CA2140785A1 - Non-native liver generation in an animal with impaired native liver function by cell implantation - Google Patents
Non-native liver generation in an animal with impaired native liver function by cell implantationInfo
- Publication number
- CA2140785A1 CA2140785A1 CA002140785A CA2140785A CA2140785A1 CA 2140785 A1 CA2140785 A1 CA 2140785A1 CA 002140785 A CA002140785 A CA 002140785A CA 2140785 A CA2140785 A CA 2140785A CA 2140785 A1 CA2140785 A1 CA 2140785A1
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- Prior art keywords
- native
- liver
- cells
- animal
- human
- Prior art date
- Legal status (The legal status is an assumption and is not a legal conclusion. Google has not performed a legal analysis and makes no representation as to the accuracy of the status listed.)
- Abandoned
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Classifications
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- A—HUMAN NECESSITIES
- A01—AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
- A01K—ANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
- A01K67/00—Rearing or breeding animals, not otherwise provided for; New or modified breeds of animals
- A01K67/027—New or modified breeds of vertebrates
- A01K67/0271—Chimeric vertebrates, e.g. comprising exogenous cells
-
- A—HUMAN NECESSITIES
- A61—MEDICAL OR VETERINARY SCIENCE; HYGIENE
- A61P—SPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
- A61P1/00—Drugs for disorders of the alimentary tract or the digestive system
- A61P1/16—Drugs for disorders of the alimentary tract or the digestive system for liver or gallbladder disorders, e.g. hepatoprotective agents, cholagogues, litholytics
Landscapes
- Life Sciences & Earth Sciences (AREA)
- Health & Medical Sciences (AREA)
- Environmental Sciences (AREA)
- Animal Behavior & Ethology (AREA)
- Chemical Kinetics & Catalysis (AREA)
- Nuclear Medicine, Radiotherapy & Molecular Imaging (AREA)
- Animal Husbandry (AREA)
- Zoology (AREA)
- Gastroenterology & Hepatology (AREA)
- Engineering & Computer Science (AREA)
- Bioinformatics & Cheminformatics (AREA)
- Chemical & Material Sciences (AREA)
- Cell Biology (AREA)
- General Chemical & Material Sciences (AREA)
- Medicinal Chemistry (AREA)
- Biodiversity & Conservation Biology (AREA)
- Organic Chemistry (AREA)
- Pharmacology & Pharmacy (AREA)
- General Health & Medical Sciences (AREA)
- Public Health (AREA)
- Veterinary Medicine (AREA)
- Medicines Containing Material From Animals Or Micro-Organisms (AREA)
- Micro-Organisms Or Cultivation Processes Thereof (AREA)
- Medicines Containing Plant Substances (AREA)
- Meat, Egg Or Seafood Products (AREA)
Abstract
Animals with impaired native liver function harboring a functioning non-native liver derived from implanted non-native cells, and a method of producing such animals are described.
Description
DescriPtion Non-Native Liver Generation in an Animal With ImPaired Native Liver Function, bY Cell ImPlantation Technical Field The invention relates to non-native functioning liver generation in animals with impaired native liver function, and to (transgenic) animals harboring functioning non-native livers.
Backqround Art There is a current notable shortage of donor livers. In 1990, illustratively, 2,656 liver transplants were performed, but 10 times more people died of liver disease. The treatment of liver disease by the implantation of healthy liver cells has long been envisioned as a potential solution to liver diseases.
Hepatocyte transplantation could be used to treat patients with congenital hepatic enzyme deficiencies to replace liver lost through disease (e.g. viral hepatitis, alcohol-related cirrhosis or fibrosis), or provide a temporary support system where acute liver dysfunction may be resolved by regeneration over a period of time. Hepatocyte transplantation also offers the opportunity to create animal models with human liver function. Such animals would be very useful for the study of viral infections affecting the liver (e.g. human hepatitis virus or cytomegalovirus infection) and/or test the effectiveness and safety of treatment or therapies for such infections. They would also be useful for the study of chemical (e.g. alcohol) toxicity in the human liver and chemical-induced cirrhosis and fibrosis and to test the - effectiveness and safety of treatments or therapies for chemical-induced liver damage.
Historically, several methods have been pursued in an attempt to create an auxiliary liver. Transplantation of liver fragments had been carried out as early as the 1930s. However, in most cases the transplanted liver tissue either degenerated or disappeared within a few days or weeks.
Greater success in hepatocyte transplants have been observed through the development of methods for isolating viable hepatocytes. Among these methods, the "digestion-perfusion"
method of Barry and Friend (J. Cell Biol.,`(1969) 43:506-520), block perfusion (Rees and Byard, In Vitro, (1981) 17:935-941), and injection-digestion (Woods et al, Transplantation, (1982) 33:123-126) have produced good yields of viable mature hepatocytes for injection. For a review see Gupta et al, HePatoloqy, (1992) 15:156-162.
In addition to problems in hepatocyte isolation, the method and site of implantation have been investigated for their effect on transplantation. Direct infusion of hepatocyte suspensions into the portal vein of rats has been investigated. However, contrary to initial beliefs, the portal blood supply was not found to be paramount to hepatocyte survival. Demonstrations have been made for hepatocyte growth following intramuscular injection, abdominal cavity injection, spleen, liver and kidney inoculation, and injection into celiac or renal arteries. While the above-mentioned methods have been able to produce small amounts of viable implanted hepatocytes, the resulting hepatic contribution to function has been relatively small and often temporary.
Another currently investigated approach to liver transplant resides in the implantation of new liver cells on scaffolds of biodegradable polymers that are hoped to regenerate into masses and take over at least some of the native liver's functions.
Although it has been reported that with this approach liver cells on a matrix can survive and function in rats six months to a year after transplantation, implanted cell survival is low, and, in some animal trials, too much connective tissue grew into the matrix, binding tightly to the polymer and forming scar tissue preventing the liver cells from dispersing through the matrix WO94/02601 2 1 4 0 7 8 ~ PCT/US93/06830 ("Technology Review~ July 1992, pp. 12, 13).
In a different vein, transgenic animal technology has provided the means to create and analyze animal models of genetic diseases affecting virtually any organ to which transgene expression can be directed. Because of its involvement in many diseases of medical importance, the liver has been a frequent target for this type of analysis.
Among transgenes reported to be associated with liver lesions are those encoding growth hormone, which alters hepatocyte size and nuclear characteristics; oncogenes, which induce hepatic tumors; the hepatitis B virus large envelope polypeptide, which induces hepatocellular necrosis and carcinoma formation in adults; transforming growth fact ~, which causes both tumors and excessive liver growth; and a variant form of ~l-antitrypsin (AAT), which reproduces some characteristics of AAT deficiency disease in humans, including neonatal and adult hepatitis.
Because of the liver's large synthetic and secretory capability, targeting transgene expression to this organ also serves as a way to determine the systemic influence of overproduction of biologically potent molecules. This approach has previously been used to study the consequences of inappropriate plasminogen activator expression in vivo by introducing into mice a transgene bearing the urokinase-type plasminogen activator (uPA) coding sequence fused to the albumin enhancer/promoter (Heckel et al. Cell (19900 62:447-456).
Plasminogen activators catalyze the proteolytic cleavage and activation of plasminogen to plasmin, which in turn degrades fibrin clots (Collen, D. and Lijnen, H.R. (1987) Fibrinolysis and the Control of Hematostasis. In the Molecular Basis of Blood Diseases. G. Stamatoyannopoulos, A.W. Nienhuis, P. Leder, and P.W. Majerus, eds. (Phila.: W.B. Saunders Co.), pp. 662-688).
2~ 40~ 4 -uPA also has been implicated in biological processes involving tissue remodeling or destruction, including ovulation, m~mm~ry gland involution, and metastasis (Dan0 et al., Adv. Cancer Res.
(1985) 44:149-265; Collen and Lijnen, (1987) supra; Saksela and Rifkin, Annu. Rev. Cell Biol. (1988) 4: 93-126) .
