WO2018067504A1 - In vitro drug metabolism reagent and uses thereof - Google Patents

In vitro drug metabolism reagent and uses thereof Download PDF

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WO2018067504A1
WO2018067504A1 PCT/US2017/054853 US2017054853W WO2018067504A1 WO 2018067504 A1 WO2018067504 A1 WO 2018067504A1 US 2017054853 W US2017054853 W US 2017054853W WO 2018067504 A1 WO2018067504 A1 WO 2018067504A1
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reagent
competent cells
cells
metabolically
metabolically competent
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PCT/US2017/054853
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French (fr)
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Albert Li
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Albert Li
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Priority to EP17858983.4A priority Critical patent/EP3519817A4/en
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    • CCHEMISTRY; METALLURGY
    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
    • C12Q1/68Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions involving nucleic acids
    • C12Q1/6876Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes
    • C12Q1/6883Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for diseases caused by alterations of genetic material
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/5005Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving human or animal cells
    • G01N33/5008Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving human or animal cells for testing or evaluating the effect of chemical or biological compounds, e.g. drugs, cosmetics
    • G01N33/5014Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving human or animal cells for testing or evaluating the effect of chemical or biological compounds, e.g. drugs, cosmetics for testing toxicity
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/5005Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving human or animal cells
    • G01N33/5008Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving human or animal cells for testing or evaluating the effect of chemical or biological compounds, e.g. drugs, cosmetics
    • G01N33/502Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving human or animal cells for testing or evaluating the effect of chemical or biological compounds, e.g. drugs, cosmetics for testing non-proliferative effects
    • G01N33/5038Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving human or animal cells for testing or evaluating the effect of chemical or biological compounds, e.g. drugs, cosmetics for testing non-proliferative effects involving detection of metabolites per se
    • GPHYSICS
    • G01MEASURING; TESTING
    • G01NINVESTIGATING OR ANALYSING MATERIALS BY DETERMINING THEIR CHEMICAL OR PHYSICAL PROPERTIES
    • G01N33/00Investigating or analysing materials by specific methods not covered by groups G01N1/00 - G01N31/00
    • G01N33/48Biological material, e.g. blood, urine; Haemocytometers
    • G01N33/50Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing
    • G01N33/5005Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving human or animal cells
    • G01N33/5008Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving human or animal cells for testing or evaluating the effect of chemical or biological compounds, e.g. drugs, cosmetics
    • G01N33/5044Chemical analysis of biological material, e.g. blood, urine; Testing involving biospecific ligand binding methods; Immunological testing involving human or animal cells for testing or evaluating the effect of chemical or biological compounds, e.g. drugs, cosmetics involving specific cell types
    • G01N33/5067Liver cells

Definitions

  • the disclosed inventions relate generally to cryopreserved mixture of metabolically competent cells with a permeabilized plasma membrane and supplemented metabolic enzyme cofactors for use in the evaluation of xenobiotic metabolism.
  • the invention relates to in vitro reagents for evaluating xenobiotic metabolism, methods of manufacturing the reagent and their methods of use for evaluating xenobiotic metabolism and as an exogenous metabolic system for cell culture assays with metabolic incompetent cells (cells that are not capable of xenobiotic metabolism).
  • the parent drug is subjected to metabolism by the small intestine before absorption into the portal circulation and subjected to metabolism by the liver.
  • Drug metabolism is critical to the system half-live of the parent drug due to metabolic elimination, toxicity due to the toxicity of the parent drug and metabolites, and efficacy due to the pharmacological effects of the parent drug and metabolites. Due to species difference in drug metabolism, studies with nonhuman animals do not always provide information useful for the assessment of human outcomes. This is overcome by the use of in vitro human-based experimental systems. Evaluation of drug metabolism using in vitro human-based system is now routinely practiced in drug development.
  • liver homogenates are mainly derived from the human liver as it is a major organ for drug metabolism.
  • Commonly used in vitro experimental systems are liver homogenates and intact hepatocytes.
  • the liver is disrupted by homogenization.
  • the homogenate is first centrifuged at a relative low speed of 9000 or 1000 x g, the resulting supernatant contains both cytosolic and microsomal enzyme and can be used to evaluate both phase I oxidation and phase II conjugation.
  • the supernatant can be centrifuged at a high speed (100,000 x g), resulting in a pellet of endoplasmic reticulum, also referred to as microsomes, which contain one of the most important drug metabolizing enzyme, cytochrome P450.
  • Liver homogenate supernatant commonly referred to as S-9 or S-10
  • liver homogenate systems represent a convenient tool for the evaluation of drug metabolism. Use of the liver homogenate systems such as S9 or microsomes requires the additional of exogenous cofactors to be added at the time of
  • a major disadvantage of the homogenate system is that tissue disruption during the preparation of the homogenates may lead to non-physiological findings that may not represent events in human in vivo.
  • Hepatocytes are isolated from a liver by enzyme digestion (e.g. collagenase digestion) and purified by centrifugation, usually a relative low speed (e.g 50 x g) to remove non-hepatocytes (e.g. kupffer cells and endothelial cells).
  • the 50 x g pellet contains mainly the parenchymal cells or hepatocytes which are the cells responsible for drug metabolism in the liver. Hepatocytes can be used directly after isolation or cryopreserved and stored in liquid nitrogen for use.
  • cryopreservation of hepatocytes to retain viability and function is one of the major reasons for routine application of hepatocytes in experimentation.
  • Cryopreserved hepatocytes from human and non-human animals are commercially available.
  • a scientist can use hepatocytes for experimentation by purchasing the cryopreserved hepatocytes and store them in liquid nitrogen.
  • the cryopreserved hepatocytes are thawed and quantified for viability and cell number, followed by use in experimentation.
  • Cryopreservation of hepatocytes allow this experimental system to be used routinely for the evaluation of drug metabolism, eliminating the need to prepare hepatocytes for each study.
  • liver homogenate-based systems S9, S 10, microsomes
  • hepatocytes A major difference between the use of liver homogenate-based systems (S9, S 10, microsomes) and hepatocytes is that liver homogenates need to be supplemented with enzyme cofactors such as NADPH for oxidative metabolism (e.g. hydroxylation of midazolam by P450 isoform 3A4 to 1-hydroxymidazolam), UDPGA for glucuronidation (e.g. formation of 7-OH coumarin glucuronide from 7-OH-coumarin), and PAPS for sulfation (e.g. formation of 7-OH- coumarin sulfate from 7-OH-coumarin).
  • enzyme cofactors such as NADPH for oxidative metabolism (e.g. hydroxylation of midazolam by P450 isoform 3A4 to 1-hydroxymidazolam)
  • UDPGA for glucuronidation
  • PAPS for sulfation (e.g.
  • S9 or S 10 can be used to evaluate both phase 1 oxidation and conjugation using all three cofactors; microsomes are used mainly for oxidation as most phase II conjugating enzymes are in the cytosol and not in the microsomal membranes.
  • Viable, intact hepatocytes contain endogenous cofactors, and a full complement of hepatic drug metabolizing enzymes. Hepatocytes therefore are considered the gold standard which can be used directly, without adding cofactors, for all hepatic metabolism pathways.
  • This invention is intended to overcome technical challenges required for the application of hepatocytes in drug metabolism.
  • the use of hepatocytes requires specific laboratory equipment such as liquid nitrogen storage system, as the cells need to be store at ⁇ -150 deg. C for long term stability, unlike liver homogenate systems that can be stored in a commonly used laboratory freezer at -20 or -80 deg. C.
  • the hepatocytes require to be purified (e.g. using the Cryopreserved Hepatocyte Recovery Medium, GIBCO or Universal Cryopreservation Recovery Medium, In Vitro ADMET Laboratories), reconstituted, quantified for cell viability, and adjustment of cell density before addition to the reaction mixture for the evaluation of drug metabolism.
  • hepatocyte isolation and cryopreservation may lead to decreases in cofactors required for drug metabolism, thereby leading to activity lower than that in vivo.
  • enterocytes A second organ important for drug metabolism are intestinal mucosal cells or enterocytes.
  • Enterocytes are now known to contain key drug metabolizing enzymes. Enterocytes can be routinely isolated and used for enteric drug metabolism studies as intact cells, akin to intact hepatocytes for the evaluation of hepatic drug metabolism.
  • Enterocyte S9 and enterocyte microsomes are also used as in vitro systems for the evaluation of enteric drug metabolism, similar to hepatic S9 and microsomes for hepatic metabolism. Enterocyte homogenates and intact enterocytes have similar advantages and drawbacks as described above for the corresponding hepatic systems.
  • the invention disclosed herein addresses those deficiencies and provides an improvement for evaluating xenobiotic metabolism using the present in vitro reagent; the invention possesses the advantages of both the tissue homogenates and intact cell models for the evaluation of drug metabolism.
  • this invention produces a reagent that eliminates the need of a liquid nitrogen freezer. The reagent can be used immediately after thawing, eliminating the multiple cell manipulation steps needed for fragile cells such as cryopreserved hepatocytes.
  • Supplementation of cells such as hepatocytes with cofactors allows restoration of the cofactors that have been diminished due to the isolation and cryopreservation processes to physiologically relevant in vivo levels.
  • an in vitro reagent manufacturing of the in vitro reagent and methods for evaluating xenobiotic metabolism using the in vitro reagent.
  • the reagent is a cryopreserved mixture comprising metabolically competent cells wherein cell membranes are permeabilized upon thawing, exogenous drug metabolizing enzyme co-factors, and a buffered solution (e.g., cell culture medium), wherein the reagent does not comprise a cryopreservative agent.
  • the in vitro reagent is thawed wherein the mixture comprises metabolically competent cells with permeabilized plasma membranes.
  • the in vitro reagent is further added to and comprises a metabolically incompetent mammalian or microbial culture, wherein the reagent provides exogenous metabolic functions for evaluation of a physiological effect of metabolites of a xenobiotic.
  • the in vitro reagent comprises co-factors required for biochemical pathways and xenobiotic metabolism.
  • the drug metabolizing enzyme co-factors are selected from ⁇ -nicotinamide adenine dinucleotide 2'-phosphate (NADPH;
  • UDPGA uridine 5'-diphosphoglucuronic acid
  • PAPS 3'-phosphoadenosine 5'-phosphosulfate
  • N- acetyl coenzyme A cofactor for N-acetylation
  • L-glutathione cofactor for glutathione conjugation
  • s-adenosyl methionine amino acids, and carnitine.
  • the metabolically competent cells are primary cells or cell lines, and may be human, rat, monkey, dog, mammals, avian or non-mammalian. In certain embodiments, the metabolically competent cells are from organs responsible for drug metabolism in vivo, such as liver (hepatocytes), intestine (enterocytes) and kidney (renal cells). In embodiments, the metabolically competent cells (primary cells) are pooled from more than one donor. The metabolically competent cells can also be cell lines engineered to contain cytochrome P450 isoforms. In embodiments, the metabolically competent cells comprise drug metabolizing enzyme (DME) activities.
  • DME drug metabolizing enzyme
  • the reagent is provided in a kit and further comprises instructions for evaluating xenobiotic metabolism using the reagent.
  • an in vitro reagent for evaluating xenobiotic metabolism wherein the reagent is a cryopreserved mixture comprising: a) metabolically competent cells selected from hepatocytes or enterocytes wherein cell membranes of the hepatocytes or enterocytes are permeabilized upon thawing; b) exogenous drug
  • metabolizing enzyme co-factors selected from ⁇ -Nicotinamide adenine dinucleotide 2'-phosphate (NADPH), Uridine 5'-diphosphoglucuronic acid (UDPGA), 3'-Phosphoadenosine 5'- phosphosulfate (PAPS), N-acetyl coenzyme A, s-adenosyl methionine, amino acids, carnitine, and L-glutathione; and, c) a buffered solution, wherein the reagent does not comprise a cryopreservative agent.
  • NADPH Uridine 5'-diphosphoglucuronic acid
  • PAPS 3'-Phosphoadenosine 5'- phosphosulfate
  • N-acetyl coenzyme A s-adenosyl methionine, amino acids, carnitine, and L-glutathione
  • a buffered solution wherein the reagent does not comprise a cry
  • the method comprises permeabilizing metabolically competent cells, adding exogenous drug metabolizing enzyme co- factors either before or after the metabolically competent cells are permeabilized and providing a buffered solution (e.g., cell culture medium), wherein the reagent does not comprise a cryopreservative agent.
  • the method further comprises storing the reagent frozen at a temperature of -10°C, or lower, such as at a temperature from about -10°C to about - 80°C.
  • the metabolically competent cells are permeabilized by freezing in the absence of a cryopreservative agent leading to permeabilization upon thawing.
  • the reagent is not stored frozen in liquid nitrogen.
  • the permeabilized metabolically competent cells are not centrifuged prior to use. In other embodiments, the permeabilized metabolically competent cells are not counted prior to use.
  • metabolizing enzyme co-factors in a cell culture medium to form a cell mixture
  • thawing the cell mixture to form the in vitro reagent wherein cell membranes of the metabolically competent cells are permeabilized via thawing.
  • the in vitro reagent is used to evaluate xenobiotic metabolism after thawing without the step of centrifuging or cell counting.
  • provided herein are methods of determining metabolism of a test compound, wherein the method comprises providing a present cyropreserved in vitro reagent, thawing the present in vitro reagent and placing in a cell culture vessel; introducing the xenobiotic test compound into the cell culture vessel, incubating the test compound for 0.5 h to 10 days at 33-40°C and performing an end point assay of the in vitro reagent or cell culture medium to determine metabolism of the xenobiotic test compound.
  • the cell culture vessel comprising the in vitro reagent and test compound is incubated at 37°C.
  • the end point assay comprises an Ames Salmonella histidine reversion assay (Ames test) for genotoxicity, a mammalian or non-mammalian genotoxicity assay, a mammalian or non-mammalian cytotoxicity assay, and/or a mammalian or non- mammalian pharmacological assay.
  • Ames test Salmonella histidine reversion assay
  • the xenobiotic agent is a drug or drug candidate, an industrial chemical and/or environmental pollutant.
  • the drug or drug candidate is selected from the group consisting of an organic compound, an inorganic compound, a hormone, a growth factor, a cytokine, a reception, an antibody, an enzyme, a peptide, an aptomer and a vaccine.
  • step b) thawing the in vitro reagent and placing in a cell culture vessel
  • step e) performing an end point assay of the in vitro reagent or cell culture medium to determine metabolism of the xenobiotic test compound.
  • the cryopreserved in vitro reagent of step a) comprises exogenous drug metabolizing enzyme co-factors used to select metabolism pathways. See Example 13.
  • the present method for determining metabolism of a test compound comprises adding a drug or drug candidate at cytotoxic concentrations for identifying and profiling metabolites. See Example 12.
  • the present method for determining metabolism of a test compound comprises evaluation of complete phase 1 oxidation and phase 2 conjugation of metabolites with the present reagent of step a) (providing the present cryopreserved in vitro reagent). See Example 8.
  • the present methods for determining metabolism of a test compound further comprises evaluating metabolic stability, metabolite profiling and identification, enzyme inhibition or metabolic activation of proto- toxicants or pro-mutagens.
  • the time to perform combined steps a) (providing a present cryopreserved in vitro reagent), b) (thawing the in vitro reagent and placing in a cell culture vessel) and c) (introducing the xenobiotic test compound into the cell culture vessel) takes about 10 minutes or less, such as from about 2 minutes to about 6 minutes.
  • an exogenous metabolic system for evaluation of a physiological effect of metabolites of a xenobiotic test compound
  • the system comprises a cell culture medium admixture of metabolically competent cells comprising permeabilized plasma membranes and exogenous drug metabolizing enzyme co-factors; and metabolically incompetent target cells.
  • the target cells are used to evaluate the metabolites produced by the metabolically competent cells, such as those salmonella bacterial cells used in an Ames test; reporter cell lines for the evaluation of cytotoxicity or pharmacologic effects.
  • the system further comprises a cell culture vessel comprising one or more assay wells, wherein the assay wells comprise the cell culture medium admixture.
  • each assay well is divided into a first and second chamber, wherein a first chamber comprises the cell culture medium admixture and the second chamber comprises the metabolically incompetent target cells provided the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture.
  • the first and second chamber are separated by a porous membrane that is liquid-permeable and cell- impermeable.
  • the metabolically incompetent target cells may be mammalian or non-mammalian, such as bacteria.
  • Figure 1 provides results from metabolism of 7-ethoxycoumarin by human enterocytes with or without exogenous drug metabolizing enzyme co-factors and with or without permeabilization. Highest activity was observed with permeabilized enterocytes with cofactors (Group D; present in vitro reagent). See Example 4
  • Figure 2A and Figure 2B provide measurement of the major P450 isoform activities as a function of cell concentrations.
  • the linear concentration versus activity curves demonstrate that permeabilized hepatocytes can be used routinely as an in vitro drug metabolism system for scientific investigations.
  • Figure 3A and 3B show P450 isoform-selective substrate metabolism in intact human hepatocytes and permeabilized human hepatocytes over a time period of 30 minutes to 240 minutes.
  • Figure 4 shows non-P450 pathway-selective substrate metabolism in intact human hepatocytes and permeabilized human hepatocytes over a time period of 30 minutes to 240 minutes.
  • Figure 5 shows phase 1 oxidation and phase 2 conjugation metabolism of coumarin.
  • Figure 6 shows coumarin metabolite formation and ethoxycoumarin formation in intact human hepatocytes and permeabilized human hepatocytes demonstrating sequential drug metabolism in the permeabilized human hepatocytes measured at 30 min., 60 min., 120 min. and 240 min.
  • Figure 7 shows a comparison of 16 drug metabolizing enzyme (DME) -selective substrates and measurement of metabolites in intact human hepatocytes (open bars) and permeabilized human hepatocytes (solid bars).
  • DME drug metabolizing enzyme
  • Figure 8 shows the advantages of permeabilized hepatocytes and permeabilized enterocytes as compared to cell free systems (S9 and microsomes) or intact hepatocytes and intact enterocytes.
  • the permeabilized hepatocytes and permeabilized enterocytes provide complete representation of organelles as intact hepatocytes and enterocytes.
  • Figure 9 shows the ease of use of the permeabilized hepatocytes and permeabilized enterocytes as compared to cell free systems and intact hepatocytes and intact enterocytes.
  • FIG 11 shows Acetaminophen metabolism (glucuronidation, sulfation and GSH conjugation to the oxidative metabolite NAPQI) at nontoxic (10 mM) and cytotoxic (100 and 200 mM) concentrations in both intact human hepatocytes (open bars) and permeabilized human hepatocytes (solid bars).
  • the permeabilized human hepatocytes can be incubated with high, cytotoxic concentrations of a xenobiotic (e.g. drug or drug candidate) for the generation of metabolites for identification and profiling while significant reduction of metabolite formation was observed in intact hepatocytes due to cytotoxicity.
  • a xenobiotic e.g. drug or drug candidate
  • Figure 12 shows cofactor-directed pathway selection scheme of coumarin metabolism.
  • Figure 13 shows cofactor-directed pathway (no cofactors; NADPH; NADP + PAPS; and, NADPH + UGPGA) selection of coumarin metabolism (7-HC; 7-HCS; and, 7-HCG) in permeabilized human hepatocytes. Selection of exogenous drug metabolizing enzyme co-factors can be used to direct metabolism to specific pathways in the present permeabilized human hepatocytes.
