animal protein for human consumption in accordance with the last studies of the FAO.
The losses of production are large and the damages devastating, in the intensive system of production, when the diseases appear.
On the other hand, it is known that efficient vaccination does not exist in the prevention of some relevant intracellular pathogens, this is the case of Pisciricketssia salmonis, SAV virus, Francisella noatunensis, Renibacterium salmoninarum, IPNv, in early stages, previous to the vaccination shot. This is due to the intracellular nature of the pathogens, which requires the activation of an Th1 immune response, activating mainly cytotoxic T lymphocytes, the ones that are in charge of destroying infective cells. The combination of bioactive molecules formed by Fucoidians + Andrographolide, which causes the production of some of the macrophages of cytokines like the il_-12 and IFN, which promote the differentiation of lymphocytes ThO to Th1, this particularity in their action mechanism, transform the combination in a new tool for prevention and control of intracellular pathogens in salmonid fishes.
The diseases cause in the fishes, symptoms like erosions, warts, eruptions or spots in the skin, flap fraying, inflammation of the abdomen, erratic swimming, bleeding, injuries and ulcers in the pancreas, esophagus, muscle spasms and ascites, among others.
Between the intracellular microorganisms for fishes, we can find: pisciricketssia; viruses such as viral hemorrhage septicemia virus (VHS), infectious pancreatic necrosis virus (IPNv), infectious hematopoietic necrosis virus (IHNV), salmon alphavirus (SAV), infectious salmon anemia (ISAv), and bacteria like Francicella sp and
Renibacterium salmoninarum.
Among diseases caused by these pathogens that are important in aquaculture we can mention piscirickettsiosis, viral hemorrhage septicemia, infectious pancreatic necrosis, infectious hematopoietic necrosis, sickness of pancreas and sleeping disease, infectious salmon anemia, francisellosis and renibacteriosis.
In particular, since 1989, in the south of Chile, a disease with high mortality in salmon has been detected, called “Salmon coho syndrome”, “Huito syndrome” or piscirickettsiosis (Larenas, J.J.). ; P. Smith; L. H. Garcés; C. Lannan, J. L. Fryer. (1994) Piscirickettsiosis of Atlantic salmon (Saimo Salar) and coho salmon {Oncorhynchus kisutch) inoculated with P. salmonis. Internationa! Symposium on Aquatic Animal Health. Seattle, Washington) and which affected various species of salmonids. At the beginning it was found only in the coho salmon, but after affected all the salmonids species cultivated in Chile, causing up to a 90% mortality in some places (Branson EJ, Nieto Diaz-Munoz D. (1991). Description of a new disease condition occurring in farmed coho salmon, Oncorhynchus kisutch (Waibaum), in South America. J Fish Dis; 14: 147-156. Cvitanich JD, Garate ON, Smith CE (1991) The isolation of rickettsial organism causing disease and mortality in Chilean salmonids and its confirmation by Koch's postulate. J Fish Dis; 14: 121-145). The disease was found mainly in sea water and estuarine (Fryer JL, Lannan CN, Gårces HL, Larenas JJ, Smith PA, (1990) Isolation of a rickettsial-like organism from diseased coho salmon (Oncorhynchus kisutch) in Chile. 25: 107-114 Branson E.J., Nieto Diaz-Munoz D. (1991) Description of a new disease condition ocurring in farmed coho salmon, Oncorhynchus kisutch (Walbaum), in South America. 156; Cvitanich JD, Garate ON, Smith CE (1991) The isolation of rickettsia-like organism causing disease and mortality of Chilean salmonids and its confirmation by Koch's postulate. Journal Fish Disease; 14: 121-145) and rarely in sweet water ( Gagero A., Castro H., Sandino A.M. (1995) First isolation of Piscirickettsia salmonis from coho salmon, Oncorhynchus kisutch (Walbaum), and rainbow trout, Oncorhynchus mykiss (Walbaum), during the freshwater stage of their life cycle. Dis; 18: 277-279).
The etiologic agent corresponded to the first isolated rickettsia and characterized from aquatic animals and was called Piscirickettsia salmonis (P. salmonis). This pathogen is a mandatory intracellular parasite, cytopathic for different salmon cells! lines and some warm-water fishes. It is Gram negative, pleomorphic, usually coconut, in pairs or in ring shapes and of a size between 0.5-1.5 µm in diameter (Fryer JL, Lannan CN, Garcés HL, Larenas JJ, Smith PA (1990) isolation of a rickettsiales. like organism from diseased coho salmon {Oncorhynchus kisutch) in Chile. Fish Pathol; 25: 107-114).
The clinical signs of the piscirickettsiosis are characterized by swimming on the surface, slowly, erratically and sometimes in a corkscrew way. In addition, lethargy, anorexia, shock against the wails of the cage raft, marring and darkening have been described. The most relevant external macroscopic lesions described include: peeling, branchial pallor, equimotic and petechial bleeding at the base of the fins, nodules and ulcers in the skin up to 2 cm in diameter (Bravo, S.; Campos, M. (1989) Chile Pesquero 54: 47-48; C ubiilos V.; Farias, C.; Aiberdi, A.; Alvarado, V.; Schafer, W.; Monrås, M. (1990). Anatomopathological characteristics of coho salmon Animal Pathology 4: 14-17; Cvitanich JD, Garate ON, Smith CE (1991) The isolation of rickettsial organism causing disease and mortality in Chilean salmonids and its confirmation by Koch's postulate. Journal Fish Disease; 14: 121-145.: Larenas J., Hidaigo L., Garcés H., Fryer J.L., Smith P. (1995). Piscirickettsiosis: injuries in Atlantic salmon (Salmon salar) naturally infected with Piscirickettsia salmonis. Cienc Vet; 10: 53-58). Hematocrit levels reveal severe anemia (Branson E.J., Nieto Diaz-Munoz D. (1991). Desorption of new disease condition occuring in farmed coho salmond, Oncorhynchus kisutch (Walbaum) in South America Journal Fish Disease; 14: 147-156.).
In the analysis of necropsy of the abdominal cavity, the presence of ascites, renomegaiy and splenomegaly was found frequently, subcapsular nodules of creamy to yellowish color in the liver, the presence of a pseudomembrane over the heart and petechial bleeding in the stomach, pyloric blind , intestine, swimming bladder, muscle and visceral fat (Schafer JW; Alvarado, V.; Enriquez, R.; Monrås, M. (1990) The coho salmon syndrome (CSS): A new disease in Chilean salmon, reared in sea water 1990 Bulletin of the European Association of Fish Pathologists 10: 130; Larenas J., Hidalgo L, Garcés H., Fryer J.L., Smith P. (1995). Piscirickettsiosis: injuries in Atlantic salmon (Salmo salar) naturally infected with Piscirickettsia salmonis, by Cienc Vet; 10: 53-58). In most cases, the intestine was filled with a yellowish mucous content and the stomach with a seromucous transparent liquid (Schafer JW; Alvarado, V.; Enriquez R.; Monrås, M. (1990) The coho salmon syndrome (CSS): A new disease in Chilean salmon, reared in sea water 1990 Bulletin of the European Association of Fish Pathologist 10: 130); The laughter gives the impression that the fish has been swallowed by some water (Alvarado V.; Schafer, W.; Enriquez, R.; Monrås, M.; Cubiilos, V.; Farias, C.; Alberdi, A. (1990) Salmon Coho Syndrome (SSC), new disease of salmonids farmed in seawater phase in Chile. Present Situation. Animal Pathology.4: 10-13).
From the histopathological point of view, the main injuries were necrosis in different organs and tissues, being most affected the kidney, liver, spleen and intestine. It was also common to see vascular injuries similar to those mentioned for rickettsias in mammals, such as endothelial necrosis and thrombus formation.
In addition, macrophages containing organisms within the cytoplasm, intravascular coagulation, perivascular inflammation, pericarditis, endocarditis, chronic inflammatory injury in the layer of the intestine, increased granule cell numbers of the intestinal granular stratum and lamellar hyperplasia and fusion were found. (Cubiilos V.; Farias, C.; Alberdi, A.; Alvarado, V.; Schafer, W.; Monrås, M. (1990) Pathological characteristics of coho salmon syndrome (SSC), new disease of the salmonidae Animal Pathology 4: 14-17, Branson E.J., Nieto Diaz-Munoz D. (1991) Description of a new disease condition occurring in farmed coho salmon, Oncorhynchus kisutch (Walbaum), in South America., Journal Fish Disease; 14: 147-156. ; Larenas J., Hidalgo L., Garcés H., Fryer J.L., Smith P. (1995). Piscirikckettsiosis: injuries in Atlantic salmon (Saimo salar) naturally infected with Piscirickettsia salmonis, Av Cienc Vet, 19: 53-58).
For the diagnosis, smear and tissue staining methods are recommended with Gram, Giemsa, acridine barabha (Cvitanich JD, Garate ON, Smith CE (1991). The isolation of rickettsia-like organism causing disease and mortality in Chilean salmonids and its confirmation by Koch's postdate. Journal Fish Disease; 14: 121-145; Lannan C., Fryer, J. (1994) Extracellular survival of Piscirickettsia salmonis. Journal of Fish Diseases 17: 545-548; Office International of Epizooties, OIE. (1997) Diagnostic manual for aquatic animal diseases. Paris, Francia, OIE, pp. 161-168) (1994) and / or toludine blue (Larenas J., Hidalgo L, Garces H., Fryer JL, Smith P. (1995). Piscirickettsiosis: Injuries in Atlantic salmon (salmo salar) naturally infected with Piscirickettsia salmonis, Av Cienc Vet, 10: 53-58). These techniques are suitable for initial routine identification. The indirect immunofluorescence method (IFAT) developed by Lannan et al. (Lannan C.N., Ewing S.A., Fryer J.L. (1991)). A fluorescent antibody test for detection of rickettsia causing disease in Chilean salmonids (J Aquat Anim Health, 3: 229-234), is nowadays one of the most sensitive and specific methods for the detection of piscirickettsiosis. This technique has been modified by the use of microwaves (Larenas, J., Astorga, C., Conteras, J., G årces, H., Fryer, J.L., Smith, P. (1996) Rapid detection of Piscirickettsia salmonis using microwave irradiation. Fish Pathology 31 (4): 231-232), markedly decreasing the incubation times of the first and second antibodies, without varying the specificity and sensitivity.
Another important disease is infectious pancreatic necrosis (IPN), a disease caused by a Birnavirus that affects several wild and cultivated aquatic organisms (Reno PW. Infectious pancreatic necrosis and associated aquatic Birnaviruses. In: Woo PTK, Bruno DW, editors, Fish Diseases and Disorders. Viral, Bacterial and Fungal Infections. London: CAB I Publishing, 1999: 1-55). Salmonidae are mainly affected, so this disease has a significant impact on salmon and trout farming, due to a high mortality of offspring and fry. IPN is on the list of fish diseases of the World Organization for Animal Health (OIE) in its International Aquatic Animal Health Code and should be notified (Worid Organization for Animal Health (OIE). International Health Code for Aquatic Animals, France: OIE, 2004).
The causal agent in a virus of the birna virus family that is icosahedral in shape, approximately 60 nm in diameter (Cerini CP, Malsberger RG, Morphology of infectious pancreatic necrosis virus, Ann NY Acad Sci 1965, 126: 315-319, Dobos P. Size and structure of the genome of infectious pancreatic necrosis virus, Nucleic Acids Res 1976; 3: 1903-1924). It contains a genome composed of two double-stranded ribonucleic acid (RNA) segments. Segment A codifies for two structural proteins (VP2 and VP3) and a non-structural protease, while segment B codifies for an RNA polymerase (Dobos P. Size and structure of the genome of infectious pancreatic necrosis virus Nucleic Acids Res 1976; 3: 1903 -1924), The VP2 protein stimulates the production of neutralizing monoclonal antibodies of a specific type (Nicholson BL. Use of monocional antibodies in identification and characterization of fish viruses. Annu Rev Fish Dis 1993; 3: 241-257) and it is thought that it contains ai! epitopes recognized by these antibodies (Casweli-Reno P, Reno PW, Nicholson BL. Monocional antibodies to infectious pancreatic virus: analysis of viral epitopes and comparison of different isolates. J Gen Viroi 1986; 67: 2193-2205). iPNV penetrates through gills and mouth, or through the sensory pores of the lateral line system (Novoa B, JL Barja, A Figueras. 1995. Entry and sequentia! distribution of an aquatic birna virus in turbot (Scophthalmus maximus). Aquaculture 131, 1- 9, Chou HY, TY Peng, SJ Chang, YL Hsu, JL Wu 1999. Effect of heavy metal stressors and salinity shock on the susceptibility of grouper (Epinepheius sp.) To infectious pancreatic necrosis virus Vir Res 63, 121-129 ), The vertical transmission has been verified in rainbow trout (Oncorhychus mykiss) and brown trout (Salmo Trutta); In other species, cases have been observed associated with infected sexual eggs or fluids, which probably correspond to a vertical infection by external contamination (Reno PW. 1999. Infectious pancreatic necrosis virus and associated aquatic Birnaviruses. In "Fish Diseases and Disorders": Viral , bacterial and fungal infections (FT Woo and DW Bruno, eds., Vol. 3, CAB Publishing, Wallingford, UK, pp. 1-55) It has been proposed that vertical infection is also associated with the concentration of viral particles (Rodriguez S, JJ Borrego, SI Pérez-Prieto, 2003. Infectious pancreatic necrosis virus: biology, pathogenesis, and diagnostic methods. Adv Vir Res 62, 113-165) After a period of undetectable viremia, at four days postinfection, aproximately necrotic areas. are observed in the exocrine pancreas and other organs (Reno PW. 1999. Infectious pancreatic necrosis virus and associated aquatic Birnaviruses. in "Fish diseases and disorders": Viral, bacterial and fungal infections (PT Woo and DW Bruno, eds., Vol. 3, CAB Publishing, Wallingford, U.K., pp. 1-55); however, the viral distribution may be variable in the different organs Eléout et al. (Eléouet JF, N Druesne, S Chilmonczyk, D Momge, M Dorson, B Delmas. 2001. Comparative study of in-situ cell death induced by the viruses of viral haemorrhagic septicaemia (VHS) and infectious pancreatic necrosis (IPN) in rainbow trout. J Comp Pathol 124, 300-307) observed that the virus could be found in several organs with the exception of the pancreas, which it may be associated with a different level of tissue tropism that presents different isolates viral.