In many transgenic founder mice the albumin-urokinase type plasminogen activator (Alb-uPA) construct directed high-level uPA
expression to hepatocytes, resulting in elevated plasma uPA and fatal hemorrhaging in newborns. Two lines of Alb-uPA transgenic mice were established from surviving founder mice that expressed lower levels of uPA. In these lines, about half of the transgenic neonates bled into either the intestine or abdomen and died within four days after birth, whereas the remaining transgenic offspring appeared normal and survived. Both bleeding and non-bleeding transgenic neonates displayed marked hypofibrinogenemia and unclottable blood, and it was concluded that any injury sufficient to initiate bleeding was rapidly fatal in affected mice (Heckel et al. (199O), supra).
A general expectation in experiments of this type is that transgene expression will be stable over time in targeted cells.
Unexpectedly, surviving mice in both of the Alb-uPA lines showed a gradual decrease in the level of plasma uPA activity accompanied by a restoration of clotting function that was complete between 1 and 2 months of age (Heckel et al., (199O) supra) . This phenomenon has been explained by a report that uPA
is cytotoxic for hepatocytes and that inactivation of transgene expression by DNA rearrangement in isolated hepatocytes in Alb-uPA mice is followed by repopulation of the entire liver by cells that no longer produce uPA (Sandgren et al, Cell (1991) 66:245-256) . Thus, Alb-uPA expression provides a transgenic mouse in which endogenous transgene-expressing hepatocytes have a selected disadvantage relative to hepatocytes (native or non-native) that are not expressing the transgene. In addition, the livers in these mice provide an environment for growth of hepatocytes (native or non-native) that are not expressing the transgene. These cells grow out at the expense of transgene-expressing cells and the result is livers with apparently normal architecture.
Disclosure of the Invention Despite progress made in the implantation and development of mature hepatocytes, present technology has not made possible the generation of a (functioning) non-native liver into an animal, particularly one with defective liver function. In humans, such technology would be useful in liver disease therapy and/or treatment. In non-human animals such technology would have considerable value, e.g. to provide models of (diseased) human liver function useful to study potential treatment and/or therapies for human liver disease.
Accordingly, one object of the invention is to provide a method of correcting defective liver function in an animal host by implanting particular non-native cells (or corresponding tissue) into the liver region of a host animal with impaired native liver function to thereby generate a functioning non-native liver in the host and correct the impaired liver function. Another object of the present invention is to provide transgenic, non-human animals (e.g. rodents such as mice) harboring a transgene that encodes a product that is disadvantageous, but not lethal, to native liver cells and thus impairs native liver function. These transgenic, non-human animals are useful as a host system for non-native (e.g. human) liver. Another object of the present invention is to provide non-human host animals that can both maintain and expand a fully-functioning non-native (e.g. human) liver tissue useful for (l) modeling liver disease, (2) liver tissue banking (e.g.
maintenance and expansion of liver tissue for later analysis and re-implantation back into donors), (3) testing pharmaceuticals for human liver toxicity in vivo, and/or (4) genetic manipulation W O 94/02601 i P(~r/US93/06830 2~ 40~ 8~ -6-prior to re-implantation (i.e., hepatocyte-directed gene therapy). Another object of the invention is to provide a method of generating a functioning non-native liver in a host animal by implanting non-native liver cells (or tissue) into a host animal with a genetically established defective liYer function. Another object of the invention is to provide non-human animals harboring a functioning non-native liver. Another object of the invention is to provide a novel method for maintaining full-differentiated, full-functioning donor (e.g. human) hepatocytes in an in vivo setting for genetic manipulation prior to return to the donors.
The genetic manipulation could include, for example, introducing expression vectors that direct the production of medically important proteins in the transplant recipient.
It has been discovered by the inventors that the above objects of the invention and other objects which will become apparent from the description of the invention given hereinbelow are satisfied by implanting non-native cells (e.g, fetal, neonatal or adult, non-hematopoietic liver stem, progenitor or mature cells; fetal, stem, progenitor or adult bile duct cells;
endodermal (e.g. pancreas or gut) cellsi (cultured) totipotent stem cells; or cultured animal cells), or corresponding tissue, into the liver region of a host animal having impaired native liver function, such that the implanted cells (or tissue) colonize the host animal and develop therein a functioning non-native liver.
Best Mode for Carryina Out the Invention Any animal having impaired native liver function may be used in accordance with the invention as a suitable host animal.
Suitable host animals therefore include fish, fowl (e.g.
chickens, ducks, geese, turkeys, etc.), or m~mm~l S such as rodents (e.g. mice or rats), guinea pigs, pigs, dogs, cats, rabbits, goats, sheep, horses, ruminants such as cows, monkeys, other non-human primates, as well as humans.
W094/02601 2 1 4 07 8 ~ PCT/US93/06830 _ Impairment of native liver function in the host animal may have occurred accidentally, e.g. through disease, such as cirrhosis, hepatitis, fibrosis or a genetic liver deficiency disease such as deficiencies in Factor IX, Factor VIII, LDL
receptor, or one of varied metabolic enzymes (e.g. phenylalanine hydroxylase), or any of the other hundreds of known metabolic diseases that affect the liver.
In a preferred embodiment, the invention is applied as therapy and/or treatment to such animals, including humans, suffering from liver failure. In this context, the invention is used as an alternative to liver transplant to restore liver function.
In another embodiment, a non-native liver is generated in a non-human animal in which liver insufficiency has been induced to obtain an animal model system with a functioning non-native (e.g. human or other animal) liver. In these non-human animals, impairment of native liver function may be purposefully achieved by compromising the native hepatocyte genetically so that they are at a selective disadvantage towards implanted non-native cells (e.g. hepatocytes).
In accordance with the invention, during normal turnover of hepatocytes, the implanted non-native hepatocytes have a proliferative advantage over the accidentally or purposely disadvantaged native hepatocytes and ultimately replace all of the native hepatocytes in the host. This provides a host harboring substantially few, if any native hepatocytes, but a functioning, substantially non-native, liver generated from the implanted non-native cells. (The liver generated is substantially non-native insofar as it is likely to comprise some non-hepatocyte cells found in the native liver and perhaps some native hepatocytes.) Genetic inducement of liver insufficiency in a non-human W O 94/02601 PC~r/US93/06830 2l407 8S -8-mammal may be achieved in accordance with this embodiment of the present invention with a transgenic, non-human animal harboring a transgene which encodes a product that is disadvantageous, but not immediately lethal, to native liver cells. Generally, any deleterious transgene product may be used that impairs cellular function to the extent that hepatocytes expressing the gene have a distinct growth disadvantage relative to cells that do not express a transgene (e.g. the implanted non-native hepatocytes).
Examples of such transgene products include any type of plasminogen activator, such as an urokinase-type or tissue-type plasminogen activator, or bacterial plasminogen activators (e.g.
strptokinase) or toxins such as an attenuated diphtheria toxin.
Other examples of transgene products useable in accordance with this embodiment of the present invention include agents that adversely affect the metabolism or growth potential of the native liver cells. Illustrative agents are agents which compromise the ability of the native liver cells to transmit growth factor signals (e.g. with dominant and negative transgenes affecting steps in signal transduction pathway) or by producing mutant proteins that clog circulatory pathway(s).
In an illustrative genetic inducement of liver failure, the expression of high levels of urokinase-type plasminogen activator (uPA) has been reported by the inventors to cause impaired liver function in m~mm~l S . Sandqren et al in Cell (1991) 99:245-256.
Surviving transgenic animals harboring Alb-uPA are born with a liver consisting of smooth, pale to nearly white tissue, "white liver," within which develop multiple reddish nodules which expand in size with age. The white areas represent original transgenic liver tissue while the red areas represent post-natal changes in some aspects of liver function and structure which give rise to red nodular growth. The white tissue samples express high levels of uPA mRNA whereas all samples of the red nodules lack detectable transgene expression.
