CA2403303A1 - Method of identifying ginko biloba in a plant extract by gene profiling - Google Patents
Method of identifying ginko biloba in a plant extract by gene profiling Download PDFInfo
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Abstract
The present invention is directed to a method of establishing an "identity" of Ginkgo biloba leaves or isolated ginkgolide B (GKB) or another component of the extract of Ginkgo biloba leaves, by obtaining a "gene regulation profile".
The invention is also directed to a method of verifying the identity of a Ginkgo biloba extract by comparing the gene regulation profile of a Gingko biloba extract of unknown or questionable origin with the gene regulation pofile of a Gingko biloba extract of known origin. The present invention is further directed to a method of establishing a gene expression profile of Ginkgolide A, Ginkgolide B or any other component isolated from a Ginkgo biloba extract, more particularly, from EGB 761®.
The invention is also directed to a method of verifying the identity of a Ginkgo biloba extract by comparing the gene regulation profile of a Gingko biloba extract of unknown or questionable origin with the gene regulation pofile of a Gingko biloba extract of known origin. The present invention is further directed to a method of establishing a gene expression profile of Ginkgolide A, Ginkgolide B or any other component isolated from a Ginkgo biloba extract, more particularly, from EGB 761®.
Description
METHOD OF PROFILING A PLANT EXTRACT
Statement Regarding Federally Sponsored Research The present invention was sponsored in part by grants ES-07747 NIEHS, from the National Institutes of Health and, thus, the U.S. government may have certain rights in the present invention.
Background of the Invention The present invention is directed to a method of establishing an "idenfiity"
of Ginkgo biloba leaves or isolated ginkgolide B (GKB), a component of the extract of Ginkgo biloba leaves, by obtaining a "gene regulation profile". The invention is also directed to a method of verifying the identity of a Ginkgo biloba extract by comparing the gene regulation profile of a Gingko biloba extract of unknown or questionable origin with the gene regulation profile of a Gingko biloba extract of known origin.
The term "known origin" refers to the commercial source of the extract. A preferred aspect of the present invention is where the Ginkgo biloba extract of known origin is EGB
761~, produced and marketed by IPSEN of Paris, France. More particularly, this invention is directed to a method for determining the authenticity of an extract of unknown origin purporting to be EGB 761~. The present invention is further directed to a method of establishing a gene expression profile of Ginkgolide A, Ginkgolide B or any other component isolated from a Ginkgo biloba extract, more particularly, from EGB
761~.
Pharmaceutical manufacturing is based on control over the composition and the consistency of the biological activity profile of a manufactured batch. This standardization and control provides reproducible material in the predictable and consistent treatment of patients. Such use of standardization and control to guard against the marketing of counterfeit extracts purporting to be EGB 761~ is beneficial to patients since it assures patients that they are obtainingireceiving an extract with a particular biological activity profile.
Ginkgo biloba is one of the most ancient trees, and extracts from its leaves have been used in traditional medicine for several hundred years. There are numerous studies describing the beneficial effects of Ginkgo biloba extracts on patients with disturbances in vigilance, memory, and cognitive functions associated with aging and senility, and on those with all types of dementias, mood changes, and the ability to cope with daily stressors. A standardized extract of Ginkgo biloba leaves, termed EGB
761~, has been used in most of these studies. This extract is also known to have cardioprotective effects (DeFeudis F.V. Ginkgo biloba extract (EGB 761~): from chemistry to clinic. Ullstein Medical, Wisbaden, Germany. 400 pp. 1998;
Tosaki, A., Droy-Lefaix, M.T., Pali, T., and Das, D.K., Free Rad. Biol. Med., 14: 361-370, 1993).
These effects have been attributed, at least in part, to the free radical scavenging properties of EGB 761~, probably due to the presence of flavonoid or terpenoid constituents in the extract. Recent in vivo and in vitro studies demonstrated that the terpene constituents of EGB 761~, ginkgolides and bilobalide, have anti-oxidant properties (Pietri, S., Maurelli, E., Drieu, K., and Culcasi, M., J. Mol.
Cell. Cardiol., 29:
7 0 733-742, 1997; Yao, Z., Boujrad, N., Drieu, K., and Papadopoulos, V., Adv.
Ginkgo Biloba Res. 7: 129-138, 1998). Other studies of EGB 761~ have reported medicinal value of the product in the treatment of a variety of clinical disorders including cerebrovascular and peripheral vascular insufficiencies associated with aging and senility. See e.g., Ginkgo biloba Extract (EGB 761~) Pharmacological Activities and Clinical Applications, DeFeudis, F.V., Eds, Elsevier, 1991; and Ullstein Medical 1998, Ginkgo biloba extract (EGB 761~), Eds. Wiesbaden, DeFeudis, F.V. The extract contains 24% ginkgo-flavone glycosides, 6% terpene lactones (ginkgolides and bilobalide), about 7% proanthocyanidins and several other constituents. See Boralle, N., et al., In: Ginkgolides, Chemistry, Biology, Pharmacology and Clinical perspectives, Ed: Braquet, P., J.R. Prous Science Publishers, 1988.