During clinical disease, mortality is inversely proportional to the age of the affected animals (Wolf K. 1988, Infectious pancreatic necrosis. In “Fish Viruses and Fish Diseases”, Cornell Univ, Press, Ithaca, NY, pp 115-157). The most characteristic disease pattern is shown in rainbow trout, brook trout, brown trout, Atlantic salmon and several species of Pacific salmon (Roberts RJ, MD Pearson, 2005. Infectious pancreatic necrosis in Atlantic salmon, Salmo salar L. J Fish Dis28, 383 -389). In offsprings that have normally completed the first feeding, the disease outbreak is usually less explosive, reaching losses of 70% or more over a period of two months. The losses in larger animals can be between 10 and 20% (Roberts RJ, MD Pearson. 2005. Infectious pancreatic necrosis in Atlantic salmon, Saimo Salar L. J Fish Dis 28, 383-389).
Generally, affected fishes show anorexia and irregular swimming (swimming in corkscrew way with ataxia lapses). These fishes change to a dark color (hyperpigmentation) and have moderate exophthalmos and abdominal distention. Gills and haemorrhages in the ventral area, the fins included, are also pale. The fishes are thin and have whiteish "hanging faeces" (Wolf K. Fish viruses and fish virus diseases. New York: Cornell University Press, Ithaca, 1988).
According to the main findings of necropsy in offspring, spleen, heart, liver and kidneys are shown pale, and most of the time no food is found in the digestive tract. Petechial haemorrhages are seen in visceras. In some cases, food is found in small amounts, confined to the distal and rectum part of the intestine. Ascitic fluid is frequently seen in the abdominal cavity. In the stomach and intestine can be observed a cohesive milky mucus, among other findings (Wolf K. Fish viruses and fish virus diseases. New York: Cornell University Press, Ithaca, 1988).
The main injuries found in the histopathological study include foci of coaguative necrosis in the pancreas, kidney and intestines. Pancreatic tissue is shown to be degenerated, even in the acinar areas, with reiease of the zymogen granules. The nuclei of the acinar cells are observed pyknotics and of variable sizes. In many cases no infiltration of inflammatory cells is shown. (McKnight i J, Roberts RJ. The pathology of infectious pancreatic necrosis. I. The sequential histopathology of the naturally occurring condition. Br Vet J 1976; 132: 76-85).
In the stomach and intestine, there are variable processes of degeneration and necrosis (Smail DA, N Bain, DW Bruno, JA King, F Thompson, DJ Pendrey, S Morrice, CO Cunningham. 2006. Infectious pancreatic necrosis virus in Atlantic salmon, Salmo salar L, post-smoits in the Shetland isles, Scotland: virus identification, histopathology, immunohistochemistry and genetic comparison with Scottish mainland isoaltes. J. Dis 29, 31-41) mucosal detachment (catarrhal enteritis) into the intestinal lumen where epithelial cells with eosinophilic and hyaline cytoplasm and swollen can be observed many times with their nucleus fragmented, making accumulations of basophilic material, distributed in ciliary periphery, showing a process of apoptosis (McKnight IJ, Roberts RJ. The pathology of infectious pancreatic necrosis. I The sequential histopathology of the naturally occurring condition (Br Vet J 1976; 132: 76-85). In the liver, it is possible to find areas of focal or generalized necrosis, which are usually severe in salmon, whereas rainbow trout are more moderate or insignificant (Roberts RJ, MD Pearson. 2005. Infectious pancreatic necrosis in Atlantic salmon, Saimo salar L. J Fish Dis28, 383-389).
The virulence, which is the relative ability of the pathogen to cause disease, is a manifestation of the interaction between the adverse effects produced by components of the virus and the defense mechanisms developed by the cells to try to eliminate the infection; however, the result of such interactivity is always determined by the virus through its virulence factors, a function that can be applied to any component of the viral particle (Lyles D, 2000. Cytophatogenesis and inhibition of host gene expression by RNA viruses. MolBiol Rev64, 709-724). The differences in the level of virulence shown between different strains of IPNV have been attributed to their genetic variation (Dobos P. 1995a. The molecular biology of infectious pancreatic necrosis virus. Annual Rev Fish Dis 5, 25-54), and with the property of the virus to modify cell signaling pathways through viral proteins encoded by its A segment, able to manipulate cellular machinery to facilitate viral synthesis and avoid the response of the defense (Hong JR, YL Hsu, JL Wu. 1999. Infectious pancreatic necrosis virus induces apoptosis due to down-regulation of survival factor MCL-1 protein expression in fish cell lines Virus Res 63, 75-83; Larsen R, TP Røkenes, B Robertsen 2004. Inhibition of infectious pancreatic necrosis virus replication by Atlantic salmon Mxi protein, J Viro! 78f 7938-7944). In this sense, the viral proteins considered as the main virulence factors of IPNV are VP2, a component of the outer cover of the viral capsid that participates in the recognition of the virus to the cells; the VP5 protein of inconclusive function, since it has been shown not to be necessary for establishing infection and the viral multiplication, but with anti-apoptotic activity that apparently has no relation in the establishment of the carrier state. Recently, it has been reported that over expression of VP3 induces apoptosis in cultured cells, but it is difficult to detect in an infection with fully viral particles. However, Vp4 and Vp1 have not been associated with adverse effects on the cellular virus, but proteins of similar activity in other viruses have been observed with implication in the pathogenicity of the strains (Lyles D. 2000. Cytopathogenesis and inhibition of host gene expression by RNA viruses Microbiol and Mol Biol Rev 64, 709-724; Liu M, VN Vakharia 2004. VP1 protein of infectious bursal disease virus modulates virulence in vivo Virol 330, 82-73; Nanda S, M Baron 2006. Rinderpest virus blocks type I and type IS interferon action: role of structural and nostructural proteins. J ViroiSO, 7555-7568).
During the infection process, the host expresses a varied response aimed at attempting to prevent infection or dissemination of the agent. For this, the non-specific defense system is the most important as a protection measure for fishes, and within this, the interferon system (IFN) is one of the first lines of defense of viral infection by inducing the synthesis of proteins having antiviral activity. ; in the case of IPNV, the Mxl protein and the kinase protein dependent on double stranded RNA (PKR) have been shown to have antiviral activity (Roberts RJ, MD Pearson. 2005. Infectious pancreatic necrosis in Atlantic salmon, Salmo saiar LJ Fish Dls28, 383-389). However, it has been reported that some viruses may inhibit or modulate the antiviral response exerted by IFN (Nanda S, M Baron. 2006. Rinderpest virus blocks type I and type II interferon action: role of structural and nonstructural proteins. J Virol 80, 7555-7568), which is also supposed for IPNV (Rodriguez S, JJ Borrego, SI Pérez-Ptieto. 2003. Infectious pancreatic necrosis virus: biology, pathogenesis, and diagnostic methods. Adv Vir Res 62, 113-165), but it has not been evaluated. IPNV shows high antigenic and genotypic variability, features that influence the virus-cell interaction, the virulence and the development of the carrier state; however, the mechanisms involved in these processes are not fully determined (Rodriguez S, JJ Borrego, SI Pérez-Prieto. 2003. Infectious pancreatic necrosis virus: biology, pathogenesis, and diagnostic methods. Adv Vir Res 62, 113-165).
The procedure for the identification of NPI, as recommended by the OiE, is based on the isolation of VNPI in ceil culture, followed by the immunological identification of the isolation by immunofluorescence tests (World Organization for Animal Health. Diagnostic Manual for Aquatic Anima! Diseases . France: OIE. 2003), serum neutralization (Lientz JC, Springer JE. Neutralization test of infectious pancreatic necrosis virus with polyvalent antiserum. J Wildl Dis 1973; 9: 120-124) and ELISA (Davis FJ, Laidler LA, Perry PW , Rossington D. Alcock R .. The detection of infectious pancreatic necrosis virus in asymptomatic carrier fish by an integrated cell culture and EUSA technique. J Fish Dis 1994; 17: 99-110).
The diagnosis of clinical cases is generally based on the histology and immunological evidence of VNPI in the infected tissues. These cases are confirmed by the isolation and immunological identification of the virus by means of such tests (World Organization for Animal Health. Diagnostic Manual for Aquatic Animal Diseases. France: OIE. 2003). Serological tests in order to identify antibodies against VNPI in infected fish have not yet been recognized by the OIE (2003), due to insufficient knowledge of the humoral immune response of the fish to this virus (Wolf K, Quimby MC. Infectious pancreatic necrosis: clinical and immune response of adult trouts to inoculation with five virus J Fish Res Board Can 1969; 26: 2511-2516).
The detection of VNPI in ceil lines is consistent and simple, mainly in lines belonging to homologous species. This is because 1) the virus is present in elevated titles in tissues; 2) The isolation can be performed from non-diseased animals; 3) there is no phase in which the virus cannot be isolated; 4) the time required for isolation and identification of the agent is from two to three weeks, which is not critical for the presentation of an epizootic, and 5) high sensitivity and cytopathic effect can be easily seen. The cell lines used for the isolation of VNPI include the RTG-2 (rainbow trout gonad), CHSE-214 (chinook salmon embryo) and BF-2 (bluegill fry) (Kelly RK, Souter BW, Miller HR. Fish cell lines: comparisons of CHSE-214, FHM, and RTG-2 in assaying IHN and IPN viruses. J Fish Res Board Can 1978; 35: 1009-1011)
Nowadays, many methods of detection have been developed by means of the technique of reverse-reaction transcription in the polymerase chain reaction (RT-PCR, by their acronyms in English: reverse transcriptase-polymerase chain reaction) (Rodriguez. S-JS, Borrego JJ, Perez-Prieto SI. Comparative evaluation of five serological methods and RT-PCR assay for the detection of IPNVin fi sh. J Virol Methods 2001; 97: 23-31). However, the sensitivity of this technique has not been greater than that of the cell culture, so that isolation of the virus and serological confirmation are the processes of choice for identifying VNPI.
On the other hand, the use of Andrographis paniculata is known in the treatment of a wide range of pathologies (Abu-Ghefreh, AA, Canatan, H. and Ezeamuzie, Cl (2008) in vitro and in vivo anti-infiammatory effects of andrographolide International Immunopharmacology, 9: 313-318); including diseases such as the common cold, dysentery, fever, tonsillitis, diarrhea, liver diseases, herpes, among others (Patarapanich, C., Laungcholatan, S., Mahaverawat, N., Chaichantipayuth, C., Pummangura, S. (2007 HPLC determination of active diterpene lactones from Andrographis paniculata Nees planted in various seasons and regions in Thailand. Thai. J. Pharm. Sci., 31: -9). It has anti-inflammatory and antimicrobial properties, (Hai, X., Gui, O., Gai, L, Jun, W. and Hong, L. (2007) Synthesis of andrographolide derivatives: A new family of α-glucosidase inhibitors. Bioorganic & Medicinal Chemistry, 15: 4247-4255), antithrombotic (Zhao, HY and Fang. WY (1991) Antithombotic effects of Andrographis paniculata again in preventing myocardial infraction. Chin, Med. J., 104 (9): 770- 5), hepaioprotective (Siripong, P., Kongkathip, B., Preechanukool, K., Picha, P., Tunsuwan, K. and Taylor, W. (1992) Cytotoxic diterpenoid constituents from Andrographis paniculata Nees leaves, J, Sci, Soc. Thailand, 18: 187-194), anti AIDS activity (Chang, RS, Oing, L, Chen, GQ, Pan, QC Zhao, ZL and Smith, KM (1991)
