WO2002064748A2 - Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof - Google Patents

Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof Download PDF

Info

Publication number
WO2002064748A2
WO2002064748A2 PCT/US2002/004652 US0204652W WO02064748A2 WO 2002064748 A2 WO2002064748 A2 WO 2002064748A2 US 0204652 W US0204652 W US 0204652W WO 02064748 A2 WO02064748 A2 WO 02064748A2
Authority
WO
WIPO (PCT)
Prior art keywords
cells
masc
cell
vivo
progeny
Prior art date
Application number
PCT/US2002/004652
Other languages
French (fr)
Other versions
WO2002064748A8 (en
WO2002064748A9 (en
WO2002064748A3 (en
Inventor
Leo T. Furcht
Catherine M. Verfaillie
Morayma Reyes
Original Assignee
Furcht Leo T
Verfaillie Catherine M
Priority date (The priority date 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 date listed.)
Filing date
Publication date
Priority to JP2002565063A priority Critical patent/JP2004529621A/en
Application filed by Furcht Leo T, Verfaillie Catherine M filed Critical Furcht Leo T
Priority to NZ527527A priority patent/NZ527527A/en
Priority to IL15733202A priority patent/IL157332A0/en
Priority to US10/467,963 priority patent/US7838289B2/en
Priority to EP02718998A priority patent/EP1367899A4/en
Priority to CA2438501A priority patent/CA2438501C/en
Publication of WO2002064748A2 publication Critical patent/WO2002064748A2/en
Publication of WO2002064748A8 publication Critical patent/WO2002064748A8/en
Priority to IL214623A priority patent/IL214623A/en
Priority to IL157332A priority patent/IL157332A/en
Priority to ZA2003/06289A priority patent/ZA200306289B/en
Publication of WO2002064748A3 publication Critical patent/WO2002064748A3/en
Priority to US11/084,809 priority patent/US20050283844A1/en
Priority to US11/587,511 priority patent/US8609412B2/en
Priority to US11/151,689 priority patent/US8075881B2/en
Priority to US11/269,736 priority patent/US8147824B2/en
Publication of WO2002064748A9 publication Critical patent/WO2002064748A9/en
Priority to US11/446,560 priority patent/US7927587B2/en
Priority to US12/093,159 priority patent/US9962407B2/en
Priority to US13/042,205 priority patent/US20110177595A1/en
Priority to US13/105,372 priority patent/US8252280B1/en
Priority to IL214623A priority patent/IL214623A0/en
Priority to US13/301,186 priority patent/US9526747B2/en
Priority to US13/345,036 priority patent/US9808485B2/en

Links

Classifications

    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K39/00Medicinal preparations containing antigens or antibodies
    • A61K39/0005Vertebrate antigens
    • A61K39/001Preparations to induce tolerance to non-self, e.g. prior to transplantation
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K67/00Rearing or breeding animals, not otherwise provided for; New or modified breeds of animals
    • A01K67/027New or modified breeds of vertebrates
    • A01K67/0271Chimeric vertebrates, e.g. comprising exogenous cells
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P1/00Drugs for disorders of the alimentary tract or the digestive system
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P1/00Drugs for disorders of the alimentary tract or the digestive system
    • A61P1/16Drugs for disorders of the alimentary tract or the digestive system for liver or gallbladder disorders, e.g. hepatoprotective agents, cholagogues, litholytics
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P1/00Drugs for disorders of the alimentary tract or the digestive system
    • A61P1/18Drugs for disorders of the alimentary tract or the digestive system for pancreatic disorders, e.g. pancreatic enzymes
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P13/00Drugs for disorders of the urinary system
    • A61P13/10Drugs for disorders of the urinary system of the bladder
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P13/00Drugs for disorders of the urinary system
    • A61P13/12Drugs for disorders of the urinary system of the kidneys
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P15/00Drugs for genital or sexual disorders; Contraceptives
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P17/00Drugs for dermatological disorders
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P19/00Drugs for skeletal disorders
    • A61P19/04Drugs for skeletal disorders for non-specific disorders of the connective tissue
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P19/00Drugs for skeletal disorders
    • A61P19/08Drugs for skeletal disorders for bone diseases, e.g. rachitism, Paget's disease
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P21/00Drugs for disorders of the muscular or neuromuscular system
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P25/00Drugs for disorders of the nervous system
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P25/00Drugs for disorders of the nervous system
    • A61P25/02Drugs for disorders of the nervous system for peripheral neuropathies
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P27/00Drugs for disorders of the senses
    • A61P27/02Ophthalmic agents
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P3/00Drugs for disorders of the metabolism
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P3/00Drugs for disorders of the metabolism
    • A61P3/08Drugs for disorders of the metabolism for glucose homeostasis
    • A61P3/10Drugs for disorders of the metabolism for glucose homeostasis for hyperglycaemia, e.g. antidiabetics
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P31/00Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P31/00Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
    • A61P31/04Antibacterial agents
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P31/00Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
    • A61P31/10Antimycotics
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P31/00Antiinfectives, i.e. antibiotics, antiseptics, chemotherapeutics
    • A61P31/12Antivirals
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P35/00Antineoplastic agents
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P37/00Drugs for immunological or allergic disorders
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P37/00Drugs for immunological or allergic disorders
    • A61P37/02Immunomodulators
    • A61P37/06Immunosuppressants, e.g. drugs for graft rejection
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P39/00General protective or antinoxious agents
    • A61P39/02Antidotes
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P41/00Drugs used in surgical methods, e.g. surgery adjuvants for preventing adhesion or for vitreum substitution
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P43/00Drugs for specific purposes, not provided for in groups A61P1/00-A61P41/00
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P7/00Drugs for disorders of the blood or the extracellular fluid
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P7/00Drugs for disorders of the blood or the extracellular fluid
    • A61P7/04Antihaemorrhagics; Procoagulants; Haemostatic agents; Antifibrinolytic agents
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P7/00Drugs for disorders of the blood or the extracellular fluid
    • A61P7/06Antianaemics
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P7/00Drugs for disorders of the blood or the extracellular fluid
    • A61P7/08Plasma substitutes; Perfusion solutions; Dialytics or haemodialytics; Drugs for electrolytic or acid-base disorders, e.g. hypovolemic shock
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P9/00Drugs for disorders of the cardiovascular system
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61PSPECIFIC THERAPEUTIC ACTIVITY OF CHEMICAL COMPOUNDS OR MEDICINAL PREPARATIONS
    • A61P9/00Drugs for disorders of the cardiovascular system
    • A61P9/10Drugs for disorders of the cardiovascular system for treating ischaemic or atherosclerotic diseases, e.g. antianginal drugs, coronary vasodilators, drugs for myocardial infarction, retinopathy, cerebrovascula insufficiency, renal arteriosclerosis
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N15/00Mutation or genetic engineering; DNA or RNA concerning genetic engineering, vectors, e.g. plasmids, or their isolation, preparation or purification; Use of hosts therefor
    • C12N15/09Recombinant DNA-technology
    • C12N15/87Introduction of foreign genetic material using processes not otherwise provided for, e.g. co-transformation
    • C12N15/873Techniques for producing new embryos, e.g. nuclear transfer, manipulation of totipotent cells or production of chimeric embryos
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N5/00Undifferentiated human, animal or plant cells, e.g. cell lines; Tissues; Cultivation or maintenance thereof; Culture media therefor
    • C12N5/06Animal cells or tissues; Human cells or tissues
    • C12N5/0602Vertebrate cells
    • C12N5/0607Non-embryonic pluripotent stem cells, e.g. MASC
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N5/00Undifferentiated human, animal or plant cells, e.g. cell lines; Tissues; Cultivation or maintenance thereof; Culture media therefor
    • C12N5/06Animal cells or tissues; Human cells or tissues
    • C12N5/0602Vertebrate cells
    • C12N5/0618Cells of the nervous system
    • C12N5/0619Neurons
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N5/00Undifferentiated human, animal or plant cells, e.g. cell lines; Tissues; Cultivation or maintenance thereof; Culture media therefor
    • C12N5/06Animal cells or tissues; Human cells or tissues
    • C12N5/0602Vertebrate cells
    • C12N5/0618Cells of the nervous system
    • C12N5/0622Glial cells, e.g. astrocytes, oligodendrocytes; Schwann cells
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N5/00Undifferentiated human, animal or plant cells, e.g. cell lines; Tissues; Cultivation or maintenance thereof; Culture media therefor
    • C12N5/06Animal cells or tissues; Human cells or tissues
    • C12N5/0602Vertebrate cells
    • C12N5/067Hepatocytes
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2217/00Genetically modified animals
    • A01K2217/05Animals comprising random inserted nucleic acids (transgenic)
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2217/00Genetically modified animals
    • A01K2217/07Animals genetically altered by homologous recombination
    • A01K2217/075Animals genetically altered by homologous recombination inducing loss of function, i.e. knock out
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2227/00Animals characterised by species
    • A01K2227/10Mammal
    • A01K2227/105Murine
    • AHUMAN NECESSITIES
    • A01AGRICULTURE; FORESTRY; ANIMAL HUSBANDRY; HUNTING; TRAPPING; FISHING
    • A01KANIMAL HUSBANDRY; AVICULTURE; APICULTURE; PISCICULTURE; FISHING; REARING OR BREEDING ANIMALS, NOT OTHERWISE PROVIDED FOR; NEW BREEDS OF ANIMALS
    • A01K2227/00Animals characterised by species
    • A01K2227/10Mammal
    • A01K2227/106Primate
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K35/00Medicinal preparations containing materials or reaction products thereof with undetermined constitution
    • A61K35/12Materials from mammals; Compositions comprising non-specified tissues or cells; Compositions comprising non-embryonic stem cells; Genetically modified cells
    • AHUMAN NECESSITIES
    • A61MEDICAL OR VETERINARY SCIENCE; HYGIENE
    • A61KPREPARATIONS FOR MEDICAL, DENTAL OR TOILETRY PURPOSES
    • A61K48/00Medicinal preparations containing genetic material which is inserted into cells of the living body to treat genetic diseases; Gene therapy
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2501/00Active agents used in cell culture processes, e.g. differentation
    • C12N2501/10Growth factors
    • C12N2501/11Epidermal growth factor [EGF]
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2501/00Active agents used in cell culture processes, e.g. differentation
    • C12N2501/10Growth factors
    • C12N2501/113Acidic fibroblast growth factor (aFGF, FGF-1)
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2501/00Active agents used in cell culture processes, e.g. differentation
    • C12N2501/10Growth factors
    • C12N2501/115Basic fibroblast growth factor (bFGF, FGF-2)
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2501/00Active agents used in cell culture processes, e.g. differentation
    • C12N2501/10Growth factors
    • C12N2501/117Keratinocyte growth factors (KGF-1, i.e. FGF-7; KGF-2, i.e. FGF-12)
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2501/00Active agents used in cell culture processes, e.g. differentation
    • C12N2501/10Growth factors
    • C12N2501/119Other fibroblast growth factors, e.g. FGF-4, FGF-8, FGF-10
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2501/00Active agents used in cell culture processes, e.g. differentation
    • C12N2501/10Growth factors
    • C12N2501/12Hepatocyte growth factor [HGF]
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2501/00Active agents used in cell culture processes, e.g. differentation
    • C12N2501/10Growth factors
    • C12N2501/135Platelet-derived growth factor [PDGF]
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2501/00Active agents used in cell culture processes, e.g. differentation
    • C12N2501/20Cytokines; Chemokines
    • C12N2501/23Interleukins [IL]
    • C12N2501/235Leukemia inhibitory factor [LIF]
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2501/00Active agents used in cell culture processes, e.g. differentation
    • C12N2501/20Cytokines; Chemokines
    • C12N2501/237Oncostatin M [OSM]
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2502/00Coculture with; Conditioned medium produced by
    • C12N2502/08Coculture with; Conditioned medium produced by cells of the nervous system
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2502/00Coculture with; Conditioned medium produced by
    • C12N2502/30Coculture with; Conditioned medium produced by tumour cells
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2503/00Use of cells in diagnostics
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2506/00Differentiation of animal cells from one lineage to another; Differentiation of pluripotent cells
    • C12N2506/03Differentiation of animal cells from one lineage to another; Differentiation of pluripotent cells from non-embryonic pluripotent stem cells
    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12NMICROORGANISMS OR ENZYMES; COMPOSITIONS THEREOF; PROPAGATING, PRESERVING, OR MAINTAINING MICROORGANISMS; MUTATION OR GENETIC ENGINEERING; CULTURE MEDIA
    • C12N2517/00Cells related to new breeds of animals
    • C12N2517/02Cells from transgenic animals