  • Figure 14 shows a scheme of the prototoxicant Acetaminophen activation.
  • Figure 15 shows a scheme of the prototoxicant Cyclophosphamide activation.
  • Figure 16 shows the activation of Acetaminophen using permeabilized human hepatocytes with boiled hepatocytes and no hepatocytes as controls.
  • Figure 17 shows the activation of Cyclophosphamide and Ifosfamine using permeabilized human hepatocytes with boiled hepatocytes and no hepatocytes as controls.
  • Figure 18 shows the versatility of using permeabilized hepatocytes
  • permeabilized enterocytes as compared to cell free systems (S9 and microsomes) or intact hepatocytes and intact enterocytes.
  • Figure 19 shows the steps of using permeabilized hepatocytes and permeabilized enterocytes as compared to cryopreserved intact hepatocytes and intact enterocytes.
  • Figure 20 shows CYP3A4 activity by permeabilized human enterocytes upon treatment by various concentrations of herbal supplements.
  • the composition is an in vitro reagent that provides improved means for testing xenobiotic metabolism, such as a drug or drug candidate.
  • the in vitro reagent is a cryopreserved mixture comprising metabolically competent cells (wherein cell membranes are permeabilized upon thawing;), exogenous drug metabolizing co-factors and a buffer solution such as cell culture medium, wherein the reagent does not comprise a cryopreservative agent.
  • the in vitro reagent is frozen (e.g.
  • cryopreserved and comprises metabolically competent cells, exogenous drug metabolizing co-factors and cell culture medium, wherein the metabolically competent cells are permeabilized when thawed provided the in vitro reagent does not comprise a cryopreservative.
  • the thawed in vitro reagent comprises metabolically competent cells with permeabilized plasma membranes, exogenous drug metabolizing co-factors and a buffer solution, wherein the metabolically competent cells are permeabilized via thawing.
  • cryopreserved refers to preserving a mixture of cells and enzyme co-factors (i.e. present in vitro reagent) that has been frozen at a temperature of about -10°C or less, such as about -20°C to about -80°C, in the absence of a cryopreservative agent.
  • the present in vitro reagent comprising permeabilized metabolically competent cells permeabilized via thawing of the cryopreserved intact metabolically competent cells provides benefits and advantages over use of organelle systems, intact cells and even metabolically competent cells permeabilized by other methods (e.g. sonication and/or detergent).
  • Permeability induced by freezing without cryopreservative allows minimum disturbance to cellular integrity. Previous methods using a detergent (saponin) and/or extensive sonication cause total cell disruption, including disruption of the organelles.
  • permeability induced by freezing without cryopreservative allows the evaluation of drug metabolism in cells with near intact cell integrity but with permeable membrane; thereby the present in vitro reagent and methods are physiologically more relevant.
  • an in vitro reagent comprising metabolically competent cells that are permeabilized upon thawing and
  • the present metabolically competent cells were not permeabilized via mechanical or detergent means.
  • the present in vitro reagent comprised of intact, permeabilized metabolically competent cells and exogenous drug metabolizing enzyme co-factors, represent a complete system with all the drug metabolizing enzymes as intact hepatocytes or intact enterocytes which is the major drawback of tissue homogenate systems such as S9 or microsomes (discussed in the Background section).
  • the metabolically competent cells are permeabilized to allow
  • the present in vitro reagent can be stored in a regular laboratory freezer at -10 or -80°C, without a need for liquid nitrogen freezers.
  • the in vitro reagent can be thawed and use directly, without a need to supplement with cofactors, such as those needed for S9 and microsomes, and without a need for cell recovery/viability determination/cell density adjustment as needed when intact hepatocytes are used.
  • the present in vitro reagent thereby has the advantage of the physiological relevance of, for example, intact hepatocytes and the ease of use of liver microsomes.
  • the composition is an exogenous metabolic system, wherein the system comprises: a) a cell culture medium admixture comprising; i) metabolically competent cells comprising permeabilized plasma membranes; and, ii) exogenous drug metabolizing enzyme co-factors, and b) metabolically incompetent target cells.
  • the cell culture admixture is also referred to herein as the thawed in vitro reagent.
  • the thawed in vitro reagent is added to a cell culture assay comprising metabolically incompetent target cells followed by addition of the test compound, incubation for a designated time duration, and quantification of the designated biological effects in the target cells, thereby allowing the evaluation of the effects of both the parent the metabolites.
  • the exogenous metabolic system comprises a separation between the cell culture admixture and the metabolically incompetent cells.
  • the exogenous metabolic system may further comprise a cell culture vessel comprising one or more assay wells, wherein the assay wells comprise the cell culture medium admixture.
  • the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture wherein, for example, each assay well is divided into a first and second chamber, wherein a first chamber comprises the cell culture medium admixture and the second chamber comprises the metabolically incompetent target cells provided the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture.
  • the present in vitro reagent, and its use in an exogenous metabolic system provides advantages as compared to the use of intact metabolically competent cells or homogenates of those cells that require the use of enzyme co-factors.
  • Those advantages include but are not limited to, A) increased drug metabolizing enzyme activity; B) increased efficiency wherein the permeabilized metabolically competent cells admixed with exogenous drug metabolizing co- factors can be used directly, without centrifugation and cell counting ⁇ See Figure 1 and Example 4); and C) improved access for researchers wherein the in vitro reagent can be stored in a freezer at -10°C or -80°C, rather than in liquid nitrogen as needed for intact hepatocytes, allowing researchers without assess to liquid nitrogen storage systems use of the instant in vitro reagent.
  • the metabolically competent cells are cryopreserved with the exogenous drug metabolizing co-factors and may be used directly to evaluate xenobiotic metabolism.
  • the metabolically competent cells are permeabilized when they are cryopreserved in the absence of a cryoprotectant, which induces membrane permeability when the cells are thawed. Once thawed, the cells may be used directly without a step of cell counting or centrifugation. The amount of time from thawing to adding of a test compound may be from about 2 minutes to about 7 minutes, or less than about 6 minutes. See Figure 19.
  • the in vitro reagent does not comprise a cryopreservative agent.
  • the metabolically competent cells may be permeabilized prior to cryopreservation. In that instance, the in vitro reagent may comprise a cryopreservative agent.
  • the in vitro reagent comprises metabolically competent cells, exogenous drug metabolizing co-factors and a buffer solution such as a cell culture medium, wherein the co-factors are admixed with the competent cells in the cell culture medium and then the admixture is cryopreserved; also referred to herein as a cryopreserved mixture.
  • a buffer solution such as a cell culture medium
  • the in vitro reagent is stored at a temperature of -10°C or less, such as about -10°C to about -80°C.
  • the exogenous drug metabolizing co-factors include, but are not limited to those for oxidative metabolism, glucuronidation or sulfation.
  • the in vitro reagent comprises, individually or in combination, ⁇ -nicotinamide adenine dinucleotide 2'-phosphate (NADPH) for oxidative metabolism, uridine 5'-diphosphoglucuronic acid
  • UDPGA glucuronidation and/or 3'-phosphoadenosine 5'-phosphosulfate (PAPS) for sulfation, N-acetyl coenzyme A, s-adenosyl methionine, amino acids, carnitine, and L- glutathione.
  • PAPS 3'-phosphoadenosine 5'-phosphosulfate
  • drug is used generically in the term “drug metabolizing enzyme co-factors” and is understood to broadly mean xenobiotic.
  • the in vitro reagent comprises co-factors required for biochemical pathways and xenobiotic metabolism.
  • the manufacturing of the instant in vitro reagent is carried out by permeabilizing metabolically competent cells and adding exogenous drug metabolizing enzyme co-factors either before or after the metabolically competent cells are permeabilized, wherein the in vitro reagent is provided in a cell culture medium.
  • the metabolically competent cells are frozen without a cryoprotectant (also referred to herein as a cryopreservative) wherein they are permeabilized during thaw of the in vitro reagent.
  • the metabolically competent cells are admixed with the exogenous drug metabolizing co-factors in the presence of cell culture medium.
  • a cryoprotectant or cryopreservative is a substance that prevents damage to cells and/or organelles during freezing, and includes but is not limited to glycols; such as glycerol, ethylene glycol and propylene glycol; and dimethyl sulfoxide (DMSO).
  • the in vitro reagent does not comprise glycerol and/or DMSO.
  • the in vitro reagent is stored without serum, in other words the frozen in vitro reagent is serum free.
  • the in vitro reagent is frozen at a temperature of -10°C or less (e.g. from about -10°C to about -80°C), and does not comprise glycerol and/or DMSO and/or serum.
  • the methods of use herein are carried out by addition of a xenobiotic test compound or test article to the thawed in vitro reagent (admixture of metabolically competent cells with permeabilized plasma membranes and enzyme co-factors), i.e. room temperature (e.g. about 20 to 25°C) to about a physiological temperature (e.g. about 35°C to 40°C), in a cell culture vessel.
  • the test compound is introduced into the cell culture vessel comprising the thawed in vitro reagent, incubated, followed by evaluation of the effects of metabolism on the test compound including quantification of the parent compound for the evaluation of metabolic stability; metabolite quantification and identification; evaluation of drug metabolizing enzyme (e.g. P450) activity for evaluation of drug-drug interaction potential.
  • the reagent is also used as an exogenous metabolic system in conjunction with a cell culture system comprising
  • a xenobiotic test compound or test article is added as an exogenous metabolic system, which comprises a thawed in vitro reagent (i.e. a cell culture medium admixture comprising metabolically competent cells comprising permeabilized plasma membranes and exogenous drug metabolizing enzyme co-factors) and metabolically incompetent target cells.
  • a thawed in vitro reagent i.e. a cell culture medium admixture comprising metabolically competent cells comprising permeabilized plasma membranes and exogenous drug metabolizing enzyme co-factors
  • metabolically incompetent target cells i.e. a cell culture medium admixture comprising metabolically competent cells comprising permeabilized plasma membranes and exogenous drug metabolizing enzyme co-factors
  • the cell culture medium, the metabolically competent cells or the metabolically incompetent cells are subjected to the end point analysis to determine metabolism of the xenobiotic test compound and any effects of the metabolites thereof.
  • test compounds used in the present invention include, but are not limited to drugs, drug candidates, biologicals, food components, herb or plant components, proteins, peptides, oligonucleotides, DNA and RNA.
  • the test compound is a drug, a drug candidate, an industrial chemical, an environmental pollutant, a pesticide, an insecticide, a biological chemical, a vaccine preparation, a cytotoxic chemical, a mutagen, a hormone, an inhibitory compound, a chemotherapeutic agent or a chemical.
  • the drug or drug candidate is selected from the group consisting of an organic compound, an inorganic compound, a hormone, a growth factor, a cytokine, a reception, an antibody, an enzyme, a peptide, an aptamer or a vaccine.
  • the test compound can be either naturally-occurring or synthetic, and can be organic or inorganic. A person skilled in the art will recognize that the test compound can be added to the in vitro reagent present in the cell culture medium in an appropriate solvent or buffer.
  • the in vitro reagent and/or exogenous metabolic system is used for high-throughput screening to test the metabolic effects or response to a range of test compounds.
  • the in vitro reagent may be used with a cell culture vessel that is a multi-well plate, such as a 6-well; 12-well; 24-well; 48-well, 96-well; 384-well, 1536-well plate or any combination thereof.
  • the methods use a cell culture vessel with a single assay well.
  • the metabolic system comprises a cell culture vessel wherein the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture.
  • the cell culture vessel comprises one or more assay wells, wherein the assay wells comprise the cell culture medium admixture and the metabolically incompetent cells in the same admixture.
  • each assay well is divided into a first and second chamber, wherein a first chamber comprises the cell culture medium admixture and the second chamber comprises the metabolically incompetent target cells provided the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture.
  • the first and second chamber are separated by a porous membrane that is liquid-permeable and cell-impermeable.
  • the exogenous metabolic system comprises a cell culture vessel with a single well plate.
  • the exogenous metabolic system comprises cell culture vessel that is a multi-well plate.
  • the porous membrane separating the first and second chamber of the cell culture vessel comprises polyethylene terephthalate (PET), polycarbonate, polystyrene, polypropylene, nylon, Mylar, stainless steel, wire mesh, aluminum, synthetic mesh, plastic, or paper.
  • the cell culture insert is a transwell.
  • the metabolically competent cells are primary cells or cell lines; and can be human, rat, monkey, dog, mammals, avian or non-mammalian cells.
  • the metabolically competent cells are from organs responsible for drug metabolism in vivo, such as liver (hepatocytes), intestine (enterocytes) and kidney (renal cells).
  • the metabolically competent cells are human hepatocytes. See, Li, A. P. (2007) Human hepatocytes: isolation, cryopreservation and applications in drug development. Chemico-biological interactions, 168(1), 16-29. Freshly prepared metabolically competent cells or cryopreserved cells (e.g.
  • hepatocytes obtained by standard methods from a human or animal liver can be used as the metabolically competent cells. See, Hewitt, Nicola J., et al. "Primary hepatocytes: current understanding of the regulation of metabolic enzymes and transporter proteins, and pharmaceutical practice for the use of hepatocytes in metabolism, enzyme induction, transport, clearance, and hep ato toxicity studies.” Drug metabolism reviews 39.1 (2007): 159-234.
  • the metabolically competent cells are hepatocytes (the parenchymal cells of the liver). Hepatic metabolism is known to be the major determinant of
  • phase 1 oxidation enzyme pathways are responsible mostly for the bioactivation of relatively inert parent compounds to reactive (toxic/carcinogenic/mutagenic) metabolites.
  • Phase 2 conjugating pathways are responsible mostly for the biotransformation of toxic parent compounds or metabolites to less toxic compounds. Both phase 1 and phase 2 pathways are present in the hepatocytes - the key hepatic cell type responsible for hepatic metabolism.
  • enterocytes can be used to model enteric metabolism for orally ingested toxicants.
  • renal proximal tubule cells can be used to model renal metabolism.
  • enterocytes can be used to model intestinal metabolism.
  • the metabolically competent cells are recombinant cells, wherein for example, they have been engineered to comprise drug metabolizing enzymes.
  • the metabolically competent cells are engineered to contain cytochrome P450 isoforms. See, Doehmer, J., Battula, N., Wolfel, C, Kudla, C, Keita, Y. and Staib, A.H., 1992. Biotransformation of caffeine and theophylline in mammalian cell lines genetically engineered for expression of single cytochrome P450 isoforms. Biochemical pharmacology, 43(2), pp.225-235; Donato, M. T., Jimenez, N., Castell, J.
  • a stable cell line such as HepG2 is used in the present in vitro reagent and methods for determining metabolism of a test compound.
  • HepG2 is a perpetual cell line derived from the liver of a 15-year-old Caucasian male with a well-differentiated
  • HepG2 cells can be a suitable model to study the intracellular trafficking and dynamics of bile canalicular and sinusoidal membrane proteins and lipids in human hepatocytes in vitro. See, Aprke et al., WIF-B cells: an in vitro model for studies of hepatocyte polarity. Journal of Cell Biology 123 (6), 1761-1775, 1993.
  • a stable cell line such as HepaRG is used in the present in vitro reagent and methods for determining metabolism of a test compound.
  • the human hepatoma HepaRG cells a highly differentiated model for studies of liver metabolism and toxicity of xenobiotics. Chemico-biological interactions, 168(1), pp.66-73.
  • present metabolically competent cells are genetically altered or modified so as to contain a non-native "recombinant” (also called “exogenous”) nucleic acid sequence, or modified by antisense technology to provide a gain or loss of genetic function.
  • recombinant also called “exogenous” nucleic acid sequence
  • antisense technology to provide a gain or loss of genetic function.
  • cells refers to metabolically competent cells.
  • the present in vitro reagent may comprise any cell type, including primary cells, stem cells, progenitor cells, normal, genetically-modified, genetically altered, immortalized, and transformed cell lines, provided the cells are metabolically competent, permeabilized (permeabilized during thaw), and admixed with exogenous drug metabolizing enzyme co-factors.
  • the present invention is suitable for use with single cell types or cell lines, or with combinations of different cell types.
  • the cultured cells maintain the ability to respond to stimuli that elicit a response in their naturally occurring counterparts. These may be derived from all sources such as eukaryotic (mammalian and non-mammalian).
  • the eukaryotic cells can be animal in nature, such as human, simian, or rodent. They may be of any tissue type (e.g., heart, stomach, kidney, intestine, lung, liver, fat, bone, cartilage, skeletal muscle, smooth muscle, cardiac muscle, bone marrow, muscle, brain, pancreas), and cell type (e.g., epithelial, endothelial, mesenchymal, adipocyte, hematopoietic).
  • tissue type e.g., heart, stomach, kidney, intestine, lung, liver, fat, bone, cartilage, skeletal muscle, smooth muscle, cardiac muscle, bone marrow, muscle, brain, pancreas
  • cell type e.g., epithelial, endothelial, mesenchymal, adipocyte, hematopoietic.
  • metabolically competent cells are cultured from a variety of genetically diverse individuals who may respond differently to biologic and pharmacologic agents. Genetic diversity can have indirect and direct effects on metabolism of a test compound.
  • the metabolically competent cells are a pool of cells from multiple individuals or donors.
  • the metabolically competent cells are reflective of the heterogeneity of a population of individuals.
  • an exogenous metabolic system comprises metabolically
  • the metabolically incompetent cells are mammalian or non-mammalian and include, but are not limited to carbiomyocytes (Doherty, Kimberly R., Robert L. Wappel, Kevin R. Talbert, Patricia B. Trusk, Diarmuid M. Moran, James W. Kramer, Arthur M. Brown, Scott A. Shell, and Sarah Bacus. "Multiparameter in vitro toxicity testing of crizotinib, sunitinib, erlotinib, and nilotinib in human cardiomyocytes.
  • EEC/COLIPA project on in vitro phototoxicity testing: First results obtained with a Balb/c 3T3 cell phototoxicity assay. Toxicology in vitro, 8(4), pp.793-796) and Chinese hamster ovary cells (Li, A.
  • examples include reporter cell lines for endocrine disruption, but are not limited to metabolically incompetent cells disclosed in the following references: Willemsen, P., Scippo, M.L., Kausel, G., Figueroa, J., Maghuin-Rogister, G., Martial, J. A. and Muller, M., 2004. Use of reporter cell lines for detection of endocrine-disrupter activity. Analytical and bioanalytical chemistry, 378(3), pp.655-663), Genotoxicity determination with the Ames salmonella typhimurium gene mutation assay; De Flora, S., Zanacchi, P., Camoirano, A., Bennicelli, C.
  • examples of metabolically incompetent cells include mammalian cell lines used for genotoxicity assays, but are not limited to metabolically incompetent cells disclosed in the following references: Moore, Martha M., et al. "Mouse lymphoma thymidine kinase gene mutation assay: Follow-up meeting of the international workshop on Genotoxicity testing— Aberdeen, Scotland, 2003— Assay acceptance criteria, positive controls, and data evaluation.”
  • examples of metabolically incompetent cells include nonhepatic primary cells for the evaluation of organ- specific dr g toxicity, but are not limited to
  • the in vitro reagent comprising metabolically competent cells and exogenous drug metabolizing enzyme co-factors are thawed and placed in a cell culture vessel with cell culture medium. If using the exogenous metabolic system, the system further comprises metabolically in competent cells in fluid communication with the thawed in vitro reagent.