This white liver tissue contains small hepatocytes with altered rough endoplasmic reticulum morphology but is neither necrotic or fibrotic. Expression of the uPA transgene appears to be deleterious to hepatocytes, but not immediately lethal.
This kind of genetic impairment of native liver function provides a suitable format for establishing regenerative liver outgrowths from either donor animals (e.g. humans) or endogenous liver cells that spontaneously cease uPA transgene expression through DNA
recombination and loss of all functional copies of the transgene tandem array.
In the later case, heterozygous Alb-uPA mice frequently develop regenerative liver nodules with normal reddish liver color that grow out at expense of surrounding "white" liver tissue and eventually reconstitute the liver. These "red" liver nodules are clonal outgrowth of single hepatocytes based on analysis of the transgene remnants left behind following transgene recombination. Hepatocytes that have deleted all functional transgenes, and lack detectable transgene express, acquire a selected advantage and quickly expand and replace the transgene-expressing hepatocytes in the surrounding "white tissue~. An embodiment that is an extension of these observations is that non-native (e.g. human) liver cells can be transplanted into these mice (or their functional equivalent) and, as a result of their inherent growth advantage over native, transgene-expressing liver cells, they grow out to reconstitute the liver at the expense of endogenous liver cells which do die or disappear.
According to this general genetic inducement method, a transgene that encodes a product which is disadvantageous, but not immediately lethal, to the liver cells of the host animal is constructed. The resulting fusion construct is inserted using known techniques into fertilized eggs followed by implantation into pregnant or pseudopregnant females. The progeny are then bred to produce offspring which express the construct, and which ~ 407 ~S -lo-have impaired native liver function.
A variety of different non-native cells (or corresponding tissue) may be used for implantation into t~he host in accordance with the invention. These cells (or tissue) may be fetal, neonatal and/or adult stem, pragenitor and/or mature non-hematopoietic liver cells. Preferably non-hematopoietic liver progenitor cells and more preferably non-hematopoietic liver stem cells are used. In this context, hepatocytes, which constitute about 60~ of the mammalian liver, may be used as the liver cells.
The non-native hepatocytic stem cells which may be used in the invention are distinct from fetal hematopoietic stem cells.
Fetal hematopoietic stem cells are precursors to the hematopoietic system, and have previously been used to generate a non-native hematopoietic system in a host.
Other non-native cells (or tissue) which may be used in accordance with the invention include (i) stem, progenitor and/or mature bile duct cells, (ii) endodermal tissue cells such as pancreas or gut cells, (iii) optionally cultured totipotent stem cells including (ES) cells or embryonic carcinoma (EC) cells, and/or (iv) cultured animal cells.
In a particularly preferred embodiment, totipotent animal stem cells are first cultured under conditions which control their differentiation, such as by using particular growth factors in the cell culture medium, and these cultured cells are then used to colonize the host animal. Totipotent animal stem cells can also (alternatively) be first treated or cultured with growth factors that enhance survival, promote replication, and/or selectively enrich for stem cells.
Animal cells (or tissue) from other sources, including but not limited to embryonic stem cells or fetal endoderm, can also be treated by growth factors or other substances to bring about differentiation of a particular cell lineage with characteristics of hepatic stem cells. Illustratively, embryonic stem cells or embryonal carcinoma cells can be stimulated to differentiate by retinoic acid or another inducer. Subsequent differentiation in culture along the endodermal or hepatocyte cell lineage can be achieved by stimulation with growth factors and/or selection, using known techniques and materials.
In an embodiment of the present invention, the non-native cells (or tissue) may by genetically engineered (using known techniques) to produce, in vivo in the host, a physiologically effective amount of one or more medically relevant protein and then transplanted in accordance with the present invention. This technique can be used to improve hepatocyte function in an animal, e.g, by producing Factor IX, LDL receptors, phenylalanine hydroxylase, etc. or to produce proteins of systemic value, e.g.
Factor VIII, adenosine de~m~n~se, or peptide hormones.
Thus, non-native cells (or tissue) to be implanted may be isolated from a donor animal, as noted below, and optionally cultured, using known techniques. For example, in accordance with an embodiment of the invention, non-hematopoietic liver stem, progenitor and/or mature cells are first isolated from the terminal or transitional bile ductiles of a mature donor animal other than the host animal, using known techniques. In another illustrative embodiment, hepatic cells may be isolated from the donor animal using known procedures, e.g. by extraction through a biopsy needle. Alternatively, hepatic cells may be isolated from the donor animal by collagenase perfusion of the portal vein.1 The donor animal used in accordance with the invention may 1See, e.g. , Soda et al, Blood (1984) 63, 270-276, or Claunig et al, In Vitro (1981) 17, 913-925.
W O 94/02601 . PC~r/US93/06830 2140~ 8S -12-be an animal of the same species or of a different species as compared to the host animal. Generally it is a different individual. The donor animal may be any animal harboring a normal functioning liver or an animal with a congenital or squired liver disease. In a preferred embodiment the donor animal is a human.
The non-native cells (or tissue) are then introduced into the host organism in a manner which provides for implantation of a sufficient number of the non-native cells into the liver region of the host animal to permit their development into a non-native liver. The present invention does not require the use of a polymeric matrix for supporting the implanted cells. Once implanted into the liver region of the host animal, the injected cells (or tissue) are subjected therein, by virtue of their location, to a variety of native biological signals to which the native liver is normally subjected and which provide for the growth and maintenance of implanted non-native liver cells in the host.
Thus, cells from a variety of sources may be used in accordance with the invention, since such cells are comprised of a mixture of cells of different degree of development (i.e., stem, progenitor and mature cells). These mixtures contain cells having a sufficiently primitive degree of development so that, when subjected to the biological environment of the host~s liver area, these cells will establish a functioning non-native liver.
Illustratively, other cells, particularly of endodermal origin, may be used to form a new liver. For example, Scarpelli et al in Laboratory Investiqation (1990) 62:552 reported identifying cells in the pancreas of hamsters, treated with carcinogens, which have the appearance of hepatocytes. These cells and others may form functional hepatocytes when placed in the appropriate environment (e.g. a failing liver) in accordance with the present invention.
Implantation into the host animal's liver area may be achieved using different techniques. Illustratively, a suspension of from lx103 to lx107, preferably lx104 to lx106, non-native cells, optionally together with additional adjuvants to promote the transplantation of the non-native cells (i.e., substances which are known to enhance non-native cell survival and/or division2), are administered (e.g. injected through a syringe needle) into any of several different sites where colonization of the non-native cells may be observed.
Suitable sites include the abdominal cavity, muscle tissue, kidney, pancreas, celiac artery, fat pads and/or subcutaneous area of the host animal. Preferred sites of administration in accordance with the invention, and which are preferably effectuated by injection, include the portal vein, the spleen, directly into the native liver, and the umbilical vein of the fetal host which leads to the fetal liver.
In accordance with the invention, if the host and donor are two different animals steps are taken prior to implantation to suppress potential host immune rejection of the implanted non-native cells. This may be achieved in a variety of ways, such as by treating the host animal with cyclosporin or any other material known to suppress the host's immunological system, e.g.
agents that are known to selectively destroy subgroups of the immune cell population of the host, such as T-cell destroying antibodies. Alternatively, tolerance in the host can be induced by transferring non-native cells to the thymus of the host before implantation (see, Rosselt et al, Science (1990) 249:1293-1295), or cells from an animal of the same strain as the host can be used. Still further, an immunodeficient host can be used, such as inbred strains of an animal (e.g. SCID mice or nude mice) bred to act as recipients of non-native cells.
2For example, cells can be introduced together with growth factors or other substances that enhance survival, implantation, and for growth.