Definitions

  • the present invention relates generally to mammalian multipotent adult stem cells (MASC), and more specifically to methods for obtaining, maintaining and differentiating MASC. Uses of MASC in the therapeutic treatment of disease are also provided.
  • MASC mammalian multipotent adult stem cells
  • Organ and tissue generation from stem cells, and their subsequent transplantation provide promising treatments for a number of pathologies, making stem cells a central focus of research in many fields.
  • Stem cell technology provides a promising alternative therapy for diabetes, Parkinson's disease, liver disease, heart disease, and autoimmune disorders, to name a few.
  • organ and tissue transplantation there are at least two major problems associated with organ and tissue transplantation.
  • the second major problem is the potential incompatibility of the transplanted tissue with the immune system of the recipient. Because the donated organ or tissue is recognized by the host immune system as foreign, immunosuppressive medications must be provided to the patient at a significant cost-both financially and physically.
  • Xenotransplantation or transplantation of tissue or organs from another species, could provide an alternative means to overcome the shortage of human organs and tissues.
  • Xenotransplantation would offer the advantage of advanced planning.
  • the organ could be harvested while still healthy and the patient could undergo any beneficial pretreatment prior to transplant surgery.
  • xenotransplantation does not overcome the problem of tissue incompatibility, but instead exacerbates it.
  • damaging viruses cross species barriers. Pigs have become likely candidates as organ and tissue donors, yet cross-species transmission of more than one virus from pigs to humans has been documented. For example, over a million pigs were recently slaughtered in Malaysia in an effort to contain an outbreak of Hendra virus, a disease that was transmitted to more than 70 humans with deadly results (Butler, D. 1999).
  • Stem cells Definition and use
  • stem cells can undergo self-renewing cell division to give rise to phenotypically and genotypically identical daughters for an indefinite time and ultimately can differentiate into at least one final cell type.
  • transplant tissues can be generated to provide the advantages associated with xenotransplantation without the associated risk of infection or tissue rejection.
  • Stem cells also provide promise for improving the results of gene therapy.
  • a patient's own stem cells could be genetically altered in vitro, then reintroduced in vivo to produce a desired gene product.
  • These genetically altered stem cells would have the potential to be induced to differentiate to form a multitude of cell types for implantation at specific sites in the body, or for systemic application.
  • heterologous stem cells could be genetically altered to express the recipient's major histocompatibility complex (MHC) antigen, or no MHC antigen, allowing transplantion of cells from donor to recipient without the associated risk of rejection.
  • MHC major histocompatibility complex
  • Stem cells are defined as cells that have extensive proliferation potential, differentiate into several cell lineages, and repopulate tissues upon transplantation.
  • the quintessential stem cell is the embryonic stem (ES) cell, as it has unlimited self- renewal and multipotent differentiation potential (Thomson, J. et al. 1995; Thomson, J. A. et al. 1998; Shamblott, M. et al. 1998; Williams, R.L. et al. 1988; Orkin, S.
  • ES and EG cells have been derived from mouse, and more recently also from non-human primates and humans. When introduced into mouse blastocysts, ES cells can contribute to all tissues of the mouse (animal) (Orkin, S. 1998). Murine ES cells are therefore pluripotent.
  • ES and EG cells When transplanted in post-natal animals, ES and EG cells generate teratomas, which again demonstrates their multipotency.
  • ES (and EG) cells can be identified by positive staining with the antibodies to stage-specific embryonic antigens (SSEA) 1 and 4.
  • SSEA stage-specific embryonic antigens
  • ES and EG cells express a number of transcription factors highly specific for these undifferentiated cells. These include oct-4 and Rex- 1, leukemia inhibitory factor receptor (LIF-R). The transcription factors sox-2 and Rox-1 are expressed in both ES and non-ES cells.
  • Oct-4 is expressed in the pregastrulation embryo, early cleavage stage embryo, cells of the inner cell mass of the blastocyst, and embryonic carcinoma (EC) cells. In the adult animal, oct-4 is only found in germ cells.
  • Oct-4 in combination with Rox-1, causes transcriptional activation of the Zn-finger protein Rex-1, and is also required for maintaining ES in an undifferentiated state.
  • the oct-4 gene is down-regulated when cells are induced to differentiate in vitro.
  • Sox-2 is required with oct-4 to retain the undifferentiated state of ES EC and to maintain murine, but not human, ES cells.
  • Human or murine primordial germ cells require presence of
  • HSC hematopoietic stem cell
  • HSC isolated from bone marrow (BM), blood, cord blood, fetal liver and yolk sac
  • BM bone marrow
  • fetal liver and yolk sac is the progenitor cell that generates blood cells or following translation reinitiates multiple hematopoietic lineages and can reinitiate hematopoiesis for the life of a recipient.
  • HSCs When transplanted into lethally irradiated animals or humans, HSCs can repopulate the erythroid, neutrophil-macrophage, megakaryocyte and lymphoid hemopoietic cell pool.
  • hemopoietic stem cells can be induced to undergo at least some self-renewing cell divisions and can be induced to differentiate to the same lineages as is seen in vivo. Therefore, this cell fulfills the criteria of a stem cell.
  • Stem cells which differentiate only to form cells of hematopoietic lineage, however, are unable to provide a source of cells for repair of other damaged tissues, for example, heart or lung tissue damaged by high-dose chemotherapeutic agents.
  • NSC neural stem cell
  • NSCs When cultured ex vivo, NSCs can be induced to proliferate, as well as to differentiate into different types of neurons and glial cells. When transplanted into the brain, NSCs can engraft and generate neural cells and glial cells. Therefore, this cell too fulfills the definition of a stem cell, albeit a hematopoetic stem cell.
  • Clarke et al. reported that NSCs from Lac-Z transgenic mice injected into murine blastocysts or in chick embryos contribute to a number of tissues of the chimeric mouse or chicken embryo (Clarke, D. L. et al. 2000). LacZ-expressing cells were found with varying degree of mosaicism, not only in the central nervous system, but also in mesodermal derivatives as well as in epithelial cells of the liver and intestine but not in other tissues, including the hematopoietic system.
  • adult NSCs may have significantly greater differentiation potential than previously realized but still do not have the pluripotent capability of ES or of the adult derived multipotent adult stem cells (MASC) described in Furcht et al. (International Application No. PCT/US00/21387) and hereia
  • the terms MASC, MAPC and MPC can also be used interchagably to describe adult derived multipotent adult stem cells. Therapies for degenerative and traumatic brain disorders would be significantly furthered with cellular replacement therapies.
  • NSC neurodegenerative senor senor senor senor senors .
  • SVZ sub-ventricular zone
  • hippocampus of the adult mammalian brain
  • SVZ sub-ventricular zone
  • hippocampus of the adult mammalian brain
  • Fetal or adult brain-derived NSC can be expanded ex vivo and induced to differentiate into astrocytes, oligodendrocytes and functional neurons (Ciccolini et al, 1998; Johansson et al, 1999; Palmer et al, 1999;- Reynolds et al, 1996; Ryder et al, 1990; Studer et al, 1996; Vescovi et al, 1993).
  • NSC neuronal and glial cells
  • GABAergic and dopaminergic neurons The most commonly used source of NSC is allogeneic fetal brain, which poses both immunological and ethical problems.
  • NSC could be harvested from the autologous brain. As it is not known whether pre-existing neural pathology will affect the ability of NSC to be cultured and induced to differentiate into neuronal and glial cells ex vivo, and because additional surgery in an already diseased brain may aggravate the underlying disease, this approach is less attractive.
  • the ideal source of neurons and glia for replacement strategies would be cells harvestable from adult, autologous tissue different than the brain that was readily accessible and that can be expanded in vitro and differentiated ex vivo or in vivo to the cell type that is deficient in the patient.
  • BM derived cells acquire phenotypic characteristics of neuroectodermal cells when cultured in vitro under NSC conditions, or when they enter the central nervous system (Sanchez-Ramos et al, 2000; Woodbury et al, 2000).
  • the phenotype of the BM cells with this capability is not known.
  • the capacity for differentiation of cells that acquire neuroectodermal features to other cell types is also unknown.
  • MSC mesenchymal stem cell
  • Fridenshtein (1982) A third tissue specific cell with stem cell properties is the mesenchymal stem cell (MSC), initially described by Fridenshtein (1982).
  • MSC originally derived from the embryonal mesoderm and isolated from adult BM, can differentiate to form muscle, bone, cartilage, fat, marrow stroma, and tendon.
  • the mesoderm develops into limb-bud mesoderm, tissue that generates bone, cartilage, fat, skeletal muscle and possibly endothelium.
  • Mesoderm also differentiates to visceral mesoderm, which can give rise to cardiac muscle, smooth muscle, or blood islands consisting of endothelium and hematopoietic progenitor cells.
  • MSCs Primitive mesodermal or MSCs, therefore, could provide a source for a number of cell and tissue types.
  • a number of MSCs have been isolated.
  • tissue-specific stem cells have been identified, including gastrointestinal stem cells (Potten, C. 1998), epidermal stem cells (Watt, F. 1997), and hepatic stem cells, also termed oval cells (Alison, M. et al. 1998). Most of these are less well characterized.
  • tissue specific stem cells Compared with ES cells, tissue specific stem cells have less self-renewal ability and, although they differentiate into multiple lineages, they are not pluripotent. No studies have addressed whether tissue specific cells express the markers described above as seen in ES cells. In addition, the degree of telomerase activity in tissue specific or lineage comitted stem cells has not been fully explored, in part because large numbers of highly enriched populations of these cells are difficult to obtain.
  • tissue specific stem cells could only differentiate into cells of the same tissue.
  • a number of recent publications have suggested that adult organ specific stem cells may be capable of differentiation into cells of different tissues.
  • the true nature of these types of cells has not been fully discerned.
  • a number of studies have shown that cells transplanted at the time of a BM transplant can differentiate into skeletal muscle (Ferrari 1998; Gussoni 1999). This could be considered within the realm of possible differentiation potential of mesenchymal cells that are present in marrow.
  • Jackson published that muscle satellite cells can differentiate into hemopoietic cells, again a switch in phenotype within the splanchnic mesoderm of the embryo (Jackson 1999).
  • stem cells from one embryonic layer can differentiate into tissues thought to be derived during embryogenesis from a different embryonic layer.
  • endothelial cells or their precursors detected in humans or animals that underwent marrow transplantation are at least in part derived from the marrow donor (Takahashi, 1999; Lin, 2000).
  • visceral mesoderm and not splanchnic mesoderm, capabilities such as MSC, derived progeny are transferred with the infused marrow.
  • stem cells isolated from a given organ may not necessarily be a lineage committed cell. Indeed most investigators did not identify the phenotype of the initiating cell. An exception is the study by Weissman and Grompe, who showed that cells that repopulated the liver were present in Lin ' Thy t LowSca ⁇ marrow cells, which are highly enriched in HSCs. Likewise, the Mulligan group showed that marrow Sp cells, highly enriched for HSC, can differentiate into muscle and endothelium, and Jackson et al. showed that muscle Sp cells are responsible for hemopoietic reconstitution (Gussoni et al, 1999).
  • ES cell research provides a promising alternative solution to the problem of a limited supply of organs for transplantation, the problems and risks associated with the need for immunosuppression to sustain transplantation of heterologous cells or tissue would remain.
  • An estimated 20 immunologically different lines of ES cells would need to be established in order to provide immunocompatible cells for therapies directed to the majority of the population.
  • stem cells with multiple differentiation potential have been isolated previously by others and by the present inventors, a progenitor cell with the potential to differentiate into a wide variety of cell types of different lineages, including fibroblasts, hepatic, osteoblasts, chondrocytes, adipocytes, skeletal muscle, endothelium, stroma, smooth muscle, cardiac muscle and hemopoietic cells, has not been described. If cell and tissue transplant and gene therapy are to provide the therapeutic advances expected, a stem cell or progenitor cell with the greatest or most extensive differentiation potential is needed. What is needed is the adult equivalent of an ES cell. BM, muscle and brain are the three tissues in which cells with apparent greater plasticity than previously thought have been identified.
  • BM contains cells that can contribute to a number of mesodermal (Ferrari G. et al, 1998; Gussoni E. et al, 1999; Rafii S. et al, 1994; Asahara T. et al, 1997; Lin Y. et al, 2000; Orlic D. et al, 2001; Jackson K. et al, 2001) endodermal (Petersen B.E. et al, 1999; Theise, N.D. et al, 2000; Lagasse E. et al, 2000; Krause D. et al, 2001) and neuroectodermal (Mezey D.S.
  • the present study demonstrates that cells with multipotent adult progenitor characteristics can be culture-isolated from multiple different organs, namely BM, muscle and the brain.
  • the cells have the same morphology, phenotype, in vitro differentiation ability and have a highly similar expressed gene profile.
  • the present invention is a multipotent adult stem cell (MASC) isolated from a mammal, preferably mouse, rat or human.
  • the cell is derived from a non- embryonic organ or tissue and has the capacity to be induced to differentiate to form at least one differentiated cell type of mesodermal, ectodermal and endodermal origin.
  • the organ or tissue from which the MASC are isolated is bone marrow, muscle, brain, umbilical cord blood or placenta.
  • the MASC of the present invention is also summarized as a cell that constitutively expresses oct4 and high levels of telomerase and is negative for CD44, MHC class I and MHC class II expression.
  • this cell administered to a patient in a therapeutically effective amount.
  • a surprising benefit of this treatment is that no teratomas are formed in vivo.
  • An object of the invention is to produce a normal, non-human animal comprising MASC.
  • the animal is chimeric.
  • Another embodiment of the invention is a composition comprising a population of MASC and a culture medium that expands the MASC population. It is advantageous in some cases for the medium to contain epidermal growth factor (EGF), platelet derived growth factor (PDGF) and leukemia inhibitory factor (LIF).
  • EGF epidermal growth factor
  • PDGF platelet derived growth factor
  • LIF leukemia inhibitory factor
  • the present invention also provides a composition comprising a population of fully or partially purified MASC progeny.
  • the progeny can have the capacity to be further differentiated, or can be terminally differentiated.
  • the progeny are of the osteoblast, chondrocyte, adipocyte, fibroblast, marrow stroma, skeletal muscle, smooth muscle, cardiac muscle, occular, endothelial, epithelial, hepatic, pancreatic, hematopoietic, glial, neuronal or oligodendrocyte cell type.
  • the present invention also provides a method for isolating and propagating MASC by obtaining tissue from a mammal, establishing a population of adherent cells, depleting the population of CD45 + cells, recovering CD45 " cells and culturing them under expansion conditions to produce an expanded cell population.
  • An object of the present invention therefore, is to produce an expanded cell population obtained by this method.
  • An aspect of the invention is a method for differentiating MASC ex vivo by isolating and propagating them, and then culturing the propagated cells in the presence of desired differentiation factors.
  • the preferred differentiation factors are basic fibroblast growth factor (bFGF), vascular endothelial growth factor (VEGF), dimethylsulfoxide (DMSO) and isoproterenol; or fibroblast growth factor4 (FGF4) and hepatocyte growth factor (HGF).
  • bFGF basic fibroblast growth factor
  • VEGF vascular endothelial growth factor
  • DMSO dimethylsulfoxide
  • FGF4 fibroblast growth factor4
  • HGF hepatocyte growth factor
  • the invention includes a method for differentiating MASC in vivo, by isolating and expanding them, and then administering the expanded cell population to a mammalian host, wherein said cell population is engrafted and differentiated in vivo in tissue specific cells, such that the function of a cell or organ, defective due to injury, genetic disease, acquired disease or iatrogenic treatments, is augmented, reconstituted or provided for the first time.
  • the MASC can undergo self-renewal in vivo.
  • a further aspect of the invention is a differentiated cell obtained by ex vivo or in vivo differentiation.
  • the differentiated cell is ectoderm, mesoderm or endoderm.
  • the differentiated cell is of the osteoblast, chondrocyte, adipocyte, fibroblast, marrow stroma, skeletal muscle, smooth muscle, cardiac muscle, occular, endothelial, epithelial, hepatic, pancreatic, hematopoietic, glial, neuronal or oligodendrocyte cell type.
  • An important application of this technology is the method of treating a patient by administering a therapeutically effective amount of MASC or their progeny.
  • the progeny can either have the capacity to be further differentiated, or can be terminally differentiated.
  • An unexpected benefit of this approach is that the need for pretreatment and/or post treatment of the patient with irradiation, chemotherapy, immunosuppressive agents or other drugs or treatments is reduced or eliminated. The induction of tolerance before or during treatment is also not required.
  • Such treatment can treat a variety of diseases and conditions, including cancer, cardiovascular disease, metabolic disease, liver disease, diabetes, hepatitis, hemophilia, degenerative or traumatic neurological conditions, autoimmune disease, genetic deficiency, connective tissue disorders, anemia, infectious disease and transplant rejection.
  • MASC or their progeny are administered via localized injection, including catheter administration, systemic injection, parenteral administration, oral administration, or intrauterine injection into an embryo. Administration can be in conjunction with a pharmaceutically acceptable matrix, which may be biodegradable.
  • MASC or their progeny, administered to a patient, alter the immune system to resist viral, bacterial or fungal infection.
  • MASC or their progeny are adminstered to a patient.
  • MASC or their progeny When administered to a patient, MASC or their progeny also are able to augment, reconstitute or provide for the first time the function of a cell or organ defective due to injury, genetic disease, acquired disease or iatrogenic treatments.
  • the organ is any of bone marrow, blood, spleen, liver, lung, intestinal tract, brain, immune system, circulatory system, bone, connective tissue, muscle, heart, blood vessels, pancreas, central nervous system, peripheral nervous system, kidney, bladder, skin, epithelial appendages, breast-mammary glands, fat tissue, and mucosal surfaces including oral esophageal, vaginal and anal.
  • diseases treatable by this method are cancer, cardiovascular disease, metabolic disease, liver disease, diabetes, hepatitis, hemophilia, degenerative or traumatic neurological conditions, autoimmune disease, genetic deficiency, connective tissue disorders, anemia, infectious disease and transplant rejection.
  • the MASC or their progeny home to one or more organs in the patient and are engrafted therein such that the function of a cell or organ, defective due to injury, genetic disease, acquired disease or iatrogenic treatments, is augmented, reconstituted or provided for the first time, which is surprising and unexpected.
  • the injury is ischemia or inflammation.
  • the MASC or their progeny enhance angiogenesis.
  • MASC or their progeny are genetically transformed to deliver a therapeutic agent, preferably an antiangiogenic agent.
  • the invention provides a therapeutic composition
  • a therapeutic composition comprising MASC and a pharmaceutically acceptable carrier, wherein the MASC are present in an amount effective to produce tissue selected from the group consisting of bone marrow, blood, spleen, liver, lung, intestinal tract, brain, immune system, bone, connective tissue,. muscle, heart, blood vessels, pancreas, central nervous system, kidney, bladder, skin, epithelial appendages, breast-mammary glands, fat tissue, and mucosal surfaces including oral esophageal, vaginal and anal.
  • tissue selected from the group consisting of bone marrow, blood, spleen, liver, lung, intestinal tract, brain, immune system, bone, connective tissue,. muscle, heart, blood vessels, pancreas, central nervous system, kidney, bladder, skin, epithelial appendages, breast-mammary glands, fat tissue, and mucosal surfaces including oral esophageal, vaginal and anal.
  • the invention further provides a therapeutic method for restoring organ, tissue or cellular function to a patient comprising the steps of removing MASC from a mammalian donor, expanding MASC to form an expanded population of undifferentiatied cells, and adminstering the expanded cells to the patient, wherein organ, tissue or cellular function is restored.
  • the restored function may be enzymatic or genetic.
  • the mammalian donor is the patient.
  • the invention provides a method of inhibiting the rejection of a heterologous MASC transplanted into a patient comprising the steps of introducing into the MASC, ex vivo, a nucleic acid sequence encoding the recipient's MHC antigen operably linked to a promotor, wherein the MHC antigen is expressed by the MASC and transplanting the MASC into the patient, wherein MHC antigen is expressed at a level sufficient to inhibit the rejection of the transplanted MASC.
  • the patient is of the same species or another mammalian species as the donor of the MASC.
  • An alternative method of inhibiting the rejection of a heterologous MASC transplanted into a patient comprises transgenically knocking out expression of MHC antigen in the MASC and transplanting the transgenic MASC into the patient MHC antigen is not expressed by the MASC and rejection of the transplanted cells is inhibited.
  • An object of the invention is a method of generating blood or individual blood components ex vivo by the process of isolating MASC and differentiating the MASC to form blood or blood components.
  • the individual blood components are red blood cells, white blood cells or platelets.
  • Another aspect of the invention is a method of drug discovery comprising the steps of analyzing the genomic or proteomic makeup of MASC or their progeny, employing analysis thereof via bioinformatics and/or computer analysis using algorithms, and assembling and comparing new data with known databases to compare and contrast these.
  • a further aspect is a method of identifying the components of a differentiation pathway comprising the steps of analyzing the genomic or proteomic makeup of MASC, inducing differentiation of MASC in vitro or in vivo, analyzing the genomic or proteomic makeup of intermediary cells in the differentiation pathway, analyzing the genomic or proteomic makeup of terminally differentiated cells in the differentiation pathway, using bioinformatics and/or algorithms to characterize the genomic or proteomic makeup of MASC and their progeny, and comparing the data obtained in (e) to identify the components of the pathway.
  • differentiation that occurs in vitro can be compared with differentiation that occurs in vivo such that fundamental differences between the two systems can be characterized.
  • the invention provides a method of generating products in vitro that have therapeutic, diagnostic or research utility by identifying the products in MASC and isolating the products from MASC.
  • the products are proteins, lipids, complex carbohydrates, DNA or RNA.
  • a method of inducing, in a mammal, tolerance to an antigen administered to said mammal comprising the step of administering to said mammal, after or simultaneously with the administration of said antigen, an effective amount of MASC or their progeny so that said mammal's humoral immune response to a subsequent challenge with said antigen is suppressed.
  • a method for removing toxins from the blood of a patient comprising contacting blood ex vivo with MASC derived cells, wherein said cells line a hollow, fiber based device.
  • the cells are kidney or liver cells.
  • An object of the invention is a method for delivering therapeutic products to a patient comprising contacting the blood of said patient ex vivo with MASC or their progeny, wherein said MASC or their progeny are genetically transformed to deliver a therapeutic agent.
  • a further object is a method for testing the toxicity of a drug comprising contacting MASC or their progeny ex vivo with said drug and monitoring cell survival.
  • the progeny are selected from the group consisting of hepatic, endothelial, epithelial and kidney.
  • Fig. 1 shows a graphical illustration of the expansion potential of of bone marrow (BM), muscle and brain derived MASC.
  • Fig. 2 shows a scatter plot representing gene expression in (A) muscle and brain MASC and (B) bone marrow and muscle MASC.
  • Fig. 3 shows a graphical illustration of FACS analysis of undifferentiated
  • MASC and MASC cultured with VEGF The plots show isotype control IgG staining profile (thin line) vs. specific antibody staining profile (thick line).
  • Panel A shows the phenotype . of undifferentiated MASC.
  • MASC express low levels of ⁇ 2- microglobulin, Flkl, Fit 1 and AC 133, but do not stain with any of the other anti- endothelial markers;
  • panel B shows the phenotype of MASC cultured for 14 days with 10 ng/mL VEGF.
  • MASC express low levels most markers associated with endothelial cells, but lost expression of AC 133; and
  • panel C shows phenotype of MASC cultured or 3-9 days with 10 ng/mL VEGF.
  • MASC lose expression of AC 133 by day 3 of culture with VEGF, acquire expression of Tek and VE-cadherin by day 3, Tie, vWF, CD34 and HIP12 by day 9.
  • Fig. 4 shows a photomicrograph of engraftment and in vivo differentiation of mMASC. Slides were examined by fluorescence or confocal microscopy. Panels A, G, J, N, Q and S represent identically stained tissues of control NOD-SCID animals that were not injected with mMASC. Panels A-F show a photomicrograph of bone marrow (BM) cytospin from a control (A) and study (B-F) animal stained with anti ⁇ -gal-FITC antibody and PE-conjugated antibodies to various hematopoietic antigens.
  • BM bone marrow
  • A control
  • B-F study
  • A-B CD45, C: CD19, D: MAC1, E: GR1, F:TER119 and DAPI;
  • panels G- I shows a photomicrograph of a spleen section from a control (G) and study animal (H, I) stained with anti- ⁇ -gal-FITC antibody and anti-CD45-PE antibody. Donor derived anti- ⁇ -gal + cells are seen in clusters. H is 10X and I are 60X magnifications;
  • panels J-M shows a photomicrograph of a liver section from a control mouse (J) and study animal (K-M) stained with anti- ⁇ -gal-FITC.
  • J-L are co-stained with mouse- anti-CK-18 / anti-mouse-Cy5 plus CD45-PE and M with mouse anti-albumin / anti- mouse Cy3 antibodies.
  • J-K, L and M are 20X, 60X and 10X magnifications respectively;
  • panels N-P show a photomicrograph of an intestine section from a control mouse and study animal (O-P), stained with anti- ⁇ -gal-FITC plus mouse- anti-pan-CK / anti-mouse-Cy5 antibodies (N-P).
  • N and P are costained with CD45- PE antibodies.
  • ⁇ -gal + Pan-CK + CD45 ' epithelial cells covered 50% (solid arrow, panel P) of the circumference of villi.
  • CD45 + / pan-CK " cells of hematopoietic origin are seen distinctly from the epithelial cells; and panels S-T show a photomicrograph of a blood vessel section from a control mouse (S) and thymic lymphoma that developed in a study animal 16 weeks after transplantation (T) stained with anti- ⁇ -gal-FITC, anti-vWF-PE and TO- PRO3.
  • ⁇ -gal + donor cells differentiated into vWF + endothelial cells in the thymic lymphoma which is of recipient origin, as the tumor cells did not stain with anti- ⁇ - Gal antibodies.
  • Fig. 5 shows immunohistochemical evaluation of MASC-derived endothelial cells using confocal fluorescence microscopy
  • Morphology in bright field of MASC at day 0 (upper panel) and day 21 (lower panel) after VEGF treatment. Bar 25 ⁇ m.
  • Fig. 6 shows a photomicrograph of MASC derived endothelial cells.
  • Panel A shows histamine-mediated release of vWF from MASC-derived endothelium. Staining with antibodies against myosin shows cytoskeletal changes with increased numbers of myosin stress fibers, and widening of gap junctions (Arrows) (Representative example of 3 experiments).
  • Scale bar 60 ⁇ m;
  • panel B shows MASC-derived endothelium takes up a-LDL. After 7 days, cells expressed Tie-1, but again did not take up a-LDL. However, acquisition of expression of vVWF on day 9 was associated with uptake of aLDL (representative example of 10 experiments).
  • Scale bar 100 ⁇ m; and panel C shows vascular tube formation by MASC-derived endothelium. After 6h, typical vascular tubes could be seen.
  • Fig. 7 shows a graphical illustration of FACS analysis of MASC derived endothelial cells.
  • the Plots show isotype control IgG staining profile (thin line) vs. specific antibody staining profile (thick line) (Representative example of >3 experiments). Number above plots is the Mean Fluorescence Intensity (MFI) for the control IgG staining and the specific antibody staining.
  • Panel A shows hypoxia upregulates Flkl and Tek expression on MASC-derived endothelial cells analyzed by flow cytometry;
  • panel B shows that hypoxia upregulates VEGF production by MASC-derived endothelial cells.
  • VEGF levels were measured by ELISA and the results are shown as Mean ⁇ SEM of 6 experiments; and panel C shows that IL-la induces expression of class II HLA antigens and increases expression of adhesion receptors.
  • Plots show isotype control IgG staining profile (thin line) vs. specific antibody staining profile (thick line) (Representative example of 3 experiments). Number above plots shows MFI for the control IgG staining and the specific antibody staining.
  • Fig. 8 shows a photomicrograph of human MASC derived endothelial cells.
  • Panels C-F show the 3-D reconstructed figures for either anti-human ⁇ 2- microglobulin-FITC (panel C) or anti-mouse-CD31-FITC (panel D) and merging of the two (Panel E), anti-vWF-Cy3 (panel F), and merging of the three staining patterns (Panel G).
  • C Cartilage.
  • D dermis.
  • Fig. 9 shows spiking behavior and expressed voltage-gated sodium currents in hMSC derived neuron-like cells.
  • Panel A shows a photomicrograph of cultured hMSC-derived neurons that showed spiking behavior and expressed voltage-gated sodium currents (the shadow of the pipette points to the cell).
  • Panel B shows graphical illustrations of current-clamp recordings from a hMSC derived neuron.
  • Panel C shows graphical illustrations of leak-subtracted current traces from the same hMSC derived neuron.
  • Fig. 10 shows quantitative RT-PCR and Western blot analysis confirming the hepatocyte-like phenotype.
  • Panels A and B show mMASC (A) and hMASC (B) cultured on MatrigelTM with FGF4 and HGF or FGF4 alone for 21 and 28 days respectively.
  • ⁇ FP Cyp2b9 and Cyp2bl3
  • numbers under the blots are relative to mRNA from liver, as no transcripts were detected in undifferentiated MASC.
  • Li mouse or human liver mRNA
  • NT no-template.
  • Panel C shows hMASC (B) cultured on MatrigelTM with FGF4 and HGF or FGF4 alone for 21 days.
  • FH FGF4 and HGF-induced hMASC on MatrigelTM
  • Huh Huh7 cell line used as control.
  • Fig. 11 shows a photomicrograph of hepatocyte-like cells.
  • MASC induced by FGF4 produce glycogen.
  • Glycogen storage is seen as accumulation of dark staining (Representative example of 3 studies).
  • Scale bar 25 ⁇ m.
  • Intermediary cells are cells produced during differentiation of a MASC that have some, but not all, of the characteristics of MASC or their terminally differentiated progeny. Intermediary cells may be progenitor cells which are committed to a specific pathway, but not to a specific cell type.
  • Normal shall mean an animal that is not diseased, mutated or malformed, i.e., healthy animals.
  • Self-renewal shall mean the ability of cells to propagate without the addition of external stimulation.
  • the presence of cytokines or other growth factors produced locally in the tissue or organ shall not constitute external stimulation.
  • Home shall mean the ability of certain MASC or their progeny to migrate specifically to sites where additional cells may be needed.
  • Knocking out expression shall mean the elimination of the function of a particular gene.
  • genomic or proteomic makeup shall mean the gene or protein components of a given cell. "High levels of telomerase activity” can be correlated to the two-fold level observed in the immortal human cell line MCF7. Soule et al. (1973) J. Cancer Inst. 51 :1409-1416. Application of this Technology
  • MASC technology could be used to replace damaged, diseased, dysfunctional or dead cells in the body of a mammal. Furthermore these cells could be injected into the host using autologous or allogeneic cells with or without nature or artificial supports, matrices or polymers to correct for loss of cells, abnormal function or cells or organs e.g. genetic such as mutations of genes affecting a protein function such as sickle cell disease, hemophilia or "storage diseases" where products accumulate in the body because of faulty processing, e.g. Guacher's, Neiman Pick's, mucopolysaccharidosis etc. Examples of restitution of dying or dead cells would be the use of MASC or their differentiated progeny in the treatment of macular degeneration and other neurodegenerative diseases.
  • Hepatocytes derived from autologous or allogeneic MASC, can be transplanted in this or other liver diseases. Such transplants may either transiently provide liver function to allow recovery of the recipient's own liver cells or permanently repopulate a damaged liver to allow recovery of normal liver function via the donor cells.
  • the progeny of the MASC could be differentiated ex vivo and then be administered as purified or even mixtures of cells to provide a therapeutic benefit.
  • MASC in the undifferentiated state could also be used as carriers or vehicles to deliver drugs or molecules of therapeutic benefit. This could be to treat any one of a number of diseases including but not limited to cancer, cardiovascular, inflammatory, immunologic, infections, etc.
  • a cell perhaps an endothelial cell expressing a novel or high levels of an angiogenic molecule could be administered to a patient which would be incorporated into existing blood vessels to promote angiogenesis, for example in the heart; correspondingly one could have endothelial cells producing molecules that might suppress angiogenesis that would be incorporated into blood cells and inhibit their further formation for example in diabetic retinopathy or in cancer where new blood vessel formation is key to the pathogenesis, spread and extent of the disease.
  • the ability to populate the BM and to form blood ex vivo has an untold use for important medical applications.
  • ex vivo production of blood the transfusion of blood and blood products around the world is still performed with variable safety because of transmission of infectious agents.
  • Blood transfusions have lead to HIV, hepatitis C and B, and now the impending threat of Mad Cow or CJD, Creuzfeldt- Jakob disease.
  • the ability to produce blood in vitro, especially red blood cells, could provide a safe and reliable alternative to collection of blood from people. It might never fully replace blood collection from donors.
  • hMASC or their hematopoietic progeny could be placed in animals in utero such as sheep which could form human hematopoietic cells and serve as a source for human blood components or proteins of therapeutic utility.
  • animals in utero such as sheep which could form human hematopoietic cells and serve as a source for human blood components or proteins of therapeutic utility.
  • the same could be true for hepatocytes, islets or many other cell types but would provide an alternative to producing human cells in vitro and use the animals as factories for the cells. It could also assist in blood shortages that are predicted to occur.
  • hMASC could also conceivably be transplanted into a human embryo to correct any one of a number of defects. Because these MASC can give rise to clonal populations of specifically differentiated cells they are a rich platform for drug discovery.
  • the information of how known drugs or agents might act could be compared to information derived from MASC, their differentiated progeny and from a population of people which could be available. Pathways, targets, and receptors could be identified. New drugs, antibodies or other compounds could be found to produce a biologically desirable responses.
  • the MASC and their differentiated progeny could be used as monitors for undesirable responses, coupled with databases, bioinformatics and algorithms.
  • MASC derived from human, mouse, rat or other mammals appear to be the only normal, non-malignant, somatic cell (non germ cell) known to date to express very high levels of telomerase even in late passage cells.
  • the telomeres are extended in MASC and they are karyotypically normal. Because MASC injected into a mammal, home to multiple organs, there is the likelihood that newly arrived MASC in a particular organ could be self renewing. As such, they have the potential to repopulate an organ not only with themselves but also with self renewing differentiated cell types that could have been damaged, died, or otherwise might have an abnormal function because of genetic or acquired disease.
  • pancreatic islets For example in type I diabetes there is a progressive loss of insulin producing beta cells in the pancreatic islets. In various renal diseases there is progressive loss of function and in some cases obliteration of glomerulus. If in the case of diabetes, MASC or differentiated progeny might home to the pancreas and themselves or via interaction with endogenous cells within the pancreas, induce islets to be formed. This would have an ameliorating impact on diabetes. Ultimately conditions, agents or drugs might be found to in vivo control, i.e.
  • MASC self renewing capability of the MASC and control, or enhance or inhibit the movement to differentiated progeny, e.g., islet precursors, hepatocyte precursors, blood precursors, neural and/or cardiac precursors using MASC one will likely find pathways, methods of activation and control that might induce endogenous precursor cells within an organ to proliferate and differentiation.
  • differentiated progeny e.g., islet precursors, hepatocyte precursors, blood precursors, neural and/or cardiac precursors using MASC
  • the present invention also provides methods for drug discovery, genomics, proteomics, and pathway identification; comprising analyzing the genomic or proteomic makeup of a MASC, coupled with analysis thereof via bioinformatics, computer analysis via algorithms, to assemble and compare new with known databases and compare and contract these. This will identify key components, pathways, new genes and/or new patterns of gene and protein expression and protein modification (proteomics) that could lead to the definition of targets for new compounds, antibodies, proteins, small molecule organic compounds, or other biologically active molecules that would have therapeutic benefit.
  • BM mononuclear cells were obtained by ficoll- hypaque separation of BM was obtained from 5-6 week old ROSA26 mice or C57/BL6 mice. Alternatively, muscle and brain tissue was obtained from 3-day old
  • Cells were dissociated by incubation with 0.1% trypsin and 0.1% DNAse (Sigma) for 30 minutes at 37 °C. Cells were then triturated vigorously and passed through a 70-um filter. Cell suspension was collected and centrifiiged for 10 minutes at 1600 rpm.
  • BMMNC or muscle or brain suspensions were plated at 1x10 /cm in expansion medium [2% FCS in low glucose Dulbecco's minimal essential medium
  • LG-DMEM 10 ng/mL each platelet derived growth factor (PDGF), epidermal growth factor (EGF) and leukemia inhibitory factor (LIF)] and maintained at
  • mMASC derived from BM, muscle and brain and cultured on FN were CD13 + , CD44 " , CD45 " , class-I and class-II histocompatibility antigen " , Flkl low and cKit " , identical to the characteristics of hMASC, as described in
  • mMASC cultured on FN were 8-10 ⁇ m in diameter with a large nucleus and scant cytoplasm. Several populations have been cultured for > 100 PDs. The morphology and phenotype of cells remained unchanged throughout culture. mMASC that had undergone 40 and 102 PDs were harvested and telomere lengths evaluated. Telomere length was measured using the Telomere Length Assay Kit from Pharmingen (New Jersey, USA) according to the manufacturer's recommendations.
  • telomere length (ATL) of mMASC cultured for 40 PDs was 27 Kb. When re-tested after 102 PDs, ATL remained unchanged.
  • karyotyping of mMASC cells were subcultured at a 1 :2 dilution 12h before harvesting, collected with trypsin-EDTA, and subjected to a 1.5h colcemid incubation followed by lysis with hypotonic KC1 and fixation in acid/alcohol as previously described (VerfaiUie et al, 1992). Cytogenic analysis was conducted on a monthly basis and showed a normal karyotype, except for a single. population that became hyperdiploid after 45 PDs, which was no longer used for studies.
  • Murine MASC obtained after 46 to >80 PDs were tested by Quantitative (Q)-
  • mRNA levels were normalized using GAPDH as housekeeping gene, and compared with levels in mouse ES cells.
  • Oct4 and Rex 1 mRNA were present at similar levels in BM, muscle and brain derived MASC.
  • Rexl mRNA levels were similar in mMASC and mES cells, while Oct4 mRNA levels were about 1,000 fold lower in MASC than in ES cells.
  • 3xl0 6 BM muscle or brain derived-MASC, cultured for 45 population doublings.
  • mMASC cultures have been maintained for more than 100 cell doublings. mMASC cultures have been initiated with marrow from C57B1/6 mice, ROSA26 mice and C57BL/6 mice transgenic for the -HMG-LacZ.
  • BM and MNC from Sprague Dawley or Wistar rats were obtained and plated under conditions similar for mMASC. After 21-28 days, cells were depleted of
  • CD45 + cells and the resulting CD45 " cells were subcultured at 10 cells/well.
  • rMASC Similar to mMASC, rMASC have been culture expanded for >100 PDs.
  • Expansion conditions of rat MASC culture required the addition of EGF, PDGF-BB and LIF and culture on FN, but not collagen type I, laminin or MatrigelTM.
  • rMASC were CD44, CD45 and MHC class I and II negative, and expressed high levels of telomerase. The ability of a normal cell to grow over 100 cell doublings is unprecedented, unexpected and goes against conventional dogma of more than two decades.
  • BM was obtained from healthy volunteer donors (age 2-50 years) after informed consent using guidelines from the University of Minnesota Committee on the use of Human Subject in Research.
  • BMMNC were obtained by Ficoll-Paque density gradient centrifugation and depleted of CD45 + and glycophorin-A + cells using micromagnetic beads (Miltenyii Biotec, Sunnyvale, CA).
  • VCAM vascular cell adhesion molecule
  • IAM intracellular adhesion molecule
  • Cultured cells were fixed with 4% paraformaldehyde and methanol at room temperature, and incubated sequentially for 30 min each with primary antibody, and with or without secondary antibody. Between steps, slides were washed with PBS/BSA. Cells were examined by fluorescence microscopy (Zeiss Axiovert; Carl Zeiss, Inc., Thornwood, NY) and confocal fluorescence microscopy (Confocal 1024 microscope; Olympus AX70, Olympus Optical Co. LTD, Japan). To assess the frequency of different cell types in a given culture, the number of cells were counted that stained positive with a given antibody in four visual fields (50-200 cells per field).
  • Antibodies Cells were fixed with 4% paraformaldehyde at room temperature or methanol at -20°C, and incubated sequentially for 30 min each with primary Ab, and FITC or Cy3 coupled anti-mouse- or anti-rabbit-IgG Ab. Between each step slides were washed with PBS+1 %BSA. PE or FITC-coupled anti-CD45, anti-CD31, anti-CD62E, anti-Macl, anti-Grl, anti-CD19, anti-CD3, and anti-Terl l9 antibodies were obtained from BD Pharmingen.
  • DAPI and TOPRO-3 were from Molecular Probes. Abs against vWF (polyclonal;
  • Neuro-D polyclonal, 1 :50
  • c-ret polyclonal, 1 :50
  • Nurrl polyclonal
  • NMDA polyclonal 1 :400 receptor from Chemicon International, Temecula, CA.
  • Anti-nestin (1 :400) Abs were a kind gift from Dr. U. Lendahl, University of Lund, Sweden.
  • Antibodies against NSE (1 :50) pan-cytokeratin (catalog number C-2562; 1 :100), CK-18 (C-8541; 1 :300), albumin (A-6684; 1 :100) were all obtained from Sigma.
  • Polyclonal antibodies against Flkl , Fltl , Tek, HNF-1 ⁇ were obtained from Santa Cruz Biotechnology Inc., Santa Cruz, CA.
  • Anti-nestin (1 :400) antibodies were a kind gift from Dr. U. Lendahl, University of Lund, Sweden.
  • Control-mouse, - rabbit or, -rat IgGs and FITC/PE/Cy3- and Cy5-labeled secondary antibodies were obtained from Sigma.
  • Rabbit anti- ⁇ -gal-FITC antibody was obtained from Rockland Immunochemicals, USA.
  • TO-PRO-3 was obtained from Molecular Probes Inc. and DAPI was obtained from Sigma.
  • X-GAL staining Tissue sections were stained by for ⁇ -galactosidase enzyme activity using ⁇ -gal staining kit from Invitrogen, pH 7.4. Manufacturer's instructions were followed except for the fixation step, during which the tissue sections were incubated for 5 min instead of 10 min.
  • FACS For FACS, undifferentiated MASC were detached and stained sequentially with anti-CD44, CD45, CD13, cKit, MHC-class I and II, or b2- microglobulin (BD Pharmingen) and secondary FITC or PE coupled antibodies, fixed with 2% paraformaldehyde until analysis using a FACS-Calibur (Becton- Dickinson).
  • the differentiation ability of mMASC or rMASC was tested by adding differentiation factors (cytokines) chosen based on what has been described for differentiation of hMASC or ES cells to mesoderm, neuroectoderm, and endoderm. Differentiation required that cells were replated at l-2xl0 4 cells/cm 2 in serum free medium, without EGF, PDGF-BB and LIF, but with lineage specific cytokines. Differentiation was determined by immunohistology for tissue specific markers
  • PDGF-BB and induced to differentiate by removal of PDGF and addition of bFGF as a differentiation factor.
  • mMASC and rMASC were plated in FN coated wells without PDGF-BB and EGF but with 100 ng/mL bFGF. Progressive maturation of neuron-like cells was seen throughout culture. After 7 days, the majority of cells expressed nestin. After 14 days, 15-20% of MASC acquired morphologic and phenotypic characteristics of astrocytes (GFAP + ), 15-20% of oligodendrocytes (galactocerebroside (GalC) + ) and 50-60% of neurons (neurofilament-200 (NF- 200) + ).
  • NF200, GFAP or GalC were never found in the same cell, suggesting that it is unlikely that neuron-like cells were hMASC or glial cells that inappropriately expressed neuronal markers.
  • Neuron-like cells also expressed Tau, MAP2 and NSE. Approximately 50% of neurons expressed gamma-amino-butyric-acid (GABA) and parvalbumin, 30% tyrosine hydroxylase and dopa-decarboxylase (DDC), and 20% serotonin and tryptophan hydroxylase. Differentiation was similar when MASC had been expanded for 40 or >90 PDs.
  • Q-RT-PCR performed as described in Example 1, confirmed expression of neuroectodermal markers: on day 2 MASC expressed otxl and otx2 mRNA, and after 7 days nestin mRNA was detected.
  • FGF-8b fibroblast growth factor-8b as a differentiation factor was tested next. This is important in vivo for midbrain development and used in vitro to induce dopaminergic and serotoninergic neurons from murine ES cells on hMASC.
  • GABA + GABA + ; 40 ⁇ 4%
  • DOPA dopaminergic
  • TrH serotoninergic
  • TrH serotonin and serotonin-transporter + , 34 ⁇ 6%
  • FGF-8b supported cultures with the glioblastoma cell line, U-87, and FGF-8b for an additional 2-3 weeks.
  • TTX tetrodotoxin
  • mMASC or rMASC were cultured in FN-coated wells with 10 ng/mL of the endothelial differentiation factor VEGF-B. Following treatment with VEGF for 14 days, >90% of MASC, irrespective of the number of PDs they had undergone, expressed Fltl, CD31, vWF or CD62, consistent with endothelial differentiation.
  • MASC-derived endothelial cells formed vascular tubes within 6 hours after replating in MatrigelTM.
  • hMASC express Flkl and Fltl but not CD34, Mucl8 (P1H12), PECAM, E- and P-selectin, CD36, or Tie/Tek.
  • VEGF vascular endothelial growth factor
  • cells expressed CD34, VE-cadherin, VCAM and Muc-18 from day 7 on.
  • Tie Tek, Flkl and Fltl, PECAM, P-selectin and E- selectin, CD36, vWF, and connexin-40.
  • LDL low- density lipoproteins
  • hMASC derived endothelial cells were administered intravenously (IN.) in ⁇ OD-SCI mice who have a human colon-carcinoma implanted under the skin, contribution of the human endothelial cells could be seen to the neovascularization in the tumors. It may therefore be possible to incorporate genetically modified endothelial cells to derive a therapeutic benefit, i.e., to inhibit angiogenesis in for example cancer or to promote it to enhance vascularization in limbs or other organs such as the heart. Further studies on MASC-derived endothelial cells are presented in Example 9. MASC Differentiation into Endoderm Whether mMASC or rMASC could differentiate to endodermal cells was tested.
  • Endodermal-like cells generated in FGF4 and HGF containing cultures also had functional characteristics of hepatocytes, determined by measuring urea levels in supernatants of undifferentiated MASC and FGF4 and HGF-induced MASC using the Sigma Urea Nitrogen Kit 640 according to the manufacturer's recommendations.. No urea was detected in undifferentiated MASC cultures. Urea production was 10 ⁇ g/cell/hr 14 days after adding FGF4 and HGF and remained detectable at similar levels until day 25. This is comparable to primary rat hepatocytes grown in monolayer. Presence of albumin together with urea production supports the notion of hepatic differentiation from MASC in vitro. Further studies on MASC-derived hepatocytes are presented in Example 11.
  • MASC likely give rise to a cell that forms various cells in the liver in the pancreas both exocrine and endocrine components and other endodermal derived cell tissue lineages.
  • MASC derived from muscle or brain were induced to differentiate to mesoderm (endothelial cells), neuroectoderm (astrocytes and neurons) and endoderm (hepatocyte-like cells) using the methods described above for BM-derived MASC.
  • hMASC hMASC + hMASC were diluted in non-transduced MASC from the same donors to obtain a final concentration of ⁇ 5% transduced cells. These mixtures were plated at 100 cells/well and culture expanded until >2xl0 7 cells were obtained. 5xl0 6 MASC each were induced to differentiate to skeletal myoblasts, endothelium and neuroectodermal lineages. After 14 days under differentiation conditions, cells were harvested and used to identify the retroviral integration site and co-expression of eGFP and neuroectodermal, muscle and endothelial markers.
  • hMASC For myoblast differentiation, hMASC were plated at 2xl0 4 cells/cm 2 in 2% FCS, EGF and PDGF containing expansion medium and treated with 3 ⁇ M 5- azacytidine in the same medium for 24h. Afterwards, cells were maintained in expansion medium with 2% FCS, EGF and PDGF-BB. For endothelial differentiation, hMASC were replated at 2xl0 4 cells/cm 2 in serum-free expansion medium without EGF and PDGF but with 10 ng/ml VEGF-B for 14 days.
  • Immunofluorescence evaluation showed that 5-10% of cells in cultures induced to differentiate with 5-azacytidine stained positive for eGFP and skeletal actin, 5- 10% of cells induced to differentiate to endothelium costained for eGFP and vWF, and 5-10% of cells induced to differentiate to neuroectoderm costained for eGFP and either NF-200, GFAP or MBP.
  • the retroviral insertion site the host genomic flanking region in MASC and differentiated progeny was sequenced. The number of retroviral inserts in the different populations was between one and seven.
  • VEGF TCCTGTCTCA TTCAAGCCAC ATCAGTTACA TCTGCATTTT
  • progeny differentiated into muscle, endothelium and neuroectoderm are derived from a single BM derived progenitor cell definitively proves for the first time that primitive cells can be cultured from BM that differentiate at the single cell level in cells of mesodermal lineage as well as the three different lineages of the neuroectoderm.
  • MSCV LTR MSCV LTR
  • Bold and underlined MSCV LTR primer used for Q-PCR
  • Flanking sequence primers used for Q-PCR Flanking sequence primers used for Q-PCR.
  • Example 6 Homing and Engraftment of Mammalian MASC into Numerous Organs in the Body mMASC were tested to determine whether they had the ability to engraft and differentiate in vivo into tissue specific cells.
  • mMASC were grown as described in Example 1 from a LacZ transgenic C57 Black 6, ROSA 26 mouse. 10 6 mMASC from the LacZ mouse were IN. injected into ⁇ OD-SCID mice tail veins with or without 250 Rads of total body radiation 4-6 hrs prior to the injection. The animals were sacrificed by cervical dislocation at 4-24 weeks after the injections. Tissue Harvest
  • Blood and bone marrow 0.5-1 ml of blood was obtained at the time animals were sacrificed.
  • BM was collected by flushing femurs and tibias.
  • red cells in blood and BM were depleted using ice cold ammonium chloride (Stem Cell Technologies Inc., Vancouver, Canada) and 10 5 cells used for cytospin centrifugation.
  • serial transplantation 5x10 cells from 2 femurs and 2 tibias were transplanted into individual secondary recipients via tail vein injection. Secondary recipients were sacrificed after 7-10 weeks.
  • Solid organs Lungs were inflated with 1 ml 1 :4 dilution of OCT compound
  • Engraftment defined as detection of >1% anti- ⁇ -gal cells, was seen in hematopoietic tissues (blood, BM and spleen) as well as epithelium of lung, liver, and intestine of all recipient animals as shown in Table 4 and Fig. 4.
  • Engraftment in the spleen occurred mostly as clusters of donor cells, consistent with the hypothesis that when MASC home to the spleen, they proliferate locally and differentiate to form a colony of donor cells, similar to CFU-S. It is not believed that differentiation of mMASC into hematopoietic cells in vivo can by attributed to contamination of the mMASC with HSC.
  • BMMNC are depleted of CD45 cells by column selection before mMASC cultures are initiated.
  • hematopoietic transcription factors including brachyury (Robertson et al, 2000), GATA-2 and GATA-1 (Weiss et al, 1995), are not expressed in undifferentiated mMASC, as shown by cDNA array analysis.
  • the culture conditions used for mMASC are not supportive for HCS.
  • each crypt contains a population of 4-5 long-lived stem cells (Potten, 1998). Progeny of these stem cells undergo several rounds of division in the middle and upper portions of cypts and give rise to epithelial cells that migrate upwards, out of the crypt, onto adjacent villi.
  • Donor derived, ⁇ -gal + panCK + CD45 epithelial cells entirely covered several villi (Fig. 40-
  • ⁇ -gal + panCK + CD45 cells constituted only 50% of the circumference (solid arrows, Fig. 4P) suggesting engraftment in one but not both crypts.
  • Several ⁇ -gal + panCK " cells were distinctly seen in the core of intestinal villi
  • ROSA26-MASC were infused and grown to confluence prior injection.
  • MASC allowed to become confluent lose their ability to differentiate ex vivo in cells outside of the mesoderm, and behave like classical MSC (Reyes, M. et al. 2001).
  • Infusion of 10 6 confluent mMASC did not yield significant levels of donor cell engraftment.
  • few ⁇ -gal + cells were seen in BM, these cells did not co-label with anti-CD45 Abs, indicating that MSC may engraft in tissues, but are no longer able to differentiate into tissue specific cells in response to local cues.
  • MASC derived cells in bone marrow of mice can be serially transferred BM from mouse engrafted with ROSA26 MASC was tested to determine whether they contained cells that would engraft in secondary recipients.
  • secondary recipients were sacrificed, and blood, BM, spleen, liver, lung and intestines of the recipient animal were analyzed for engraftment of ROSA26 donor cells by immunohistochemistry and Q- PCR for the ⁇ EO gene. A similar pattern of engraftment was seen in secondary recipients as in the primary recipients.
  • BM, spleen and PB cells were ⁇ - gal + CD45 + ; six and 8% of intestinal epithelial cells were ⁇ -gal + pan-CK + , and 4 and 5% of lung epithelial cells were ⁇ -gal + pan-CK + .
  • Levels of engraftment in the liver of secondary recipients were lower than in the primary recipients (1 and 3% vs. 5 and 8% ⁇ -gaf CK18 + ). This suggests that mMASC may persist in the BM of the primary recipient and differentiate into hematopoietic cells as well as epithelial cells when transferred to a second recipient.
  • MASC derived cells can produce insulin in vivo.
  • MASC from ROSA26 mice were injected into irradiated ⁇ OD-SCID mice as described herein.
  • the resulting MASC derived cells co-stain for LacZ and insulin in a model of streptozotocin-induced diabetes.
  • Summary One of the critical questions in "stem cell plasticity" is whether the engrafted and differentiated donor mMASC are functional. The results described herein show that one animal developed a lymphoma in thymus and spleen after 16 weeks, as is commonly see in aging ⁇ OD-SCID mice (Prochazka et al, 1992). Phenotypic analysis showed that this B-cell lymphoma was host-derived: CD19 + cells were ⁇ - gal " .
  • neoangiogenesis in the tumor was in part derived from donor mMASC (Fig. 4T). This suggests that MASC give rise to functioning progeny in vivo.
  • higher levels of mMASC engraftment and differentiation in radiosensitive organs, such as the hematopoietic system and intestinal epithelium (Table 4, p ⁇ 0.001), following low dose irradiation suggests that mMASC may contribute functionally to host tissues.
  • mammalian MASC can be purified, expanded ex vivo, and infused IN., homed to various sites in the body, engraft into numerous organs, and that the cells are alive in these various organs one month or longer.
  • donor cells, undifferentiated, and differentiated progeny are found, by virtue of the fluorescent marker, in organs including, but not limited to, the BM, spleen, liver and lung. These cells can be used to repopulate one or more compartment(s) to augment or restore cell or organ function.
  • MASC from, human BM differentiate at the single cell level into neuroectodermal, endodermal and many mesodermal lineages, including endothelial cells. Because endothelium and blood are very closely related in ontogeny, it can be hypothesized that MASC can differentiate into hematopoietic cells.
  • Remaining cells were transferred to methylcellulose cultures containing 10% fetal calf serum supplemented with 10 ng/mL bone morphogenic protein (BMP)4, VEGF, bFGF, stem cell factor (SCF), Flt3L, hyper IL6, thrombopoietin (TPO), and erythropoietin (EPO) for 2 weeks.
  • BMP bone morphogenic protein
  • VEGF bFGF
  • SCF stem cell factor
  • Flt3L Flt3L
  • TPO thrombopoietin
  • EPO erythropoietin
  • Adherent cells stained positive for vWF formed vascular tubes when plated on ECM, and were able to uptake a-LDL, indicating their endothelial nature. 5-50% of the non-adherent cells stained positive for human specific GlyA and HLA-class I by flow cytometry. Gly-A + /HLA-class-I + cells were selected by FACS. On Wright -Giemsa, these cells exhibited the characteristic morphology and staining pattern of primitive erythroblasts. Cells were benzidine + and human Hb + by immunoperoxidase. By RT-PCR these cells expressed human specific Hb-e, but not Hb-a.
  • MASC mononuclear sarcoma
  • ES cells ES cells that should be capable of contributing to the full constellation of tissues and organs in the body.
  • MASC mononuclear sarcoma
  • MASC were generated from marrow of ROS A26 mice that are transgenic for the ⁇ -galactosidase ( ⁇ -gal) gene (Rafii, S., et al. 1994, Blood. 84:10-13) and expanded as described in Example 1.
  • ⁇ -galactosidase ⁇ -gal
  • One or 10-12 ROSA26 MASC obtained after 55-65 PDs were microinjected into 88 and 40 3.5-day C57BL/6 blastocysts, respectively.
  • Blastocysts (8/mother) were transferred to 16 foster mothers and mice allowed to develop and be born as shown in Table 5.
  • Table 5 Degree of chimerism following MASC injection in blastocyst
  • mice Seven litters were born, in line with the birth rate seen in other studies during this period. The number of mice per litter varied between 1 and 8, for a total of 37 mice. Animals born from microinjected blastocysts were of similar size as normal animals and did not display any overt abnormalities.
  • mice were evaluated for chimerism by clipping their tails and assessing the contribution of ⁇ -gal/NEO transgene containing cells to the tails by Q-PCR for NEO. Percent chimerism was determined by comparing the number of NEO copies in test samples with that in tissue from ROSA26 mice according to manufacturer's recommendations (7700 ABI PRISM Detector Software 1.6). Chimerism could be detected in 70% of mice derived from blastocysts in which 10 to 12 MASC had been injected and 50% of mice derived from blastocysts microinjected with 1 MASC (Table 5). The degree of chimerism ranged between 0.1 % to >45%. After 6 to 20 weeks, animals were sacrificed.
  • mice were frozen in liquid nitrogen and thin sections were cut as described. Whole-mouse sections were stained with X-Gal. One thousand sets of digital images covering completely each section were then assembled to create a composite image of each whole-mouse section.
  • a representative non-chimeric animal (by Q-PCR for NEO) derived from a blastocyst in which a single MASC was injected, no X-Gal staining was seen.
  • the animal was 45% chimeric by R-PCR for NEO by tail clip analysis and had contribution of a single ROS A26-derived MASC to all somatic tissues.
  • Chimerism was detected by X-Gal staining and anti- ⁇ -gal staining in the animals generated from blastocysts microinjected with ROSA26 MASC.
  • ⁇ -gal + cells expressed markers typical for the tissue in which they had incorporated.
  • ⁇ -gal + cells co-stained with anti- ⁇ -gal + FITC and anti-NF200 or GFAP and TOPRO3
  • Intestine was stained with anti- ⁇ -gal-FITC, pan-CK-PE, and TOPR03 was observed at 20X magnification.
  • Kidney was stained with anti- ⁇ -gal-FITC (glomerulus, tubulus) was observed at 20X magnification.
  • Marrow staining was observed with anti- ⁇ -gal-FITC and CD45-PE, GR1-PE and MAC1-PE.
  • Spleen staining was observed with anti- ⁇ -gal-FITC and CD45-PE, CD3-PE and CD 19-PE.
  • Levels of engraftment estimated by Q-PCR for NEO were concordant with those estimated by X-GAL and anti- ⁇ -gal-FITC staining. Summary
  • angioblasts primitive endothelial progenitors
  • angiogenesis defined as the formation of new blood vessels by a process of sprouting from preexisting vessels, occurs both during development and in postnatal life (Holash et al, 1999; Yang et al, 2001).
  • endothelial "stem cells” may persist into adult life, where they contribute to the formation of new blood vessels (Peichev et al, 2000;
  • endothelial cells are derived from mesoderm.
  • the VEGF receptor 2, Flkl characterizes the hemangioblasts, a bipotent stem cell found in the aorto-gonad-mesonephros region (Medvinsky et al, 1996; Fong et al, 1999; Peault, 1996) and in fetal liver (Fong et al, 1999), and commitment of embryoid bodies to hemangioblasts is accompanied with expression of Flkl (Choi et al, 1998; Choi, 1998). Whether hemangioblasts persist in adult life is not known, and only HSC and endothelial progenitors have,been documented.
  • endothelial progenitors express Flkl (Peichev et al, 2000) and one report suggested that HSC in post-natal life express Flkl (Ziegler et al, 1999).
  • Flkl Flkl
  • HSC HSC in post-natal life express Flkl
  • CD34 CD34
  • endothelial progenitors In post-natal life, endothelial progenitors have been selected from BM and blood using Abs against AC 133, Flkl, CD34, and the H1P12 Ab (Peichev et al, 2000; Lin et al, 2000; Gehling et al, 2000). AC 133 has also been found on other cells, including NSCs (Uchida et al, 2000) and gastrointestinal epithelial cells (Corbeil et al, 2000). Upon differentiation to mature endothelium, the AC 133 receptor is quickly lost (Peichev et al, 2000; Gehling et al, 2000).
  • MUC18 Another receptor found on circulating endothelial cells is a mucin, MUC18, recognized by the H1P12 Ab (Lin et al, 2000). MUC18 is lost upon differentiation of endothelial progenitors to endothelium. CD34 is expressed on endothelial progenitors, as well as on hematopoietic progenitors
  • MASC can be culture expanded for >80 PDs and endothelial cells generated from MASC can be expanded for at least and additional 20 PDs. MASC may therefore be an ideal source of endothelial cells for clinical therapies. In addition, as MASC are ontogenically less mature than the "angioblast", this model should be useful to characterize endothelial commitment and differentiation. hMASC differentiate into cells with phenotypic characteristics of endothelium
  • MASC were obtained and cultured as described in Example 3. To induce endothelial differentiation, MASC were replated at 2xl0 4 cells/cm 2 in FN-coated wells in serum-free expansion medium without EGF and PDGF-BB but with 10 ng/mL VEGF. In some instances, FCS was added. Cultures were maintained by media exchange every 4-5 days. In some instances, cells were subcultured after day 9 at a 1 :4 dilution under the same culture conditions for 20+ PDs. In order to define endothelial differentiation from MASC more extensively,
  • CD34 present on endothelial and hematopoietic progenitors (Peichev et al, 2000; Asahara et al, 1997; Rafii et al, 1994), was not present on undifferentiated MASC (Fig. 4A) but was expressed from day 9 until day 18.
  • the mucin, MUC18, recognized by the Ab H1P12 has been used to purify endothelial progenitors from blood (Lin et al, 2000). Although MASC did not stain with H1P12 MASC treated with VEGF for 9 days stained positive, but expression was lost by day 18.
  • integrins The endothelium specific integrin, ⁇ v ⁇ 3, (Eliceiri et al, 2000) was not present on undifferentiated MASC, whereas ⁇ v ⁇ 5 was expressed at very low levels. Expression of integrins increased progressively during differentiation and was maximal by day 14 (Fig. 5).
  • MASC also do not express vWF, but vWF was expressed from day 9 on (Rosenberg et al, 1998; Wagner et al, 1982).
  • More mature endothelial markers including CD31, CD36, CD62-P (Tedder et al, 1995) (Fig. 7), and the adhesion junction proteins ZO-1, ⁇ -catenin, and ⁇ -catenin (Fig. 5) were detected after day 14 (Li et al, 1990; Van Rijen et al, 1997; Petzelbauer et al, 2000).
  • VCAM or CD62- E were not expressed at high level at any time point during differentiation, unless endothelium was activated with IL-l ⁇ , as described below. Differentiation to endothelium was associated with acquisition of ⁇ 2-microglobulin and low levels of HLA-class I antigens, but not HLA-class II.
  • endothelial differentiation can only be obtained from MASC expanded with 2% FCS or less, but not when expanded with 10% FCS (Reyes et al, 2001) as higher concentrations of FCS supports growth of classical MSC that differentiate only into osteoblasts, chondroblasts and adipocytes (Reyes et al, 2001 ; Pittenger et al, 1999).
  • FCS was present during the initial 7 days of differentiation, endothelial differentiation could not be induced.
  • non-confluent MASC ⁇ lxl0 4 cells/cm 2
  • VEGF-induced differentiated progeny of hMASC had functional characteristics of endothelial cells. Endothelial cells respond to hypoxia by upregulating expression of VEGF as well as the VEGF receptors Flkl and the angiogenesis receptors, Tie-1 and Tek (Kourembanas et al, 1998). hMASC and hMASC-derived endothelial cells were incubated at 37°C in 20% or 10% O 2 for
  • VEGF concentrations in the culture supematants was measured using an ELISA kit (AP biotech, Piscataway, NJ). MASC-derived endothelial cells and undifferentiated MASC were exposed to hypoxic conditions for 24h.
  • MASC-derived endothelial cells would upregulate expression of HLA-antigens and cell adhesion ligands in response to inflammatory cytokines, such as IL-l ⁇ (Meager, 1999; Steeber et al, 2001). 10 6 MASC and MASC-derived endothelial cells were incubated with 75 ng/ml IL-l ⁇ (R&D Systems) in serum-free medium for 24h.
  • IL-l ⁇ IL-l ⁇
  • Tek was detected but no uptake of a-LDL. After 7 days, cells expressed Tie-1, but did not take up significant amounts of a-LDL. However, acquisition of expression of vWF on day 9 was associated with uptake of aLDL (Fig. 6B).
  • Endothelial cells contain vWF stored in Weibel Pallade bodies that is released in vivo when endothelium is activated (Wagner et al, 1982). This can be induced in vitro by stimulating cells with histamine (Rosenberg et al, 1998), which also results in activation of the cell cytoskeleton (Vischer et al, 2000).
  • MASC- derived endothelial cells were plated at high confluency (10 4 cells/cm 2 ) in FN-coated chamber slides. After 24h, cells were treated with 10 ⁇ M histamine (Sigma) in serum free medium for 25 min. and stained with Abs against vWF and myosin.
  • vWF was present throughout the cytoplasm of untreated endothelial cells. Cytoplasm of endothelial cells treated with histamine contained significantly less vWF and vWF was only detectable in the perinuclear region, likely representing vWF present in the endoplasmic reticulum (Fig. 6A). Histamine treatment caused widening of gap junctions and cytoskeletal changes with increased numbers of myosin stress fibers (Fig. 6A).
  • endothelial cells were tested to determine if they could form "vascular tubes” when plated on MatrigelTM or extracellular matrix (ECM) (Haralabopoulos et al, 1997).
  • 0.5 ml extracellular matrix (Sigma) was added per well of a 24 well plate, incubated for 3h at 37°C.
  • MASC and MASC-derived endothelial cells were added per well in 0.5 ml of serum free plus VEGF medium and incubated at 37°C.
  • culture of MASC derived endothelial cells on ECM resulted in vascular tube formation within 6 hours.
  • hMASC-derived endothelial cells contribute to tumor-angiogenesis in vivo
  • mice A breeding colony of NOD-SCID mice was established from mice obtained from the Jackson Laboratories (Bar Harbor, ME). Mice were kept in specific pathogen free conditions and maintained on acidified water and autoclaved food. Trimethoprim 60 mg and sulphamethoxazole 300 mg (Hoffmann-La Roche Inc., Nutley, NJ) per 100 ml water was given twice weekly. Three Lewis lung carcinoma spheroids were implanted subcutaneously in the shoulder. 3 and 5 days after implantation of the tumor, mice were injected with Trimethoprim 60 mg and sulphamethoxazole 300 mg (Hoffmann-La Roche Inc., Nutley, NJ) per 100 ml water was given twice weekly. Three Lewis lung carcinoma spheroids were implanted subcutaneously in the shoulder. 3 and 5 days after implantation of the tumor, mice were injected with
  • MASC-derived endothelial cells were also analyzed whether they contribute to wound healing angiogenesis. The area of the ear that had been clipped to tag the mouse was then examined. Neoangiogenesis in the ear wounds was in part derived from the MASC derived endothelial cells. Similar to blood vessels in the tumor the percent human endothelial cells present in the healed skin wound was 30-45% (Fig.
  • Tumors or normal tissue The tissue was sliced using a cryostat in 5-10 ⁇ m thick slices. Slices were fixed with acetone for 10 min at room temperature and permeabilized with 0.1 Triton X for 5 min. Slides were incubated overnight for vWF, Tie or Tek, followed by secondary incubation with FITC, PE or Cy5 coupled anti-mouse-, goat- or rabbit-IgG Abs and sequential incubation with Abs against mouse CD45-PE or human CD45-FITC, human ⁇ 2-microglobulin-FITC, mouse CD31 -FITC or TOPRO-3 for 60min. Between each step, slides were washed with PBS + 1% BSA.
  • 3D-reconstruction consisted of the collection of sequential 0.5 ⁇ m confocal photos from 35 slides of 5 ⁇ m thick to a total of 350 photos. Slides were stained with vWF-Cy3 and alternately double stained with human ⁇ 2- microglobulin-FITC or mouse CD31-FITC. The photos from each slide were aligned with the next slide in Metamorph software (Universal Imaging Corp) and the 3D reconstruction was made in 3D Doctor Software (Able software Corp).
  • volume of relative contribution of human (green) and murine endothelial cells (false colored as blue) to the 3D vessel was calculated as cubic pixels of each color.
  • the area of each color was also calculated as square pixels in 4 vessels through the 35 slides to obtain an accurate percentage of contribution.
  • the area of each color was also calculated in alternate slides of four different tumors. Summary
  • the central finding of this study is that cells that co-purify with MSC from BM have the ability to differentiate to endothelial cells that have in vitro functional characteristics indistinguishable from mature endothelial cells. It is also showv that such endothelial cells contribute to neoangiogenesis in vivo in the setting of wound healing and tumorigenesis, and that undifferentiated MASC can respond to local cues in vivo to differentiate into endothelial cells contributing to tumor angiogenesis. As the same cell that differentiates to endothelium also differentiates to other mesodermal cell types, as well as cells of non-mesodermal origin, the cell defined here precedes the angioblast, and even the hemangioblast in ontogeny.
  • MASC differentiate into cells that express markers of endothelial cells, but proved that VEGF induced MASC function like endothelial cells.
  • Endothelial cells modify lipoproteins during transport in the artery wall (Adams et al, 2000). Endothelial cells maintain a permeability barrier through intercellular junctions that widen when exposed to hemodynamic forces or vasoactive agents, such as histamine (Rosenberg et al, 1998; Li et al, 1990; Van
  • Endothelial cells release prothrombotic molecules such as vWF, tissue factor, and plasminogen activator inhibitor to prevent bleeding (Vischer et al, 2000), and regulate egress of leukocytes by changing expression levels of adhesion molecules in response to inflammation (Meager, 1999; Steeber et al, 2001). Endothelium also reacts to hypoxia by producing VEGF and expressing VEGF receptor aimed at increasing vascular density (Kourembanas et al, 1998). Therefore it has been demonstrated that endothelial cells generated from MASC can perform all of these tasks when tested in vitro.
  • prothrombotic molecules such as vWF, tissue factor, and plasminogen activator inhibitor to prevent bleeding (Vischer et al, 2000), and regulate egress of leukocytes by changing expression levels of adhesion molecules in response to inflammation (Meager, 1999; Steeber et al, 2001). Endothelium also reacts to hypoxia by producing VEGF and expressing
  • hNPC Human neural progenitor cells
  • Electrophysiology Standard whole-cell patch-clamp recording was used to examine the physiological properties of MASC-derived neurons. Voltage-clamp and current-clamp recordings were obtained using a Dagan 3900 A patch-clamp amplifier (Dagan Corporation, Minneapolis) which was retrofitted with a Dagan 3911 expander unit. Patch pipettes, made from borosilicate glass, were pulled on a Narishige pipette puller (model PP-83), and polished using a Narishige microforge (model MF-83).
  • Patch pipettes were filled with an intracellular saline consisting of (in mM) 142.0 KF, 7.0 Na 2 S0 4 , 3.0 MgS0 4 , 1.0 CaCl 2 , 5.0 HEPES, 11.0 EGTA, 1.0 glutathione, 2.0 glucose, 1.0 ATP (magnesium salt), 0.5 GTP (sodium salt).
  • the fluorescent dye 5,6-carboxyfluorescein (0.5 mm; Eastman Kodak Chemicals) was also added to the pipette solution to confirm visually, using fluorescence microscopy, that the whole-cell patch recording configuration had been achieved. Pipette resistances ranged from 11 to 24 Mohm.
  • the standard extracellular recording saline was comprised of the following (in mM): 155 NaCl, 5.0 KC1, CaCl 2 , 1.0 MgCl 2 , 10 HEPES, 5 glucose.
  • 1 ⁇ M TTX was added to the standard control solution.
  • the pH of the intracellular and extracellular recording solutions was adjusted to 7.4 and 7.8, respectively, using NaOH. All chemicals were from Sigma.
  • PClamp 8.0 (Axon Instruments, Foster City) was used to run experiments, and to collect and store data. The data presented were corrected for a 8.4 mV liquid junctional potential, which was calculated using the JPCALC software package.
  • Off-line analyses and graphical representations of the data were constructed using Clampfit 8.0 (Axon Instruments, Foster City) and Prism (Graphpad, San Diego).
  • Retroviral supernatant was produced by incubating MFG- eGFP-containing PG13 cells, provided by Dr. G.Wagemaker, U. of Rotterdam, Netherlands (Bierhuizen et al, 1997), with MASC expansion medium for 48h, filtered and frozen at -80°C. MASC were incubated with retroviral supematants and
  • PCR analysis for retroviral insert PCR was used o amplify the flanking sequence 3' from the 3' LTR of the MFG vector in the human genomic DNA.
  • DNA from 10 6 MASC or endothelial, myoblast or neuroectodermal differentiated progeny was prepared from cells by standard methods. 300 ng of genomic DNA was digested with Ascl and a splinkerette linker was ligated to the 5' end (Devon R. S. et al, 1995).
  • the two oligonucleotides used for the splinkerette linker were as follows: aattTAGCGGCCGCTTGAATTtttttttgcaaaa, (the hairpin loop forming sequence is in lower case and the upper case is the reverse complement of the second splinkerette oligo), and agtgtgagtcacagtagtctc gc gttc gAATTAAGCGGCCGCTA, (the underlined sequence is also the sequence of the linker-specific primer (LS Primer) used for the PCR and RT steps).
  • LS Primer linker-specific primer
  • a 5'-biotin-T7 coupled primer was used that recognizes a sequence in the eGFP gene [Biotin-ggc- cag-tga-att-gta-ata-cga-ctc-act-ata-ggc-tgg-CAC-ATG-GTC-CTG-CTG-GAG-TTC- GTG-AC; underlined portion shows the minimum promoter sequence needed for efficient in vitro transcription and the upper case is the eGFP specific sequence] and LS primer to amplify the flanking regions for 10 rounds using Advantage 2 polymerase (Clontech).
  • the biotin labeled amplified product was captured using streptavidin-magnetic beads (Streptavidin Magnetic Particles; Roche) and the resultant product was further amplified using the T7 RNA polymerase an approximately 1 ,000 fold and then DNAase 1 treated.
  • the resultant product was reverse transcribed using the agtgtgagtcacagtagtctcgcgttc splinkerette primer according to the superscript II protocol (Gibco), and subsequently amplified by 30 rounds of nested PCR using the primer for the 3 'LTR [ggc caa gaa cag atg gaa cag ctg aat atg].
  • the flanking sequence in the human genome from endothelium, muscle, and neuroectodermal differentiated cells and undifferentiated MASC was sequenced.
  • LTR primer CCA-ATA-AAC-CCT-CTT-GCA-GTT-G
  • Flanking sequence chromosome 7 TCC-TGC-CAC-CAG-AAA-TAA-CC
  • LTR primer GGA-GGG-TCT-CCT-CTG-AGT-GAT-T
  • Flanking sequence CAG-TGG-CCA-GAT-CTC-ATC-TCA-C
  • flanking sequence was calculated in comparison with eGFP sequence according to manufacturer's recommendations using the 7700 ABI PRISM Detector Software 1.6.
  • Neural transplantation Newborn (P1-P3) male Sprague Dawley rats (Charles
  • hMASC were harvested with 0.25% trypsin/EDTA, washed twice, and resuspended in PBS. The viability of the hMASC was more than 85%.
  • a 2 ⁇ l volume of hMASC suspended in phosphate buffered saline at a concentration of 0.7x10 4 cells/ ⁇ l was stereotaxically injected intracerebroventricularly with a tapered glass micropipette attached to a Hamilton syringe using the following coordinates (mm from bregma): AP -0.6, ML 0.8, DV 2.1, toothbar was set at -1. Following the injections, the scalp was sutured and the pups allowed to recover.
  • the rats were anaesthetized with chloral hydrate (350mg/kg, i.p.), decapitated the brains removed, frozen in powered dry ice, and stored at -80°C.
  • Fresh frozen brains were sectioned using a cryostat and fixed with 4% paraformaldehyde for 20 min immediately before staining. Sections were incubated for one hour at room temperature with blocking/permeabilization solution consisting of 2% normal donkey serum (Jackson Immuno Labs) and 0.3% triton X.
  • Primary and secondary antibodies were diluted in the same blocking/permeabilization solution for subsequent steps.
  • cells were cultured in FN-coated chamberslides or culture plates with serum-free medium consisting of 60% DMEM-LG, 40% MCDB-201 (Sigma Chemical Co, St Louis, MO), supplemented with IX ITS, IX LA-BSA, 10 '8 M dexamethasone, lO ⁇ M ascorbic acid 2-phosphate (AA) (all from Sigma), 100 U penicillin and 1,000 U streptomycin (Gibco).
  • serum-free medium consisting of 60% DMEM-LG, 40% MCDB-201 (Sigma Chemical Co, St Louis, MO), supplemented with IX ITS, IX LA-BSA, 10 '8 M dexamethasone, lO ⁇ M ascorbic acid 2-phosphate (AA) (all from Sigma), 100 U penicillin and 1,000 U streptomycin (Gibco).
  • AA ascorbic acid 2-phosphate
  • Gibco 100 U penicillin and 1,000 U streptomycin
  • astrocyte-, oligodendrocyte- and neuron-like cells did not differ when differentiation was induced with hMASC that had undergone 20 or 60 PDs.
  • hMASC expanded for 20 PDs were cultured with bFGF, >50% of cells died while >70% of hMASC culture expanded for >30 PDs survived and acquired a neuron-, astrocyte- or oligodendrocyte-like phenotype.
  • astrocyte- and oligodendrocyte-like cells died after 3 weeks. Progressive maturation of neuron-like cells was seen throughout culture. After 1 week, bFGF treated hMASC stained positive for NeuroD, Nestin, polysialated neural cell adhesion molecule (PSA-NCAM), and tubulin- ⁇ -III (TuJI) (Table 6).
  • bFGF treated cells stained positive for NF68, -160, and -200, NSE, MAP2-AB, and Tau.
  • bFGF-induced neurons did not express markers of GABAergic, serotonergic or dopaminergic neurons, but expressed glutamate as well as the glutamate-receptors-5, -6 and -7 and N-methyl-D-aspartate (NMDA)-receptor, and Na + -gated voltage channels.
  • MASH I mammalian achaete-scute homolog 1
  • astrocyte specific markers GFAP and S100A5 and oligodendrocyte specific markers, myelin-oligodendrocyte glycoprotein precursor and myelin protein zero (PMZ), as well as Huntingtin, and major prion protein precursor mRNA were expressed >2-fold higher after exposure to bFGF.
  • bFGF induced expression of BDNF and glia-derived neurotrophic factor (GDNF).
  • GDNF glia-derived neurotrophic factor
  • mMASC expanded for 40-90 PDs were replated at 10 4 cells/cm in conditions identical to those used for hMASC. After 14 days, mMASC acquired morphologic and phenotypic characteristics of astrocytes (GFAP + ), oligodendrocytes (MBP + ) and neurons (NF-200 + , NSE + and Tau). NF200 and GFAP or MBP were never found in the same cell. In contrast to undifferentiated mMASC, mMASC treated with bFGF were significantly larger and extended processes for >40 ⁇ m.
  • hMASC acquire a midbrain dopaminergic, serotonergic and GABAergic phenotype when cultured with EGF and FGF-8b.
  • FGF-8b expressed at the mid-hindbrain boundary and by the rostral forebrain, induces differentiation of dopaminergic neurons in midbrain and forebrain and serotonergic neurons in the hindbrain (Ye et al, 1998).
  • FGF-8b has been used to induce dopaminergic and serotonergic neurons from murine ES cells (Lee et al, 2000).
  • FGF-8b and EGF induced differentiation into cells staining positive for neuronal markers (Table 6) (day 7: PSA-NCAM, Nestin and TuJl; day 14: NF-68, NF-160, NF-200; and day 21 : MAP2-AB, NSE, Tau, and Na + -gated voltage channels) but not oligodendrocytes and astrocytes.
  • day 7 PSA-NCAM, Nestin and TuJl
  • day 14 day 14
  • day 21 MAP2-AB, NSE, Tau, and Na + -gated voltage channels
  • results from immunohistochemical studies were confirmed by cDNA array analysis on hMASC induced to differentiate for 14 days with FGF-8b+EGF. Consistent with the immunohistochemical characterization, a >2 fold increase in mRNA for TH, TrH, glutamate, several glutamate-receptors, and sodium-gated voltage channels was detected. As parvalbumin and GABA are not present on the array, their expression could not be confirmed by mRNA analysis. Consistent with the almost exclusive neural differentiation seen by immunhistochemnistry, there was no increase in expression of GFAP, S 100 A5 mRNA nor mRNA for the oligodendrocyte specific marker, PMZ.
  • Trk tyrosine kinase receptor
  • BDNF BDNF
  • GDNF glycine-, GABA-and hydroxytryptamine-receptors
  • synaptic proteins Coculture with the glioblastoma cell line U87 enhances neuron maturation. Irrespective of the culture conditions used, hMASC-derived neurons did not survive more than 3-4 weeks in culture. As neither culture contained glial cells after 3 weeks, it is possible that neuronal cells that express both glutamate and glutamate- receptors died due to glutamate toxicity (Anderson and Swanson, 2000). Alternatively, factors required for neural cell survival, differentiation and maturation provided by glial cells might not be present in the cultures
  • hMASC derived neurons were labeled with the membrane dye, PKH26, prior to coculture with U-87 cells to allow us to identify the hMASC-derived cells by fluorescence microscopy.
  • FGF-8b+EGF induced neurons cocultured after 3 weeks with U-87 cells and the same cytokines survived for at least 2 additional weeks.
  • Neurons acquired a more mature morphology with increased cell size as well increased number, length and complexity of the neurites.
  • the electrophysiological characteristics of PKH26 labeled neural cells derived from hMASC after coculture with U-87 cells by whole-cell current clamp and voltage-clamp after current-injection was evaluated (Fig. 9B).
  • Fig. 9B An example of one of the cells in which w observed spiking behavior is shown in Fig. 9B.
  • the top panel shows a family of voltage traces which was elicited from a spiking cell under control conditions. A DC current was first injected in the cell to hold them in the range of -100 to -120 mV. A current injection protocol, as shown in the middle panel, was then used to drive the membrane potential to different levels. As shown in this example, depolarizing current steps that were sufficiently large to bring the cell to threshold for action potential, evoked a single spike.
  • the lower panel shows that the spiking behavior of the cells could be blocked by 1 ⁇ M TTX, suggesting that the action potentials are mediated by Na-gated voltage channels.
  • Leak-subtracted current records obtained in voltage-clamp mode from the same cells (Fig. 9C), demonstrated an inward current that was transient in time course and activated at voltages more positive than -58 mV, as well as outward currents. The transient inward current was blocked reversibly by 1 ⁇ M TTX.
  • Human cells identified by staining with a antibodies against human nuclei or human nuclear membrane could be seen in the SVZ up to 400 ⁇ m away from the ventricle in animals analyzed after 4 weeks, and after 12 weeks, human cells could also be seen deeper in the brain parenchyma such as in the hippocampus and along the fomix. Some human cells had typical astrocyte morphology and stained positive with anti-GFAP antibodies, whereas other cells stained positive with anti-Neu-N antibodies, NF-200 and anti-human nuclear membrane antibodies.
  • Retroviral marking studies were used to demonstrate that the neurons, astrocytes and oligodendrocytes were derived from a single MASC that also differentiates into muscle and endothelium, as the sequence of the host cell genomic region flanking the retroviral vector was identical in all lineages.
  • hMASC did not only acquire phenotypic but also electrophysiological characteristics of mature neurons, namely TTX-sensitive voltage-gated Na + currents.
  • MASC can differentiate in vivo into cells expressing neuronal and astrocyte markers.
  • hMASC transplanted in the ventricle of newborn rats can migrate in the neurogenic subventricular zone and into the hippocampus where they respond to local cues to differentiate into cells expressing astrocyte and neuronal markers.
  • This model was chosen because migration and differentiation of NSC to specific neuronal phenotypes occurs to a much greater extent when transplantation is done in germinal areas of the brain than in non-neurogenic areas, and when transplants are done in newborn animals compared with adult animals (Bjorklund and Lindvall, 2000; Svendsen and Caldwell, 2000).
  • hMASC are multipotent and differentiate into cells outside of the neuroectoderm, hMASC did not form teratomas.
  • liver morphogenesis is a thickening of the ventral endodermal epithelium, which occurs between e7.5 and e8.5 in the mouse (Zaret K.S., 2001). Little is known about the signals involved in initial endoderm formation and subsequent endoderm specification. Early in gastrulation
  • BMP's Basic morphogenetic proteins produced by the transversum mesenchyme are also required as they increase levels of the GATA4 transcription factor which promote the ability of endoderm to respond to FGF's (Zaret K.S., 2001).
  • GATA4 and HNF3 ⁇ are required for hepatic specification and are important effectors of downstream events leading to hepatocyte differentiation, as they upregulate markers of hepatocyte specific expression such as albumin, among others.
  • liver stem cell a population of smaller cells with oval shape, termed oval cells, emerges and proliferates (Petersen, B.E., 2001). These oval cells may constitute the "stem cell” compartment in the liver. Oval cells reside in the smallest units of the biliary tree, called the canals of Herring, from where they migrate into the liver parenchyma (Theise N.D., et al, 1999).
  • Oval cells are bi-potential, giving rise in vitro and in vivo to both hepatocytes and bile ductular epithelium.
  • Oval cells express several hematopoietic markers such as Thy 1.1, CD34, Flt3 -receptor, and c- Kit, and also express ⁇ FP, CKl 9, ⁇ -glutamyl-transferase, and OV-6.
  • the origin of oval cells is not known (Petersen, B.E., 2001; Kim T.H. et al, 1997; Petersen, B.E.,
  • hepatocytes could only be derived from cells of endodermal origin and their progenitors.
  • non-endodermal cells may also form hepatocytes in vivo and in vitro (Petersen,
  • HSC hematopoietic stem cells
  • Exocrine pancreatic tumor cells treated in vitro with dexamethasone (Dex) with or without oncostatin M (OSM) may acquire a hepatocyte phenotype (Shen C.N. et al, 2000).
  • mouse embryonic stem (ES) cells spontaneously acquire a hepatocyte phenotype, a process that is enhanced by treatment with aFGF, HGF, OSM, and Dex (Hamazaki T. et al, 2001).
  • mMASC, rMASC, and hMASC acquire a hepatocyte-like phenotype when cultured with FGF4 and/or HGF.
  • mMASC, rMASC and hMASC were selected and cultured as described.
  • CKl 8 and HNF3 ⁇ positive epithelioid cells were seen when MASC were plated at 21.5x10 3 cells/cm 2 in the presence of 10 ng/ml FGF4 and 20 ng/ml HGF on MatrigelTM as shown in Table 7A. After 14 days, the percent albumin, CKl 8 and HNF3 ⁇ positive epithelioid cells was 61.4+4.7%, and 17.3% of cells were binucleated. When plated on FN, differentiation to CKl 8 and HNF3 ⁇ positive epithelioid cells was also seen, even though only 53.1+6.3% of cells stained and fewer (10.9%) binucleated cells were seen.
  • hepatocyte markers When cell densities between 2.5 and 25x10 3 cells/cm 2 were tested, the highest percent cells with hepatocyte markers was seen in cultures seeded at 21.5x 10 3 cells/cm 2 . No hepatocyte differentiation was seen when cells were plated at ⁇ 12.5xl0 3 cells/cm 2 .
  • hMASC were plated at 3-30x10 3 cells/cm 2 on lOng/mL FN or 1% MatrigelTM with aFGF, bFGF, FGF7, 1% DMSO, HGF, and / or FGF4.
  • the percent albumin, CK18 and HNF3 ⁇ positive epithelioid cells was higher when hMASC were cultured on MatrigelTM (91.3% ⁇ 4.4) than on FN (89.5% ⁇ 5.4), and the percent binucleated cells was higher on MatrigelTM (31.3%) than on FN (28.7%) as shown in Table 7B.
  • Table 7 Optimization of MASC differentiation into hepatocyte like cells.
  • Hepatocyte differentiation was further evaluated over time by immunofluorescence and confocal microscopy for early (HNF3 ⁇ , GATA4, CKl 9, ⁇ FP) and late (CK18, albumin, HNFl ⁇ ) markers of hepatocyte differentiation.
  • mMASC or rMASC plated on MatrigelTM with FGF4 and HGF enlarged from 8 ⁇ m to 15 ⁇ m diameter as shown in Table 8 A.
  • Undifferentiated mMASC or rMASC did not express any of the liver specific transcription factors or cytoplasmic markers. After 4 days, cells expressed HNF3 ⁇ , GATA4 and ⁇ FP, low levels of CKl 9, and very rare cells stained positive for HNFl ⁇ , albumin or CKl 8. At seven days, the large epithelioid cells stained positive for HNF3 ⁇ , GATA4, HNFl ⁇ with increasing staining for albumin and CKl 8. Only rare cells expressed ⁇ FP. After 14, 21 and 28 days, the large epithelioid cells stained positive for GATA4, HNF3 ⁇ , HNFl ⁇ , CK18 and albumin, but not ⁇ FP or CKl 9.
  • hMASC was plated on MatrigelTM with FGF4 and HGF or FGF4 alone enlarged from 10-12 ⁇ m to 20-30 ⁇ m diameter by d21. After 7 days, cells expressed HNF3 ⁇ , GATA4 and low levels of CKl 9, while few cells stained positive for albumin or CKl 8. After 14 and 21 days, >90% of epithelioid cells stained positive for GATA4, HNF3 ⁇ , HNFl ⁇ , HNF4, CK18 and albumin, while only rare cells stained positive for ⁇ FP or CKl 9 as shown in Figure 10B.
  • Hepatocyte-like cells are derived from the same single hMASC that differentiated into neuroectoderm and endoderm
  • mMASC or rMASC differentiate into endothelium, neuroectoderm and CKl 8 and albumin positive endodermal cells. It has also been shown that single hMASC differentiate into mesoderm and neuroectoderm. The same single hMASC was tested to determine whether they can differentiate into hepatocyte-like cells. MASC were obtained, cultured and expanded as described. For differentiation, mMASC or rMASC were plated at 5- 25xl0 3 cells/cm 2 on 0.01-lO ⁇ g/ml fibronectin (FN), 0.01-8 ⁇ g/ml collagen (Sigma Chemical Co, St.
  • DMEM-LG low glucose DMEM
  • MCDB-201 40% MCDB-201 (Sigma), supplemented with IX insulin/transferrin/selenium, 4.7 ⁇ g/ml linoleic acid, 1 mg/ml bovine serum albumin (BSA), 10 "8 M dexamethasone, 10 "4 M ascorbic acid 2-phosphate (all from Sigma), lOOU/ml penicillin, 100/ml U streptomycin (Gibco)], with 2% FCS (Hyclone, Logan Utah) and 10 ng/mL each epidermal growth factor (EGF) (Sigma), leukemia inhibitory factor (LIF; Chemicon, Temecula, CA), and platelet derived growth factor (PDGF-BB; R&D Systems, Minneapolis, MN).
  • EGF epidermal growth factor
  • LIF leukemia inhibitory factor
  • PDGF-BB platelet derived growth factor
  • hMASC were plated at 15-30xl0 3 cells/cm 2 on 0.1 ⁇ g/ml FN, or 1 % MatrigelTM in the same medium without LIF (Reyes M., 2002). After 8-12h, media were removed, cells washed twice with phosphate buffered saline (PBS) (Fischer) and cultured in serum-free medium supplemented with 5-50ng/ml HGF, aFGF, bFGF, FGF4, FGF7, or OSM; or 10 mg/ml dimethyl-sulphoxide (DMSO), or 0.1-1 mM sodium butyrate.
  • PBS phosphate buffered saline
  • DMSO dimethyl-sulphoxide
  • Transduction of hMASC with eGFP was performed using an eGFP-cDNA containing retrovirus and expanded to >5X10 6 cells. Twenty percent was induced to differentiate into muscle, endothelium, neuroectoderm and endoderm. For clone A16 a single retroviral insertion site was present in undifferentiated MASC as well as mesodermal and neuroectodermal differentiated cells and eGFP + clone A16 MASC differentiated into CKl 8 and albumin positive cells.
  • FGF4-treated MASC generated from the same cell population (5'- TAG CGGCCGCTTGAATTCGAACGCGAGACTACTGTGACT CACACT-3', Chromosome 7), proving that single hMASC differentiate into endoderm aside from mesoderm and neuroectoderm.
  • Quantitative RT-PCR demonstrates that FGF4 and HGF induces hepatocyte specification and differentiation.
  • mRNA levels were normalized using ⁇ -actin (mouse and human) or 18S (rat) as housekeeping genes and compared with mRNA levels in freshly isolated rat or mouse hepatocytes, rat hepatocytes cultured for 7 days, or mRNA from human adult liver RNA purchased from Clontech, Palo Alto, California.
  • mMASC and rMASC expressed low levels of albumin ⁇ FP, CKl 8, CKl 9, TTR, HNF3 ⁇ , HNFl ⁇ and GATA4 mRNA, but no CYP2B9 and CYP2B13 (mouse) or CYP2B1 (rat) mRNA (Fig. 10).
  • FGF4 and HGF expression of HNF3 ⁇ and GATA4 mRNA increased on d2, became maximal by d4, decreasing slightly and leveling off by dl4.
  • mRNA for ⁇ FP, and CKl 9 increased after d2, and became maximal by d4 and decreased thereafter.
  • TTR mRNA increased after d4, was maximal by d7 and leveled off.
  • CK18, Albumin, HNFl ⁇ and P450 enzyme mRNA increased after d7 and was maximal on dl4.
  • CKl 8, CKl 9, CYP1B1 mRNA increased significantly in hMASC cultured with
  • CYP1B1 is not a specific hepatocyte marker, its upregulation suggests hepatocyte commitment and maturation.
  • Low levels of CYP2B6, 0.5% to 1.0% of fresh liver mRNA's could be seen on dl4 and d21 but not dO.
  • mRNA levels of immature hepatocyte markers decreased as differentiation progressed and were higher in cultures induced with FGF4 alone, whereas mRNA levels for mature hepatocytes (CKl 8 and albumin) were higher in FGF4 and HGF-induced hMASC.
  • hepatocyte-specific genes were also confirmed by Western Blot and performed as described by Reyes et al. (2000). Abs to ⁇ FP, human albumin, CKl 8 were diluted 1 : 1000 in blocking buffer. Goat anti- ⁇ -actin (1 :1000) was from Santa Cruz. Secondary Abs were HRP-linked goat anti-mouse and HRP-linked donkey anti-goat (Amersham, Arlington Heights). ECL was performed according to manufacturers instructions (Amersham). Undifferentiated hMASC did not express CKl 8, albumin, or ⁇ FP protein (Fig. 10B).
  • hMASC expressed albumin and CKl 8, but not ⁇ FP, consistent with the histochemical analysis.
  • mMASC, rMASC and hMASC acquire hepatocyte functional activity
  • Urea production and secretion by hepatocyte-like cells was measured at various time points throughout differentiation. Urea concentrations were determined by colorimetric assay (Sigma Cat. 640-1) per manufacturer's instructions. Rat hepatocytes grown in monolayer and fetal mouse liver buds were used as positive controls, and culture medium as negative control. The assay can detect urea concentrations as low as 10 mg/ml. As the assay also measures ammonia, samples were assessed before and after urease addition.
  • MASC did not produce urea.
  • urea production by MASC increased in a time dependent manner. The time course for urea production in mouse and rat cultures was similar.
  • urea was not detected on d4
  • dl2 was similar to mouse and rat cultures by dl2
  • d21 was similar to mouse and rat cultures by dl2
  • levels of urea produced by MASC-derived hepatocytes were similar to that in monolayer cultures of primary rat hepatocytes. For all three species, significantly more urea was produced by cells differentiated on MatrigelTM compared to FN. Albumin production was measured at various time points throughout the differentiation.
  • Rat albumin concentrations were determined by a competitive enzyme linked immunoassay (ELISA) described previously (Tzanakakis E.S., et al, 2001 ; Wells J.M. et al, 2000). Human and mouse albumin concentrations were determined using a similar ELISA method with substitution of human or mouse albumin and anti-human or anti-mouse albumin Abs for the rat components where appropriate.
  • ELISA enzyme linked immunoassay
  • Peroxidase conjugated anti-human-albumin and reference human albumin were from Cappel.
  • Peroxidase conjugated and affinity purified anti-mouse albumin and reference mouse albumin were from Bethyl Laboratories (Montgomery, Texas).
  • ELISA's had a sensitivity of at least 1 ng/ml.
  • Cytochrome P450 activity was next assessed in aggregates of MASC-derived hepatocytes and primary rat liver hepatocyte spheroids using the PROD assay.
  • mMASC-hepatocyte aggregates were formed by plating dl4 FGF4 and HGF treated mMASC at 5xl0 4 cells/cm on non-tissue culture plates, which were placed on a shaker at 10 revolutions per minute for 5h. Cell aggregates were transferred to
  • hMASC-hepatocyte aggregates were formed by hanging drop method. Briefly, 10 3 hMASC treated for 24 days with FGF4 and HGF were placed into lOO ⁇ L drops with or without ImM phenobarbital. After 4 days, aggregates were collected and cytochrome P450 activity assessed by PROD assay.
  • Pentoxyresorufin (PROD) (Molecular Probes, Eugene, Oregon) is O-dealkylated by Cytochrome P450, changing a non-fluorescent compound into a fluorescent compound, resorufin (Tzanakakis E.S. et al, 2001). Fluorescence intensity caused by PROD metabolism consequently estimates cytochrome P450 (CYP) activity. Assessment and detection of resorufin in situ was performed using confocal microscopy as described (Tzanakakis E.S. et al, 2001).
  • PROD activity in MASC-derived hepatocyte aggregates was similar to that of primary rat hepatocyte aggregates.
  • a number of different cells have P450 activity, but P450 activity up-regulation by phenobarbital is only seen in hepatocytes. Therefore, P450 was also tested in the presence or absence of phenobarbital. Without phenobarbital, several P450 enzymes partially participate in PROD metabolism giving an inflated fluorescence value for those samples.
  • MASC-derived hepatocytes were also assessed for their ability to take up
  • LDL by incubating FGF4 treated hMASC with LDL-dil-acil. Cells were co-labeled either with anti-CKl 8 or anti-Pan-CK and HNF-3 ⁇ or GATA4 Abs. After 7 days, low level uptake of a-LDL was detected, which increased to become maximal on d21.
  • glycogen production or gluconeogenesis Another metabolic function of hepatocytes is glycogen production or gluconeogenesis.
  • the levels of glycogen storage were analyzed by periodic acid Schiff (PAS) staining of FGF4 and HGF induced mouse MASC and FGF induced hMASC at d3, d7, dl4, and d21.
  • PAS periodic acid Schiff
  • slides were oxidized in 1% periodic acid for 5' and rinsed 3 times in dH O. Afterwards slides were treated with Schiff s reagent for 15', rinsed in dH 2 O for 5-10', stained with Mayer's hematoxylin for 1 ' and rinsed in dH 2 O.
  • Glycogen storage was first seen by dl4 and maximum levels were seen after d21 (Fig. 11).
  • Hepatocytes were harvested from 4-6 week old male Sprague-Dawley rats as described (Seglen P.O., 1976). Hepatocyte viability after the harvest ranged from 90-95%. Hepatocytes were cultured as described (Tzanakakis E.S. et al, 2001; Tzanakakis E.S. et al, 2001). To form a monolayer, hepatocytes were cultured on 35 mM Fischer culture plates (Fischer Scientific, Pittsburgh, PA) coated with 8 ⁇ g/cm collagen (Cohesion Technologies, Palo Alto, CA). To form spheroids, hepatocytes were cultured on 35-mm PrimariaTM dishes (Becton Dickinson). Under both conditions, seeding density was 5xl0 4 cells/cm 2 . 12h after initial plating, medium was changed to remove dead and unattached cells. Medium was replaced every 48 hours thereafter. Summary
  • MASC multi-natal mouse, rat and human BM-derived MASC can differentiate in vitro into an endodermal cell type with hepatocyte phenotype and function.
  • MASC cultured under hepatocyte differentiation conditions, expressed in a time-dependent fashion primitive and mature hepatocyte markers, shown by immunofluorescence microscopy of double and triple labeled cells.
  • the protein expression profile was hepatocyte specific and not spurious, as non-hepatocyte markers were not co-expressed with hepatocyte antigens. Results from immunohistochemistry were confirmed by Western blot.
  • MASC into cells with morphological and phenotypic characteristics of hepatocytes, this alone does not prove that cells have differentiated into hepatocytes unless one can demonstrate acquisition of functional characteristics of hepatocytes. Therefore, several functional tests were done in combination to identify functional hepatocytes.
  • mMASC, rMASC or hMASC produced urea and albumin, contained phenobarbital inducible cytochrome P450 activity, could take up Dil-acil-LDL, and contained glycogen granules. Although urea production is characteristic of hepatocyte activity, kidney tubular epithelium also produces urea (Hedlund E. et al, 2001).
  • albumin production is a specific test for the presence and metabolic activity of hepatocytes (Hedlund E. et al, 2001).
  • Cytochrome P450 although found in hepatocytes, is also present in many other cell types (Jarukamjorn K. et al, 1999).
  • Cyp2bl activity in rat (Tzanakakis E.S. et al, 2001), Cyp2b9 and Cyp2bl3 in mouse (Li-Masters T. et al, 2001; Zelko I. Et al, 2000), and CYP2B6 in human is considered relatively hepatocyte specific. Presence of these forms of P450 was shown by RT-PCR.
  • hepatocytes The specificity for hepatocytes is enhanced further when P450 activity is inducible by phenobarbital (Rader D J. et al, 2000), as shown. Although LDL uptake is seen in hepatocytes (Oh S.H. et al, 2000), other cells such as endothelium have a similar capability (Avital I. et al, 2001). Finally, only hepatocytes can generate and store glycogen. When taken together, these functional tests demonstrate that MASC from mouse, rat or humans treated in vitro with FGF4 and HGF not only express hepatocyte markers but also have functional characteristics consistent with hepatocyte metabolic activities.
  • BM derived cells may differentiate into hepatocyte-like cells in vivo and in vitro (Petersen B.E. et al, 1999; Theise N.D. et al, 2000; Krause D.S. et al, 2001; Pittenger M.F. et al, 1999; Wang S. et al, 2001; Lagasse E. et al, 2000).
  • most studies have not addressed the phenotype of the BM cell that differentiates into cells with hepatocyte phenotype.
  • Insulin-like growth facor-I is a differentiation factor for postmitotic C ⁇ S stem cell-derived neuronal precursors: distinct actions from those of brain-derived neurotrophic factor. JNeurosci 18:118- 28.
  • Rex- 1 a gene encoding a transcription factor expressed in the early embryo, is regulated via Oct-3/4 and Oct-6 binding to an octamer site and a novel protein, Rox- 1, binding to an adjacent site. Mol Cell Biol 18:1866-78. Bierhuizen, M. F., Westerman, Y., Visser, T. P., Dimjati, W., Wognum, A.
  • Choi, K. (1998). Hemangioblast development and regulation. Biochem Cell Biol 76:947-956. Choi, K., M. Kennedy, A. Kazarov, J.C. Papadimitriou, and G. Keller.
  • Fibroblast growth factor 2 promotes acquisition of epidermal growth factor (EGF) reponsiveness in mouse striata] precursor cells: Identification of neural precursors responding to both EGF and FGF-2. J Neuroscience 18:7869-7880.
  • the human AC 133 HSC antigen is also expressed in epithelial cells and targeted to plasma membrane protrusions. J Biol Chem. 275:5512-5530.
  • Subventricular zone astrocytes are NSCs in the adult mammalian brain. Cell 97:703-716.
  • Engraftable human NSCs respond to developmental cues replace neurons and express foreign genes. Nature Biotech 16:1033-1038.
  • Epidermal and fibroblast growth factors behave as mitogenic regulators for a single multipotent stem cell-like population from the subventricular region of the adult mouse forebrain. J Neurosci.
  • Marrow stromal cells migrate throughout forebrain and cerebellum, and they differentiate into astrocytes after injection into neonatal mouse brains. Proc Natl Acad Sci U S A. 96:1071 1-10716.
  • Immunity. 8:761-769. Niwa, H., Miyazaki, J., and Smith, A. G. (2000). Quantitative expression of
  • Oct-3/4 defines differentiation, dedifferentiation or self-renewal of ES cells. Nat Genet 24:372-6.
  • Hepatocyte growth factor induces differentiation of adult rat bone marrow cells into a hepatocyte lineage in vitro. Biochem Biophys Res Commun 279:500-504.
  • Fibroblast growth factor-2 activates a latent neurogenic program in NSCs from diverse regions of the adult CNS. J Neurosci 19:8487-97.
  • Nurrl is essential for the induction of the dopaminergic phenotype and the survival of ventral mesencephalic late dopaminergic precursor neurons. Proc Natl Acad Sci USA 95: 4013-8.
  • Adhesion molecule cascades direct lymphocyte recirculation and leukocyte migration during inflammation. Immunol Res. 22:299-317.
  • bFGF regulates the proliferative fate of unipotent (neuronal) and bipotent (neuronal/astroglial) EGF- generated CNS progenitor cells. Neuron 11 : 951-66.
  • Myeloid leukemia inhibitory factor maintains the developmental potential of ES cells. Nature 336:684-7.
  • KDR Receptor A Key Marker Defining HSCs. Science. 285:1553 1558.