  • culture condition encompasses cells, media, factors, time and temperature, atmospheric conditions, pH, salt composition, minerals, etc. Cell culturing is typically performed in a sterile environment mimicking physiological conditions, for example, at 37°C in an incubator containing a humidified 92-95% air/5-8% CO2 atmosphere.
  • the cell culture temperate is a range from 33-40°C.
  • Cell culturing may be carried out in nutrient mixtures containing undefined biological fluids such a fetal calf serum, or media that is fully defined and serum free.
  • undefined biological fluids such as a fetal calf serum, or media that is fully defined and serum free.
  • a variety of culture media are known in the art and are commercially available.
  • the metabolically competent cells are not checked for viability, centrifuged, counted or cultured prior to addition of the xenobiotic test compound.
  • the in vitro reagent may be cultured for a time period from a few hours to days prior to use in the instant methods.
  • the xenobiotic test compound is placed in the cell culture vessel wherein the thawed in vitro reagent (i.e. cell culture medium admixture comprising permeabilized metabolically competent cells and exogenous drug metabolizing enzyme co-factors) is then incubated under appropriate cell culture conditions as disclosed herein for a time period of 30 minutes to up to 10 days.
  • the incubation period can be at least 1 hours, 2 hours, 5 hours, 10 hours, 15 hours, 24 hours, 2 days, 3 days, 4 days, 5 days, 6 days, 7 days, 8 days, 9 days or at least 10 days.
  • the incubation time period is not longer than 1 day, 2 days, 5 days, 6 days, 7 days, 8 days, 9 days or not longer than 10 days.
  • the cell culture conditions replicate physiological conditions as much as possible.
  • physiological conditions as used herein is defined to mean that the cell culturing conditions are very specifically monitored to mimic as closely as possible the natural tissue conditions for a particular type of cell in vivo.
  • the xenobiotic test compound is considered an input variable, and is used interchangeably herein with a test compound.
  • the test compounds are screened for biological activity by adding to a pharmacokinetic -based culture system (e.g. present in vitro reagent), and then assessing the metabolically competent cells (or culture medium) for changes in output variables of interest, e.g., consumption of O2, production of CO2, cell viability, expression of proteins of interest (protein expression), cell function, expression of genes of interest (gene expression), metabolite formation or metabolite profiles.
  • the test compound is typically added in solution, or readily soluble form, to the medium of cells in culture.
  • the test compound can be added using a flow through system, or alternatively, adding a bolus to an otherwise static solution.
  • a flow-through system two fluids are used, where one is a physiologically neutral solution, and the other is the same solution with the test compound added. The first fluid is passed over the cells, followed by the second.
  • a bolus of the test compound is added to the volume of medium surrounding the cells. The overall composition of the culture medium should not change significantly with the addition of the bolus, or between the two solutions in a flow through method.
  • test compound includes pharmacologically active drugs or drug candidates and genetically active molecules.
  • Test compounds of interest include
  • chemotherapeutic agents anti-inflammatory agents, hormones or hormone antagonists, ion channel modifiers, and neuroactive agents.
  • exemplary of pharmaceutical agents suitable for this invention are those described in "The Pharmacological Basis of Therapeutics," Goodman and Gilman, McGraw-Hill, New York, N.Y., (1996), Ninth edition, under the sections: Drugs Acting at Synaptic and Neuroeffector Junctional Sites; Drugs Acting on the Central Nervous System; Autacoids: Drug Therapy of Inflammation; Water, Salts and Ions; Drugs Affecting Renal Function and Electrolyte Metabolism; Cardiovascular Drugs; Drugs Affecting Gastrointestinal Function; Drugs Affecting Uterine Motility; Chemotherapy of Parasitic Infections;
  • Chemotherapy of Microbial Diseases Chemotherapy of Neoplastic Diseases; Drugs Used for Immunosuppression; Drugs Acting on Blood-Forming Organs; Hormones and Hormone Antagonists; Vitamins, Dermatology; and Toxicology, all incorporated herein by reference.
  • toxins Also included are toxins, and biological and chemical warfare agents, for example see Somani, S. M. (Ed.), "Chemical Warfare Agents,” Academic Press, New York, 1992).
  • test compound includes all of the classes of molecules disclosed herein, and may further or separately comprise samples of unknown content. While many samples will comprise compounds in solution, solid samples that can be dissolved in a suitable solvent may also be assayed. Samples containing test compounds of interest include
  • Samples of interest include test compounds being assessed for potential therapeutic value, e.g., drug candidates from plant or fungal cells.
  • Test compounds are obtained from a wide variety of sources including libraries of synthetic or natural compounds. For example, numerous means are available for random and directed synthesis of a wide variety of organic compounds and biomolecules, including expression of randomized oligonucleotides and oligopeptides. Alternatively, libraries of natural compounds in the form of bacterial, fungal, plant and animal extracts are available or readily produced. Additionally, naturally or synthetically produced libraries and compounds are readily modified through conventional chemical, physical and biochemical means, and may be used to produce combinatorial libraries. Known pharmacological agents may be subjected to directed or random chemical modifications, such as acylation, alkylation, esterification, amidification to produce structural analogs.
  • an end point analysis is performed to determine the effect of the test compound on the metabolically competent cells.
  • the end point analysis identifies the output variable (e.g. the effect of the test compound) of the in vitro reagent.
  • output variables are quantifiable elements of the cells, particularly elements that can be accurately measured in a cell culture system.
  • An output variable can be any cell component or cell product including, e.g., viability, respiration, metabolism, cell surface determinant, receptor, protein or conformational or posttranslational modification thereof, lipid, carbohydrate, organic or inorganic molecule, mRNA, DNA, or a portion derived from such a cell component.
  • the output variable is directly or indirectly a result of the test compound or its metabolite. While most output variables will provide a quantitative readout, in some instances a semi-quantitative or qualitative result will be obtained. Readouts may include a single determined value, or may include mean, median value or the variance. Characteristically a range of readout values will be obtained for each output. Variability is expected and a range of values for a set of test outputs can be established using standard statistical methods.
  • the end point assay is an Ames Salmonella histidine reversion assay (Ames test) for genotoxicity, a mammalian or non-mammalian genotoxicity assay, a mammalian or non-mammalian pharmacological assay.
  • Ames test Salmonella histidine reversion assay
  • Various methods can be utilized for quantifying the presence of selected metabolism markers. Liquid chromatography (LC), mass spectrometry (MS), and their combination
  • LC/MS-MS are routinely used for the quantification of metabolites.
  • a convenient method is to label the molecule with a detectable moiety, which may be fluorescent, luminescent, radioactive, or enzymatically active. Fluorescent and luminescent moieties are readily available for labeling virtually any biomolecule, structure, or cell type. Immunofluorescent moieties can be directed to bind not only to specific proteins but also specific conformations, cleavage products, or site modifications like phosphorylation.
  • peptides and proteins can be engineered to autofluoresce, e.g., by expressing them as green fluorescent protein chimeras inside cells (for a review, See Jones et al. (1999) Trends Biotechnol. 17(12):477-81).
  • Output variables may be measured by immunoassay techniques such as,
  • RIA radioimmunoassay
  • ELISA enzyme linked immunosorbance assay
  • Cell based ELISA or related non-enzymatic or fluorescence-based methods enable measurement of cell surface parameters. Readouts from such assays may be the mean fluorescence associated with individual fluorescent antibody-detected cell surface molecules or cytokines, or the average fluorescence intensity, the median fluorescence intensity, the variance in fluorescence intensity, or some relationship among these.
  • outputs can include measurement of cell viability such as enzyme release, cellular ATP contents, reactive oxygen species formation, decrease of reduced glutathione, protein synthesis, protein contents, DNA contents, dye exclusion, dye inclusion, and cell detachment.
  • cell viability such as enzyme release, cellular ATP contents, reactive oxygen species formation, decrease of reduced glutathione, protein synthesis, protein contents, DNA contents, dye exclusion, dye inclusion, and cell detachment.
  • pharmacological assays specific disease target related assays can be used.
  • endpoints measured may include DNA damage, chromosomal aberration, mutant generation, and induction of DNA repair.
  • the results of screening assays may be compared to results obtained from a reference compound, concentration curves, controls (with and without metabolically competent cells), etc.
  • the comparison of results is accomplished by the use of suitable deduction protocols, Al systems, statistical comparisons, etc.
  • a database of reference output data can be compiled. These databases may include results from known agents or combinations of agents, as well as references from the analysis of cells treated under environmental conditions in which single or multiple environmental conditions or parameters are removed or specifically altered.
  • a data matrix may be generated, where each point of the data matrix corresponds to a readout from an output variable, where data for each output may come from replicate determinations, e.g., multiple individual cells of the same type.
  • the readout may be a mean, average, median or the variance or other statistically or mathematically derived value associated with the measurement.
  • the output readout information may be further refined by direct comparison with the corresponding reference readout.
  • the absolute values obtained for each output under identical conditions will display a variability that is inherent in live biological systems and also reflects individual cellular variability as well as the variability inherent between individuals.
  • the in vitro reagent is a cryopreserved mixture comprising metabolically competent cells (cells wherein cell membranes are permeabilized upon thawing), exogenous drug metabolizing enzyme co-factors and a buffered solution such as cell culture medium, wherein the reagent does not comprise a cryopreservative agent.
  • metabolically competent cells cells wherein cell membranes are permeabilized upon thawing
  • exogenous drug metabolizing enzyme co-factors and a buffered solution such as cell culture medium
  • a buffered solution such as cell culture medium
  • the present in vitro reagent is prepared for use to evaluate the metabolic effects of a test compound using cryopreserved metabolically competent cells with a permeabilized cell membrane, comprising the following steps: A) permeabilizing metabolically competent cells (e.g. hepatocytes or enterocytes); B) adding exogenous drug metabolizing enzyme co-factors either before or after the metabolically competent cells are permeabilized (e.g. NADPH, UDPGA, and PAPS); C) providing a cell culture medium.
  • the in vitro reagent is further stored at a temperature of -10°C or lower.
  • the cell membrane of the metabolically competent cells is permeabilized when thawed.
  • the present in vitro reagent is used to evaluate the metabolic effects of a xenobiotic test compound comprising the following steps: A) thawing the in vitro reagent (prepared as disclosed herein) and placing in a cell culture vessel; B) introducing the xenobiotic test compound into the cell culture vessel; C) incubating the test compound for 0.5 h to 10 days at 33-40°C; and; D) performing an end point assay of the in vitro reagent or cell culture medium to determine metabolism of the xenobiotic test compound. See Examples 1-15 and Figures 1-20.
  • Example 1 In vitro reagent containing permeabilized hepatocytes for the evaluation of a xenobiotic test compound.
  • Hepatocytes are isolated from human livers by collagena.se digestion.
  • the hepatocytes may be utilized from a single donor, or pooled from multiple donors.
  • the hepatocytes are then cryopreserved in a serum free cell culture medium (Hepatocyte Incubation Medium (HQM), In Vitro ADMET Laboratories Inc., Columbia, MD)) in the presence of drug metabolizing enzyme cof actors: 2 niM NADPH, 5 mM UDPGA, and 1 mM PAPS at a concentration of 1 mil lion cells per mL.
  • the cells are ali quoted at 5 raL aliquots and frozen in a -80 deg. C freezer.
  • the hepatocyte/cofactor mixture i.e. in vitro reagent
  • 50 ih of the mixture is added to 50 xL of HQM containing a xenobiotic test article at an appropriate concentration in wells of a 96-well plate.
  • the plate is incubated in a ceil culture incubator maintained at 37°C for a specific time period (e.g. 60 minutes) after which an organic solvent (e.g. acetonitrile) as added at a volume of 100 ⁇ lL to each well.
  • an organic solvent e.g. acetonitrile
  • the hepatocytes are isolated from human livers by collagenase digestion and pooled from multiple donors to manufacture the present in vitro reagent containing permeabilized hepatocytes.
  • Example 2 In vitro reagent containing permeabilized enterocytes for the evaluation of a xenobiotic test compound
  • enterocytes are isolated from human intestines by collagenase digestion.
  • the enterocytes may be utilized from a single donor, or pooled from multiple donors.
  • the enterocytes are then cryopreserved in a serum free cell culture medium in the presence of drug metabolizing enzyme cof actors: 2 mM NADPH, 5 mM UDPGA, and 1 mM PAPS at a concentration of 1 mil lion cells per mL.
  • the cells are aliquoted at 5 mL aliquots and frozen in a -80 deg. C freezer. On the day of use, the
  • enterocyte/cofactor mixture i.e. in vitro reagent
  • enterocyte/cofactor mixture i.e. in vitro reagent
  • 50 , u,L of HQM containing a xenobiotic test article at an appropriate concentration in wells of a 96-well plate.
  • the plate is incubated in a cell culture incubator maintained a 37°C for a specific time period (e.g. 60 minutes) after which an organic solvent (e.g. acetonitrile) as added at a volume of 100 ⁇ . to each well.
  • an organic solvent e.g. acetonitrile
  • the enterocytes are isolated from human intestines by collagenase digestion and pooled from multiple donors to manufacture the present in vitro reagent containing permeabilized enterocytes.
  • Example 3 In vitro reagent containing permeabilized hepatocyte cell line for the evaluation of a xenobiotic test compound
  • the assay was performed essentially as disclosed in Example 1, except a hepatocyte cell line (e.g. HepaRG) known to contain drug metabolizing enzyme activity is used instead of primary hepatocytes.
  • the hepatocyte cell line is cryopreserved in a serum free cell culture medium (Hepatocyte Incubation Medium (HQM), In Vitro ADMET Laboratories Inc.,
  • hepatocyte/cofactor mixture i.e. in vitro reagent
  • 50 lL of the mixture is added to 50 ⁇ , of HQM containing a xenobiotic test article at an appropriate concentration in wells of a 96-well plate.
  • the plate is incubated in a cell culture incubator maintained at 37°C for a specific time period (e.g. 60 minutes) after which an organic solvent (e.g. acetonitrile) as added at a volume of 100 uL to each well.
  • an organic solvent e.g. acetonitrile
  • the contents of the wells are collected for LC/MS-MS quantification of drug metabolism (e.g. parent disappearance; metabolite formation).
  • Example 4 Comparison of the in vitro reagent as compared to intact (non- permeabilized) metabolically competent cells (with or without enzyme co-factor added to the intact cells)
  • the assay was performed essentially as disclosed in Example 2, wherein the in vitro reagent comprises enterocytes and exogenous drug metabolizing enzyme co-factors (NADPH, UPGA, and PAPS), herein referred to as "cofactors".
  • the in vitro reagent comprises enterocytes and exogenous drug metabolizing enzyme co-factors (NADPH, UPGA, and PAPS), herein referred to as "cofactors”.
  • NADPH exogenous drug metabolizing enzyme co-factors
  • UPGA exogenous drug metabolizing enzyme co-factors
  • test groups were: Group A - intact enterocytes incubated without cofactors; Group B - intact enterocytes incubated with cofactors; Group C - permeabilized enterocytes incubated without cofactors (control); Group D - the in vitro reagent (permeabilized enterocytes incubated with cofactors).
  • Metabolism of 7-ethoxycoumarin (7-ethoxycoumarin O-deethylation (ECOD) activity) was used as a test xenobiotic compound to demonstrate the difference in metabolism of each test group. Highest activity was observed with permeabilized enterocytes with cofactors (+cofactors) Group D, demonstrating the advantage of the present in vitro reagent.
  • Permeabilization by freezing without cryoprotectants followed by thawing allows maximal interaction of the intracellular enzymes with the substrate (7-ethoxycoumarin), and the addition of cofactors overcomes the dilution of intracellular cofactors due to permeabilization.
  • Example 5 Evaluation and Detection of Key Drug Metabolizing Enzyme Activity
  • the assay was performed essentially as disclosed in Example 1.
  • the cryopreserved hepatocyte/cof actor mixture i.e. in vitro reagent
  • the cryopreserved hepatocyte/cof actor mixture i.e. in vitro reagent
  • HQM containing metabolic enzyme substrates at an appropriate concentration in wells of a 96-well plate.
  • the plate was incubated in a cell culture incubator maintained at 37°C for a specific time period (e.g. 60 minutes) after which an organic solvent (e.g. acetonitrile) was added at a volume of 100 lL to each well.
  • the contents of the wells are collected for LC/MS-MS quantification of metabolite formation.
  • the assay was performed essentially as disclosed in Example 1.
  • the cryopreserved permeabilized hepatocytes/cofactor mixture was thawed at 37°C and 50 jjL of the mixture was added to 50 , u,L of HQM containing metabolic enzyme substrates at an appropriate concentration in wells of a 96-weil plate.
  • the plate was incubated in a cell culture incubator maintained at 37°C for 30, 60, 120 and 240 minutes after which an organic solvent (e.g. acetonitrile) was added at a volume of 100 ⁇ , to each well.
  • the contents of the wells were collected for LC/MS-MS quantification of metabolite formation.
  • the intact hepatocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to UCRM, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells per mL, followed by incubation with drug metabolism substrates as described above for the permeabilized hepatocytes.
  • Example 7 Evaluation and Detection of Non-P450 Pathway-Selective Substrate in Intact Human Hepatocytes and the Present Permeabilized Hepatocytes over a period of 30 minutes to 240 minutes.
  • the assay was performed essentially as disclosed in Example 1.
  • the cryopreserved permeabilized hepatocytes/cofactor mixture was thawed at 37°C and 50 .L of the mixture is added to 50 ,LlL of HQM containing metabolic enzyme substrates at an appropriate concentration in wells of a 96-well plate.
  • the plate was incubated in a cel l culture incubator maintained at 37°C for 30, 60, 120 and 240 minutes after which an organic solvent (e.g. acetonitrile) was added at a volume of 100 .L to each well.
  • the contents of the wells are collected for LC/MS-MS quantification of metabolite formation.
  • the intact hepatocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to UCRM, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells per mL, followed by incubation with drug metabolism substrates as described above for the permeabilized hepatocytes.
  • the results demonstrate a similar trend in the linear time course of metabolite formation in both the intact human hepatocytes and the present permeabilized hepatocytes. See Figure 4
  • Example 8 Evaluation of Coumarin Metabolism Demonstrating Sequential Metabolism: Phase 1 Oxidation followeded by Phase 2 Conjugation of Metabolites.
  • the assay was performed essentially as disclosed in Example 1.
  • the cryopreserved permeabilized hepatocytes/cofactor mixture was thawed at 37°C and 50 U.L of the mixture was added to 50 ⁇ , of HQM containing 75 micromolar coumarin in wells of a 96-well plate. See Figure 5 for a cartoon drawing of coumarin metabolism.
  • the plate was incubated in a cell culture incubator maintained at 37°C for 30 minutes after which an organic solvent (e.g.
  • hepatocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to UCRM, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells per mL, followed by incubation with drug metabolism substrates as described above for the permeabilized
  • Example 9 Evaluation of Drug Metabolizing Enzymes in Intact Human Hepatocytes and Present Permeabilized Hepatocytes
  • the permeabilized hepatocytes were prepared essentially as disclosed in Example 1, wherein the hepatocytes were pooled from multiple donors.