Dehydroandrographoiide succinic acid monoester as an inhibitor against the human immunodeficiency virus. Proc. Soc. Exp. Bite. Med., 197 (1): 59-66), antidiabetic, (Zhang, Z., Jiang, J., Yu, P.Zeng.X., Larrick, J. and Wang, Y. (2009) Hypogiycemic and beta cei protective effects of andrographoid analogues for diabetes treatment, J.of T. Medicine, 7:62) and antitumorals (Rao, S., Suseno, G., Matthews, C., Sazali, A., Haji, L, Said, Saad, M., Stevens, M. and Stanslas, J. (2007) Semisynthesis and in vitro anticancer activities of andrographoid analogues. Phytochemistry, 68: 904-912).
The plant is extremely bitter in each of its parts (Sheeja, K. and Kuttan. G. (2006) Protective effect of Andrographis paniculata and andrographoiide on cyclophosphamide-induced urothelial toxicity. Integr. Cancer Ther., 5 (3): 244- 51), however, the aerial portions of Andrographis paniculata are used to extract the active principles phytocbemicais. The extract contains diterpene, flavonoid, and stigmasters (Koteswara, R., Vimalamma, G., Venkata, R. and Yew, T. (2004) Flavonoids and andrographolides from Andrographis paniculata. Phyto., Volume 65, issue 16, Pages 2317 -2321). Being the andrographoid, the first and best isolated active principle, which has been chemically defined as a bicyclic diterpene lactone (thamlikitkui, V., Dechatiwongse, T., Theerapong, S., Chantrakul, C., Boonroj; P ,, Punkrut, W., Ekpalakorn, W., Bootaeng, N., Yaechaiya, S. and Petcharoen, S. (1991) Efficacy of Andrographis panicuiata, Nees for pharyngotonsillitis in adults. J. Med. Assoc. Thai., 74 (10): 437-42.
Different preciinical and clinical studies have been performed to identify the pharmacological properties of the components of Andrographis paniculata, for this, both the raw extract of the plant and the purified andrographoiide have been used, like the purified Andrographoiide. In preciinical studies, the plant extract has shown several activities, such as: hepatoprotective effect administered intraperitoneally in rats (Sharma, A., Lal, K. and Handa, S. (1992) Standardization of the Indian crude drug. Kalmegh at high pressure liquid chromatographic determination of andrographolide (Phytochem. Anal., 3, 129-131). antidiarrheal activity in animal models treated with enterotoxin of Escherichia coil (Gupta, S., Choudhry, MA and Yadava, JNS (1990) Antidiarrhoeal activity of diterpenes of Andrographis paniculata (Kal-Megh) against Escherichia coli enterotoxin in vivo models Int. J. Crude Drug Res., 28: 273-283), and immunostimulatory capacity in mice BALB / c (Puri, A., Saxena, R., Saxena, R. P., Saxena, K. C., Srivastava, V. and Tandon, J. S. (1993) immunogenic stimulants from Andrographis paniculata. J. of Natural Products 56: 995-999). Another active principle, but less studied, is the 14-deoxyandrgrapholide which has demonstrated a hypotensive effect (Zhang, C. Y.,
Kuroyangi, M. and Tan, B. K. H. (1998) Cardiovascular activity os 14-Deoxy-11, 12-didehydroandrograpbolide in the anesthetized ray and isolated right atria. The Italian Pharmacol. Society, 1: 1-5) and anti-inflammatory and antipyretic properties (Zhang, CY and Tan, BKH (1998) Vasorelaxation of rat thoracic aorta caused by 14-deoxyandrographolide. Clin. Exp. Pharmacol. Physiol., 25: 424- 429).
Other species that may be used instead of Andrographis paniculata are: Andrographis affinis Nees, Andrographis beddomei, Andrographis echioides Nees, Andrographis eiongata, Andrographis humifusa, Andrographis iineata Nees, Andrographis macrobotrys Nees, Andrographis paniculata Nees, Andrographis paniculata Nees, , Andrographis Rothii, Andrographis serpyilifoUa, Andrographis viscosuia Nees, Andrographis viscosula var, expiicata y Andrographis wightiana.
Also, in a study conducted at the Research Cluster for Health, Southern Cross University of Lismore, Australia, it is reported that extracts of brown algae containing fucoidan have been shown to have modulating effect of immunity. This study aimed to determine whether marine algae containing a mixture of extracts from three different species of brown algae is safe to administer, and if it has, biological potential as an immunomodulator. The results allowed to conclude that the complex of nutrients was safe to administer and furthermore that the preparation proved to have the potential as an immune modulator efectively (Myers SP, O'Connor J, Fitton JH, Brooks L, Roife M, Connellan P, Wohlmuth H, Cheras PA, Morris C. (2001) A combined Phase I and II open-label study on the immunomodulatory effects of seaweed extrae! Nutrient complex Research Cluster Far Health and Welibeing, Southern Cross University, Lismore, NSW, Australia; 5: 45-60).
Numerous studies indicate that sulfated polyanions, mainly heparin, dextran sulfate, lambda and kappa carrageenan xyiogalactans, xylomanans and fucoidians, possess potent therapeutic activity against viral diseases such as other anticoagulant and antitumor properties (Chapman VJ, Chapman DJ. 1980. Seaweed and Their Uses . In: Chapman and Hall (eds. Londres, p. 327).
The mechanism of antiviral action of sulfated polysaccharides is primarily to inhibit the entry of enveloped viruses, such as Herpesvirus (HSV), inside the host cell, by competence for the ceil surface receivers (Luscher-Mattli M. 2000. Polyanions a ios! Chance in the fight against HIV and other viral diseases, Antiviral chemistry; Schaeffer DJ, Krylov VS. 2000. Anti-HIV activity of extracts and compounds from alga! and cyanobacteria. Ecotoxicology and environmental safety 45: 208-227;
Witvrouw M, Pannecouque C, De Clerq E. 1997, In: Carbohydrates in drug design, Witczak ZJ and Nieforth KA (eds), Marcel Dekker, ine: New York, pp. 157-207). There are a number of receivers including the heparin sulfate receiver, expressed in various cell types, which provide the incoming points for the Herpes virus. Antiviral activity, in part, is due to the similarity of sulfated polyanions to heparin sulfate molecules in mammals (Campadeiii-Fiume et al., 2000).
Fucoidan was tested against several viruses involved in DNA and RNA, such as HSV, HCMV, VSV and HIV, and proved to be a potent and selective inhibitor of these viruses, regardless of their type of nucleic acid (Baba M, Snoeck R, Pauwels R, De Ciercq E. 1988. Antimicrob sulfated polysaccharides are potent and selective inhibitors of various enveloped viruses, including herpes simplex virus, cytomegalovirus, vesicular stomatitis virus, and human immunodeficiency virus Antimicrobial agents and chemotherapy 32: 1742-1745; Ponce NM, Pujo! CA, Damonte EB, Flores ML, Stortz CA. 2003. Fucoidans from the brown seaweed Adenocystis utricularis: extraction methods, antiviral activity and structural studies. Carbohydrate research 338: 153-65),
As an example, various immuno-stimulating compositions containing andrographolide or derivatives or fucoidians are disclosed for use in humans, see, for example, the following patent literature: W02005087223, WO9617605, W02006008115, WO2013117149, CN102399245, RU2381807, CN1939480, CN1939413, CN1939480 , WO0185709, WO0185710, US2002032229, JPH11228602, JPH01313433.Also, immuno-stimulating pharmaceutical compositions of fucoidans and chitosan, and fucoidians and lactobaciiius, are known as example JP2005060327 and JP2010235528.
Also, vaccines for fish comprising fucoidians are known, see JP2006312595.
The prior art also discloses various immunostimulators, nutritional compositions or others to treat and prevent diseases in humans, which comprise terpenes or their derivatives and fiavonoids and their derivatives, see, as is an example, the following patent literature: W02005020881, US5108750, US4906471, US4842859, WO2014201637, CN 103923795, CN 103735654, CN103417630, CN103005447, MX2011002765, CN102614228 and EA201001289.
The prior art also discloses compositions comprising terpenes or their derivatives and fiavonoids and their derivatives in order to restore the color of cultured fish or to pigment them, promote their growth or the foods that enhance their immunity, see as a way of example the following patent literature: JPH4166040, W02006123939, JP2010124768 and CN103355491.
Likewise, antiviral or sporozoal compositions are known, comprising terpenes or their derivatives and flavonoids and their derivatives, are known to treat fishes' diseases, see as a way of example the following patent literature: CN103989865 and KR20120118805.
However, the present invention relates to a synergistic immunostimulating composition for fishes comprising fucoidians and andrographolide.
Regarding the fucoidians it is important to point out that they belong to different species of brown algae, and they differ in accordance with the orders corresponding to brown algae.
Thus, the fucal order comprises the binding of Fucose units which varies according to the species to be analyzed but mainly shows giycosidic bonds of the type (1-> 3) or (1 - + 4) and the sulfated groups can be located in the positions C-2, C-3 or C-4. Examples of algae from which fucoids can be obtained from the fucal order are: Fucus vesiculosus, Fucus evanescens, Fucus distichus, Fucus serratus, Pelvetia wrightii, Ascophyi / um nodosum, Himantha / ia Lorea, Bifurcarfa bifurcata, Sargassum stenophilia, Sargassum antårctica.
In the order Laminare and another brown algae, the binding of Fucose units varies by species but mainly shows giycosidic bonds of the type (1- + 2) or (1- + 3) and the sulfated groups can be located in positions C- 2 or C-4. It is also mentioned that the Galactan fraction present is given by bonds (1 -> 3) and (1- + 6) with suiphated groups especially in position C-4. Examples of algae from which fucoids of laminar order and other brown algae can be obtained are: Lessonia nigrescens, Lessonia trabecu / ata, Lessonia vadosa, Macrocystis pyrifera, Undaria pinnatifida, Padina pavonia, Laminaria angustata, Laminaria japonica, Eckionia kuma, Adenocytis aris, Dictyota menstrua / is, Spatog / ossum schroederi y Chordaria fiagellifonnis.
LETTER DESCRIPTION OF THE INVENTION
The present invention relates to a synergistic immunostimulating composition for fishes comprising fucoidians and andrographolide. More preferably, the present invention relates to a synergistic immunostimulating composition for fishes comprising fucoidians and andrographoid, and allowing effective control and prevention of infections produced by intracellular microorganisms. Still more particularly, the present invention relates more closely to a synergistic composition comprising fucoidians and andrographoid, and allowing effective control and prevention of piscirickettsiosis and infectious pancreatic necrosis (IPN) in fishes.
LETTER DESCRIPTION OF THE FIGURES
Figure 1. It illustrates the conformation of distribution in fish ponds prior to challenge with P. salmonis, where DE indicates the diet with the composition of the present invention and C means the diet without the composition of the present invention.
Figure 2. it illustrates the conformation of distribution in the ponds during the challenge with P. salmonis, where DE indicates the diet with the composition of the present invention, C means the diet without the composition of the present invention and T stands for trojans.
Figure 3. it illustrates the expression analysis of IL-12 in SHK-1 cells treated with algae extract (FUTERPENOL®, a composition of botanical extracts and derivatives of seaweeds with bioactive molecules that promote immunity against intracellular pathogens), at different concentrations (0.01- 1 pg / ml) and re-suspended in ethanol and water. Analysis of the effect of IL-12 expression was performed at 4 hours post-treatment in SHK-1 cells treated with the extract 0.001 pg / mL, 0.01 pg / mL and 0.1 pg / mL. The results show the averages ± standard error of triplicate samples. The * indicate significant differences in relation to the control without stimulus, analyzed by t-student, p <0.05, ns, not significant.
Figures 4A and 4B. Illustrates the analysis of the expression kinetics of IL-12 (4A) and IFN-1 (4B) in SHN-1 cells treated with 0.5 nM Andrographoiide (AP), 1 pg / ml seaweed extract (BC), the composition of the invention (AP + BC) and diet alone as control (C). Analysis of the effect of IL-12 and IFN-1 expression was performed on SHK-1 cells treated with the composition of the present invention. The differences were statistically significant in relation to the t-Student control. * p <0.05, n = 3.
Figure 5. It illustrates the detection of P. salmonis in cells surviving the infection. The bacterial change was determined in SHK-1 cells treated with 0.5 nM Andrographoiide (AP), 1 pg / ml seaweed extract (BiendC), the composition of the invention (AP + BiendC) and the diet alone as control (C). analysis was determined based on the differences of Ct, The differences were statistically significant in relation to untreated cell control and infected with P. salmonis, t-Student. * p <0.05, n = 3.
Figures 6A and 6B. It illustrates the analysis of the expression of IL-12 (6A) and IFN-I (6B) on surviving cells to the infection with IPNv: The expression of IL-12 and IFN-I was done in SHK-1 cell treated with seaweed (BiendC) 1 pg / ml, the composition of the invention (AP + BiendC) and the diet alone as a control (C) and infected by the virus. The differences were statistically significant in relation to control * p <0.05, n = 3.