Landscapes

  • Health & Medical Sciences (AREA)
  • Life Sciences & Earth Sciences (AREA)
  • Engineering & Computer Science (AREA)
  • Chemical & Material Sciences (AREA)
  • Organic Chemistry (AREA)
  • Bioinformatics & Cheminformatics (AREA)
  • General Health & Medical Sciences (AREA)
  • Biomedical Technology (AREA)
  • Animal Behavior & Ethology (AREA)
  • Medicinal Chemistry (AREA)
  • Pharmacology & Pharmacy (AREA)
  • Public Health (AREA)
  • Veterinary Medicine (AREA)
  • Nuclear Medicine, Radiotherapy & Molecular Imaging (AREA)
  • General Chemical & Material Sciences (AREA)
  • Chemical Kinetics & Catalysis (AREA)
  • Genetics & Genomics (AREA)
  • Zoology (AREA)
  • Wood Science & Technology (AREA)
  • Biotechnology (AREA)
  • Microbiology (AREA)
  • General Engineering & Computer Science (AREA)
  • Biochemistry (AREA)
  • Cell Biology (AREA)
  • Neurology (AREA)
  • Diabetes (AREA)
  • Immunology (AREA)
  • Hematology (AREA)
  • Neurosurgery (AREA)
  • Developmental Biology & Embryology (AREA)
  • Communicable Diseases (AREA)
  • Oncology (AREA)
  • Environmental Sciences (AREA)
  • Physical Education & Sports Medicine (AREA)
  • Gastroenterology & Hepatology (AREA)
  • Transplantation (AREA)
  • Urology & Nephrology (AREA)
  • Orthopedic Medicine & Surgery (AREA)
  • Cardiology (AREA)
  • Mycology (AREA)

Abstract

The present invention relates generally to mammalian multipotent adult stem cells (MASC), and more specifically to methods for obtaining, maintaining and differentiating MASC to cells of multiple tissue types. Uses of MASC in the therapeutic treatment of disease are also provided.