  • the cryopreserved permeabilized hepatocytes/cofactor mixture was thawed at 37°C and 50 uL of the mixture was added to 50 uL of HQM containing metabolic pathway-selective substrates (Se Table 2 below).
  • the plate was incubated in a cell culture incubator maintained at 37°C for 30 minutes after which an organic solvent (e.g. acetonitrile) was added at a volume of 100 ⁇ to each well.
  • the contents of the wells were collected for LC/MS-MS quantification of metabolite formation.
  • the intact hepatocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to UCRM, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells mL, followed by incubation with drug metabolism substrates as described above for the permeabilized hepatocytes.
  • Example 10 Evaluation of Drug Metabolizing Enzymes in Intact Human Enterocytes and Present Permeabilized Enterocytes
  • the permeabilized enterocytes were prepared essentially as disclosed in Example 2, wherein the enterocytes were pooled from multiple donors.
  • the cryopreserved permeabilized enterocytes/cofactor mixture was (hawed at 37°C and 50 , u,L of the mixture was added to 50 ⁇ . of HQM containing metabolic pathway-selective substrates (See Table 3).
  • the plate was incubated in a cell culture incubator maintained at 37°C for 30 minutes after which an organic solvent (e.g. acetonitriie) was added at a volume of 100 ⁇ L ⁇ to each well.
  • the contents of the wells were collected for LC/MS-MS quantification of metabolite formation.
  • the intact enterocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to Cryopreserved Enterocytes Recovery Medium, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells per mL, followed by incubation with drug metabolism substrates as described above for the permeabilized enterocytes.
  • Example 11 Metabolic Stability Screening - Evaluation of Intrinsic Hepatic
  • Dextromethorphan CYP2D6 > 3A/2C19 8.6 10.3 0.6 7.3 0.7
  • Imipramine 8 10.5 0.3 8.9 0.6
  • Nifedipine CYP3A4 15 10.5 0.2 10.4 1.0
  • Example 12 Metabolite Profiling - Metabolite Formation at Cytotoxic Drug
  • the permeabilized hepatocytes were prepared essentially as disclosed in Example 1, wherein the hepatocytes were pooled from multiple donors.
  • the cryopreserved permeabilized hepatocytes/cofactor mixture was thawed at 37°C and 50 ⁇ of the mixture was added to 50 ⁇ of HQM containing a noncytotoxic concentration (10 iiiM), and two cytotoxic concentrations (100 and 200 mM) of acetaminophen (APAP) in wells of a 96-well plate.
  • the plate was incubated in a cell culture incubator maintained at 37°C for 30 minutes after which an organic solvent (e.g. acetonitriie) as added at a volume of 100 ⁇ to each well.
  • an organic solvent e.g. acetonitriie
  • the contents of the wells are collected for LC/MS-MS quantification of metabolite formation (giucuronide, sulfate, and glutathione conjugated acetaminophen).
  • the intact hepatocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to UCRM, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells per mL, followed by incubation with drug metabolism substrates as described above for the permeabilized hepatocytes.
  • Example 13 Cofactor-Directed Metabolic Pathway Selection
  • Intact human hepatocytes allow metabolism of a drug by all hepatic pathways, selection of a specific metabolic pathway for evaluation is not easily accomplished.
  • the experiment disclosed herein demonstrates the present permeabilized human hepatocytes can be used to direct metabolism to specific pathways via selection of cofactors (e.g., exogenous drug metabolizing enzyme co-factors).
  • metabolizing enzyme co-factors used were 2 mM NADPH, 2 mM NADPH + 1 mM PAPS and 2 mM NADPH + 5 mM UDGPGA, and no cofactor addition used as a control.
  • the cryopreserved permeabilized hepatocytes with the various cofactor compositions were thawed at 37°C and 50 ⁇ L of the mixture was added to 50 ⁇ !_, of HQM containing 75 microniolar of coumarin.
  • the plate is incubated in a cell culture incubator maintained at 37°C for 30 minutes after which an organic solvent (e.g. acetonitriie) as added at a volume of 100 ⁇ . to each well.
  • an organic solvent e.g. acetonitriie
  • Example 14 Evaluation of the Present Permeabilized Human Hepatocytes as Exogenous Metabolic Activation System for the Evaluation of Prototoxicants
  • Acetaminophen See Figure 14
  • Cyclophosphamide See Figure 15
  • Ifosfamide were evaluated in the following prototoxicant activation assay.
  • permeabilized human hepatocytes were used in an exogenous metabolic system for evaluation of the physiological effect of metabolites of the prototoxicants towards a target cell line, the HEK293 cells which are devoid of xenobiotic drug metabolism activities.
  • Inactivated (boiled) permeabilized human hepatocytes were used as a metabolic negative control.
  • HEK293 cells were cultured in DMEM in a 96-well plate (10,000 cells per well; 50 ⁇ ) followed by addition of an equal volume of various concentrations of the prototoxicants acetaminophen, cyclophosphamide, and ifosfamide and an equal volume of medium containing permeabilized human hepatocytes (cofactor supplemented), boiled permeabilized hepatocytes or no hepatocytes.
  • the cell cultures were incubated in a cell culture incubator maintained in a 37 C highly humidified atmosphere of 5% carbon dioxide and 95% air for 24 hours.
  • cellular ATP content of the HEK293 cells in each well were quantified using Promega GloTM, a luminescent ATP quantification reagent (Promega Inc., Madison, WI), with luminescence quantified using a Perkin Elmer Victor 3 plate reader.
  • Example 15 Evaluation of the inhibition of intestinal CYP3A4 from orally administered drugs - Drug-Drug Interactions and Food-Drug Interactions.
  • Permeabilized cofactor supplemented enterocytes were prepared from cryopreserved intact enterocytes from 10 donors, see Example 2. Effects of herbal supplements on enterocyte CYP3A4 activity was evaluated using luciferin IPA as CYP3A4 substrate (LIPA ; Promega, Madison, WI) with luminescence quantified on a Perkin Elmer Wallac 1420 Victor microplate reader. The herbal supplements were obtained commercially. The daily recommended dose was dissolved in 50 mL (4X of 100% concentration) of HQM (IVAL), pH adjusted to 7.0 to 7.2, and sterilized by filtration.
  • HQM HQM
  • CYP3A4 activity was quantified after an incubation period of 60 minutes.
  • Fig. 20 The results show that permeabilized enterocytes can be used for the evaluation of food-drug interactions.
  • Herbal supplements with significant CYP3A4 inhibitory effects e.g. green tea extract; grapefruit juice

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Abstract

The present disclosure provides an in vitro reagent for evaluating xenobiotic metabolism in a cell culture based assay. The in vitro reagent is an admixture of metabolically competent cells and exogenous drug metabolizing enzyme co-factors follow by cryopreservation in the absence of cryopreservation agent so that the cells would be rendered permeable upon thawing due to plasma membrane disruption (while maintaining the integrity of organelles). The permeabilized plasma membranes allow ready diffusion of the exogenous cofactors into the cells to enhance the activities of cellular drug metabolizing enzymes. Addition of a xenobiotic test compound to the thawed in vitro reagent allows metabolism of the test compound by the metabolically competent cells, with metabolites readily diffusible outside the cells due to the permeabilized plasma membranes.

Description

IN VITRO DRUG METABOLISM REAGENT AND USES THEREOF
CROSS-REFERENCE TO RELATED APPLICATIONS
[0001] This application claims the benefit of U.S. Provisional Patent Application No.
62/403,435; filed on 03 October 2016, the content of which is incorporated herein by reference in its entirety.
FIELD OF THE INVENTION
[0002] The disclosed inventions relate generally to cryopreserved mixture of metabolically competent cells with a permeabilized plasma membrane and supplemented metabolic enzyme cofactors for use in the evaluation of xenobiotic metabolism.
BACKGROUND OF THE INVENTION
[0003] The invention relates to in vitro reagents for evaluating xenobiotic metabolism, methods of manufacturing the reagent and their methods of use for evaluating xenobiotic metabolism and as an exogenous metabolic system for cell culture assays with metabolic incompetent cells (cells that are not capable of xenobiotic metabolism).
[0004] Drug metabolism is an important aspect of drug development. As a drug is
administered to the human body, the parent drug is subjected to metabolism by the small intestine before absorption into the portal circulation and subjected to metabolism by the liver. Drug metabolism is critical to the system half-live of the parent drug due to metabolic elimination, toxicity due to the toxicity of the parent drug and metabolites, and efficacy due to the pharmacological effects of the parent drug and metabolites. Due to species difference in drug metabolism, studies with nonhuman animals do not always provide information useful for the assessment of human outcomes. This is overcome by the use of in vitro human-based experimental systems. Evaluation of drug metabolism using in vitro human-based system is now routinely practiced in drug development.
[0005] There are myriad assays using bacterial and mammalian cell cultures to estimate biological effects of a substance in the human body. A major drawback of these assays is that the target cells do not possess xenobiotic drug metabolizing enzymes, therefore can only detect results of the parent test substance, but not the metabolites as would occur in the human body. To overcome this major defect of in vitro experimental systems, an exogenous metabolic system is needed to provide xenobiotic metabolism to these cell culture assays. Exogenous metabolic systems are presently not readily available except for the use of rat liver homogenate in genotoxicity assays which may yield results not relevant to human due to species difference.
[0006] In vitro drug metabolism systems are mainly derived from the human liver as it is a major organ for drug metabolism. Commonly used in vitro experimental systems are liver homogenates and intact hepatocytes. For liver homogenate systems, the liver is disrupted by homogenization. In general, the homogenate is first centrifuged at a relative low speed of 9000 or 1000 x g, the resulting supernatant contains both cytosolic and microsomal enzyme and can be used to evaluate both phase I oxidation and phase II conjugation. The supernatant can be centrifuged at a high speed (100,000 x g), resulting in a pellet of endoplasmic reticulum, also referred to as microsomes, which contain one of the most important drug metabolizing enzyme, cytochrome P450. Liver homogenate supernatant, commonly referred to as S-9 or S-10
(supernatant form after centrifugation at 9,000 x g or 10,000 x g, respectively) and the microsomes are the most commonly used in vitro cell-free experimental system for the evaluation of drug metabolism. The liver homogenate systems represent a convenient tool for the evaluation of drug metabolism. Use of the liver homogenate systems such as S9 or microsomes requires the additional of exogenous cofactors to be added at the time of
experimentation. A major disadvantage of the homogenate system is that tissue disruption during the preparation of the homogenates may lead to non-physiological findings that may not represent events in human in vivo.
[0007] Another commonly used in vitro hepatic drug metabolic system is intact hepatocytes. Hepatocytes are isolated from a liver by enzyme digestion (e.g. collagenase digestion) and purified by centrifugation, usually a relative low speed (e.g 50 x g) to remove non-hepatocytes (e.g. kupffer cells and endothelial cells). The 50 x g pellet contains mainly the parenchymal cells or hepatocytes which are the cells responsible for drug metabolism in the liver. Hepatocytes can be used directly after isolation or cryopreserved and stored in liquid nitrogen for use. Successful cryopreservation of hepatocytes to retain viability and function is one of the major reasons for routine application of hepatocytes in experimentation. Cryopreserved hepatocytes from human and non-human animals are commercially available. A scientist can use hepatocytes for experimentation by purchasing the cryopreserved hepatocytes and store them in liquid nitrogen. On the day of experimentation, the cryopreserved hepatocytes are thawed and quantified for viability and cell number, followed by use in experimentation. Cryopreservation of hepatocytes allow this experimental system to be used routinely for the evaluation of drug metabolism, eliminating the need to prepare hepatocytes for each study.
[0008] A major difference between the use of liver homogenate-based systems (S9, S 10, microsomes) and hepatocytes is that liver homogenates need to be supplemented with enzyme cofactors such as NADPH for oxidative metabolism (e.g. hydroxylation of midazolam by P450 isoform 3A4 to 1-hydroxymidazolam), UDPGA for glucuronidation (e.g. formation of 7-OH coumarin glucuronide from 7-OH-coumarin), and PAPS for sulfation (e.g. formation of 7-OH- coumarin sulfate from 7-OH-coumarin). S9 or S 10 can be used to evaluate both phase 1 oxidation and conjugation using all three cofactors; microsomes are used mainly for oxidation as most phase II conjugating enzymes are in the cytosol and not in the microsomal membranes. Viable, intact hepatocytes contain endogenous cofactors, and a full complement of hepatic drug metabolizing enzymes. Hepatocytes therefore are considered the gold standard which can be used directly, without adding cofactors, for all hepatic metabolism pathways.
[0009] This invention is intended to overcome technical challenges required for the application of hepatocytes in drug metabolism. The use of hepatocytes requires specific laboratory equipment such as liquid nitrogen storage system, as the cells need to be store at <-150 deg. C for long term stability, unlike liver homogenate systems that can be stored in a commonly used laboratory freezer at -20 or -80 deg. C. After thawing, the hepatocytes require to be purified (e.g. using the Cryopreserved Hepatocyte Recovery Medium, GIBCO or Universal Cryopreservation Recovery Medium, In Vitro ADMET Laboratories), reconstituted, quantified for cell viability, and adjustment of cell density before addition to the reaction mixture for the evaluation of drug metabolism. Researchers need to be trained with specific skills to work with hepatocytes as the cells are fragile and can be easily damaged by inexperience practitioners. Lastly, hepatocyte isolation and cryopreservation may lead to decreases in cofactors required for drug metabolism, thereby leading to activity lower than that in vivo.
[0010] A second organ important for drug metabolism are intestinal mucosal cells or enterocytes. Enterocytes are now known to contain key drug metabolizing enzymes. Enterocytes can be routinely isolated and used for enteric drug metabolism studies as intact cells, akin to intact hepatocytes for the evaluation of hepatic drug metabolism. Enterocyte S9 and enterocyte microsomes are also used as in vitro systems for the evaluation of enteric drug metabolism, similar to hepatic S9 and microsomes for hepatic metabolism. Enterocyte homogenates and intact enterocytes have similar advantages and drawbacks as described above for the corresponding hepatic systems.
[0011] The invention disclosed herein addresses those deficiencies and provides an improvement for evaluating xenobiotic metabolism using the present in vitro reagent; the invention possesses the advantages of both the tissue homogenates and intact cell models for the evaluation of drug metabolism. For metabolically competent cells isolated from human or animal organs, this invention produces a reagent that eliminates the need of a liquid nitrogen freezer. The reagent can be used immediately after thawing, eliminating the multiple cell manipulation steps needed for fragile cells such as cryopreserved hepatocytes.
Supplementation of cells such as hepatocytes with cofactors (which is not a useful approach as the exogenous cofactors have limited permeability to plasma membranes and therefore not assessable to the cellular drug metabolizing enzymes) in the reagent allows restoration of the cofactors that have been diminished due to the isolation and cryopreservation processes to physiologically relevant in vivo levels.
SUMMARY OF THE INVENTION
[0012] Herein are provided an in vitro reagent, manufacturing of the in vitro reagent and methods for evaluating xenobiotic metabolism using the in vitro reagent. In embodiments provided herein is an in vitro reagent wherein the reagent is a cryopreserved mixture comprising metabolically competent cells wherein cell membranes are permeabilized upon thawing, exogenous drug metabolizing enzyme co-factors, and a buffered solution (e.g., cell culture medium), wherein the reagent does not comprise a cryopreservative agent. In embodiments, the in vitro reagent is thawed wherein the mixture comprises metabolically competent cells with permeabilized plasma membranes. In embodiments, the in vitro reagent is further added to and comprises a metabolically incompetent mammalian or microbial culture, wherein the reagent provides exogenous metabolic functions for evaluation of a physiological effect of metabolites of a xenobiotic.
[0013] In embodiments, the in vitro reagent comprises co-factors required for biochemical pathways and xenobiotic metabolism. In certain embodiments, the drug metabolizing enzyme co-factors are selected from β-nicotinamide adenine dinucleotide 2'-phosphate (NADPH;
cofactor for oxidative metabolism), uridine 5'-diphosphoglucuronic acid (UDPGA; cofactor for glucuronidation), 3'-phosphoadenosine 5'-phosphosulfate (PAPS; cofactor for sulfation), N- acetyl coenzyme A (cofactor for N-acetylation), L-glutathione (cofactor for glutathione conjugation), s-adenosyl methionine, amino acids, and carnitine.
[0014] In embodiments, the metabolically competent cells are primary cells or cell lines, and may be human, rat, monkey, dog, mammals, avian or non-mammalian. In certain embodiments, the metabolically competent cells are from organs responsible for drug metabolism in vivo, such as liver (hepatocytes), intestine (enterocytes) and kidney (renal cells). In embodiments, the metabolically competent cells (primary cells) are pooled from more than one donor. The metabolically competent cells can also be cell lines engineered to contain cytochrome P450 isoforms. In embodiments, the metabolically competent cells comprise drug metabolizing enzyme (DME) activities.
[0015] In embodiments, the reagent is provided in a kit and further comprises instructions for evaluating xenobiotic metabolism using the reagent.
[0016] In certain embodiments, provided herein is an in vitro reagent for evaluating xenobiotic metabolism, wherein the reagent is a cryopreserved mixture comprising: a) metabolically competent cells selected from hepatocytes or enterocytes wherein cell membranes of the hepatocytes or enterocytes are permeabilized upon thawing; b) exogenous drug
metabolizing enzyme co-factors selected from β -Nicotinamide adenine dinucleotide 2'-phosphate (NADPH), Uridine 5'-diphosphoglucuronic acid (UDPGA), 3'-Phosphoadenosine 5'- phosphosulfate (PAPS), N-acetyl coenzyme A, s-adenosyl methionine, amino acids, carnitine, and L-glutathione; and, c) a buffered solution, wherein the reagent does not comprise a cryopreservative agent.
[0017] In certain embodiments, provided herein are methods for manufacturing the in vitro reagent for evaluating xenobiotic metabolism. In embodiments, the method comprises permeabilizing metabolically competent cells, adding exogenous drug metabolizing enzyme co- factors either before or after the metabolically competent cells are permeabilized and providing a buffered solution (e.g., cell culture medium), wherein the reagent does not comprise a cryopreservative agent. In embodiments, the method further comprises storing the reagent frozen at a temperature of -10°C, or lower, such as at a temperature from about -10°C to about - 80°C.
[0018] In embodiments, the metabolically competent cells are permeabilized by freezing in the absence of a cryopreservative agent leading to permeabilization upon thawing. In embodiments, the reagent is not stored frozen in liquid nitrogen. In certain embodiments, the permeabilized metabolically competent cells are not centrifuged prior to use. In other embodiments, the permeabilized metabolically competent cells are not counted prior to use.
[0019] Provided herein are methods for manufacturing the present in vitro reagent, comprising: a) combining intact metabolically competent cells with exogenous drug
metabolizing enzyme co-factors in a cell culture medium to form a cell mixture; b) freezing the cell mixture at a temperature from about -10°C to about -80°C, wherein the cell mixture does not comprise a cryopreservative agent; and, c) thawing the cell mixture to form the in vitro reagent wherein cell membranes of the metabolically competent cells are permeabilized via thawing.
[0020] In embodiments, the in vitro reagent is used to evaluate xenobiotic metabolism after thawing without the step of centrifuging or cell counting.