More frequently, counterfeit formulations purporting to be EGB 761 ~ are being placed in the stream of commerce. Such counterfeits do not possess the same composition of components that constitute authentic EGB 761~. Patients who obtain counterfeit EGB 761~, believing that the counterfeit is authentic, are being deprived the benefit of EGB 761 ~'s full range of biological activity. Further, the good will associated with EGB 761 ~ is being eroded. Hence, there is a need for a method of establishing the biological activity profile of EGB 761~, which can then be used to compare with the biological activity profile of a counterfeit EGB 761 to screen such counterfeits from the marketplace.
Statement Regarding Federally Sponsored Research The present invention was sponsored in part by grants ES-07747 NIEHS, from the National Institutes of Health and, thus, the U.S. government may have certain rights in the present invention.
Background of the Invention The present invention is directed to a method of establishing an "idenfiity"
of Ginkgo biloba leaves or isolated ginkgolide B (GKB), a component of the extract of Ginkgo biloba leaves, by obtaining a "gene regulation profile". The invention is also directed to a method of verifying the identity of a Ginkgo biloba extract by comparing the gene regulation profile of a Gingko biloba extract of unknown or questionable origin with the gene regulation profile of a Gingko biloba extract of known origin.
The term "known origin" refers to the commercial source of the extract. A preferred aspect of the present invention is where the Ginkgo biloba extract of known origin is EGB
761~, produced and marketed by IPSEN of Paris, France. More particularly, this invention is directed to a method for determining the authenticity of an extract of unknown origin purporting to be EGB 761~. The present invention is further directed to a method of establishing a gene expression profile of Ginkgolide A, Ginkgolide B or any other component isolated from a Ginkgo biloba extract, more particularly, from EGB
761~.
Pharmaceutical manufacturing is based on control over the composition and the consistency of the biological activity profile of a manufactured batch. This standardization and control provides reproducible material in the predictable and consistent treatment of patients. Such use of standardization and control to guard against the marketing of counterfeit extracts purporting to be EGB 761~ is beneficial to patients since it assures patients that they are obtainingireceiving an extract with a particular biological activity profile.
Ginkgo biloba is one of the most ancient trees, and extracts from its leaves have been used in traditional medicine for several hundred years. There are numerous studies describing the beneficial effects of Ginkgo biloba extracts on patients with disturbances in vigilance, memory, and cognitive functions associated with aging and senility, and on those with all types of dementias, mood changes, and the ability to cope with daily stressors. A standardized extract of Ginkgo biloba leaves, termed EGB
761~, has been used in most of these studies. This extract is also known to have cardioprotective effects (DeFeudis F.V. Ginkgo biloba extract (EGB 761~): from chemistry to clinic. Ullstein Medical, Wisbaden, Germany. 400 pp. 1998;
Tosaki, A., Droy-Lefaix, M.T., Pali, T., and Das, D.K., Free Rad. Biol. Med., 14: 361-370, 1993).
These effects have been attributed, at least in part, to the free radical scavenging properties of EGB 761~, probably due to the presence of flavonoid or terpenoid constituents in the extract. Recent in vivo and in vitro studies demonstrated that the terpene constituents of EGB 761~, ginkgolides and bilobalide, have anti-oxidant properties (Pietri, S., Maurelli, E., Drieu, K., and Culcasi, M., J. Mol.
Cell. Cardiol., 29:
7 0 733-742, 1997; Yao, Z., Boujrad, N., Drieu, K., and Papadopoulos, V., Adv.
Ginkgo Biloba Res. 7: 129-138, 1998). Other studies of EGB 761~ have reported medicinal value of the product in the treatment of a variety of clinical disorders including cerebrovascular and peripheral vascular insufficiencies associated with aging and senility. See e.g., Ginkgo biloba Extract (EGB 761~) Pharmacological Activities and Clinical Applications, DeFeudis, F.V., Eds, Elsevier, 1991; and Ullstein Medical 1998, Ginkgo biloba extract (EGB 761~), Eds. Wiesbaden, DeFeudis, F.V. The extract contains 24% ginkgo-flavone glycosides, 6% terpene lactones (ginkgolides and bilobalide), about 7% proanthocyanidins and several other constituents. See Boralle, N., et al., In: Ginkgolides, Chemistry, Biology, Pharmacology and Clinical perspectives, Ed: Braquet, P., J.R. Prous Science Publishers, 1988.