21 40~ 8S -14-In an illustrative and preferred embodiment, the recipient for the non-native cells is a transgenic mouse with defective liver function, and human non-hematopoietic liver cells are used to generate the non-native liver. A suitable transgenic mouse is described by Sandgren et al in Cell, (l99l) 66:245-256, which is hereby incorporated by reference. The transgenic mouse described in this publication of the inventors exhibits a high expression of albumin-urokinase-type plasminogen activator (Alb-uPA) fusion construct. This mouse with impaired liver function is a good recipient for human non-hematopoietic liver cell implantation (but mice with liver impairment resulting from other causes may be used).
The transgenic mouse with impaired liver function is injected with non-native, preferably human non-hematopoietic liver cells such that the injected human hepatocytic stem cells colonize the native liver at the expense of the endogenous "white tissue~ of the transgenic mouse. The human liver cells proliferate to form nodules which ultimately reconstitute the entire native liver of the host with human hepatocytes and establish human liver function. This includes the replacement of most mouse plasma proteins with their corresponding human plasma proteins.
The resulting mouse or any other non-human host produced in accordance with the invention, is well suited for (l) modeling study of human liver function, including screening pharmaceutical agents for treating human liver disease, (2) modeling human congenital diseases affecting the liver (including those in which the cause is unknown) by implanting patient liver cells into host mice, (3) liver cell banking (e.g. maintenance and expansion of liver tissue for later analysis or re-implantation into the donor), (4) genetic manipulation of full-functioning, full-differentiated hepatocytes for later re-implantation into donors (i.e., hepatocyte-directed gene therapy such as hepatitis virus resistant human liver cells that express antisense against the virus), and/or (5) modeling human liver for analysis of therapeutic agents that can promote liver regeneration.
More particularly, the present invention provides:
(i) Methods for maintaining and generating fully-functional, full-differentiated liver tissue for future analysis and therapeutic uses;
(ii) Therapeutic uses including: (a) re-implantation of healthy liver tissue into donor patients once an infectious agent or diseased tissue has been eliminated, and (b) genetic modification of donor cells and subsequent re-implantation into donor patients (e.g. hepatocyte-directed gene therapy);
(iii) Animal model systems with functioning, non-native liver (e.g. human hepatocytes) for the study of viral infections (e.g. human hepatitis virus or cytomegalovirus infection) and to test the effectiveness and safety of treatments or therapies for such infections;
(iv) Animal model systems with functioning, non-native (e.g. human) liver for the study of chemical (e.g. alcohol) toxicity in the liver and chemical-induced cirrhosis and fibrosis and to test the effectiveness and safety of treatments or therapies for chemical-induced liver damage;
(v) Methods for generating non-human animal models of congenital human liver disorders (even when the cause is not known) by reconstitution of host animal livers with human liver hepatocytes collected from patients diagnosed with liver disease;
(vi) Animal model systems with functioning, non-native (e.g. human) liver which models congenital human liver disorders (e.g. , glycogen storage diseases, a,-antitrypsin deficiency, coagulation factor disorders and deficiencies) for use in testing W O 94/02601 PC~r/US93/06830 the effectiveness and safety of treatments and therapies;
(vii) Methods for generating non-human animals in which the liver-derived plasma proteins (which comprise >90~ of the total plasma proteins) are derived from transplanted, non-native (e.g.
human) liver cells;
(viii) Animal systems with a functioning, non-native (e.g.
human) liver in which to generate and study normal or abnormal donor-liver derived plasma proteinsi (ix) Animal systems with a functioning, non-native (e.g.
human) liver for testing the effectiveness and safety of treatments or therapies for disorders affecting donor liver-derived plasma proteins; and (x) Systems for generating in large quantities of recombinant plasma proteins for therapeutic or diagnostic use.
Hepatocytes are equipped to assemble, and appropriately modify, copious amounts of plasma proteins; thus, transplanted hepatocytes, or their genetically engineered derivatives, may be used to generate valuable donor proteins or other derived proteins.
* * * * *
Obviously, numerous modifications and variations of the present invention are possible in light of the above teachings.
It is therefore to be understood that within the scope of the appended claims, the invention may be practiced otherwise than as specifically described herein.
Backqround Art There is a current notable shortage of donor livers. In 1990, illustratively, 2,656 liver transplants were performed, but 10 times more people died of liver disease. The treatment of liver disease by the implantation of healthy liver cells has long been envisioned as a potential solution to liver diseases.
Hepatocyte transplantation could be used to treat patients with congenital hepatic enzyme deficiencies to replace liver lost through disease (e.g. viral hepatitis, alcohol-related cirrhosis or fibrosis), or provide a temporary support system where acute liver dysfunction may be resolved by regeneration over a period of time. Hepatocyte transplantation also offers the opportunity to create animal models with human liver function. Such animals would be very useful for the study of viral infections affecting the liver (e.g. human hepatitis virus or cytomegalovirus infection) and/or test the effectiveness and safety of treatment or therapies for such infections. They would also be useful for the study of chemical (e.g. alcohol) toxicity in the human liver and chemical-induced cirrhosis and fibrosis and to test the - effectiveness and safety of treatments or therapies for chemical-induced liver damage.
Historically, several methods have been pursued in an attempt to create an auxiliary liver. Transplantation of liver fragments had been carried out as early as the 1930s. However, in most cases the transplanted liver tissue either degenerated or disappeared within a few days or weeks.
Greater success in hepatocyte transplants have been observed through the development of methods for isolating viable hepatocytes. Among these methods, the "digestion-perfusion"
method of Barry and Friend (J. Cell Biol.,`(1969) 43:506-520), block perfusion (Rees and Byard, In Vitro, (1981) 17:935-941), and injection-digestion (Woods et al, Transplantation, (1982) 33:123-126) have produced good yields of viable mature hepatocytes for injection. For a review see Gupta et al, HePatoloqy, (1992) 15:156-162.
In addition to problems in hepatocyte isolation, the method and site of implantation have been investigated for their effect on transplantation. Direct infusion of hepatocyte suspensions into the portal vein of rats has been investigated. However, contrary to initial beliefs, the portal blood supply was not found to be paramount to hepatocyte survival. Demonstrations have been made for hepatocyte growth following intramuscular injection, abdominal cavity injection, spleen, liver and kidney inoculation, and injection into celiac or renal arteries. While the above-mentioned methods have been able to produce small amounts of viable implanted hepatocytes, the resulting hepatic contribution to function has been relatively small and often temporary.
Another currently investigated approach to liver transplant resides in the implantation of new liver cells on scaffolds of biodegradable polymers that are hoped to regenerate into masses and take over at least some of the native liver's functions.
Although it has been reported that with this approach liver cells on a matrix can survive and function in rats six months to a year after transplantation, implanted cell survival is low, and, in some animal trials, too much connective tissue grew into the matrix, binding tightly to the polymer and forming scar tissue preventing the liver cells from dispersing through the matrix WO94/02601 2 1 4 0 7 8 ~ PCT/US93/06830 ("Technology Review~ July 1992, pp. 12, 13).
In a different vein, transgenic animal technology has provided the means to create and analyze animal models of genetic diseases affecting virtually any organ to which transgene expression can be directed. Because of its involvement in many diseases of medical importance, the liver has been a frequent target for this type of analysis.
Among transgenes reported to be associated with liver lesions are those encoding growth hormone, which alters hepatocyte size and nuclear characteristics; oncogenes, which induce hepatic tumors; the hepatitis B virus large envelope polypeptide, which induces hepatocellular necrosis and carcinoma formation in adults; transforming growth fact ~, which causes both tumors and excessive liver growth; and a variant form of ~l-antitrypsin (AAT), which reproduces some characteristics of AAT deficiency disease in humans, including neonatal and adult hepatitis.
Because of the liver's large synthetic and secretory capability, targeting transgene expression to this organ also serves as a way to determine the systemic influence of overproduction of biologically potent molecules. This approach has previously been used to study the consequences of inappropriate plasminogen activator expression in vivo by introducing into mice a transgene bearing the urokinase-type plasminogen activator (uPA) coding sequence fused to the albumin enhancer/promoter (Heckel et al. Cell (19900 62:447-456).