[0021] In certain embodiments, provided herein are methods of determining metabolism of a test compound, wherein the method comprises providing a present cyropreserved in vitro reagent, thawing the present in vitro reagent and placing in a cell culture vessel; introducing the xenobiotic test compound into the cell culture vessel, incubating the test compound for 0.5 h to 10 days at 33-40°C and performing an end point assay of the in vitro reagent or cell culture medium to determine metabolism of the xenobiotic test compound. In embodiments, the cell culture vessel comprising the in vitro reagent and test compound is incubated at 37°C.
[0022] In embodiments, the end point assay comprises an Ames Salmonella histidine reversion assay (Ames test) for genotoxicity, a mammalian or non-mammalian genotoxicity assay, a mammalian or non-mammalian cytotoxicity assay, and/or a mammalian or non- mammalian pharmacological assay.
[0023] In embodiments, the xenobiotic agent is a drug or drug candidate, an industrial chemical and/or environmental pollutant. In certain embodiments, the drug or drug candidate is selected from the group consisting of an organic compound, an inorganic compound, a hormone, a growth factor, a cytokine, a reception, an antibody, an enzyme, a peptide, an aptomer and a vaccine.
[0024] In embodiments, step b) (thawing the in vitro reagent and placing in a cell culture vessel) of the present methods for determining metabolism of a test compound does not further comprise a centrifugation or cell counting step. In certain embodiments, the present method does not comprise use of a microscope before step e) (performing an end point assay of the in vitro reagent or cell culture medium to determine metabolism of the xenobiotic test compound).
[0025] In embodiments, the cryopreserved in vitro reagent of step a) comprises exogenous drug metabolizing enzyme co-factors used to select metabolism pathways. See Example 13. In certain embodiments, the present method for determining metabolism of a test compound comprises adding a drug or drug candidate at cytotoxic concentrations for identifying and profiling metabolites. See Example 12. In certain embodiments, the present method for determining metabolism of a test compound comprises evaluation of complete phase 1 oxidation and phase 2 conjugation of metabolites with the present reagent of step a) (providing the present cryopreserved in vitro reagent). See Example 8. In certain embodiments, the present methods for determining metabolism of a test compound further comprises evaluating metabolic stability, metabolite profiling and identification, enzyme inhibition or metabolic activation of proto- toxicants or pro-mutagens.
[0026] In embodiments, the time to perform combined steps a) (providing a present cryopreserved in vitro reagent), b) (thawing the in vitro reagent and placing in a cell culture vessel) and c) (introducing the xenobiotic test compound into the cell culture vessel) takes about 10 minutes or less, such as from about 2 minutes to about 6 minutes.
[0027] In embodiments provided herein is an exogenous metabolic system for evaluation of a physiological effect of metabolites of a xenobiotic test compound, wherein the system comprises a cell culture medium admixture of metabolically competent cells comprising permeabilized plasma membranes and exogenous drug metabolizing enzyme co-factors; and metabolically incompetent target cells. The target cells are used to evaluate the metabolites produced by the metabolically competent cells, such as those salmonella bacterial cells used in an Ames test; reporter cell lines for the evaluation of cytotoxicity or pharmacologic effects. [0028] In embodiments, the system further comprises a cell culture vessel comprising one or more assay wells, wherein the assay wells comprise the cell culture medium admixture. In embodiments, each assay well is divided into a first and second chamber, wherein a first chamber comprises the cell culture medium admixture and the second chamber comprises the metabolically incompetent target cells provided the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture. In embodiments, the first and second chamber are separated by a porous membrane that is liquid-permeable and cell- impermeable.
[0029] In embodiments, the metabolically incompetent target cells may be mammalian or non-mammalian, such as bacteria.
BRIEF DESCRIPTION OF THE DRAWINGS
[0030] Figure 1 provides results from metabolism of 7-ethoxycoumarin by human enterocytes with or without exogenous drug metabolizing enzyme co-factors and with or without permeabilization. Highest activity was observed with permeabilized enterocytes with cofactors (Group D; present in vitro reagent). See Example 4
[0031] Figure 2A and Figure 2B provide measurement of the major P450 isoform activities as a function of cell concentrations. The linear concentration versus activity curves demonstrate that permeabilized hepatocytes can be used routinely as an in vitro drug metabolism system for scientific investigations.
[0032] Figure 3A and 3B show P450 isoform-selective substrate metabolism in intact human hepatocytes and permeabilized human hepatocytes over a time period of 30 minutes to 240 minutes.
[0033] Figure 4 shows non-P450 pathway-selective substrate metabolism in intact human hepatocytes and permeabilized human hepatocytes over a time period of 30 minutes to 240 minutes.
[0034] Figure 5 shows phase 1 oxidation and phase 2 conjugation metabolism of coumarin.
[0035] Figure 6 shows coumarin metabolite formation and ethoxycoumarin formation in intact human hepatocytes and permeabilized human hepatocytes demonstrating sequential drug metabolism in the permeabilized human hepatocytes measured at 30 min., 60 min., 120 min. and 240 min.
[0036] Figure 7 shows a comparison of 16 drug metabolizing enzyme (DME) -selective substrates and measurement of metabolites in intact human hepatocytes (open bars) and permeabilized human hepatocytes (solid bars). The permeabilized human hepatocytes showed similar or higher activity than the intact human hepatocytes in the metabolism of 16 pathway- selective DME pathways.
[0037] Figure 8 shows the advantages of permeabilized hepatocytes and permeabilized enterocytes as compared to cell free systems (S9 and microsomes) or intact hepatocytes and intact enterocytes. The permeabilized hepatocytes and permeabilized enterocytes provide complete representation of organelles as intact hepatocytes and enterocytes.
[0038] Figure 9 shows the ease of use of the permeabilized hepatocytes and permeabilized enterocytes as compared to cell free systems and intact hepatocytes and intact enterocytes.
[0039] Figure 10 shows metabolic stability screening wherein the present permeabilized human hepatocytes (filled symbols; y = 0.79x; R2 = 0.4067) accurately predict human hepatic clearance in vivo of drugs with known in vivo hepatic clearance as compared to intact hepatocytes (open symbols; y = 0.7375x; R2 = 0.13). See Table 4 for a list of the drugs tested and observed results.
[0040] Figure 11 shows Acetaminophen metabolism (glucuronidation, sulfation and GSH conjugation to the oxidative metabolite NAPQI) at nontoxic (10 mM) and cytotoxic (100 and 200 mM) concentrations in both intact human hepatocytes (open bars) and permeabilized human hepatocytes (solid bars). The permeabilized human hepatocytes can be incubated with high, cytotoxic concentrations of a xenobiotic (e.g. drug or drug candidate) for the generation of metabolites for identification and profiling while significant reduction of metabolite formation was observed in intact hepatocytes due to cytotoxicity.
[0041] Figure 12 shows cofactor-directed pathway selection scheme of coumarin metabolism.
[0042] Figure 13 shows cofactor-directed pathway (no cofactors; NADPH; NADP + PAPS; and, NADPH + UGPGA) selection of coumarin metabolism (7-HC; 7-HCS; and, 7-HCG) in permeabilized human hepatocytes. Selection of exogenous drug metabolizing enzyme co-factors can be used to direct metabolism to specific pathways in the present permeabilized human hepatocytes.
[0043] Figure 14 shows a scheme of the prototoxicant Acetaminophen activation.
[0044] Figure 15 shows a scheme of the prototoxicant Cyclophosphamide activation.
[0045] Figure 16 shows the activation of Acetaminophen using permeabilized human hepatocytes with boiled hepatocytes and no hepatocytes as controls.
[0046] Figure 17 shows the activation of Cyclophosphamide and Ifosfamine using permeabilized human hepatocytes with boiled hepatocytes and no hepatocytes as controls.
[0047] Figure 18 shows the versatility of using permeabilized hepatocytes and
permeabilized enterocytes as compared to cell free systems (S9 and microsomes) or intact hepatocytes and intact enterocytes.
[0048] Figure 19 shows the steps of using permeabilized hepatocytes and permeabilized enterocytes as compared to cryopreserved intact hepatocytes and intact enterocytes.
[0049] Figure 20 shows CYP3A4 activity by permeabilized human enterocytes upon treatment by various concentrations of herbal supplements.
DETAILED DESCRIPTION OF THE INVENTION
[0050] Provided herein are methods, compositions, and kits for evaluating xenobiotic metabolism, including both effects of the parent xenobiotic and its metabolites. In embodiments, the composition is an in vitro reagent that provides improved means for testing xenobiotic metabolism, such as a drug or drug candidate. In certain embodiments, the in vitro reagent is a cryopreserved mixture comprising metabolically competent cells (wherein cell membranes are permeabilized upon thawing;), exogenous drug metabolizing co-factors and a buffer solution such as cell culture medium, wherein the reagent does not comprise a cryopreservative agent. In embodiments, the in vitro reagent is frozen (e.g. cryopreserved) and comprises metabolically competent cells, exogenous drug metabolizing co-factors and cell culture medium, wherein the metabolically competent cells are permeabilized when thawed provided the in vitro reagent does not comprise a cryopreservative. In embodiments, the thawed in vitro reagent comprises metabolically competent cells with permeabilized plasma membranes, exogenous drug metabolizing co-factors and a buffer solution, wherein the metabolically competent cells are permeabilized via thawing. As used herein, cryopreserved refers to preserving a mixture of cells and enzyme co-factors (i.e. present in vitro reagent) that has been frozen at a temperature of about -10°C or less, such as about -20°C to about -80°C, in the absence of a cryopreservative agent.
[0051] The present in vitro reagent comprising permeabilized metabolically competent cells permeabilized via thawing of the cryopreserved intact metabolically competent cells provides benefits and advantages over use of organelle systems, intact cells and even metabolically competent cells permeabilized by other methods (e.g. sonication and/or detergent). Permeability induced by freezing without cryopreservative allows minimum disturbance to cellular integrity. Previous methods using a detergent (saponin) and/or extensive sonication cause total cell disruption, including disruption of the organelles. In contrast, we found permeability induced by freezing without cryopreservative allows the evaluation of drug metabolism in cells with near intact cell integrity but with permeable membrane; thereby the present in vitro reagent and methods are physiologically more relevant. In embodiments is provided an in vitro reagent comprising metabolically competent cells that are permeabilized upon thawing and
supplemented with metabolic cofactors for drug metabolism studies and wherein the reagent does not comprise a cryopreservative agent. In embodiments, the present metabolically competent cells were not permeabilized via mechanical or detergent means.
[0052] The present in vitro reagent comprised of intact, permeabilized metabolically competent cells and exogenous drug metabolizing enzyme co-factors, represent a complete system with all the drug metabolizing enzymes as intact hepatocytes or intact enterocytes which is the major drawback of tissue homogenate systems such as S9 or microsomes (discussed in the Background section). The metabolically competent cells are permeabilized to allow
supplementation of the in vitro reagent with exogenous metabolism enzyme cofactors to overcome the loss of cofactors due to cell isolation from the intact organ and the subsequent cryopreservation. The present in vitro reagent can be stored in a regular laboratory freezer at -10 or -80°C, without a need for liquid nitrogen freezers. In embodiments, the in vitro reagent can be thawed and use directly, without a need to supplement with cofactors, such as those needed for S9 and microsomes, and without a need for cell recovery/viability determination/cell density adjustment as needed when intact hepatocytes are used. The present in vitro reagent thereby has the advantage of the physiological relevance of, for example, intact hepatocytes and the ease of use of liver microsomes.
[0053] In embodiments, the composition is an exogenous metabolic system, wherein the system comprises: a) a cell culture medium admixture comprising; i) metabolically competent cells comprising permeabilized plasma membranes; and, ii) exogenous drug metabolizing enzyme co-factors, and b) metabolically incompetent target cells. The cell culture admixture is also referred to herein as the thawed in vitro reagent. In embodiments, the thawed in vitro reagent is added to a cell culture assay comprising metabolically incompetent target cells followed by addition of the test compound, incubation for a designated time duration, and quantification of the designated biological effects in the target cells, thereby allowing the evaluation of the effects of both the parent the metabolites.
[0054] In certain embodiments, the exogenous metabolic system comprises a separation between the cell culture admixture and the metabolically incompetent cells. The exogenous metabolic system may further comprise a cell culture vessel comprising one or more assay wells, wherein the assay wells comprise the cell culture medium admixture. In particular the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture wherein, for example, each assay well is divided into a first and second chamber, wherein a first chamber comprises the cell culture medium admixture and the second chamber comprises the metabolically incompetent target cells provided the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture.
[0055] The present in vitro reagent, and its use in an exogenous metabolic system, provides advantages as compared to the use of intact metabolically competent cells or homogenates of those cells that require the use of enzyme co-factors. Those advantages, include but are not limited to, A) increased drug metabolizing enzyme activity; B) increased efficiency wherein the permeabilized metabolically competent cells admixed with exogenous drug metabolizing co- factors can be used directly, without centrifugation and cell counting {See Figure 1 and Example 4); and C) improved access for researchers wherein the in vitro reagent can be stored in a freezer at -10°C or -80°C, rather than in liquid nitrogen as needed for intact hepatocytes, allowing researchers without assess to liquid nitrogen storage systems use of the instant in vitro reagent. [0056] In embodiments, the metabolically competent cells are cryopreserved with the exogenous drug metabolizing co-factors and may be used directly to evaluate xenobiotic metabolism. In embodiments, the metabolically competent cells are permeabilized when they are cryopreserved in the absence of a cryoprotectant, which induces membrane permeability when the cells are thawed. Once thawed, the cells may be used directly without a step of cell counting or centrifugation. The amount of time from thawing to adding of a test compound may be from about 2 minutes to about 7 minutes, or less than about 6 minutes. See Figure 19. In certain embodiments, the in vitro reagent does not comprise a cryopreservative agent. In other embodiments, the metabolically competent cells may be permeabilized prior to cryopreservation. In that instance, the in vitro reagent may comprise a cryopreservative agent.
[0057] In embodiments, the in vitro reagent comprises metabolically competent cells, exogenous drug metabolizing co-factors and a buffer solution such as a cell culture medium, wherein the co-factors are admixed with the competent cells in the cell culture medium and then the admixture is cryopreserved; also referred to herein as a cryopreserved mixture. In
embodiments, the in vitro reagent is stored at a temperature of -10°C or less, such as about -10°C to about -80°C. In embodiments, the exogenous drug metabolizing co-factors include, but are not limited to those for oxidative metabolism, glucuronidation or sulfation. In embodiments, the in vitro reagent comprises, individually or in combination, β -nicotinamide adenine dinucleotide 2'-phosphate (NADPH) for oxidative metabolism, uridine 5'-diphosphoglucuronic acid
(UDPGA) for glucuronidation and/or 3'-phosphoadenosine 5'-phosphosulfate (PAPS) for sulfation, N-acetyl coenzyme A, s-adenosyl methionine, amino acids, carnitine, and L- glutathione. See Example 1. As used herein, "drug" is used generically in the term "drug metabolizing enzyme co-factors" and is understood to broadly mean xenobiotic. In
embodiments, the in vitro reagent comprises co-factors required for biochemical pathways and xenobiotic metabolism.
[0058] In embodiments, the manufacturing of the instant in vitro reagent is carried out by permeabilizing metabolically competent cells and adding exogenous drug metabolizing enzyme co-factors either before or after the metabolically competent cells are permeabilized, wherein the in vitro reagent is provided in a cell culture medium. In certain embodiments, the metabolically competent cells are frozen without a cryoprotectant (also referred to herein as a cryopreservative) wherein they are permeabilized during thaw of the in vitro reagent. In that instance, the metabolically competent cells (prior to being permeabilized) are admixed with the exogenous drug metabolizing co-factors in the presence of cell culture medium. As used in the art, a cryoprotectant or cryopreservative, is a substance that prevents damage to cells and/or organelles during freezing, and includes but is not limited to glycols; such as glycerol, ethylene glycol and propylene glycol; and dimethyl sulfoxide (DMSO). In embodiments, the in vitro reagent does not comprise glycerol and/or DMSO. In embodiments, the in vitro reagent is stored without serum, in other words the frozen in vitro reagent is serum free. In embodiments, the in vitro reagent is frozen at a temperature of -10°C or less (e.g. from about -10°C to about -80°C), and does not comprise glycerol and/or DMSO and/or serum.
[0059] The methods of use herein are carried out by addition of a xenobiotic test compound or test article to the thawed in vitro reagent (admixture of metabolically competent cells with permeabilized plasma membranes and enzyme co-factors), i.e. room temperature (e.g. about 20 to 25°C) to about a physiological temperature (e.g. about 35°C to 40°C), in a cell culture vessel. The test compound is introduced into the cell culture vessel comprising the thawed in vitro reagent, incubated, followed by evaluation of the effects of metabolism on the test compound including quantification of the parent compound for the evaluation of metabolic stability; metabolite quantification and identification; evaluation of drug metabolizing enzyme (e.g. P450) activity for evaluation of drug-drug interaction potential. The reagent is also used as an exogenous metabolic system in conjunction with a cell culture system comprising
metabolically incompetent target cells.
[0060] In embodiments, a xenobiotic test compound or test article is added as an exogenous metabolic system, which comprises a thawed in vitro reagent (i.e. a cell culture medium admixture comprising metabolically competent cells comprising permeabilized plasma membranes and exogenous drug metabolizing enzyme co-factors) and metabolically incompetent target cells. In embodiments, the cell culture medium, the metabolically competent cells or the metabolically incompetent cells are subjected to the end point analysis to determine metabolism of the xenobiotic test compound and any effects of the metabolites thereof.
[0061] The test compounds used in the present invention include, but are not limited to drugs, drug candidates, biologicals, food components, herb or plant components, proteins, peptides, oligonucleotides, DNA and RNA. In embodiments, the test compound is a drug, a drug candidate, an industrial chemical, an environmental pollutant, a pesticide, an insecticide, a biological chemical, a vaccine preparation, a cytotoxic chemical, a mutagen, a hormone, an inhibitory compound, a chemotherapeutic agent or a chemical. In certain embodiments, the drug or drug candidate is selected from the group consisting of an organic compound, an inorganic compound, a hormone, a growth factor, a cytokine, a reception, an antibody, an enzyme, a peptide, an aptamer or a vaccine. The test compound can be either naturally-occurring or synthetic, and can be organic or inorganic. A person skilled in the art will recognize that the test compound can be added to the in vitro reagent present in the cell culture medium in an appropriate solvent or buffer.
[0062] In certain embodiments, the in vitro reagent and/or exogenous metabolic system is used for high-throughput screening to test the metabolic effects or response to a range of test compounds. In that instance, the in vitro reagent may be used with a cell culture vessel that is a multi-well plate, such as a 6-well; 12-well; 24-well; 48-well, 96-well; 384-well, 1536-well plate or any combination thereof. In alternative embodiments, the methods use a cell culture vessel with a single assay well.
[0063] In embodiments, the metabolic system comprises a cell culture vessel wherein the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture. In embodiments, the cell culture vessel comprises one or more assay wells, wherein the assay wells comprise the cell culture medium admixture and the metabolically incompetent cells in the same admixture. In alternative embodiments, each assay well is divided into a first and second chamber, wherein a first chamber comprises the cell culture medium admixture and the second chamber comprises the metabolically incompetent target cells provided the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture. In certain embodiments, the first and second chamber are separated by a porous membrane that is liquid-permeable and cell-impermeable.