Description

MULTIPOTENT ADULT STEM CELLS, SOURCES THEREOF, METHODS
OF OBTAINING AND MAINTAINING SAME, METHODS OF
DIFFERENTIATION THEREOF, METHODS OF USE THEREOFAND
CELLS DERIVED THEREOF
RELATED CASES
This application claims the benefit of U.S. Provisional Application No.
60/343,386, filed October 25, 2001, U.S. Provisional Application No. 60/310,625, filed August 7, 2001, U.S. Provisional Application No. 60/269,062, filed February 15, 2001, U.S. Provisional Application No. 60/268,786, filed February 14, 2001, which are hereby incorporated by reference for all purposes. Applicants also claim priority of WO 01/11011, 60/147,324 and 60/164,650 and these applications are hereby incorporated by reference into this text; any teachings therein may be used in the practice of this invention. The present application is a continuation-in-part of WO 01/11011, which is attached herein at Appendix 1 and is part of the present application. Documents incorporated by reference into this text are not admitted to be prior art.
FIELD OF THE INVENTION The present invention relates generally to mammalian multipotent adult stem cells (MASC), and more specifically to methods for obtaining, maintaining and differentiating MASC. Uses of MASC in the therapeutic treatment of disease are also provided.
BACKGROUND OF THE INVENTION
Organ and tissue generation from stem cells, and their subsequent transplantation provide promising treatments for a number of pathologies, making stem cells a central focus of research in many fields. Stem cell technology provides a promising alternative therapy for diabetes, Parkinson's disease, liver disease, heart disease, and autoimmune disorders, to name a few. However, there are at least two major problems associated with organ and tissue transplantation.
First, there is a shortage of donor organs and tissues. As few as 5 percent of the organs needed for transplant in the United States alone ever become available to a recipient (Evans, et al. 1992). According to the American Heart Association, only 2,300 of the 40,000 Americans who needed a new heart in 1997 received one. The American Liver Foundation reports that there are fewer than 3,000 donors for the nearly 30,000 patients who die each year from liver failure.
The second major problem is the potential incompatibility of the transplanted tissue with the immune system of the recipient. Because the donated organ or tissue is recognized by the host immune system as foreign, immunosuppressive medications must be provided to the patient at a significant cost-both financially and physically.
Xenotransplantation, or transplantation of tissue or organs from another species, could provide an alternative means to overcome the shortage of human organs and tissues. Xenotransplantation would offer the advantage of advanced planning. The organ could be harvested while still healthy and the patient could undergo any beneficial pretreatment prior to transplant surgery. Unfortunately, xenotransplantation does not overcome the problem of tissue incompatibility, but instead exacerbates it. Furthermore, according to the Centers for Disease Control, there is evidence that damaging viruses cross species barriers. Pigs have become likely candidates as organ and tissue donors, yet cross-species transmission of more than one virus from pigs to humans has been documented. For example, over a million pigs were recently slaughtered in Malaysia in an effort to contain an outbreak of Hendra virus, a disease that was transmitted to more than 70 humans with deadly results (Butler, D. 1999). Stem cells: Definition and use
The most promising source of organs and tissues for transplantation, therefore, lies in the development of stem cell technology. Theoretically, stem cells can undergo self-renewing cell division to give rise to phenotypically and genotypically identical daughters for an indefinite time and ultimately can differentiate into at least one final cell type. By generating tissues or organs from a patient's own stem cells, or by genetically altering heterologous cells so that the recipient immune system does not recognize them as foreign, transplant tissues can be generated to provide the advantages associated with xenotransplantation without the associated risk of infection or tissue rejection.
Stem cells also provide promise for improving the results of gene therapy. A patient's own stem cells could be genetically altered in vitro, then reintroduced in vivo to produce a desired gene product. These genetically altered stem cells would have the potential to be induced to differentiate to form a multitude of cell types for implantation at specific sites in the body, or for systemic application. Alternately, heterologous stem cells could be genetically altered to express the recipient's major histocompatibility complex (MHC) antigen, or no MHC antigen, allowing transplantion of cells from donor to recipient without the associated risk of rejection. Stem cells are defined as cells that have extensive proliferation potential, differentiate into several cell lineages, and repopulate tissues upon transplantation. The quintessential stem cell is the embryonic stem (ES) cell, as it has unlimited self- renewal and multipotent differentiation potential (Thomson, J. et al. 1995; Thomson, J. A. et al. 1998; Shamblott, M. et al. 1998; Williams, R.L. et al. 1988; Orkin, S.
1998; Reubinoff, B.E., et al. 2000). These cells are derived from the inner cell mass y of the blastocyst (Thomson, J. et al. 1995; Thomson, J.A. et al. 1998; Martin, G.R. 1981), or can be derived from the primordial germ cells from a post-implantation embryo (embryonal germ cells or EG cells). ES and EG cells have been derived from mouse, and more recently also from non-human primates and humans. When introduced into mouse blastocysts, ES cells can contribute to all tissues of the mouse (animal) (Orkin, S. 1998). Murine ES cells are therefore pluripotent. When transplanted in post-natal animals, ES and EG cells generate teratomas, which again demonstrates their multipotency. ES (and EG) cells can be identified by positive staining with the antibodies to stage-specific embryonic antigens (SSEA) 1 and 4. At the molecular level, ES and EG cells express a number of transcription factors highly specific for these undifferentiated cells. These include oct-4 and Rex- 1, leukemia inhibitory factor receptor (LIF-R). The transcription factors sox-2 and Rox-1 are expressed in both ES and non-ES cells. Oct-4 is expressed in the pregastrulation embryo, early cleavage stage embryo, cells of the inner cell mass of the blastocyst, and embryonic carcinoma (EC) cells. In the adult animal, oct-4 is only found in germ cells.
Oct-4, in combination with Rox-1, causes transcriptional activation of the Zn-finger protein Rex-1, and is also required for maintaining ES in an undifferentiated state. The oct-4 gene is down-regulated when cells are induced to differentiate in vitro. Several studies have shown that oct-4 is required for maintaining the undifferentiated phenotype of ES cells, and that it plays a major role in determining early steps in embryogenesis and differentiation. Sox-2, is required with oct-4 to retain the undifferentiated state of ES EC and to maintain murine, but not human, ES cells. Human or murine primordial germ cells require presence of
LIF. Another hallmark of ES cells is presence of high levels of telomerase, which provides these cells with an unlimited self-renewal potential in vitro. Stem cells have been identified in most organs or tissues. The best characterized is the hematopoietic stem cell (HSC). This mesoderm-derived cell has been purified based on cell surface markers and functional characteristics. The
HSC, isolated from bone marrow (BM), blood, cord blood, fetal liver and yolk sac, is the progenitor cell that generates blood cells or following translation reinitiates multiple hematopoietic lineages and can reinitiate hematopoiesis for the life of a recipient. (See Fei, R., et al, U.S. Patent No. 5,635,387; McGlave, et al, U.S. Patent No. 5,460,964; Simmons, P., et al, U.S. Patent No. 5,677,136; Tsukamoto, et al, U.S. Patent No. 5,750,397; Schwartz, et al, U.S. Patent No. ,759,793; DiGuisto, et al, U.S. Patent No. 5,681,599; Tsukamoto, et al, U.S. Patent No. 5,716,827; Hill, B., et al. 1996.) When transplanted into lethally irradiated animals or humans, HSCs can repopulate the erythroid, neutrophil-macrophage, megakaryocyte and lymphoid hemopoietic cell pool. In vitro, hemopoietic stem cells can be induced to undergo at least some self-renewing cell divisions and can be induced to differentiate to the same lineages as is seen in vivo. Therefore, this cell fulfills the criteria of a stem cell. Stem cells which differentiate only to form cells of hematopoietic lineage, however, are unable to provide a source of cells for repair of other damaged tissues, for example, heart or lung tissue damaged by high-dose chemotherapeutic agents.
A second stem cell that has been studied extensively is the neural stem cell (NSC) (Gage F.H. 2000; Svendsen C.N. et al, 1999; Okabe S. et al. 1996). NSCs were initially identified in the subventricular zone and the olfactory bulb of fetal brain. Until recently, it was believed that the adult brain no longer contained cells with stem cell potential. However, several studies in rodents, and more recently also non-human primates and humans, have shown that stem cells continue to be present in adult brain. These stem cells can proliferate in vivo and continuously regenerate at least some neuronal cells in vivo. When cultured ex vivo, NSCs can be induced to proliferate, as well as to differentiate into different types of neurons and glial cells. When transplanted into the brain, NSCs can engraft and generate neural cells and glial cells. Therefore, this cell too fulfills the definition of a stem cell, albeit a hematopoetic stem cell.
Clarke et al. reported that NSCs from Lac-Z transgenic mice injected into murine blastocysts or in chick embryos contribute to a number of tissues of the chimeric mouse or chicken embryo (Clarke, D. L. et al. 2000). LacZ-expressing cells were found with varying degree of mosaicism, not only in the central nervous system, but also in mesodermal derivatives as well as in epithelial cells of the liver and intestine but not in other tissues, including the hematopoietic system. These studies therefore suggested that adult NSCs may have significantly greater differentiation potential than previously realized but still do not have the pluripotent capability of ES or of the adult derived multipotent adult stem cells (MASC) described in Furcht et al. (International Application No. PCT/US00/21387) and hereia The terms MASC, MAPC and MPC can also be used interchagably to describe adult derived multipotent adult stem cells. Therapies for degenerative and traumatic brain disorders would be significantly furthered with cellular replacement therapies. NSC have been identified in the sub-ventricular zone (SVZ) and the hippocampus of the adult mammalian brain (Ciccolini et al, 1998; Morrison et al, 1999; Palmer et al, 1997; Reynolds and Weiss, 1992; Vescovi et al, 1999) and may also be present in the ependyma and other presumed non-neurogenic areas of the brain (Doetsch et al,
1999; Johansson et al, 1999; Palmer et al, 1999). Fetal or adult brain-derived NSC can be expanded ex vivo and induced to differentiate into astrocytes, oligodendrocytes and functional neurons (Ciccolini et al, 1998; Johansson et al, 1999; Palmer et al, 1999;- Reynolds et al, 1996; Ryder et al, 1990; Studer et al, 1996; Vescovi et al, 1993). In vivo, undifferentiated NSC cultured for variable amounts of time differentiate into glial cells, GABAergic and dopaminergic neurons (Flax et al, 1998; Gage et al, 1995; Suhonen et al, 1996). The most commonly used source of NSC is allogeneic fetal brain, which poses both immunological and ethical problems. Alternatively, NSC could be harvested from the autologous brain. As it is not known whether pre-existing neural pathology will affect the ability of NSC to be cultured and induced to differentiate into neuronal and glial cells ex vivo, and because additional surgery in an already diseased brain may aggravate the underlying disease, this approach is less attractive. The ideal source of neurons and glia for replacement strategies would be cells harvestable from adult, autologous tissue different than the brain that was readily accessible and that can be expanded in vitro and differentiated ex vivo or in vivo to the cell type that is deficient in the patient. Recent reports have suggested that BM derived cells acquire phenotypic characteristics of neuroectodermal cells when cultured in vitro under NSC conditions, or when they enter the central nervous system (Sanchez-Ramos et al, 2000; Woodbury et al, 2000). The phenotype of the BM cells with this capability is not known. The capacity for differentiation of cells that acquire neuroectodermal features to other cell types is also unknown. A third tissue specific cell with stem cell properties is the mesenchymal stem cell (MSC), initially described by Fridenshtein (1982). MSC, originally derived from the embryonal mesoderm and isolated from adult BM, can differentiate to form muscle, bone, cartilage, fat, marrow stroma, and tendon. During embryogenesis, the mesoderm develops into limb-bud mesoderm, tissue that generates bone, cartilage, fat, skeletal muscle and possibly endothelium. Mesoderm also differentiates to visceral mesoderm, which can give rise to cardiac muscle, smooth muscle, or blood islands consisting of endothelium and hematopoietic progenitor cells. Primitive mesodermal or MSCs, therefore, could provide a source for a number of cell and tissue types. A number of MSCs have been isolated. (See, for example, Caplan, A., et al, U.S. Patent No. 5,486,359; Young, H., et al, U.S. Patent No. 5,827,735; Caplan, A., et al, U.S. Patent No. 5,811,094; Bruder, S., et al, U.S. Patent No. 5,736,396; Caplan, A., et al, U.S. Patent No. 5,837,539; Masinovsky, B., U.S. Patent No. 5,837,670; Pittenger, M., U.S. Patent No. 5,827,740; Jaiswal, N., et al, 1997,; Cassiede P., et al, 1996; Johnstone, B., et al, 1998; Yoo, et al, 1998; Gronthos, S., 1994).
Of the many MSC that have been described, all have demonstrated limited differentiation to form cells generally considered to be of mesenchymal origin. To date, the most multipotent MSC reported is the cell isolated by Pittenger, et al, which expresses the SH2+ SH4+ CD29+ CD44+ CD71+ CD90+ CD106+ CD120a+ CD 124" CD 14" CD34" CD45" phenotype. This cell is capable of differentiating to form a number of cell types of mesenchymal origin, but is apparently limited in differentiation potential to cells of the mesenchymal lineage, as the team who isolated it noted that hematopoietic cells were never identified in the expanded cultures (Pittenger, et al, 1999).
Other tissue-specific stem cells have been identified, including gastrointestinal stem cells (Potten, C. 1998), epidermal stem cells (Watt, F. 1997), and hepatic stem cells, also termed oval cells (Alison, M. et al. 1998). Most of these are less well characterized.
Compared with ES cells, tissue specific stem cells have less self-renewal ability and, although they differentiate into multiple lineages, they are not pluripotent. No studies have addressed whether tissue specific cells express the markers described above as seen in ES cells. In addition, the degree of telomerase activity in tissue specific or lineage comitted stem cells has not been fully explored, in part because large numbers of highly enriched populations of these cells are difficult to obtain.
Until recently, it was thought that tissue specific stem cells could only differentiate into cells of the same tissue. A number of recent publications have suggested that adult organ specific stem cells may be capable of differentiation into cells of different tissues. However, the true nature of these types of cells has not been fully discerned. A number of studies have shown that cells transplanted at the time of a BM transplant can differentiate into skeletal muscle (Ferrari 1998; Gussoni 1999). This could be considered within the realm of possible differentiation potential of mesenchymal cells that are present in marrow. Jackson published that muscle satellite cells can differentiate into hemopoietic cells, again a switch in phenotype within the splanchnic mesoderm of the embryo (Jackson 1999). Other studies have shown that stem cells from one embryonic layer (for instance splanchnic mesoderm) can differentiate into tissues thought to be derived during embryogenesis from a different embryonic layer. For instance, endothelial cells or their precursors detected in humans or animals that underwent marrow transplantation are at least in part derived from the marrow donor (Takahashi, 1999; Lin, 2000). Thus, visceral mesoderm and not splanchnic mesoderm, capabilities such as MSC, derived progeny are transferred with the infused marrow. Even more surprising are the reports demonstrating both in rodents and humans that hepatic epithelial cells and biliary duct epithelial cells can be seen in recipients that are derived from the donor marrow (Petersen, 1999; Theise, 2000; Theise, 2000). Likewise, three groups have shown that NSCs can differentiate into hemopoietic cells. Finally, Clarke et al. reported that cells be termed NSCs when injected into blastocysts can contribute to all tissues of the chimeric mouse (Clarke et al, 2000). It is necessary to point out that most of these studies have not conclusively demonstrated that a single cell can differentiate into tissues of different organs. Also, stem cells isolated from a given organ may not necessarily be a lineage committed cell. Indeed most investigators did not identify the phenotype of the initiating cell. An exception is the study by Weissman and Grompe, who showed that cells that repopulated the liver were present in Lin'ThytLowSca^ marrow cells, which are highly enriched in HSCs. Likewise, the Mulligan group showed that marrow Sp cells, highly enriched for HSC, can differentiate into muscle and endothelium, and Jackson et al. showed that muscle Sp cells are responsible for hemopoietic reconstitution (Gussoni et al, 1999).
Transplantation of tissues and organs generated from heterologous ES cells requires either that the cells be further genetically modified to inhibit expression of certain cell surface markers, or that the use of chemotherapeutic immune suppressors continue in order to protect against transplant rejection. Thus, although ES cell research provides a promising alternative solution to the problem of a limited supply of organs for transplantation, the problems and risks associated with the need for immunosuppression to sustain transplantation of heterologous cells or tissue would remain. An estimated 20 immunologically different lines of ES cells would need to be established in order to provide immunocompatible cells for therapies directed to the majority of the population.
Using cells from the developed individual, rather than an embryo, as a source of autologous or from tissue typing matched allogeneic stem cells would mitigate or overcome the problem of tissue incompatibility associated with the use of transplanted ES cells, as well as solve the ethical dilemma associated with ES cell research. The greatest disadvantage associated with the use of autologous stem cells for tissue transplant thus far lies in their relatively limited differentiation potential. A number of stem cells have been isolated from fully-developed organisms, particularly humans, but these cells, although reported to be multipotent, have demonstrated limited potential to differentiate to multiple cell types. Thus, even though stem cells with multiple differentiation potential have been isolated previously by others and by the present inventors, a progenitor cell with the potential to differentiate into a wide variety of cell types of different lineages, including fibroblasts, hepatic, osteoblasts, chondrocytes, adipocytes, skeletal muscle, endothelium, stroma, smooth muscle, cardiac muscle and hemopoietic cells, has not been described. If cell and tissue transplant and gene therapy are to provide the therapeutic advances expected, a stem cell or progenitor cell with the greatest or most extensive differentiation potential is needed. What is needed is the adult equivalent of an ES cell. BM, muscle and brain are the three tissues in which cells with apparent greater plasticity than previously thought have been identified. BM contains cells that can contribute to a number of mesodermal (Ferrari G. et al, 1998; Gussoni E. et al, 1999; Rafii S. et al, 1994; Asahara T. et al, 1997; Lin Y. et al, 2000; Orlic D. et al, 2001; Jackson K. et al, 2001) endodermal (Petersen B.E. et al, 1999; Theise, N.D. et al, 2000; Lagasse E. et al, 2000; Krause D. et al, 2001) and neuroectodermal (Mezey D.S. et al, 2000; Brazelton T.R., et al, 2000, Sanchez- Ramos J. et al, 2000; Kopen G. et al, 1999) and skin (Krause, D. et al, 2001) structures. Cells from muscle may contribute to the hematopoietic system (Jackson K. et al, 1999; Seale P. et al, 2000). There is also evidence that NSC may differentiate into hematopoietic cells (Bjornson C. et al, 1999; Shih C. et al, 2001), smooth muscle myoblasts (Tsai R.Y. et al, 2000) and that NSC give rise to several cell types when injected in a mouse blastocyst (Clarke, D.L. et al, 2000).
The present study demonstrates that cells with multipotent adult progenitor characteristics can be culture-isolated from multiple different organs, namely BM, muscle and the brain. The cells have the same morphology, phenotype, in vitro differentiation ability and have a highly similar expressed gene profile.
SUMMARY OF THE INVENTION The present invention is a multipotent adult stem cell (MASC) isolated from a mammal, preferably mouse, rat or human. The cell is derived from a non- embryonic organ or tissue and has the capacity to be induced to differentiate to form at least one differentiated cell type of mesodermal, ectodermal and endodermal origin. In a preferred embodiment, the organ or tissue from which the MASC are isolated is bone marrow, muscle, brain, umbilical cord blood or placenta.
Examples of differentiated cells that can be derived from MASC are osteoblasts, chondrocytes, adipocytes, fibroblasts, marrow stroma, skeletal muscle, smooth muscle, cardiac muscle, occular, endothelial, epithelial, hepatic, pancreatic, hematopoietic, glial, neuronal or oligodendrocytes. Differentiation can be induced in vivo or ex vivo.
The MASC of the present invention is also summarized as a cell that constitutively expresses oct4 and high levels of telomerase and is negative for CD44, MHC class I and MHC class II expression. As a method of treatment, this cell administered to a patient in a therapeutically effective amount. A surprising benefit of this treatment is that no teratomas are formed in vivo.
An object of the invention is to produce a normal, non-human animal comprising MASC. Preferably, the animal is chimeric. Another embodiment of the invention is a composition comprising a population of MASC and a culture medium that expands the MASC population. It is advantageous in some cases for the medium to contain epidermal growth factor (EGF), platelet derived growth factor (PDGF) and leukemia inhibitory factor (LIF).
The present invention also provides a composition comprising a population of fully or partially purified MASC progeny. The progeny can have the capacity to be further differentiated, or can be terminally differentiated.
In a preferable embodiment, the progeny are of the osteoblast, chondrocyte, adipocyte, fibroblast, marrow stroma, skeletal muscle, smooth muscle, cardiac muscle, occular, endothelial, epithelial, hepatic, pancreatic, hematopoietic, glial, neuronal or oligodendrocyte cell type.
The present invention also provides a method for isolating and propagating MASC by obtaining tissue from a mammal, establishing a population of adherent cells, depleting the population of CD45+ cells, recovering CD45" cells and culturing them under expansion conditions to produce an expanded cell population. An object of the present invention, therefore, is to produce an expanded cell population obtained by this method.
An aspect of the invention is a method for differentiating MASC ex vivo by isolating and propagating them, and then culturing the propagated cells in the presence of desired differentiation factors. The preferred differentiation factors are basic fibroblast growth factor (bFGF), vascular endothelial growth factor (VEGF), dimethylsulfoxide (DMSO) and isoproterenol; or fibroblast growth factor4 (FGF4) and hepatocyte growth factor (HGF). Another aspect of the invention is the differentiated cell itself.
The invention includes a method for differentiating MASC in vivo, by isolating and expanding them, and then administering the expanded cell population to a mammalian host, wherein said cell population is engrafted and differentiated in vivo in tissue specific cells, such that the function of a cell or organ, defective due to injury, genetic disease, acquired disease or iatrogenic treatments, is augmented, reconstituted or provided for the first time. Using this method, the MASC can undergo self-renewal in vivo.
A further aspect of the invention is a differentiated cell obtained by ex vivo or in vivo differentiation. In a preferred embodiment, the differentiated cell is ectoderm, mesoderm or endoderm. In another preferred embodiment, the differentiated cell is of the osteoblast, chondrocyte, adipocyte, fibroblast, marrow stroma, skeletal muscle, smooth muscle, cardiac muscle, occular, endothelial, epithelial, hepatic, pancreatic, hematopoietic, glial, neuronal or oligodendrocyte cell type. An important application of this technology is the method of treating a patient by administering a therapeutically effective amount of MASC or their progeny. The progeny can either have the capacity to be further differentiated, or can be terminally differentiated. An unexpected benefit of this approach is that the need for pretreatment and/or post treatment of the patient with irradiation, chemotherapy, immunosuppressive agents or other drugs or treatments is reduced or eliminated. The induction of tolerance before or during treatment is also not required.
Such treatment can treat a variety of diseases and conditions, including cancer, cardiovascular disease, metabolic disease, liver disease, diabetes, hepatitis, hemophilia, degenerative or traumatic neurological conditions, autoimmune disease, genetic deficiency, connective tissue disorders, anemia, infectious disease and transplant rejection. MASC or their progeny are administered via localized injection, including catheter administration, systemic injection, parenteral administration, oral administration, or intrauterine injection into an embryo. Administration can be in conjunction with a pharmaceutically acceptable matrix, which may be biodegradable.
MASC or their progeny, administered to a patient, alter the immune system to resist viral, bacterial or fungal infection.
Surprisingly, teratomas are not formed when MASC or their progeny are adminstered to a patient. When administered to a patient, MASC or their progeny also are able to augment, reconstitute or provide for the first time the function of a cell or organ defective due to injury, genetic disease, acquired disease or iatrogenic treatments. The organ is any of bone marrow, blood, spleen, liver, lung, intestinal tract, brain, immune system, circulatory system, bone, connective tissue, muscle, heart, blood vessels, pancreas, central nervous system, peripheral nervous system, kidney, bladder, skin, epithelial appendages, breast-mammary glands, fat tissue, and mucosal surfaces including oral esophageal, vaginal and anal. Examples of diseases treatable by this method are cancer, cardiovascular disease, metabolic disease, liver disease, diabetes, hepatitis, hemophilia, degenerative or traumatic neurological conditions, autoimmune disease, genetic deficiency, connective tissue disorders, anemia, infectious disease and transplant rejection.
The MASC or their progeny home to one or more organs in the patient and are engrafted therein such that the function of a cell or organ, defective due to injury, genetic disease, acquired disease or iatrogenic treatments, is augmented, reconstituted or provided for the first time, which is surprising and unexpected. In a preferred embodiment, the injury is ischemia or inflammation.
In another preferred embodiment, the MASC or their progeny enhance angiogenesis.
In an additional aspect of the invnetion, MASC or their progeny are genetically transformed to deliver a therapeutic agent, preferably an antiangiogenic agent.
The invention provides a therapeutic composition comprising MASC and a pharmaceutically acceptable carrier, wherein the MASC are present in an amount effective to produce tissue selected from the group consisting of bone marrow, blood, spleen, liver, lung, intestinal tract, brain, immune system, bone, connective tissue,. muscle, heart, blood vessels, pancreas, central nervous system, kidney, bladder, skin, epithelial appendages, breast-mammary glands, fat tissue, and mucosal surfaces including oral esophageal, vaginal and anal.
The invention further provides a therapeutic method for restoring organ, tissue or cellular function to a patient comprising the steps of removing MASC from a mammalian donor, expanding MASC to form an expanded population of undifferentiatied cells, and adminstering the expanded cells to the patient, wherein organ, tissue or cellular function is restored. The restored function may be enzymatic or genetic. In a preferred embodiment, the mammalian donor is the patient.
The invention provides a method of inhibiting the rejection of a heterologous MASC transplanted into a patient comprising the steps of introducing into the MASC, ex vivo, a nucleic acid sequence encoding the recipient's MHC antigen operably linked to a promotor, wherein the MHC antigen is expressed by the MASC and transplanting the MASC into the patient, wherein MHC antigen is expressed at a level sufficient to inhibit the rejection of the transplanted MASC. The patient is of the same species or another mammalian species as the donor of the MASC. An alternative method of inhibiting the rejection of a heterologous MASC transplanted into a patient comprises transgenically knocking out expression of MHC antigen in the MASC and transplanting the transgenic MASC into the patient MHC antigen is not expressed by the MASC and rejection of the transplanted cells is inhibited. An object of the invention is a method of generating blood or individual blood components ex vivo by the process of isolating MASC and differentiating the MASC to form blood or blood components. Preferably, the individual blood components are red blood cells, white blood cells or platelets.
Another aspect of the invention is a method of drug discovery comprising the steps of analyzing the genomic or proteomic makeup of MASC or their progeny, employing analysis thereof via bioinformatics and/or computer analysis using algorithms, and assembling and comparing new data with known databases to compare and contrast these. A further aspect is a method of identifying the components of a differentiation pathway comprising the steps of analyzing the genomic or proteomic makeup of MASC, inducing differentiation of MASC in vitro or in vivo, analyzing the genomic or proteomic makeup of intermediary cells in the differentiation pathway, analyzing the genomic or proteomic makeup of terminally differentiated cells in the differentiation pathway, using bioinformatics and/or algorithms to characterize the genomic or proteomic makeup of MASC and their progeny, and comparing the data obtained in (e) to identify the components of the pathway. Using this method, differentiation that occurs in vitro can be compared with differentiation that occurs in vivo such that fundamental differences between the two systems can be characterized.
The invention provides a method of generating products in vitro that have therapeutic, diagnostic or research utility by identifying the products in MASC and isolating the products from MASC. In a preferred embodiment, the products are proteins, lipids, complex carbohydrates, DNA or RNA.
Included in the invention is a method of inducing, in a mammal, tolerance to an antigen administered to said mammal, the method comprising the step of administering to said mammal, after or simultaneously with the administration of said antigen, an effective amount of MASC or their progeny so that said mammal's humoral immune response to a subsequent challenge with said antigen is suppressed. Also included is a method for removing toxins from the blood of a patient comprising contacting blood ex vivo with MASC derived cells, wherein said cells line a hollow, fiber based device. In a preferred embodiment, the cells are kidney or liver cells. An object of the invention is a method for delivering therapeutic products to a patient comprising contacting the blood of said patient ex vivo with MASC or their progeny, wherein said MASC or their progeny are genetically transformed to deliver a therapeutic agent.
A further object is a method for testing the toxicity of a drug comprising contacting MASC or their progeny ex vivo with said drug and monitoring cell survival. In a preferred embodiment, the progeny are selected from the group consisting of hepatic, endothelial, epithelial and kidney. BRIEF DESCRIPTION OF DRAWINGS
The following Detailed Description, given by way of example, but not intended to limit the invention to specific embodiments described, may be understood in conjunction with the accompanying drawings, incorporated herein by reference, in which:
Fig. 1 shows a graphical illustration of the expansion potential of of bone marrow (BM), muscle and brain derived MASC.
Fig. 2 shows a scatter plot representing gene expression in (A) muscle and brain MASC and (B) bone marrow and muscle MASC. Fig. 3 shows a graphical illustration of FACS analysis of undifferentiated
MASC and MASC cultured with VEGF. The plots show isotype control IgG staining profile (thin line) vs. specific antibody staining profile (thick line). Panel A shows the phenotype. of undifferentiated MASC. MASC express low levels of β2- microglobulin, Flkl, Fit 1 and AC 133, but do not stain with any of the other anti- endothelial markers; panel B shows the phenotype of MASC cultured for 14 days with 10 ng/mL VEGF. MASC express low levels most markers associated with endothelial cells, but lost expression of AC 133; and panel C shows phenotype of MASC cultured or 3-9 days with 10 ng/mL VEGF. MASC lose expression of AC 133 by day 3 of culture with VEGF, acquire expression of Tek and VE-cadherin by day 3, Tie, vWF, CD34 and HIP12 by day 9.
Fig. 4 shows a photomicrograph of engraftment and in vivo differentiation of mMASC. Slides were examined by fluorescence or confocal microscopy. Panels A, G, J, N, Q and S represent identically stained tissues of control NOD-SCID animals that were not injected with mMASC. Panels A-F show a photomicrograph of bone marrow (BM) cytospin from a control (A) and study (B-F) animal stained with antiβ-gal-FITC antibody and PE-conjugated antibodies to various hematopoietic antigens. A-B: CD45, C: CD19, D: MAC1, E: GR1, F:TER119 and DAPI; panels G- I shows a photomicrograph of a spleen section from a control (G) and study animal (H, I) stained with anti-β-gal-FITC antibody and anti-CD45-PE antibody. Donor derived anti-β-gal+ cells are seen in clusters. H is 10X and I are 60X magnifications; panels J-M shows a photomicrograph of a liver section from a control mouse (J) and study animal (K-M) stained with anti-β-gal-FITC. J-L are co-stained with mouse- anti-CK-18 / anti-mouse-Cy5 plus CD45-PE and M with mouse anti-albumin / anti- mouse Cy3 antibodies. J-K, L and M are 20X, 60X and 10X magnifications respectively; panels N-P show a photomicrograph of an intestine section from a control mouse and study animal (O-P), stained with anti-β-gal-FITC plus mouse- anti-pan-CK / anti-mouse-Cy5 antibodies (N-P). N and P are costained with CD45- PE antibodies. β-gal+ Pan-CK+CD45' epithelial cells covered 50% (solid arrow, panel P) of the circumference of villi. Pan-CK" / β-gal+ cells in the core of the villi (open arrow-panel O) co-stained for CD45 (P); panels Q-R show a photomicrograph of a lung section from a control mouse (Q) and study animal (R) stained with anti-β- gal-FITC plus mouse-anti-pan-CK / anti-mouse-Cy5 plus CD45-PE antibodies. Several β-gal+ pan-CK+ donor cells are seen lining the alveoli of the recipient animal (R). CD45+ / pan-CK" cells of hematopoietic origin are seen distinctly from the epithelial cells; and panels S-T show a photomicrograph of a blood vessel section from a control mouse (S) and thymic lymphoma that developed in a study animal 16 weeks after transplantation (T) stained with anti-β-gal-FITC, anti-vWF-PE and TO- PRO3. β-gal+ donor cells differentiated into vWF+ endothelial cells in the thymic lymphoma which is of recipient origin, as the tumor cells did not stain with anti-β- Gal antibodies.
Fig. 5 shows immunohistochemical evaluation of MASC-derived endothelial cells using confocal fluorescence microscopy, (a) MASC grown for 14 days in VEGF. Typical membrane staining is seen for the adhesion receptor, vβ5, and for the adherens junction proteins, ZO-1, β- and γ-catenin. Scale bar = 50 μm. (b) Morphology in bright field of MASC at day 0 (upper panel) and day 21 (lower panel) after VEGF treatment. Bar = 25 μm.
Fig. 6 shows a photomicrograph of MASC derived endothelial cells. Panel A shows histamine-mediated release of vWF from MASC-derived endothelium. Staining with antibodies against myosin shows cytoskeletal changes with increased numbers of myosin stress fibers, and widening of gap junctions (Arrows) (Representative example of 3 experiments). Scale bar = 60 μm; panel B shows MASC-derived endothelium takes up a-LDL. After 7 days, cells expressed Tie-1, but again did not take up a-LDL. However, acquisition of expression of vVWF on day 9 was associated with uptake of aLDL (representative example of 10 experiments). Scale bar = 100 μm; and panel C shows vascular tube formation by MASC-derived endothelium. After 6h, typical vascular tubes could be seen.
(Representative example of 6 experiments). Scale bar = 200 μm
Fig. 7 shows a graphical illustration of FACS analysis of MASC derived endothelial cells. The Plots show isotype control IgG staining profile (thin line) vs. specific antibody staining profile (thick line) (Representative example of >3 experiments). Number above plots is the Mean Fluorescence Intensity (MFI) for the control IgG staining and the specific antibody staining. Panel A shows hypoxia upregulates Flkl and Tek expression on MASC-derived endothelial cells analyzed by flow cytometry; panel B shows that hypoxia upregulates VEGF production by MASC-derived endothelial cells. VEGF levels were measured by ELISA and the results are shown as Mean ± SEM of 6 experiments; and panel C shows that IL-la induces expression of class II HLA antigens and increases expression of adhesion receptors. Plots show isotype control IgG staining profile (thin line) vs. specific antibody staining profile (thick line) (Representative example of 3 experiments). Number above plots shows MFI for the control IgG staining and the specific antibody staining.
Fig. 8 shows a photomicrograph of human MASC derived endothelial cells. Panels C-F show the 3-D reconstructed figures for either anti-human β2- microglobulin-FITC (panel C) or anti-mouse-CD31-FITC (panel D) and merging of the two (Panel E), anti-vWF-Cy3 (panel F), and merging of the three staining patterns (Panel G). Panels A and B show the confocal image of a single slice stained with either anti -human β2-microglobulin-FITC and anti-vWF-Cy3, or anti-mouse- CD31-Cy5 and anti-vWF-Cy3. Scale bar = 100 μm. Panel H shows wound healing resulting in a highly vascularized area in the punched ear stained with anti-β2- microglobulin-FITC and anti-vWF in mice injected with human MASC-derived endothelial cells (Top panel) or human foreskin fibroblasts (Bottom panel). Scale bar = 20 μm. C= Cartilage. D= dermis. Panel I shows that tumor angiogenesis is derived from endothelial cells generated in vivo from MASC resulting in a highly vascularized area in the tumor stained with anti-X32-microglobulin-FITC, anti-vWF and TOPRO-3. Scale bar = 20 μm.
Fig. 9 shows spiking behavior and expressed voltage-gated sodium currents in hMSC derived neuron-like cells. Panel A shows a photomicrograph of cultured hMSC-derived neurons that showed spiking behavior and expressed voltage-gated sodium currents (the shadow of the pipette points to the cell). Panel B shows graphical illustrations of current-clamp recordings from a hMSC derived neuron.
Panel C shows graphical illustrations of leak-subtracted current traces from the same hMSC derived neuron. Fig. 10 shows quantitative RT-PCR and Western blot analysis confirming the hepatocyte-like phenotype. Panels A and B show mMASC (A) and hMASC (B) cultured on Matrigel™ with FGF4 and HGF or FGF4 alone for 21 and 28 days respectively. For αFP, Cyp2b9 and Cyp2bl3, numbers under the blots are relative to mRNA from liver, as no transcripts were detected in undifferentiated MASC. Li = mouse or human liver mRNA; NT = no-template. Representative example of 5 mouse and 1 human studies, Panel C shows hMASC (B) cultured on Matrigel™ with FGF4 and HGF or FGF4 alone for 21 days. FH= FGF4 and HGF-induced hMASC on Matrigel™, Huh= Huh7 cell line used as control.
Fig. 11 shows a photomicrograph of hepatocyte-like cells. MASC induced by FGF4 produce glycogen. Glycogen storage is seen as accumulation of dark staining (Representative example of 3 studies). Scale bar = 25 μm.
DETAILED DESCRIPTION OF THE INVENTION Defifnitions As used herein, the following terms shall have the following meanings:
"Expansion" shall mean the propogation of a cell without differentiation. "Intermediary cells" are cells produced during differentiation of a MASC that have some, but not all, of the characteristics of MASC or their terminally differentiated progeny. Intermediary cells may be progenitor cells which are committed to a specific pathway, but not to a specific cell type.
"Normal" shall mean an animal that is not diseased, mutated or malformed, i.e., healthy animals.
"Self-renewal" shall mean the ability of cells to propagate without the addition of external stimulation. The presence of cytokines or other growth factors produced locally in the tissue or organ shall not constitute external stimulation.
"Home" shall mean the ability of certain MASC or their progeny to migrate specifically to sites where additional cells may be needed. "Knocking out expression" shall mean the elimination of the function of a particular gene.
As used herein, "genomic or proteomic makeup" shall mean the gene or protein components of a given cell. "High levels of telomerase activity" can be correlated to the two-fold level observed in the immortal human cell line MCF7. Soule et al. (1973) J. Cancer Inst. 51 :1409-1416. Application of this Technology
MASC technology could be used to replace damaged, diseased, dysfunctional or dead cells in the body of a mammal. Furthermore these cells could be injected into the host using autologous or allogeneic cells with or without nature or artificial supports, matrices or polymers to correct for loss of cells, abnormal function or cells or organs e.g. genetic such as mutations of genes affecting a protein function such as sickle cell disease, hemophilia or "storage diseases" where products accumulate in the body because of faulty processing, e.g. Guacher's, Neiman Pick's, mucopolysaccharidosis etc. Examples of restitution of dying or dead cells would be the use of MASC or their differentiated progeny in the treatment of macular degeneration and other neurodegenerative diseases.
Given the ability to have these MASC to "home" to and incorporate into organs/tissues of a host animal proliferate and differentiation they could potentially be used to provide new endothelial cells to an ischemic heart and also myocardial cells themselves, numerous other examples exist.
There may be medical circumstances where transient benefits to a tissue or organs function could have desirable effects. For example, there are now cases with liver failure patients hooked up to a bioartificial liver, which was sufficient to allow for the recovery of normal liver function, obviating the need for a liver transplant. This is a serious unmet medical need, for example in one liver disease alone - hepatitis C. There are 4-5 million Americans currently infected with hepatitis C and there are estimates that 50% of these people will get cirrhosis and need a liver transplant. This is a huge public health problem that is begging for a remedy.
Hepatocytes, derived from autologous or allogeneic MASC, can be transplanted in this or other liver diseases. Such transplants may either transiently provide liver function to allow recovery of the recipient's own liver cells or permanently repopulate a damaged liver to allow recovery of normal liver function via the donor cells.
In addition to many cell therapies where the undifferentiated MASC are administered to a human or other mammal to then differentiate into specific cells in the donor, the progeny of the MASC could be differentiated ex vivo and then be administered as purified or even mixtures of cells to provide a therapeutic benefit.
These MASC in the undifferentiated state could also be used as carriers or vehicles to deliver drugs or molecules of therapeutic benefit. This could be to treat any one of a number of diseases including but not limited to cancer, cardiovascular, inflammatory, immunologic, infections, etc. So by example, a cell perhaps an endothelial cell expressing a novel or high levels of an angiogenic molecule could be administered to a patient which would be incorporated into existing blood vessels to promote angiogenesis, for example in the heart; correspondingly one could have endothelial cells producing molecules that might suppress angiogenesis that would be incorporated into blood cells and inhibit their further formation for example in diabetic retinopathy or in cancer where new blood vessel formation is key to the pathogenesis, spread and extent of the disease.
The ability to populate the BM and to form blood ex vivo has an untold use for important medical applications. For example regarding ex vivo production of blood, the transfusion of blood and blood products around the world is still performed with variable safety because of transmission of infectious agents. Blood transfusions have lead to HIV, hepatitis C and B, and now the impending threat of Mad Cow or CJD, Creuzfeldt- Jakob disease. The ability to produce blood in vitro, especially red blood cells, could provide a safe and reliable alternative to collection of blood from people. It might never fully replace blood collection from donors. hMASC or their hematopoietic progeny could be placed in animals in utero such as sheep which could form human hematopoietic cells and serve as a source for human blood components or proteins of therapeutic utility. The same could be true for hepatocytes, islets or many other cell types but would provide an alternative to producing human cells in vitro and use the animals as factories for the cells. It could also assist in blood shortages that are predicted to occur. hMASC could also conceivably be transplanted into a human embryo to correct any one of a number of defects. Because these MASC can give rise to clonal populations of specifically differentiated cells they are a rich platform for drug discovery. This would involve doing gene expression, analyzing gene expression, discovery of new genes activated patterns of activation, proteomics and patterns of protein expression and modification surrounding this. This would be analyzed with bioinformatics, using data bases and algorithms for analyzing these data compared to publicly available or proprietary data bases. The information of how known drugs or agents might act could be compared to information derived from MASC, their differentiated progeny and from a population of people which could be available. Pathways, targets, and receptors could be identified. New drugs, antibodies or other compounds could be found to produce a biologically desirable responses. Correspondingly, the MASC and their differentiated progeny could be used as monitors for undesirable responses, coupled with databases, bioinformatics and algorithms.
These MASC derived from human, mouse, rat or other mammals appear to be the only normal, non-malignant, somatic cell (non germ cell) known to date to express very high levels of telomerase even in late passage cells. The telomeres are extended in MASC and they are karyotypically normal. Because MASC injected into a mammal, home to multiple organs, there is the likelihood that newly arrived MASC in a particular organ could be self renewing. As such, they have the potential to repopulate an organ not only with themselves but also with self renewing differentiated cell types that could have been damaged, died, or otherwise might have an abnormal function because of genetic or acquired disease.
For example in type I diabetes there is a progressive loss of insulin producing beta cells in the pancreatic islets. In various renal diseases there is progressive loss of function and in some cases obliteration of glomerulus. If in the case of diabetes, MASC or differentiated progeny might home to the pancreas and themselves or via interaction with endogenous cells within the pancreas, induce islets to be formed. This would have an ameliorating impact on diabetes. Ultimately conditions, agents or drugs might be found to in vivo control, i.e. promote or inhibit their self renewing capability of the MASC and control, or enhance or inhibit the movement to differentiated progeny, e.g., islet precursors, hepatocyte precursors, blood precursors, neural and/or cardiac precursors using MASC one will likely find pathways, methods of activation and control that might induce endogenous precursor cells within an organ to proliferate and differentiation.
This same ability to repopulate a cellular tissue or organ compartment and self renew and also differentiate could have numerous uses and be of unprecedented usefulness to meet profound unmet medical needs. So for example certain genetic diseases where there are enzyme deficiencies have been treated by BM transplantation. Often times this may help but not cure the complications of the disease where residual effects of the disease might persist in the brain or bones or elsewhere, MASC and genetically engineered MASC offer the hope to ameliorate numerous genetic and acquired diseases. They will also be useful for diagnostic and research purposes and drug discovery.
The present invention also provides methods for drug discovery, genomics, proteomics, and pathway identification; comprising analyzing the genomic or proteomic makeup of a MASC, coupled with analysis thereof via bioinformatics, computer analysis via algorithms, to assemble and compare new with known databases and compare and contract these. This will identify key components, pathways, new genes and/or new patterns of gene and protein expression and protein modification (proteomics) that could lead to the definition of targets for new compounds, antibodies, proteins, small molecule organic compounds, or other biologically active molecules that would have therapeutic benefit.
EXAMPLES
The following examples are provided to illustrate but not limit the invention.
Example 1. Selection, Culture and Characterization of Mouse Multipotent Adult Stem Cells (mMASC)
Cell Isolation and Expansion
All tissues were obtained according to guidelines from the University of
Minnesota IACUC. BM mononuclear cells (BMMNC) were obtained by ficoll- hypaque separation of BM was obtained from 5-6 week old ROSA26 mice or C57/BL6 mice. Alternatively, muscle and brain tissue was obtained from 3-day old
129 mice. Muscles from the proximal parts of fore and hind limbs were excised from and thoroughly minced. The tissue was treated with 0.2% collagenase (Sigma
Chemical Co, St Louis, MO) for 1 hour at 37°C, followed by 0.1% trypsin
(Invitrogen, Grand Island, NY) for 45 minutes. Cells were then triturated vigorously and passed through a 70-um filter. Cell suspensions were collected and centrifiiged for 10 minutes at 1600 rpm. Brain tissues was dissected and minced thoroughly.
Cells were dissociated by incubation with 0.1% trypsin and 0.1% DNAse (Sigma) for 30 minutes at 37 °C. Cells were then triturated vigorously and passed through a 70-um filter. Cell suspension was collected and centrifiiged for 10 minutes at 1600 rpm.
BMMNC or muscle or brain suspensions were plated at 1x10 /cm in expansion medium [2% FCS in low glucose Dulbecco's minimal essential medium
(LG-DMEM), 10 ng/mL each platelet derived growth factor (PDGF), epidermal growth factor (EGF) and leukemia inhibitory factor (LIF)] and maintained at
5x10 /cm . After 3-4 weeks, cells recovered by trypsin/EDTA were depleted of CD45+/glycophorin (Gly)-A+ cells with micromagnetic beads. Resulting CD45" /Gly-A" cells were replated at 10 cells/well in 96-well plates coated with FN and were expanded at cell densities between 0.5 and 1.5x 10 /cm . The expansion potential of MASC was similar regardless of the tissue from which they were derived (Fig. 1). Characterization of MASC
Phenotypically, mMASC derived from BM, muscle and brain and cultured on FN were CD13+, CD44", CD45", class-I and class-II histocompatibility antigen", Flkllow and cKit", identical to the characteristics of hMASC, as described in
Internation Application No. PCT/USOO/21387. Although cell expansion during the initial 2-3 months was greater when cells were cultured on collagen type IV, laminin or Matrigel™, cells had phenotypic characteristics of MSC, i.e., expressed CD44 and did not express CD13. As with human cells, mMASC cultured on FN expressed transcripts for oct-4, and the LIF-R.
Approximately 1 % of wells seeded with 10 CD457GlyA" cells yielded continuous growing cultures. This suggests that the cells capable of initiating MASC cultures are rare and likely less that 1/1,000 of CD457GlyA" cells. mMASC cultured on FN were 8-10 μm in diameter with a large nucleus and scant cytoplasm. Several populations have been cultured for > 100 PDs. The morphology and phenotype of cells remained unchanged throughout culture. mMASC that had undergone 40 and 102 PDs were harvested and telomere lengths evaluated. Telomere length was measured using the Telomere Length Assay Kit from Pharmingen (New Jersey, USA) according to the manufacturer's recommendations. Average telomere length (ATL) of mMASC cultured for 40 PDs was 27 Kb. When re-tested after 102 PDs, ATL remained unchanged. For karyotyping of mMASC, cells were subcultured at a 1 :2 dilution 12h before harvesting, collected with trypsin-EDTA, and subjected to a 1.5h colcemid incubation followed by lysis with hypotonic KC1 and fixation in acid/alcohol as previously described (VerfaiUie et al, 1992). Cytogenic analysis was conducted on a monthly basis and showed a normal karyotype, except for a single. population that became hyperdiploid after 45 PDs, which was no longer used for studies. Murine MASC obtained after 46 to >80 PDs were tested by Quantitative (Q)-
RT-PCR for expression levels of Oct4 and Rexl, two transcription factors important in maintaining an undifferentiated status of ES cells. RNA was extracted from mouse MASC, neuroectodermal differentiated progeny (day 1- 7 after addition of bFGF) and mouse ES cells. RNA was reverse transcribed and the resulting cDNA underwent 40 rounds of amplification (ABI PRISM 7700, Perkin Elmer/ Applied Biosystems) with the following reaction conditions: 40 cycles of a two step PCR (95°C for 15 seconds, 60°C for 60 seconds) after initial denaturation (95°C for 10 minutes) with 2 μl of DNA solution, IX TaqMan SYBR Green Universal Mix PCR reaction buffer. Primers are listed in Table 1. Table 1 : Primers used
Figure imgf000025_0001
mRNA levels were normalized using GAPDH as housekeeping gene, and compared with levels in mouse ES cells. Oct4 and Rex 1 mRNA were present at similar levels in BM, muscle and brain derived MASC. Rexl mRNA levels were similar in mMASC and mES cells, while Oct4 mRNA levels were about 1,000 fold lower in MASC than in ES cells.
Expressed gene profile of mouse BM. muscle and brain derived MASC is highly similar To further evaluate whether MASC derived from different tissues were similar, the expressed gene profile of BM, muscle and brain derived MASC was examined using U74A Affimetrix gene array. Briefly, mRNA was extracted from 2-
3xl06 BM, muscle or brain derived-MASC, cultured for 45 population doublings.
Preparation of cDNA, hybridization to the U74A array containing 6,000 murine genes and 6,000 EST clusters, and data acquisition were done per manufacturer's recommendations (all from Affimetrix, Santa Clara, CA). Data analysis was done using GeneChip® software (Affimetrix). Increased or decreased expression by a factor of 2.2 fold (Iyer V.R. et al, 1999; Scherf U. et al, 2000; Alizadeh A. A. et al, 2000) was considered significant, r value was determined using linear regression analysis (Fig.2).
Comparison between the expressed gene profile in MASC from the three tissues showed that <1% of genes were expressed at >2.2-fold different levels in MASC from BM than muscle. Likewise, only <1% of genes were expressed > 2.2- fold different level in BM than brain derived MASC. As the correlation coefficient between the different MASC populations was > 0.975, it was concluded that MASC derived from the different tissues are highly homologous, in line with the phenotypic described above and the differentiation characteristics described in Example 5.
Using the mouse-specific culture conditions, mMASC cultures have been maintained for more than 100 cell doublings. mMASC cultures have been initiated with marrow from C57B1/6 mice, ROSA26 mice and C57BL/6 mice transgenic for the -HMG-LacZ.
Example 2. Selection and Culture of Rat Multipotent Adult Stem Cells (rMASC)
BM and MNC from Sprague Dawley or Wistar rats were obtained and plated under conditions similar for mMASC. After 21-28 days, cells were depleted of
CD45+ cells, and the resulting CD45" cells were subcultured at 10 cells/well.
Similar to mMASC, rMASC have been culture expanded for >100 PDs.
Expansion conditions of rat MASC culture required the addition of EGF, PDGF-BB and LIF and culture on FN, but not collagen type I, laminin or Matrigel™. rMASC were CD44, CD45 and MHC class I and II negative, and expressed high levels of telomerase. The ability of a normal cell to grow over 100 cell doublings is unprecedented, unexpected and goes against conventional dogma of more than two decades.
Rat MASC that had undergone 42 PDs, 72 PDs, 80 PDs, and 100 PDs, were harvested and telomere lengths evaluated. Telomeres did not shorten in culture, as was determined by Southern blot analysis after 42 PDs, 72 PDs, 80 PDs, and 100
PDs. Monthly cytogenetic analysis of rat MASC revealed normal karyotype.
Example 3. Selection and Culture of Human Multipotent Adult Stem Cells (hMASC)
BM was obtained from healthy volunteer donors (age 2-50 years) after informed consent using guidelines from the University of Minnesota Committee on the use of Human Subject in Research. BMMNC were obtained by Ficoll-Paque density gradient centrifugation and depleted of CD45+ and glycophorin-A+ cells using micromagnetic beads (Miltenyii Biotec, Sunnyvale, CA).
Expansion conditions: 5x 103 CD457GlyA" cells were diluted in 200 μL expansion medium [58% DMEM-LG, 40% MCDB-201 (Sigma Chemical Co, St Louis, MO), supplemented with IX insulin-transferrin-selenium (ITS), IX linoleic- acid bovine serum albumin (LA-BS A), 10"8 M Dexamethasone, 10"4 M ascorbic acid 2-phosphate (all from Sigma), 100 U penicillin and 1,000 U streptomycin (Gibco)] and 0-10% fetal calf serum (FCS) (Hyclone Laboratories, Logan, UT) with 10 ng/ml of EGF (Sigma) and 10 ng/ml PDGF-BB (R&D Systems, Minneapolis, MN)] and plated in wells of 96 well plates that had been coated with 5 ng/ml of FN (Sigma). Medium was exchanged every 4-6 days. Once wells were >40-50% confluent, adherent cells were detached with 0.25% trypsin-EDTA (Sigma) and replated at 1 :4 dilution in MASC expansion medium and bigger culture vessels coated with 5 ng/ml FN to maintain cell densities between 2 and 8x10 cells/cm . Undifferentiated MASC did not express CD31 , CD34, CD36, CD44, CD45,
CD62-E, CD62-L, CD62-P, HLA-class I and II, cKit, Tie, Tek, αvβ3, VE-cadherin, vascular cell adhesion molecule (VCAM), intracellular adhesion molecule (ICAM)- 1. MASC expressed low/very low levels of β2-microglobulin, αvβs, CDw90, AC133, Flkl and Fltl, and high levels of CD13 and CD49b (Fig. 3). Example 4. Immunophenotypic Analysis
Immunofluorescence
1. Cultured cells were fixed with 4% paraformaldehyde and methanol at room temperature, and incubated sequentially for 30 min each with primary antibody, and with or without secondary antibody. Between steps, slides were washed with PBS/BSA. Cells were examined by fluorescence microscopy (Zeiss Axiovert; Carl Zeiss, Inc., Thornwood, NY) and confocal fluorescence microscopy (Confocal 1024 microscope; Olympus AX70, Olympus Optical Co. LTD, Japan). To assess the frequency of different cell types in a given culture, the number of cells were counted that stained positive with a given antibody in four visual fields (50-200 cells per field).
2. Harvested tissues: Cytospin specimens of blood and BM were fixed with acetone (Fisher Chemicals) for 10 min at room temperature. For solid organs, 5 μm thick fresh frozen sections of tissues were mounted on glass slides and immediately fixed in acetone for 10 min at room temperature. Following incubation with isotype sera for 20 min, cytospin preparations or tissue sections were serially stained for tissue specific antigens, β-gal and a nuclear counter stain (DAPI or TO-PRO-3). Cover slips were mounted using Slowfade-antifade kit (Molecular Probes Inc., Eugene, OR, USA). Slides were examined by fluorescence microscopy and confocal fluorescence microscopy.
3. Antibodies: Cells were fixed with 4% paraformaldehyde at room temperature or methanol at -20°C, and incubated sequentially for 30 min each with primary Ab, and FITC or Cy3 coupled anti-mouse- or anti-rabbit-IgG Ab. Between each step slides were washed with PBS+1 %BSA. PE or FITC-coupled anti-CD45, anti-CD31, anti-CD62E, anti-Macl, anti-Grl, anti-CD19, anti-CD3, and anti-Terl l9 antibodies were obtained from BD Pharmingen. Abs against GFAP (clone G-A-5, 1 :400), galactocerebroside (GalC) (polyclonal, 1 :50), MBP (polyclonal, 1 :50), GAB A (clone GB-69, 1 :100), parvalbumin (clone PARV-19, 1 :2000), TuJl (clone SDL.3D10, 1 :400), NF-68 (clone NR4, 1 :400), NF-160 (clone NN 18, 1 :40), and NF-200 (clone N52, 1 :400), NSE (polyclonal, 1 :50), MAP2-AB (clone AP20, 1 :400), Tau (polyclonal, 1 :400), TH (clone TH-2, 1 :1000), DDC (clone DDC-109, 1 :100), TrH (clone WH-3, 1 :1000), serotonin (polyclonal, 1 :2000), glutamate (clone GLU-4, 1 :400), fast twitch myosin (clone MY-32; 1 :400 dilution) were from Sigma.
DAPI and TOPRO-3 were from Molecular Probes. Abs against vWF (polyclonal;
1 :50) Neuro-D (polyclonal, 1 :50), c-ret (polyclonal, 1 :50) and Nurrl (polyclonal,
1 :50) were from Santa Cruz Biotechnology Inc., Santa Cruz, CA. Abs against PSA- NCAM (polyclonal, 1 :500) from Phanmingen, San Diego, CA and against serotonin transporter (clone MAB 1564, 1 :400), DTP (polyclonal, 1 :200), Na-gated voltage channel (polyclonal, 1 :100), glutamate-receptors-5, -6 and -7 (clone 3711 :500) and
NMDA (polyclonal 1 :400) receptor from Chemicon International, Temecula, CA.
Anti-nestin (1 :400) Abs were a kind gift from Dr. U. Lendahl, University of Lund, Sweden. Antibodies against NSE (1 :50) pan-cytokeratin (catalog number C-2562; 1 :100), CK-18 (C-8541; 1 :300), albumin (A-6684; 1 :100) were all obtained from Sigma. Polyclonal antibodies against Flkl , Fltl , Tek, HNF-1 β were obtained from Santa Cruz Biotechnology Inc., Santa Cruz, CA. Anti-nestin (1 :400) antibodies were a kind gift from Dr. U. Lendahl, University of Lund, Sweden. Control-mouse, - rabbit or, -rat IgGs and FITC/PE/Cy3- and Cy5-labeled secondary antibodies were obtained from Sigma. Rabbit anti-β-gal-FITC antibody was obtained from Rockland Immunochemicals, USA. TO-PRO-3 was obtained from Molecular Probes Inc. and DAPI was obtained from Sigma.
B. X-GAL staining: Tissue sections were stained by for β-galactosidase enzyme activity using β-gal staining kit from Invitrogen, pH 7.4. Manufacturer's instructions were followed except for the fixation step, during which the tissue sections were incubated for 5 min instead of 10 min.
C. FACS: For FACS, undifferentiated MASC were detached and stained sequentially with anti-CD44, CD45, CD13, cKit, MHC-class I and II, or b2- microglobulin (BD Pharmingen) and secondary FITC or PE coupled antibodies, fixed with 2% paraformaldehyde until analysis using a FACS-Calibur (Becton- Dickinson).
Example 5. Single Cell Origin of Differentiated Lineages from MASC
The differentiation ability of mMASC or rMASC was tested by adding differentiation factors (cytokines) chosen based on what has been described for differentiation of hMASC or ES cells to mesoderm, neuroectoderm, and endoderm. Differentiation required that cells were replated at l-2xl04 cells/cm2 in serum free medium, without EGF, PDGF-BB and LIF, but with lineage specific cytokines. Differentiation was determined by immunohistology for tissue specific markers
[slow twitch myosin and MyoD (muscle), von-Willebrand factor (vWF) and Tek
(endothelium), NF200 and MAP2 (neuroectodermal), and cytokeratin-18 and albumin (endodermal)], RT-PCR, and functional studies. MASC Differentiation into Neuroectodermal Cells
Palmer et al. showed that neuroprogenitors can be culture expanded with
PDGF-BB and induced to differentiate by removal of PDGF and addition of bFGF as a differentiation factor. Based on those studies and studies conducted using hMASC, mMASC and rMASC were plated in FN coated wells without PDGF-BB and EGF but with 100 ng/mL bFGF. Progressive maturation of neuron-like cells was seen throughout culture. After 7 days, the majority of cells expressed nestin. After 14 days, 15-20% of MASC acquired morphologic and phenotypic characteristics of astrocytes (GFAP+), 15-20% of oligodendrocytes (galactocerebroside (GalC)+) and 50-60% of neurons (neurofilament-200 (NF- 200)+). NF200, GFAP or GalC were never found in the same cell, suggesting that it is unlikely that neuron-like cells were hMASC or glial cells that inappropriately expressed neuronal markers. Neuron-like cells also expressed Tau, MAP2 and NSE. Approximately 50% of neurons expressed gamma-amino-butyric-acid (GABA) and parvalbumin, 30% tyrosine hydroxylase and dopa-decarboxylase (DDC), and 20% serotonin and tryptophan hydroxylase. Differentiation was similar when MASC had been expanded for 40 or >90 PDs. Q-RT-PCR, performed as described in Example 1, confirmed expression of neuroectodermal markers: on day 2 MASC expressed otxl and otx2 mRNA, and after 7 days nestin mRNA was detected.
The effect of fibroblast growth factor (FGF)-8b as a differentiation factor was tested next. This is important in vivo for midbrain development and used in vitro to induce dopaminergic and serotoninergic neurons from murine ES cells on hMASC. When confluent hMASC (n=8) were cultured with 10 ng/mL FGF-8b + EGF, differentiation into cells staining positive for neuronal markers but not oligodendrocytes and astrocytes was seen. Neurons had characteristics of GABAergic (GABA+; 40±4%), dopaminergic (DOPA, TH, DCC and DTP+, 26±5%) and serotoninergic (TrH, serotonin and serotonin-transporter+, 34±6%) neurons. DOPA+ neurons stained with Abs against Nurrl suggesting differentiation to midbrain DA neurons. FGF-8b induced neurons did not have electrophysiological characteristics of mature neurons. Therefore, cocultured cells from 3 -week old
FGF-8b supported cultures with the glioblastoma cell line, U-87, and FGF-8b for an additional 2-3 weeks.
Neurons acquired a more mature morphology with increased cell size and number, length and complexity of the neurites, and acquired electrophysiological characteristics of mature neurons (a transient inward current, blocked reversibly by 1 μM tetrodotoxin (TTX) together with the transient time course and the voltage- dependent activation of the inward current is typical for voltage-activated sodium currents, found only in mature neurons). When hMASC (n=13) were cultured with 10 ng/m brain-derived neurotrophic factor (BDNF) + EGF, differentiation was to exclusively DOPA, TH, DCC, DTP and Nurrl positive neurons. Although BDNF supports neural differentiation from ES cells and NSC (Peault, 1996; Choi et al. 1998), no studies have shown exclusive differentiation to DA-like neurons. Similar results were seen for mMASC induced with bFGF and rMASC with bFGF and BDNF. Further studies on MASC-derived neuronal cells are presented in Example 10. MASC Differentiation into Endothelial Cells
As an example of mesoderm, differentiation was induced to endothelium. Undifferentiated mMASC or rMASC did not express the endothelial markers CD31 , CD62E, Tek or vWF, but expressed low levels of Flkl . mMASC or rMASC were cultured in FN-coated wells with 10 ng/mL of the endothelial differentiation factor VEGF-B. Following treatment with VEGF for 14 days, >90% of MASC, irrespective of the number of PDs they had undergone, expressed Fltl, CD31, vWF or CD62, consistent with endothelial differentiation. Like primary endothelial cells, MASC-derived endothelial cells formed vascular tubes within 6 hours after replating in Matrigel™.