Plasminogen activators catalyze the proteolytic cleavage and activation of plasminogen to plasmin, which in turn degrades fibrin clots (Collen, D. and Lijnen, H.R. (1987) Fibrinolysis and the Control of Hematostasis. In the Molecular Basis of Blood Diseases. G. Stamatoyannopoulos, A.W. Nienhuis, P. Leder, and P.W. Majerus, eds. (Phila.: W.B. Saunders Co.), pp. 662-688).
2~ 40~ 4 -uPA also has been implicated in biological processes involving tissue remodeling or destruction, including ovulation, m~mm~ry gland involution, and metastasis (Dan0 et al., Adv. Cancer Res.
(1985) 44:149-265; Collen and Lijnen, (1987) supra; Saksela and Rifkin, Annu. Rev. Cell Biol. (1988) 4: 93-126) .
In many transgenic founder mice the albumin-urokinase type plasminogen activator (Alb-uPA) construct directed high-level uPA
expression to hepatocytes, resulting in elevated plasma uPA and fatal hemorrhaging in newborns. Two lines of Alb-uPA transgenic mice were established from surviving founder mice that expressed lower levels of uPA. In these lines, about half of the transgenic neonates bled into either the intestine or abdomen and died within four days after birth, whereas the remaining transgenic offspring appeared normal and survived. Both bleeding and non-bleeding transgenic neonates displayed marked hypofibrinogenemia and unclottable blood, and it was concluded that any injury sufficient to initiate bleeding was rapidly fatal in affected mice (Heckel et al. (199O), supra).
A general expectation in experiments of this type is that transgene expression will be stable over time in targeted cells.
Unexpectedly, surviving mice in both of the Alb-uPA lines showed a gradual decrease in the level of plasma uPA activity accompanied by a restoration of clotting function that was complete between 1 and 2 months of age (Heckel et al., (199O) supra) . This phenomenon has been explained by a report that uPA
is cytotoxic for hepatocytes and that inactivation of transgene expression by DNA rearrangement in isolated hepatocytes in Alb-uPA mice is followed by repopulation of the entire liver by cells that no longer produce uPA (Sandgren et al, Cell (1991) 66:245-256) . Thus, Alb-uPA expression provides a transgenic mouse in which endogenous transgene-expressing hepatocytes have a selected disadvantage relative to hepatocytes (native or non-native) that are not expressing the transgene. In addition, the livers in these mice provide an environment for growth of hepatocytes (native or non-native) that are not expressing the transgene. These cells grow out at the expense of transgene-expressing cells and the result is livers with apparently normal architecture.
Disclosure of the Invention Despite progress made in the implantation and development of mature hepatocytes, present technology has not made possible the generation of a (functioning) non-native liver into an animal, particularly one with defective liver function. In humans, such technology would be useful in liver disease therapy and/or treatment. In non-human animals such technology would have considerable value, e.g. to provide models of (diseased) human liver function useful to study potential treatment and/or therapies for human liver disease.
Accordingly, one object of the invention is to provide a method of correcting defective liver function in an animal host by implanting particular non-native cells (or corresponding tissue) into the liver region of a host animal with impaired native liver function to thereby generate a functioning non-native liver in the host and correct the impaired liver function. Another object of the present invention is to provide transgenic, non-human animals (e.g. rodents such as mice) harboring a transgene that encodes a product that is disadvantageous, but not lethal, to native liver cells and thus impairs native liver function. These transgenic, non-human animals are useful as a host system for non-native (e.g. human) liver. Another object of the present invention is to provide non-human host animals that can both maintain and expand a fully-functioning non-native (e.g. human) liver tissue useful for (l) modeling liver disease, (2) liver tissue banking (e.g.
maintenance and expansion of liver tissue for later analysis and re-implantation back into donors), (3) testing pharmaceuticals for human liver toxicity in vivo, and/or (4) genetic manipulation W O 94/02601 i P(~r/US93/06830 2~ 40~ 8~ -6-prior to re-implantation (i.e., hepatocyte-directed gene therapy). Another object of the invention is to provide a method of generating a functioning non-native liver in a host animal by implanting non-native liver cells (or tissue) into a host animal with a genetically established defective liYer function. Another object of the invention is to provide non-human animals harboring a functioning non-native liver. Another object of the invention is to provide a novel method for maintaining full-differentiated, full-functioning donor (e.g. human) hepatocytes in an in vivo setting for genetic manipulation prior to return to the donors.
The genetic manipulation could include, for example, introducing expression vectors that direct the production of medically important proteins in the transplant recipient.
It has been discovered by the inventors that the above objects of the invention and other objects which will become apparent from the description of the invention given hereinbelow are satisfied by implanting non-native cells (e.g, fetal, neonatal or adult, non-hematopoietic liver stem, progenitor or mature cells; fetal, stem, progenitor or adult bile duct cells;
endodermal (e.g. pancreas or gut) cellsi (cultured) totipotent stem cells; or cultured animal cells), or corresponding tissue, into the liver region of a host animal having impaired native liver function, such that the implanted cells (or tissue) colonize the host animal and develop therein a functioning non-native liver.
Best Mode for Carryina Out the Invention Any animal having impaired native liver function may be used in accordance with the invention as a suitable host animal.
Suitable host animals therefore include fish, fowl (e.g.
chickens, ducks, geese, turkeys, etc.), or m~mm~l S such as rodents (e.g. mice or rats), guinea pigs, pigs, dogs, cats, rabbits, goats, sheep, horses, ruminants such as cows, monkeys, other non-human primates, as well as humans.
W094/02601 2 1 4 07 8 ~ PCT/US93/06830 _ Impairment of native liver function in the host animal may have occurred accidentally, e.g. through disease, such as cirrhosis, hepatitis, fibrosis or a genetic liver deficiency disease such as deficiencies in Factor IX, Factor VIII, LDL
receptor, or one of varied metabolic enzymes (e.g. phenylalanine hydroxylase), or any of the other hundreds of known metabolic diseases that affect the liver.
In a preferred embodiment, the invention is applied as therapy and/or treatment to such animals, including humans, suffering from liver failure. In this context, the invention is used as an alternative to liver transplant to restore liver function.
In another embodiment, a non-native liver is generated in a non-human animal in which liver insufficiency has been induced to obtain an animal model system with a functioning non-native (e.g. human or other animal) liver. In these non-human animals, impairment of native liver function may be purposefully achieved by compromising the native hepatocyte genetically so that they are at a selective disadvantage towards implanted non-native cells (e.g. hepatocytes).
In accordance with the invention, during normal turnover of hepatocytes, the implanted non-native hepatocytes have a proliferative advantage over the accidentally or purposely disadvantaged native hepatocytes and ultimately replace all of the native hepatocytes in the host. This provides a host harboring substantially few, if any native hepatocytes, but a functioning, substantially non-native, liver generated from the implanted non-native cells. (The liver generated is substantially non-native insofar as it is likely to comprise some non-hepatocyte cells found in the native liver and perhaps some native hepatocytes.) Genetic inducement of liver insufficiency in a non-human W O 94/02601 PC~r/US93/06830 2l407 8S -8-mammal may be achieved in accordance with this embodiment of the present invention with a transgenic, non-human animal harboring a transgene which encodes a product that is disadvantageous, but not immediately lethal, to native liver cells. Generally, any deleterious transgene product may be used that impairs cellular function to the extent that hepatocytes expressing the gene have a distinct growth disadvantage relative to cells that do not express a transgene (e.g. the implanted non-native hepatocytes).
Examples of such transgene products include any type of plasminogen activator, such as an urokinase-type or tissue-type plasminogen activator, or bacterial plasminogen activators (e.g.
strptokinase) or toxins such as an attenuated diphtheria toxin.
Other examples of transgene products useable in accordance with this embodiment of the present invention include agents that adversely affect the metabolism or growth potential of the native liver cells. Illustrative agents are agents which compromise the ability of the native liver cells to transmit growth factor signals (e.g. with dominant and negative transgenes affecting steps in signal transduction pathway) or by producing mutant proteins that clog circulatory pathway(s).