[0064] In embodiments, the exogenous metabolic system comprises a cell culture vessel with a single well plate. Alternatively, the exogenous metabolic system comprises cell culture vessel that is a multi-well plate. In embodiments, the porous membrane separating the first and second chamber of the cell culture vessel comprises polyethylene terephthalate (PET), polycarbonate, polystyrene, polypropylene, nylon, Mylar, stainless steel, wire mesh, aluminum, synthetic mesh, plastic, or paper. In embodiments, the cell culture insert is a transwell.
[0065] In embodiments, the metabolically competent cells are primary cells or cell lines; and can be human, rat, monkey, dog, mammals, avian or non-mammalian cells. In certain embodiments, the metabolically competent cells are from organs responsible for drug metabolism in vivo, such as liver (hepatocytes), intestine (enterocytes) and kidney (renal cells). In certain embodiments, the metabolically competent cells are human hepatocytes. See, Li, A. P. (2007) Human hepatocytes: isolation, cryopreservation and applications in drug development. Chemico-biological interactions, 168(1), 16-29. Freshly prepared metabolically competent cells or cryopreserved cells (e.g. hepatocytes) obtained by standard methods from a human or animal liver can be used as the metabolically competent cells. See, Hewitt, Nicola J., et al. "Primary hepatocytes: current understanding of the regulation of metabolic enzymes and transporter proteins, and pharmaceutical practice for the use of hepatocytes in metabolism, enzyme induction, transport, clearance, and hep ato toxicity studies." Drug metabolism reviews 39.1 (2007): 159-234.
[0066] In embodiments, the metabolically competent cells are hepatocytes (the parenchymal cells of the liver). Hepatic metabolism is known to be the major determinant of
metabolism-dependent xenobiotic toxicity. P450 and non-P450 phase 1 oxidation enzyme pathways are responsible mostly for the bioactivation of relatively inert parent compounds to reactive (toxic/carcinogenic/mutagenic) metabolites. Phase 2 conjugating pathways are responsible mostly for the biotransformation of toxic parent compounds or metabolites to less toxic compounds. Both phase 1 and phase 2 pathways are present in the hepatocytes - the key hepatic cell type responsible for hepatic metabolism. In embodiments, enterocytes can be used to model enteric metabolism for orally ingested toxicants. In other
embodiments, renal proximal tubule cells can be used to model renal metabolism. In certain other embodiments, enterocytes can be used to model intestinal metabolism.
[0067] In certain embodiments, the metabolically competent cells are recombinant cells, wherein for example, they have been engineered to comprise drug metabolizing enzymes. In certain embodiments, the metabolically competent cells are engineered to contain cytochrome P450 isoforms. See, Doehmer, J., Battula, N., Wolfel, C, Kudla, C, Keita, Y. and Staib, A.H., 1992. Biotransformation of caffeine and theophylline in mammalian cell lines genetically engineered for expression of single cytochrome P450 isoforms. Biochemical pharmacology, 43(2), pp.225-235; Donato, M. T., Jimenez, N., Castell, J. V., & Gomez-Lechon, M. J. (2004). Fluorescence-based assays for screening nine cytochrome P450 (P450) activities in intact cells expressing individual human P450 enzymes. Drug Metabolism and Disposition, 32(7), 699-706.
[0068] In embodiments, a stable cell line such as HepG2 is used in the present in vitro reagent and methods for determining metabolism of a test compound. HepG2 is a perpetual cell line derived from the liver of a 15-year-old Caucasian male with a well-differentiated
hepatocellular carcinoma. Because of the high degree of morphological and functional differentiation in vitro, HepG2 cells can be a suitable model to study the intracellular trafficking and dynamics of bile canalicular and sinusoidal membrane proteins and lipids in human hepatocytes in vitro. See, Ihrke et al., WIF-B cells: an in vitro model for studies of hepatocyte polarity. Journal of Cell Biology 123 (6), 1761-1775, 1993. In certain embodiments, a stable cell line such as HepaRG is used in the present in vitro reagent and methods for determining metabolism of a test compound. See, Guillouzo, A., Corlu, A., Aninat, C, Glaise, D., Morel, F. and Guguen-Guillouzo, C, 2007. The human hepatoma HepaRG cells: a highly differentiated model for studies of liver metabolism and toxicity of xenobiotics. Chemico-biological interactions, 168(1), pp.66-73.
[0069] In embodiments, present metabolically competent cells are genetically altered or modified so as to contain a non-native "recombinant" (also called "exogenous") nucleic acid sequence, or modified by antisense technology to provide a gain or loss of genetic function. As used herein, "cells", unless specified otherwise, refers to metabolically competent cells.
Methods for generating genetically modified cells are known in the art, see for example "Current Protocols in Molecular Biology," Ausubel et al., eds, John Wiley & Sons, New York, N.Y., 2000.
[0070] Accordingly, in embodiments, the present in vitro reagent may comprise any cell type, including primary cells, stem cells, progenitor cells, normal, genetically-modified, genetically altered, immortalized, and transformed cell lines, provided the cells are metabolically competent, permeabilized (permeabilized during thaw), and admixed with exogenous drug metabolizing enzyme co-factors. The present invention is suitable for use with single cell types or cell lines, or with combinations of different cell types. Preferably the cultured cells maintain the ability to respond to stimuli that elicit a response in their naturally occurring counterparts. These may be derived from all sources such as eukaryotic (mammalian and non-mammalian). The eukaryotic cells can be animal in nature, such as human, simian, or rodent. They may be of any tissue type (e.g., heart, stomach, kidney, intestine, lung, liver, fat, bone, cartilage, skeletal muscle, smooth muscle, cardiac muscle, bone marrow, muscle, brain, pancreas), and cell type (e.g., epithelial, endothelial, mesenchymal, adipocyte, hematopoietic).
[0071] In embodiments, metabolically competent cells are cultured from a variety of genetically diverse individuals who may respond differently to biologic and pharmacologic agents. Genetic diversity can have indirect and direct effects on metabolism of a test compound. In embodiments, the metabolically competent cells are a pool of cells from multiple individuals or donors. In certain embodiments, the metabolically competent cells are reflective of the heterogeneity of a population of individuals.
[0072] In embodiments, an exogenous metabolic system comprises metabolically
incompetent cells (in addition to a thawed in vitro reagent wherein the metabolically competent cells have a permeabilized plasma membrane). In embodiments, the metabolically incompetent cells are mammalian or non-mammalian and include, but are not limited to carbiomyocytes (Doherty, Kimberly R., Robert L. Wappel, Dominique R. Talbert, Patricia B. Trusk, Diarmuid M. Moran, James W. Kramer, Arthur M. Brown, Scott A. Shell, and Sarah Bacus. "Multiparameter in vitro toxicity testing of crizotinib, sunitinib, erlotinib, and nilotinib in human cardiomyocytes. "Toxicology and applied pharmacology 272, no. 1 (2013): 245-255), vascular endothelia cells (Louise, C.B. and Obrig, T.G., 1991. Shiga toxin-associated hemolytic-uremic syndrome: combined cytotoxic effects of Shiga toxin, interleukin- 1 beta, and tumor necrosis factor alpha on human vascular endothelial cells in vitro. Infection and immunity, 59(11), pp.4173-4179) and cell lines such as mouse 3T3 fibroblasts (Spielmann, H., Balls, M., Brand, M., Doring, B., Holzhiitter, H.G., Kalweit, S., Klecak, G., Eplattenier, H.L., Liebsch, M., Lovell, W.W. and Maurer, T., 1994. EEC/COLIPA project on in vitro phototoxicity testing: First results obtained with a Balb/c 3T3 cell phototoxicity assay. Toxicology in vitro, 8(4), pp.793-796) and Chinese hamster ovary cells (Li, A. P., Carver, J.H., Choy, W.N., Hsie, A.W., Gupta, R.S., Loveday, K.S., O'neill, J.P., Riddle, J.C., Stankowski, L.F. and Yang, L.L., 1987. A guide for the performance of the Chinese hamster ovary cell/hypoxanthine-guanine phosphoribosyl transferase gene mutation assay. Mutation Research/Genetic Toxicology, 189(2), pp.135-141). [0073] In embodiment, examples include reporter cell lines for endocrine disruption, but are not limited to metabolically incompetent cells disclosed in the following references: Willemsen, P., Scippo, M.L., Kausel, G., Figueroa, J., Maghuin-Rogister, G., Martial, J. A. and Muller, M., 2004. Use of reporter cell lines for detection of endocrine-disrupter activity. Analytical and bioanalytical chemistry, 378(3), pp.655-663), Genotoxicity determination with the Ames salmonella typhimurium gene mutation assay; De Flora, S., Zanacchi, P., Camoirano, A., Bennicelli, C. and Badolati, G.S., 1984. Genotoxic activity and potency of 135 compounds in the Ames reversion test and in a bacterial DNA -repair test. Mutation Research/Reviews in Genetic Toxicology, 133(3), pp.161-198.
[0074] In embodiments, examples of metabolically incompetent cells include mammalian cell lines used for genotoxicity assays, but are not limited to metabolically incompetent cells disclosed in the following references: Moore, Martha M., et al. "Mouse lymphoma thymidine kinase gene mutation assay: Follow-up meeting of the international workshop on Genotoxicity testing— Aberdeen, Scotland, 2003— Assay acceptance criteria, positive controls, and data evaluation." Environmental and molecular mutagenesis 47.1 (2006): 1-5; Aaron, C.S.,
Bolcsfoldi, G., Glatt, H.R., Moore, M., Nishi, Y., Stankowski, L., Theiss, J. and Thompson, E., 1994. Mammalian cell gene mutation assays working group report. Mutation
Research/Environmental Mutagenesis and Related Subjects, 312(3), pp.235-239.).
[0075] In embodiments, examples of metabolically incompetent cells include nonhepatic primary cells for the evaluation of organ- specific dr g toxicity, but are not limited to
metabolically incompetent cells disclosed in the following references: Pfaller, W. and
Gstraunthaler, G., 1998. Nephrotoxicity testing in vitro— what we know and what we need to know. Environmental health perspectives, i0<5(Suppl 2), p.559; Mordwinkin, N.M., Burridge, P.W. and Wu, J.C., 2013. A review of human pluripotent stem cell-derived cardiomyocytes for high-throughput drug discovery, cardio toxicity screening, and publication standards. Journal of cardiovascular translational research, 6(1), pp.22-30).
[0076] For screening test compounds using the in vitro reagent and/or exogenous metabolic system for their metabolic effect on the cells, the in vitro reagent comprising metabolically competent cells and exogenous drug metabolizing enzyme co-factors are thawed and placed in a cell culture vessel with cell culture medium. If using the exogenous metabolic system, the system further comprises metabolically in competent cells in fluid communication with the thawed in vitro reagent. The term "culture condition" encompasses cells, media, factors, time and temperature, atmospheric conditions, pH, salt composition, minerals, etc. Cell culturing is typically performed in a sterile environment mimicking physiological conditions, for example, at 37°C in an incubator containing a humidified 92-95% air/5-8% CO2 atmosphere. In
embodiments, the cell culture temperate is a range from 33-40°C. Cell culturing may be carried out in nutrient mixtures containing undefined biological fluids such a fetal calf serum, or media that is fully defined and serum free. A variety of culture media are known in the art and are commercially available.
[0077] In embodiments, the metabolically competent cells (with permeabilized plasma membrane) are not checked for viability, centrifuged, counted or cultured prior to addition of the xenobiotic test compound. In alternative embodiments, the in vitro reagent may be cultured for a time period from a few hours to days prior to use in the instant methods. In embodiments, the xenobiotic test compound is placed in the cell culture vessel wherein the thawed in vitro reagent (i.e. cell culture medium admixture comprising permeabilized metabolically competent cells and exogenous drug metabolizing enzyme co-factors) is then incubated under appropriate cell culture conditions as disclosed herein for a time period of 30 minutes to up to 10 days. In embodiments, the incubation period can be at least 1 hours, 2 hours, 5 hours, 10 hours, 15 hours, 24 hours, 2 days, 3 days, 4 days, 5 days, 6 days, 7 days, 8 days, 9 days or at least 10 days. In embodiments, the incubation time period is not longer than 1 day, 2 days, 5 days, 6 days, 7 days, 8 days, 9 days or not longer than 10 days. In embodiments, the cell culture conditions replicate physiological conditions as much as possible. The term "physiological conditions" as used herein is defined to mean that the cell culturing conditions are very specifically monitored to mimic as closely as possible the natural tissue conditions for a particular type of cell in vivo.
[0078] In embodiments, the xenobiotic test compound is considered an input variable, and is used interchangeably herein with a test compound. The test compounds are screened for biological activity by adding to a pharmacokinetic -based culture system (e.g. present in vitro reagent), and then assessing the metabolically competent cells (or culture medium) for changes in output variables of interest, e.g., consumption of O2, production of CO2, cell viability, expression of proteins of interest (protein expression), cell function, expression of genes of interest (gene expression), metabolite formation or metabolite profiles. The test compound is typically added in solution, or readily soluble form, to the medium of cells in culture. The test compound can be added using a flow through system, or alternatively, adding a bolus to an otherwise static solution. In a flow-through system, two fluids are used, where one is a physiologically neutral solution, and the other is the same solution with the test compound added. The first fluid is passed over the cells, followed by the second. In a single solution method, a bolus of the test compound is added to the volume of medium surrounding the cells. The overall composition of the culture medium should not change significantly with the addition of the bolus, or between the two solutions in a flow through method.
[0079] In embodiments, the test compound includes pharmacologically active drugs or drug candidates and genetically active molecules. Test compounds of interest include
chemotherapeutic agents, anti-inflammatory agents, hormones or hormone antagonists, ion channel modifiers, and neuroactive agents. Exemplary of pharmaceutical agents suitable for this invention are those described in "The Pharmacological Basis of Therapeutics," Goodman and Gilman, McGraw-Hill, New York, N.Y., (1996), Ninth edition, under the sections: Drugs Acting at Synaptic and Neuroeffector Junctional Sites; Drugs Acting on the Central Nervous System; Autacoids: Drug Therapy of Inflammation; Water, Salts and Ions; Drugs Affecting Renal Function and Electrolyte Metabolism; Cardiovascular Drugs; Drugs Affecting Gastrointestinal Function; Drugs Affecting Uterine Motility; Chemotherapy of Parasitic Infections;
Chemotherapy of Microbial Diseases; Chemotherapy of Neoplastic Diseases; Drugs Used for Immunosuppression; Drugs Acting on Blood-Forming Organs; Hormones and Hormone Antagonists; Vitamins, Dermatology; and Toxicology, all incorporated herein by reference. Also included are toxins, and biological and chemical warfare agents, for example see Somani, S. M. (Ed.), "Chemical Warfare Agents," Academic Press, New York, 1992).
[0080] In embodiments, the test compound includes all of the classes of molecules disclosed herein, and may further or separately comprise samples of unknown content. While many samples will comprise compounds in solution, solid samples that can be dissolved in a suitable solvent may also be assayed. Samples containing test compounds of interest include
environmental samples, e.g., ground water, sea water, or mining waste; biological samples, e.g., lysates prepared from crops or tissue samples; manufacturing samples, e.g., time course during preparation of pharmaceuticals; as well as libraries of compounds prepared for analysis; and the like. Samples of interest include test compounds being assessed for potential therapeutic value, e.g., drug candidates from plant or fungal cells.
[0081] Test compounds are obtained from a wide variety of sources including libraries of synthetic or natural compounds. For example, numerous means are available for random and directed synthesis of a wide variety of organic compounds and biomolecules, including expression of randomized oligonucleotides and oligopeptides. Alternatively, libraries of natural compounds in the form of bacterial, fungal, plant and animal extracts are available or readily produced. Additionally, naturally or synthetically produced libraries and compounds are readily modified through conventional chemical, physical and biochemical means, and may be used to produce combinatorial libraries. Known pharmacological agents may be subjected to directed or random chemical modifications, such as acylation, alkylation, esterification, amidification to produce structural analogs.
[0082] In embodiments, following incubation of the thawed in vitro reagent with the test compound an end point analysis is performed to determine the effect of the test compound on the metabolically competent cells. In embodiments, the end point analysis identifies the output variable (e.g. the effect of the test compound) of the in vitro reagent. In embodiments, output variables are quantifiable elements of the cells, particularly elements that can be accurately measured in a cell culture system. An output variable can be any cell component or cell product including, e.g., viability, respiration, metabolism, cell surface determinant, receptor, protein or conformational or posttranslational modification thereof, lipid, carbohydrate, organic or inorganic molecule, mRNA, DNA, or a portion derived from such a cell component. In embodiments, the output variable is directly or indirectly a result of the test compound or its metabolite. While most output variables will provide a quantitative readout, in some instances a semi-quantitative or qualitative result will be obtained. Readouts may include a single determined value, or may include mean, median value or the variance. Characteristically a range of readout values will be obtained for each output. Variability is expected and a range of values for a set of test outputs can be established using standard statistical methods.
[0083] In embodiments, the end point assay is an Ames Salmonella histidine reversion assay (Ames test) for genotoxicity, a mammalian or non-mammalian genotoxicity assay, a mammalian or non-mammalian pharmacological assay. [0084] Various methods can be utilized for quantifying the presence of selected metabolism markers. Liquid chromatography (LC), mass spectrometry (MS), and their combination
(LC/MS-MS) are routinely used for the quantification of metabolites. For non-LC/MS measurement of the amount of a molecule that is present, a convenient method is to label the molecule with a detectable moiety, which may be fluorescent, luminescent, radioactive, or enzymatically active. Fluorescent and luminescent moieties are readily available for labeling virtually any biomolecule, structure, or cell type. Immunofluorescent moieties can be directed to bind not only to specific proteins but also specific conformations, cleavage products, or site modifications like phosphorylation. Individual peptides and proteins can be engineered to autofluoresce, e.g., by expressing them as green fluorescent protein chimeras inside cells (for a review, See Jones et al. (1999) Trends Biotechnol. 17(12):477-81).
[0085] Output variables may be measured by immunoassay techniques such as,
immunohistochemistry, radioimmunoassay (RIA) or enzyme linked immunosorbance assay (ELISA) and related non-enzymatic techniques. These techniques utilize specific antibodies as reporter molecules that are particularly useful due to their high degree of specificity for attaching to a single molecular target. Cell based ELISA or related non-enzymatic or fluorescence-based methods enable measurement of cell surface parameters. Readouts from such assays may be the mean fluorescence associated with individual fluorescent antibody-detected cell surface molecules or cytokines, or the average fluorescence intensity, the median fluorescence intensity, the variance in fluorescence intensity, or some relationship among these. For toxicity assays, outputs can include measurement of cell viability such as enzyme release, cellular ATP contents, reactive oxygen species formation, decrease of reduced glutathione, protein synthesis, protein contents, DNA contents, dye exclusion, dye inclusion, and cell detachment. For
pharmacological assays, specific disease target related assays can be used. For genotoxicity assays, endpoints measured may include DNA damage, chromosomal aberration, mutant generation, and induction of DNA repair.
[0086] In embodiments, the results of screening assays may be compared to results obtained from a reference compound, concentration curves, controls (with and without metabolically competent cells), etc. The comparison of results is accomplished by the use of suitable deduction protocols, Al systems, statistical comparisons, etc. [0087] A database of reference output data can be compiled. These databases may include results from known agents or combinations of agents, as well as references from the analysis of cells treated under environmental conditions in which single or multiple environmental conditions or parameters are removed or specifically altered. A data matrix may be generated, where each point of the data matrix corresponds to a readout from an output variable, where data for each output may come from replicate determinations, e.g., multiple individual cells of the same type.