Similarly, hMASC express Flkl and Fltl but not CD34, Mucl8 (P1H12), PECAM, E- and P-selectin, CD36, or Tie/Tek. When hMASC 2xl04 cells/cm2 were cultured in serum free medium with 20 ng/mL vascular endothelial growth factor (VEGF), cells expressed CD34, VE-cadherin, VCAM and Muc-18 from day 7 on. On day 14, they also expressed Tie, Tek, Flkl and Fltl, PECAM, P-selectin and E- selectin, CD36, vWF, and connexin-40. Furthermore, cells could uptake low- density lipoproteins (LDL). Results from the histochemical staining were confirmed by Western blot. To induce vascular tube formation, MASC cultured for 14 days with VEGF were replated on Matrigel™ with 10 ng/mL VEGF-B for 6h.
Endothelial differentiation was not seen when hMASC cultured in >2% FCS were used. In addition, when FCS was left in the media during differentiation, no endothelial cells were generated.
At least 1000-fold expansion was obtained when hMASC were sub-cultured, suggesting that endothelial precursors generated from hMASC continue to have significant proliferative potential. Cell expansion was even greater when FCS was added to the cultures after day 7.
When hMASC derived endothelial cells were administered intravenously (IN.) in ΝOD-SCI mice who have a human colon-carcinoma implanted under the skin, contribution of the human endothelial cells could be seen to the neovascularization in the tumors. It may therefore be possible to incorporate genetically modified endothelial cells to derive a therapeutic benefit, i.e., to inhibit angiogenesis in for example cancer or to promote it to enhance vascularization in limbs or other organs such as the heart. Further studies on MASC-derived endothelial cells are presented in Example 9. MASC Differentiation into Endoderm Whether mMASC or rMASC could differentiate to endodermal cells was tested. A number of different culture conditions were tested including culture with the diffentiation factors keratinocyte growth factor (KGF), hepatocyte growth factor (HGF) and FGF-4, either on laminin, collagen, FΝ or Matrigel™ coated wells. When re-plated on Matrigel™ with 10 ng/mL FGF4 + 10 ng/mL HGF, approximately 70% of MASC acquired morphologic and phenotypic characteristics of hepatocyte-like cells. Cells became epithelioid, approximately 10% of cells became binucleated, and about 70% of cells stained positive for albumin, cytokeratin (CK)-18, and HΝF-lP.
Endodermal-like cells generated in FGF4 and HGF containing cultures also had functional characteristics of hepatocytes, determined by measuring urea levels in supernatants of undifferentiated MASC and FGF4 and HGF-induced MASC using the Sigma Urea Nitrogen Kit 640 according to the manufacturer's recommendations.. No urea was detected in undifferentiated MASC cultures. Urea production was 10 μg/cell/hr 14 days after adding FGF4 and HGF and remained detectable at similar levels until day 25. This is comparable to primary rat hepatocytes grown in monolayer. Presence of albumin together with urea production supports the notion of hepatic differentiation from MASC in vitro. Further studies on MASC-derived hepatocytes are presented in Example 11.
Given the likely existence of an endodermal lineage precursor cell, MASC likely give rise to a cell that forms various cells in the liver in the pancreas both exocrine and endocrine components and other endodermal derived cell tissue lineages. MASC derived from muscle or brain were induced to differentiate to mesoderm (endothelial cells), neuroectoderm (astrocytes and neurons) and endoderm (hepatocyte-like cells) using the methods described above for BM-derived MASC. Transduction To demonstrate that differentiated cells were single cell derived and MASC are indeed "clonal" multipotent cells, cultures were made in which MASC had been transduced with a retroviral vector and undifferentiated cells and their progeny were found to have the retrovirus inserted in the same site in the genome.
Studies were done using two independently derived ROSA26 MASC, two C57BL/6 MASC and one rMASC population expanded for 40 to >90PDs, as well as with the eGFP transduced "clonal" mouse and "clonal" rMASC. No differences were seen between eGFP transduced and untransduced cells. Of note, eGFP expression persisted in differentiated MASC.
Specifically, murine and rat BMMNC cultured on FN with EGF, PDGF-BB and LIF for three weeks were transduced on two sequential days with an eGFP oncoretro viral vector. Afterwards, CD45+ and GlyA+ cells were depleted and cells sub-cultured at 10 cells/well. eGFP-transduced rat BMMNC were expanded for 85 PDs. Alternatively, mouse MASC expanded for 80 PDS were used. Subcultures of undifferentiated MASC were generated by plating 100 MASC from cultures maintained for 75 PDs and re-expanding them to > 5xl06 cells. Expanded MASC were induced to differentiate in vitro to endothelium, neuroectoderm and endoderm. Lineage differentiation was shown by staining with antibodies specific for these cell types, as described in Example 4. Single cell origin of mesodermal and neuroectodermal progeny
To prove single cell origin of mesodermal and neuroectodermal differentiated progeny retroviral marking was used (Jordan et al, 1990; Nolta et al,
1996). A fraction of hMASC obtained after 20 PDs was transduced with an MFG- eGFP retrovirus. eGFP+ hMASC were diluted in non-transduced MASC from the same donors to obtain a final concentration of ~5% transduced cells. These mixtures were plated at 100 cells/well and culture expanded until >2xl07 cells were obtained. 5xl06 MASC each were induced to differentiate to skeletal myoblasts, endothelium and neuroectodermal lineages. After 14 days under differentiation conditions, cells were harvested and used to identify the retroviral integration site and co-expression of eGFP and neuroectodermal, muscle and endothelial markers. For myoblast differentiation, hMASC were plated at 2xl04 cells/cm2 in 2% FCS, EGF and PDGF containing expansion medium and treated with 3 μM 5- azacytidine in the same medium for 24h. Afterwards, cells were maintained in expansion medium with 2% FCS, EGF and PDGF-BB. For endothelial differentiation, hMASC were replated at 2xl04 cells/cm2 in serum-free expansion medium without EGF and PDGF but with 10 ng/ml VEGF-B for 14 days.
Immunofluorescence evaluation showed that 5-10% of cells in cultures induced to differentiate with 5-azacytidine stained positive for eGFP and skeletal actin, 5- 10% of cells induced to differentiate to endothelium costained for eGFP and vWF, and 5-10% of cells induced to differentiate to neuroectoderm costained for eGFP and either NF-200, GFAP or MBP. To define the retroviral insertion site, the host genomic flanking region in MASC and differentiated progeny was sequenced. The number of retroviral inserts in the different populations was between one and seven. As shown in Table 2, a single, identical sequence flanking the retroviral insert in muscle, endothelium and neuroectodermal cells in population A16 that mapped to chromosome 7 was identified. Table 2: Single cell origin of endothelium, muscle and neuroectodermal cells
Sequence: 3,-LTR-ccaaatt
Clone A16 TAG CGGCCGCTTG AATTCGAACG CGAGACTACT GTGACTCACA CT (Chrom. 7)
5- TAG CGGCCGCTTG AATTCGAACG CGAGACTACT GTGACTCACA CT Azacytidine
VEGF TAG CGGCCGCTTG AATTCGAACG CGAGACTACT GTGACTCACA CT bFGF TAG CGGCCGCTTG AATTCGAACG CGAGACTACT GTGACTCACA CT
Clone A12- ATTTATA TTCTAGTTTAT TTGTGTTTGGG GCAGACGAGG
A (Chrom.
9)
5- ATTTATA TTCTAGTTTAT TTGTGTTTGGG GCAGACGAGG
Azacytidine
VEGF ATTTATA TTCTAGTTTAT TTGTGTTTGGG GCAGACGAGG bFGF ATTTATA TTCTAGTTTAT TTGTGTTTGGG GCAGACGAGG
Clone A12- TCCTGTCTCA TTCAAGCCAC ATCAGTTACA TCTGCATTTT
A (Chrom.
12)
TCCTGTCTCA TTCAAGCCAC ATCAGTTACA TCTGCATTTT
Azacytidine
VEGF TCCTGTCTCA TTCAAGCCAC ATCAGTTACA TCTGCATTTT bFGF TCCTGTCTCA TTCAAGCCAC ATCAGTTACA TCTGCATTTT
Primers specific for the 3' LTR were designed and for the flanking genomic sequence are shown in Table 3 and using Real-time PCR, it was confirmed that the retroviral insert site was identical in undifferentiated and differentiated cells. These results proved that the flanking sequence and the eGFP DNA sequence was present in similar quantities. Clone A12 contained two retroviral inserts, located on chromosome 1 and 7 respectively, and both flanking sequences could be detected not only in hMASC but also muscle, endothelium and neuroectodermal lineages. To determine whether this represented progeny of a single cell with two retroviral integrants or progeny of two cells, Real -Time PCR was used to compare the relative amount of the chromosome 1 and 7 flanking sequence to eGFP. It was found that similar amounts of both flanking regions were present in hMASC, muscle, endothelium and neuroectodermal cells, suggesting that a single cell with two retroviral inserts was likely responsible for the eGFP positive hMASC and differentiated progeny. In the other populations containing 3 or more retroviral inserts we were not able to determine whether the inserts were due to multiple insertion sites in a single cells or multiple cells contributing to the eGFP positive fraction. Nevertheless, our finding that in 2 populations, progeny differentiated into muscle, endothelium and neuroectoderm are derived from a single BM derived progenitor cell definitively proves for the first time that primitive cells can be cultured from BM that differentiate at the single cell level in cells of mesodermal lineage as well as the three different lineages of the neuroectoderm.
Table 3: Flankin re ions and rimers
Figure imgf000036_0001
Bold: MSCV LTR; Bold and underlined: MSCV LTR primer used for Q-PCR
Italics and underlined: Flanking sequence primers used for Q-PCR.
Example 6. Homing and Engraftment of Mammalian MASC into Numerous Organs in the Body mMASC were tested to determine whether they had the ability to engraft and differentiate in vivo into tissue specific cells. mMASC were grown as described in Example 1 from a LacZ transgenic C57 Black 6, ROSA 26 mouse. 106 mMASC from the LacZ mouse were IN. injected into ΝOD-SCID mice tail veins with or without 250 Rads of total body radiation 4-6 hrs prior to the injection. The animals were sacrificed by cervical dislocation at 4-24 weeks after the injections. Tissue Harvest
Blood and bone marrow: 0.5-1 ml of blood was obtained at the time animals were sacrificed. BM was collected by flushing femurs and tibias. For phenotyping, red cells in blood and BM were depleted using ice cold ammonium chloride (Stem Cell Technologies Inc., Vancouver, Canada) and 105 cells used for cytospin centrifugation. For serial transplantation, 5x10 cells from 2 femurs and 2 tibias were transplanted into individual secondary recipients via tail vein injection. Secondary recipients were sacrificed after 7-10 weeks. Solid organs: Lungs were inflated with 1 ml 1 :4 dilution of OCT compound
(Sakura-Finetek Inc, USA) in PBS. Specimens of spleen, liver, lung, intestine, skeletal muscle, myocardium, kidney and brain of the recipient animals were harvested and cryopreserved in OCT at -80°C and in RNA Later (Ambion Inc.,
Austin, TX, USA) at -20°C for quantitative PCR. mMASC engraft and differentiate in tissue specific cells in vivo
Engraftment of the β-gal/neomycin (NEO) transgene-containing cells (Zambrowicz et al, 1997) was tested by immunohistochemistry for β-gal and by Q- PCR for NEO. Immunohistochemistry and Q-PCR were performed as described in Examples 5 and 1 respectively. Primers are listed in Table 1.
Engraftment, defined as detection of >1% anti-β-gal cells, was seen in hematopoietic tissues (blood, BM and spleen) as well as epithelium of lung, liver, and intestine of all recipient animals as shown in Table 4 and Fig. 4.
Table 4: Engraftment levels in NOD-SCID mice transplanted with ROSA26
MASC.
Figure imgf000037_0001
β-gal+ cells in BM (Fig. 4B-F) and spleen (Fig. 4H-I) co-labeled with anti-
CD45, anti-CD19, anti-Macl, anti-Grl and anti-TERl 19 Abs. Similar results were seen for peripheral blood. Of note, no β-gal+CD3+ T cells were seen in either blood,
BM or spleen even though β-gal+CD3+ T-cells were seen in chimeric mice. The reason for this is currently not known.
Engraftment in the spleen occurred mostly as clusters of donor cells, consistent with the hypothesis that when MASC home to the spleen, they proliferate locally and differentiate to form a colony of donor cells, similar to CFU-S. It is not believed that differentiation of mMASC into hematopoietic cells in vivo can by attributed to contamination of the mMASC with HSC. First, BMMNC are depleted of CD45 cells by column selection before mMASC cultures are initiated. Second, early mesodermal or hematopoietic transcription factors, including brachyury (Robertson et al, 2000), GATA-2 and GATA-1 (Weiss et al, 1995), are not expressed in undifferentiated mMASC, as shown by cDNA array analysis. Third, the culture conditions used for mMASC are not supportive for HCS. Fourth all attempts at inducing hematopoietic differentiation from hMASC in vitro, by co- culturing hMASC with hematopoietic supportive feeders and cytokines, have been unsuccessful (Reyes et al, 2001).
Significant levels of mMASC engraftment were also seen in liver, intestine and lung. Triple-color immunohistochemistry was used to identify epithelial (CK+) and hematopoietic (CD45+) cells in the same tissue sections of the liver, intestine and lung. In the liver, β-gal+ donor-derived cells formed cords of hepatocytes (CK18+CD45+ or albumin+), occupying about 5-10% of a given 5μm section (Fig. 4K-M). Several CKl 8+CD45+β-gal" hematopoietic cells of recipient origin were distinctly identified from the epithelial cells. Albumin+β-gal+ and CKl 8+β-gal+ cells engrafted in cords of hepatocytes surrounding portal tracts, a pattern seen in hepatic regeneration from hepatic stem cells and oval cells (Alison et al, 1998; Petersen et al, 1999). This and the fact that only 5/20 sections contained donor cells, is consistent with the notion that stem cells engraft in some but not all areas of the liver, where they proliferate and differentiate into hepatocytes.
Engraftment in the intestine was also consistent with what is known about intestinal epithelial stem cells. In the gut, each crypt contains a population of 4-5 long-lived stem cells (Potten, 1998). Progeny of these stem cells undergo several rounds of division in the middle and upper portions of cypts and give rise to epithelial cells that migrate upwards, out of the crypt, onto adjacent villi. Donor derived, β-gal+panCK+CD45" epithelial cells entirely covered several villi (Fig. 40-
P). In some villi, β-gal+panCK+CD45" cells constituted only 50% of the circumference (solid arrows, Fig. 4P) suggesting engraftment in one but not both crypts. Several β-gal+panCK" cells were distinctly seen in the core of intestinal villi
(open arrow, Fig. 40). These cells co-stained for CD45 (Fig. 4P), indicating that they were donor-derived hematopoietic cells. In the lung, the majority of donor cells gave rise to β-gal+panCK+CD45" alveolar epithelial cells whereas, most hematopoietic cells were of recipient-origin (panCK"CD45+β-gal") (Fig. 4R).
Levels of engraftment detected by immunohistochemistry were concordant with levels determined by Q-PCR for NEO (Table 4). Engraftment levels were similar in animals analyzed after 4 to 24 weeks following IN. injection of MASC (Table 4). No contribution was seen to skeletal or cardiac muscle. In contrast to epithelial tissues and the hematopoietic system, little to no cell turnover is seen in skeletal or cardiac muscle in the absence of tissue injury. Therefore, one may not expect significant contribution of stem cells to these tissues. However, engraftment was not found in skin and kidney, two organs in which epithelial cells undergo rapid turnover. It is shown in the blastocyst injection experiments (Example 8) that mMASC can differentiate into these cell types; one possible explanation for the lack of engraftment in these organs in post-natal recipients is that mMASC do not home to these organs, a hypothesis that is currently being evaluated. Although mMASC differentiated into neuroectoderm-like cells ex vivo, no significant engraftment of mMASC was seen in the brain, and rare donor cells found in the brain did not co- label with neuroectodermal markers. Two recent publications demonstrated that donor derived cells with neuroectodermal characteristics can be detected in the brain of animals that underwent BM transplantation. However, a fully ablative preparative regimen prior to transplantation or transplantation in newborn animals was used, conditions associated with break-down of the blood-brain barrier. Cells were infused in non-irradiated adult animals, or animals treated with low dose radiation, where the blood-brain barrier is intact or only minimally damaged. This may explain the lack of mMASC engraftment in the CNS. Confluent MASCdo not differentiate in vivo
As control, ROSA26-MASC were infused and grown to confluence prior injection. MASC allowed to become confluent lose their ability to differentiate ex vivo in cells outside of the mesoderm, and behave like classical MSC (Reyes, M. et al. 2001). Infusion of 106 confluent mMASC did not yield significant levels of donor cell engraftment. Although few β-gal+ cells were seen in BM, these cells did not co-label with anti-CD45 Abs, indicating that MSC may engraft in tissues, but are no longer able to differentiate into tissue specific cells in response to local cues.
MASC derived cells in bone marrow of mice can be serially transferred BM from mouse engrafted with ROSA26 MASC was tested to determine whether they contained cells that would engraft in secondary recipients. 1.5x 107 BM cells, recovered from primary recipients 11 weeks after IN. infusion of mMASC, were transferred to secondary irradiated ΝOD-SCID recipients (Table 4: animal SR-1 and SR-2). After 7 and 10 weeks, secondary recipients were sacrificed, and blood, BM, spleen, liver, lung and intestines of the recipient animal were analyzed for engraftment of ROSA26 donor cells by immunohistochemistry and Q- PCR for the ΝEO gene. A similar pattern of engraftment was seen in secondary recipients as in the primary recipients. Four-8% of BM, spleen and PB cells were β- gal+CD45+; six and 8% of intestinal epithelial cells were β-gal+pan-CK+, and 4 and 5% of lung epithelial cells were β-gal+pan-CK+. Levels of engraftment in the liver of secondary recipients were lower than in the primary recipients (1 and 3% vs. 5 and 8% β-gaf CK18+). This suggests that mMASC may persist in the BM of the primary recipient and differentiate into hematopoietic cells as well as epithelial cells when transferred to a second recipient. MASC derived cells can produce insulin in vivo. MASC from ROSA26 mice were injected into irradiated ΝOD-SCID mice as described herein. The resulting MASC derived cells co-stain for LacZ and insulin in a model of streptozotocin-induced diabetes. Summary One of the critical questions in "stem cell plasticity" is whether the engrafted and differentiated donor mMASC are functional. The results described herein show that one animal developed a lymphoma in thymus and spleen after 16 weeks, as is commonly see in aging ΝOD-SCID mice (Prochazka et al, 1992). Phenotypic analysis showed that this B-cell lymphoma was host-derived: CD19+ cells were β- gal". Approximately 40% of CD45'vWF+ cells in the vasculasture of the tumor stained with anti- β-gal Abs, indicating that neoangiogenesis in the tumor was in part derived from donor mMASC (Fig. 4T). This suggests that MASC give rise to functioning progeny in vivo. Likewise, higher levels of mMASC engraftment and differentiation in radiosensitive organs, such as the hematopoietic system and intestinal epithelium (Table 4, p<0.001), following low dose irradiation suggests that mMASC may contribute functionally to host tissues.
These results showed that mammalian MASC can be purified, expanded ex vivo, and infused IN., homed to various sites in the body, engraft into numerous organs, and that the cells are alive in these various organs one month or longer. Such donor cells, undifferentiated, and differentiated progeny are found, by virtue of the fluorescent marker, in organs including, but not limited to, the BM, spleen, liver and lung. These cells can be used to repopulate one or more compartment(s) to augment or restore cell or organ function.
Example 7. Demonstration of in vitro Hematopoiesis and Erythropoiesis
MASC from, human BM differentiate at the single cell level into neuroectodermal, endodermal and many mesodermal lineages, including endothelial cells. Because endothelium and blood are very closely related in ontogeny, it can be hypothesized that MASC can differentiate into hematopoietic cells. eGFP transduced human MASC, that are GlyA, CD45 and CD34 negative (n=20), were cocultured with the mouse yolk sac mesodermal cell line, YSM5, as suspension cell aggregates for 6 days in serum free medium supplemented with 10 ng/mL bFGF and VEGF. After six days, only eGFP+ cells (i.e., MASC progeny) remained and YSM5 cells had died.
Remaining cells were transferred to methylcellulose cultures containing 10% fetal calf serum supplemented with 10 ng/mL bone morphogenic protein (BMP)4, VEGF, bFGF, stem cell factor (SCF), Flt3L, hyper IL6, thrombopoietin (TPO), and erythropoietin (EPO) for 2 weeks. In these cultures, both adherent eGFP+ cells and small, round non-adherent cells, which formed many colonies attached to the adherent cells were detected. The non- adherent and adherent fractions were collected separately and cultured in 10%FCS containing medium with 10 ng/mL VEGF and bFGF for 7 days. Adherent cells stained positive for vWF, formed vascular tubes when plated on ECM, and were able to uptake a-LDL, indicating their endothelial nature. 5-50% of the non-adherent cells stained positive for human specific GlyA and HLA-class I by flow cytometry. Gly-A+/HLA-class-I+ cells were selected by FACS. On Wright -Giemsa, these cells exhibited the characteristic morphology and staining pattern of primitive erythroblasts. Cells were benzidine+ and human Hb+ by immunoperoxidase. By RT-PCR these cells expressed human specific Hb-e, but not Hb-a.
When replated in methylcellulose assay with 20%FCS and EPO, small erythroid colonies were seen after 10 days, and 100% of these colonies stained positive for human specific GlyA and Hb. As selection of MASC depends on the depletion of CD45+ and Gly A+ cells from BM, and cultured MASC are CD45" and
GlyA" at all times examined using both FACS and cDNA array analysis, contamination of MASC with hematopoietic cells is very unlikely.
Example 8. In vivo proof of the Multipotent Nature of MASC as Shown by Multiple Organ Chimerism following Blastocyst Injections of the Cells
Important for therapeutic applications of these cells is the ability of MASC to proliferate and differentiate into the appropriate cell types in vivo. Up until this point the only cells that should be capable of contributing to the full constellation of tissues and organs in the body are ES cells. In order to analyze whether MASC could show the full capability of ES cells, they were assayed to determine their contribution to the formation of various tissues by introducing them into the early blastocyst and observing the fate of their progeny.
MASC were generated from marrow of ROS A26 mice that are transgenic for the β-galactosidase (β-gal) gene (Rafii, S., et al. 1994, Blood. 84:10-13) and expanded as described in Example 1. One or 10-12 ROSA26 MASC obtained after 55-65 PDs were microinjected into 88 and 40 3.5-day C57BL/6 blastocysts, respectively. Blastocysts (8/mother) were transferred to 16 foster mothers and mice allowed to develop and be born as shown in Table 5. Table 5: Degree of chimerism following MASC injection in blastocyst
MASC/ Litters Total # NEO positive bv O-PCR blastocyst born pups born
0% 1-10% 10-20% 20-40% >40%
10-12 4/11 22 5/22 13/22 2/22 1/22 1/22
(23%) (59%) (9%) (4.5%) (4.5%)
1 3/5 15 8/15 5/15 0/15 0/15 2/15
(53%) (33%) (0%) (0%) (13%)
Seven litters were born, in line with the birth rate seen in other studies during this period. The number of mice per litter varied between 1 and 8, for a total of 37 mice. Animals born from microinjected blastocysts were of similar size as normal animals and did not display any overt abnormalities.
After four weeks, animals were evaluated for chimerism by clipping their tails and assessing the contribution of β-gal/NEO transgene containing cells to the tails by Q-PCR for NEO. Percent chimerism was determined by comparing the number of NEO copies in test samples with that in tissue from ROSA26 mice according to manufacturer's recommendations (7700 ABI PRISM Detector Software 1.6). Chimerism could be detected in 70% of mice derived from blastocysts in which 10 to 12 MASC had been injected and 50% of mice derived from blastocysts microinjected with 1 MASC (Table 5). The degree of chimerism ranged between 0.1 % to >45%. After 6 to 20 weeks, animals were sacrificed. Some mice were frozen in liquid nitrogen and thin sections were cut as described. Whole-mouse sections were stained with X-Gal. One thousand sets of digital images covering completely each section were then assembled to create a composite image of each whole-mouse section. In a representative non-chimeric animal (by Q-PCR for NEO) derived from a blastocyst in which a single MASC was injected, no X-Gal staining was seen. In contrast, the animal was 45% chimeric by R-PCR for NEO by tail clip analysis and had contribution of a single ROS A26-derived MASC to all somatic tissues.
For other animals, multiple organs were harvested and analyzed for the presence of MASC derived cells by X-GAL staining, staining with an anti-β-gal- FITC antibody, and Q-PCR for NEO. Animals that had NEO+ cells in tail-clippings had contribution of the ROSA26-derived MASC in all tissues, including the brain, retina, lung, cardiac and skeletal muscle, liver, intestine, kidney, spleen, BM, blood, and skin as shown by X-GAL staining and staining with an anti-β-gal-FITC antibody.
Chimerism was detected by X-Gal staining and anti-β-gal staining in the animals generated from blastocysts microinjected with ROSA26 MASC. β-gal+ cells expressed markers typical for the tissue in which they had incorporated. β-gal+ cells co-stained with anti-β-gal+ FITC and anti-NF200 or GFAP and TOPRO3
(observed at 20X magnification)for NF200 and GFAP in the central nervous system and for dystrophin in the skeletal muscle. Lung tissue was stained for anti-β-gal- FITC and pan-CK in alveoli and bronchi (also TOPRO3) (observed at 20X magnification). Skeletal muscle was stained with anti-β-gal-FITC, dystrophin-PE, and TOPRO3 was observed at 20X magnification. Heart was stained with anti-β- gal-FITC and cardiac troponin-I-Cy3, TOPRO3 was observed at 20X magnification. Liver was stained with anti-β-gal-FITC and pan-CK-PE and TOPRO3 (was observed with 40X magnification and 10X magnification). Intestine was stained with anti-β-gal-FITC, pan-CK-PE, and TOPR03 was observed at 20X magnification. Kidney was stained with anti-β-gal-FITC (glomerulus, tubulus) was observed at 20X magnification. Marrow staining was observed with anti-β-gal-FITC and CD45-PE, GR1-PE and MAC1-PE. Spleen staining was observed with anti-β-gal-FITC and CD45-PE, CD3-PE and CD 19-PE. Levels of engraftment estimated by Q-PCR for NEO were concordant with those estimated by X-GAL and anti-β-gal-FITC staining. Summary
These data demonstrate for the first time that BM derived single MASC integrate into the developing mouse, giving rise to cells of various fates, and contributing to the generation of all tissues and organs of the three germ layers of the mouse. As all live animals, irrespective of the degree of chimerism, had normal functioning organs, these studies also suggest that MASC can differentiate in vivo in functional cells of the three germ layers. Whether MASC contribute to germ cells, when injected in a blastocyst or when injected postnatally, has not yet been tested.
Example 9. Origin of Endothelial Progenitors
Vasculogenesis, the in situ differentiation of primitive endothelial progenitors, termed angioblasts, into endothelial cells that aggregate into a primary capillary plexus is responsible for the development of the vascular system during embryogenesis (Hirashima et al, 1999). In contrast, angiogenesis, defined as the formation of new blood vessels by a process of sprouting from preexisting vessels, occurs both during development and in postnatal life (Holash et al, 1999; Yang et al, 2001). Until recently, it was thought that blood vessel formation in post-natal life was mediated by sprouting of endothelial cells from existing vessels. However, recent studies have suggested that endothelial "stem cells" may persist into adult life, where they contribute to the formation of new blood vessels (Peichev et al, 2000;
Lin et al, 2000; Gehling et al, 2000; Asahara et al, 1997; Shi et al, 1998), suggesting that like during development neoangiogenesis in the adult may at least in part depend on a process of vasculogenesis. Precursors for endothelial cells have been isolated from BM and peripheral blood (Peichev et al, 2000; Watt et al, 1995). The ontogeny of these endothelial progenitors is unknown.
During development, endothelial cells are derived from mesoderm. The VEGF receptor 2, Flkl, characterizes the hemangioblasts, a bipotent stem cell found in the aorto-gonad-mesonephros region (Medvinsky et al, 1996; Fong et al, 1999; Peault, 1996) and in fetal liver (Fong et al, 1999), and commitment of embryoid bodies to hemangioblasts is accompanied with expression of Flkl (Choi et al, 1998; Choi, 1998). Whether hemangioblasts persist in adult life is not known, and only HSC and endothelial progenitors have,been documented. Like hemangioblasts, endothelial progenitors express Flkl (Peichev et al, 2000) and one report suggested that HSC in post-natal life express Flkl (Ziegler et al, 1999). During embryology, commitment of the hemangioblast to the endothelial lineage is characterized by the sequential expression of VE-cadherin, CD31, and shortly afterwards CD34 (Nishikawa et al, 1998; Yamashita et al, 2000). In post-natal life, endothelial progenitors have been selected from BM and blood using Abs against AC 133, Flkl, CD34, and the H1P12 Ab (Peichev et al, 2000; Lin et al, 2000; Gehling et al, 2000). AC 133 has also been found on other cells, including NSCs (Uchida et al, 2000) and gastrointestinal epithelial cells (Corbeil et al, 2000). Upon differentiation to mature endothelium, the AC 133 receptor is quickly lost (Peichev et al, 2000; Gehling et al, 2000). Another receptor found on circulating endothelial cells is a mucin, MUC18, recognized by the H1P12 Ab (Lin et al, 2000). MUC18 is lost upon differentiation of endothelial progenitors to endothelium. CD34 is expressed on endothelial progenitors, as well as on hematopoietic progenitors
(Peichev et al, 2000; Baumhueter et al, 1994) and hepatic oval cells (Crosby et al,
2001). This antigen is also lost upon differentiation of endothelial progenitors to endothelium. Most mature endothelial cells, but microvascular endothelial cells, no longer express CD34.
It is described here for the first time, the in vitro generation of vast numbers of endothelial cells that engraft in vivo and contribute to neoangiogenesis from a
MASC. MASC can be culture expanded for >80 PDs and endothelial cells generated from MASC can be expanded for at least and additional 20 PDs. MASC may therefore be an ideal source of endothelial cells for clinical therapies. In addition, as MASC are ontogenically less mature than the "angioblast", this model should be useful to characterize endothelial commitment and differentiation. hMASC differentiate into cells with phenotypic characteristics of endothelium
MASC were obtained and cultured as described in Example 3. To induce endothelial differentiation, MASC were replated at 2xl04 cells/cm2 in FN-coated wells in serum-free expansion medium without EGF and PDGF-BB but with 10 ng/mL VEGF. In some instances, FCS was added. Cultures were maintained by media exchange every 4-5 days. In some instances, cells were subcultured after day 9 at a 1 :4 dilution under the same culture conditions for 20+ PDs. In order to define endothelial differentiation from MASC more extensively,
FACS and immunohistochemical analysis of cells after 3-18 days was performed. Expression of Flkl and Fltl on undifferentiated MASC was low, was maximal at day 9, and persisted until day 18. VE-cadherin, present on BM or blood endothelial progenitors (Peichev et al, 2000; Nishikawa et al, 1998), was not expressed on undifferentiated MASC, but was expressed after 3 days of culture with VEGF and persisted until day 18. MASC expressed low levels of AC133, found on endothelial as well as hematopoietic progenitors (Peichev et al, 2000; Gehling et al, 2000) but was no longer detectable after day 3. CD34, present on endothelial and hematopoietic progenitors (Peichev et al, 2000; Asahara et al, 1997; Rafii et al, 1994), was not present on undifferentiated MASC (Fig. 4A) but was expressed from day 9 until day 18. The mucin, MUC18, recognized by the Ab H1P12 has been used to purify endothelial progenitors from blood (Lin et al, 2000). Although MASC did not stain with H1P12 MASC treated with VEGF for 9 days stained positive, but expression was lost by day 18.
The endothelium specific integrin, αvβ3, (Eliceiri et al, 2000) was not present on undifferentiated MASC, whereas αvβ5 was expressed at very low levels. Expression of integrins increased progressively during differentiation and was maximal by day 14 (Fig. 5). The tyrosine kinase receptors, Tie and Tek, important for angiogenesis but not endothelial cell differentiation (Partanen et al, 1999), were not expressed on MASC. Expression of Tek could be seen after day 3 and Tie after day 7 (Fig. 6). MASC also do not express vWF, but vWF was expressed from day 9 on (Rosenberg et al, 1998; Wagner et al, 1982). More mature endothelial markers, including CD31, CD36, CD62-P (Tedder et al, 1995) (Fig. 7), and the adhesion junction proteins ZO-1, β-catenin, and γ-catenin (Fig. 5) were detected after day 14 (Li et al, 1990; Van Rijen et al, 1997; Petzelbauer et al, 2000). VCAM or CD62- E were not expressed at high level at any time point during differentiation, unless endothelium was activated with IL-lα, as described below. Differentiation to endothelium was associated with acquisition of β2-microglobulin and low levels of HLA-class I antigens, but not HLA-class II.
It has been reported previously, that endothelial differentiation can only be obtained from MASC expanded with 2% FCS or less, but not when expanded with 10% FCS (Reyes et al, 2001) as higher concentrations of FCS supports growth of classical MSC that differentiate only into osteoblasts, chondroblasts and adipocytes (Reyes et al, 2001 ; Pittenger et al, 1999). When FCS was present during the initial 7 days of differentiation, endothelial differentiation could not be induced. When non-confluent MASC (<lxl04 cells/cm2) were induced to differentiate, endothelial was not seen. When MASC were subcultured 9-days after exposure to VEGF using serum free medium with 10 ng/mL VEGF, cells could undergo at least an additional 12 PDs. When 10% FCS and 10 ng/mL VEGF was added to the medium for subculturing, MASC-derived endothelial cells could undergo an additional 20+ PDs, irrespective of the number of PDs that MASC had undergone. Compared with undifferentiated MASC, endothelial cells were larger, and had a lower nuclear/cytoplasm ratio. Results were similar when MASC were used from cultures that had undergone 20 (n=30) or 50+ (n=25) PDs. Functional characteristics of MASC-derived endothelium
It was tested whether VEGF-induced differentiated progeny of hMASC had functional characteristics of endothelial cells. Endothelial cells respond to hypoxia by upregulating expression of VEGF as well as the VEGF receptors Flkl and the angiogenesis receptors, Tie-1 and Tek (Kourembanas et al, 1998). hMASC and hMASC-derived endothelial cells were incubated at 37°C in 20% or 10% O2 for
24h. Cells were stained with Abs against Flkl, Fltl, Tek and IgG control, fixed in
2% paraformaldehyde and analyzed by flow cytometry. In addition, VEGF concentrations in the culture supematants was measured using an ELISA kit (AP biotech, Piscataway, NJ). MASC-derived endothelial cells and undifferentiated MASC were exposed to hypoxic conditions for 24h.
Expression of Flkl and Tek was significantly increased on MASC-derived endothelial cells exposed to hypoxia (Fig. 7), while the levels of these receptors remained unchanged on undifferentiated MASC. In addition, levels of VEGF in culture supematants of hypoxic endothelial cultures was increased by 4 fold (Fig. 7B) whereas VEGF levels in MASC cultures exposed to hypoxia remained unchanged.
It was next tested whether MASC-derived endothelial cells would upregulate expression of HLA-antigens and cell adhesion ligands in response to inflammatory cytokines, such as IL-lα (Meager, 1999; Steeber et al, 2001). 106MASC and MASC-derived endothelial cells were incubated with 75 ng/ml IL-lα (R&D Systems) in serum-free medium for 24h. Cells were fixed in 2% paraformaldehyde and stained with Abs against HLA-class I, class II, β2-microglobulin, vWF, CD31 , VCAM, CD62E and CD62P, or control Abs, and analyzed using a FACScalibur (Becton Dickinson).
Significantly increased levels of HLA-Class I and II, β2-microglobulin, VCAM, ECAM, CD62E, CD62P were seen by FACS analysis (Fig. 7C) on endothelial cells. In contrast, on undifferentiated MASC only upregulation of Flk was seen. Another characteristic of endothelial cells is that they take up LDL
(Steinberg et al, 1985). This was tested by incubating MASC induced to differentiate with VEGF for 2, 3, 5, 7, 9, 12 and 15 and 21 with LDL-dil-acil. The dil-Ac-LDL staining kit was purchased from Biomedical Technologies (Stoughton, MA). The assay was performed as per manufacture's recommendations. Cells were co-labeled either with anti-Tek, -Tie-1 or -vWF Abs. After 3 days, expression of
Tek was detected but no uptake of a-LDL. After 7 days, cells expressed Tie-1, but did not take up significant amounts of a-LDL. However, acquisition of expression of vWF on day 9 was associated with uptake of aLDL (Fig. 6B).
Endothelial cells contain vWF stored in Weibel Pallade bodies that is released in vivo when endothelium is activated (Wagner et al, 1982). This can be induced in vitro by stimulating cells with histamine (Rosenberg et al, 1998), which also results in activation of the cell cytoskeleton (Vischer et al, 2000). MASC- derived endothelial cells were plated at high confluency (104 cells/cm2) in FN-coated chamber slides. After 24h, cells were treated with 10 μM histamine (Sigma) in serum free medium for 25 min. and stained with Abs against vWF and myosin. Untreated and treated cells were fixed with methanol at -20°C for 2 min, stained with Abs against vWF and myosin, and analyzed using fluorescence and/or confocal microscopy. vWF was present throughout the cytoplasm of untreated endothelial cells. Cytoplasm of endothelial cells treated with histamine contained significantly less vWF and vWF was only detectable in the perinuclear region, likely representing vWF present in the endoplasmic reticulum (Fig. 6A). Histamine treatment caused widening of gap junctions and cytoskeletal changes with increased numbers of myosin stress fibers (Fig. 6A).
Finally, endothelial cells were tested to determine if they could form "vascular tubes" when plated on Matrigel™ or extracellular matrix (ECM) (Haralabopoulos et al, 1997). 0.5 ml extracellular matrix (Sigma) was added per well of a 24 well plate, incubated for 3h at 37°C. 104 MASC and MASC-derived endothelial cells were added per well in 0.5 ml of serum free plus VEGF medium and incubated at 37°C. As shown in Fig. 6C, culture of MASC derived endothelial cells on ECM resulted in vascular tube formation within 6 hours. hMASC-derived endothelial cells contribute to tumor-angiogenesis in vivo
A breeding colony of NOD-SCID mice was established from mice obtained from the Jackson Laboratories (Bar Harbor, ME). Mice were kept in specific pathogen free conditions and maintained on acidified water and autoclaved food. Trimethoprim 60 mg and sulphamethoxazole 300 mg (Hoffmann-La Roche Inc., Nutley, NJ) per 100 ml water was given twice weekly. Three Lewis lung carcinoma spheroids were implanted subcutaneously in the shoulder. 3 and 5 days after implantation of the tumor, mice were injected with
0.25x10° human MASC-derived endothelial cells or human foreskin fibroblasts via tail vein injection. After 14 days, animals were sacrificed, tumors removed and cryopreserved using OTC compound (Santura Finetek USA Inc, Torrance, CA) at -
80°C. In addition, the ears that were clipped to tag the mouse were also removed and cryopreserved using OTC compound at -80°C. Five μm thick sections of the tissues were mounted on glass slides and were fixed and stained as described below.
Computer-aided analysis of length and number of branches counted on five sections of each tumor showed that tumors in mice that received human MASC- derived endothelial cells had a 1.45+0.04 fold greater vascular mass than tumors in control mice that did with anti-human-β2-microglobulin or HLA-Class I Abs, combined with anti-mouse-anti-CD31 Abs and anti-vWF, anti-Tek or anti-Tie- 1 Abs, which recognize both human and mouse endothelial cells. These initial studies showed that some blood vessels in the tumor contained anti-human-β2- microglobulin or HLA-Class I positive cells that co-labeled for either vWF, Tie or Tek, but not with mouse-CD31 , indicating that human MASC-derived endothelial cells contributed to tumor neoangiogenesis in vivo.
To better address the degree of contribution, 35 sequential 5 μm slides were obtained and were stained in an alternate fashion with either anti-human β2- microglobulin-FITC or anti-mouse-CD31 -Cy5 and anti-vWF-Cy3. All slides were examined by confocal microscopy. The different figures were then assembled in 3- D to determine the relative contribution of human and murine endothelial cells to the tumor vessels. When tumors obtained from animals injected with human-MASC derived endothelial cells were analyzed approximately 35% of the tumor vessels were positive for anti-human β2-microglobulin as well as vWF whereas approximately 40% of endothelial cells stained positive with anti-mouse CD31 Abs (Fig. 8A-G). Tumors in animals that did not receive endothelial cells or received human fibroblasts did not contain endothelial cells that stained positive with the anti-β2-microglobulin or anti-HLA-class-I Abs Abs.
MASC-derived endothelial cells were also analyzed whether they contribute to wound healing angiogenesis. The area of the ear that had been clipped to tag the mouse was then examined. Neoangiogenesis in the ear wounds was in part derived from the MASC derived endothelial cells. Similar to blood vessels in the tumor the percent human endothelial cells present in the healed skin wound was 30-45% (Fig.
9H).
Undifferentiated hMASC differentiate in endothelial cells in vivo 106 undifferentiated MASC were injected IN. in 6-week old ΝOD-SCID mice. Animals were maintained for 12 weeks and then sacrificed. In one animal, a thymic tumor was detected, which is commonly seen in aging ΝOD-SCID mice
(Prochazka et al, 1992).. The thymus was removed and cryopreserved in OTC compound at -80°C. Ten μm thick sections of the tissues were mounted on glass slides and were fixed and stained as described below.
All hematopoietic cells stained positive for mouse CD45 but not human CD45, indicating that they were murine in origin. The tumor was then stained with an anti-human β2-microglobulin-FITC Ab and an anti-vWF-Cy3 Ab that recognizes both human and mouse endothelial cells. Approximately 12% of the vasculature was derived from hMASC (Fig. 91). These studies further confirmed that the hematopoietic elements were not of human origin, as no human β2-microglobulin was detected outside of the vascular structures. Immunohistochemistry and Data Analysis
In vitro cultures: Undifferentiated MASC or MASC induced to differentiate to endothelium for 2-18 days, plated in FΝ coated chamber slides were fixed with 2% paraformaldehyde (Sigma) for 4 min at room temperature. For cytoskeleton staining chamber slides were fixed with methanol for 2 min at -20°C. For intracellular ligands, cells were permeabilized with 0.1 Triton-X (Sigma) for lOmin and incubated sequentially for 30h in each with primary antibody (Ab), and FITC, PE or Cy5 coupled anti-mouse-, goat- or rabbit-IgG Ab. Between each step, slides were washed with PBS+1%BSA. Primary Abs against CD31, CD34, CD36, CD44, HLA-class I and -II,β2-microglobulin were used at a 1 :50 dilution. Primary Abs against NCAM, ICAM, VE-cadherin, selectins, HIP 12, ZO-1, connexin-40, connexin-43, MUC18, avb3, avb5, B-catenin and γ-catenin (Chemicon) and Tek, Tie, vWF (Santa Cruz) were used at a 1 :50 dilution. Stress fibers were stained with Abs against myosin (light chain 20kD, clone no. MY-21 ; 1 :200). Secondary Abs were purchased from Sigma and used at the following dilutions: anti-goat IgG-Cy-3 (1 :40), anti-goat IgG-FITC (1 :160), anti-mouse IgG-Cy-3 (1 :150) and anti-mouse IgG-FITC (1 :320), anti-rabbit-FITC (1 : 160) and anti-rabbit-Cy-3 (1 :30). TOPRO-3 was purchased from Sigma. Cells were examined by fluorescence microscopy using a Zeiss Axiovert scope (Carl Zeiss, Inc., Thomwood, NY) as well as by confocal fluorescence microscopy using a Confocal 1024 microscope (Olympus AX70, Olympus Optical Co. LTD, Japan).
Tumors or normal tissue: The tissue was sliced using a cryostat in 5-10 μm thick slices. Slices were fixed with acetone for 10 min at room temperature and permeabilized with 0.1 Triton X for 5 min. Slides were incubated overnight for vWF, Tie or Tek, followed by secondary incubation with FITC, PE or Cy5 coupled anti-mouse-, goat- or rabbit-IgG Abs and sequential incubation with Abs against mouse CD45-PE or human CD45-FITC, human β2-microglobulin-FITC, mouse CD31 -FITC or TOPRO-3 for 60min. Between each step, slides were washed with PBS + 1% BSA. Slides were examined by fluorescence microscopy using a Zeiss Axiovert scope as well as by confocal fluorescence microscopy using a Confocal 1024 microscope. 3D-reconstruction consisted of the collection of sequential 0.5 μm confocal photos from 35 slides of 5μm thick to a total of 350 photos. Slides were stained with vWF-Cy3 and alternately double stained with humanβ2- microglobulin-FITC or mouse CD31-FITC. The photos from each slide were aligned with the next slide in Metamorph software (Universal Imaging Corp) and the 3D reconstruction was made in 3D Doctor Software (Able software Corp).
Volume of relative contribution of human (green) and murine endothelial cells (false colored as blue) to the 3D vessel was calculated as cubic pixels of each color. The area of each color was also calculated as square pixels in 4 vessels through the 35 slides to obtain an accurate percentage of contribution. The area of each color was also calculated in alternate slides of four different tumors. Summary
The central finding of this study is that cells that co-purify with MSC from BM have the ability to differentiate to endothelial cells that have in vitro functional characteristics indistinguishable from mature endothelial cells. It is also showv that such endothelial cells contribute to neoangiogenesis in vivo in the setting of wound healing and tumorigenesis, and that undifferentiated MASC can respond to local cues in vivo to differentiate into endothelial cells contributing to tumor angiogenesis. As the same cell that differentiates to endothelium also differentiates to other mesodermal cell types, as well as cells of non-mesodermal origin, the cell defined here precedes the angioblast, and even the hemangioblast in ontogeny.
It has also been shown that MASC differentiate into cells that express markers of endothelial cells, but proved that VEGF induced MASC function like endothelial cells. Endothelial cells modify lipoproteins during transport in the artery wall (Adams et al, 2000). Endothelial cells maintain a permeability barrier through intercellular junctions that widen when exposed to hemodynamic forces or vasoactive agents, such as histamine (Rosenberg et al, 1998; Li et al, 1990; Van
Rijen et al, 1997; Vischer et al, 2000). Endothelial cells release prothrombotic molecules such as vWF, tissue factor, and plasminogen activator inhibitor to prevent bleeding (Vischer et al, 2000), and regulate egress of leukocytes by changing expression levels of adhesion molecules in response to inflammation (Meager, 1999; Steeber et al, 2001). Endothelium also reacts to hypoxia by producing VEGF and expressing VEGF receptor aimed at increasing vascular density (Kourembanas et al, 1998). Therefore it has been demonstrated that endothelial cells generated from MASC can perform all of these tasks when tested in vitro.
Finally it has been proved that in vitro generated MASC-derived endothelial cells respond to angiogenic stimuli by migrating to the tumor site and contributing to tumor vascularization as well as wound healing in vivo. This finding confirms that endothelial cells generated from MASC have all the functional characteristics of mature endothelium. The degree of contribution of endothelial cells to tumor angiogenesis and neo-angiogenesis was 35-45%, levels similar to what has been described for other sources of endothelial cells (Conway et al, 2001; Ribatti et al, 2001). In addition, it has been found that angiogenic stimuli in vivo provided in a tumor microenvironment are sufficient to recruit MASC to the tumor bed and induce their differentiation into endothelial cells that contribute to the tumor vasculature. These studies therefore extend studies reported by other groups demonstrating that cells present in marrow can contribute to new blood vessel formation (Peichev et al, 2000; Lin et al, 2000; Gehling et al, 2000; Asahara et al, 1997), in a process similar to vasculogenesis, precursor responsible for this process has been identified the. This is to our knowledge the first report that identifies a cell present in postnatal BM as a very early progenitor for endothelial cells. Example 10. Derivation of Neurons
Single adult BM-derived hMASC or mMASC were tested to determine whether they can differentiate ex vivo to functional neurons, as well astrocytes and oligodendrocytes aside from mesodermal cell types. mMASC and hMASC were selected and culture expanded as previously described in Examples 1 and 3, respectively. Human neural progenitor cells (hNPC) were purchased from Clonetics (San Diego, CA). hNPC were cultured and differentiated per manufactures' recommendations .
Electrophysiology: Standard whole-cell patch-clamp recording was used to examine the physiological properties of MASC-derived neurons. Voltage-clamp and current-clamp recordings were obtained using a Dagan 3900 A patch-clamp amplifier (Dagan Corporation, Minneapolis) which was retrofitted with a Dagan 3911 expander unit. Patch pipettes, made from borosilicate glass, were pulled on a Narishige pipette puller (model PP-83), and polished using a Narishige microforge (model MF-83). Patch pipettes were filled with an intracellular saline consisting of (in mM) 142.0 KF, 7.0 Na2S04, 3.0 MgS04, 1.0 CaCl2, 5.0 HEPES, 11.0 EGTA, 1.0 glutathione, 2.0 glucose, 1.0 ATP (magnesium salt), 0.5 GTP (sodium salt). For most recordings, the fluorescent dye 5,6-carboxyfluorescein (0.5 mm; Eastman Kodak Chemicals) was also added to the pipette solution to confirm visually, using fluorescence microscopy, that the whole-cell patch recording configuration had been achieved. Pipette resistances ranged from 11 to 24 Mohm. The standard extracellular recording saline was comprised of the following (in mM): 155 NaCl, 5.0 KC1, CaCl2, 1.0 MgCl2, 10 HEPES, 5 glucose. For some experiments 1 μM TTX was added to the standard control solution. The pH of the intracellular and extracellular recording solutions was adjusted to 7.4 and 7.8, respectively, using NaOH. All chemicals were from Sigma. PClamp 8.0 (Axon Instruments, Foster City) was used to run experiments, and to collect and store data. The data presented were corrected for a 8.4 mV liquid junctional potential, which was calculated using the JPCALC software package. Off-line analyses and graphical representations of the data were constructed using Clampfit 8.0 (Axon Instruments, Foster City) and Prism (Graphpad, San Diego).
Transduction: Retroviral supernatant was produced by incubating MFG- eGFP-containing PG13 cells, provided by Dr. G.Wagemaker, U. of Rotterdam, Netherlands (Bierhuizen et al, 1997), with MASC expansion medium for 48h, filtered and frozen at -80°C. MASC were incubated with retroviral supematants and
8 μg/ml protamine (Sigma) for 6h. This was repeated 24h later. Transduction efficiency was analyzed by FACS. Gene microarrav analysis: RNA was isolated from hMASC, bFGF or FGF-
8b+EGF induced cells using the RNeasy mini kit (Qiagene), digested with DNase I
(Promega) at 37°C for lh and re-purified using the RNeasy. The [32P] dATP labeled cDNA probe, generated according to the manufacturers recommendations, was hybridzed to the Human Neurobiology Atlas Array (Clonetech # 7736-1, Clonetech Laboratories, Palo Alto, CA, USA) at 68°C for 18-20h, followed by 4 washes in 2x SSC, 1% SDS at 68°C for 30min each time, O.lx SSC, 0.5% SDS at 68°C for 30 min, and once in 2x SSC at room temperature for 5 min. The arrays were read by a phosphorimager screen scanner (Molecular Dynamics, Storm 860) and analyzed using Atlas Image 1.0 (Clontech). Differences between undifferentiated and differentiated cells greater than 2-fold were considered significant.
PCR analysis for retroviral insert: PCR was used o amplify the flanking sequence 3' from the 3' LTR of the MFG vector in the human genomic DNA. DNA from 106 MASC or endothelial, myoblast or neuroectodermal differentiated progeny was prepared from cells by standard methods. 300 ng of genomic DNA was digested with Ascl and a splinkerette linker was ligated to the 5' end (Devon R. S. et al, 1995). The two oligonucleotides used for the splinkerette linker were as follows: aattTAGCGGCCGCTTGAATTtttttttgcaaaaa, (the hairpin loop forming sequence is in lower case and the upper case is the reverse complement of the second splinkerette oligo), and agtgtgagtcacagtagtctc gc gttc gAATTAAGCGGCCGCTA, (the underlined sequence is also the sequence of the linker-specific primer (LS Primer) used for the PCR and RT steps). A 5'-biotin-T7 coupled primer was used that recognizes a sequence in the eGFP gene [Biotin-ggc- cag-tga-att-gta-ata-cga-ctc-act-ata-ggc-tgg-CAC-ATG-GTC-CTG-CTG-GAG-TTC- GTG-AC; underlined portion shows the minimum promoter sequence needed for efficient in vitro transcription and the upper case is the eGFP specific sequence] and LS primer to amplify the flanking regions for 10 rounds using Advantage 2 polymerase (Clontech). The biotin labeled amplified product was captured using streptavidin-magnetic beads (Streptavidin Magnetic Particles; Roche) and the resultant product was further amplified using the T7 RNA polymerase an approximately 1 ,000 fold and then DNAase 1 treated. The resultant product was reverse transcribed using the agtgtgagtcacagtagtctcgcgttc splinkerette primer according to the superscript II protocol (Gibco), and subsequently amplified by 30 rounds of nested PCR using the primer for the 3 'LTR [ggc caa gaa cag atg gaa cag ctg aat atg]. The flanking sequence in the human genome from endothelium, muscle, and neuroectodermal differentiated cells and undifferentiated MASC was sequenced.
To demonstrate that the same insertion site was present in multiple differentiated progeny, specific primers were generated in the host-flanking genome. Real time PCR amplification (ABI PRISM 7700, Perkin Elmer/Applied Biosystems) was used to quantitate the flanking sequence compared to the eGFP sequence. Reaction conditions for amplification were as follows: 40 cycles of a two step PCR (95°C for 15 sec, 60°C for 60 sec) after initial denaturation (95°C for 10 min.) with 2 μl of DNA solution, IX TaqMan SYBR GreenUniversal Mix (Perkin Elmer/ Applied Biosystems) PCR reaction buffer. Primers used were as follows: Clone A16: LTR primer = CCA-ATA-AAC-CCT-CTT-GCA-GTT-G; Flanking sequence chromosome 7 = TCC-TGC-CAC-CAG-AAA-TAA-CC; Clone A 12 chromosome 7 sequence: LTR primer = GGA-GGG-TCT-CCT-CTG-AGT-GAT-T, Flanking sequence = CAG-TGG-CCA-GAT-CTC-ATC-TCA-C; Clone A12 chromosome 1 sequence: LTR = GGA-GGG-TCT-CCT-CTG-AGT-GAT-T; Flanking sequence = GCA-GAC-GAG-GTA-GGC-ACT-TG. The relative amount of the flanking sequence was calculated in comparison with eGFP sequence according to manufacturer's recommendations using the 7700 ABI PRISM Detector Software 1.6. Neural transplantation: Newborn (P1-P3) male Sprague Dawley rats (Charles
River Laboratories) were used in this study. The rats were anaesthetized by cryoanesthesia. The cranium was immobilized using a modified stereotaxic head holder and the scalp reflected to expose the skull. hMASC were harvested with 0.25% trypsin/EDTA, washed twice, and resuspended in PBS. The viability of the hMASC was more than 85%. A 2 μl volume of hMASC suspended in phosphate buffered saline at a concentration of 0.7x104 cells/μl was stereotaxically injected intracerebroventricularly with a tapered glass micropipette attached to a Hamilton syringe using the following coordinates (mm from bregma): AP -0.6, ML 0.8, DV 2.1, toothbar was set at -1. Following the injections, the scalp was sutured and the pups allowed to recover.
Four and 12 weeks after transplantation, the rats were anaesthetized with chloral hydrate (350mg/kg, i.p.), decapitated the brains removed, frozen in powered dry ice, and stored at -80°C. Fresh frozen brains were sectioned using a cryostat and fixed with 4% paraformaldehyde for 20 min immediately before staining. Sections were incubated for one hour at room temperature with blocking/permeabilization solution consisting of 2% normal donkey serum (Jackson Immuno Labs) and 0.3% triton X. Primary and secondary antibodies were diluted in the same blocking/permeabilization solution for subsequent steps. Primary antibodies (mouse anti human nuclei (1 :25), anti human nuclear membrane (1 :25) and anti NeuN (1 :200) from Chemicon; rabbit anti GFAP (1 :250) from DAKO, rabbit anti NF200 (1 :300) from Sigma were incubated overnight at 4°C, rinsed 3x10 minutes each in PBS and followed by secondary Cy3 (1 :200) anti and FITC (1 :100) antibodies (all from Jackson Immuno Labs) for two hours at room temperature. Slides were examined by fluorescence microscopy using a Zeiss Axiovert scope as well as by confocal fluorescence microscopy using a Confocal 1024 microscope. hMASC acquire a neuron, astrocyte and oligodendrocyte phenotype when cultured with bFGF. Neuroectodermal differentiation was done as described in Example 5.
Briefly, cells were cultured in FN-coated chamberslides or culture plates with serum-free medium consisting of 60% DMEM-LG, 40% MCDB-201 (Sigma Chemical Co, St Louis, MO), supplemented with IX ITS, IX LA-BSA, 10'8 M dexamethasone, lO^ M ascorbic acid 2-phosphate (AA) (all from Sigma), 100 U penicillin and 1,000 U streptomycin (Gibco). In some cultures, we added lOOng/mL bFGF whereas in other cultures 10 ng/mL EGF + 10 ng/mL FGF-8b were added (all from R&D Systems). Cells were not subcultured, but media was exchanged every 3-5 days.
Two weeks after re-plating with bFGF, 26+4% of cells expressed astrocyte (GFAP+), 28+3% oligodendrocyte (MBP+) and 46+5% neuron (NF200+) markers as shown in Table 6. Table 6: Differentiation markers on bFGF and FGF-8b induced hMSC
Figure imgf000058_0001
When hMASC were replated at higher cell densities (2xl04 cells/cm2) to induce differentiation, no cells with neuroectodermal phenotype could be detected, suggesting that cell-cell interactions prevent bFGF-induced neuroectodermal differentiation.
The distribution of astrocyte-, oligodendrocyte- and neuron-like cells did not differ when differentiation was induced with hMASC that had undergone 20 or 60 PDs. However, when hMASC expanded for 20 PDs were cultured with bFGF, >50% of cells died while >70% of hMASC culture expanded for >30 PDs survived and acquired a neuron-, astrocyte- or oligodendrocyte-like phenotype. This suggests that not all hMASC can be induced to acquire neural characteristics but that a subpopulation of hMASC that survives long-term in vitro may be responsible for neuronal differentiation. It has been shown that the karyotype of hMASC is normal irrespective of culture duration (Reyes et al, 2001). Differentiation of hMASC into neuroectodermal-like cells is therefore not likely due to transformation of MASC following long-term culture.
Most astrocyte- and oligodendrocyte-like cells died after 3 weeks. Progressive maturation of neuron-like cells was seen throughout culture. After 1 week, bFGF treated hMASC stained positive for NeuroD, Nestin, polysialated neural cell adhesion molecule (PSA-NCAM), and tubulin-β-III (TuJI) (Table 6).
After 2 weeks, bFGF treated cells stained positive for NF68, -160, and -200, NSE, MAP2-AB, and Tau. bFGF-induced neurons did not express markers of GABAergic, serotonergic or dopaminergic neurons, but expressed glutamate as well as the glutamate-receptors-5, -6 and -7 and N-methyl-D-aspartate (NMDA)-receptor, and Na+-gated voltage channels.
Further confirmation of neuroectodermal differentiation was obtained from cDNA array analysis of two independent hMASC populations induced to differentiate for 14 days with 100 ng/mL bFGF. Expression levels of nestin, otx 1 and otx2Consistent with the immunohistochemical characterization, a >2 fold increase in mRNA for nestin was detected, GFAP, glutamate-receptors 4, 5, and 6, and glutamate, and several sodium-gated voltage channels, but did not detect increases in TH or TrH mRNA levels. A >2 fold increase in mRNA levels was also found for mammalian achaete-scute homolog 1 (MASH I) mRNA, a transcription factor found only in brain (Franco Del Amo et al, 1993) and ephrin-A5 mRNA
(O'Leary and Wilkinson, 1999). The astrocyte specific markers GFAP and S100A5, and oligodendrocyte specific markers, myelin-oligodendrocyte glycoprotein precursor and myelin protein zero (PMZ), as well as Huntingtin, and major prion protein precursor mRNA were expressed >2-fold higher after exposure to bFGF. A greater than 2 fold increase was also seen for several glycine receptors, GAB A- receptors, the hydroxytryptophan receptor-A and neuronal acetylcholine receptor, glycine transporter proteins, synaptobrevin and synaptosomal-associated protein (SNAP)25. Finally, bFGF induced expression of BDNF and glia-derived neurotrophic factor (GDNF). Like hMASC. mMASC acquire a neuron, astrocyte and oligodendrocyte phenotype when cultured with bFGF.
MASC derived from other species was tested to determine whether similar results could be obtained. mMASC expanded for 40-90 PDs were replated at 104 cells/cm in conditions identical to those used for hMASC. After 14 days, mMASC acquired morphologic and phenotypic characteristics of astrocytes (GFAP+), oligodendrocytes (MBP+) and neurons (NF-200+, NSE+ and Tau). NF200 and GFAP or MBP were never found in the same cell. In contrast to undifferentiated mMASC, mMASC treated with bFGF were significantly larger and extended processes for >40 μm.
To determine whether neuron-like cells had functional characteristics of neurons, and if bFGF-induced cells showed evidence of voltage-gated Na+ currents a patch clamp was used. No sodium currents or fast spiking behavior was seen in any of the mMASC derived neuron-like cells (n=59), even though some . cells expressed calcium currents, and in 4 cells there was evidence of spiking behavior mediated by calcium currents. Thus, bFGF induced cells did not have functional voltage-gated
Na+ currents, despite expression of sodium-gated voltage channel mRNA and protein. hMASC acquire a midbrain dopaminergic, serotonergic and GABAergic phenotype when cultured with EGF and FGF-8b.
FGF-8b, expressed at the mid-hindbrain boundary and by the rostral forebrain, induces differentiation of dopaminergic neurons in midbrain and forebrain and serotonergic neurons in the hindbrain (Ye et al, 1998). In vitro, FGF-8b has been used to induce dopaminergic and serotonergic neurons from murine ES cells (Lee et al, 2000). hMASC (n=8), expanded = for 20 to 60 PDs, were replated at 2x104 cells/cm2 on FN in serum free medium with ITS and AA and with 10 ng/mL FGF-8b and lOng/mL EGF. More than 80% of cells survived for 3 weeks. FGF-8b and EGF induced differentiation into cells staining positive for neuronal markers (Table 6) (day 7: PSA-NCAM, Nestin and TuJl; day 14: NF-68, NF-160, NF-200; and day 21 : MAP2-AB, NSE, Tau, and Na+-gated voltage channels) but not oligodendrocytes and astrocytes. In contrast to our observation for bFGF induced differentiation, cells plated at 104 cells/cm2 with EGF and FGF-8b did not lead to differentiation. After 2-3 weeks, cells had characteristics of GABAergic (GAB A+, parvalbumin+), dopaminergic (TH+, DCC+, and DTP+) and serotonergic (TrH+ and serotonin"1") neurons (Table 6). Cells also expressed the GABA-A-receptor and glutamate receptors. Cells with a dopaminergic phenotype also stained positive with Abs against the nuclear transcription factor, Nurrl, expressed only in midbrain dopaminergic neurons (Saucedo-Cardenas et al, 1998) as well as the proto- oncogene cRet, a membrane-associated receptor protein tyrosine kinase, which is a component of the glial cell line-derived neurotrophic factor (GDNF) receptor complex expressed on dopaminergic neurons (Trupp et al, 1996). This suggests that FGF-8b induces a phenotype consistent with midbrain dopaminergic neurons.
Again, results from immunohistochemical studies were confirmed by cDNA array analysis on hMASC induced to differentiate for 14 days with FGF-8b+EGF. Consistent with the immunohistochemical characterization, a >2 fold increase in mRNA for TH, TrH, glutamate, several glutamate-receptors, and sodium-gated voltage channels was detected. As parvalbumin and GABA are not present on the array, their expression could not be confirmed by mRNA analysis. Consistent with the almost exclusive neural differentiation seen by immunhistochemnistry, there was no increase in expression of GFAP, S 100 A5 mRNA nor mRNA for the oligodendrocyte specific marker, PMZ. FGF-8b+EGF induced cells expressed >2 fold more tyrosine kinase receptor (Trk)A, BDNF and GDNF, several glycine-, GABA-and hydroxytryptamine-receptors, and. several synaptic proteins. Coculture with the glioblastoma cell line U87 enhances neuron maturation. Irrespective of the culture conditions used, hMASC-derived neurons did not survive more than 3-4 weeks in culture. As neither culture contained glial cells after 3 weeks, it is possible that neuronal cells that express both glutamate and glutamate- receptors died due to glutamate toxicity (Anderson and Swanson, 2000). Alternatively, factors required for neural cell survival, differentiation and maturation provided by glial cells might not be present in the cultures (Blondel et al, 2000;
Daadi and Weiss, 1999; Wagner et al, 1999). To test this hypothesis, cells from 3- week old FGF-8b+EGF cultures were cocultured with the glioblastoma cell line, U- 87, in serum-free medium supplemented with FGF-8b+EGF for an additional 2 weeks. The glioma cell line, U-87, [American Tissue Cell Collection (Rockville,
MD)] was maintained in DMEM+10% FCS (Hyclone Laboratories, Logan, UT). Cells from 3 -week old FGF-8b+EGF containing cultures were labeled with the lipophylic dye, PKH26 (Sigma), as per manufacturer's recommendations. Labeled cells were replated in FN coated chamber slides in FGF-8b+EGF containing serum free medium together with 1,000 U-87 cells and maintained an additional 2-3 weeks with media changes every 3-5 days. To assure that PKH26 present in MASC- derived cells did not transfer to the U-87 cell line, U-87 cells were cultured in BSA- containing medium and 20 μl PKH26 dye for 7 days. No labeling of glioma cells was detected.
Under these serum-free conditions, U-87 cells ceased to proliferate but survived. hMASC derived neurons were labeled with the membrane dye, PKH26, prior to coculture with U-87 cells to allow us to identify the hMASC-derived cells by fluorescence microscopy. FGF-8b+EGF induced neurons cocultured after 3 weeks with U-87 cells and the same cytokines survived for at least 2 additional weeks. Neurons acquired a more mature morphology with increased cell size as well increased number, length and complexity of the neurites. The electrophysiological characteristics of PKH26 labeled neural cells derived from hMASC after coculture with U-87 cells by whole-cell current clamp and voltage-clamp after current-injection was evaluated (Fig. 9B). Current-clamp demonstrated spiking behavior in response to injected current in 4/8 of PKH26 labeled hMASC-derived cells present in FGF-8b+EGF/U-87 cultures. The resting membrane potential of spiking and non-spiking cells was -64.9+5.5mV and -
29.7±12.4mV, respectively. For each cell studied, input resistance of spiking and . non-spiking cells was 194.3 (37.3) and 216.3 (52.5) Mohm, respectively. An example of one of the cells in which w observed spiking behavior is shown in Fig. 9B. The top panel shows a family of voltage traces which was elicited from a spiking cell under control conditions. A DC current was first injected in the cell to hold them in the range of -100 to -120 mV. A current injection protocol, as shown in the middle panel, was then used to drive the membrane potential to different levels. As shown in this example, depolarizing current steps that were sufficiently large to bring the cell to threshold for action potential, evoked a single spike. The lower panel shows that the spiking behavior of the cells could be blocked by 1 μM TTX, suggesting that the action potentials are mediated by Na-gated voltage channels. Leak-subtracted current records, obtained in voltage-clamp mode from the same cells (Fig. 9C), demonstrated an inward current that was transient in time course and activated at voltages more positive than -58 mV, as well as outward currents. The transient inward current was blocked reversibly by 1 μM TTX. This pharmacology, together with the transient time course and the voltage-dependent activation of the inward current is typical for voltage-gated Na+ currents, found only in mature neurons and skeletal muscle cells (Sah et al, 1997; Whittemore et al, 1999). Skeletal muscle markers in these neuron-like cells was not detected. These studies suggest that treatment with FGF-8b+EGF and co-culture with glioblastoma cellsfresults ininaturation to cells with the fundamental characteristics of excitable neurons, TTX-sensitive voltage-gated Na+ currents. hMASC transplanted in ventricles of newborn rats differentiate in cells expressing astrocyte and neuronal markers