More frequently, counterfeit formulations purporting to be EGB 761 ~ are being placed in the stream of commerce. Such counterfeits do not possess the same composition of components that constitute authentic EGB 761~. Patients who obtain counterfeit EGB 761~, believing that the counterfeit is authentic, are being deprived the benefit of EGB 761 ~'s full range of biological activity. Further, the good will associated with EGB 761 ~ is being eroded. Hence, there is a need for a method of establishing the biological activity profile of EGB 761~, which can then be used to compare with the biological activity profile of a counterfeit EGB 761 to screen such counterfeits from the marketplace.
Summary of the Invention The present invention is directed to a method of establishing a gene regulation profile of a Gingko biloba extract or a component of the Ginkgo biloba extract, which comprises the steps of:
obtaining at least one batch of untreated cells;
treating a first batch of cells with an extract of Ginkgo biloba or a component of the Ginkgo biloba extract to obtain a treated batch of cells;
quantifying an affect on the expression of one or more genes of the treated cells to obtain a quantity of affected genes; and comparing the quantity of affected genes with a quantity of genes of cells not treated with Ginkgo biloba or a component of the Ginkgo biloba extract to obtain the gene regulation profile of the Ginkgo biloba extract or a component of the Ginkgo biloba extract.
A preferred method of the foregoing method is where the quantifying step comprises:
isolating poly A+ RNA from the treated batch of cells to obtain treated poly A+
RNA;
isolating poly A+ RNA from a batch of untreated cells to obtain untreated poly A+ RNA;
generating labeled cDNA probes from the treated poly A+ RNA to obtain treated labeled cDNA probes;
generating labeled cDNA probes from the untreated poly A+ RNA to obtain untreated labeled cDNA probes;
hybridizing the treated cDNA probes to an array having one or more cDNA to obtain a treated hybridized array of cDNA;
hybridizing the untreated cDNA probes to an array having one or more cDNA to obtain an untreated hybridized array of cDNA;
quantifying each of the cDNA of the treated hybridized array of cDNA to obtain quantities of treated cDNA;
quantifying each of the cDNA of the untreated hybridized array of cDNA to obtain quantities of untreated cDNA; and comparing the quantities of each of the treated cDNA with the quantities of untreated cDNA to obtain the gene regulation profile.
obtaining at least one batch of untreated cells;
treating a first batch of cells with an extract of Ginkgo biloba or a component of the Ginkgo biloba extract to obtain a treated batch of cells;
quantifying an affect on the expression of one or more genes of the treated cells to obtain a quantity of affected genes; and comparing the quantity of affected genes with a quantity of genes of cells not treated with Ginkgo biloba or a component of the Ginkgo biloba extract to obtain the gene regulation profile of the Ginkgo biloba extract or a component of the Ginkgo biloba extract.
A preferred method of the foregoing method is where the quantifying step comprises:
isolating poly A+ RNA from the treated batch of cells to obtain treated poly A+
RNA;
isolating poly A+ RNA from a batch of untreated cells to obtain untreated poly A+ RNA;
generating labeled cDNA probes from the treated poly A+ RNA to obtain treated labeled cDNA probes;
generating labeled cDNA probes from the untreated poly A+ RNA to obtain untreated labeled cDNA probes;
hybridizing the treated cDNA probes to an array having one or more cDNA to obtain a treated hybridized array of cDNA;
hybridizing the untreated cDNA probes to an array having one or more cDNA to obtain an untreated hybridized array of cDNA;
quantifying each of the cDNA of the treated hybridized array of cDNA to obtain quantities of treated cDNA;
quantifying each of the cDNA of the untreated hybridized array of cDNA to obtain quantities of untreated cDNA; and comparing the quantities of each of the treated cDNA with the quantities of untreated cDNA to obtain the gene regulation profile.
A preferred method of the immediately foregoing method is where the cells are MDA-231 cells; the Ginkgo biloba extract is EGB 761~; and the array is a gene chip having multiple genes.
A preferred method of the immediately foregoing method is where the gene regulation profile of EGB 761~ comprises increased expression of c-Myc protooncogene, and decreased expression of the following genes: prothymosin-a, CDK2, p55CDC, myeloblastin p120 proliferating-cell nuclear antigen, NET1, ERK2, Adenosine A2A Receptor, FIt3 ligand, Grb2, Clusterin, RXR-j3, Glutathione S-transferase P, N-Myc, TRADD, SGP-2, NIP-1, Id-2, ATF-4, ETR101, ETR-103, macrophage colony-stimulating factor-1, heparin-binding EGF-like growth factor, hepatocyte growth factor-like protein, inhibin a, CD19 B-lymphocyte antigen, L1CAM, (3-catenin, integrin subunit a3, integrin subunit a4, integrin subunit a6, integrin subunit [35, integrin subunit aM, APC, PE-1, RhoA, c-Jun, prothymosin-a, CDK2, p55CDC and myeloblastin.