[0088] The readout may be a mean, average, median or the variance or other statistically or mathematically derived value associated with the measurement. The output readout information may be further refined by direct comparison with the corresponding reference readout. The absolute values obtained for each output under identical conditions will display a variability that is inherent in live biological systems and also reflects individual cellular variability as well as the variability inherent between individuals.
[0089] Exemplary Embodiments
[0090] In illustrative embodiments, the in vitro reagent is a cryopreserved mixture comprising metabolically competent cells (cells wherein cell membranes are permeabilized upon thawing), exogenous drug metabolizing enzyme co-factors and a buffered solution such as cell culture medium, wherein the reagent does not comprise a cryopreservative agent. The xenobiotic test article or compound (e.g. drug candidate) is metabolized by the metabolically competent cells in the presence of the exogenous co-factors.
[0091] In exemplary embodiments the present in vitro reagent is prepared for use to evaluate the metabolic effects of a test compound using cryopreserved metabolically competent cells with a permeabilized cell membrane, comprising the following steps: A) permeabilizing metabolically competent cells (e.g. hepatocytes or enterocytes); B) adding exogenous drug metabolizing enzyme co-factors either before or after the metabolically competent cells are permeabilized (e.g. NADPH, UDPGA, and PAPS); C) providing a cell culture medium. In embodiments, the in vitro reagent is further stored at a temperature of -10°C or lower. In illustrative embodiments, the cell membrane of the metabolically competent cells is permeabilized when thawed. [0092] In exemplary embodiments, the present in vitro reagent is used to evaluate the metabolic effects of a xenobiotic test compound comprising the following steps: A) thawing the in vitro reagent (prepared as disclosed herein) and placing in a cell culture vessel; B) introducing the xenobiotic test compound into the cell culture vessel; C) incubating the test compound for 0.5 h to 10 days at 33-40°C; and; D) performing an end point assay of the in vitro reagent or cell culture medium to determine metabolism of the xenobiotic test compound. See Examples 1-15 and Figures 1-20.
EXAMPLES
[0093] The following examples are put forth so as to provide those of ordinary skill in the art with a complete disclosure and description of how to use the embodiments provided herein, and are not intended to limit the scope of the disclosure nor are they intended to represent that the Examples below are all of the experiments or the only experiments performed. Efforts have been made to ensure accuracy with respect to numbers used (e.g. amounts, temperature, etc.) but some experimental errors and deviations should be accounted for. Unless indicated otherwise, parts are parts by volume, and temperature is in degrees Centigrade. It should be understood that variations in the methods as described can be made without changing the fundamental aspects that the Examples are meant to illustrate.
[0094] Example 1: In vitro reagent containing permeabilized hepatocytes for the evaluation of a xenobiotic test compound.
[0095] Hepatocytes are isolated from human livers by collagena.se digestion. The hepatocytes may be utilized from a single donor, or pooled from multiple donors. The hepatocytes are then cryopreserved in a serum free cell culture medium (Hepatocyte Incubation Medium (HQM), In Vitro ADMET Laboratories Inc., Columbia, MD)) in the presence of drug metabolizing enzyme cof actors: 2 niM NADPH, 5 mM UDPGA, and 1 mM PAPS at a concentration of 1 mil lion cells per mL. The cells are ali quoted at 5 raL aliquots and frozen in a -80 deg. C freezer. On the day of use, the hepatocyte/cofactor mixture (i.e. in vitro reagent) is thawed at 4°C and 50 ih of the mixture is added to 50 xL of HQM containing a xenobiotic test article at an appropriate concentration in wells of a 96-well plate. The plate is incubated in a ceil culture incubator maintained at 37°C for a specific time period (e.g. 60 minutes) after which an organic solvent (e.g. acetonitrile) as added at a volume of 100 ^lL to each well. The contents of the wells are collected for LC/MS-MS quantification of drug metabolism (e.g. parent disappearance; metabolite formation).
[§096] In embodiments, the hepatocytes are isolated from human livers by collagenase digestion and pooled from multiple donors to manufacture the present in vitro reagent containing permeabilized hepatocytes.
[0097] Example 2: In vitro reagent containing permeabilized enterocytes for the evaluation of a xenobiotic test compound
[0098] The assay was performed essentially as disclosed in Example 1 except enterocytes are isolated from human intestines by collagenase digestion. The enterocytes may be utilized from a single donor, or pooled from multiple donors. The enterocytes are then cryopreserved in a serum free cell culture medium in the presence of drug metabolizing enzyme cof actors: 2 mM NADPH, 5 mM UDPGA, and 1 mM PAPS at a concentration of 1 mil lion cells per mL. The cells are aliquoted at 5 mL aliquots and frozen in a -80 deg. C freezer. On the day of use, the
enterocyte/cofactor mixture (i.e. in vitro reagent) is thawed a 4°C and 50 μΐ,, of the mixture is added to 50 ,u,L of HQM containing a xenobiotic test article at an appropriate concentration in wells of a 96-well plate. The plate is incubated in a cell culture incubator maintained a 37°C for a specific time period (e.g. 60 minutes) after which an organic solvent (e.g. acetonitrile) as added at a volume of 100 μΐ. to each well. The contents of the wells are collected for LC/MS-MS quantification of drug metabolism (e.g. parent disappearance; metabolite formation).
[0099] In embodiments, the enterocytes are isolated from human intestines by collagenase digestion and pooled from multiple donors to manufacture the present in vitro reagent containing permeabilized enterocytes.
[00100] Table 1 : Drug Metabolism Enzyme Activities of Human Enterocytes
Figure imgf000027_0001
HE3013 NA NA 0.2 NA NA NA NA
HE3014 0.44 0.11 0.4 3.55 2.66 1.18 0.17
HE3015 2.50 0.49 2.55 7.33 5.23 0.95 0.51
HE3016 2.05 1.08 1.0 5.71 4.13 0.93 0.34
HE3019 0.24 0.11 0.30 1.47 1.89 0.26 0.30
HE3020 0.31 0.14 0.5 5.83 1.84 0.58 0.59
HE3021 0.20 0.06 0.17 1.49 1.64 0.19 0.08
HE3027 2.02 0.31 0.7 3.68 2.69 0.76 0.19
HE3028 0.68 0.21 0.82 3.84 9.02 0.71 0.30
HE3029 0.86 0.12 0.6 6.55 3.65 0.76 0.08
HE3031 0.34 0.09 0.16 1.60 0.79 0.49 0.18
[00101] Example 3: In vitro reagent containing permeabilized hepatocyte cell line for the evaluation of a xenobiotic test compound
[00102] The assay was performed essentially as disclosed in Example 1, except a hepatocyte cell line (e.g. HepaRG) known to contain drug metabolizing enzyme activity is used instead of primary hepatocytes. The hepatocyte cell line is cryopreserved in a serum free cell culture medium (Hepatocyte Incubation Medium (HQM), In Vitro ADMET Laboratories Inc.,
Columbia, MD) in the presence of drug metabolizing enzyme cof actors: 2 mM NADPH, 5 mM UDPGA, and 1 mM PAPS at a concentration of 1 million cells per mL. The cells are ali quoted at 5 mL aliquots and frozen in a -80 deg. C freezer. On the day of use, the hepatocyte/cofactor mixture (i.e. in vitro reagent) is thawed at 4°C and 50 lL of the mixture is added to 50 μΐ, of HQM containing a xenobiotic test article at an appropriate concentration in wells of a 96-well plate. The plate is incubated in a cell culture incubator maintained at 37°C for a specific time period (e.g. 60 minutes) after which an organic solvent (e.g. acetonitrile) as added at a volume of 100 uL to each well. The contents of the wells are collected for LC/MS-MS quantification of drug metabolism (e.g. parent disappearance; metabolite formation).
[00103] Example 4: Comparison of the in vitro reagent as compared to intact (non- permeabilized) metabolically competent cells (with or without enzyme co-factor added to the intact cells)
[00104] The assay was performed essentially as disclosed in Example 2, wherein the in vitro reagent comprises enterocytes and exogenous drug metabolizing enzyme co-factors (NADPH, UPGA, and PAPS), herein referred to as "cofactors". As comparators, intact enterocytes, that were not permeabilized, were used wherein one group was incubated with cofactors and another group was incubated without cofactors, each in the presence of the xenobiotic test compound. Permeabilized enterocytes incubated without cofactors were used as a control. The test groups were: Group A - intact enterocytes incubated without cofactors; Group B - intact enterocytes incubated with cofactors; Group C - permeabilized enterocytes incubated without cofactors (control); Group D - the in vitro reagent (permeabilized enterocytes incubated with cofactors). Metabolism of 7-ethoxycoumarin (7-ethoxycoumarin O-deethylation (ECOD) activity) was used as a test xenobiotic compound to demonstrate the difference in metabolism of each test group. Highest activity was observed with permeabilized enterocytes with cofactors (+cofactors) Group D, demonstrating the advantage of the present in vitro reagent. Permeabilization (by freezing without cryoprotectants followed by thawing) allows maximal interaction of the intracellular enzymes with the substrate (7-ethoxycoumarin), and the addition of cofactors overcomes the dilution of intracellular cofactors due to permeabilization. The results demonstrate
permeabilization and cofactor supplementation provides significantly higher enteric xenobiotic metabolism. See Figure 1.
[00105] Example 5: Evaluation and Detection of Key Drug Metabolizing Enzyme Activity
[00106] The assay was performed essentially as disclosed in Example 1. The cryopreserved hepatocyte/cof actor mixture (i.e. in vitro reagent) was thawed at 37°C and 50 μί, of the mixture is added to 50 ί. of HQM containing metabolic enzyme substrates at an appropriate concentration in wells of a 96-well plate. The plate was incubated in a cell culture incubator maintained at 37°C for a specific time period (e.g. 60 minutes) after which an organic solvent (e.g. acetonitrile) was added at a volume of 100 lL to each well. The contents of the wells are collected for LC/MS-MS quantification of metabolite formation.
[00107] The results demonstrated the permeabilized human hepatocytes possessed all key drug metabolizing enzyme activities. The major P450 isoform activities as a function of cell concentrations are shown. The linear concentration versus activity curves demonstrate that permeabilized hepatocytes can be used routinely as an in vitro drug metabolism system for scientific investigations. See Figure 2. [00108] Example 6: Evaluation and Detection of P450 Isoform-Selective Substrate in Intact Human Hepatocytes and the Present Permeabilized Hepatocytes over a period of 30 minutes to 240 minutes.
[00109] The assay was performed essentially as disclosed in Example 1. The cryopreserved permeabilized hepatocytes/cofactor mixture was thawed at 37°C and 50 jjL of the mixture was added to 50 ,u,L of HQM containing metabolic enzyme substrates at an appropriate concentration in wells of a 96-weil plate. The plate was incubated in a cell culture incubator maintained at 37°C for 30, 60, 120 and 240 minutes after which an organic solvent (e.g. acetonitrile) was added at a volume of 100 ΐ, to each well. The contents of the wells were collected for LC/MS-MS quantification of metabolite formation. The intact hepatocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to UCRM, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells per mL, followed by incubation with drug metabolism substrates as described above for the permeabilized hepatocytes.
[00110] The results demonstrate a similar trend in the linear time course of metabolite formation in both the intact human hepatocytes and the present permeabilized hepatocytes. See Figure 3
[00111] Example 7: Evaluation and Detection of Non-P450 Pathway-Selective Substrate in Intact Human Hepatocytes and the Present Permeabilized Hepatocytes over a period of 30 minutes to 240 minutes.
[00112] The assay was performed essentially as disclosed in Example 1. The cryopreserved permeabilized hepatocytes/cofactor mixture was thawed at 37°C and 50 .L of the mixture is added to 50 ,LlL of HQM containing metabolic enzyme substrates at an appropriate concentration in wells of a 96-well plate. The plate was incubated in a cel l culture incubator maintained at 37°C for 30, 60, 120 and 240 minutes after which an organic solvent (e.g. acetonitrile) was added at a volume of 100 .L to each well. The contents of the wells are collected for LC/MS-MS quantification of metabolite formation. The intact hepatocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to UCRM, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells per mL, followed by incubation with drug metabolism substrates as described above for the permeabilized hepatocytes. [00113] The results demonstrate a similar trend in the linear time course of metabolite formation in both the intact human hepatocytes and the present permeabilized hepatocytes. See Figure 4
[00114] Example 8: Evaluation of Coumarin Metabolism Demonstrating Sequential Metabolism: Phase 1 Oxidation Followed by Phase 2 Conjugation of Metabolites.
[00115] The assay was performed essentially as disclosed in Example 1. The cryopreserved permeabilized hepatocytes/cofactor mixture was thawed at 37°C and 50 U.L of the mixture was added to 50 μΐ, of HQM containing 75 micromolar coumarin in wells of a 96-well plate. See Figure 5 for a cartoon drawing of coumarin metabolism. The plate was incubated in a cell culture incubator maintained at 37°C for 30 minutes after which an organic solvent (e.g.
acetonitrile) as added at a volume of 100 μΐ, to each well. The contents of the wells were collected for LC/MS-MS quantification of metabolite formation (7-hydroxycoumarin and its conjugated metabolites, 7-glucuronide and 7-sulfate coumarin). The intact hepatocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to UCRM, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells per mL, followed by incubation with drug metabolism substrates as described above for the permeabilized
hepatocytes.
[00116] The results demonstrate the present permeabilized hepatocytes are capable of sequential drug metabolism, similar to intact human hepatocytes. See Figure 6.
[00117] Example 9: Evaluation of Drug Metabolizing Enzymes in Intact Human Hepatocytes and Present Permeabilized Hepatocytes
[00118] The permeabilized hepatocytes were prepared essentially as disclosed in Example 1, wherein the hepatocytes were pooled from multiple donors. The cryopreserved permeabilized hepatocytes/cofactor mixture was thawed at 37°C and 50 uL of the mixture was added to 50 uL of HQM containing metabolic pathway-selective substrates (Se Table 2 below). The plate was incubated in a cell culture incubator maintained at 37°C for 30 minutes after which an organic solvent (e.g. acetonitrile) was added at a volume of 100 Ε to each well. The contents of the wells were collected for LC/MS-MS quantification of metabolite formation. The intact hepatocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to UCRM, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells mL, followed by incubation with drug metabolism substrates as described above for the permeabilized hepatocytes.
[00119] Table 2: drug metabolizing enzyme substrates evaluated:
Figure imgf000032_0001
[00120] The results demonstrate the present permeabilized hepatocytes and intact human hepatocytes possess similar activities in the metabolism of 17 pathway- selective drug metabolizing enzyme pathways. See Figure 7. The results suggest the present permeabilized human hepatocytes can be used in lieu of intact human hepatocytes for drug metabolism studies. The convenience of the permeabilized human hepatocytes allows it to be a more efficient experimental system than the conventional human intact hepatocytes.
[00121] Example 10: Evaluation of Drug Metabolizing Enzymes in Intact Human Enterocytes and Present Permeabilized Enterocytes
[00122] The permeabilized enterocytes were prepared essentially as disclosed in Example 2, wherein the enterocytes were pooled from multiple donors. The cryopreserved permeabilized enterocytes/cofactor mixture was (hawed at 37°C and 50 ,u,L of the mixture was added to 50 ΐ. of HQM containing metabolic pathway-selective substrates (See Table 3). The plate was incubated in a cell culture incubator maintained at 37°C for 30 minutes after which an organic solvent (e.g. acetonitriie) was added at a volume of 100 μL· to each well. The contents of the wells were collected for LC/MS-MS quantification of metabolite formation. The intact enterocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to Cryopreserved Enterocytes Recovery Medium, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells per mL, followed by incubation with drug metabolism substrates as described above for the permeabilized enterocytes.
[00123] The following drug metabolizing enzyme substrates (See Table 3) were evaluated in intact human enterocytes, pooled intact human enterocytes and permeabilized enterocytes and the metabolite activity measured. The results demonstrate the present permeabilized human enterocytes are equal or more active than the intact human enterocytes in all pathways evaluated.
[00124] Table 3: Enhanced drug metabolism enzyme activities of permeabilized
cryopreserved human enterocytes
Figure imgf000033_0001
CYP3A4- 6βΟΗ-
Testosterone 10.6 + 3.3 10.1 + 2.59 147 ± 14.5
2 testosterone
7-
7-OH-
UGT Hydroxycoumarin 16.05 + 0.32 6.31 + 0.43 275 ± 79.5
Coumarin
Glucuronide
7-
7-OH-
SULT Hydroxycoumarin 7.24 + 0.34 4.64 + 0.15 13 ± 0.69
Coumarin
Sulfate
O-Demethyl
2J2 Astemizole 0.92 + 0.43 BLQ 5.14 ± 1.53
Astemizole
CES2 Irinotecan SN38 0.37 + 0.14 0.03 + 0.07 0.38 ± 0.27
[00125] Example 11: Metabolic Stability Screening - Evaluation of Intrinsic Hepatic
Clearance.
[00126] Eighteen drugs (See Table 4) with known in vivo hepatic clearance were evaluated in both intact human hepatocytes and the present permeabilized hepatocytes, which were prepared essentially as disclosed in Example 1 wherein the hepatocytes from multiple donors were pooled. The drugs evaluated were added at a concentration of 1 μΜ to a hepatocyte culture of 1 million cells/ml. The cell culture was incubated and metabolites measured at time points: 0, 5, 15, 30 and 45 minutes and in vivo clearance measured. See Table 4, wherein in vivo clearance and predicted clearance using intact human hepatocytes and the present permeabilized hepatocytes are provided.
[00127] Table 4: Evaluation of drugs with known in vivo hepatic clearance
Figure imgf000034_0001
CYP1A2 » UGT,
Clozapine 6.1 4.6 1.4 3.2 3.1
2D6, 3A4
Desipr amine CYP2D6 > UGT 10.3 3.1 0.1 5.0 1.4
Dextromethorphan CYP2D6 > 3A/2C19 8.6 10.3 0.6 7.3 0.7
Diazepam CYP2C19 > 3 A 0.4 3.7 0.5 2.5 0.9
Diclofenac CYP2C9 4.2 13.9 0.8 16.9 0.5
Diltiazem CYP3A4 12 8.2 0.5 4.8 1.8
Furosemide P450 1.7 4.8 2.4 2.0 1.7
CYP2D6/1A2/2C19/
Imipramine 8 10.5 0.3 8.9 0.6
3A/UGT1A4
Lorazepam UGT 1.1 2.0 1.0 0.7 0.6
Nifedipine CYP3A4 15 10.5 0.2 10.4 1.0
CYP2D6 >
Propranolol 13 10.7 0.4 7.6 0.7
1A2/2C19/UGT
Verapamil CYP3A4 14 13.6 0.5 12.9 1.0
Warfarin CYP2C9, 3A4 0.05 2.9 0.9 1.5 0.8
[00128] The results demonstrated a linear correlation with in vivo hepatic clearance, wherein a similar result is shown for both the intact human hepatocytes and the present permeabilized human hepatocytes. However, the present permeabilized human hepatocytes yield a higher coefficient of correlation than intact human hepatocytes. See Figure 10.