In an illustrative genetic inducement of liver failure, the expression of high levels of urokinase-type plasminogen activator (uPA) has been reported by the inventors to cause impaired liver function in m~mm~l S . Sandqren et al in Cell (1991) 99:245-256.
Surviving transgenic animals harboring Alb-uPA are born with a liver consisting of smooth, pale to nearly white tissue, "white liver," within which develop multiple reddish nodules which expand in size with age. The white areas represent original transgenic liver tissue while the red areas represent post-natal changes in some aspects of liver function and structure which give rise to red nodular growth. The white tissue samples express high levels of uPA mRNA whereas all samples of the red nodules lack detectable transgene expression.
This white liver tissue contains small hepatocytes with altered rough endoplasmic reticulum morphology but is neither necrotic or fibrotic. Expression of the uPA transgene appears to be deleterious to hepatocytes, but not immediately lethal.
This kind of genetic impairment of native liver function provides a suitable format for establishing regenerative liver outgrowths from either donor animals (e.g. humans) or endogenous liver cells that spontaneously cease uPA transgene expression through DNA
recombination and loss of all functional copies of the transgene tandem array.
In the later case, heterozygous Alb-uPA mice frequently develop regenerative liver nodules with normal reddish liver color that grow out at expense of surrounding "white" liver tissue and eventually reconstitute the liver. These "red" liver nodules are clonal outgrowth of single hepatocytes based on analysis of the transgene remnants left behind following transgene recombination. Hepatocytes that have deleted all functional transgenes, and lack detectable transgene express, acquire a selected advantage and quickly expand and replace the transgene-expressing hepatocytes in the surrounding "white tissue~. An embodiment that is an extension of these observations is that non-native (e.g. human) liver cells can be transplanted into these mice (or their functional equivalent) and, as a result of their inherent growth advantage over native, transgene-expressing liver cells, they grow out to reconstitute the liver at the expense of endogenous liver cells which do die or disappear.
According to this general genetic inducement method, a transgene that encodes a product which is disadvantageous, but not immediately lethal, to the liver cells of the host animal is constructed. The resulting fusion construct is inserted using known techniques into fertilized eggs followed by implantation into pregnant or pseudopregnant females. The progeny are then bred to produce offspring which express the construct, and which ~ 407 ~S -lo-have impaired native liver function.
A variety of different non-native cells (or corresponding tissue) may be used for implantation into t~he host in accordance with the invention. These cells (or tissue) may be fetal, neonatal and/or adult stem, pragenitor and/or mature non-hematopoietic liver cells. Preferably non-hematopoietic liver progenitor cells and more preferably non-hematopoietic liver stem cells are used. In this context, hepatocytes, which constitute about 60~ of the mammalian liver, may be used as the liver cells.
The non-native hepatocytic stem cells which may be used in the invention are distinct from fetal hematopoietic stem cells.
Fetal hematopoietic stem cells are precursors to the hematopoietic system, and have previously been used to generate a non-native hematopoietic system in a host.
Other non-native cells (or tissue) which may be used in accordance with the invention include (i) stem, progenitor and/or mature bile duct cells, (ii) endodermal tissue cells such as pancreas or gut cells, (iii) optionally cultured totipotent stem cells including (ES) cells or embryonic carcinoma (EC) cells, and/or (iv) cultured animal cells.
In a particularly preferred embodiment, totipotent animal stem cells are first cultured under conditions which control their differentiation, such as by using particular growth factors in the cell culture medium, and these cultured cells are then used to colonize the host animal. Totipotent animal stem cells can also (alternatively) be first treated or cultured with growth factors that enhance survival, promote replication, and/or selectively enrich for stem cells.
Animal cells (or tissue) from other sources, including but not limited to embryonic stem cells or fetal endoderm, can also be treated by growth factors or other substances to bring about differentiation of a particular cell lineage with characteristics of hepatic stem cells. Illustratively, embryonic stem cells or embryonal carcinoma cells can be stimulated to differentiate by retinoic acid or another inducer. Subsequent differentiation in culture along the endodermal or hepatocyte cell lineage can be achieved by stimulation with growth factors and/or selection, using known techniques and materials.
In an embodiment of the present invention, the non-native cells (or tissue) may by genetically engineered (using known techniques) to produce, in vivo in the host, a physiologically effective amount of one or more medically relevant protein and then transplanted in accordance with the present invention. This technique can be used to improve hepatocyte function in an animal, e.g, by producing Factor IX, LDL receptors, phenylalanine hydroxylase, etc. or to produce proteins of systemic value, e.g.
Factor VIII, adenosine de~m~n~se, or peptide hormones.
Thus, non-native cells (or tissue) to be implanted may be isolated from a donor animal, as noted below, and optionally cultured, using known techniques. For example, in accordance with an embodiment of the invention, non-hematopoietic liver stem, progenitor and/or mature cells are first isolated from the terminal or transitional bile ductiles of a mature donor animal other than the host animal, using known techniques. In another illustrative embodiment, hepatic cells may be isolated from the donor animal using known procedures, e.g. by extraction through a biopsy needle. Alternatively, hepatic cells may be isolated from the donor animal by collagenase perfusion of the portal vein.1 The donor animal used in accordance with the invention may 1See, e.g. , Soda et al, Blood (1984) 63, 270-276, or Claunig et al, In Vitro (1981) 17, 913-925.
W O 94/02601 . PC~r/US93/06830 2140~ 8S -12-be an animal of the same species or of a different species as compared to the host animal. Generally it is a different individual. The donor animal may be any animal harboring a normal functioning liver or an animal with a congenital or squired liver disease. In a preferred embodiment the donor animal is a human.
The non-native cells (or tissue) are then introduced into the host organism in a manner which provides for implantation of a sufficient number of the non-native cells into the liver region of the host animal to permit their development into a non-native liver. The present invention does not require the use of a polymeric matrix for supporting the implanted cells. Once implanted into the liver region of the host animal, the injected cells (or tissue) are subjected therein, by virtue of their location, to a variety of native biological signals to which the native liver is normally subjected and which provide for the growth and maintenance of implanted non-native liver cells in the host.
Thus, cells from a variety of sources may be used in accordance with the invention, since such cells are comprised of a mixture of cells of different degree of development (i.e., stem, progenitor and mature cells). These mixtures contain cells having a sufficiently primitive degree of development so that, when subjected to the biological environment of the host~s liver area, these cells will establish a functioning non-native liver.
Illustratively, other cells, particularly of endodermal origin, may be used to form a new liver. For example, Scarpelli et al in Laboratory Investiqation (1990) 62:552 reported identifying cells in the pancreas of hamsters, treated with carcinogens, which have the appearance of hepatocytes. These cells and others may form functional hepatocytes when placed in the appropriate environment (e.g. a failing liver) in accordance with the present invention.
Implantation into the host animal's liver area may be achieved using different techniques. Illustratively, a suspension of from lx103 to lx107, preferably lx104 to lx106, non-native cells, optionally together with additional adjuvants to promote the transplantation of the non-native cells (i.e., substances which are known to enhance non-native cell survival and/or division2), are administered (e.g. injected through a syringe needle) into any of several different sites where colonization of the non-native cells may be observed.
Suitable sites include the abdominal cavity, muscle tissue, kidney, pancreas, celiac artery, fat pads and/or subcutaneous area of the host animal. Preferred sites of administration in accordance with the invention, and which are preferably effectuated by injection, include the portal vein, the spleen, directly into the native liver, and the umbilical vein of the fetal host which leads to the fetal liver.
