Multicellular living organisms and unmodified parts thereof and – Nonhuman animal – Transgenic nonhuman animal
Reexamination Certificate
1999-05-06
2002-04-16
Clark, Deborah J. R. (Department: 1633)
Multicellular living organisms and unmodified parts thereof and
Nonhuman animal
Transgenic nonhuman animal
C800S013000, C800S025000, C435S320100, C435S325000, C435S455000, C514S04400A, C536S023100, C536S023500, C536S023510
Reexamination Certificate
active
06372959
ABSTRACT:
BACKGROUND OF THE INVENTION
1. Field of the Invention
The present invention relates to an expression vector of a mud loach growth hormone gene and a fast-growing transgenic mud loach transformed with the expression vector thereof. More particularly, it relates to a cDNA gene encoding of a growth hormone which is isolated from a mud loach, an expression vector of a mud loach growth hormone gene containing a &bgr;-actin gene regulation site of a mud loach, and a method of producing a mud loach of high growth rate by transforming it with the expression vector, and a fast-growing transgenic mud loach produced thereby.
2. Description of the Prior Art
A mud loach (
Misgurnus mizolepis
), which inhabits the northeastern Asian area including China, Taiwan, Japan, Russia, etc., is a representative fresh-water fish species in Korea and has been widely used as an excellent food and oriental medicine. Not long ago, the mud loach was profusely found in rice fields and rivers. However, due to an accelerated contamination of rivers and fields along with the abuse of pesticides, the amount of natural catch decreases every year. Considering that such a condition is not limited to only mud loaches, development of new fish culturing techniques as well as the improvement of fish breeds is required for an effective use and preservation of native fish resources. For this purpose, such research on the production of genetically improved fish through the recombination technology using a useful fish gene should be required.
The research for the production of a transformed fish by the recombinant gene began in the late 1970's, in which a growth hormone gene was widely used. A growth hormone is a protein hormone whose structure and biological characteristics are similar with prolactin (PRL), chorionic somatomammotropin (CS; placental lactogen) and somato-lactin (SL). In all vertebrates, the growth hormone and PRL are produced in somatotroph and lactotroph of hypophysis, respectively, CS is produced in syncytotrophoblast of mammalian placenta, and SL in the pars intermedia cell of fish hypophysis. Synthesis and release of growth hormones are controlled by the GH releasing hormone (GRH) and GH release-inhibiting hormone (GIH; somatostatin). In case the glucose concentration in blood decreases, growth hormones are synthesized and released through the stimulation of GRH (Ecker, R., 1988,
Chemical messengers and regulators, In: Animal physiology,
3rd ed. Freeman and company. pp. 266-328).
Growth hormones are expressed during a germ generation process (Pantaleon, M., E. J. Whiteside, M. B. Harvey, R. T.
Barnard, M. J. Waters, and P. L. Kaye, 1997,
Proc. Natl. Acad. Sci. USA.,
94: 5125-5130) and involved in all normal metabolism needed for the growth process, including tissue growth, especially stimulates growth of bones due to cartilage proliferation. Tissue growth is due, to the increase of the number of cells. The growth process through the growth hormone is achieved by stimulation of the production of growth promoting factors (somatomedins) such as IGF-1 not by the direct stimulation of cell growth. As biochemical functions of the growth hormone in living bodies occur, they increase the transportation of amino acids into muscle cells and protein synthesis. Further, they are involved in carbohydrate metabolism, that is, decreasing glucose utilization and increasing glucose synthesis in the liver, which is an antagonistic action to insulin. With relation to lipid metabolism, the growth hormone stimulates the release of fatty acids and glycerol from adipose tissue. Also, it relates to inorganic metabolism such as ion balance and stimulates cartilage formation and bone growth (Bentley, P. J., 1982,
Comparative vertebrate endocrinology,
2nd ed. Cambridge Univ. Press, Cambridge. pp. 179-209; Murray, R. K., D. K. Granner, P. A. Mayers, and V. W. Rodwell, 1993,
Pituitary and hypothalamic hormones, In: Harper's Biochemistry.
23rd ed. Prentice-Hall Int., Inc. pp. 499-508).