Figure 7. it illustrates the detection of IPNv in surviving ceilings from the infection. The virus-shifting times were determined on SHK-1 cells treated with the seaweed extract (BiendC) 1 pg / ml, and the diet aiones as a control (C). This analysis was determined on the basis of the differences of Ct. The differences were statistically significant in relation to the control of cells without treatment or infected by the virus, t-Student. * p <0.05, n = 3.
Figure 8. It illustrates the distribution of daily mortality of the fish from the group fed only with the diet without the composition of the present invention, the trojans and the treated, during the 60 days of study by SRS challenge.
Figure 9. It illustrates the percentage distribution accumulated of daily mortality of the fish from the group fed with the diet only without the composition of the present invention, the trojans and the treated, during the 60 days of study by SRS challenge.
DETAILED DESCRIPTION OF THE INVENTION
The present invention is related to a synergistic immunostimulant composition for fishes that comprise fucoidians and andrographolide, where the fucoidians are obtained from extracts prepared from Fucus vesiculosus, Fucus evanescens, Fucus distichus, Fucus serratus, Pe / vetia wrightii, Ascophyl / um nodosum, Lorea, Bifurcaria bifurcata, Sargassum stenophyl / um, Hizikia fusiforme, Durviliaea antårtica, Lessonia nigrescens, Lessonia trabeculata, Lessonia vadosa, Macrocystis pyrifera, Undaria pinnatifida, Padina pavonia, Laminaria angusiaia, Laminaria angusiaia, Laminaria angusiaia, Laminaria angusiaia / is, Spatog / ossum screwdrivers o
Chordaria flagelliformis. While the andrographolide are obtained from extracts prepared belongin from Andrographis affinis Nees, Andrographis beddomei, Andrographis echioides Nees, Andrographis e / ongata, Andrographis humifusa, Andrographis lineata Nees, Andrographis macrobotrys Nees, Andrographis nallamalayana, Androgis Andrographis, rothii, Andrographis serpyliifolia, Andrographis viscosula Nees Andrographis viscosula var. explicate y Andrographis wightiana. in the synergistic immunostimulating composition, the ratio of fucoidian to andrographoid is in the range of 5:95 to 20:80. Preferably, the ratio of fucoidian to anrographolide is 10:90.
The present invention is related mainly to a synergistic immunostimulating composition for fish comprising fucoidians and andrographoid, which allows effective control and prevention of infections produced by intracellular microorganisms.
The present invention is related more particularly to a synergistic composition comprising fucoidians and andrographoid, which allows effective control and prevention of piscirickettsiosis, viral haemorrhagic septicemia, infectious pancreatic necrosis, infectious haematopoietic necrosis, pancreas disease and sleeping disease, infectious anemia and renibacteriosis.
The present composition comprises synergistic comprising fucoidian and andrographoid, which allow effective control and prevention of piscirickettsiosis and infectious pancreatic necrosis (IPN) in fishes.
Example 1: Preparation of Aqueous Flour Extract containing Fucoidian
The dried brown algae were first pulverized by freezing them in liquid N2, and using a porcelain mortar, to obtain a 300 micron algae powder.
Ten grams of the ground dried algae mixture were extracted with 200 ml of distilled water with continuous stirring for 4 hours at 25 ° C. The algal tissue was removed by simple filtration. The aqueous extract was centrifuged until a clarified solution. The solution is precipitated by the addition of 3 volumes of ethanol. The precipitate was recovered by centrifugation and dried in an electric oven at 50 ° C
Example 2: Preparation of Andrographoid and Preparation of Extract.
For the preparation of the extract of andrographoid, dried leaves of Andrographis sp were used, the extraction was carried out using an 80% v / v water-ethanol mixture, the final extract is a composition containing 80% of the native extract and 20% or maitodextrin.
Example 3: Preparation of a Composition Aodrographolide and Fucosdån. A mechanical mixture of both dry extracts was performed in a ratio of 90/10 of algae extract and extract of Andrographis sp., Respectively. For this, a KitchenAid Heavy Duty mixer (Model KS5SS, USA) was used with stainless steel container, adjustable speed and capacity> 1.5 L. The selected mixing speed was, according to the equipment, level 2 equivalent to ± 70 rpm of the upper shaft. The mixing time was 10 minutes, the mixture was prepared according to the proportions of ingredients and the densities of these were determined by a gravimetric method with results of 0.77 grs / cmf
Example 4: results of immune effect in fucosdan cell lines
The SHK-1 cell line, derived from Salmo safaris kidney, was used. The assay was started when the cells showed 90% of confluence, and then they were stimulated with algae extract (5% of Fucoidian).
The treatment was applied independently to SHK-1 cells, in L15 medium supplemented with 10% fetal bovine serum at a dose of 1 pg / ml, the cells were incubated at 20 ° C during 24 hours of stimulation time.
After treatment, the cell supernatant was discarded and the cells were lysed with 200 µl of TRK lysis buffer and stored in 1.5 ml tubes at -80 ° C. RNA extraction from the cells was performed using the RNA extraction kit (Omega-bio-tek), according to the manufacturer's protocol.
Once the total RNA was obtained, the mRNAs were transformed into cDNA by means of the reverse transcription reaction, which was performed in a total volume of 20 μ! of solution, divided into two parts. The first reaction was performed in a mixture containing 1.6 μΙ of oligo-dT (1.25 μg / mi) for analysis of gene expression of the markers 1.0 μΙ of dNTPs (10 mM); 8.0 µl of total RNA (5 µg) and 0.1 µl of nuclease-free water and it was incubated for 10 min at 60 ° C to elute secondary structures of the mRNAs. Subsequently, a second mixture comprised of 1 μ! of M-MLV reverse transcriptase (200 U), 4 μΙ of 5X enzyme buffer and 0.5 μΙ of recombinant RNAseOUT ribonuclease inhibitor (40 U) was added to the solution, in a total volume of 5.5 μΙ and it will be incubated for 1 h at 37 ° C. Finally, for the inactivation of reverse transcriptase, the reaction mixture was incubated at 72 ° C for 10 min. The synthesized cDNA was stored at -20 ° C for its subsequent amplification for PCR or its real-time quantification (qPCR) for IFN-i and IL-12 genes relative to EF-1a expression using the primers listed in Table 1 below:
Table 1
Each amplification reaction was performed using 2 μ! of cDNA as the annealing, 0.2 μΜ (Table 1) primers, 0.8 μΙ MgCI 2 (25 mM), 1 μ! Lightcycler® Fast Start DNA Master SYBR Green amplification mixture in a volume of 10 μΙ. The reaction was carried out in a LightCycler® 1.5 thermal cycler. The program consists of the following steps: initial denaturation at 95 ° C for 10 min, followed by a PCR reaction of 35 cycles each composed of denaturation at 95 ° C for 10 seconds, mating at 58 ° C for 10 seconds and extension at 70 ° C for 10 seconds. Subsequently a cycle to obtain the melting curve for 20 s at 95 ° C, and finally a cooling cycle at 40 ° C for 30 s. For the relative quantification, it was performed with a standard curve consisting of reactions containing dilutions of the purified PCR product of known concentration for the gene of interest. After obtaining and quantifying the PCR product corresponding to each gene, dilutions were made in a range of 107 to 102 numbers of copies / μ! for each gene under study, for the subsequent calculation of the efficiency of the reaction, where the foiiowing relation, E = 10 (-1 / slope) -1 will be used. For the caiculation of relative expression by the qPCR technique amplification reactions of the ELF-1 gene cDNA were performed on each RNA sample from cells treated with the different stimuli in vitro. Then, the expression changes were calculated using the comparative CT method (Pfaffl, 2001).
The results are illustrated in Figure 3.
Example 5: Result of Immune Effect in Andrographolide Cell Lines
The SHK-1 cell line, derived from Salmo's kidney, was used. The assay was started when the cells showed 90% confluency, where they were stimulated with an extract of Andrographis sp (10% total Andrograpbolide).
The treatment was applied independently to SHK-1 cells in L15 medium supplemented with 10% fetal bovine serum at a dose of 5 nM of the Andrographis sp extract, the cells were incubated at 20 ° C for 24 hours of stimulation time.
After the treatment was finished, the cell supernatant was discarded and the cells were lysed with 200 μl! of TRK lysis buffer and stored in 1.5 ml tubes at -8G ° C. RNA extraction from the cells was performed using the RNA extraction kit (Omega-bio-tek), in accordance with the manufacturer's protocol.
Once the total RNA was obtained, the mRNAs were transformed into cDNA by means of the reverse transcription reaction, which was performed in a total volume of 20 μΙ of solution divided into two parts. The first reaction was performed in a mixture containing 1.6 μΙ of oiigo-dT (1.25 pg / mi) for analysis of gene expression of the 1.0 μΙ markers of dNTPs (10 mM); 8.0 μΙ of total RNA (5 μg) and 0.1 μί of water free of nucleases and incubated for 10 min at 60 ° C to remove secondary structures from the mRNAs. After this a second mixture comprised of 1 µl of M-MLV reverse transcriptase (200U), 4μΙ or 5X enzyme buffer and 0.5µ! of RNAsaOUT 40 U recombinant ribonuclease inhibitor was added to this solution, in a total volume of 5.5 µl and will be incubated for 1 hour at 37 ° C. Finalized for inactivation of reverse transcriptase, the reaction mixture was incubated at 72 ° C for 10 min. The synthesized cDNA was stored at -20 ° C for subsequent PCR amplification or quantification by real-time PCR (qPCR) for the IFN-1 and IL-12 genes relative to the expression of EF ~ 1a using the primers indicated in Table 2 below. :
Table 2
Each amplification reaction was performed using 2 µl of CDNA as a tempi ate, primers of 0.2 µM (Tabie 2), 0.8 µg MgCI 2 (25 mM), 1 µl Lightcycler® Fast Start DNA Master SYBR Green amplification mixture in a volume of 10 µl . The reaction was carried out in a LightCycler® 1.5 thermal cycler. The program consisted of the following steps: initial denaturation at 95 ° C for 10 min, followed by a PCR reaction of 35 cycles each composed of denaturation at 95 ° C for 10 s, mating at 58 ° C for 10 s and an extension at 70 ° C during 10 s. Subsequently, a cycle to obtain the melting curve for 20 s at 95 ° C., and finally a cooling cycle at 40 ° C during 30 s. The relative quantification was performed with a standard curve consisting of reactions containing dilutions of the purified PCR product of a concentration known to the gene of interest. After obtaining and quantifying the PCR product corresponding to each gene, successive dilutions were performed in a range of 107 to 102 numbers of copies / p! for each gene under study, for the subsequent calculation of the efficiency of the reaction, where the following relation, E = 10 (-1 / slope) -1 will be used. For the calculation of relative expression by the qPCR technique amplification reactions of the ELF-1 gene cDNA were performed on each RNA sample from cells treated with the different stimuli in vitro. Then, the expression changes were calculated using the comparative CT method (Pfaffl, 2001).
The results are illustrated in Figures 4A and 4B.
Example 6: Result of immune effect on ceil lines of the mixture fucoidian plus Andrographolide
The SHK-1 cell line, derived from Saimo salad kidney, was used. The assay was started when the cells had 90% confluence, where they were stimulated with an extract of Andrographs sp and an extract of brown algae.
The treatment was applied at the same time to SHK-1 cells, in a half of L15 supplemented with 10% fetal bovine serum at doses of 1 pg / ml of brown algae extract (5% total fucoidians) and 5 nM extract of Andrographis sp (10% total andrographolide) cells were incubated at 20 ° C during 24 hours of stimulation time.
After treatment, the cell supernatant was discarded and cells were lysed with 200 µl of TRK lysis buffer and stored in 1.5 mi tubes at -80 ° C. RNA extraction from the cells was performed using the RNA extraction kit (Omega-bio-tek), according to the manufacturer's protocol.
Once the total RNA was obtained, the mRNAs were transformed into cDNA by means of the reverse transcription reaction, which was performed in a total volume of 20 μΐ of soiuiion, divided into two parts. The first reaction was performed in a mixture containing 1.6 μ! or oligo-dT (1.25 pg / ml) for analysis of gene expression of the 1.0 pi markers of dNTPs (10 mM); 8.0 µl of total RNA (5 µg) and 0.1 µl of water free of nucleases and it was incubated for 10 min at 60 ° C to remove secondary structures from the mRNAs. Subsequently, to this solution was added a second mixture comprised of 1 µl of M-MLV reverse transcriptase (200 U), 4 µl of 5X enzyme buffer and 0.5 µl! or recombinant RNAseOUT ribonuclease inhibitor (40 U), in a total volume of 5.5 µl and it will be incubated for 1 hour at 37 ° C. Finally, for inactivation of reverse transcriptase, the reaction mixture was incubated at 72 ° C for 10 min. The synthesized cDNA was stored at -20 ° C for further amplification by PCR or quantification by real-time PCR (qPCR) for the IFN-1 and IL-12 genes relative to EF-1a expression using the primers indicated in Table 3 below:
Table 3
Each amplification reaction was performed using 2 μΙ of cDNA as a template, primers of 0.2 μΜ (Table 3), 0.8 μΙ MgCI (25 mM), 1 μ! Light Cycler © Fast Start DNA Master SYBR Green amplification mixture in a volume of 10 μΙ. The reaction was carried out in a LighiCycier® 1.5 thermal cycler. The program consisted of the following steps: initial denaturation at 95 ° C for 10 min, followed by a PCR reaction of 35 cycles each composed of denaturation at 95 ° C for 10 s, mating at 58 ° C for 10 sec and extension at 70 ° C for 10 sec. Subsequently a cycle to obtain the melting curve during 20 s at 95 ° C, and finally a cooling cycle at 40 ° C during 30 s. The relative quantification was performed with a standard curve consisting of reactions containing dilutions of the purified PCR product of known concentration for the gene of interest. After obtaining and quantifying the PCR product corresponding to each gene, successive dilutions were performed in a range of 10 / to 102 number of copies / μΙ for each gene under study, for the subsequent calculation of the efficiency of the reaction, where the following relation , E = 10 (-1 / slope) -1 will be used. For the calculation of the relative expression by the qPCR technique amplification reactions of the ELF-1 gene cDNA were performed in each RNA sample from cells treated with the different stimuli in vitro. Then, the expression changes were calculated using the comparative CT method (Pfaffi, 2001).
The results are illustrated in Figures 4A and 4B.
Example 7: result of immune effect by challenge P. salmonis
The SHK-1 cell line, derived from Salmo salar's kidney, was used. The assay was started when the cells showed a 90% confluence, where they were stimulated with a combination that will ensure a concentration of the brown algae extract of 1 pg / ml and 5 nM of the extract of Andrographis sp, as well as the individual stimulation with a concentration of 1 pg / mi extract of brown algae, and individual stimulation with a concentration of 5 nM of the extract of Andrographis sp. The treatments were applied independently to SHK-1 cells in L15 supplemented with 10% fetal bovine serum at the above-mentioned doses, cells were incubated at 20 ° C during 24 hrs incubation.
Infection with P. salmonis was carried out after the incubation period. For the challenge, a strain of Piscirickettsia salmonis PPT005 grown on a SHK-1 cell line, which was originally isolated from a dying population of Atlantic salmon (Salmo salar) from a farm salmond center near Puerto Montt, Chile, using CHSE-214 cells . The cells were infected and incubated at 18 ° C in L-15 medium supplemented with 2% SFB. The bacteria were harvested from the infected cells when they had a 90% cytopathic effect (CPE). Finally, functional assays were performed by sowing ΙΟ'1 bacteria per mL in SHK-1 cells at 90% of confluence.
The duration of the challenge test was 9 days, time required to obtain a 50% cytopathic effect in the control monolayers.
After the treatment was complete, the supernatants were harvested and the surviving cells were lysed with 200 µl of TRK lysis buffer and stored in tubes of 1.5 ml at -80 ° C. 1 ml of each culture supernatant from SHK-1 cells was taken with 9 days of infection. These supernatants were centrifuged at 700 xg for 10 min to remove the cell residue, and then at 16,000 xg for 45 min to recover the bacteria in an Eppendorf 5402 centrifuge. All the sediments were processed by the Chelex method for obtaining the DMA to amplify. Briefly, they were suspended in 100 µ! of 6% Instagene p / v (Chelex 100, Bio-Rad), they were shaken at maximum speed in a vortex and centrifuged at 11,600 xg during 5 min in an Eppendorf centrifuge to coiiect the pearls of Chelex in the sediment and DNA in the supernatant. For the estimation of bacterial numbers, standard numbers were used as reference with known numbers of P. salmonis copies, obtained by cloning the ITS of this bacterium in the vector pCR® 2.1 TOPO TA (invitrogen). The standards of 104 to 1010 number of copies and the DNAs obtained by Chelex were amplified in parallel. Each reaction was performed in a volume of 30 μ! with 1 µg of each DNA sample, and 0.5 mM of the ITS primers (Marshall et al. 1998) labeled with FAM (495-535 nm). For amplification an initial denaturation of 10 minutes at 95 ° C was performed, followed by 35 cycles with the following segments: denaturation at 95 ° C for 15 seconds, alignment at 60 ° C for 30 seconds, and an extension at 72 ° C for 45 seconds. seconds, and then a final extension of 6 min at 72 ° C. From the amplification curves obtained for each sample, the Ct (crossing threshold) values of the copy number standards were estimated, in accordance with the method described by Phaffi, 2001, the results are plotted in Figure 5. In the case of the suriing ceils An RNA extraction from the cells was performed using the RNA extraction kit (Omega-bio-tek), in accordance with the manufacturer's protocol.
Once the total RNA was obtained, the mRNAs were transformed into cDNA by means of the reverse transcription reaction, which was performed in a total volume of 20 μΙ of solution divided into two parts. The first reaction was carried out in a mixture containing 1.6 μ! or oligo- <1T (1.25 pg / ml) for analysis of gene expression of the markers 1.0 pi of dNTPs (10 mM); 8.0 µl of total RNA (5 µg) and 0.1 µl of water free of nucleases and it was incubated for 10 min at 60 ° C to remove secondary structures from the mRNAs. After, a second mixture comprised of 1 µl of M-MLV reverse transcriptase (200 U), 4 µl of 5X enzyme buffer and 0.5 µl of recombinant RNAseOUT ribonuclease inhibitor (40 U) was then added to this solution, in a total volume of 5.5 µl and it will be incubated for 1 hour at 37 ° C. Finally, for inactivation of the reverse transcriptase, the reaction mixture was incubated at 72 ° C for 10 min. The synthesized cDNA was stored at -20 ° C for subsequent PCR amplification or quantification by real-time PCR (qPCR) for the IFN-1 and IL-12 genes related to EF-1a expression using the primers indicated in Table 4 below:
Table 4
Each amplification reaction was performed using a 2 μ template! or cDNA, 0.2 μΜ primers (Table 1), 0.8 μ! MgCl2 (25 mM), 1 μ! of Lightcycler® Fast Start DNA Master SYBR Green amplification mixture in a volume of 10μί. The reaction was carried out in a LigbtCycler® 1.5 thermal cycler. The program consisted of the following steps: initial denaturation at 95 ° C for 10 min, followed by a PCR reaction of 35 cycles each composed of denaturation at 95 ° C for 10 s, mating at 58 ° C for 10 s, and extension at 70 ° C during 10 s. Subsequently a cycle to obtain the melting curve during 20 s at 95 ° C, and finally a cooling cycle at 40 ° C during 30 s. Relative quantification was performed with a curve standard consisting of reactions containing dilutions of the purified PCR product of known concentration for the gene of interest. After obtaining and quantifying the PCR product corresponding to each gene, successive dilutions were performed in a range of 107 to 102 number of copies / μ! for each gene under study, for the subsequent calculation of the efficiency of the reaction, where the following relationship, E = 10 (-1 / slope) -1. For the calculation of the relative expression by the qPCR technique amplification reactions of the ELF-1 gene cDNA were performed on each RNA sample of cells treated with the different stimuli in vitro. Then, the expression changes were calculated using the comparative CT method (Pfaffl, 2001).
Example 8. Immunostimulation against intracellular microorganisms (IPNv) with the composition of the present invention in salmonid fishes cell lines. A study was performed on salmonid fishes ceil lines, where the composition of the present invention was evaluated. Cell lines exposed to the combination of fucoidians + Andrographolide, cell lines exposed only to fucoidians, and subsequently, molecular markers relevant in ThO to Th1 differentiation such as IL-12 and IFN-1 were evaluated. The separate fucoidians and the combination of these + Andrographolide are significantly different in surviving cells following a challenge with IPNV. At the same time, there is a decrease in the copy numbers of the pathogen agents significantly higher than the cells that received the composition of the present invention in relation to the use of only the fucoidians or the aqueous extract of brown algae.
See Figures 6A, 6B and 7
The studies in fishes were carried out in ponds, where the composition of the present invention was an aqueous extract of seaweed with a reference percentage of 5% fucoidians obtained from Macrocystes Pyrifera in combination with an extract from the Andrographis sp plant with a 10% of total andrographolide in a proportion of 10% and 90%, respectively, the fish feed or diet was incorporated, at a dose in the range of 0.5 to 2.5 Kh per ton of food. Preferably, at a dose of 1 kg per ton of food.
We used 450 specimens of rainbow trout (Oncorhynchus mykiss) with average weight of 100-120 g. However, additional fishes were available to achieve a coefficient of variation of less than or equal to 15%.
Samples of 30 fish were taken to be analyzed in the laboratory by real-time RT-PCR technique, to discard the presence of IPNv, BKD and SRS.
An exploratory sampling was done to know the average weight of the population and to carry out the selection of the fishes chosen for the test. Only animals presenting the required weight, good condition of adaptation to the saline environment and sanitary condition approved by the veterinarian (free of IPNv, SRS and BKD) were included.
With the selection data, all animals with weight outside the selection range, as well as those with peels or those whose condition was not appropriate for the present study, were excluded when marking.
The fishes were marked with pittags 10 days before the start of the test, proceeding as follows: a) The fishes were extracted from the pond and placed in a pan with an anesthetic solution, Tricaine methanesulfonate 80%. b) Once stage II (deep anesthesia) was reached, they were taken individually and arranged on the working table, in a lateral way, so that the head is left to the left side of the operator. c) A needle was inserted to make the incision flank at the level of ventral fins through which the chip was inserted. Then he performed a small massage to slide the chip into the ventral cavity. (d) The fishes were transferred to the basin of origin for their recovery and waiting for conformation of test ponds.
Six ponds of 1 rn3 were formed from fishes previously marked with pittags. In each pond 50 fish were deposited and of which the code of the chip was read, creating a database that associated, initial weight and length and pond number. The database allowed to track the traceability of the tagged fishes, related to productive indexes and subsequent challenge with the pathogen. Simultaneously 2 ponds with 75 fish each were formed, according to the same procedure, which were kept until the challenge stage, see Figure 1.
The fish were kept in the ponds during 10 days as acclimatization period, under controlled conditions; average temperature of 14 ° C (± 1 ° C), salinity in a range of 31-32 ppt, oxygen 80-100% saturation and pH of 7-8. The environmental parameters were monitored daily.
During this stage, the ponds were fed with diet without the present composition, manually at 2-2.5% PC, with a 100% ration in the morning.
Daily, the unconsumed food of each pound was recovered, to later estimate the actual feeding rate of each group. Existing mortality, it was extracted and recorded in the corresponding pond, and necropsy was carried out by trained fish farming personnel.
The fish were fed 2-2.5% pc / day, during acclimatization, treatment administration and challenge stage with pathogen. The food was administered manually, delivering 100% of the ration during the morning. It should be noted that during the acclimatization and challenge a commercial diet without additives was administered.
The amount of food supplied was adjusted regularly according to the expected growth rate for the species and mortality. On a daily basis, unconsumed food was collected from the ponds, thus obtaining the actual feed intake for the estimation of subsequent productive indexes,
During the development of the test, tissue samples were taken, considering the kidney, proximal intestine and blood samples for plasma collection. The number of samples and sample time are shown in Table 3 below.
Kidney samples were taken in two 0.5 cm'5 pieces, which were immersed in 2 mi eppendorf tubes (individually for each fish) containing 800 pL of later RNA (Ambion). These samples were labeled and refrigerated (4-6 ° C) for 24 h, then cooled to -80 ° C.