In accordance with the invention, if the host and donor are two different animals steps are taken prior to implantation to suppress potential host immune rejection of the implanted non-native cells. This may be achieved in a variety of ways, such as by treating the host animal with cyclosporin or any other material known to suppress the host's immunological system, e.g.
agents that are known to selectively destroy subgroups of the immune cell population of the host, such as T-cell destroying antibodies. Alternatively, tolerance in the host can be induced by transferring non-native cells to the thymus of the host before implantation (see, Rosselt et al, Science (1990) 249:1293-1295), or cells from an animal of the same strain as the host can be used. Still further, an immunodeficient host can be used, such as inbred strains of an animal (e.g. SCID mice or nude mice) bred to act as recipients of non-native cells.
2For example, cells can be introduced together with growth factors or other substances that enhance survival, implantation, and for growth.
21 40~ 8S -14-In an illustrative and preferred embodiment, the recipient for the non-native cells is a transgenic mouse with defective liver function, and human non-hematopoietic liver cells are used to generate the non-native liver. A suitable transgenic mouse is described by Sandgren et al in Cell, (l99l) 66:245-256, which is hereby incorporated by reference. The transgenic mouse described in this publication of the inventors exhibits a high expression of albumin-urokinase-type plasminogen activator (Alb-uPA) fusion construct. This mouse with impaired liver function is a good recipient for human non-hematopoietic liver cell implantation (but mice with liver impairment resulting from other causes may be used).
The transgenic mouse with impaired liver function is injected with non-native, preferably human non-hematopoietic liver cells such that the injected human hepatocytic stem cells colonize the native liver at the expense of the endogenous "white tissue~ of the transgenic mouse. The human liver cells proliferate to form nodules which ultimately reconstitute the entire native liver of the host with human hepatocytes and establish human liver function. This includes the replacement of most mouse plasma proteins with their corresponding human plasma proteins.
The resulting mouse or any other non-human host produced in accordance with the invention, is well suited for (l) modeling study of human liver function, including screening pharmaceutical agents for treating human liver disease, (2) modeling human congenital diseases affecting the liver (including those in which the cause is unknown) by implanting patient liver cells into host mice, (3) liver cell banking (e.g. maintenance and expansion of liver tissue for later analysis or re-implantation into the donor), (4) genetic manipulation of full-functioning, full-differentiated hepatocytes for later re-implantation into donors (i.e., hepatocyte-directed gene therapy such as hepatitis virus resistant human liver cells that express antisense against the virus), and/or (5) modeling human liver for analysis of therapeutic agents that can promote liver regeneration.
More particularly, the present invention provides:
(i) Methods for maintaining and generating fully-functional, full-differentiated liver tissue for future analysis and therapeutic uses;
(ii) Therapeutic uses including: (a) re-implantation of healthy liver tissue into donor patients once an infectious agent or diseased tissue has been eliminated, and (b) genetic modification of donor cells and subsequent re-implantation into donor patients (e.g. hepatocyte-directed gene therapy);
(iii) Animal model systems with functioning, non-native liver (e.g. human hepatocytes) for the study of viral infections (e.g. human hepatitis virus or cytomegalovirus infection) and to test the effectiveness and safety of treatments or therapies for such infections;
(iv) Animal model systems with functioning, non-native (e.g. human) liver for the study of chemical (e.g. alcohol) toxicity in the liver and chemical-induced cirrhosis and fibrosis and to test the effectiveness and safety of treatments or therapies for chemical-induced liver damage;
(v) Methods for generating non-human animal models of congenital human liver disorders (even when the cause is not known) by reconstitution of host animal livers with human liver hepatocytes collected from patients diagnosed with liver disease;
(vi) Animal model systems with functioning, non-native (e.g. human) liver which models congenital human liver disorders (e.g. , glycogen storage diseases, a,-antitrypsin deficiency, coagulation factor disorders and deficiencies) for use in testing W O 94/02601 PC~r/US93/06830 the effectiveness and safety of treatments and therapies;
(vii) Methods for generating non-human animals in which the liver-derived plasma proteins (which comprise >90~ of the total plasma proteins) are derived from transplanted, non-native (e.g.
human) liver cells;
(viii) Animal systems with a functioning, non-native (e.g.
human) liver in which to generate and study normal or abnormal donor-liver derived plasma proteinsi (ix) Animal systems with a functioning, non-native (e.g.
human) liver for testing the effectiveness and safety of treatments or therapies for disorders affecting donor liver-derived plasma proteins; and (x) Systems for generating in large quantities of recombinant plasma proteins for therapeutic or diagnostic use.
Hepatocytes are equipped to assemble, and appropriately modify, copious amounts of plasma proteins; thus, transplanted hepatocytes, or their genetically engineered derivatives, may be used to generate valuable donor proteins or other derived proteins.
* * * * *
Obviously, numerous modifications and variations of the present invention are possible in light of the above teachings.
It is therefore to be understood that within the scope of the appended claims, the invention may be practiced otherwise than as specifically described herein.
Claims (41)
1. A non-human animal harboring substantially no native functioning hepatocytes and a functioning substantially non-native liver generated from implanted non-native cells or tissues.
2. The non-human animal of Claim 1, wherein said substantially functioning non-native functioning liver is a human liver.
3. A primate according to Claim 1.
4. A primate according to Claim 2.
5. A mammal according to Claim 1.
6. A mammal according to Claim 2.
7. A rodent according to Claim 1.
8. A rodent according to Claim 2.
9. A non-human animal harboring a functioning substantially non-native liver, obtained by:
(i) implanting into the liver area of a non-human animal host having impaired native liver function, cells which are non-native to said non-human animal and which are at least one member selected from the group consisting of (i) non-native fetal, neonatal and adult non-hematopoietic liver stem, progenitor and mature cells, (ii) stem, progenitor and mature bile duct cells, (iii) non-native fetal, neonatal or adult stem, progenitor and mature endodermal tissue cells, (iv) totipotent stem cells, and (v) cultured animal cells, and (ii) allowing the non-native cells to develop into a functioning substantially non-native liver in said non-human animal host and thereby obtaining a non-human animal harboring substantially no native functioning hepatocytes and a functioning substantially non-native liver.
(i) implanting into the liver area of a non-human animal host having impaired native liver function, cells which are non-native to said non-human animal and which are at least one member selected from the group consisting of (i) non-native fetal, neonatal and adult non-hematopoietic liver stem, progenitor and mature cells, (ii) stem, progenitor and mature bile duct cells, (iii) non-native fetal, neonatal or adult stem, progenitor and mature endodermal tissue cells, (iv) totipotent stem cells, and (v) cultured animal cells, and (ii) allowing the non-native cells to develop into a functioning substantially non-native liver in said non-human animal host and thereby obtaining a non-human animal harboring substantially no native functioning hepatocytes and a functioning substantially non-native liver.
10. The non-human animal of Claim 9, wherein said non-native cells are fetal stem, progenitor or mature non-hematopoietic liver cells.
11. The non-human animal of Claim 9, wherein said non-native cells are stem, progenitor or adult bile duct cells.
12. The non-human animal of Claim 9, wherein said non-native cells are stem, progenitor or mature endodermal tissue cells.
13. The non-human animal of Claim 9, wherein said non-native cells are totipotent stem cells.
14. The non-human animal of Claim 9, wherein said animal and said non-native cells are from the same species.
15. The non-human animal of Claim 9, wherein said animal and said non-native cells are from different species.
16. The non-human animal of Claim 9, wherein said non-native cells are human cells.
17. The non-human animal of Claim 9, wherein said non-human animal is a transgenic animal harboring an albuminplasminogen activator transgene or its functional equivalent with regard to native liver function.
18. A rodent according to Claim 17.
19. A mouse according to Claim 17.
20. A non-human animal harboring substantially no native functioning hepatocytes and a functioning substantially non-native liver, obtained by implanting into the liver area of a non-human animal host suffering from impaired native liver function, non-native fetal, neonatal or adult stem, progenitor or mature non-hematopoietic liver cells and allowing said non-native cells to develop into a non-native liver in said non-human animal host.
21. A method for restoring liver function in a human host suffering from impaired native liver function, comprising implanting into the liver area of said human, fetal, neonatal or adult human non-hematopoietic liver stem, progenitor or mature cells which are non-native to said human host, and allowing said non-native cells to develop into a functioning non-native human liver in said human host.