A preferred method of the immediately foregoing method is where the gene regulation profile of EGB 761~ is about c-Myc = +75%, c-Jun = -78%, RhoA = -93%, APC = -59%, PE-1 = -42%, Prothymosin-a = -79%, Myeloblastin = -66%, p55CDC = -63%, p120 Proliferating-cell Nuclear Antigen = -68%, CDK2 = -83%, NET1 = -55%, ERK2 = -46%, Adenosine A2A Receptor = -40%, Flt3 ligand = -58%, Grb2 = -70%, Clusterin = -54%, RXR-(3 = -55%, Glutathione S-transferase P = -39%, N-Myc = -74%, TRADD = -51 %, NIP-1 = -40%, Id-2 = -65%, ATF4 = -42%, ETR103 = -65%, ETR101 = -60%, CD19 B-lymphocyte Antigen = -62%, L1CAM=-72%, /3-catenin = -58%, Integrin Subunit aM = -41 %, Integrin Subunit /35 = -55%, Integrin Subunit a4 = -49%, Integrin Subunit a3 = -77%, Integrin Subunit a6 = -53%, Macrophage Colony-stimulating Factor-1 (CSF-1) _ -31%, Heparin-binding EGF-like Growth Factor (HB-EGF) _ -62%, Hepatocyte Growth Factor-like Protein (HGFLP) _ -81 %, and Inhibin a = -69%, wherein the percentages shown can be ~20%, A preferred method of any of the foregoing methods is where the cells are MDA-231 cells; the component of the Ginkgo biloba extract is Ginkgolide B; and the array is a gene chip having multiple genes.
In another aspect, the present invention provides a method of verifying the identity of a Ginkgo biloba extract which comprises the steps of:
obtaining a gene regulation profile of the Gingko biloba extract to obtain a gene regulation profile;
obtaining a gene regulation profile of EGB 761 ~ to yield an EGB 761 ~ gene regulation profile;
comparing the gene regulation profile of the Gingko biloba extract with the EGB
761 ~ gene regulation profile;
A preferred method of the immediately foregoing method is where the gene regulation profile of EGB 761~ comprises increased expression of c-Myc protooncogene, and decreased expression of the following genes: prothymosin-a, CDK2, p55CDC, myeloblastin p120 proliferating-cell nuclear antigen, NET1, ERK2, Adenosine A2A Receptor, FIt3 ligand, Grb2, Clusterin, RXR-j3, Glutathione S-transferase P, N-Myc, TRADD, SGP-2, NIP-1, Id-2, ATF-4, ETR101, ETR-103, macrophage colony-stimulating factor-1, heparin-binding EGF-like growth factor, hepatocyte growth factor-like protein, inhibin a, CD19 B-lymphocyte antigen, L1CAM, (3-catenin, integrin subunit a3, integrin subunit a4, integrin subunit a6, integrin subunit [35, integrin subunit aM, APC, PE-1, RhoA, c-Jun, prothymosin-a, CDK2, p55CDC and myeloblastin.
A preferred method of the immediately foregoing method is where the gene regulation profile of EGB 761~ is about c-Myc = +75%, c-Jun = -78%, RhoA = -93%, APC = -59%, PE-1 = -42%, Prothymosin-a = -79%, Myeloblastin = -66%, p55CDC = -63%, p120 Proliferating-cell Nuclear Antigen = -68%, CDK2 = -83%, NET1 = -55%, ERK2 = -46%, Adenosine A2A Receptor = -40%, Flt3 ligand = -58%, Grb2 = -70%, Clusterin = -54%, RXR-(3 = -55%, Glutathione S-transferase P = -39%, N-Myc = -74%, TRADD = -51 %, NIP-1 = -40%, Id-2 = -65%, ATF4 = -42%, ETR103 = -65%, ETR101 = -60%, CD19 B-lymphocyte Antigen = -62%, L1CAM=-72%, /3-catenin = -58%, Integrin Subunit aM = -41 %, Integrin Subunit /35 = -55%, Integrin Subunit a4 = -49%, Integrin Subunit a3 = -77%, Integrin Subunit a6 = -53%, Macrophage Colony-stimulating Factor-1 (CSF-1) _ -31%, Heparin-binding EGF-like Growth Factor (HB-EGF) _ -62%, Hepatocyte Growth Factor-like Protein (HGFLP) _ -81 %, and Inhibin a = -69%, wherein the percentages shown can be ~20%, A preferred method of any of the foregoing methods is where the cells are MDA-231 cells; the component of the Ginkgo biloba extract is Ginkgolide B; and the array is a gene chip having multiple genes.
In another aspect, the present invention provides a method of verifying the identity of a Ginkgo biloba extract which comprises the steps of:
obtaining a gene regulation profile of the Gingko biloba extract to obtain a gene regulation profile;
obtaining a gene regulation profile of EGB 761 ~ to yield an EGB 761 ~ gene regulation profile;
comparing the gene regulation profile of the Gingko biloba extract with the EGB
761 ~ gene regulation profile;
determining whether the values of the gene regulation profile of the Ginkgo biloba extract is within ~10% of the values of the EGB 761~ gene regulation profile to obtain verification of the identity of the Ginkgo biloba extract.