[00129] Example 12: Metabolite Profiling - Metabolite Formation at Cytotoxic Drug
Concentrations
[00130] Human hepatocytes, with complete drug metabolizing enzyme (DME) pathways, should be ideal for metabolite profiling studies. However, due to cytotoxicity, hepatocytes in general cannot be incubated with high drug concentrations to allow the production of adequate quantity of metabolites for identification.
[00131] The permeabilized hepatocytes were prepared essentially as disclosed in Example 1, wherein the hepatocytes were pooled from multiple donors. The cryopreserved permeabilized hepatocytes/cofactor mixture was thawed at 37°C and 50 μΕ of the mixture was added to 50 μΕ of HQM containing a noncytotoxic concentration (10 iiiM), and two cytotoxic concentrations (100 and 200 mM) of acetaminophen (APAP) in wells of a 96-well plate. The plate was incubated in a cell culture incubator maintained at 37°C for 30 minutes after which an organic solvent (e.g. acetonitriie) as added at a volume of 100 μΐϋ to each well. The contents of the wells are collected for LC/MS-MS quantification of metabolite formation (giucuronide, sulfate, and glutathione conjugated acetaminophen). The intact hepatocytes were thawed at 37°C, recovered by adding the thawed hepatocytes to UCRM, centrifuged at 100 x g for 10 minutes, resuspended in HQM followed by microscopic evaluation of viability based on trypan blue, cell concentration adjusted with HQM to 2 million cells per mL, followed by incubation with drug metabolism substrates as described above for the permeabilized hepatocytes.
[00132] The results demonstrate a similar metabolite profiles for giucuronide, sulfate and GDH conjugate at the noncytotoxic (10 mM) concentration. However, the present permeabilized human hepatocytes demonstrated an enhanced metabolite formation as compared to intact human hepatocytes at cytotoxic concentrations (100 and 200 mM) of acetaminophen. See Figure 11. These results suggest the present permeabilized human hepatocytes can be incubated with high, cytotoxic concentrations of a xenobiotic, such as a drug, for the generation of sufficient amounts of metabolites for identification and profiling.
[00133] Example 13: Cofactor-Directed Metabolic Pathway Selection
[00134] Intact human hepatocytes allow metabolism of a drug by all hepatic pathways, selection of a specific metabolic pathway for evaluation is not easily accomplished. However, the experiment disclosed herein demonstrates the present permeabilized human hepatocytes can be used to direct metabolism to specific pathways via selection of cofactors (e.g., exogenous drug metabolizing enzyme co-factors).
[00135] The metabolism of coumarin was used as a model for cofactor directed metabolic pathway selection. See Figure 12 for the co-factor directed pathway selection of coumarin metabolism with the present permeabilized human hepatocytes. The exogenous drug
metabolizing enzyme co-factors used were 2 mM NADPH, 2 mM NADPH + 1 mM PAPS and 2 mM NADPH + 5 mM UDGPGA, and no cofactor addition used as a control. The cryopreserved permeabilized hepatocytes with the various cofactor compositions were thawed at 37°C and 50 μL of the mixture was added to 50 μ!_, of HQM containing 75 microniolar of coumarin. The plate is incubated in a cell culture incubator maintained at 37°C for 30 minutes after which an organic solvent (e.g. acetonitriie) as added at a volume of 100 μί. to each well. The contents of the wells were collected for LC/MS-MS quantification of metabolite formation. The metabolites 7-OH coumarin (7-HC), 7-HC-sulfate (7-HCS) and 7-HC-glucuronide (7-HCG) were measured. See Figure 13.
[00136] Table 5: Cofactor selection
Figure imgf000037_0001
[00137] Example 14: Evaluation of the Present Permeabilized Human Hepatocytes as Exogenous Metabolic Activation System for the Evaluation of Prototoxicants
[00138] Acetaminophen (See Figure 14), Cyclophosphamide (See Figure 15) and Ifosfamide were evaluated in the following prototoxicant activation assay. In this assay permeabilized human hepatocytes were used in an exogenous metabolic system for evaluation of the physiological effect of metabolites of the prototoxicants towards a target cell line, the HEK293 cells which are devoid of xenobiotic drug metabolism activities. Inactivated (boiled) permeabilized human hepatocytes were used as a metabolic negative control.
[00139] In this assay, HEK293 cells were cultured in DMEM in a 96-well plate (10,000 cells per well; 50 μί) followed by addition of an equal volume of various concentrations of the prototoxicants acetaminophen, cyclophosphamide, and ifosfamide and an equal volume of medium containing permeabilized human hepatocytes (cofactor supplemented), boiled permeabilized hepatocytes or no hepatocytes. The cell cultures were incubated in a cell culture incubator maintained in a 37 C highly humidified atmosphere of 5% carbon dioxide and 95% air for 24 hours. After incubation, cellular ATP content of the HEK293 cells in each well were quantified using Promega Glo™, a luminescent ATP quantification reagent (Promega Inc., Madison, WI), with luminescence quantified using a Perkin Elmer Victor 3 plate reader.
[00140] The results demonstrate the cytotoxicity of Acetaminophen, Cyclophosphamide and Ifosfamide on HEK 293 cells was enhanced by the present permeabilized human hepatocytes, wherein the present permeabilized human hepatocytes can be used as an exogenous activating system for the evaluation of prototoxicants. See Figure 16 for activation of Acetaminophen and Figure 17 for activation of Ifosfamide and Cyclophosphamide.
[00141] Example 15: Evaluation of the inhibition of intestinal CYP3A4 from orally administered drugs - Drug-Drug Interactions and Food-Drug Interactions.
[00142] Permeabilized cofactor supplemented enterocytes were prepared from cryopreserved intact enterocytes from 10 donors, see Example 2. Effects of herbal supplements on enterocyte CYP3A4 activity was evaluated using luciferin IPA as CYP3A4 substrate (LIPA ; Promega, Madison, WI) with luminescence quantified on a Perkin Elmer Wallac 1420 Victor microplate reader. The herbal supplements were obtained commercially. The daily recommended dose was dissolved in 50 mL (4X of 100% concentration) of HQM (IVAL), pH adjusted to 7.0 to 7.2, and sterilized by filtration. For the drug interaction studies, aliquots of 50 of permeabilized enterocyte suspension per well were added to 96-well plates, followed by an addition of 25 of the 4X herbal supplements and 25 of 4X LIPA. CYP3A4 activity was quantified after an incubation period of 60 minutes.
[00143] The results are shown in Fig. 20. The results show that permeabilized enterocytes can be used for the evaluation of food-drug interactions. Herbal supplements with significant CYP3A4 inhibitory effects (e.g. green tea extract; grapefruit juice) are likely to inhibit enteric metabolism of orally-administered drugs that are CYP3A4 substrates.
[00144] Those skilled in the art can devise many modifications and other embodiments within the scope and spirit of the presently disclosed inventions. Indeed, variations in the materials, methods, drawings, experiments examples and embodiments described may be made by skilled artisans without changing the fundamental aspects of the disclosed inventions. Any of the disclosed embodiments can be used in combination with any other disclosed embodiment.
[00145] The disclosed embodiments, examples and experiments are not intended to limit the scope of the disclosure nor to represent that the experiments below are all or the only
experiments performed. Efforts have been made to ensure accuracy with respect to numbers used (e.g., amounts, temperature, etc.) but some experimental errors and deviations should be accounted for. It should be understood that variations in the methods as described may be made without changing the fundamental aspects that the experiments are meant to illustrate.

Claims

1. An in vitro reagent for evaluating xenobiotic metabolism, wherein the reagent is a
cryopreserved mixture comprising:
a) metabolically competent cells wherein cell membranes are permeabilized upon
thawing; b) exogenous drug metabolizing enzyme co-factors, and c) a buffered solution, wherein the reagent does not comprise a cryopreservative agent.
2. The reagent of claim 1, wherein the metabolically competent cells are hepatocytes.
3. The reagent of claim 1, wherein the metabolically competent cells are enterocytes.
4. The reagent of claim 1, wherein the metabolically competent cells are engineered to
contain cytochrome P450 isoforms.
5. The reagent of claim 1, wherein the metabolically competent cells comprise drug
metabolizing enzyme (DME) activities.
6. The reagent of claim 1, wherein the metabolically competent cells are human, rat,
monkey, dog, mammals, avian or non-mammalian.
7. The reagent of claim 1, wherein the metabolically competent cells are primary cells.
8. The reagent of claim 7, wherein the metabolically competent cells are pooled from more than one donor.
9. The reagent of claim 1, wherein the metabolically competent cells are a cell line.
10. The reagent of claim 1, wherein the drug metabolizing enzyme co-factors are selected from β-Nicotinamide adenine dinucleotide 2'-phosphate (NADPH), Uridine 5'- diphosphoglucuronic acid (UDPGA), 3'-Phosphoadenosine 5 '-phosphosulfate (PAPS), N- acetyl coenzyme A, s-adenosyl methionine, amino acids, carnitine, and L-glutathione.
11. The reagent of claim 1, wherein the reagent is stored frozen at a temperature of -10°C to about -80°C.
12. The reagent of claim 11, wherein the reagent is thawed prior to use for evaluating
xenobiotic metabolism.
13. The reagent of claim 1, wherein the reagent is further added to and comprises a mammalian or non-mammalian culture, wherein the reagent provides exogenous metabolic functions for evaluation of a physiological effect of metabolites of a xenobiotic.
14. The method of claim 13, wherein the non-mammalian culture comprises Salmonella bacteria used in an Ames Salmonella histidine reversion assay (Ames test) for geno toxicity.
15. The method of claim 13, wherein the mammalian or non-mammalian culture comprises cells used in a genotoxicity assay.
16. The method of claim 13, wherein the mammalian or non-mammalian culture comprises cells used in a cytotoxicity assay.
17. The method of claim 13, wherein the mammalian or non-mammalian culture comprises cells used in a pharmacological assay.
18. The reagent of claim 1, wherein the reagent is provided in a kit and further comprises instructions for evaluating xenobiotic metabolism using the reagent.
19. The reagent of claim 1, wherein the metabolically competent cells comprise
permeabilized plasma membranes.
20. An in vitro reagent for evaluating xenobiotic metabolism, wherein the reagent is a cryopreserved mixture comprising: a) metabolically competent cells selected from hepatocytes or enterocytes wherein cell membranes of the hepatocytes or enterocytes are permeabilized upon thawing; b) exogenous drug metabolizing enzyme co-factors selected from β -Nicotinamide adenine dinucleotide 2'-phosphate (NADPH), Uridine 5'-diphosphoglucuronic acid (UDPGA), 3'-Phosphoadenosine 5'-phosphosulfate (PAPS), N-acetyl coenzyme A, s- adenosyl methionine, amino acids, carnitine, and L-glutathione; and, c) a buffered solution, wherein the reagent does not comprise a cryopreservative agent.
21. A method for manufacturing an in vitro reagent for evaluating xenobiotic metabolism, comprising: a) permeabilizing metabolically competent cells; b) adding exogenous drug metabolizing enzyme co-factors either before or after the metabolically competent cells are permeabilized; and c) providing a buffered solution, wherein the reagent does not comprise a cryopreservative agent.
22. The method of claim 21, wherein the reagent is further stored frozen at a temperature of - 10°C to about -80°C.
23. The method of claim 21, wherein the reagent is not stored frozen in liquid nitrogen.
24. The method of claim 21, wherein the metabolically competent cells are permeabilized by freezing and thawing in the absence of a cryopreservative agent.
25. The method of claim 24, wherein the permeabilized metabolically competent cells are not centrifuged prior to use.
26. The method of claim 24, wherein the permeabilized metabolically competent cells are not counted prior to use.
27. The method of claim 21, wherein the metabolically competent cells are hepatocytes.
28. The method of claim 21, wherein the metabolically competent cells are enterocytes.
29. The method of claim 21, wherein the metabolically competent cells are engineered to contain cytochrome P450 isoforms.
30. The method of claim 21, wherein the metabolically competent cells comprise drug
metabolizing enzyme (DME) activities.
31. The method of claim 21, wherein the metabolically competent cells are human, rat,
monkey, dog, mammals, avian or non-mammalian.
32. The method of claim 21, wherein the metabolically competent cells are primary cells.
33. The method of claim 32, wherein the metabolically competent cells are pooled from more than one donor
34. The method of claim 21, wherein the metabolically competent cells are a cell line.
35. The method of claim 21, wherein the drug metabolizing enzyme co-factors are selected from β-Nicotinamide adenine dinucleotide 2'-phosphate (NADPH), Uridine 5'- diphosphoglucuronic acid (UDPGA), 3'-Phosphoadenosine 5 '-phosphosulfate (PAPS), N- acetyl coenzyme A, s-adenosyl methionine, amino acids, carnitine, and L-glutathione.
36. A method for manufacturing an in vitro reagent for evaluating xenobiotic metabolism, comprising:
a) combining intact metabolically competent cells with exogenous drug metabolizing enzyme co-factors in a cell culture medium to form a cell mixture;
b) freezing the cell mixture at a temperature from about -10°C to about -80°C, wherein the cell mixture does not comprise a cryopreservative agent; and,
c) thawing the cell mixture to form the in vitro reagent wherein cell membranes of the metabolically competent cells are permeabilized via thawing.
37. The method of claim 36, wherein the in vitro reagent is used to evaluate xenobiotic
metabolism after thawing without the step of centrifuging or cell counting.
38. The method of claim 36, wherein the metabolically competent cells are hepatocytes.
39. The method of claim 36, wherein the metabolically competent cells are enterocytes.
40. The method of claim 36, wherein the metabolically competent cells are engineered to contain cytochrome P450 isoforms.
41. The method of claim 36, wherein the metabolically competent cells comprise drug
metabolizing enzyme (DME) activities.
42. The method of claim 36, wherein the metabolically competent cells are human, rat,
monkey, dog, mammals, avian or non-mammalian.
43. The method of claim 36, wherein the metabolically competent cells are primary cells.
44. The method of claim 43, wherein the metabolically competent cells are pooled from more than one donor.
45. The method of claim 36, wherein the metabolically competent cells are a cell line.
46. The method of claim 36, wherein the drug metabolizing enzyme co-factors are selected from β-Nicotinamide adenine dinucleotide 2'-phosphate (NADPH), Uridine 5'- diphosphoglucuronic acid (UDPGA), 3'-Phosphoadenosine 5 '-phosphosulfate (PAPS), N- acetyl coenzyme A, s-adenosyl methionine, amino acids, carnitine, and L-glutathione.
47. A method for evaluating xenobiotic metabolism, comprising: a) providing the cryopreserved in vitro reagent of claim 1 ; b) thawing the in vitro reagent and placing in a cell culture vessel; c) introducing the xenobiotic test compound into the cell culture vessel; d) incubating the test compound for 0.5 h to 10 days at 33-40°C; and, e) performing an end point assay of the in vitro reagent or cell culture medium to determine metabolism of the xenobiotic test compound.
48. The method of claim 47, wherein the end point assay is an Ames Salmonella histidine reversion assay (Ames test) for genotoxicity.
49. The method of claim 47, wherein the end point assay is a mammalian or non-mammalian genotoxicity assay.
50. The method of claim 47, wherein the end point assay is a mammalian or non-mammalian cytotoxicity assay.
51. The method of claim 47, wherein the end point assay is a mammalian or non-mammalian pharmacological assay.
52. The method of claim 47, wherein the cell culture vessel comprising the in vitro reagent and test compound is incubated at 37°C.
53. The method of claim 47, wherein the xenobiotic agent is a drug or drug candidate.
54. The method of claim 47, wherein the xenobiotic agent is an industrial chemical.
55. The method of claim 47, wherein the xenobiotic agent is an environmental pollutant.
56. The method of claim 53, wherein the drug or drug candidate is selected from the group consisting of an organic compound, an inorganic compound, a hormone, a growth factor, a cytokine, a reception, an antibody, an enzyme, a peptide, an aptomer and a vaccine.
57. The method of claim 47, wherein step b) does not further comprise a centrifugation or cell counting step.
58. The method of claim 47, wherein the cryopreserved in vitro reagent of step a) comprises exogenous drug metabolizing enzyme co-factors used to select metabolism pathways.
59. The method of claim 47, wherein drug or drug candidate is added at cytotoxic
concentrations for identifying and profiling metabolites.
60. The method of claim 47, wherein complete phase 1 oxidation and phase 2 conjugation of metabolites are evaluated with the reagent of step a).
61. The method of claim 47, wherein time to perform combined steps a), b) and c) takes about 10 minutes or less.
62. The method of claim 47, wherein time to perform combined steps a), b) and c) takes about 2 minutes to 6 minutes.
63. The method of claim 47, further comprising evaluating metabolic stability, metabolite profiling and identification, enzyme inhibition or metabolic activation of proto-toxicants or pro-mutagens.
64. The method of claim 47, wherein the method does not comprise use of a microscope before step e).
65. An exogenous metabolic system for evaluation of a physiological effect of metabolites of a xenobiotic test compound; comprising: a) a cell culture medium admixture comprising; i) metabolically competent cells comprising permeabilized plasma membranes; and, ii) exogenous drug metabolizing enzyme co-factors, and b) metabolically incompetent target cells.
66. The exogenous metabolic system of claim 65, further comprising a cell culture vessel comprising one or more assay wells, wherein the assay wells comprise the cell culture medium admixture and metabolically incompetent cells.
67. The exogenous metabolic system of claim 65, wherein the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture.
68. The exogenous metabolic system of claim 66, wherein each assay well is divided into a first and second chamber, wherein a first chamber comprises the cell culture medium admixture and the second chamber comprises the metabolically incompetent target cells provided the metabolically incompetent target cells are in fluid communication with the cell culture medium admixture.
69. The exogenous metabolic system of claim 68, wherein the first and second chamber are separated by a porous membrane that is liquid-permeable and cell-impermeable.
70. The exogenous metabolic system of claim 65, wherein the metabolically incompetent target cells are mammalian or non-mammalian cells.
71. The exogenous metabolic system of claim 65, wherein the metabolically competent cells are hepatocytes.
72. The exogenous metabolic system of claim 65, wherein the metabolically competent cells are enterocytes.
73. The exogenous metabolic system of claim 65, wherein the metabolically competent cells are engineered to contain cytochrome P450 isoforms.
74. The exogenous metabolic system of claim 65, wherein the metabolically competent cells comprise drug metabolizing enzyme activities.
75. The exogenous metabolic system of claim 65, wherein the metabolically competent cells are human, rat, monkey, dog, mammals, avian or non-mammalian.
76. The exogenous metabolic system of claim 65, wherein the metabolically competent cells are primary cells.
77. The exogenous metabolic system of claim 65, wherein the metabolically competent cells are a cell line.
78. The exogenous metabolic system of claim 65, wherein the drug metabolizing enzyme co- factors are selected from β-Nicotinamide adenine dinucleotide 2'-phosphate (NADPH), Uridine 5'-diphosphoglucuronic acid (UDPGA), 3'-Phosphoadenosine 5'-phosphosulfate (PAPS), N-acetyl coenzyme A, s-adenosyl methionine, amino acids, carnitine, and L- glutathione.
PCT/US2017/054853 2016-10-03 2017-10-03 In vitro drug metabolism reagent and uses thereof WO2018067504A1 (en)

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