22. The method of Claim 21, wherein said human host suffering from impaired native liver function has been diagnosed as suffering from cirrhosis or fibrosis of the liver.
23. The method of Claim 21, wherein said human host suffering from impaired native liver function has been diagnosed as suffering from hepatitis.
24. The method of Claim 21, wherein said human host suffering from impaired native liver function has been diagnosed as suffering from a genetic deficiency disease causing said impaired native liver function.
25. The method of Claim 21, wherein said human host suffering from impaired native liver function has suffered a trauma causing said defective liver function.
26. The method of Claim 21, wherein said implantation is achieved by injecting said non-native cells into the portal vein of said human host suffering from impaired native liver function.
27. The method of Claim 21, wherein said implantation is achieved by injecting said non-native cells into the spleen of said human host suffering from impaired native liver function.
28. The method of Claim 21, wherein said implantation is achieved by injecting said non-native cells into the liver of said human host suffering from impaired native liver function.
29. The method of Claim 21, wherein said implantation is achieved by injecting said non-native cells into the celiac artery of said human host suffering from impaired native liver function.
30. A method of restoring liver function in an animal with impaired liver function, said method comprising:
(a) implanting into the liver area of a host animal in need of restoration of liver function, cells which are non-native to said host animal and which are at least one member selected from the group consisting of (i) fetal, neonatal and adult non-hematopoietic liver stem, progenitor and mature cells, (ii) stem, progenitor and adult bile duct Cells, (iii) fetal, neonatal and adult stem, progenitor and mature endodermal tissue cells, and (iv) totipotent stem cells, and (v) cultured animal cells;
and (b) allowing said non-native cells to develop into a functioning non-native liver in said host animal.
(a) implanting into the liver area of a host animal in need of restoration of liver function, cells which are non-native to said host animal and which are at least one member selected from the group consisting of (i) fetal, neonatal and adult non-hematopoietic liver stem, progenitor and mature cells, (ii) stem, progenitor and adult bile duct Cells, (iii) fetal, neonatal and adult stem, progenitor and mature endodermal tissue cells, and (iv) totipotent stem cells, and (v) cultured animal cells;
and (b) allowing said non-native cells to develop into a functioning non-native liver in said host animal.
31. The method of Claim 30, wherein said implantation is achieved by injecting said non-native cells into the portal vein, spleen, liver, or celiac artery, of said host animal.
32. A method for obtaining an animal with a functioning non-native liver, said method comprising:
(a) implanting into a host animal with impaired native liver function, cells which are non-native to said host animal and which are least one member selected from the group consisting of (i) fetal, neonatal and adult non-hematopoietic liver stem, progenitor and mature cells, (ii) stem, progenitor and adult bile duct cells, (iii) fetal, neonatal and adult stem, progenitor and mature endodermal tissue cells, (iv) totipotent stem cells, and (v) cultured animal cells; and (b) allowing said non-native cells in said host to develop into a functioning non-native liver.
(a) implanting into a host animal with impaired native liver function, cells which are non-native to said host animal and which are least one member selected from the group consisting of (i) fetal, neonatal and adult non-hematopoietic liver stem, progenitor and mature cells, (ii) stem, progenitor and adult bile duct cells, (iii) fetal, neonatal and adult stem, progenitor and mature endodermal tissue cells, (iv) totipotent stem cells, and (v) cultured animal cells; and (b) allowing said non-native cells in said host to develop into a functioning non-native liver.
33. The method of Claim 34, wherein said host animal is a transgenic animal harboring a transgene which compromises native hepatocytes.
34. A method for screening a pharmaceutical agent for treatment or therapy of a human liver disorder or disease comprising using the animal of Claim 2.
35. A method for screening a pharmaceutical agent for treatment or therapy of a human liver disorders or disease comprising using the primate of Claim 4.
36. A method for screening a pharmaceutical agent for treatment or therapy of a human liver disorder or disease comprising using the mammal of Claim 6.
37. A method for screening a pharmaceutical agent for treatment or therapy of a human liver disorder or disease comprising using the rodent of Claim 8.
38. A method of using the animal of Claim 1, comprising using said animal for maintaining and generating fully-functional, fully-differentiated liver tissue for future analysis or therapeutic use.
39. A method of using the animal of Claim 9, wherein said animal is used for maintaining and generating fully-functional, fully-differentiated liver tissue for future analysis or therapeutic use.
40. The method of Claim 39, wherein said therapeutic use comprises: the reimplantation of healthy liver tissue into a donor patient from whom said cells which were non-native to said non-human animal were obtained, once an infectious agent or disease tissue has been eliminated from said donor patient.
41. A method for hepatocyte-directed gene therapy, comprising obtaining hepatocytes from a donor animal, genetically modifying said cells to enable them to produce a physiologically effective amount of at least one medically relevant protein, implanting said genetically modified cells into the non-human animal of Claim 1 to generate fully-functional, fully-differentiated and genetically modified liver tissue, and reimplanting said generated liver tissue into said donor animal.
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KR950703640A (en) * | 1992-10-09 | 1995-09-20 | 가일 케이,나우톤. | LIVER RESERVE CELLS |
US5980886A (en) * | 1994-12-14 | 1999-11-09 | University Of Washington | Recombinant vectors for reconstitution of liver |
US6107027A (en) * | 1994-12-14 | 2000-08-22 | University Of Washington | Ribozymes for treating hepatitis C |
WO1996039810A1 (en) * | 1995-06-07 | 1996-12-19 | Novartis Ag | Human hepatocellular tissue in chimeric immunocompromised animals |
US6034297A (en) * | 1997-09-26 | 2000-03-07 | Cedars-Sinai Medical Center | In vivo, animal model for expression of hepatitis C virus |
US6132708A (en) * | 1997-10-10 | 2000-10-17 | Oregon Health Sciences University | Liver regeneration using pancreas cells |
US6864402B1 (en) | 1998-09-18 | 2005-03-08 | Albert Einstein College Of Medicine Of Yeshiva University | Chronic hepatitis virus infection and clonal hepatocellular carcinoma in mouse repopulated livers |
WO2000040083A1 (en) * | 1999-01-05 | 2000-07-13 | Surrogen, Inc. | Chimeric animal with engrafted xenogeneic tissue and method for producing same |
US6525242B1 (en) | 1999-11-02 | 2003-02-25 | The University Of Connecticut | Propagation of human hepatocytes in non-human mammals |
US6995299B2 (en) | 1999-11-02 | 2006-02-07 | University Of Connecticut | Propagation of human hepatocytes in non-human animals |
US6509514B1 (en) | 2000-03-17 | 2003-01-21 | Kmt Hepatech, Inc. | Chimeric animal model susceptible to human hepatitis C virus infection |
WO2001087059A1 (en) * | 2000-05-19 | 2001-11-22 | Japan Science And Technology Corporation | Chimeric animal |
WO2003080821A1 (en) * | 2002-03-25 | 2003-10-02 | Japan Science And Technology Agency | Method of proliferating human hepatocytes and method of obtaining human hepatocytes |
JPWO2004006664A1 (en) * | 2002-07-16 | 2005-11-10 | 独立行政法人科学技術振興機構 | Model animal transplanted with non-cancerous liver tissue and production method thereof |
DE602005020042D1 (en) * | 2004-08-20 | 2010-04-29 | Phoenixbio Co Ltd | METHOD FOR EVALUATING THE METABOLISM OF A MEDICAMENT IN THE HUMAN LIVER AND THE LIVER FUNCTION |
JP2008510465A (en) | 2004-08-20 | 2008-04-10 | ケイエムティー ヒパテック インコーポレイテッド | Malaria animal model with chimeric human liver |
US11172657B2 (en) | 2017-09-19 | 2021-11-16 | Pormedtec Co., Ltd. | Method for developing organ that lacks specific functional cell |
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WO1994002601A1 (en) | 1994-02-03 |
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