The proximal intestine was destined for histological analysis, for which they were deposited in falcon tubes with buffered formalin. In this case, the number of samples per pound (3) was placed in the same tube, labeled with date, pond number and treatment.
Blood samples were deposited immediately after collection in eppendorf tubes prepared with heparin (25! U). They were then centrifuged to remove the plasma, which was placed in a new tube (previously labeled) and stored in the ultra-freezer (-80 ° C) until taken off.
Table 1. Number and time of doing tissue sampling
The food containing the composition of the present invention was distributed to three ponds (triplicate), as indicated in Table 4, during 30 consecutive days. The remaining ponds (controls) continued their feeding with a standard diet throughout the evaluation period. Administration of treatment was as described above.
During this time, temperature, pH, salinity and oxygen were monitored daily. If there was mortality at this stage, it was taken out and recorded in the corresponding pond, performing an anatomopathological test.
Table 5. Detail administration treatment N ° Pond N ° of Group Diet Type Time fishes administration (days) 1 47 Treatment immunostimulant 30 2 47 Control Commercial 30 3 47 Treatment immunostimulant 30 4 47 Control Commercial 30 5 47 Treatment immunostimulant 30 6 47 Control Commercial 30
Control corresponds to the commercial diet.
The immuno-modulating agent corresponds to the composition of the present invention
Then, a challenge was performed with P. salmonis. Table 3 details the specifications of the P. salmonis isolate that was used in the inoculation of Trojan fishes.
Table 6. P. salmonis isolate specifications
Laboratory of original ADL Diagnostic Chiie Ltda.
Agent Piscirickeit hits salmon
Laboratory code PM-341 52 species of original isolate Rainbow Trout species where it was realized Atlantic Salmon- Rainbow Trout date original isolation 05-11- i 2
Organ of isolation Kidney N ° oianimaiizations in isolation condition Reanimated cr / opreserved
Inoculum production type Bacterial culture
The inoculum was administered with TC! D5G / ml determined by the Karber Spearman method by the laboratory ADL Diagnostic Chiie Ltda. In addition, the purity of the inoculum was evaluated, considering iSAv, IPNv, BKD, F. psycrophilum RT-PCR analysis and bacteriological cultures in medium TSA and TSA / s at 18 and 35 ° of incubation.
At the end of the administration of the diet with the composition of the present invention, the fishes were redistributed to perform the challenge. Three ponds of 1 m3 were formed, considering the mixture of treated and untreated fish at random in the new ponds, as indicated in table 6. At the time of the new distribution the pittag was read, assigning to each chip the group and pond, see Figure 2.
Table 7. Redistribution of fishes for challenge
Origin ΤΚ-Ϊ TK-2 TK-3 TK-4 TK-5 ΊΓΚ-6 'total n = 40 n: 40 n = 40 n = 40 n = 40 n = 40 N ° Treated Control Treated Control Treated Control challenge pounds 7 13 14 13 13 14 13 80 8 13 13 14 13 13 14 80 9 14 13 13 14 13 13 80
Observation: The number of fishes is estimated considering mortality and samping in the treatment administration stage, if not, the number will be adjusted to the real n.
Treated means that a diet comprising the composition of the present Invention has been provided. Control means that only a commercial diet has been provided.
The challenge was achieved by cohabitation, which involved introducing fish infected with P. salmonis, trojans, into healthy fish ponds (treated and controlled), as indicated in Table 7, considering an infection pressure of 33%. The inoculum was administered intraperitoneally to the trojan group at a rate of 0.2 m / fish. The inoculation was performed according to the following procedure: a) The fish were extracted from the pond and placed in a container with anesthetic solution (Tricaina 80% ASL). b) Once the anesthetic stage III was reached, they were taken individually and held with the ventral face upwards. c) The needle was inserted at an angle of approximately 45 ° into the ventral midline, between the pectoral and pelvic fins, injecting 0.2 ml per fish. d) At this stage the pittag was read by assigning to the chip code the group 'trojans', pond number and inoculation date. e) Post application the fishes were transferred to the assigned pond, constantly monitoring the state of recovery.
Table 8 Distribution of challenge groups by cohabitation group TK-7 TK ~ 8 TK-9
N η N
Treated 40 40 40
Control 40 40 40
Trojans 40 40 40
Total 120 120 120
Treated means that: it has received the diet with the composition of the present invention.
Control means you have only received a commercial diet.
Subsequently, the fishes were left in the ponds waiting for the appearance of mortality. During this stage, feeding was carried out in accordance with point 6.8 and daily environmental parameters such as temperature, salinity, oxygen and pH were recorded. Mortality was identified according to the number of pittag from the database, registering daily.
The challenge lasted for 60 days, period of time that, the accumulated mortality of the control group was expected to reach 40-60%, thus ending the test.
The mortality recorded during the days of challenge was sent to the diagnostic laboratory to be analyzed by anatomopathological observations. In parallel, molecular analyzes were performed by real-time RT-PCR, for IPN and SRS viruses, to 20% of the total, considering 15 Trojans, 30 of the treated group and 30 of the control group, to confirm the presence of the pathogen.
Weight and length were measured at day 0 (Beginning Acclimatization), at 30 days of treatment administration and at the end of the challenge with P. salmonis, on the 100% of the fish in each group. From the data, condition factor (K), feed rate (SFR), specific growth rate (SGR),% growth, thermal growth rate (GF3) and food conversion rate (FCRb).
Below are summarized in tables some of the productive variables such as average body weight, condition factor K, coefficient of variation and weight gain at the end of treatment administration. As can be seen, the final weight (see Fig. 12) increased in all ponds.
Table 9: Body weight, condition factor, coefficient of variation and weight gain at the end of the treatment administration stage.
Treated means that the diet has been supplied with the composition of the invention Control means that only a commercial diet has been supplied.
Table 10: Food supplied.% SFR and feed conversion factor.
Treated means that the diet has been supplied with the composition of the invention Control means that only a commercial diet has been supplied.
Table 10 summarizes the production parameters obtained during the treatment administration period (Diet with the present composition of the present invention). From the table it can be seen that the growth indicators (% growth, SGR and SFR) were similar between the treated group and the control group. The data from each group did not present significant differences in weight, obtained at the end of administration (p> 0.05), in the SGR specific growth rate (p> 0.05) and in the thermal growth rate GF3 (p> 0.05).
Table 11: Summary of productive variables by treatment group
Control means that only commercial diet has been provided.
Treatment means that a commercial diet has been provided with the composition of the present invention.
Table 11 shows the biomass increase and cumulative growth (%) post-administration of the commercial diet with the composition of the present invention. The increase in biomass fluctuated from 6.35 to 7.28 kg and the accumulated growth of 135.7 to 162.2% between the different test ponds.
The specific growth rate (SGR) ranged from 1.65 to 1.85 among different replicates, however, no differences were observed between the group to which a commercial diet was supplied with the composition of the present invention and the group to which only the commercial diet been supplied. The same happened for the growth rate term (GF3), with a range of 2.16 to 2.42 behaving similarly in both groups.
Table 12 Biomass, percentage of relative growth, rate of thermal growth and specific rate of growth at the end of the treatment administration stage
Accumulated growth is calculated from the beginning of acclimatization and at the end of treatment administration.
Control means that only a commercial diet has been provided.
Treaty means that it has supplied a commercial diet with the composition of the present invention.
From the results obtained, T test was performed for independent samples, not observing significant differences (p> 0.05) for the growth variable, between the control group and the group treated with experimental additives.
For the specific rate of thermal growth and specific rate, the same analysis was applied, not registering significant differences (p <0.05) between the treated group and the control group.
In the challenge stage with P. salmonis, post challenge mortality was analyzed. To do this, during the period of cohabitation the rainbow trout groups presented a similar percentage of cumulative mortality among replicates in the group of trojans.
In the control group and the one administered with food of the composition of the present invention, it was higher in one of the replicates (TK C9), whereas replicates 2 and 3 (TK C10 and C11) had similar mortality, however, the trend was similar between the replicates, where the control group had higher mortality than the treated groups. Figures 17 and 18 show the evolution of daily and accumulated mortality per pound.
In order to confirm the reason for mortality of the challenged groups, dead fish were analyzed by molecular techniques (RT-PCR real time) with a total of 63 samples, obtaining 100% of positive cases with P. salmonis presence, and 0 positive samples for IPNV, evaluated in the different groups (see Table 10). The average Ct for the control group was 21.71 and for the experimental group 23.1.
Table 13 Results of the P. salmonis PCR analysis in rainbow trout during the cohabitation challenge
control means that only a commercial diet has been added, treated means that a commercial diet plus the composition of the present invention has been supplied. in addition to moiecuiar analysis, necropsy of the mortality was performed, externally! and internal lesions associated with SRS were seen, in general, the most recurrent injuries were ulcerative lesions on the skin, fin-hemorrhages, congestive intestinal serous, congestive brain, renomegaiy, congestive adipose tissue, splenomegaly, and congestive pyloric blinds.
Table 14 shows the average weight, condition factor (K) and percentage of growth obtained at the end of the challenge for the controi group and the treated group. As noted, the group treated with the composition of the present invention achieved higher average weight, condition factor and cumulative% growth at the end of the challenge.
Table 14: Average weight at the end of the challenge with P. salmonis
control means that only a commercial diet has been supplied means that the commercial diet plus the composition of the present invention has been supplied.
For the interpretation of the efficacy results of the treatment, the relative percentage of survival (RPS) was calculated based on the mortality recorded during the challenge. The RPS is the ratio between the cumulative mortality of treated fish at the time the cumulative mortality of control (untreated) fish reaches 40-60%. The RPS is expressed according to the following formula: RPS = 1 - (% mortality of fishes treated /% mortality of untreated fishes (control) · 100
Also, the cumulative mortality of the control group was calculated at day 60 post challenge and at the end of the study (day 80). The RPS for the group treated by pond and as a group is presented below in Tables 15 and 16.
Table 15 Relative Survival Rate (RPS) in rainbow trout at 60 days post challenge
Control means that only a commercial diet has been supplied means that the commercial diet plus the composition of the present invention has been supplied
Table 16 Relative Survival Rate (RPS) at end-time rainbow trout
control means that only a commercial diet has been added means that a commercial diet plus the composition of the present invention has been supplied.
As seen in the tables, the RPS at day 60 was 62.3% and then decreasing to day 80 post challenge with 57.14%.
The study concluded after 133 days, having 23 days of acclimatization period, a 30 days of treatment administration period, and an 80 days cohabitation challenge. The results showed that the incorporation of the composition into the diet substantially improved the survival of the fish when exposed to Piscirickettsia salmonis via natural infestation (cohabitation), obtaining significant differences with respect to the group that was not treated. On the other hand, at the productive level, no differences were observed significantly in food consumption, conversion, increasing weight and specific growth rate, behaving in a similar way to a normal diet without additives.