A preferred method of the immediately foregoing method is where the method of obtaining a gene regulation profile of the Ginkgo biloba extract and the gene regulation profile comprises the steps of:
isolating poly A+ RNA from the treated batch of cells to obtain treated poly A+
RNA;
isolating poly A+ RNA from a batch of untreated cells to obtain untreated poly A+ RNA;
generating labeled cDNA probes from the treated poly A+ RNA to obtain treated labeled cDNA probes;
generating labeled cDNA probes from the untreated poly A+ RNA to obtain untreated labeled cDNA probes;
hybridizing the treated cDNA probes to an array having one or more cDNA to obtain a treated hybridized array of cDNA;
hybridizing the untreated cDNA probes to an array having one or more cDNA to obtain an untreated hybridized array of cDNA;
quantifying each of the cDNA of the treated hybridized array of cDNA to obtain quantities of treated cDNA;
quantifying each of the cDNA of the untreated hybridized array of cDNA to obtain quantities of untreated cDNA; and comparing the quantities of each of the treated cDNA with the quantities of untreated cDNA to obtain the gene regulation profile.
Brief Description of the Drawings Figure 1. Transcriptional response to EGB 761~ suggests an effect on genes involved in cell proliferation. Results shown represent quantitative analysis of the Atlas human cDNA expression array containing 588 PCR-amplified cDNA fragments (Clontech Inc.).
mRNAs were obtained from control or EGB 761 ~ (20 ,ug/ml) treated, for 48 h, cells. For normalizing the mRNA abundance, the densitometric values obtained from image analysis were normalized using the housekeeping genes provided in the array.
Only consistent significant changes above 30% were considered.
A preferred method of the immediately foregoing method is where the method of obtaining a gene regulation profile of the Ginkgo biloba extract and the gene regulation profile comprises the steps of:
isolating poly A+ RNA from the treated batch of cells to obtain treated poly A+
RNA;
isolating poly A+ RNA from a batch of untreated cells to obtain untreated poly A+ RNA;
generating labeled cDNA probes from the treated poly A+ RNA to obtain treated labeled cDNA probes;
generating labeled cDNA probes from the untreated poly A+ RNA to obtain untreated labeled cDNA probes;
hybridizing the treated cDNA probes to an array having one or more cDNA to obtain a treated hybridized array of cDNA;
hybridizing the untreated cDNA probes to an array having one or more cDNA to obtain an untreated hybridized array of cDNA;
quantifying each of the cDNA of the treated hybridized array of cDNA to obtain quantities of treated cDNA;
quantifying each of the cDNA of the untreated hybridized array of cDNA to obtain quantities of untreated cDNA; and comparing the quantities of each of the treated cDNA with the quantities of untreated cDNA to obtain the gene regulation profile.
Brief Description of the Drawings Figure 1. Transcriptional response to EGB 761~ suggests an effect on genes involved in cell proliferation. Results shown represent quantitative analysis of the Atlas human cDNA expression array containing 588 PCR-amplified cDNA fragments (Clontech Inc.).
mRNAs were obtained from control or EGB 761 ~ (20 ,ug/ml) treated, for 48 h, cells. For normalizing the mRNA abundance, the densitometric values obtained from image analysis were normalized using the housekeeping genes provided in the array.
Only consistent significant changes above 30% were considered.
Detailed Descriation The term "ginkgo terpenoid" includes all of the naturally occurring terpenes which are derived from the gymnosperms tree Ginkgo biloba as well as synthetically produced ginkgo terpenoids and pharmaceutically active derivatives and salts thereof and mixtures thereof. Examples of ginkgo terpenoids include ginkgolides.
Examples of ginkgo terpenoids are disclosed in Ginkgolides, Chemistry, Biology, Pharmacology, and Clinical Perspectives, J.R. Provs. Science Publishers, Edited by P. Braguet (1988); F.V.
DeFeudis, Ginkgo Biloba Extract (EGB 761~); Pharmacological Activities and Clinical Applications, Elsevier, Chapter II (1991).
The term "ginkgolide" as used herein include the various ginkgolides disclosed in the books cited above as well as non-toxic pharmaceutically active derivatives thereof. Examples of ginkgolide derivatives include tetrahydro derivatives, acetyl derivatives, and alkyl esters such as the monoacetate derivatives and triacetate derivatives disclosed in Okabe, et al., J. Chem. Soc. (c), pp. 2201-2206 (1967).
Ginkgolide B has the following structure and as used herein, refers to isolated ginkgolide B:
HO
'"' H H
\,0H ',~~~C(CH3)3 H
H3C v,~ _ , H HO ~ ~'H H
O
The term "Ginkgo biloba extract" as used herein includes a collection of natural molecules, including terpenoids, derived from the leaves of the Ginkgo biloba tree.