1.4xl04 hMASC were stereotactically injected in the lateral ventricles of Pl-
P3 Sprague Dawley rats. After 4 and 12 weeks, animals were sacrificed and analyzed for presence of human cells and evidence of differentiation of hMASC to neuroectoderm. Human cells, identified by staining with a antibodies against human nuclei or human nuclear membrane could be seen in the SVZ up to 400 μm away from the ventricle in animals analyzed after 4 weeks, and after 12 weeks, human cells could also be seen deeper in the brain parenchyma such as in the hippocampus and along the fomix. Some human cells had typical astrocyte morphology and stained positive with anti-GFAP antibodies, whereas other cells stained positive with anti-Neu-N antibodies, NF-200 and anti-human nuclear membrane antibodies. Triple staining showed that human nuclear antigen positive Neu-N positive cells did not coexpress and GFAP. Summary The central finding of this work is that single post-natal BM-derived MASC can be induced to differentiate not only into mesodermal cell types but also cells with mature neuronal characteristics, as well as astrocyte and oligodendrocyte characteristics. Time-dependent as well as culture-method-dependent maturation of MASC to cells with neuroectodermal features was shown. Double staining definitively demonstrated that neuronal or glial cells were authentic and results were not due to inappropriately expressed neuronal or glial markers. These results were confirmed at the mRNA level. Retroviral marking studies were used to demonstrate that the neurons, astrocytes and oligodendrocytes were derived from a single MASC that also differentiates into muscle and endothelium, as the sequence of the host cell genomic region flanking the retroviral vector was identical in all lineages. hMASC did not only acquire phenotypic but also electrophysiological characteristics of mature neurons, namely TTX-sensitive voltage-gated Na+ currents. Finally, it was also shown that MASC can differentiate in vivo into cells expressing neuronal and astrocyte markers.
Using retroviral marking of hMASC combined with PCR-based sequencing of the genomic sequence flanking the 3'-LTR of the retroviral insert, it was shown that neurons are derived from the same hMASC that differentiate into astrocytes and oligodendrocytes, as well as into endothelium and muscle (Jordan et al, 1990). This conclusively demonstrates that MASC can, at the single cell level, differentiate to cells of mesodermal and neuroectodermal lineages. The cells with the ability to differentiate not only into mesodermal cell types but also neuroectodermal cell types multipotent adult stem cells, or MASC were re-named. Sanchez-Ramos et al.
(Sanchez-Ramos et al, 2000) and Woodbury et al. (Woodbury et al, 2000) showed that populations of human or rodent MSC can express markers of astrocytes and neurons, but not oligodendrocytes in vitro. However, neither study provided evidence that the same cell that acquired neuroectodermal markers could also differentiate into mesodermal cells. Furthermore, neither study showed that cells expressing neuronal markers also acquired functional neuronal characteristics. Thus, although suggestive for neural differentiation, these reports did not conclusively demonstrate neural and glial differentiation from MSC.
It was also shown that hMASC transplanted in the ventricle of newborn rats can migrate in the neurogenic subventricular zone and into the hippocampus where they respond to local cues to differentiate into cells expressing astrocyte and neuronal markers. This model was chosen because migration and differentiation of NSC to specific neuronal phenotypes occurs to a much greater extent when transplantation is done in germinal areas of the brain than in non-neurogenic areas, and when transplants are done in newborn animals compared with adult animals (Bjorklund and Lindvall, 2000; Svendsen and Caldwell, 2000). Although hMASC are multipotent and differentiate into cells outside of the neuroectoderm, hMASC did not form teratomas. The number of cells that had migrated outside the subventricular area was low after 4 weeks, but increased after 12 weeks. The ease with which MASC can be isolated from post-natal BM, expanded and induced to differentiate in vitro to astrocytes, oligodendrocytes or neuronal cell types may circumvent one of the key problems in NSC transplantation, namely the availability of suitable donor tissue. Example 11. MASC Differentiation into Hepatocyte-like Cells
During embryogenesis, the first sign of liver morphogenesis is a thickening of the ventral endodermal epithelium, which occurs between e7.5 and e8.5 in the mouse (Zaret K.S., 2001). Little is known about the signals involved in initial endoderm formation and subsequent endoderm specification. Early in gastrulation
(e6-e7) endoderm is not specified, not even in an anterior/posterior direction
(Melton D., 1997). However, recent studies showed that ex vivo exposure of endoderm to FGF4 posteriorizes the early endoderm, which is now competent to express hepatic markers (Wells J.M. et al, 1999). By e8.5 in the mouse, definitive endoderm has formed the gut tube and expresses HNF3β (Zaret K.S., 2000). The foregut endoderm is induced to the hepatocyte lineage by acidic (a)FGF and bFGF, both produced by the adjacent cardiac mesoderm (Zaret K.S., 2001), which are required to induce a hepatic fate and not the default pancreatic fate (Zaret K.S., 2001). Basic morphogenetic proteins (BMP's) produced by the transversum mesenchyme are also required as they increase levels of the GATA4 transcription factor which promote the ability of endoderm to respond to FGF's (Zaret K.S., 2001). GATA4 and HNF3β are required for hepatic specification and are important effectors of downstream events leading to hepatocyte differentiation, as they upregulate markers of hepatocyte specific expression such as albumin, among others.
In most instances, mature hepatocytes can undergo several cell divisions and are responsible for hepatic cell replacement. As a result, there has been great controversy about the existence and function of a liver stem cell. During extensive liver necrosis due to chemical injury or when hepatocytes are treated with chemicals that block their proliferation, a population of smaller cells with oval shape, termed oval cells, emerges and proliferates (Petersen, B.E., 2001). These oval cells may constitute the "stem cell" compartment in the liver. Oval cells reside in the smallest units of the biliary tree, called the canals of Herring, from where they migrate into the liver parenchyma (Theise N.D., et al, 1999). Oval cells are bi-potential, giving rise in vitro and in vivo to both hepatocytes and bile ductular epithelium. Oval cells express several hematopoietic markers such as Thy 1.1, CD34, Flt3 -receptor, and c- Kit, and also express αFP, CKl 9, γ-glutamyl-transferase, and OV-6. The origin of oval cells is not known (Petersen, B.E., 2001; Kim T.H. et al, 1997; Petersen, B.E.,
2001).
Until recently, it was believed that hepatocytes could only be derived from cells of endodermal origin and their progenitors. However, recent studies suggest that non-endodermal cells may also form hepatocytes in vivo and in vitro (Petersen,
B.E., 2001 ; Pittenger M.F. et al, 1999). Following bone marrow (BM) transplantation, oval cells are derived from the donor BM (Theise N.D., et al,
1999). Transplantation of enriched hematopoietic stem cells (HSC) in FAH ' ' mice, an animal model of tyrosenimia type I, resulted in the proliferation of large numbers of donor LacZ+ hepatocytes and animals had restored biochemical function of the liver (Lagasse E. et al, 2000). Furthermore, single HSC may not only repopulate the hematopoietic system but also contribute to epithelium of lung, skin, liver and gut (Krause D.S. et al, 2001). Exocrine pancreatic tumor cells treated in vitro with dexamethasone (Dex) with or without oncostatin M (OSM) may acquire a hepatocyte phenotype (Shen C.N. et al, 2000). Finally, mouse embryonic stem (ES) cells spontaneously acquire a hepatocyte phenotype, a process that is enhanced by treatment with aFGF, HGF, OSM, and Dex (Hamazaki T. et al, 2001).
It was demonstrated here that single MASC not only differentiate into mesodermal and neuroectodermal cells, but also into cells with morphological, phenotypic and functional characteristics of hepatocytes in vitro. mMASC, rMASC, and hMASC acquire a hepatocyte-like phenotype when cultured with FGF4 and/or HGF. mMASC, rMASC and hMASC were selected and cultured as described. To determine optimal conditions for MASC differentiation into hepatocyte-like cells, the effect of different extracellular matrix (ECM) components was tested and cytokines known to induce hepatocyte differentiation in vivo or from ES cells (Zaret K.S., 2001) on mMASC or rMASC differentiation to hepatocytes. As differentiation requires cell cycle arrest, the effect of cell density was also tested. To demonstrate differentiation to hepatocyte like cells, cells were stained after 14 days with Abs against albumin, CKl 8, and HNF3 β.
Optimal differentiation of mMASC or rMASC to albumin, CKl 8 and HNF3β positive epithelioid cells was seen when MASC were plated at 21.5x103 cells/cm2 in the presence of 10 ng/ml FGF4 and 20 ng/ml HGF on Matrigel™ as shown in Table 7A. After 14 days, the percent albumin, CKl 8 and HNF3β positive epithelioid cells was 61.4+4.7%, and 17.3% of cells were binucleated. When plated on FN, differentiation to CKl 8 and HNF3β positive epithelioid cells was also seen, even though only 53.1+6.3% of cells stained and fewer (10.9%) binucleated cells were seen.
Culture with either FGF4 or HGF yielded albumin, CKl 8 and HNF3β positive epithelioid cells, but the percent albumin, CKl 8 and HNF3β positive cells was higher when mMASC or rMASC were treated with both FGF4 and HGF as shown in Table 7A. Addition of aFGF, bFGF, FGF7, BMP's, or OSM did not increase the percent cells positive for hepatocyte markers, while 1% DMSO and 0.1 mM-10 mM Sodium Butyrate did not support differentiation of mMASC or rMASC to cells positive for hepatocyte markers.
When cell densities between 2.5 and 25x103 cells/cm2 were tested, the highest percent cells with hepatocyte markers was seen in cultures seeded at 21.5x 103 cells/cm2. No hepatocyte differentiation was seen when cells were plated at <12.5xl03 cells/cm2. hMASC were plated at 3-30x103 cells/cm2 on lOng/mL FN or 1% Matrigel™ with aFGF, bFGF, FGF7, 1% DMSO, HGF, and / or FGF4. Only cells treated with lOng/ml FGF4 alone, 20ng/ml HGF alone, or a combination of both differentiated into epithelioid cells that expressed albumin, CKl 8 and HNF3β. hMASC plated at 15-30x10 cell/cm differentiated into epithelioid cells whereas hMASC plated at 3xl03 cell/cm2 died. Like mMASC or rMASC, the percent albumin, CK18 and HNF3β positive epithelioid cells was higher when hMASC were cultured on Matrigel™ (91.3% ± 4.4) than on FN (89.5% ± 5.4), and the percent binucleated cells was higher on Matrigel™ (31.3%) than on FN (28.7%) as shown in Table 7B. Table 7: Optimization of MASC differentiation into hepatocyte like cells.
Figure imgf000067_0001
Matrigelτ
Albumin ++/++ +/+ NT CK.18 ++/++ ++/+ +++/+++ NT HNF3β +++/++ f+++/+++ NT
Collagen
Albumin NT NT NT CK18 NT NT NT HNF3β NT NT NT
- = 0% + = 20%, ++ = 30%, +++ = 40%, ++++ = 60%, +++++ = 80% cells staining positive for specific markers and NT = not tested.
Phenotypic characterization of MASC differentiation to hepatocyte-like cells Hepatocyte differentiation was further evaluated over time by immunofluorescence and confocal microscopy for early (HNF3β, GATA4, CKl 9, αFP) and late (CK18, albumin, HNFlα) markers of hepatocyte differentiation. mMASC or rMASC plated on Matrigel™ with FGF4 and HGF enlarged from 8μm to 15μm diameter as shown in Table 8 A. On d21-d28, approximately 60% of cells were epithelioid and surrounded by smaller round or spindle shaped cells.
Undifferentiated mMASC or rMASC did not express any of the liver specific transcription factors or cytoplasmic markers. After 4 days, cells expressed HNF3β, GATA4 and αFP, low levels of CKl 9, and very rare cells stained positive for HNFlα, albumin or CKl 8. At seven days, the large epithelioid cells stained positive for HNF3β, GATA4, HNFlα with increasing staining for albumin and CKl 8. Only rare cells expressed αFP. After 14, 21 and 28 days, the large epithelioid cells stained positive for GATA4, HNF3β, HNFlα, CK18 and albumin, but not αFP or CKl 9. The smaller cells surrounding the nodules of epithelioid cells stained positive for CK19 and αFP. hMASC was plated on Matrigel™ with FGF4 and HGF or FGF4 alone enlarged from 10-12μm to 20-30μm diameter by d21. After 7 days, cells expressed HNF3β, GATA4 and low levels of CKl 9, while few cells stained positive for albumin or CKl 8. After 14 and 21 days, >90% of epithelioid cells stained positive for GATA4, HNF3β, HNFlα, HNF4, CK18 and albumin, while only rare cells stained positive for αFP or CKl 9 as shown in Figure 10B.
Table 8: Immunohistochemistry Pattern of Hepatocyte Marker Expression
Figure imgf000069_0001
+ = Marker is expressed, - = Marker is not expressed and NT = not tested
Hepatocyte-like cells are derived from the same single hMASC that differentiated into neuroectoderm and endoderm
It has been shown that single mMASC or rMASC differentiate into endothelium, neuroectoderm and CKl 8 and albumin positive endodermal cells. It has also been shown that single hMASC differentiate into mesoderm and neuroectoderm. The same single hMASC was tested to determine whether they can differentiate into hepatocyte-like cells. MASC were obtained, cultured and expanded as described. For differentiation, mMASC or rMASC were plated at 5- 25xl03 cells/cm2 on 0.01-lOμg/ml fibronectin (FN), 0.01-8μg/ml collagen (Sigma Chemical Co, St. Louis, MO), or 1% Matrigel™ (Becton-Dickinson) in serum-free medium [60% low glucose DMEM (DMEM-LG; Gibco-BRL, Grand Island, NY), 40% MCDB-201 (Sigma), supplemented with IX insulin/transferrin/selenium, 4.7 μg/ml linoleic acid, 1 mg/ml bovine serum albumin (BSA), 10"8 M dexamethasone, 10"4 M ascorbic acid 2-phosphate (all from Sigma), lOOU/ml penicillin, 100/ml U streptomycin (Gibco)], with 2% FCS (Hyclone, Logan Utah) and 10 ng/mL each epidermal growth factor (EGF) (Sigma), leukemia inhibitory factor (LIF; Chemicon, Temecula, CA), and platelet derived growth factor (PDGF-BB; R&D Systems, Minneapolis, MN). hMASC were plated at 15-30xl03 cells/cm2 on 0.1 μg/ml FN, or 1 % Matrigel™ in the same medium without LIF (Reyes M., 2002). After 8-12h, media were removed, cells washed twice with phosphate buffered saline (PBS) (Fischer) and cultured in serum-free medium supplemented with 5-50ng/ml HGF, aFGF, bFGF, FGF4, FGF7, or OSM; or 10 mg/ml dimethyl-sulphoxide (DMSO), or 0.1-1 mM sodium butyrate.
Transduction of hMASC with eGFP was performed using an eGFP-cDNA containing retrovirus and expanded to >5X106 cells. Twenty percent was induced to differentiate into muscle, endothelium, neuroectoderm and endoderm. For clone A16 a single retroviral insertion site was present in undifferentiated MASC as well as mesodermal and neuroectodermal differentiated cells and eGFP+ clone A16 MASC differentiated into CKl 8 and albumin positive cells. The same insertion site was present in FGF4-treated MASC generated from the same cell population (5'- TAG CGGCCGCTTGAATTCGAACGCGAGACTACTGTGACT CACACT-3', Chromosome 7), proving that single hMASC differentiate into endoderm aside from mesoderm and neuroectoderm. Quantitative RT-PCR demonstrates that FGF4 and HGF induces hepatocyte specification and differentiation.
Hepatocyte differentiation by quantitative RT-PCR was confirmed for early (HNF3β, GATA4, CKl 9, αFP) and late (CKl 8, albumin, HNFlα, cytochrome P450) markers of hepatocyte differentiation. RNA was extracted from 3xl05 MASC or MASC induced to differentiate to hepatocytes. mRNA was reverse transcribed and cDNA was amplified as follows: 40 cycles of a two step PCR (95°C for 15", 60°C for 60") after initial denaturation (95°C for 10') with 2μl of DNA solution, IX TaqMan SYBR Green Universal Mix PCR reaction buffer using a ABI PRISM 7700 (Perkin Elmer/ Applied Biosystems). Primers used for amplification are listed in Table 9. Table 9: Primers used
Figure imgf000070_0001
Figure imgf000071_0001
mRNA levels were normalized using β-actin (mouse and human) or 18S (rat) as housekeeping genes and compared with mRNA levels in freshly isolated rat or mouse hepatocytes, rat hepatocytes cultured for 7 days, or mRNA from human adult liver RNA purchased from Clontech, Palo Alto, California.
On dO, mMASC and rMASC expressed low levels of albumin αFP, CKl 8, CKl 9, TTR, HNF3β, HNFlα and GATA4 mRNA, but no CYP2B9 and CYP2B13 (mouse) or CYP2B1 (rat) mRNA (Fig. 10). Following treatment of mMASC or rMASC with FGF4 and HGF, expression of HNF3β and GATA4 mRNA increased on d2, became maximal by d4, decreasing slightly and leveling off by dl4. mRNA for αFP, and CKl 9 increased after d2, and became maximal by d4 and decreased thereafter. TTR mRNA increased after d4, was maximal by d7 and leveled off.
CK18, Albumin, HNFlα and P450 enzyme mRNA increased after d7 and was maximal on dl4. Between dl4 and d21, FGF4 and HGF induced MASC expressed albumin, TTR, CKl 8, CYP2B9 and CYP2B13 (mouse) and CYP2B1 (rat) mRNA. Undifferentiated hMASC expressed low levels of albumin, CKl 8, and
CKl 9, CYP1B1, but not αFP (Fig. 10) and CYP2B6 mRNA. Levels of albumin,
CKl 8, CKl 9, CYP1B1 mRNA increased significantly in hMASC cultured with
FGF4 alone or with FGF4 and HGF for 14 days compared to day 0 (MASC) cultures. Levels of albumin, CKl 8 and CYP1B1 mRNA continued to increase and were higher on d28. Although, CYP1B1 is not a specific hepatocyte marker, its upregulation suggests hepatocyte commitment and maturation. Low levels of CYP2B6, 0.5% to 1.0% of fresh liver mRNA's could be seen on dl4 and d21 but not dO. mRNA levels of immature hepatocyte markers (CKl 9 and αFP) decreased as differentiation progressed and were higher in cultures induced with FGF4 alone, whereas mRNA levels for mature hepatocytes (CKl 8 and albumin) were higher in FGF4 and HGF-induced hMASC.
Western Blot demonstrates that FGF4+HGF induces hepatocyte specification and differentiation
Expression of hepatocyte-specific genes was also confirmed by Western Blot and performed as described by Reyes et al. (2000). Abs to αFP, human albumin, CKl 8 were diluted 1 : 1000 in blocking buffer. Goat anti- β-actin (1 :1000) was from Santa Cruz. Secondary Abs were HRP-linked goat anti-mouse and HRP-linked donkey anti-goat (Amersham, Arlington Heights). ECL was performed according to manufacturers instructions (Amersham). Undifferentiated hMASC did not express CKl 8, albumin, or αFP protein (Fig. 10B). After treatment for 35 days with FGF4 alone or FGF4 and HGF, hMASC expressed albumin and CKl 8, but not αFP, consistent with the histochemical analysis. mMASC, rMASC and hMASC acquire hepatocyte functional activity
Five different assays were used to determine whether cells with morphologic and phenotypic characteristics of hepatocytes also had functional hepatocyte attributes.
Urea production and secretion by hepatocyte-like cells was measured at various time points throughout differentiation. Urea concentrations were determined by colorimetric assay (Sigma Cat. 640-1) per manufacturer's instructions. Rat hepatocytes grown in monolayer and fetal mouse liver buds were used as positive controls, and culture medium as negative control. The assay can detect urea concentrations as low as 10 mg/ml. As the assay also measures ammonia, samples were assessed before and after urease addition.
No urea or ammonia was detected in culture medium alone. Undifferentiated
MASC did not produce urea. Following treatment with FGF4 and HGF, urea production by MASC increased in a time dependent manner. The time course for urea production in mouse and rat cultures was similar. For hMASC treated with FGF4 and HGF, urea was not detected on d4, was similar to mouse and rat cultures by dl2, and exceeded that in mouse or rat cultures on d21. Levels of urea produced by MASC-derived hepatocytes were similar to that in monolayer cultures of primary rat hepatocytes. For all three species, significantly more urea was produced by cells differentiated on Matrigel™ compared to FN. Albumin production was measured at various time points throughout the differentiation. Rat albumin concentrations were determined by a competitive enzyme linked immunoassay (ELISA) described previously (Tzanakakis E.S., et al, 2001 ; Wells J.M. et al, 2000). Human and mouse albumin concentrations were determined using a similar ELISA method with substitution of human or mouse albumin and anti-human or anti-mouse albumin Abs for the rat components where appropriate. Peroxidase conjugated anti-human-albumin and reference human albumin were from Cappel. Peroxidase conjugated and affinity purified anti-mouse albumin and reference mouse albumin were from Bethyl Laboratories (Montgomery, Texas). To ensure specificity of the ELISA, human, mouse, and rat Abs were incubated for 2 hrs at 37°C with 3% BSA in distilled water (dH2O). ELISA's had a sensitivity of at least 1 ng/ml.
Undifferentiated MASC did not secrete albumin. Following treatment with FGF4 and HGF, mMASC, rMASC and hMASC produced albumin in a time dependent manner. As was seen for urea production, MASC differentiated on Matrigel™ produced higher amounts of albumin than when cultured on FN. Mouse, rat, and human cells secreted similar levels of albumin, even though albumin was not detected in human cultures on d3. Levels of albumin produced by mouse, rat and human MASC-derived hepatocytes were similar to those seen in monolayer cultures of primary rat hepatocytes.
Cytochrome P450 activity was next assessed in aggregates of MASC-derived hepatocytes and primary rat liver hepatocyte spheroids using the PROD assay. mMASC-hepatocyte aggregates were formed by plating dl4 FGF4 and HGF treated mMASC at 5xl04 cells/cm on non-tissue culture plates, which were placed on a shaker at 10 revolutions per minute for 5h. Cell aggregates were transferred to
Primaria™ dishes and allowed to compact for 4 days in the presence or absence of
ImM phenobarbital. hMASC-hepatocyte aggregates were formed by hanging drop method. Briefly, 103 hMASC treated for 24 days with FGF4 and HGF were placed into lOOμL drops with or without ImM phenobarbital. After 4 days, aggregates were collected and cytochrome P450 activity assessed by PROD assay. Pentoxyresorufin (PROD) (Molecular Probes, Eugene, Oregon) is O-dealkylated by Cytochrome P450, changing a non-fluorescent compound into a fluorescent compound, resorufin (Tzanakakis E.S. et al, 2001). Fluorescence intensity caused by PROD metabolism consequently estimates cytochrome P450 (CYP) activity. Assessment and detection of resorufin in situ was performed using confocal microscopy as described (Tzanakakis E.S. et al, 2001).
No PROD activity was seen in aggregates of undifferentiated mMASC or hMASC. However, mMASC (18 days with FGF4 and HGF) and hMASC (28 days, FGF4 alone) induced to form aggregates had significant PROD activity. PROD activity in MASC-derived hepatocyte aggregates was similar to that of primary rat hepatocyte aggregates. A number of different cells have P450 activity, but P450 activity up-regulation by phenobarbital is only seen in hepatocytes. Therefore, P450 was also tested in the presence or absence of phenobarbital. Without phenobarbital, several P450 enzymes partially participate in PROD metabolism giving an inflated fluorescence value for those samples. In contrast, in the phenobarbital induced aggregates, PROD activity is almost wholly metabolized by mouse cytochromes Cyp2b9, Cyp2bl0, and Cyp2bl3, rat cytochrome Cyp2bl/2 (Tzanakakis E.S. et al, 2001), and in human, by CYP2B6. Therefore increased fluorescent activity is smaller than the actual increase in the protein expression of the stated cytochrome P450 enzymes. When aggregates were cultured for 96 hours with phenobarbital, a 32% to 39% increase in PROD activity was seen, suggesting presence of functional hepatocyte specific Cyp2b9, Cyp2bl0, and Cyp2bl3 in mMASC and CYP2B6 in hMASC-derived hepatocytes.
MASC-derived hepatocytes were also assessed for their ability to take up
LDL by incubating FGF4 treated hMASC with LDL-dil-acil. Cells were co-labeled either with anti-CKl 8 or anti-Pan-CK and HNF-3β or GATA4 Abs. After 7 days, low level uptake of a-LDL was detected, which increased to become maximal on d21.
Another metabolic function of hepatocytes is glycogen production or gluconeogenesis. The levels of glycogen storage were analyzed by periodic acid Schiff (PAS) staining of FGF4 and HGF induced mouse MASC and FGF induced hMASC at d3, d7, dl4, and d21. For PAS, slides were oxidized in 1% periodic acid for 5' and rinsed 3 times in dH O. Afterwards slides were treated with Schiff s reagent for 15', rinsed in dH2O for 5-10', stained with Mayer's hematoxylin for 1 ' and rinsed in dH2O. Glycogen storage was first seen by dl4 and maximum levels were seen after d21 (Fig. 11).
Hepatocyte Isolation and Culture
Hepatocytes were harvested from 4-6 week old male Sprague-Dawley rats as described (Seglen P.O., 1976). Hepatocyte viability after the harvest ranged from 90-95%. Hepatocytes were cultured as described (Tzanakakis E.S. et al, 2001; Tzanakakis E.S. et al, 2001). To form a monolayer, hepatocytes were cultured on 35 mM Fischer culture plates (Fischer Scientific, Pittsburgh, PA) coated with 8μg/cm collagen (Cohesion Technologies, Palo Alto, CA). To form spheroids, hepatocytes were cultured on 35-mm Primaria™ dishes (Becton Dickinson). Under both conditions, seeding density was 5xl04 cells/cm2. 12h after initial plating, medium was changed to remove dead and unattached cells. Medium was replaced every 48 hours thereafter. Summary
It has been shown that a single post-natal mouse, rat and human BM-derived MASC can differentiate in vitro into an endodermal cell type with hepatocyte phenotype and function. MASC, cultured under hepatocyte differentiation conditions, expressed in a time-dependent fashion primitive and mature hepatocyte markers, shown by immunofluorescence microscopy of double and triple labeled cells. The protein expression profile was hepatocyte specific and not spurious, as non-hepatocyte markers were not co-expressed with hepatocyte antigens. Results from immunohistochemistry were confirmed by Western blot. In addition, RT-PCR corroborated upregulation of the transcription factors HNF3β and GATA4 known to be important in endoderm specification and transcription factors required for subsequent hepatocyte differentiation, such as HNF3β, and cytoplasmic proteins such as CKl 9, CKl 8, αFP and albumin.
Although it was shown that FGF4 alone or both FGF4 and HGF induced
MASC into cells with morphological and phenotypic characteristics of hepatocytes, this alone does not prove that cells have differentiated into hepatocytes unless one can demonstrate acquisition of functional characteristics of hepatocytes. Therefore, several functional tests were done in combination to identify functional hepatocytes. mMASC, rMASC or hMASC produced urea and albumin, contained phenobarbital inducible cytochrome P450 activity, could take up Dil-acil-LDL, and contained glycogen granules. Although urea production is characteristic of hepatocyte activity, kidney tubular epithelium also produces urea (Hedlund E. et al, 2001). In contrast, albumin production is a specific test for the presence and metabolic activity of hepatocytes (Hedlund E. et al, 2001). Cytochrome P450, although found in hepatocytes, is also present in many other cell types (Jarukamjorn K. et al, 1999). However, Cyp2bl activity in rat (Tzanakakis E.S. et al, 2001), Cyp2b9 and Cyp2bl3 in mouse (Li-Masters T. et al, 2001; Zelko I. Et al, 2000), and CYP2B6 in human is considered relatively hepatocyte specific. Presence of these forms of P450 was shown by RT-PCR. The specificity for hepatocytes is enhanced further when P450 activity is inducible by phenobarbital (Rader D J. et al, 2000), as shown. Although LDL uptake is seen in hepatocytes (Oh S.H. et al, 2000), other cells such as endothelium have a similar capability (Avital I. et al, 2001). Finally, only hepatocytes can generate and store glycogen. When taken together, these functional tests demonstrate that MASC from mouse, rat or humans treated in vitro with FGF4 and HGF not only express hepatocyte markers but also have functional characteristics consistent with hepatocyte metabolic activities. Several studies have shown that BM derived cells may differentiate into hepatocyte-like cells in vivo and in vitro (Petersen B.E. et al, 1999; Theise N.D. et al, 2000; Krause D.S. et al, 2001; Pittenger M.F. et al, 1999; Wang S. et al, 2001; Lagasse E. et al, 2000). However, most studies have not addressed the phenotype of the BM cell that differentiates into cells with hepatocyte phenotype. It is unknown whether the cells staining positive for hepatocyte markers had functional characteristics of hepatocytes, and whether cells that differentiate into hepatocytes can also differentiate into mesodermal cells, such as hematopoietic cells. Lagasse et al. demonstrated that cKit+Thyι o Scal+ Lin+" cells present in murine BM differentiate into cells with not only hepatocyte phenotype but also hepatocyte function (Lagasse
E. et al, 2000). Even though such results could be seen when as few as 50 cells were transplanted, this study did not prove that the same cell that differentiates into hematopoietic cells also differentiates into hepatocytes. Krause et al showed that a single cell can repopulate the hematopoietic system and give rise to rare hepatocytes. However, no functional assessment of the hepatocytes was done (Krause D.S. et al, 2001). Avital et al recently published that β2m", Thy-1+ cells in mouse BM express albumin, HNF4, C/EBPα, and Cytochrome P450 3A2 mRNA and protein (Wilmut I., et al, 1997), a phenotype of hepatocyte progenitors usually found in the liver. Thus, presence of such hepatocyte progenitor cells in BM could explain the in vivo differentiation of bone marrow into hepatocytes noted in recent studies (Krause D.S. et al, 2001 ; Lagasse E. et al, 2000).
To address the question whether cells giving rise to functional hepatocyte- like cells also give rise to other cell types, retroviral marking was used (Reyes M. et al, 2001; Jiang Y., 2002). It has been recently shown that cells expressing albumin, CKl 8 and HNFlα can be generated from the same mMASC and rMASC that differentiate into cells with endothelial and neuroectodermal phenotype (Jiang Y., 2002). It is confirmed that similar results are seen for hMASC. Extending recently published studies demonstrating derivation of cells with mesodermal and neuroectodermal phenotype and function from single hMASC (Reyes M., 2002), it is shown here that the same single hMASC also differentiates into cells with hepatocyte morphology and phenotype. Thus, it is demonstrated for the first time that MASC that do not express hepatocyte markers and have no functional hepatocyte activity exist in BM, which depending on the culture conditions, acquire a hepatocyte phenotype and functional characteristics of hepatocytes, or phenotypic and functional characteristics of mesodermal and neuroectodermal cells. Example 12. Transplantation of LacZ Transgenic MASC to Treat Hemophiliac
Mice
MASC were derived from ROSA26 mice containing the β-gal/NEO transgene (106 cells/mouse) and were IN. injected into hemophiliac mice (Ν=5) without prior irradiation. The animals were sacrificed at 1 (N=2) and 2 months (N=3) post-MASC transplantation. Bone marrow cytospins and frozen sections of liver, spleen, skeletal muscle, heart, lung and intestine were stained for presence of β-gal antigen using a FITC-conjugated anti-β-gal antibody and pan-cytokeratin or CD45. Tissues were also analyzed by Q-PCR for the β-gal gene as described in Example 6.
Preliminary analysis indicates that one of the three animals (M3) analyzed at 2 months post-injection had 0.1% of pulmonary epithelial cells derived from the donor cells by immunohistochemistry and Q-PCR. Immunohistochemistry also showed that animal M5 had <1% engraftment of CD45+ donor cells in the spleen, marrow and intestine. Tissues of the animal M4 had some donor derived cells on immunohistochemistry; PCR data on this animal is pending.
All publications, patents and patent applications are incorporated herein by reference as though individually incorporated by reference. While in the foregoing specification this invention has been described in relation to certain preferred embodiments thereof, and many details have been set forth for purposes of illustration, it will be apparent to those skilled in the art that the invention is susceptible to additional embodiments and that certain of the details described herein may be varied considerably without departing from the basic principles of the invention. REFERENCES
Adams, R.H., and Klein, R. (2000). Eph receptors and ephrin ligands. Essential mediators of vascular development. Trends Cardiovasc Med. 10:183-188.
Alison, M., and Sarraf, C. (1998). Hepatic stem cells. J Hepatol 29: 678-83. Alizadeh, A.A., M.B. Eisen, R.E. Davis, C. Ma, I.S. Lossos, A. Rosenwald,
J.C. Boldrick, H. Sabet, T. Tran, X. Yu, J.I. Powell, L. Yang, G.E. Marti, T. Moore, J.J. Hudson, L. LU. D.B. Lewis, R. Tibshirani, G. Sherlock, W.C. Chan, T.C. Greiner, D.D. Weisenburger, J.O. Armitage, R. Warnke, and L.M. Staudt. 2000. Distinct types of diffuse large B-cell lymphoma identified by gene expression profiling. Nature. 403:503-511.
Anderson, C. M., and Swanson, R. A. (2000). Astrocyte glutamate transport: review of properties, regulation, and physiological functions. Glia 31 :1-14.
Anderson, D. J., Gage, F. H., and Weissman, I. L. (2001). Can stem cells cross lineage boundaries? Nat Med., 393-5. Arsenijevic, Y., and Weiss, S. (1998). Insulin-like growth facor-I is a differentiation factor for postmitotic CΝS stem cell-derived neuronal precursors: distinct actions from those of brain-derived neurotrophic factor. JNeurosci 18:118- 28.
Asahara, T., Masuda, H., Takahashi, T., Kalka, C, Pastore, C, Silver, M., Keame, M., Magner, M., and Isner, J. M. (1999). Bone marrow origin of endothelial progenitor cells responsible for postnatal vasculogenesis in physiological and pathological neovascularization. Circ Res 85:221-8.
Asahara, T., Murohara, T., Sullivan, A., Silver, M., van der Zee, R., Li, T., Witzenbichler, B., Schatteman, G., and Isner, J. (1997). Isolation of putative progenitor endothelial cells for angiogenesis. Science 275, 964-967.
Avital, I., Inderbitzin, D., Aoki, T., Tyan, D.B., Cohen, A.H., Ferraresso, C,
Baumhueter, S., Dybdal, Ν., Kyle, C, and Lasky, L. (1994). Global vascular expression of murine CD34 a sialomucin-like endothelial ligand for L-selectin. Blood 84:2554. Ben-Shushan, E., Thompson, J. R., Gudas, L. J., and Bergman, Y. (1998).
Rex- 1 , a gene encoding a transcription factor expressed in the early embryo, is regulated via Oct-3/4 and Oct-6 binding to an octamer site and a novel protein, Rox- 1, binding to an adjacent site. Mol Cell Biol 18:1866-78. Bierhuizen, M. F., Westerman, Y., Visser, T. P., Dimjati, W., Wognum, A.
W., and Wagemaker , G. (1997). Enhanced green fluorescent protein as selectable marker of retroviral-mediated gene transfer in immature hematopoietic bone marrow cells. Blood 90:3304-15. Bjorklund, A., and Lindvall, O. (2000). Cell replacement therapies for central nervous system disorders. Nat Neurosci 3: 537-44.
Bjomson, C, R. Rietze, B. Reynolds, M. Magli, and A. Vescovi. (1999). Turning brain into blood: a hematopoietic fate adopted by adult neural stem cells in vivo. Science. 283:354-357. Blondel, O., Collin, C, McCarran, W. J., Zhu, S., Zamostiano, R., Gozes, I.,
Brenneman, D. E., and McKay, R. D. (2000). A glia-derived signal regulating neuronal differentiation. J Neurosci. 20:8012-20.
Bradley, A. (1987). Production and analysis of chimaeric mice. In Teratocarcinomas and ES Cells: A Practical Approach. E.J. Robertson, ed. Oxford: IRL Press, 113-151.
Brazelton, T. R., Rossi, F. M. N., Keshet, G. I., and Blau, H. E. (2000). From Marrow to Brain: Expression of Neuronal Phenotypes in Adult Mice. Science 290:1775-1779.
Bruder, S., et al, U.S. Patent No. 5,736,396 Brustle, O., Jones, K., Learish, R., Karram, K, Choudhary, K, Wiestler, O.,
Duncan, I., and McKay, R. (1999). ES Cell-Derived Glial Precursors: A Source of Myelinating Transplants. Science 285:754-6.
Brustle, O., Spiro, A. C, Karram, K., Choudhary, K., Okabe, S., and McKay, R. D. (1997). ES cells differentiate into oligodendrocytes and myelinate in culture and after spinal cord transplantation. Proc. Natl. Acad. Sci. USA 94:14809-14814.
Butler, D., (1999) FDA warns on primate xenotransplants. Nature 398:549.
Caplan, A., et al, U.S. Patent No. 5,486,359
Caplan, A., et al, U.S. Patent No. 5,811,094
Caplan, A., et al, U.S. Patent No. 5,837,539 Cassiede P., Dennis, J. E., Ma, F., Caplan, A. I., (1996). Osteochondrogenic potential of marrow mesenchymal progenitor cells exposed to TGF-beta 1 or PDGF- BB as assayed in vivo and in vitro. J Bone Miner Res. 9:1264-73. Cereghini, S. (1996). Liver-enriched transcription factors and hepatocyte differentiation. FASEB J.10:267-82.
Choi, K. (1998). Hemangioblast development and regulation. Biochem Cell Biol 76:947-956. Choi, K., M. Kennedy, A. Kazarov, J.C. Papadimitriou, and G. Keller.
(1998). A common precursor for hematopoietic and endothelial cells. Development. 125:725-732.
Ciccolini, F., and Svendsen, C. N. (1998). Fibroblast growth factor 2 (FGF- 2) promotes acquisition of epidermal growth factor (EGF) reponsiveness in mouse striata] precursor cells: Identification of neural precursors responding to both EGF and FGF-2. J Neuroscience 18:7869-7880.
Clarke, D. L., Johansson, C. B., Wilbertz, J., Veress, B., Nilsson, E., Karlstrom, H., Lendahl, U., and Frisen, J. (2000). Generalized potential of adult NSCs. Science 288:1660-3. Conway, E.M., Collen, D., and Carmeliet, P. (2001). Molecular mechanisms of blood vessel growth. Cardiovasc Res. 49:507-521.
Corbeil, D., Roper, K, Hellwig, A., Tavian, M., Miraglia, S,. Watt, S.M., Simmons, P.J., Peault, B., Buck, D.W., and Huttner, W.B. (2000). The human AC 133 HSC antigen is also expressed in epithelial cells and targeted to plasma membrane protrusions. J Biol Chem. 275:5512-5530.
Crosby, H.A., Kelly, D.A., and Strain, A.J. 2001. Human hepatic stem-like cells isolated using c-kit or CD34 can differentiate into biliary epithelium. Gastroenterology. 120:534-544.
Daadi, M. M., and Weiss, S. (1999). Generation of tyrosine hydroxylase- producing neurons from precursors of the embryonic and adult forebrain. J New rø.19:4484-97.
Dahlstrand, J., Lardelli, M., and Lendahl, U. (1995). Nestin mRNA expression correlates with the central nervous system progenitor cell state in many, but not all, regions of developing central nervous system. Brain Res Dev Brain Res. 84:109-29.
Devon R. S., Porteous D. J., and J., B. A. (1995). Splink-erettes improved vectorettes for greater efficiency in PCR walking. Nucleic Acids Res 23:1644-1645.
DiGuisto, et al, U.S. Patent No. 5,681,599 Doetsch, F., Caille, I., Lim, D. A., Garcia- Verdugo, J. M., and Alvarez- Buylla, A. (1999). Subventricular zone astrocytes are NSCs in the adult mammalian brain. Cell 97:703-716.
Eliceiri, B.P., and Cheresh, D.A. (2000). Role of alpha v integrins during angiogenesis. Cancer J Sci Am. 6, Suppl 13:S245-249.
Evans, et al., (1992). J. Am. Med. Assoc, 267:239-246.
Faloon, P., Arentson, E., Kazarov, A., Deng, C. X., Porcher, C, Orkin, S., and Choi, K. (2000). Basic fibroblast growth factor positively regulates hematopoietic development. Development. 127:1931-1941. Fei, R., et al, U.S. Patent No. 5,635,387
Ferrari, G., Cusella-De Angelis, G., Coletta, M., Paolucci, E., Stomaiuolo, A., Cossu, G., and Mavilio, F. (1998). Muscle regeneration by bone marrow- derived myogenic progenitors. Science 279:528-30.
Flax, J. D., Sanjay, A., Yang, C, Simonin, C, Wills, A. M., Billinghurst, L. L., Jendoubi, M., Sidman, R. L., Wolfe, J. H., Kim, S. E., and Snyder, E. Y. (1998). Engraftable human NSCs respond to developmental cues replace neurons and express foreign genes. Nature Biotech 16:1033-1038.
Fong, G. H., Zhang, L., Bryce, D. M., and Peng, J. (1999). Increased hemangioblast commitment, not vascular disorganization, is the primary defect in fit- 1 knock-out mice. Development. 126:3015-3025.
Franco Del Amo, F., Gendron-Maguire, M., Swiatek, P. J., and Gridley, T. (1993). Cloning, sequencing and expression pf the mouse mammalian achaete-scute homolog a (MASH 1). Biochem Biophys Acta 1171 :323-7.
Frankel, M. S. (2000). In Search of Stem Cell Policy. Science 298:1397. Fridenshtein, A. (1982). Stromal bone marrow cells and the hematopoietic microenvironment. Arkh Patol 44:3-11.
Furcht et al. International Application No. PCT/USOO/21387.
Gage, F. H. (2000). Mammalian NSCs. Science 287:1433-1438.
Gage, F., Coates, P., Palmer, T., Kuhn, H., Fisher, L., Suhonen, J., Peterson, D., Suhr, S., and Ray, J. (1995). Survival and differentiation of adult neuronal progenitor cells transplanted to the adult brain. Proc Natl Acad Sci USA 92:11879- 83. Gehling, U.M., Ergun, S., Schumacher, U., Wagener, C, Pantel , K., Otte,
M., Schuch, G., Schafhausen, P., Mende, T., Kilic, N., Kluge, K., Schafer, B.,
Hossfeld, D.K. and Fiedler, W. (2000). In vitro differentiation of endothelial cells from AC 133-positive progenitor cells. Blood. 95:3106-31 12. Gritti, A., Frolichsthal-Schoeller, P., Galli, R., Parati, E. A., Cova, L.,
Pagano, S. F., Bjomson, C. R., and Vescovi, A. L. (1999). Epidermal and fibroblast growth factors behave as mitogenic regulators for a single multipotent stem cell-like population from the subventricular region of the adult mouse forebrain. J Neurosci.
19:3287-97. Gronthos, S., Graves, S., Ohta, S., and Simmons, P. (1994). The STRO-1+ fraction of adult human bone marrow contains the osteogenic precursors. Blood 84:
4164-73.
Guenechea, G., Gan, O., Dorrell, C, and Dick, J. E. (2001). Distinct classes of human stem cells that differ in proliferative and self-renewal potential. Nat Immunol 2:75-82.
Gussoni, E., Soneoka, Y., Strickland, C, Buzney, E., Khan, M., Flint, A., Kunkel, L., and Mulligan, R. (1999). Dystrophin expression in the mdx mouse restored by stem cell transplantation. Nature 401 :390-4.
Hamazaki, T., liboshi, Y., Oka, M., Papst, P.J., Meacham, A.M., Zon, L.I., and Terada, N. 2007. Hepatic maturation in differentiating embryonic stem cells in vitro. FEBSLett 497:15-19.
Haralabopoulos, G.C., D.S. Grant, H.K. Kleinman, and M.E. Maragoudakis. (1997). Thrombin promotes endothelial cell alignment in Matrigel in vitro and angiogenesis in vivo. Am J Physiol. 273:C239-245. Hedlund, E., Gustafsson, J.A., and Warner, M. (2001). Cytochrome P450 in the brain; a review. Curr Drug Metab 2:245-263.
Hill, B., Rozler, E., Travis, M., Chen, S., Zannetino, A., Simmons, P., Galy, A., Chen, B., Hoffman, R. (1996). High-level expression of a novel epitope of CD59 identifies a subset of CD34+ bone marrow cells highly enriched for pluripotent stem cells. Exp Hematol. 8:936-43.
Hirashima, M., H. Kataoka, S. Nishikawa, N. Matsuyoshi , and S.Nishikawa. (1999). Maturation of ES cells into endothelial cells in an invitro model of vasculogenesis. Blood. 93:1253-1263. Holash, J., Maisonpierre, P.C., Compton, D., Boland, P., Alexander, C.R.,
Zagzag, D., Yancopoulos, G.D., and Wiegand, S.J. (1999). Vessel cooption, regression, and growth in tumors mediated by angiopoietins and VEGF. Science.
284:994-998. Hu, Z., Evarts, R. P., Fujio, K., Marsden, E. R., and Thorgeirsson, S. S.
(1993). Expression of hepatocyte growth factor and c-met genes during hepatic differentiation and liver development in the rat. Am JPathol.142: 1823-30.
Iyer, V.R., Eisen, M.B., Ross, D.T., Schuler, G., Moore, T., Lee, J.C.F., Trent, J.M., Staudt, L.M., Hudson, J.J., Boguski, M.S., Lashkari, D., Shalon, D., Botstein, D., and Brown, P.O. (1999). The transcriptional program in the response of human fibroblasts to serum. Science. 283:83-87.
Jackson, K., Majka, S. M., Wang, H., Pocius, J., Hartley, C, Majesky, M. W., Entman, M. L., Michael, L., Hirschi, K. K., and M.A., G. (2001). Regeneration of ischemic cardiac muscle and vascular endothelium by adult stem cells. J Clin Invest 107:1395-1402.
Jackson, K., Mi, T., and Goodell, M. A. (1999). Hematopoietic potential of stem cells isolated from murine skeletal muscle. Proc Natl Acad Sci USA 96:14482-6.
Jaiswal, N., et al, (1997). J. Cell Biochem. 64(2):295-312. Jarukamjorn, K, Sakuma, T., Miyaura, J., and Nemoto, N. (1999). Different regulation of the expression of mouse hepatic cytochrome P450 2B enzymes by glucocorticoid and phenobarbital. Arch Biochem Biophys 369:89-99.
Jiang, Y. 2002. Submitted.
Johansson, C. B., Momma, S., Clarke, D. L., Risling, M., Lendahl, U., and Frisen, J. (1999). Identification of a NSC in the adult mammalian central nervous system. Cell. 96:25-34.
Johnstone, B., Hering, T. M., Caplan, A. I., Goldgberg, V. M., Yoo, J. U. (1998). In vitro chondrogenesis of bone marrow-derived mesenchymal progenitor cells. Exp Cell Res. 1 :265-72. Jordan, C. T., and Van Zant, G. (1998). Recent progress in identifying genes regulating HSC function and fate. Curr Opin Cell Biol 10:716-20.
Jordan, C, McKearn, J., and Lemischka, I. (1990). Cellular and developmental properties of fetal HSCs. Cell 61 :953-963. Kim, T.H., Mars, W.M., Stolz, D.B., Petersen, B.E., and Michalopoulos,
G.K. (1997). Extracellular matrix remodeling at the early stages of liver regeneration in the rat. Hepatology 26:896-904.
Kopen, G., D. Prockop, and D. Phinney. 1999. Marrow stromal cells migrate throughout forebrain and cerebellum, and they differentiate into astrocytes after injection into neonatal mouse brains. Proc Natl Acad Sci U S A. 96:1071 1-10716.
Kourembanas, S., Morita, T., Christou, H., Liu, Y., Koike, H., Brodsky, D., Arthur, V., and Mitsial, S.A. (1998). Hypoxic responses of vascular cells. Chest. 11 (Suppl 1):25S-28S. Krause, D. S., Theise, N. D., Collector, M. I., Henegariu, O., Hwang, S.,
Gardner, R., Neutzel, S., and Sharkis, S. I. (2001). Multi-organ, multi-lineage engraftment by a single bone marrow-derived stem cell. Cell 105:369-77.
Lagasse, E., Connors, H., AI-Dhalimy, M., Reitsma, M., Dohse, M., Osbome, L., Wang, X., Finegold, M., Weissman, I.L., and Grompe, M. (2000). Purified hematopoietic stem cells can differentiate into hepatocytes in vivo. Nat Med. 6:1229-1234.
Larsson, J., Goumans, M.J., Sjostrand, L.J., van Rooijen, M.A., Ward, D., Leveen, P., Xu, X., ten Dijke, P., Mummery, C.L., and Karlsson, S. (2001). Abnormal angiogenesis but intact hematopoietic potential in TGF-beta type I receptor-deficient mice. EMBOJ. 20:1663-1673.
Lazar, A., Peshwa, M. V., Wu, F. J., Chi, C. M., Cerra, F. B., and Hu, W. S. (1995). Formation of porcine hepatocyte spheroids for use in a bioartificial liver. Cell Transplant 4:259-68.
Lee, S. H., Lumelsky, N., Studer, L., Auerbach, J. M., and McKay, R. D. (2000). Efficient generation of midbrain and hindbrain neurons from mouse ES cells. Nat Biotechnol 18:675-9.
Lewis, I. D., Almeida-Porada, G., Du, J., Lemischka, I. R., Moore, K. A., Zanjani, E. D., and VerfaiUie, C. M. (2001). Long-term repopulating cord blood stem cells are preserved after ex-vivo culture in a non-contact system. Blood 97:441- 9.
Li, C.X., and Poznansky, M.J. (1990). Characterization of the ZO-1 protein in endothelial and other cell lines. J Cell Sci. 2:231 -7. 97:231 -237. Li-Masters, T., and Morgan, E.T. 2001. Effects of bacterial lipopolysaccharide on Phenobarbital-induced CYP2B expression in mice. Drug
Metab Dispos 29:252-257.
Lin, Y., Weisdorf, D. J., Solovey, A., and Hebbel, R. P. (2000). Origins of circulating endothelial cells and endothelial outgrowth from blood. JClin Inves.t 105:71-7.
Liu, S., Qu, Y., Stewart, T. J., Howard, M. J., Chakrabortty, S., Holekamp, T. F., and McDonald, J. W. (2000). ES cells differentiate into oligodendrocytes and myelinate in culture and after spinal cord transplantation. Proc Natl Acad Sci USA 97:6126-31.
Mahley, R.W., and Ji, Z.S. (1999). Remnant lipoprotein metabolism: key pathways involving cell-surface heparan sulfate proteoglycans and apolipoprotein E. J LipidRes 40:1-16.
Martin, G.R. (1981). Isolation of a pluripotent cell line from early mouse embryos cultured in medium conditioned by teratocaracinoma stem cells. Proc Natl Acad Sci U.S.A. 12:7634-8.
Masinovsky, B., U.S. Patent No. 5,837,670
Mathon, N. F., Malcolm, D. S., Harrisingh, M. C, Cheng, L., and Lloyd, A. C. (2001). Lack of Replicative Senescence in Normal Rodent Glia. Science 291 :872- 875.
McGlave, et al, U.S. Patent No. 5,460,964
Meager, A. (1999). Cytokine regulation of cellular adhesion molecule expression in inflammation. Cytokine Growth Factor Rev. 10:27-39.
Medvinsky, A., and Dzierzak, E. (1996). Definitive hematopoiesis is autonomously initiated by the AGM region. Cell. 86:897.
Melton, D. (1997). Signals for tissue induction and organ formation in vertebrate embryos. Harvey Lect 93:49-64.
Mezey, E., Chandross, K. J., Harta, G., Maki, R.A., and McKercher, S. R. (2000). Turning Blood into Brain: Cells Bearing Neuronal Antigens Generated in vivo from Bone Marrow. Science 290: 1779- 1782.
Miyajima, A., Kinoshita, T., Tanaka, M., Kamiya, A., Mukouyama, Y., arid Hara, T. (2000). Role of Oncostatin M in hematopoiesis and liver development. Cytokine Growth Factor Rev 11 : 177-183. Morrison, S. J., White, P. M., Zock, C, and Anderson, D. J. (1999). Prospective identification isolation by flow cytometry and in vivo self-renewal of multipotent mammalian neural crest stem cells. Cell. 96:737-749.
Nichols, J., Zevnik, B., Anastassiadis, K., Niwa, H., Klewe-Nebenius, D., Chambers, I., Scholer, H., and Smith, A. (1998). Formation of pluripotent stem cells in the mammalian embryo depends on the POU transcription factor Oct 4. Cell 95:379-91.
Nishikawa, S., Nishikawa, S., Hirashima, M., Matsuyoshi, N., and Kodama, H. (1998). Progressive lineage analysis by cell sorting and culture identifies FLKI+VEcadherin+ cells at a diverging point of endothelial and hemopoietic lineages. Development. 125:1747-1757.
Nishikawa, S.I., Nishikawa, S., Kawamoto, H., Yoshida, H., Kizumoto, M., Kataoka, H. and Katsura, Y. (1998). In vitro generation of lymphohematopoietic cells from endothelial cells purified from murine embryos. Immunity. 8:761-769. Niwa, H., Miyazaki, J., and Smith, A. G. (2000). Quantitative expression of
Oct-3/4 defines differentiation, dedifferentiation or self-renewal of ES cells. Nat Genet 24:372-6.
Nolta, J., Dao, M., Wells, S., Smogorzewska, E., and Kohn, D. (1996). Transduction of pluripotent human HSCs demonstrated by clonal analysis after engraftment in immune-deficient mice. Proc Natl Acad Sci U S A 93 :2414-9.
Odorico, J. S., Kaufman, D. S., and Thomson, J. A. (2001). Multilineage differentiation from human ES cell lines. Stem Cells 19:193-204.
Oh, S.H., Miyazaki, M., Kouchi, H., Inoue, Y., Sakaguchi, M., Tsuji, T., Shima, N., Higashio, K., and Namba, M. (2000). Hepatocyte growth factor induces differentiation of adult rat bone marrow cells into a hepatocyte lineage in vitro. Biochem Biophys Res Commun 279:500-504.
Okabe, S., Forsberg-Nilsson, K., Spiro, A. C, Segal, M., and McKay,-R. D. (1996). Development of neuronal precursor cells and functional postmitotic neurons from ES cells in vitro. Mech Dev 59:89-102. O'Leary, D. D., and Wilkinson, D. G. (1999). Eph receptors and ephrins in neural development. CuffOpin Neurobiol 9:65-73.
Orkin, S. (1998). Embryonic stem cells and transgenic mice in the study of hematopoiesis. 7«t. J. Dev. Biol. 42:927-34. Orlic, D., Kajstura, J., Chimenti, S., Jakoniuk, I., Anderson, S. M., Li, B.,
Pickel, J., McKay, R., Nadal-Ginard, B., Bodine, D. M., Leri, A., and Anversa, P.
(2001). Bone marrow cells regenerate infarcted myocardium. Nature 410:701-5.
O'Shea, K. (1999). ES cell models of development. Anat Rec 15:32-41. Palmer, T. D., Markakis, E. A., Willhoite, A. R, Safar, F., and Gage, F. H.
(1999). Fibroblast growth factor-2 activates a latent neurogenic program in NSCs from diverse regions of the adult CNS. J Neurosci 19:8487-97.
Palmer, T. D., Takahashi, J., and Gage, F. H. (1997). The adult rat hippocampus contains primordial NSCs. Mol Cell Neurosci 8:389-404. Partanen, J., and D.J. Dumont. (1999). Functions of Tie 1 and Tie2 receptor tyrosine kinases in vascular development. Curr Top Microbiol Immunol. 237:159- 172.
Peault, B. 1996. Hematopoiedc stem cell emergence in embryonic life: developmental hematology revisited. J. Hematother. 5:369. Peichev, M., Naiyer, A.J., Pereira, D., Zhu, Z., Lane, W.J., Williams, M., Oz,
M.C., Hicklin, D.J., Witte, L., Moore, M.A., and Rafii, S. (2000). Expression of VEGFR 2 and AC 133 by circulating human CD34(+) cells identifies a population of functional endothelial precursors. Blood. 95:952-958.
Peshwa MV, WU FJ, Follstad BD, Cerra, F.B., and Hu, W.S. 1994. Kinetics of hepatocyte spheroid formation. Biotechnology Progress 10:460-466.
Petersen, B. E., Bowen, W. C, Patrene, K. D., Mars, W. M., Sullivan, A. K., Murase, N., Boggs, S. S., Greenberger, J. S., and Goff, J. P. (1999). Bone marrow as a potential source of hepatic oval cells. Science 284:1168-1170.
Petersen, B.E. 2001. Hepatic "stem" cells: coming full circle. Blood Cells Mol Dis 27:590-600.
Petersen, B.E., Bowen, W.C., Patrene, K.D., Mars, W.M., Sullivan, A.K., Murase, N., Boggs, S.S., Greenberger, J.S., and Goff, J.P. 1999. Bone marrow as a potential source of hepatic oval cells. Science 284:1168-1170.
Petzelbauer, P., Halama, T., and Groger, M. (2000). Endothelial adherens junctions. Jlnvestig Dermatol Symp Proc. 5:10-13.
Pittenger, M. F., Mackay, A. M., Beck, S. C, Jaiswal, R. K., Douglas, R., Mosca, J. D., Moorman, M. A., Simonetti, D. W., Craig, S., and Marshak, D. R. (1999). Multilineage potential of adult human MSCs. Science 284:143-147. Pittenger, M., U.S. Patent No. 5,827,740
Ploemacher, R. E., and Brons, N. H. (1988). Isolation of hemopoietic stem cell subsets from murine bone marrow: I. Radioprotective ability of purified cell suspensions differing in the proportion of day-7 and day- 12 CFU-S. Exp Hematol 16:21-6.
Potten, C. (1998). Stem cells in gastrointestinal epithelium: numbers, characteristics and death. Philos Trans R Soc LondB Biol Sci 353:821-30.
Prochazka, M., H.R. Gaskins, L.D. Shultz, and E.H. Leiter. (1992). The nonobese diabetic scid mouse: model for spontaneous thymomagenesis associated with immunodeficiency. Proc Natl Acad Sci USA. 89:3290-3294.
Rader, D.J., and Dugi, K.A. (2000). The endothelium and lipoproteins: insights from recent cell biology and animal studies. Semin Thromb Hemost 26:521-528.
Rafii, S., F. Shapiro, J. Rimarachin, R. Nachman, B. Ferris, B. Weksler, M. Moore, arid A. Asch. (1994). Isolation and characterization of human bone marrow microvascular endothelial cells: hematopoietic progenitor cell adhesion. Blood. 84:10-20.
Rafii, S., Shapiro, F., Pettengell, R., Ferris, B., Nachman, R., Moore, M., and Asch, A. (1995). Human bone marrow microvascular endothelial cells support long- term proliferation and differentiation of myeloid and megakaryocytic progenitors. Blood 86:3353-61.
Reinhardt, R. L., Khoruts, A., Merica, R., Zell, T., and Jenkins, M. K. (2001). Visualizing the generation of memory CD4 T cells in the whole body. Nature 401:101-105. Reubinoff, B. E., Pera, M. F., Fong, C. Y., Trounson, A., and Bongso, A.
(2000). ES cell lines from human blastocysts: somatic differentiation in vitro. Nat Biotech 18:399-404.
Reyes, M., and VerfaiUie, CM. (2001). Characterization of multipotent adult progenitor cells, a subpopulation of mesenchymal stem cells. Ann N Y Acad Sci 938:231-233; discussion 233-235.
Reyes, M., Lund, T., Lenvik, T., Aguiar, D., Koodie, L., and VerfaiUie, CM. (2001). Purification and ex vivo expansion of postnatal human marrow mesodermal progenitor cells. Blood. 98:2615-2625. Reynolds, B., and Weiss, S. (1992). Generation of neurons and astrocytes from isolated cells of the adult mammalian central nervous system. Science 255:1707-10.
Reynolds, B., and Weiss, S. (1996). Clonal and population analyses demonstrate that an EGF-responsive mammalian embryonic CNS precursor is a stem cell. Dev Biol 175:1-13
Ribatti, D., A. Vacca, B. Nico, L. Roncali, and F. Dammacco. (2001). Postnatal vasculogenesis. Mech Dev. 100:157-163.
Richards, L. J., Kilpatrick, T. J., and Bartlett, P. F. (1992). De novo generation of neuronal cells from the adult mouse brain. Proc Natl Acad Sci USA. 89:8591-5.
Rideout, W. M., 3rd, Wakayama, T., Wutz, A., Eggan, K., Jackson-Grusby, L., Dausman, J., Yanagimachi, R., and Jaenisch, R. (2000). Generation of mice from wild-type and targeted ES cells by nuclear cloning. Nat Genet 24:109-10. Robertson, S. M., Kennedy, M., Shannon, J. M., Keller, G. (2000). A transitional stage in the commitment of mesoderm to hematopoiesis requiring the transcription factor SCL/tal-1. Development. 11 :2447-59.
Rosenberg, J.B., P.A. Foster, R.J. Kaufman, E.A. Vokac, M. Moussalli, P.A. Kroner, and R.R. Montgomery. (1998). Intracellular trafficking of factor VIII to von Willebrand factor storage granules. J Clin Invest. 101 :613-624.
Rozga, J., Arnaout, W.S., and Demetriou, A.A. (2001). Isolation, characterization, -derived hepatocyte stem cells. Biochem Biophys Res Commun 288:156-164.
Ryder, E. F., Snyder, E. Y., and Cepko, C. L. (1990). Establishment and characterization of multipotent neural cell lines using retrovirus vector-mediated oncogene transfer. JNeurobiol 21 :356-375.
Sah, D. W., Ray, J., and Gage, F. H. (1997). Regulation of voltage- and ligand-gated currents in rat hippocampal progenitor cells in vitro. JNeurobiol 32:95- 110. Sanchez-Ramos, J., Song, S., Cardozo-Pelaez, F., Hazzi, C, Stedeford, T.,
Willing, A., Freeman, T. B., Saporta, S., Janssen, W., Patel, N., Cooper, D. R., and Sanberg, P. R. (2000). Adult bone marrow stromal cells differentiate into neural cells in vitro. Exp Neurol. 164:247-56. Saucedo-Cardenas, O., Quintana-Hau, J. D., Le, W. D., Smidt, M. P., Cox, J.
J., De Mayo, F., Burbach, J. P., and Conneely, O. M. (1998). Nurrl is essential for the induction of the dopaminergic phenotype and the survival of ventral mesencephalic late dopaminergic precursor neurons. Proc Natl Acad Sci USA 95: 4013-8.
Scherf, U., D.T. Ross, M. Waltham, L.H. Smith, J.K. Lee, L. Tanabe, K.W. Kohn, W.C. Reinhold, T.G. Myers, D.T. Andrews, D.A. Scudiero, M.B. Eisen, E.A. Sausville, Y. Pommier, D. Botstein, P.O. Brown, and J.N. Weinstein. (2000). A gene expression database for the molecular phafmacology of cancer. Nat Biotech. 24:236-244.
Scholer, H. R., Hatzopoulos, A. K, Balling, R., Suzuki, N., and Gruss, P. (1989). A family of octamer-specific proteins present during mouse embryogenesis: evidence for germline-specific expression of an Oct factor. EMBO J 8:2543-50.
Schuldiner, M., Yanuka, O., Itskovitz-Eldor, J., Melton, D. A., and Benvenisty, N. (2000). From the cover: effects of eight growth factors on the differentiation of cells derived from human ES cells. Proc Natl Acad Sci USA 97:11307-12.
Schwartz, et al, U.S. Patent No. ,759,793
Seglen, P.O. (1976). Preparation of isolated rat liver cells. Methods Cell Biol 13:29-83.
Shamblott, M., Axelman, J., Wang, S., Bugg, E., Littlefield, J., Donovan, P., Blumenthal, P., Huggins, G., Gearhart, J.: (1998) Derivation of pluripotent stem cells from cultured human primordial germ cells. Proc. Natl. Acad. Sci. U.S.A. 95:13726-31. Shen, C.N., Slack, J.M., and Tosh, D. (2000). Molecular basis of transdifferentiation of pancreas to liver. Nat Cell Biol. 2:879-887.
Shi, Q., S. Rafii, M. Hong-De Wu, E.S. Wijelath, C. Yu, A. Ishida, Y. Fujita, S. Kothari, R. Mohle, L.R. Sauvage, M.A.S. Moore, R.F. Storb, and W.P. Hammond. (1998). Evidence for circulating bone marrow-derived endothelial cells. Blood. 92:362-367.
Shih, C.C, Y. Weng, A. Mamelak, T. LeBon, M.C Hu, and S. Forman. (2001). Identification of a candidate human neurohematopoietic stem-cell population. Blood. 98:2412-2422. Simeone, A. (1998). Otxl and Otx2 in the development and evolutionof the mammalian brain. EMBO 117:6790-8.
Simmons, P., et al, U.S. Patent No. 5,677,136
Soule HD, et al. (1973) A human cell line from a pleural effusion derived from a breast carcinoma. J Natl Cancer Inst; 51 (5): 1409-16.
Southern, P. J., Blount, P., and Oldstone, M. B. (1984). Analysis of persistent vims infections by in situ hybridization to whole-mouse sections. Nature 312:555-8.
Steeber, D.A., and T. Tedder, F. (2001). Adhesion molecule cascades direct lymphocyte recirculation and leukocyte migration during inflammation. Immunol Res. 22:299-317.
Steinberg, D., Pittman, R.C. and Carew, T.E. (1985). Mechanisms involved in the uptake and degradation of low density lipoprotein by the artery wall in vivo. Ann N Y Acad Sci. 454:195-206. Studer, L., Spenger, C, Seiler, R., Othberg, A., Lindvall, O., and Odin, P.
(1996). Effects of brain-derived neurotrophic factor on neuronal structure of dopaminergic neurons in dissociated cultures of human fetal mesencephalon. Exp Brain Res 108:328-36.
Suhonen, J., Peterson, D., Ray, J., and Gage, F. (1996). Differentiation of adult hippocampus-derived progenitors into olfactory neurons in vivo. Nature 383:624-7.
Svendsen, C. N., and Caldwell, M. A. (2000). NSCs in the developing central nervous system: implications for cell therapy through transplantation. Prog Brain Res. 127:13-34. Svendsen, C. N., Caldwell, M. A., Ostenfeld, T. (1999). Human neural stem cells: Isolation, expansion and transplantation. Brain Path 9:499-513.
Tang, D. G., Tokumoto, Y. M., Apperly, J. A., Lloyd, A. C, and Raff, M. C (2001). Lack of replicative senescence in cultured rat oligodendrocyte precursor cells. Science 291 :868-71. Tedder, T., Steeber, D., Chen, A., and Engel, P. (1995). The selections: vascular adhesion molecules. FASEB J. 9:866. Theise, N. D., Badve, S., Saxena, R., Henegariu, O., Sell, S., Crawford, J.
M., and Krause, D. S. (2000). Derivation of hepatocytes from bone marrow cells in mice after radiation-induced myeloablation. Hepatology 31 :235-40.
Theise, N.D., Saxena, R., Portmann, B.C., Thung, S.N., Yee, H., Chiriboga, L., Kumar, A., and Crawford, J.M. (1999). The canals of Hering and hepatic stem cells in humans. Hepatology 30:1425-1433.
Thomson, J. A., Itskovitz-Eldor, J., Shapiro, S. S., Waknitz, M. A., Swiergiel, J. J., Marshall, V. S., and Jones, J. M. (1998). ES cell lines derived from human blastocysts. Science 282: 114-7. Thomson, J., Kalisman J., Golos, J., Durning, M., Harris, C, Becker, R.,
Hearn, J. (1995) Isolation of a primate embryonic stem cell line. Proc. Natl Acad. Sci. U.S.A. 92:7844-8,
Trupp, M., Arenas, E., Fainzilber, M., Nilsson, A. S., Sieber, B. A., Grigoriou, M., Kilkenny, C, Salazar-Grueso, E., Pachnis, V., and Arumae, U. (1996). Functional receptor for GDNF encoded by the c-ret proto-oncogene. Nature 381 :785-9.
Tsai, R.Y. and McKay, R.D. (2000). Cell contact regulates fate choice by cortical stem cells. J. Neurosci. 20:3725-35.
Tsukamoto, et al, U.S. Patent No. 5,750,397 Tsukamoto, et al, U.S. Patent No. 5,716,827
Tzanakakis, E.S., Hansen, L.K., and Hu, W.S. (2001). The role of actin filaments and microtubules in hepatocyte spheroid self-assembly. Cell Motil Cytoskeleton 48:175-189.
Tzanakakis, E.S., Hsiao, C.C., Matsushita, T., Remmel, R.P., and Hu, W.S. (2001). Probing enhanced cytochrome P450 2B1/2 activity in rat hepatocyte spheroids through confocal laser scanning microscopy. Cell Transplant. 10:329342.
Uchida, N., Buck, D.W., He, D., Reitsma, M.J., Masek, M., Phan, T.V., Tsukamoto, A.S., Gage, F.H., and Weissman, I.L. (2000). Direct isolation of human central nervous system stem cells. Proc Natl Acad Sci USA. 97:14720-14725. Van Rijen, H., van Kempen, M.J., Analbers, L.J., Rook, M.B., van
Ginneken, A.C, Gros, D., and Jongsma, H.J. (1997). Gap junctions in human umbilical cord endothelial cells contain multiple connexins. Am J Physiol. 272:C117-130. VerfaiUie, C, Miller, W., Boylan, K., McGlave, P. (1992). Selection of benign primitive hematopoietic progenitors in chronic myelogenous leukemia on the basis of HLA-DR antigen expression. Blood. 79:1003-1010.
Vescovi, A. L., Paraati, E. A., Gritti, A., Poulin, P., Ferrario, M., Wanke, E., Frolichsthal-Schoeller, P., Cova, L., Arcellana-Panlilio, M., Colombo, A., and Galli, R. (1999). Isolation and cloning of multipotential stem cells from the embryonic human CNS and establishment of transplantable human NSC lines by epigenetic stimulation. Exp Neurol 156:71-83.
Vescovi, A., Reynolds, B., Fraser, D., and Weiss, S. (1993). bFGF regulates the proliferative fate of unipotent (neuronal) and bipotent (neuronal/astroglial) EGF- generated CNS progenitor cells. Neuron 11 : 951-66.
Vischer, U.M., H. Barth, and C.B. Wollheim. (2000). Regulated von Willebrand factor secretion is associated with agonist-specific patterns of cytoskeletal remodeling in cultured endothelial cells. Arterioscler Thromb Vase Biol. 20:883-891.
Wagner, D.D., Olmsted, J.B., and Marder, V.J. (1982). Immunolocalization of von Willebrand protein in Weibel-Palade bodies of human endothelial cells. J. Cell Biol. 95:355-360.
Wagner, J., Akerud, P., Castro, D. S., Holm, P. C, Canals, J. M., Snyder, E. Y., Perlmann, T., and Arenas, E. (1999). Induction of a midbrain dopaminergic phenotype in Nurrl-overexpressing NSCs by type 1 astrocytes. Nat Biotech 17:653- 9.
Wakitani, S., Saito, T., and Caplan, A. (1995). Myogenic cells derived from rat bone marrow MSCs exposed to 5-azacytidine. Muscle Nerve 18:1417-26. Wang, X., AI-Dhalimy, M., Lagasse, E., Finegold, M., and Grompe, M.
(2001). Liver repopulation and correction of metabolic liver disease by transplanted adult mouse pancreatic cells. Am JPathol 158:571-579.
Watt, F. (1997). Epidermal stem cells: markers patterning and the control of stem cell fate. Philos Trans R Soc LondB Biol Sci 353: 831-6. Watt, S., Gschmeissner, S., and Bates,P. (1995). PECAM-1 : its expression and function as a cell adhesion molecule on hemopoietic and endothelial cells. Leuk Lymph. 17:229. Weiss, M. J., Orkin, S. H. (1995) GATA transcription factors: key regulators of hematopoiesis. Exp Hematol. 2:99-107.
Weissman, I. L. (2000). Translating stem and progenitor cell biology to the clinic: barriers and opportunities. Science 287:1442-6. Wells, J. M., and Melton, D. A. (2000). Early mouse endoderm is patterned by soluble factors from adjacent germ layers. Development. 127:1563-72.
Wells, J.M., and Melton, D.A. (1999). Vertebrate endoderm development. Annu Rev Cell Dev Biol 15:393-410.
Whittemore, S. R., Morassutti, D. J., Walters, W. M., Liu, R. H., and Magnuson, D. S. (1999). Mitogen and substrate differentially affect the lineage restriction of adult rat subventricular zone neural precursor cell populations. Exp Cell Res 252:75-95.
Williams, R. L., Hilton, D. J., Pease, S., Willson, T. A., Stewart, C If, Gearing, D. P., Wagner, E. F., Metcalf, D., Nicola, N. A., and Gough, N. M. (1988). Myeloid leukemia inhibitory factor maintains the developmental potential of ES cells. Nature 336:684-7.
Wilmut, I., Schnieke, A. E., McWhir, J., Kind, A. J., and Campbell, K. H. (1997). Viable offspring derived from fetal and adult mammalian cells. Nature 385:810-3. Woodbury, D., Schwarz, E. J., Prockop, D. J., and Black, I. B. (2000). Adult rat and human bone marrow stromal cells differentiate into neurons. J Neurosci Res 15:364-70.
Yamashita, J., Itoh, H., Hirashima, M., Ogawa, M., Nishikawa, S., Yurugi, T., Naito, M., Nakao, K, and Nishikawa, S. (2000). Flkl-positive cells derived from ES cells serve as vascular progenitors. Nature. 408:92-96.
Yang, J., Nagavarapu, U., Relloma, K., Sjaastad, M.D., Moss, W.C, Passaniti, A., and Herron, G.S. (2001). Telomerized human microvasculature is functional in vivo. Nat Biotechnol. 19:219-224.
Ye, W., Shimamura, K., Rubenstein, J., Hynes, M., and Rosenthal, A. (1998). FGF and Shh signals control dopaminergic and serotonergic cell fate in the anterior neural plate. Cell 93:755-66. Yoneya, T., Tahara, T., Nagao, K., Yamada, Y., Yamamoto, T., Osawa, M., Miyatani, S., and Nishikawa, M. (2001). Molecular cloning of delta-4, a new mouse and human Notch ligand. J Biochem. 129:27-34.
Yoo, J. U., Barthel, T. S., Nishimura, K., Solchaga, L., Caplan, A. I., Goldberg, V. M., Johnstone, B. (1998). Then chondrogenic potential of human bone-marrow-derived mesenchymal progenitor cells. J Bone Joint SurgAm. 12:1745-57.
Young, H., et al, U.S. Patent No. 5,827,735
Zambrowicz, B. P., imamoto, A., Hering, S., Herzenberg, L. A., Kerr, W. G., and Soriano, P. (1997). Dismption of overlapping transcripts in the ROSA beta geo 26 gene trap strain leads to widespread expression of beta-galactosidase in mouse embryos and hematopoietic cells. Proc Natl Acad Sci USA. 94:3789-94.
Zaret, K.S. (2000). Liver specification and early morphogenesis. Mech Dev 92:83- 88. Zaret, K.S. (2001). Hepatocyte differentiation: from the endoderm and beyond. Curr Opin Genet Dev. 11 :568-574.
Zelko, I., and Negishi, M. (2000). Phenobarbital-elicited activation of nuclear receptor CAR in induction of cytochrome P450 genes. Biochem Biophys Res Commun. 277:1-6. Zhao, R. C. H., Jiang, Y., and VerfaiUie, C. M. (2000). A model of human p210BCW"BL mediated CML by transducing primary normal human CD34+ cells with a BCR/ABL containing retroviral vector. Blood. 97:2406-12.
Ziegler, B., M. Valtieri, G. Porada, R. De Maria, R. Muller, B. Masella, M. Gabbianelli, I. Casella, E. Pelosi, T. Bock, E. Zanjani, and C. Peschle. (1999). KDR Receptor: A Key Marker Defining HSCs. Science. 285:1553 1558.