权利要求:
Claims (11)
[1] CLAMS
1. Fishes composition characterized because it comprises an aqueous extract of seaweed with a percentage of fucoidians of at least 5% and an extract of Andrographis sp plant with a percentage of total andrographolide of at least 5%, where the fucoidian: andrographolide ratio is in the range of 5:95 to 20:80.
[2] 2. The composition of claim 1, characterized because the fucoidian: andrographolide ratio is in the range of 10:90.
[3] 3. The composition of claim 1, characterized because the aqueous extract of seaweed is selected from an aqueous extract of selected brown aigae Fucus vesiculosus, Fucus evanescens, Fucus distichus, Fucus serratus, Pelvetia wrightii, Ascophyllum nodosum, Himanthaiia Lores, Bifurcaria bifurcata, Sargassum stenophylium, Hizikia fusiforme, Durvillaea antarctica, Lessonia nigrescens, Lessonia trabeculata, Lessonia vadosa, Macrocystis pyrifera, Undaria pinnatifida, Padina pavonia, Laminaria angustata, Laminaria japonica, Eckionia kurome, Adenocytis utricuiaris, Dictyota menstrua/is, Spatoglossum schroederi and Chordaria flagelliformis.
[4] 4. The composition of claim 1, characterized because the Andrographis sp plant extract is selected from an extract of Andrographis panicuiata, Andrographis affinis Nees, Andrographis beddomei, Andrographis echioides Nees, Andrographis elongate, Andrographis humifusa, Andrographis lineata Nees, Andrographis macrobotrys Nees, Andrographis nallamaiayana, Andrographis neesiana, Andrographis ovata, andrographis panicuiata nees, Andrographis rothii, andrographis serpyliifolia, Andrographis viscosula Nees, Andrographis viscolusa var. explicata and Andrographis wightiana.
[5] 5. The composition of claim 1, characterized because the aqueous extract of seaweed is selected from an aqueous extract of Macrocystes Pyrifera,
[6] 6. The use of the composition of any of the preceding claims, characterized because it serves to prepare a medicine useful for controlling and preventing infections caused by intracellular microorganisms in fishes.
[7] 7. The use of claim 6, characterized because the infections are produced by intracellular microorganisms selected from piscirickettsia, viral haemorrhagic septicemia virus (HSV), infectious pancreatic necrosis virus (IPNv); infectious hematopoietic necrosis virus (IHNV), salmon Aiphavirus (SAV), infectious salmon anemia (SAV) and bacteria including Franciceila sp and Renibacterium salmoninarum.
[8] 8. The use of claim 7, characterized because the infections are produced by intracellular microorganisms selected from piscirickettsiosis and IPNv.
[9] 9. A method for controlling and preventing infections caused by intracellular microorganisms in fishes which comprises mixing the composition of claim 1 with the fishes food or diet.
[10] 10. The method of claim 9, characterized because it comprises mixing the composition according to any of the preceding ciaims with the fishes food or diet, in a ratio in the range of 0.5 to 2.5 kg per ton of food.
[11] 11. The method of claim 10, characterized in that it comprises mixing the composition according to any one of the preceding claims with the fishes food or diet, at a rate of 1 kg per ton of food.