Preferably, the extract is the specific formulation of Ginkgo biloba extract known as EGB 761~.
A gene expression profile of an extract of Ginkgo bifoba or a component thereof can be obtained by methods known in the art. Traditionally such a profile was obtained by RNA Northern blot analysis or ribonuclease protection assay for each individual gene product. However, these assays were time consuming and took about 2-3 days to analyze each gene. Currently a gene expression profile can be established through the utilization of nucleic acid array technology such as the Atlas human cDNA
expression array I from Clontech (Palo Alto, CA); GeneFilters Microarrays by Research Genetics (Huntsville, AL); and the Gene Expression Microarrays by Genome Systems, Inc.
(St.
Louis, MO). The Gene Filters Microarray are high density DNA arrays produced on 5 cm x 7 cm membranes. At present there are four membranes available for human genes and one for rat genes. Each membrane contains approximately 5,000 sequences. Some of these sequences are known genes, while most sequences represent ESTs of unknown function. Research Genetics will soon make available gene arrays on the Affymetrix Gene chip platform, where the genes are immobilized on a silicon chip. In the case of silicon chips, the hybridization results (with the mRNA of choice) are detected by fluorescence and analyzed by pattern recognition compared to either fluorescence or radioactivity that can be used for the detection of the hybridization results in the membrane arrays.
Genome System's method utilizes the GEM technology where a collection of complementary DNA (cDNA) molecules that contain the genetic information from the biological systems of interest are deposited and bonded on a glass surface in an array format. Next, large portions from one half of the DNA's double strand are removed, thus activating the individual elements of the array, preparing them to react with their uniquely matched DNA counterparts in the cells being tested. GEM technology can fit 10,000 unique genes on a single array. GEM technology also uses a color coded technique to examine the difference in expression between two mRNA samples.
An array of cDNA will contain numerous animal, such as rat or human, preferably human, PCR-amplified cDNA fragments immobilized on a positively charged nylon membrane or a glass slide or a silicon chip or any other surface to be developed where a DNA/matrix interaction is allowed. A cell type of interest is treated with and without a Ginkgo biloba extract or a component thereof for about 43 hours.
Poly A+
RNA is isolated from control and extract-treated cells. 32P-labeled, fluorescent, chemiluminescent or colorimetric cDNA probes, preferably fluorescent or colorimetric labeling when using glass or silicon chip arrays, are generated from each poly A+RNA
and hybridized to the array according to the manufacturer's recommendations.
Autoradiography is performed by exposing the blots to film at about -70°C for 4-96 hr.
Quantification of the hybridization is carried out using an imaging system, which can detect the fluorescence or chemiluminesence then capture the image and analyze the data, such as the SigmaGel software. Multiple exposures are used in order to detect -g_ genes expressed at low levels. The three internal controls, ubiquitin, G3PDH
and J3 actin are used to compare the relative expression levels of the detected gene products in the control and the extract-treated cells. Experimental variations are corrected using the ratios of gene expression versus the internal controls. The effect of the extract treatment on each gene product is expressed as % of control (untreated) cells.
An example of the foregoing type of gene expression profile is as follows. The Atlas human cDNA expression array I from Clontech (Palo AIto,CA) contains 588 human PCR-amplified cDNA fragments of 200-500 by long immobilized on a positively charged nylon membrane. MDA-231 cells were treated with and without 20 p,glml EGB
761 ~ for 48 hours. Poly A+ RNA was isolated from control and EGB 761 ~-treated cells. 32P-labeled cDNA probes were generated from each poly A+RNA and hybridized to the Atlas array according to the manufacturer's recommendations.
Autoradiography was performed by exposing the blots to X-GMAT AR film (Kodak, Rochester, NY) at -70°C for 4-96 hr. Quantification of the hybridization seen was carried out using the SigmaGel software (Jandel Scientific, San Rafael, CA). Multiple exposures were used in order to detect genes expressed at low levels. The three internal controls, ubiquitin, G3PDH and (3-actin were used to compare the relative expression levels of the detected gene products in the control and EGB 761 ~-treated cells.
Experimental variations were corrected using the ratios of gene expression versus the internal controls. The effect of the EGB 761~ treatment on each gene product is expressed as of control (untreated) cells. The results of this experiment, which is presented in Table I, show genes affected consistently, at a level above 30% of control, by the EGB
761~ treatment. In summary, Table I shows that the treatment increased the expression of the c-Myc protooncogene and decreased the expression of 35 gene products, including oncogenes (AP-1, PE-1, RhoA, n-Myc), cell cycle regulators (CDK2, p55CDC, PCNA p120), signal transduction modulators (NET1, ERK2), apoptosis related products (SGP-2, NIP1) receptors (A2A, RXR-beta, Grb2), transcription factors (Id-2, ATF-4, ETR101, ETR-103), growth factors (HB-EGF, HGF-like), and cell adhesion molecules (CD19, L1CAM, integrins a3, a4, a6, ~i5, Mac-1, ~i-catenin) which are directly involved in various pathways regulating cell proliferation.