Claims

WHAT IS CLAIMED IS:
1. An isolated multipotent adult stem cell (MASC), wherein the cell has the capacity to be induced to differentiate to form at least one differentiated cell type of mesodermal, ectodermal and endodermal origin.
2. The cell of claim 1, wherein said cell is derived from a non- embryonic organ or tissue of a mammal.
3. The cell of claim 1, wherein the cell has the capacity to be induced to differentiate to form cells selected from the group consisting of osteoblast, chondrocyte, adipocyte, fibroblast, marrow stroma, skeletal muscle, smooth muscle, cardiac muscle, occular, endothelial, epithelial, hepatic, pancreatic, hematopoietic, glial, neuronal and oligodendrocyte cell type.
4. The cell of claim 1, wherein the organ or tissue is selected from the group consisting of bone marrow, muscle, brain, umbilical cord blood and placenta.
5. The cell of claim 2, wherein the mammal is a mouse.
6. The cell of claim 2, wherein the mammal is a rat.
7. The cell of claim 2, wherein the mammal is a human.
8. The cell of claim 1, wherein differentiation is induced in vivo or ex vivo.
9. The cell of claim 3, wherein differentiation is induced in vivo or ex vivo.
10. The cell of claim 1, wherein the cell constitutively expresses oct4 and high levels of telomerase.
11. The cell of claim 10, wherein the cell is negative for CD44, MHC class I and MHC class II expression.
12. A method of creating a normal non-human animal comprising the steps of:
(a) introducing the cell of claim 1 into a blastocyst;
(b) implanting the blastocyst of (a) into a surrogate mother; and
(c) allowing the pups to develop and be bom.
13. The animal of claim 12, wherein said animal is chimeric.
14. A composition comprising a population of MASC and a culture medium, wherein the culture medium expands the MASC.
15. The composition of claim 14, wherein the medium comprises epidermal growth factor (EGF) and platelet derived growth factor (PDGF).
16. The composition of claim 15, wherein the medium further comprises leukemia inhibitory factor (LIF).
17. A composition comprising a population of fully or partially purified
MASC progeny.
18. The composition of claim 17, wherein the progeny have the capacity to be further differentiated.
19. The composition of claim 17, wherein the progeny are terminally differentiated.
20. The composition of claim 17, wherein the progeny are of the osteoblast, chondrocyte, adipocyte, fibroblast, marrow stroma, skeletal muscle, smooth muscle, cardiac muscle, occular, endothelial, epithelial, hepatic, pancreatic, hematopoietic, glial, neuronal or oligodendrocyte cell type.
21. A method for isolating and propagating the cell of claim 1 comprising the steps of:
(a) obtaining tissue from a mammal;
(b) establishing a population of adherent cells;
(c) depleting said population of CD45+ cells; (d) recovering CD45" cells; and
(e) culturing CD45" cells under expansion conditions to produce an expanded cell population.
22. An expanded cell population obtained by the method of claim 21.
23. A method for differentiating MASC ex vivo comprising the steps of claim 21 and further comprising culturing the propagated cells in the presence of desired differentiation factors.
24. The method of claim 23, wherein the differentiation factors are selected from the group consisting of basic fibroblast growth factor (bFGF); vascular endothelial growth factor (VEGF); dimethylsulfoxide (DMSO) and isoproterenol; and, fibroblast growth factor4 (FGF4) and hepatocyte growth factor (HGF).
25. A differentiated cell obtained by the method of claim 23.
26. The differentiated cell of claim 25, wherein the cell is ectoderm, mesoderm or endoderm.
27. The differentiated cell of claim 25, wherein the cell is of the osteoblast, chondrocyte, adipocyte, fibroblast, marrow stroma, skeletal muscle, smooth muscle, cardiac muscle, occular, endothelial, epithelial, hepatic, pancreatic, hematopoietic, glial, neuronal or oligodendrocyte cell type.
28. A method for differentiating MASC in vivo comprising the steps of claim 21 and further comprising administering the expanded cell population to a mammalian host, wherein said cell population is engrafted and differentiated in vivo in tissue specific cells, such that the function of a cell or organ, defective due to injury, genetic disease, acquired disease or iatrogenic treatments, is augmented, reconstituted or provided for the first time.
29. The method of claim 28, wherein the tissue specific cells are of the osteoblast, chondrocyte, adipocyte, fibroblast, marrow stroma, skeletal muscle, smooth muscle, cardiac muscle, occular, endothelial, epithelial, hepatic, pancreatic, hematopoietic, glial, neuronal or oligodendrocyte cell type.
30. The method of claim 28, wherein the MASC undergo self-renewal in vivo.
31. The method of claim 28, wherein cells are administered in conjunction with a pharmaceutically acceptable matrix.
32. The method of claim 31 , wherein the matrix is biodegradable.
33. The method of claim 28, wherein administration is via localized injection, systemic injection, parenteral administration, oral administration, or intrauterine injection into an embryo.
34. The method of claim 33, wherein localized injection comprises catheter administration.
35. The method of claim 28, wherein the disease is selected from the group consisting of cancer, cardiovascular disease, metabolic disease, liver disease, diabetes, hepatitis, hemophilia, degenerative or traumatic neurological conditions, autoimmune disease, genetic deficiency, connective tissue disorders, anemia, infectious disease and transplant rejection.
36. A differentiated cell obtained by the method of claim 28.
37. A method of treatment comprising administering to a patient in need thereof a therapeutically effective amount of the cell of claim 11.
38. The method of claim 37, wherein no teratomas are formed in the patient.
39. A method of treatment comprising administering to a patient in need thereof a therapeutically effective amount of MASC or their progeny.
40. The method of claim 39, wherein reduced or no pretreatment of the patient is required.
41. The method of claim 40, wherein pretreatment comprises myeloablation via irradiation or chemotherapy.
42. The method of claim 39, wherein it is unnecessary to induce tolerance prior to or simultaneous with administration of MASC or their progeny.
43. The method of claim 39, wherein post immunosuppressive treatment of the patient is reduced compared with traditional pharmacological doses.
44. The method of claim 39, wherein the progeny have the capacity to be further differentiated.
45. The method of claim 39, wherein the progeny are terminally differentiated.
46. The method of claim 39, wherein the MASC or their progeny are administered via localized injection, systemic injection, parenteral administration, oral administration, or intrauterine injection into an embryo.
47. The method of claim 46, wherein localized injection comprises catheter administration.
48. The method of claim 39, wherein cells are administered in conjunction with a pharmaceutically acceptable matrix.
49. The method of claim 48, wherein the matrix is biodegradable.
50. The method of claim 39, wherein the MASC or their progeny alter the immune system to resist viral, bacterial or fungal infection.
51. The method of claim 39, wherein the MASC or their progeny augment, reconstitute or provide for the first time the function of a cell or organ defective due to injury, genetic disease, acquired disease or iatrogenic treatments.
52. The method of claim 51, wherein the organ is selected from the group consisting of bone marrow, blood, spleen, liver, lung, intestinal tract, eye, brain, immune system, circulatory system, bone, connective tissue, muscle, heart, blood vessels, pancreas, central nervous system, peripheral nervous system, kidney, bladder, skin, epithelial appendages, breast-mammary glands, fat tissue, and mucosal surfaces including oral esophageal, vaginal and anal.
53. The method of claim 51 , wherein the MASC undergo self-renewal in vivo.
54. The method of claim 51, wherein the disease is selected from the group consisting of cancer, cardiovascular disease, metabolic disease, liver disease, diabetes, hepatitis, hemophilia, degenerative or traumatic neurological conditions, autoimmune disease, genetic deficiency, connective tissue disorders, anemia, infectious disease and transplant rejection.
55. The method of claim 44, wherein the progeny are differentiated ex vivo or in vivo.
56. The method of claim 45, wherein the progeny are differentiated ex vivo or in vivo.
57. The method of claim 45, wherein the progeny are selected from the group consisting of osteoblasts, chondrocytes, adipocytes, fibroblasts, marrow stroma, skeletal muscle, smooth muscle, cardiac muscle, occular endothelial, epithelial, hepatic, pancreatic, hematopoietic, glial, neuronal and oligodendrocytes.
58. The method of claim 39, wherein the MASC or their progeny home to one or more organs in the patient and are engrafted therein such that the function of a cell or organ, defective due to injury, genetic disease, acquired disease or iatrogenic treatments, is augmented, reconstituted or provided for the first time.
59. The method of claim 58, wherein the disease is selected from the group consisting of cancer, cardiovascular disease, metabolic disease, liver disease, diabetes, hepatitis, hemophilia, degenerative or traumatic neurological conditions, autoimmune disease, genetic deficiency, connective tissue disorders, anemia, infectious disease and transplant rejection.
60. The method of claim 58, wherein the injury is ischemia or inflammation.
61. The method of claim 58, wherein the organ is selected from the group consisting of bone marrow, blood, spleen, liver, lung, intestinal tract, eye, brain, immune system, circulatory system, bone, connective tissue, muscle, heart, blood vessels, pancreas, central nervous system, peripheral nervous system, kidney, bladder, skin, epithelial appendages, breast-mammary glands, fat tissue, and mucosal surfaces including oral esophageal, vaginal and anal.
62. The method of claim 58, wherein the MASC undergo self-renewal in vivo.
63. The method of claim 39, wherein the MASC or their progeny enhance angiogenesis.
64. The method of claim 39, wherein the MASC or their progeny are genetically transformed to deliver a therapeutic agent.
65. The method of claim 64, wherein the therapeutic agent is an antiangiogenic agent.
66. The method of claim 39, wherein administration is via a three dimensional matrix comprising an artificial vein.
67. The method of claim 66, wherein the treatment is directed to abdominal aortic aneurysm, cardiac bypass surgery, peripheral vascular disease or coronary vascular disease.
68. A therapeutic composition comprising MASC and a pharmaceutically acceptable carrier, wherein the MASC are present in an amount effective to produce tissue selected from the group consisting of bone marrow, blood, spleen, liver, lung, intestinal tract, eye, brain, immune system, bone, connective tissue, muscle, heart, blood vessels, pancreas, central nervous system, kidney, bladder, skin, epithelial appendages, breast-mammary glands, fat tissue, and mucosal surfaces including oral esophageal, vaginal and anal.
69. A therapeutic method for restoring organ, tissue or cellular function to a patient in need thereof comprising the steps of: (a) removing MASC from a mammalian donor;
(b) expanding MASC to form an expanded population of undifferentiatied cells; and
(c) adminstering the expanded cells to the patient, wherein organ, tissue or cellular function is restored.
70. The method of claim 69, wherein the function is enzymatic.
71. The method of claim 69, wherein the function is genetic.
72. The method of claim 69, wherein the mammalian donor is the patient.
73. The method of claim 69, wherein the organ, tissue or cell is selected from the group consisting of bone marrow, blood, spleen, liver, lung, intestinal tract, eye, brain, immune system, bone, connective tissue, muscle, heart, blood vessels, pancreas, central nervous system, peripheral nervous system, kidney, bladder, skin, epithelial appendages, breast-mammary glands, fat tissue, and mucosal surfaces including oral esophageal, vaginal and anal.
74. A method of inhibiting the rejection of a heterologous MASC transplanted into a patient comprising the steps of:
(a) introducing into the MASC, ex vivo, a nucleic acid sequence encoding the recipient's MHC antigens operably linked to a promotor, wherein the MHC antigens are expressed by the MASC; and
(b) transplanting the MASC into the patient, wherein MHC antigens are expressed at, a level sufficient to inhibit the rejection of the transplanted MASC.
75. The method of claim 74, wherein the patient is of the same species or another mammalian species as the donor of the MASC.
76. The method of claim 74, wherein the MASC are transplanted into the patient via localized injection, systemic injection, parenteral administration, oral administration, or intrauterine injection into an embryo.
77. The method of claim 76, wherein localized injection comprises catheter administration.
78. The method of claim 74, wherein cells are transplanted in conjunction with a pharmaceutically acceptable matrix.
79. The method of claim 78, wherein the matrix is biodegradable.
80. A method of inhibiting the rejection of a heterologous MASC transplanted into a patient comprising the steps of:
(a) transgenically knocking out expression of MHC antigens in the MASC; and
(b) transplanting the transgenic MASC into the patient, wherein said MHC antigens are not expressed by the MASC such that rejection of the transplanted MASC is inhibited.
81. The method of claim 80, wherein the patient is of the same species or another mammalian species as the donor of the MASC.
82. The method of claim 80, wherein the MASC are transplanted into the patient via localized injection, systemic injection, parenteral administration, oral administration, or intrauterine injection into an embryo.
83. The method of claim 82, wherein localized injection comprises catheter administration.
84. The method of claim 80, wherein cells are transplanted in conjunction with a pharmaceutically acceptable matrix.
85. The method of claim 84, wherein the matrix is biodegradable.
86. A method of generating blood or individual blood components ex vivo comprising the steps of:
(a) isolating MASC; and
(b) differentiating the MASC to form blood or blood components.
87. The method of claim 86, wherein the individual blood components are red blood cells, white blood cells or platelets.
88. A method of drug discovery comprising the steps of:
(a) analyzing the genomic or proteomic makeup of MASC or their progeny; (b) employing analysis thereof via bioinformatics and/or computer analysis using algorithms; and (c) assembling and comparing new data with known databases to discover new drugs.
89. A method of identifying the components of a differentiation pathway comprising the steps of:
(a) analyzing the genomic or proteomic makeup of MASC; (b) inducing differentiation of MASC;
(c) analyzing the genomic or proteomic makeup of intermediary cells in the differentiation pathway;
(d) analyzing the genomic or proteomic makeup of terminally differentiated cells in the differentiation pathway; (e) using bioinformatics and/or algorithms to characterize the genomic or proteomic makeup of MASC and their progeny; and (f) comparing the data obtained in (e) to identify the components of the pathway.
90. The method of claim 89, wherein the differentiation occurs in vitro.
91. The method of claim 89, wherein the differentiation occurs in vivo.
92. A method for comparing differentiation in vitro with differentiation in vivo comprising comparing the results of the method of claim 90 with the results of the method of claim 91.
93. A method of identifying the molecular components of disease or injury comprising the steps of: (a) analyzing the genomic or proteomic makeup of MASC isolated from a healthy donor;
(b) analyzing the genomic or proteomic makeup of MASC isolated from a donor afflicted with the disease or injury;
(c) using bioinformatics and/or algorithms to characterize the data
Figure imgf000105_0001
(d) using bioinformatics and/or algorithms to characterize the data
Figure imgf000105_0002
(e) comparing the data obtained in (c) with that obtained in (d) to identify the molecular components of the disease or injury.
94. A method of generating products in vitro that have therapeutic, diagnostic or research utility comprising the steps of:
(a) identifying the products in MASC; and
(b) isolating the products from MASC.
95. The method of claim 94 wherein the products are selected from the group consisting of proteins, lipids, complex carbohydrates, DNA and RNA.
96. A method of inducing, in a mammal, tolerance to an antigen administered to said mammal, the method comprising the step of administering to said mammal, after or simultaneously with the administration of said antigen, an effective amount of MASC or their progeny so that said mammal's humoral immune response to a subsequent challenge with said antigen is suppressed.
97. A method for removing toxins from the blood of a patient comprising contacting blood ex vivo with MASC derived cells, wherein said cells line a hollow, fiber based device.
98. The method of claim 97 wherein the cells are kidney or liver cells.
99. A method for delivering therapeutic products to a patient comprising contacting the blood of said patient ex vivo with MASC or their progeny, wherein said MASC or their progeny are genetically transformed to deliver a therapeutic agent.
100. A method for testing the toxicity of a d g comprising contacting MASC or their progeny ex vivo with said dmg and monitoring cell survival.
101. The method of claim 100, wherein the progeny are selected from the group consisting of hepatic, endothelial, epithelial and kidney.
PCT/US2002/004652 1999-08-05 2002-02-14 Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof WO2002064748A2 (en)

Priority Applications (20)

Application Number Priority Date Filing Date Title
CA2438501A CA2438501C (en) 2001-02-14 2002-02-14 Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
NZ527527A NZ527527A (en) 2001-02-14 2002-02-14 Mammalian multipotent adult stem cells (MASC) with the capacity to differentiate into cells of mesodermal, ectodermal or endodermal origin and uses thereof
IL15733202A IL157332A0 (en) 2001-02-14 2002-02-14 Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
US10/467,963 US7838289B2 (en) 2001-02-14 2002-02-14 Assay utilizing multipotent adult stem cells
EP02718998A EP1367899A4 (en) 2001-02-14 2002-02-14 Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
JP2002565063A JP2004529621A (en) 2001-02-14 2002-02-14 Pluripotent adult stem cells, their origin, methods of obtaining and maintaining them, methods of differentiating them, methods of their use, and cells derived therefrom
IL157332A IL157332A (en) 2001-02-14 2003-08-11 Method for providing cell population from umbilical cord blood or placenta which can differentiate into cell types of the embryonic lineage
IL214623A IL214623A (en) 2001-02-14 2003-08-11 Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof. methods of use thereof and cells derived therefrom
ZA2003/06289A ZA200306289B (en) 2001-02-14 2003-08-13 Multipotent adult stem cells sources thereof methods of obtaining and maintaining same methods of differentiation thereof methods of use thereof and cells derived thereof
US11/084,809 US20050283844A1 (en) 2001-02-14 2005-03-21 Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
US11/587,511 US8609412B2 (en) 1999-08-05 2005-04-21 Mapc generation of lung tissue
US11/151,689 US8075881B2 (en) 1999-08-05 2005-06-13 Use of multipotent adult stem cells in treatment of myocardial infarction and congestive heart failure
US11/269,736 US8147824B2 (en) 1999-08-05 2005-11-09 Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
US11/446,560 US7927587B2 (en) 1999-08-05 2006-06-02 MAPC administration for the treatment of lysosomal storage disorders
US12/093,159 US9962407B2 (en) 1999-08-05 2006-11-09 Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
US13/042,205 US20110177595A1 (en) 2001-02-14 2011-03-07 Multipotent Adult Stem Cells, Sources Thereof, Methods of Obtaining and Maintaining Same, Methods of Differentiation Thereof, Methods of Use Thereof and Cells Derived Thereof
US13/105,372 US8252280B1 (en) 1999-08-05 2011-05-11 MAPC generation of muscle
IL214623A IL214623A0 (en) 2001-02-14 2011-08-11 Method for providing cell population from umbilical cord blood or placenta
US13/301,186 US9526747B2 (en) 1999-08-05 2011-11-21 Use of multipotent adult stem cells in treatment of myocardial infarction and congestive heart failure
US13/345,036 US9808485B2 (en) 1999-08-05 2012-01-06 Immunomodulatory properties of multipotent adult progenitor cells and uses thereof

Applications Claiming Priority (8)

Application Number Priority Date Filing Date Title
US26878601P 2001-02-14 2001-02-14
US60/268,786 2001-02-14
US26906201P 2001-02-15 2001-02-15
US60/269,062 2001-02-15
US31062501P 2001-08-07 2001-08-07
US60/310,625 2001-08-07
US34338601P 2001-10-25 2001-10-25
US60/343,386 2001-10-25

Related Child Applications (9)

Application Number Title Priority Date Filing Date
PCT/US2000/021387 Continuation-In-Part WO2001011011A2 (en) 1999-08-05 2000-08-04 Multipotent adult stem cells and methods for isolation
US10/467,963 A-371-Of-International US7838289B2 (en) 1999-08-05 2002-02-14 Assay utilizing multipotent adult stem cells
US10467963 A-371-Of-International 2002-02-14
US10/048,757 Continuation-In-Part US7015037B1 (en) 1999-08-05 2002-08-21 Multiponent adult stem cells and methods for isolation
US96344404A Continuation-In-Part 1999-08-05 2004-10-11
US10/587,511 Continuation-In-Part US20070149331A1 (en) 2004-01-30 2005-01-28 Power transmission chain, manufacture method thereof and power transmission assembly
US11/084,809 Continuation US20050283844A1 (en) 2001-02-14 2005-03-21 Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
US11/446,560 Continuation-In-Part US7927587B2 (en) 1999-08-05 2006-06-02 MAPC administration for the treatment of lysosomal storage disorders
US12/907,495 Continuation US10638734B2 (en) 1999-08-05 2010-10-19 Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof

Publications (4)

Publication Number Publication Date
WO2002064748A2 true WO2002064748A2 (en) 2002-08-22
WO2002064748A8 WO2002064748A8 (en) 2003-04-24
WO2002064748A3 WO2002064748A3 (en) 2003-08-21
WO2002064748A9 WO2002064748A9 (en) 2006-03-30

Family

ID=27500956

Family Applications (1)

Application Number Title Priority Date Filing Date
PCT/US2002/004652 WO2002064748A2 (en) 1999-08-05 2002-02-14 Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof

Country Status (6)

Country Link
US (3) US7838289B2 (en)
EP (2) EP1367899A4 (en)
JP (1) JP2004529621A (en)
CA (1) CA2438501C (en)
IL (4) IL157332A0 (en)
WO (1) WO2002064748A2 (en)

Cited By (55)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
WO2004011012A2 (en) * 2002-07-29 2004-02-05 Asahi Kasei Kabushiki Kaisha Stem cells for treating pancreatic damage
WO2004087896A2 (en) * 2003-03-31 2004-10-14 Pfizer Products Inc. Hepatocyte differentiation of stem cells
WO2005001072A1 (en) 2003-06-23 2005-01-06 Fraunhofer Gesellschaft Zur Förderung Der Angewandten Forschung E. V. Isolated pluripotent adult stem cells and methods for isolating and cultivating the same
WO2005059113A1 (en) * 2003-12-19 2005-06-30 Omnicyte Ltd Stem cells
EP1572949A2 (en) * 2002-06-07 2005-09-14 The Regents Of The University Of California Maintenance of islet cells
WO2005095588A1 (en) * 2004-03-31 2005-10-13 Kyoto University Cortex glutamatergic neuron precursor providing cortex glutamatergic neuron and cortex glutamatergic neuron precursor alone in vivo
EP1585968A2 (en) * 2002-10-22 2005-10-19 BioMerieux, Inc. ISOTHERMAL AMPLIFICATION BASED ASSAY FOR THE DETECTION AND QUANTITATION OF ALPHA-FETOPROTEIN mRNA
WO2005114178A1 (en) * 2004-05-21 2005-12-01 Fraunhofer-Gesellschaft zur Förderung der angewandten Forschung e.V. Multi-cellular test systems
WO2005113748A3 (en) * 2004-04-21 2006-02-02 Univ Minnesota Mapc generation of lung tissue
WO2006028723A1 (en) * 2004-09-03 2006-03-16 Moraga Biotechnology Inc. Non-embryonic totipotent blastomer-like stem cells and methods therefor
WO2006049336A1 (en) * 2004-11-05 2006-05-11 Okada, Alan Method of preparing stem cells and tissue remedy
SG129236A1 (en) * 2002-07-26 2007-02-26 Food Industry Res & Dev Inst Somatic pluripotent cells
WO2006134602A3 (en) * 2005-06-16 2007-03-01 Univ Ramot Isolated cells and populations comprising same for the treatment of cns diseases
WO2007056578A1 (en) * 2005-11-09 2007-05-18 Athersys, Inc. Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
WO2007064090A1 (en) 2005-12-02 2007-06-07 Seoul National University Industry Foundation Multipotent adult stem cells having an ability of oct4 expression derived from umbilical cord blood and method for preparing the same
WO2007087292A2 (en) 2006-01-23 2007-08-02 Athersys, Inc. Mapc treatment of brain injuries and diseases
JP2007526017A (en) * 2003-06-25 2007-09-13 エイセル インコーポレイテッド Matrix composition tailored for tissue repair
WO2007117262A2 (en) * 2005-07-29 2007-10-18 Athersys, Inc. Culture of non-embryonic cells at high cell density
WO2006121454A3 (en) * 2005-05-05 2008-09-12 Univ Minnesota Use of mapc or progeny therefrom to populate lymphohematopoietic tissues
US7618621B2 (en) 2002-01-14 2009-11-17 The Board Of Trustees Of The University Of Illinois Mammalian multipotent neural stem cells and compositions, methods of preparation and methods of administration thereof
GB2467982A (en) * 2008-05-08 2010-08-25 Coretherapix Slu Pluripotent adult stem cells
WO2010140464A1 (en) * 2009-06-05 2010-12-09 国立大学法人 熊本大学 Method for induction of cell differentiation
US7875273B2 (en) 2004-12-23 2011-01-25 Ethicon, Incorporated Treatment of Parkinson's disease and related disorders using postpartum derived cells
US7875272B2 (en) 2003-06-27 2011-01-25 Ethicon, Incorporated Treatment of stroke and other acute neuraldegenerative disorders using postpartum derived cells
WO2011011500A1 (en) 2009-07-21 2011-01-27 Abt Holding Company Use of stem cells to reduce leukocyte extravasation
US7947266B2 (en) 2003-03-28 2011-05-24 Angioblast Systems Inc. Perivascular mesenchymal precursor cells
EP1824965B1 (en) * 2004-10-27 2011-10-05 Vrije Universiteit Brussel Hepatic differentiation of stem cells
EP2428563A1 (en) 2005-02-10 2012-03-14 Regents Of The University Of Minnesota Vascular/lymphatic endothelial cells
EP2456860A1 (en) * 2009-07-21 2012-05-30 ABT Holding Company Use of stem cells to reduce leukocyte extravasation
US8252280B1 (en) 1999-08-05 2012-08-28 Regents Of The University Of Minnesota MAPC generation of muscle
US8309070B2 (en) 2004-05-17 2012-11-13 Regents Of The University Of Minnesota Use of umbilical cord blood stem cells to treat ischemic event
US8318483B2 (en) 2003-06-27 2012-11-27 Advanced Technologies And Regenerative Medicine, Llc Postpartum cells derived from umbilical cord tissue, and methods of making and using the same
US8609412B2 (en) 1999-08-05 2013-12-17 Regents Of The University Of Minnesota Mapc generation of lung tissue
JP2014503219A (en) * 2011-01-12 2014-02-13 常雄 城戸 A culture method for obtaining and maintaining a pure or enriched population of mammalian neural stem cells and / or neural progenitor cells that are susceptible to differentiation into oligodendrocyte lineage cells in vitro
US8652846B2 (en) 2008-10-13 2014-02-18 Omnicyte Limited Medium derived from stem cells as a pharmaceutical composition
US8663987B2 (en) 2008-05-28 2014-03-04 Ramot At Tel-Aviv University Ltd. Mesenchymal stem cells for the treatment of CNS diseases
US9005964B2 (en) 2006-11-24 2015-04-14 Regents Of The University Of Minnesota Endodermal progenitor cells
US9175261B2 (en) 2005-12-16 2015-11-03 DePuy Synthes Products, Inc. Human umbilical cord tissue cells for inhibiting adverse immune response in histocompatibility-mismatched transplantation
WO2016200340A1 (en) * 2015-06-12 2016-12-15 Agency For Science, Technology And Research Derivation of hepatic stem cells and mature liver cell types and uses thereof
US9539341B2 (en) 2011-03-30 2017-01-10 Board Of Regents Of The University Of Texas System Methods and compositions for targeting adipose cells in mammals
US9611513B2 (en) 2011-12-23 2017-04-04 DePuy Synthes Products, Inc. Detection of human umbilical cord tissue derived cells
WO2017062401A1 (en) 2015-10-05 2017-04-13 ORIG3N Inc. Diagnosis and treatment of parkinson's disease based on identification and amelioration of liver dysfunction
US9834787B2 (en) 2009-04-09 2017-12-05 Sangamo Therapeutics, Inc. Targeted integration into stem cells
EP2589390B1 (en) * 2010-07-01 2018-03-07 Aktsionernoe Obschestvo "Pharm-Sintez" Pharmaceutical composition for treating central and peripheral nervous system diseases of vascular, traumatic, toxic, hypoxic and autoimmune origin
EP2589389B1 (en) * 2010-07-01 2018-03-07 Aktsionernoe Obschestvo "Pharm-Sintez" Method for producing a biologically active complex. biologically active protein/polypeptide complex
US9943552B2 (en) 2009-03-26 2018-04-17 DePuy Synthes Products, Inc. hUTC as therapy for Alzheimer's disease
EP3345610A1 (en) 2006-01-23 2018-07-11 Athersys, Inc. Mapc therapeutics without adjunctive immunosuppressive treatment
US10117900B2 (en) 2005-11-09 2018-11-06 Athersys, Inc. MAPC treatment of brain injuries and diseases
US10179900B2 (en) 2008-12-19 2019-01-15 DePuy Synthes Products, Inc. Conditioned media and methods of making a conditioned media
US10557116B2 (en) 2008-12-19 2020-02-11 DePuy Synthes Products, Inc. Treatment of lung and pulmonary diseases and disorders
WO2020160274A1 (en) 2019-02-01 2020-08-06 Abt Holding Company Multipotent adult progenitor cells for use in treating intracerebral hemorrhage
US10744164B2 (en) 2003-06-27 2020-08-18 DePuy Synthes Products, Inc. Repair and regeneration of ocular tissue using postpartum-derived cells
US11000546B2 (en) 2005-11-09 2021-05-11 Athersys, Inc. Immunomodulatory properties of MAPCs and uses thereof
EP4379046A1 (en) 2022-11-30 2024-06-05 Universidade Nova De Lisboa A 3d cellular model of early diabetic retinopathy
WO2024116114A1 (en) 2022-11-30 2024-06-06 Universidade Nova De Lisboa A 3d cellular model of early diabetic retinopathy