Mammal growth hormone gene, whose size is about 2.5 kb, consists of five exons and four introns. Growth hormone genes of such fishes as rainbow trout, salmon and tilapia, whose size is about 4.5-5 kb, has six exons in which the 5th exon is divided by the 5th intron. Common carp have the same gene structure as humans and its gene size is about 3.5 kb. Tissue-specific expression of growth hormone and PRL is controlled by the transcription regulation protein, pit-1 and its upper transcription regulation factor, pit-1 binding site AA/TA/TTANCAT (SEQ ID NO:17) (Bodner, M., J. L. Castrillo, L. E. Theill, T. Deerinck, M. Ellisman, and M. Karin, 1988,
Cell
55: 505-518). It is also known that the thyroid hormones T3, T4 and glucocorticoid are involved in the synthesis of the growth hormone in mammals (Evans, R. M., N. C. Birnberg, and M. G. Rosenfield, 1982,
Proc. Natl. Acad. Sci. USA.
79: 7659-7663). However, such relations are not certain in fishes.
In early production of transformed fishes, mammal genes and their regulation sites are used. After a human growth hormone (hGH) was microinjected into goldfish (Zhu, Z., G. Liu, L. He, and S. Chen, 1985,
Z. Angew. Ichthyol.,
1: 31-43), it has been microinjected into many fishes including tilapia (Brem, G., B. Brenig, G. Horsgen-Schwark, and E. L. Winnacker, 1988,
Aquaculture,
68: 209-219), rainbow trout (Chourrout, D., R. Guyomard, C. Leroux, F. Pourrain, and L. M. Houdebine, 1988,
J. Cell Biochem. Suppl.,
121: 188) and catfish (Dunham, R. A., J. Eash, J. Askins, and T. M. Towners, 1987,
Trans. Am. Fish Soc.,
116: 87-91). Further, mouse growth hormone gene (Penman, D. J., A. J. Beeching, S. Penn, and N. Maclean, 1990, Aquaculture, 85: 35-50) and bovine growth hormone gene (Gross, M. L., J. F. Schneider, N. Moav, C. Alvarez, S. Myster, Z. Liu, C. L. Hew, E. M. Hallerman, P. B. Hackett, K. S. Guise, A. J. Faras, and A. R. Kapuscinski, 1991,
Aquaculture,
85: 115-128) are also used in microinjecting into fish genes.
In the experiments for producing transformed fish, such transgenes genes may be expressed and cause physiological changes. In some cases, however, such genes may be expressed without causing any physiological changes, or cannot be expressed at all. It is explained that non-expression is due to the fact that the gene regulation site of mammals cannot be recognized in fishes. Further, the reason that a specific hetero-gene cannot cause any physiological change despite its expression is that substrate-specific protein-protein interaction does not occur in cells. For example, growth hormone can effect its action through its binding with the growth hormone receptor in the surface of the cell wall. Likewise, in order that mammal growth hormone may be expressed in fishes and effect its action, interaction of mammal growth hormone with the fish growth hormone receptor must occur. Therefore, for effectiveness, the expression product of the gene to be transferred into fishes should have a structural similarity with that of fishes.
Among the successful cases of transfer of mammal growth hormone genes into fish cells, only few cases induced the increase of their growth rate, which shows the limitation of the expression of mammal genes in fish cells. Therefore, it is suggested that for an effective gene expression in fishes, genes and their regulation site should be selected from fishes, especially those of close classes. Therefore, for the improvement of a fish breed through gene recombination, cloning of fish-specific promoters and structural genes, along with the development of expression vectors used thereof is required.
After the growth hormone gene cDNA of rainbow trout was cloned and its sequence was identified (Agellon, L. B., and T. T. Chen, 1986,
DNA,
5: 463-471), the growth hormone gene cDNA and genome clone of several fishes including common carp have been separated. Zhang et al. (Zhang, P., M. Hyat, C. Joyce, L. I. Gonzalez-Villasenor, C. M. Lin, R. A. Dunham, T. T. Chen, and D. A. Powers, 1990,
Mol. Rep. Dev.,
25: 3-13) reported that growth hormone can be expressed
Cho Kyou-Nam
Kim Chul-Geun
Kim Dong-Soo
Nam Yoon-Kwon
Noh Jae-Koo
Chen Shin-Lin
Clark Deborah J. R.
Larson & Taylor PLC
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