Gene expression profiles can be established for Ginkgo biloba extracts of known origin and then can be compared with the gene expression profile of Ginkgo bifoba extracts of unknown origin or extracts that purport to be a certain commercial _g_ extract. The comparison of the profiles can thus be used as a screening means to authenticate the origin of an extract.
Table I: Effect of EGB 761~ on MDA-231 gene expression examined using the Atlas human cDNA expression array as described under Nucleic Acid Arrays.
Function Oncoaenes and Tumor Suppressers c-Myc +7596 -basic helix-loop-helix-leucine (37) zipper transcription factor -Myc/Max heterodimers induce cell-cycle progression, apoptosis, and malignant transformation c-Jun -7896 -part of the AP-1 transcription (38) factor that regulates genes involved in cell proliferation RhoA -93.b -GTP-binding protein that is an (39) important regulator of cell proliferation -RhoA inactivation inhibits HL60 (40) cell proliferation APC -59~ -APC mutations are associated with (41 both hereditary and sporadic ) colorectal cancers (42) -a negative post-translational regulator of p-catenin PE-1 -42,6 -transcription factor (43) Cell C,~cle Control Proteins Prothymosin-a -7996 -acidic nuclear protein that is (44) upregulated in proliferating thymocytes, lymphocytes from leukemia patients, and in malignant breast lesions Myeloblastin -66~ -a serine protease involved in leukemia(45) cell differentiation p55CDC -6396 -similar to mitosis regulators CDC4(46) and CDC20 -expression positively correlated with cell proliferation status p120 Proliferating-cell-6896 -nucleolar protein expressed in (47) proliferating cells Nuclear Antigen -a prognostic indicator for breast (48) cancer patients and prostate adenocarcinoma CDK2 -83% -cyclin-dependent tyrosine kinase (49) involved in progression through the cell cycle -cyclin ElCdk2 inactivates the retinoblastoma tumor suppresser to allow the cell to progress to S (50) phase -Vitamin D inhibition of LNCaP cell proliferation coincided with a reduction in Cdk2 activity Intracellular Transducers NET1 -5596 -RhoA-specific guanine exchange (51 factor ) -NIH3T3-transforming protein ERK2 -466 -member of the extracellular signal-related(52) protein kinase family -activated upon cell stimulation A~optosis-Related Proteins Adenosine A2A -40.6 -G protein-coupled receptor involved(53) Receptor in the cAMP signaling pathway FIt3 ligand -58~ -ligand for the FIt3 cytokine receptor(54) tyrosine kinase -induces proliferation of leukemic myeloid cells Grb2 -70~ -an adapter protein that links receptor(55) tyrosine kinases to the Ras/MAPK signaling pathway via its SH2 domain Clusterin -5496 -a glycoprotein associated with (56, cell adhesion and apoptosis 57) -increased expression is linked (58) to Alzheimer's disease RXR-[3 -5596 -retiniod-activated transcription (59) factor -inhibition of chondrocyte proliferation(60) by retinoic acid causes a reduction in RXR-p mRNA expression Glutathione -3996 -a multi-drug resistance gene that (61, S-transferase is overexpressed in various human 62) P tumors (63) -chemical inhibition of GST-P inhibits proliferation of Jurkat T cells N-Myc -7496 -c-myc family member (64) -associated with early-onset retinoblastoma TRADD -5196 -TNFR-associated death domain protein(65) -involved in TNFR-induced cell growth and differentiation NIP-1 -406 -originally described as a yeast (66) nuclear transport protein -part of the translation initiation(67) facfor 3 (eIF3) core complex DNA-BindinglTranscription Factors Id-2 -65~6 -a member of the Id helix-loop-helix(68) family of transcriptional inhibitors -involved in proliferation of human pancreatic cancer cells ATF4 -4296 -a member of the ATFICREB family (69) of transcription factors -regulates Ras-induced transformation of NIH3T3 cells ETR103 -65,6 -a macrophage-associated immediate (70) early gene ETR101 -6096 -a lymphocyte-associated immediate (71 early gene ) References Cell Surface Antioens and Adhesion Molecules CD19 B-lymphocyte-62,6 -B-lymphocyte integral membrane (72) protein Antigen -expression is down-regulated during retinoid-inhibition of lymphoblastoid B-cell proliferation L1 CAM -72~, -neural cell adhesion molecule (73) -increased L1 CAM expression is associated with high-grade migration of glioma cells p-catenin -58,6 -involved in cadherin-mediated cell-cell(74) interactions -interacts with the TCF/LEF transcription factors in the Wnt signaling pathway Integrin Subunits aM -41 ,b -mediates cellular adherence of (75) human neutrophils with LFA-1 p -cc subunit of the elastase receptor [35 -55.6 -[3 subunit of the vitronectin receptor(76) (VR) -involved in cessation of oligodendrocyte(77) proliferation -involved in murine retinal angiogenesis (78) a4 -49,6 -cross-linking a4 integrins inhibits(79) LB lymphoma cell proliferation -also involved in metastasis of melanoma (80) and lymphoma cells a3 -7796 -a