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同族专利:

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公开号 | 公开日

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EP3281633A4|2018-12-12|

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DK179845B1|2019-07-31|

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MX2017012895A|2018-06-13|

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CL2015000876A1|2015-08-28|

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EP3281633A1|2018-02-14|

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US20180289759A1|2018-10-11|

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WO2016161534A1|2016-10-13|

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BR112017021442A2|2018-07-03|

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CR20170457A|2018-05-09|

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CA2981989A1|2016-10-13|

引用文献:

---

公开号 | 申请日 | 公开日 | 申请人 | 专利标题

---

---

ID22487A|1997-03-21|1999-10-21|Yakult Honsha Cs Kk|PROFILACTIC AND THERAPEUTIC SUBSTANCE FOR INFECTION DISEASE FROM FISH AND FRAMES|

---

JP4398172B2|2003-04-02|2010-01-13|株式会社ヤクルト本社|Infection prevention and treatment agent for fish|

---

WO2006008115A1|2004-07-16|2006-01-26|Universidad Austral De Chile|Diterpenic labdans as immunostimulants for treating infectious diseases|

---

MX2011012297A|2009-05-21|2012-04-19|Bioatlantis Ltd|The improvement of gastrointestinal health, immunity and performance by dietary intervention.|

---

US20120189706A1|2009-10-06|2012-07-26|Knocean Sciences, Inc.|Macrocystis Pyrifera Derived Health and Wellness Products and Methods of Using the Same|

---

CN102764308A|2012-08-14|2012-11-07|天津生机集团股份有限公司|Drug for preventing bacterial diseases of fish and preparation method thereof|

---

CN103989852A|2014-05-26|2014-08-20|湖州天健兽药有限公司|Veterinary traditional Chinese medicine for preventing and treating fish diseases|CL2018003878A1|2018-12-28|2019-05-17|Univ De Santiago De Chile 50%|Formulation comprising extract of crynodendron patagua and essential oil of satureja montana for the prevention and treatment of diseases caused by piscirickettsia salmonis in individuals of the genus Salmo.|

---

WO2021162742A1|2020-02-12|2021-08-19|HP Ingredients Corp.|Improved aquaculture feed additive|

法律状态:
2019-07-31| PME| Patent granted|Effective date: 20190731 |

优先权:

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申请号 | 申请日 | 专利标题

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CL2015000876A|CL2015000876A1|2015-04-08|2015-04-08|Veterinary composition of seaweed extract with at least 5% of fucoidians and andrographis sp plant extract with at least 5% of andrographolides, useful in the control and prevention of infections caused by intracellular microorganisms in fish.|

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CL876-2015|2015-04-08|

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PCT/CL2016/050015|WO2016161534A1|2015-04-08|2016-04-06|Veterinary composition of marine algae and andrographis sp extracts, which can be used to treat infections in fish|

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