Families Citing this family (108)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US20040242520A1 (en) * 1997-09-06 2004-12-02 Mayo Foundation For Medical Education And Research, A Minnesota Corporation Expression of immonogenic substances
AUPQ147799A0 (en) * 1999-07-07 1999-07-29 Medvet Science Pty. Ltd. Mesenchymal precursor cell
US7670628B2 (en) * 1999-07-07 2010-03-02 Angioblast Systems, Inc. Mesenchymal precursor cell
US20050158289A1 (en) * 1999-07-07 2005-07-21 Simmons Paul J. Mesenchymal precursor cell and use thereof in the repair of bone defects and fractures in mammals
US8062675B2 (en) * 1999-07-07 2011-11-22 Angioblast Systems, Inc. Mesenchymal precursor cell
US10638734B2 (en) 2004-01-05 2020-05-05 Abt Holding Company Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
US7015037B1 (en) 1999-08-05 2006-03-21 Regents Of The University Of Minnesota Multiponent adult stem cells and methods for isolation
US7291597B2 (en) * 2000-04-06 2007-11-06 Franco Wayne P Growth factor therapy mobilization of stem cells into the peripheral blood
US7311905B2 (en) * 2002-02-13 2007-12-25 Anthrogenesis Corporation Embryonic-like stem cells derived from post-partum mammalian placenta, and uses and methods of treatment using said cells
ES2522890T3 (en) 2000-12-06 2014-11-19 Anthrogenesis Corporation Method to collect placental stem cells
EP1367899A4 (en) 2001-02-14 2004-07-28 Leo T Furcht Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
EP2336299A1 (en) * 2001-02-14 2011-06-22 Anthrogenesis Corporation Post-partum mammalian placenta, its use and placental stem cells therefrom
ES2522526T3 (en) 2001-02-14 2014-11-14 Anthrogenesis Corporation Post-partum placenta of mammals, their use and placental stem cells thereof
DE10144326B4 (en) * 2001-09-10 2005-09-22 Siemens Ag Method and system for monitoring a tire air pressure
US9969980B2 (en) * 2001-09-21 2018-05-15 Garnet Biotherapeutics Cell populations which co-express CD49c and CD90
US20040052771A1 (en) * 2002-07-12 2004-03-18 Lim Sai Kiang Hemangioblast progenitor cells
WO2004007698A1 (en) * 2002-07-12 2004-01-22 National University Of Singapore Hemangioblast progenitor cells
AU2003278212B2 (en) * 2002-07-31 2009-07-09 Centre National De La Recherche Scientifique Stem cells derived from adipous tissue and differentiated cells derived from said cells
US9969977B2 (en) * 2002-09-20 2018-05-15 Garnet Biotherapeutics Cell populations which co-express CD49c and CD90
US9572840B2 (en) 2003-06-27 2017-02-21 DePuy Synthes Products, Inc. Regeneration and repair of neural tissue using postpartum-derived cells
US9592258B2 (en) 2003-06-27 2017-03-14 DePuy Synthes Products, Inc. Treatment of neurological injury by administration of human umbilical cord tissue-derived cells
WO2005003317A2 (en) * 2003-07-01 2005-01-13 Regents Of The University Of Minnesota Engineered blood vessels
CA2542120C (en) 2003-10-08 2018-07-10 Vet-Stem Inc. Methods of preparing and using stem cell compositions and kits comprising the same
AU2005241008C1 (en) * 2004-04-23 2010-11-04 Bioe, Inc. Multi-Lineage Progenitor Cells
US7622108B2 (en) * 2004-04-23 2009-11-24 Bioe, Inc. Multi-lineage progenitor cells
EP2361970A1 (en) 2004-09-24 2011-08-31 Angioblast Systems Incorporated Method of enhancing proliferation and/or survival of mesenchymal precursor cells (MPC)
JP2008514214A (en) * 2004-09-29 2008-05-08 セルアーティス アーベー Method for generating hepatocyte-like cells from human blastocyst-derived stem cells (hBS)
CA2526327C (en) 2004-11-09 2014-01-07 Institut National D'optique Device for transmitting multiple optically-encoded stimulation signals to multiple cell locations
AU2005331559B2 (en) * 2005-05-05 2012-04-19 Regents Of The University Of Minnesota Use of NK cell inhibition to facilitate persistence of engrafted MHC-I negative cells
JP2009509911A (en) * 2005-05-05 2009-03-12 リージェンツ オブ ザ ユニバーシティ オブ ミネソタ Use of MAPCs or their progeny to establish lymphatic hematopoietic tissue
WO2007025166A2 (en) 2005-08-25 2007-03-01 Repair Technologies, Inc. Devices, compositions and methods for the protection and repair of cells and tissues
WO2007047468A2 (en) 2005-10-13 2007-04-26 Anthrogenesis Corporation Immunomodulation using placental stem cells
US9125906B2 (en) 2005-12-28 2015-09-08 DePuy Synthes Products, Inc. Treatment of peripheral vascular disease using umbilical cord tissue-derived cells
KR20190104428A (en) 2005-12-29 2019-09-09 안트로제네시스 코포레이션 Placental stem cell populations
US8455250B2 (en) 2005-12-29 2013-06-04 Anthrogenesis Corporation Co-culture of placental stem cells and stem cells from a second source
AP2949A (en) 2006-03-07 2014-07-31 Shroff Geeta Compositions comprising human embryonic stem cellsand their derivatives, methods of use, and method s of preparation
WO2007106351A2 (en) * 2006-03-10 2007-09-20 The University Of Rochester Porous silicon materials and devices
KR100871984B1 (en) 2006-04-12 2008-12-05 주식회사 알앤엘바이오 Multipotent Stem Cell Derived from Placenta Tissue and Cellular Therapeutic Agents Comprising the Same
WO2007121443A2 (en) * 2006-04-17 2007-10-25 Bioe, Inc. Differentiation of multi-lineage progenitor cells to respiratory epithelial cells
WO2007127454A2 (en) 2006-04-28 2007-11-08 Cythera, Inc. Hepatocyte lineage cells
KR100792184B1 (en) * 2006-05-12 2008-01-07 재단법인서울대학교산학협력재단 Mutipotent Adult Stem Cell Derived from Canine Umbilical Cord Blood, Placenta and Canine Fetus Heart, Method for Preparing the Same and Cellular Therapeutics Containing the Same
WO2007146106A2 (en) * 2006-06-05 2007-12-21 Cryo- Cell International, Inc. Procurement, isolation and cryopreservation of maternal placental cells
US20080050814A1 (en) * 2006-06-05 2008-02-28 Cryo-Cell International, Inc. Procurement, isolation and cryopreservation of fetal placental cells
EP2035552A2 (en) * 2006-06-09 2009-03-18 Anthrogenesis Corporation Placental niche and use thereof to culture stem cells
US7875453B2 (en) * 2006-06-14 2011-01-25 Bioe Llc Differentiation of multi-lineage progenitor cells to hepatocytes
US7993918B2 (en) * 2006-08-04 2011-08-09 Anthrogenesis Corporation Tumor suppression using placental stem cells
KR100818213B1 (en) 2006-09-22 2008-04-01 재단법인서울대학교산학협력재단 Human Cord Blood Multipotent Stem Cell Having Enhanced Proliferation Ability With Osteoclast-based Niche-like Structure and Method for Preparing the Same
KR100818214B1 (en) 2006-09-29 2008-04-01 재단법인서울대학교산학협력재단 Multipotent stem cell derived from amnion or decidua isolated from human term placenta and method for preparing the same
PL2578081T3 (en) 2006-10-11 2016-09-30 Compositions, methods, and devices for treating liver disease
NZ595854A (en) 2006-10-23 2013-04-26 Anthrogenesis Corp Methods and compositions for treatment of bone defects with placental cell populations (ELOVL2, ST3GAL6, STGALNAC5, SLC12A8)
CA2668673A1 (en) * 2006-11-08 2008-05-22 Aldagen, Inc. Methods for improved engraftment following stem cell transplantation
MX349225B (en) 2007-02-12 2017-07-19 Anthrogenesis Corp Treatment of inflammatory diseases using placental stem cells.
WO2008101100A2 (en) * 2007-02-14 2008-08-21 Indiana University Research And Technology Corporation Composition for stimulating formation of vascular structures
US8574567B2 (en) * 2007-05-03 2013-11-05 The Brigham And Women's Hospital, Inc. Multipotent stem cells and uses thereof
WO2008137115A1 (en) * 2007-05-03 2008-11-13 The Brigham And Women's Hospital, Inc. Multipotent stem cells and uses thereof
TWM322542U (en) * 2007-05-23 2007-11-21 Universal Scient Ind Co Ltd Testing machine
EP2171043B1 (en) * 2007-06-15 2015-03-18 Garnet BioTherapeutics, Inc Treatment of diseases and disorders using self-renewing colony forming cells cultured and expanded in vitro
WO2008156659A1 (en) 2007-06-18 2008-12-24 Children's Hospital & Research Center At Oakland Method of isolating stem and progenitor cells from placenta
CN101835479A (en) * 2007-07-25 2010-09-15 佰欧益有限公司 Differentiation of multi-lineage progenitor cells to chondrocytes
KR20210022148A (en) 2007-09-28 2021-03-02 안트로제네시스 코포레이션 Tumor suppression using human placental perfusate and human placenta-derived intermediate natural killer cells
WO2009061442A1 (en) * 2007-11-06 2009-05-14 Children's Medical Center Corporation Method to produce induced pluripotent stem (ips) cells form non-embryonic human cells
EP2245141B1 (en) 2008-01-18 2018-03-14 Regents of the University of Minnesota Stem cell aggregates and methods for making and using
US20090233993A1 (en) * 2008-03-06 2009-09-17 Burnham Institute For Medical Research Compositions and methods for inhibiting gsk3 activity and uses thereof
EP2294187A2 (en) * 2008-05-21 2011-03-16 BioE LLC Differentiation of multi-lineage progenitor cells to pancreatic cells
EP3539380A3 (en) 2008-08-20 2019-12-18 Celularity, Inc. Improved cell composition and methods of making the same
MX2011001991A (en) 2008-08-20 2011-03-29 Anthrogenesis Corp Treatment of stroke using isolated placental cells.
WO2010021756A1 (en) 2008-08-22 2010-02-25 Anthrogenesis Corporation Methods and compositions for treatment of bone defects with placental cell populations
DK2367932T3 (en) 2008-11-19 2019-09-23 Celularity Inc AMNION-derived adherent cells
US8771677B2 (en) 2008-12-29 2014-07-08 Vladimir B Serikov Colony-forming unit cell of human chorion and method to obtain and use thereof
US8372642B2 (en) * 2009-02-27 2013-02-12 Cellular Dynamics International, Inc. Differentiation of pluripotent cells
KR100950195B1 (en) * 2009-03-20 2010-03-29 서울대학교산학협력단 Method for isolation of umbilical cord blood derived-pluripotent stem cell expressing znf281
WO2010144696A1 (en) 2009-06-11 2010-12-16 Burnham Institute For Medical Research Directed differentiation of stem cells
RU2583287C2 (en) * 2009-07-09 2016-05-10 Янссен Байотек, Инк. Cells being derivatives of cardiac tissue
WO2011082339A2 (en) * 2009-12-31 2011-07-07 Cedars-Sinai Medical Center Regeneration of, reestablishing function in and replacing microvasculature in organs and tissues
ES2646750T3 (en) 2010-01-26 2017-12-15 Anthrogenesis Corporation Treatment of bone-related cancers using placental stem cells
SG183497A1 (en) 2010-02-25 2012-09-27 Abt Holding Co Modulation of macrophage activation
SG10201913904PA (en) 2010-02-25 2020-03-30 Abt Holding Co Modulation of angiogenesis
HUE029144T2 (en) 2010-04-07 2017-02-28 Anthrogenesis Corp Angiogenesis using placental stem cells
CA2795401A1 (en) 2010-04-08 2011-10-13 Anthrogenesis Corporation Treatment of sarcoidosis using placental stem cells
WO2011143415A1 (en) 2010-05-12 2011-11-17 Abt Holding Company Modulation of splenocytes in cell therapy
WO2011158125A2 (en) 2010-06-17 2011-12-22 Katholieke Universiteit Leuven Methods for differentiating cells into hepatic stellate cells and hepatic sinusoidal endothelial cells, cells produced by the methods, and methods for using the cells
EP2593542B1 (en) 2010-07-13 2018-01-03 Anthrogenesis Corporation Methods of generating natural killer cells
WO2012027474A1 (en) 2010-08-24 2012-03-01 Regents Of The University Of Minnesota Non-static suspension culture of cell aggregates
EP2625577B1 (en) 2010-10-08 2019-06-26 Terumo BCT, Inc. Customizable methods and systems of growing and harvesting cells in a hollow fiber bioreactor system
US8574899B2 (en) 2010-12-22 2013-11-05 Vladimir B Serikov Methods for augmentation collection of placental hematopoietic stem cells and uses thereof
WO2012092485A1 (en) 2010-12-31 2012-07-05 Anthrogenesis Corporation Enhancement of placental stem cell potency using modulatory rna molecules
EP3443968A1 (en) 2011-06-01 2019-02-20 Celularity, Inc. Treatment of pain using placental stem cells
US20120308531A1 (en) 2011-06-06 2012-12-06 ReGenesys BVBA Expansion of Stem Cells in Hollow Fiber Bioreactors
WO2013055476A1 (en) 2011-09-09 2013-04-18 Anthrogenesis Corporation Treatment of amyotrophic lateral sclerosis using placental stem cells
WO2013151725A1 (en) 2012-04-05 2013-10-10 The Regents Of The University Of California Regenerative sera cells and mesenchymal stem cells
CN105142651A (en) 2013-02-05 2015-12-09 人类起源公司 Natural killer cells from placenta
CA2909267C (en) 2013-04-12 2022-10-25 Saverio LA FRANCESCA Improving organs for transplantation
DK2992088T3 (en) 2013-04-30 2019-11-11 Univ Leuven Kath CELL THERAPY FOR MYELODYSPLASTIC SYNDROMES
JP6633522B2 (en) 2013-11-16 2020-01-22 テルモ ビーシーティー、インコーポレーテッド Cell growth in bioreactors
WO2015148704A1 (en) 2014-03-25 2015-10-01 Terumo Bct, Inc. Passive replacement of media
WO2016049421A1 (en) 2014-09-26 2016-03-31 Terumo Bct, Inc. Scheduled feed
WO2017004592A1 (en) 2015-07-02 2017-01-05 Terumo Bct, Inc. Cell growth with mechanical stimuli
EP3405566B1 (en) 2016-01-21 2023-10-18 ABT Holding Company Stem cells for healing of skin ulcers
US11965175B2 (en) 2016-05-25 2024-04-23 Terumo Bct, Inc. Cell expansion
US11104874B2 (en) 2016-06-07 2021-08-31 Terumo Bct, Inc. Coating a bioreactor
US11685883B2 (en) 2016-06-07 2023-06-27 Terumo Bct, Inc. Methods and systems for coating a cell growth surface
KR20190017985A (en) * 2016-06-14 2019-02-20 리전츠 오브 더 유니버스티 오브 미네소타 Genetically modified cells, tissues, and organs for treating diseases
EP3656841A1 (en) 2017-03-31 2020-05-27 Terumo BCT, Inc. Cell expansion
US11624046B2 (en) 2017-03-31 2023-04-11 Terumo Bct, Inc. Cell expansion
EP3880704A4 (en) * 2018-11-09 2022-10-19 Figene, LLC Regenerative abscopal effects
US11697799B2 (en) * 2019-04-15 2023-07-11 Ossium Health, Inc. System and method for extraction and cryopreservation of bone marrow
JP2023516484A (en) 2020-03-11 2023-04-19 ビット バイオ リミテッド Hepatocyte production method
US12043823B2 (en) 2021-03-23 2024-07-23 Terumo Bct, Inc. Cell capture and expansion

Family Cites Families (82)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US4965204A (en) * 1984-02-06 1990-10-23 The Johns Hopkins University Human stem cells and monoclonal antibodies
US5130144B1 (en) * 1984-02-06 1995-08-15 Univ Johns Hopkins Human stem cells and monoclonal antibodies
US4714680B1 (en) * 1984-02-06 1995-06-27 Univ Johns Hopkins Human stem cells
US5087570A (en) * 1988-05-10 1992-02-11 Weissman Irving L Homogeneous mammalian hematopoietic stem cell composition
US5635386A (en) * 1989-06-15 1997-06-03 The Regents Of The University Of Michigan Methods for regulating the specific lineages of cells produced in a human hematopoietic cell culture
US5061620A (en) * 1990-03-30 1991-10-29 Systemix, Inc. Human hematopoietic stem cell
US5486359A (en) * 1990-11-16 1996-01-23 Osiris Therapeutics, Inc. Human mesenchymal stem cells
US5197985A (en) * 1990-11-16 1993-03-30 Caplan Arnold I Method for enhancing the implantation and differentiation of marrow-derived mesenchymal cells
US5733542A (en) * 1990-11-16 1998-03-31 Haynesworth; Stephen E. Enhancing bone marrow engraftment using MSCS
AU4543193A (en) * 1992-06-22 1994-01-24 Henry E. Young Scar inhibitory factor and use thereof
US5654183A (en) * 1992-07-27 1997-08-05 California Institute Of Technology Genetically engineered mammalian neural crest stem cells
US5672499A (en) * 1992-07-27 1997-09-30 California Institute Of Technology Immoralized neural crest stem cells and methods of making
US5589376A (en) * 1992-07-27 1996-12-31 California Institute Of Technology Mammalian neural crest stem cells
GB9308271D0 (en) * 1993-04-21 1993-06-02 Univ Edinburgh Method of isolating and/or enriching and/or selectively propagating pluripotential animal cells and animals for use in said method
NZ314644A (en) 1993-05-24 2000-11-24 Immunex Corp Use of flt3-ligands as a growth stimulator of stem cells in the transplantation of tissue
WO1995003062A1 (en) 1993-07-21 1995-02-02 Cellpro, Incorporated Methods and compositions for preventing immune rejection of solid organ grafts
WO1995010599A1 (en) 1993-10-15 1995-04-20 The University Of Melbourne Embryonic stem cell-like cells
US6015671A (en) * 1995-06-07 2000-01-18 Indiana University Foundation Myocardial grafts and cellular compositions
US5602301A (en) * 1993-11-16 1997-02-11 Indiana University Foundation Non-human mammal having a graft and methods of delivering protein to myocardial tissue
US5486659A (en) * 1994-03-08 1996-01-23 Rosenbush; Stuart W. Stethoscope protection device and method for using same
DE4441327C1 (en) * 1994-11-22 1995-11-09 Inst Pflanzengenetik & Kultur Embryonic heart muscle cells, their production and their use
US5648248A (en) * 1994-12-30 1997-07-15 Boehringer Ingelheim International Gmbh Methods for producing differentiated cells from immature hematopoietic cells
US5843780A (en) * 1995-01-20 1998-12-01 Wisconsin Alumni Research Foundation Primate embryonic stem cells
US5736396A (en) * 1995-01-24 1998-04-07 Case Western Reserve University Lineage-directed induction of human mesenchymal stem cell differentiation
GB9502022D0 (en) * 1995-02-02 1995-03-22 Abuljadayel Ilham M S A method for preparing lymphohaematopoietic progenitor cells
US5906934A (en) 1995-03-14 1999-05-25 Morphogen Pharmaceuticals, Inc. Mesenchymal stem cells for cartilage repair
US6653134B2 (en) * 1995-03-28 2003-11-25 Cp Hahnemann University Isolated stromal cells for use in the treatment of diseases of the central nervous system
US6306575B1 (en) * 1995-06-16 2001-10-23 Stemcell Technologies, Inc. Methods for preparing enriched human hematopoietic cell preparations
CA2191655C (en) 1995-12-01 2010-01-12 Terry E. Thomas Novel antibody compositions for preparing enriched human hematopoietic and tumor cell preparations
US20010012513A1 (en) * 1996-08-19 2001-08-09 University Of Massachusetts Embryonic or stem-like cell lines produced by cross species nuclear transplantation
US6787355B1 (en) 1996-08-26 2004-09-07 Mcgill University Multipotent neural stem cells from peripheral tissues and uses thereof
AU4984697A (en) * 1996-10-11 1998-05-11 The Texas A & M University System Methods for the generation of primordial germ cells and transgenic animal species
US6090622A (en) * 1997-03-31 2000-07-18 The Johns Hopkins School Of Medicine Human embryonic pluripotent germ cells
US5968829A (en) 1997-09-05 1999-10-19 Cytotherapeutics, Inc. Human CNS neural stem cells
JP2001517428A (en) 1997-09-25 2001-10-09 サイトマトリックス,エルエルシー Methods and devices for long-term culture of hematopoietic progenitor cells
US6093531A (en) 1997-09-29 2000-07-25 Neurospheres Holdings Ltd. Generation of hematopoietic cells from multipotent neural stem cells
WO1999027076A1 (en) 1997-11-25 1999-06-03 Arc Genomic Research Pluripotent embryonic stem cells and methods of obtaining them
EP1045697A2 (en) 1998-01-12 2000-10-25 Cold Spring Harbor Laboratory Extension of cellular lifespan, methods and reagents
CA2324591A1 (en) 1998-04-09 1999-10-21 Bresagen Limited Cell differentiation/proliferation and maintenance factor and uses thereof
US6225119B1 (en) * 1998-05-22 2001-05-01 Osiris Therapeutics, Inc. Production of megakaryocytes by the use of human mesenchymal stem cells
DE19833476B4 (en) * 1998-07-24 2005-08-25 Huss, Ralf, Dr. Genetically modified CD34 negatives, adherently growing hematopoietic stem cells and their use in gene therapy
AU3881499A (en) 1998-09-01 2000-03-21 Wisconsin Alumni Research Foundation Primate embryonic stem cells with compatible histocompatibility genes
EP1146837A4 (en) 1998-11-30 2002-10-31 Ivf Sciences Colorado Inc System and sequential culture media for in vitro fertilization
US6777231B1 (en) * 1999-03-10 2004-08-17 The Regents Of The University Of California Adipose-derived stem cells and lattices
US20050169896A1 (en) * 1999-05-14 2005-08-04 Henry Ford Health System Bone marrow transplantation for treatment of stroke
AUPQ147799A0 (en) 1999-07-07 1999-07-29 Medvet Science Pty. Ltd. Mesenchymal precursor cell
AU759643B2 (en) 1999-07-20 2003-04-17 University Of Southern California Identification of pluripotent pre-mesenchymal, pre-hematopoietic progenitor cell
AU782396B2 (en) 1999-07-29 2005-07-21 Steven Baranowitz Methods for transdifferentiation of body tissues
IL147990A0 (en) * 1999-08-05 2002-09-12 Mcl Llc Multipotent adult stem cells and methods for isolation
US8609412B2 (en) * 1999-08-05 2013-12-17 Regents Of The University Of Minnesota Mapc generation of lung tissue
US8075881B2 (en) * 1999-08-05 2011-12-13 Regents Of The University Of Minnesota Use of multipotent adult stem cells in treatment of myocardial infarction and congestive heart failure
US7927587B2 (en) * 1999-08-05 2011-04-19 Regents Of The University Of Minnesota MAPC administration for the treatment of lysosomal storage disorders
US8147824B2 (en) * 1999-08-05 2012-04-03 Athersys, Inc. Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
US7015037B1 (en) * 1999-08-05 2006-03-21 Regents Of The University Of Minnesota Multiponent adult stem cells and methods for isolation
WO2001021766A2 (en) 1999-09-23 2001-03-29 Cell Science Therapeutics Methods and devices for obtaining non-hematopoietic lineage cells from hematopoietic progenitor cells
WO2001021767A2 (en) 1999-09-24 2001-03-29 Morphogen Pharmaceuticals, Inc. Pluripotent embryonic-like stem cells, compositions, methods and uses thereof
EP1224259A4 (en) 1999-09-27 2005-04-27 Univ Florida Reversal of insulin-dependent diabetes by islet-producing stem cells, islet progenitor cells and islet-like structures
CA2388497A1 (en) 1999-10-15 2001-04-26 Advanced Cell Technology, Inc. Method of producing differentiated progenitor cells by culturing morula or inner cell mass cells
US6280718B1 (en) * 1999-11-08 2001-08-28 Wisconsin Alumni Reasearch Foundation Hematopoietic differentiation of human pluripotent embryonic stem cells
AU778929B2 (en) * 1999-12-06 2004-12-23 General Hospital Corporation, The Pancreatic stem cells and their use in transplantation
CA2397292A1 (en) 2000-01-14 2001-07-19 Bresagen Limited Cell production
US6602711B1 (en) 2000-02-21 2003-08-05 Wisconsin Alumni Research Foundation Method of making embryoid bodies from primate embryonic stem cells
CA2400485C (en) * 2000-02-26 2014-04-29 Artecel Sciences, Inc. Pleuripotent stem cells generated from adipose tissue-derived stromal cells and uses thereof
US7005252B1 (en) 2000-03-09 2006-02-28 Wisconsin Alumni Research Foundation Serum free cultivation of primate embryonic stem cells
JP4889902B2 (en) 2000-03-14 2012-03-07 イーエス・セル・インターナショナル・プライヴェート・リミテッド Method for producing human neural progenitor cells from human embryonic stem (hES) cells, method for producing neurons using the method, method for producing oligodendrocytes or astrocytes
EP1176189A1 (en) 2000-07-21 2002-01-30 Fornix Biosciences N.V. Stem cell-like cells
WO2002009650A2 (en) * 2000-07-31 2002-02-07 New York Medical College Methods and compositions for the repair and/or regeneration of damaged myocardium
GB0026252D0 (en) 2000-10-26 2000-12-13 Univ Edinburgh Pluripotential stem cells
US7560280B2 (en) * 2000-11-03 2009-07-14 Kourion Therapeutics Gmbh Human cord blood derived unrestricted somatic stem cells (USSC)
US7311905B2 (en) * 2002-02-13 2007-12-25 Anthrogenesis Corporation Embryonic-like stem cells derived from post-partum mammalian placenta, and uses and methods of treatment using said cells
ES2522890T3 (en) * 2000-12-06 2014-11-19 Anthrogenesis Corporation Method to collect placental stem cells
EP1367899A4 (en) * 2001-02-14 2004-07-28 Leo T Furcht Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
EP2336299A1 (en) * 2001-02-14 2011-06-22 Anthrogenesis Corporation Post-partum mammalian placenta, its use and placental stem cells therefrom
US7056738B2 (en) * 2001-03-23 2006-06-06 Tulane University Early stage multipotential stem cells in colonies of bone marrow stromal cells
KR100449141B1 (en) * 2001-04-19 2004-09-21 (주)라이프코드 Method for differentiating a mesenchymal stem cell into neural cells
US20030003090A1 (en) * 2001-05-31 2003-01-02 Prockop Darwin J. Directed in vitro differentiation of marrow stromal cells into neural cell progenitors
US9969980B2 (en) * 2001-09-21 2018-05-15 Garnet Biotherapeutics Cell populations which co-express CD49c and CD90
AU2003298016A1 (en) * 2002-11-27 2004-06-23 Regents Of The University Of Minnesota Homologous recombination in multipotent adult progenitor cells
US20040235165A1 (en) * 2003-05-19 2004-11-25 Darwin Prockop In vitro differentiation of adult stem cells
WO2005003317A2 (en) * 2003-07-01 2005-01-13 Regents Of The University Of Minnesota Engineered blood vessels
WO2005003320A2 (en) * 2003-07-02 2005-01-13 Regents Of The University Of Minnesota Neuronal differentiation of stem cells
EP1660644A1 (en) * 2003-08-29 2006-05-31 Regents Of The University Of Minnesota Kidney derived stem cells and methods for their isolation, differentiation and use

Non-Patent Citations (11)

* Cited by examiner, † Cited by third party
Title
CARGILL M. ET AL.: 'Characterization of single-nucleotide polymorphisms in coding regions of human genes' NATURE GENETICS vol. 22, July 1999, pages 231 - 238, XP002121300 *
GEIGER H. ET AL.: 'Globin gene expression is reprogrammed in chimeras generated by injecting adult hematopoietic stem cells into mouse blastocysts' CELL vol. 93, no. 6, 12 June 1998, pages 1055 - 1065, XP000941662 *
GEISSLER E.K. ET AL.: 'Effective use of donor MHC class I gene therapy in organ transplantation prevention of antibody-mediated hyperacute heart allograft rejection in highly sensitized rat recipients' HUMAN GENE THERAPY vol. 11, no. 3, 2000, pages 459 - 469, XP002954855 *
GRIGORIADOU K. ET AL.: 'MHC class in molecules alone control NK-mediated bone marrow graft rejection' EUROPEAN JOURNAL OF IMMUNOLOGY vol. 29, no. 11, November 1999, pages 3683 - 3690, XP002954854 *
GULCHER J. ET AL.: 'Population genetics: laying the groundwork for genetic disease modeling and targeting' CLINICAL CHEMICAL LABORATORY MEDICINE vol. 36, no. 8, 1998, pages 523 - 527, XP002941805 *
HUILIN Q. ET AL.: 'Identification of genes responsible for bone differentiation from human bone marrow derived multipotent adult stem cells (MASC)' BLOOD vol. 96, no. 11, PART 1, 16 November 2000, pages 70A - 71A, ABS. 298, XP002955582 *
KEENE C.D. ET AL.: 'Phenotypic expression of transplanted human bone marrow-derived multipotent adult stem cells into the rat CNS' EXPERIMENTAL NEUROLOGY vol. 164, no. 2, August 2000, page 465, XP002954852 *
KUZNETSOV S.A. ET AL.: 'Factors required for bone marrow stromal fibroblast colony formation in vitro' BRITISH JOURNAL OF HEMATOLOGY vol. 97, no. 3, June 1997, pages 561 - 570, XP002954851 *
MARMUR R. ET AL.: 'Isolation and developmental characterization of cerebral cortical multipotent progenitors' DEVELOPMENTAL BIOLOGY vol. 204, no. 2, 1998, pages 577 - 591, XP002954853 *
REYES M. ET AL.: 'Characterization of multipotent adult progenitor cells, a subpopulation of mesenchymal stem cells' ANNALS OF THE NEW YORK ACADEMY OF SCIENCES vol. 938, 2001, pages 231 - 235, XP002954850 *
See also references of EP1367899A2 *

Cited By (118)

* Cited by examiner, † Cited by third party
Publication number Priority date Publication date Assignee Title
US9808485B2 (en) 1999-08-05 2017-11-07 Athersys, Inc. Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
US8147824B2 (en) 1999-08-05 2012-04-03 Athersys, Inc. Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
US8252280B1 (en) 1999-08-05 2012-08-28 Regents Of The University Of Minnesota MAPC generation of muscle
US8609412B2 (en) 1999-08-05 2013-12-17 Regents Of The University Of Minnesota Mapc generation of lung tissue
US9962407B2 (en) 1999-08-05 2018-05-08 Athersys, Inc. Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
US8192732B2 (en) 2002-01-14 2012-06-05 University Of Central Florida Research Foundation, Inc. Mammalian multipotent stem cells and compositions, methods of preparation and methods of administration thereof
US9084789B2 (en) 2002-01-14 2015-07-21 Board Of Trustees Of The University Of Illinois Use of modified pyrimidine compounds to promote stem cell migration and proliferation
US7687505B2 (en) 2002-01-14 2010-03-30 Board Of Trustees Of The University Of Illinois Use of modified pyrimidine compounds to promote stem cell migration and proliferation
US9358234B2 (en) 2002-01-14 2016-06-07 The Board Of Trustees Of The University Of Illinois Mammalian multipotent stem cells and compositions, methods of preparation and methods of administration thereof
US7635467B2 (en) 2002-01-14 2009-12-22 The Board Of Trustees Of The University Of Illinois Mammalian multipotent stem cells and compositions, methods of preparation and methods of administration thereof
US7618621B2 (en) 2002-01-14 2009-11-17 The Board Of Trustees Of The University Of Illinois Mammalian multipotent neural stem cells and compositions, methods of preparation and methods of administration thereof
US8273756B2 (en) 2002-01-14 2012-09-25 University Of Central Florida Research Foundation, Inc. Use of modified pyrimidine compounds to promote stem cell migration and proliferation
EP1572949A4 (en) * 2002-06-07 2007-01-03 Univ California Maintenance of islet cells
EP1572949A2 (en) * 2002-06-07 2005-09-14 The Regents Of The University Of California Maintenance of islet cells
US7422736B2 (en) 2002-07-26 2008-09-09 Food Industry Research And Development Institute Somatic pluripotent cells
SG129236A1 (en) * 2002-07-26 2007-02-26 Food Industry Res & Dev Inst Somatic pluripotent cells
US7527968B2 (en) 2002-07-29 2009-05-05 Robarts Research Institute Regeneration initiating cells
WO2004011012A2 (en) * 2002-07-29 2004-02-05 Asahi Kasei Kabushiki Kaisha Stem cells for treating pancreatic damage
WO2004011012A3 (en) * 2002-07-29 2004-03-25 Asahi Chemical Ind Stem cells for treating pancreatic damage
EP1585968A4 (en) * 2002-10-22 2006-11-22 Bio Merieux Inc ISOTHERMAL AMPLIFICATION BASED ASSAY FOR THE DETECTION AND QUANTITATION OF ALPHA-FETOPROTEIN mRNA
EP1585968A2 (en) * 2002-10-22 2005-10-19 BioMerieux, Inc. ISOTHERMAL AMPLIFICATION BASED ASSAY FOR THE DETECTION AND QUANTITATION OF ALPHA-FETOPROTEIN mRNA
US7947266B2 (en) 2003-03-28 2011-05-24 Angioblast Systems Inc. Perivascular mesenchymal precursor cells
US10421946B2 (en) 2003-03-28 2019-09-24 Mesoblast, Inc. Perivascular mesenchymal precursor cells
JP2013208130A (en) * 2003-03-28 2013-10-10 Mesoblast Inc Perivascular mesenchymal precursor cell
WO2004087896A3 (en) * 2003-03-31 2004-11-11 Pfizer Prod Inc Hepatocyte differentiation of stem cells
WO2004087896A2 (en) * 2003-03-31 2004-10-14 Pfizer Products Inc. Hepatocyte differentiation of stem cells
EP2446892A2 (en) 2003-06-23 2012-05-02 Fraunhofer-Gesellschaft zur Förderung der angewandten Forschung Isolated adult pluripotent stem cells and method for isolating and cultivating same
US9206393B2 (en) 2003-06-23 2015-12-08 Fraunhofer Gesellschaft Zur Forderung De Angewandten Forschung E.V. Isolated adult pluripotent stem cells and methods for isolating and cultivating thereof
US8603809B2 (en) 2003-06-23 2013-12-10 Fraunhofer Gesellschaft Zur Forderung Der Angewandten Forschung E. V. Isolated adult pluripotent stem cells and methods for isolating and cultivating thereof
WO2005001072A1 (en) 2003-06-23 2005-01-06 Fraunhofer Gesellschaft Zur Förderung Der Angewandten Forschung E. V. Isolated pluripotent adult stem cells and methods for isolating and cultivating the same
JP2007526017A (en) * 2003-06-25 2007-09-13 エイセル インコーポレイテッド Matrix composition tailored for tissue repair
US10500234B2 (en) 2003-06-27 2019-12-10 DePuy Synthes Products, Inc. Postpartum cells derived from umbilical cord tissue, and methods of making and using the same
US10039793B2 (en) 2003-06-27 2018-08-07 DePuy Synthes Products, Inc. Soft tissue repair and regeneration using postpartum-derived cells and cell products
US8703121B2 (en) 2003-06-27 2014-04-22 DePuy Synthes Products, LLC Postpartum-derived cells for use in treatment of disease of the heart and circulatory system
US7875272B2 (en) 2003-06-27 2011-01-25 Ethicon, Incorporated Treatment of stroke and other acute neuraldegenerative disorders using postpartum derived cells
US10758576B2 (en) 2003-06-27 2020-09-01 DePuy Synthes Products, Inc. Soft tissue repair and regeneration using postpartum-derived cells and cell products
US9504719B2 (en) 2003-06-27 2016-11-29 DePuy Synthes Products, Inc. Soft tissue repair and regeneration using postpartum-derived cells and cell products
US9579351B2 (en) 2003-06-27 2017-02-28 DePuy Synthes Products, Inc. Postpartum cells derived from placental tissue, and methods of making and using the same
US8318483B2 (en) 2003-06-27 2012-11-27 Advanced Technologies And Regenerative Medicine, Llc Postpartum cells derived from umbilical cord tissue, and methods of making and using the same
US9717763B2 (en) 2003-06-27 2017-08-01 DePuy Synthes Products, Inc. Postpartum cells derived from umbilical cord tissue, and methods of making and using the same
US11191789B2 (en) 2003-06-27 2021-12-07 DePuy Synthes Products, Inc. Cartilage and bone repair and regeneration using postpartum-derived cells
US10383898B2 (en) 2003-06-27 2019-08-20 DePuy Synthes Products, Inc. Postpartum cells derived from placental tissue, and methods of making and using the same
US10195233B2 (en) 2003-06-27 2019-02-05 DePuy Synthes Products, Inc. Postpartum cells derived from placental tissue, and methods of making and using the same
US10744164B2 (en) 2003-06-27 2020-08-18 DePuy Synthes Products, Inc. Repair and regeneration of ocular tissue using postpartum-derived cells
US11000554B2 (en) 2003-06-27 2021-05-11 DePuy Synthes Products, Inc. Postpartum cells derived from placental tissue, and methods of making and using the same
US10220059B2 (en) 2003-06-27 2019-03-05 DePuy Synthes Products, Inc. Postpartum cells derived from placental tissue, and methods of making and using the same
US11179422B2 (en) 2003-06-27 2021-11-23 DePuy Synthes Products, Inc. Method of differentiating umbilical cord tissue into a chondrogenic phenotype
CN1918284B (en) * 2003-12-19 2012-07-04 奥姆尼赛特有限公司 Stem cells
WO2005059113A1 (en) * 2003-12-19 2005-06-30 Omnicyte Ltd Stem cells
WO2005095588A1 (en) * 2004-03-31 2005-10-13 Kyoto University Cortex glutamatergic neuron precursor providing cortex glutamatergic neuron and cortex glutamatergic neuron precursor alone in vivo
WO2005113748A3 (en) * 2004-04-21 2006-02-02 Univ Minnesota Mapc generation of lung tissue
US8309070B2 (en) 2004-05-17 2012-11-13 Regents Of The University Of Minnesota Use of umbilical cord blood stem cells to treat ischemic event
WO2005114178A1 (en) * 2004-05-21 2005-12-01 Fraunhofer-Gesellschaft zur Förderung der angewandten Forschung e.V. Multi-cellular test systems
WO2006028723A1 (en) * 2004-09-03 2006-03-16 Moraga Biotechnology Inc. Non-embryonic totipotent blastomer-like stem cells and methods therefor
EP1824965B1 (en) * 2004-10-27 2011-10-05 Vrije Universiteit Brussel Hepatic differentiation of stem cells
WO2006049336A1 (en) * 2004-11-05 2006-05-11 Okada, Alan Method of preparing stem cells and tissue remedy
US7875273B2 (en) 2004-12-23 2011-01-25 Ethicon, Incorporated Treatment of Parkinson's disease and related disorders using postpartum derived cells
EP2428563A1 (en) 2005-02-10 2012-03-14 Regents Of The University Of Minnesota Vascular/lymphatic endothelial cells
WO2006121454A3 (en) * 2005-05-05 2008-09-12 Univ Minnesota Use of mapc or progeny therefrom to populate lymphohematopoietic tissues
US8647874B2 (en) 2005-06-16 2014-02-11 Ramot At Tel-Aviv University Ltd. Isolated cells and populations comprising same for the treatment of CNS diseases
WO2006134602A3 (en) * 2005-06-16 2007-03-01 Univ Ramot Isolated cells and populations comprising same for the treatment of cns diseases
US9879225B2 (en) 2005-06-16 2018-01-30 Ramot At Tel-Aviv University Ltd. Isolated cells and populations comprising same for the treatment of CNS diseases
EP2465924A3 (en) * 2005-06-16 2013-01-02 Ramot at Tel-Aviv University Ltd. Isolated cells and populations comprising same for the treament of cns diseases
US10869899B2 (en) 2005-06-16 2020-12-22 Ramot At Tel-Aviv University Ltd. Isolated cells and populations comprising same for the treatment of CNS diseases
WO2007117262A2 (en) * 2005-07-29 2007-10-18 Athersys, Inc. Culture of non-embryonic cells at high cell density
WO2007117262A3 (en) * 2005-07-29 2008-01-10 Athersys Inc Culture of non-embryonic cells at high cell density
KR101423786B1 (en) * 2005-11-09 2014-07-25 오레곤 헬스 앤드 사이언스 유니버시티 Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
US11000546B2 (en) 2005-11-09 2021-05-11 Athersys, Inc. Immunomodulatory properties of MAPCs and uses thereof
EP3808373A1 (en) 2005-11-09 2021-04-21 ABT Holding Company Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
US10117900B2 (en) 2005-11-09 2018-11-06 Athersys, Inc. MAPC treatment of brain injuries and diseases
US11351202B2 (en) 2005-11-09 2022-06-07 Abt Holding Company MAPC treatment of brain injuries and diseases
US11197889B2 (en) 2005-11-09 2021-12-14 Abt Holding Company Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
WO2007056578A1 (en) * 2005-11-09 2007-05-18 Athersys, Inc. Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
EP2684571A1 (en) * 2005-11-09 2014-01-15 Athersys, Inc. Immunomodulatory properties of multipotent adult progenitor cells and uses thereof
WO2007064090A1 (en) 2005-12-02 2007-06-07 Seoul National University Industry Foundation Multipotent adult stem cells having an ability of oct4 expression derived from umbilical cord blood and method for preparing the same
EP1954803A4 (en) * 2005-12-02 2009-03-25 Seoul Nat Univ Ind Foundation Multipotent adult stem cells having an ability of oct4 expression derived from umbilical cord blood and method for preparing the same
EP1954803A1 (en) * 2005-12-02 2008-08-13 Seoul National University Industry Foundation Multipotent adult stem cells having an ability of oct4 expression derived from umbilical cord blood and method for preparing the same
US9175261B2 (en) 2005-12-16 2015-11-03 DePuy Synthes Products, Inc. Human umbilical cord tissue cells for inhibiting adverse immune response in histocompatibility-mismatched transplantation
US11992507B2 (en) 2006-01-23 2024-05-28 Abt Holding Company MAPC therapeutics without adjunctive immunosuppressive treatment
EP3345610A1 (en) 2006-01-23 2018-07-11 Athersys, Inc. Mapc therapeutics without adjunctive immunosuppressive treatment
WO2007087292A2 (en) 2006-01-23 2007-08-02 Athersys, Inc. Mapc treatment of brain injuries and diseases
US9005964B2 (en) 2006-11-24 2015-04-14 Regents Of The University Of Minnesota Endodermal progenitor cells
GB2467982A (en) * 2008-05-08 2010-08-25 Coretherapix Slu Pluripotent adult stem cells
US11185572B2 (en) 2008-05-28 2021-11-30 Ramot At Tel-Aviv University Ltd. Mesenchymal stem cells for the treatment of CNS diseases
US10052363B2 (en) 2008-05-28 2018-08-21 Ramot At Tel-Aviv University Ltd. Mesenchymal stem cells for the treatment of CNS diseases
US8663987B2 (en) 2008-05-28 2014-03-04 Ramot At Tel-Aviv University Ltd. Mesenchymal stem cells for the treatment of CNS diseases
US8900574B2 (en) 2008-05-28 2014-12-02 Ramot At Tel-Aviv University Ltd. Mesenchymal stem cells for the treatment of CNS diseases
US9474787B2 (en) 2008-05-28 2016-10-25 Ramot At Tel-Aviv University Ltd. Mesenchymal stem cells for the treatment of CNS diseases
US8652846B2 (en) 2008-10-13 2014-02-18 Omnicyte Limited Medium derived from stem cells as a pharmaceutical composition
US10179900B2 (en) 2008-12-19 2019-01-15 DePuy Synthes Products, Inc. Conditioned media and methods of making a conditioned media
US10557116B2 (en) 2008-12-19 2020-02-11 DePuy Synthes Products, Inc. Treatment of lung and pulmonary diseases and disorders
US9943552B2 (en) 2009-03-26 2018-04-17 DePuy Synthes Products, Inc. hUTC as therapy for Alzheimer's disease
US9834787B2 (en) 2009-04-09 2017-12-05 Sangamo Therapeutics, Inc. Targeted integration into stem cells
WO2010140464A1 (en) * 2009-06-05 2010-12-09 国立大学法人 熊本大学 Method for induction of cell differentiation
KR101962477B1 (en) * 2009-07-21 2019-03-26 에이비티 홀딩 컴퍼니 Use of stem cells to reduce leukocyte extravasation
EP2456860B1 (en) * 2009-07-21 2018-09-05 ABT Holding Company Use of stem cells to reduce leukocyte extravasation
EP2456860A1 (en) * 2009-07-21 2012-05-30 ABT Holding Company Use of stem cells to reduce leukocyte extravasation
CN104962512A (en) * 2009-07-21 2015-10-07 Abt控股公司 Use of stem cells to reduce leukocyte extravasation
CN104962512B (en) * 2009-07-21 2022-09-09 Abt控股公司 Use of stem cells for reducing leukocyte extravasation
EP2456853A4 (en) * 2009-07-21 2015-08-19 Abt Holding Co Use of stem cells to reduce leukocyte extravasation
EP3831930A1 (en) * 2009-07-21 2021-06-09 ABT Holding Company Use of stem cells to reduce leukocyte extravasation
KR20120098997A (en) * 2009-07-21 2012-09-06 에이비티 홀딩 컴퍼니 Use of stem cells to reduce leukocyte extravasation
WO2011011500A1 (en) 2009-07-21 2011-01-27 Abt Holding Company Use of stem cells to reduce leukocyte extravasation
EP2589389B1 (en) * 2010-07-01 2018-03-07 Aktsionernoe Obschestvo "Pharm-Sintez" Method for producing a biologically active complex. biologically active protein/polypeptide complex
EP2589390B1 (en) * 2010-07-01 2018-03-07 Aktsionernoe Obschestvo "Pharm-Sintez" Pharmaceutical composition for treating central and peripheral nervous system diseases of vascular, traumatic, toxic, hypoxic and autoimmune origin
JP2014503219A (en) * 2011-01-12 2014-02-13 常雄 城戸 A culture method for obtaining and maintaining a pure or enriched population of mammalian neural stem cells and / or neural progenitor cells that are susceptible to differentiation into oligodendrocyte lineage cells in vitro
US9539341B2 (en) 2011-03-30 2017-01-10 Board Of Regents Of The University Of Texas System Methods and compositions for targeting adipose cells in mammals
US9611513B2 (en) 2011-12-23 2017-04-04 DePuy Synthes Products, Inc. Detection of human umbilical cord tissue derived cells
US10724105B2 (en) 2011-12-23 2020-07-28 DePuy Synthes Products, Inc. Detection of human umbilical cord tissue-derived cells
WO2016200340A1 (en) * 2015-06-12 2016-12-15 Agency For Science, Technology And Research Derivation of hepatic stem cells and mature liver cell types and uses thereof
US10683484B2 (en) 2015-06-12 2020-06-16 National University Of Singapore Derivation of hepatic stem cells and mature liver cell types and uses thereof
US11795436B2 (en) 2015-06-12 2023-10-24 Agency For Science, Technology And Research Derivation of hepatic stem cells and mature liver cell types and uses thereof
EP3359169A4 (en) * 2015-10-05 2019-03-13 Orig3N, Inc. Diagnosis and treatment of parkinson's disease based on identification and amelioration of liver dysfunction
WO2017062401A1 (en) 2015-10-05 2017-04-13 ORIG3N Inc. Diagnosis and treatment of parkinson's disease based on identification and amelioration of liver dysfunction
US10842822B2 (en) 2015-10-05 2020-11-24 Orig3N, Inc. Diagnosis and treatment of parkinson's disease based on identification and amelioration of liver dysfunction
WO2020160274A1 (en) 2019-02-01 2020-08-06 Abt Holding Company Multipotent adult progenitor cells for use in treating intracerebral hemorrhage
EP4379046A1 (en) 2022-11-30 2024-06-05 Universidade Nova De Lisboa A 3d cellular model of early diabetic retinopathy
WO2024116114A1 (en) 2022-11-30 2024-06-06 Universidade Nova De Lisboa A 3d cellular model of early diabetic retinopathy

Also Published As

Publication number Publication date
US7838289B2 (en) 2010-11-23
EP1491093B1 (en) 2013-07-31
US20110177595A1 (en) 2011-07-21
EP1491093A3 (en) 2005-05-04
CA2438501C (en) 2014-09-16
CA2438501A1 (en) 2002-08-22
US20050283844A1 (en) 2005-12-22
EP1367899A4 (en) 2004-07-28
WO2002064748A8 (en) 2003-04-24
US20040107453A1 (en) 2004-06-03
IL157332A0 (en) 2004-02-19
JP2004529621A (en) 2004-09-30
IL214623A0 (en) 2011-09-27
EP1367899A2 (en) 2003-12-10
IL214623A (en) 2012-10-31
WO2002064748A3 (en) 2003-08-21
EP1491093A2 (en) 2004-12-29
IL157332A (en) 2011-11-30

Similar Documents

Publication Publication Date Title
US7838289B2 (en) Assay utilizing multipotent adult stem cells
US10638734B2 (en) Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
WO2002064748A9 (en) Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
US20180042968A1 (en) Human cord blood as a source of neural tissue repair of the brain and spinal cord
Stocum Stem cells in regenerative biology and medicine
US10226485B2 (en) Multipotent adult stem cells and methods for isolation
JP2004529621A5 (en)
Dabeva et al. Hepatic stem cells and liver repopulation
AU2001243464A1 (en) Human cord blood as a source of neural tissue for repair of the brain and spinal cord
Sell Stem cells: What are they? Where do they come from? Why are they here? When do they go wrong? Where are they going?
JP2009017891A (en) Multipotent adult stem cell, source thereof, method of obtaining and maintaining the same, method of differentiation thereof, method of use thereof, and cells derived therefrom
Bunting et al. Integrative molecular and developmental biology of adult stem cells
Bunnell et al. Potential application for mesenchymal stem cells in the treatment of cardiovascular diseases
AU2011203281B2 (en) Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
AU2008201936B2 (en) Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
Furcht Multipotent adult stem cells, sources thereof, methods of obtaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
Class et al. Patent application title: Multipotent Adult Stem Cells, Sources Thereof, Methods of Obtaining and Maintaining Same, Methods of Differentiation Thereof, Methods of Use Thereof and Cells Derived Thereof Inventors: Leo T. Furcht (Minneapolis, MN, US) Catherine M. Verfaillie (Leuven, BE) Morayma Reyes (Minneapolis, MN, US) Assignees: ABT Holding Company Regents of the University of Minnesota
AU2002250106A1 (en) Multipotent adult stem cells, sources thereof, methods of obtaining and maintaining same, methods of differentiation thereof, methods of use thereof and cells derived thereof
Tweedell Embryos, clones, and stem cells: a scientific primer
YIJUN Generation of hepatocyte-like cells from mouse embryonic stem (ES) and bone marrow (BM) cells
ES2368809T3 (en) MULTIPOTENT ADULT MOTHER CELLS AND PROCEDURES FOR ISOLATION.

Legal Events

Date Code Title Description
AK Designated states

Kind code of ref document: A2

Designated state(s): AE AG AL AM AT AU AZ BA BB BG BR BY BZ CA CH CN CO CR CU CZ DE DK DM DZ EC EE ES FI GB GD GE GH GM HR HU ID IL IN IS JP KE KG KP KR KZ LC LK LR LS LT LU LV MA MD MG MK MN MW MX MZ NO NZ OM PH PL PT RO RU SD SE SG SI SK SL TJ TM TN TR TT TZ UA UG US UZ VN YU ZA ZM ZW

AL Designated countries for regional patents

Kind code of ref document: A2

Designated state(s): GH GM KE LS MW MZ SD SL SZ TZ UG ZM ZW AM AZ BY KG KZ MD RU TJ TM AT BE CH CY DE DK ES FI FR GB GR IE IT LU MC NL PT SE TR BF BJ CF CG CI CM GA GN GQ GW ML MR NE SN TD TG

121 Ep: the epo has been informed by wipo that ep was designated in this application
CFP Corrected version of a pamphlet front page

Free format text: REVISED ABSTRACT RECEIVED BY THE INTERNATIONAL BUREAU AFTER COMPLETION OF THE TECHNICAL PREPARATIONS FOR INTERNATIONAL PUBLICATION

WWE Wipo information: entry into national phase

Ref document number: 157332

Country of ref document: IL

WWE Wipo information: entry into national phase

Ref document number: 527527

Country of ref document: NZ

WWE Wipo information: entry into national phase

Ref document number: 2003/06289

Country of ref document: ZA

Ref document number: 2438501

Country of ref document: CA

Ref document number: 200306289

Country of ref document: ZA

WWE Wipo information: entry into national phase

Ref document number: 2002565063

Country of ref document: JP

WWE Wipo information: entry into national phase

Ref document number: 2002250106

Country of ref document: AU

WWE Wipo information: entry into national phase

Ref document number: 2002718998

Country of ref document: EP

WWP Wipo information: published in national office

Ref document number: 2002718998

Country of ref document: EP

REG Reference to national code

Ref country code: DE

Ref legal event code: 8642

WWE Wipo information: entry into national phase

Ref document number: 10467963

Country of ref document: US

WWW Wipo information: withdrawn in national office

Ref document number: 2002718998

Country of ref document: EP

DFPE Request for preliminary examination filed prior to expiration of 19th month from priority date (pct application filed before 20040101)
WWP Wipo information: published in national office

Ref document number: 527527

Country of ref document: NZ

WWG Wipo information: grant in national office

Ref document number: 527527

Country of ref document: NZ

COP Corrected version of pamphlet

Free format text: PAGES 1-95, DESCRIPTION, REPLACED BY NEW PAGES 1-225; PAGES 96-105, CLAIMS, REPLACED BY NEW PAGES 226-235

WWE Wipo information: entry into national phase

Ref document number: 214623

Country of ref document: IL