functionally perturbing a3 integrin(81 antibody inhibits human epithelial ) cell proliferation a6 -53~ -overexpression of a6 integrin collaborates(82) with ErbB2 to induce a more malignant phenotype in NIH3T3 cells Extracellular signalin4lCommunication Proteins Macrophage Colony--31 ~ -regulates the proliferation, differentiation,(83) and survival of monocytes, stimulating macrophages and their precursors (84) Factor-1 (CSF-1) -initiates a mitogenic signal that is required throughout G1 phase -CSF-1 stably transfected ovarian granulosa cells exhibit enhanced cell proliferation Heparin-binding-6296 -overexpressed in numerous human (85) EGF-like glioma cell lines and in a majority Growth Factor of glioblastomas (HB-EGF) -sfimulates human glioma ce!! proliferation Hepatocyte Growth-8196 -a transmembrane protein tyrosine (86) kinase found to be overexpressed Factor-like in hepatoblastoma and In human primary (87) Protein liver carcinoma (HGFLP) -induces proliferation and migration of murine keratinocytes Inhibin a -69.6 -a member of the inhibin family (88) of heterodimeric growth factors -inhibin a is a marker of trophoblastic (89) neoplasia and is highly References:
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Examples of ginkgo terpenoids are disclosed in Ginkgolides, Chemistry, Biology, Pharmacology, and Clinical Perspectives, J.R. Provs. Science Publishers, Edited by P. Braguet (1988); F.V.
DeFeudis, Ginkgo Biloba Extract (EGB 761~); Pharmacological Activities and Clinical Applications, Elsevier, Chapter II (1991).
The term "ginkgolide" as used herein include the various ginkgolides disclosed in the books cited above as well as non-toxic pharmaceutically active derivatives thereof. Examples of ginkgolide derivatives include tetrahydro derivatives, acetyl derivatives, and alkyl esters such as the monoacetate derivatives and triacetate derivatives disclosed in Okabe, et al., J. Chem. Soc. (c), pp. 2201-2206 (1967).
Ginkgolide B has the following structure and as used herein, refers to isolated ginkgolide B:
HO
'"' H H
\,0H ',~~~C(CH3)3 H
H3C v,~ _ , H HO ~ ~'H H
O
The term "Ginkgo biloba extract" as used herein includes a collection of natural molecules, including terpenoids, derived from the leaves of the Ginkgo biloba tree.
Preferably, the extract is the specific formulation of Ginkgo biloba extract known as EGB 761~.
A gene expression profile of an extract of Ginkgo bifoba or a component thereof can be obtained by methods known in the art. Traditionally such a profile was obtained by RNA Northern blot analysis or ribonuclease protection assay for each individual gene product. However, these assays were time consuming and took about 2-3 days to analyze each gene. Currently a gene expression profile can be established through the utilization of nucleic acid array technology such as the Atlas human cDNA
expression array I from Clontech (Palo Alto, CA); GeneFilters Microarrays by Research Genetics (Huntsville, AL); and the Gene Expression Microarrays by Genome Systems, Inc.
(St.
Louis, MO). The Gene Filters Microarray are high density DNA arrays produced on 5 cm x 7 cm membranes. At present there are four membranes available for human genes and one for rat genes. Each membrane contains approximately 5,000 sequences. Some of these sequences are known genes, while most sequences represent ESTs of unknown function. Research Genetics will soon make available gene arrays on the Affymetrix Gene chip platform, where the genes are immobilized on a silicon chip. In the case of silicon chips, the hybridization results (with the mRNA of choice) are detected by fluorescence and analyzed by pattern recognition compared to either fluorescence or radioactivity that can be used for the detection of the hybridization results in the membrane arrays.
Genome System's method utilizes the GEM technology where a collection of complementary DNA (cDNA) molecules that contain the genetic information from the biological systems of interest are deposited and bonded on a glass surface in an array format. Next, large portions from one half of the DNA's double strand are removed, thus activating the individual elements of the array, preparing them to react with their uniquely matched DNA counterparts in the cells being tested. GEM technology can fit 10,000 unique genes on a single array. GEM technology also uses a color coded technique to examine the difference in expression between two mRNA samples.
An array of cDNA will contain numerous animal, such as rat or human, preferably human, PCR-amplified cDNA fragments immobilized on a positively charged nylon membrane or a glass slide or a silicon chip or any other surface to be developed where a DNA/matrix interaction is allowed. A cell type of interest is treated with and without a Ginkgo biloba extract or a component thereof for about 43 hours.
Poly A+
RNA is isolated from control and extract-treated cells. 32P-labeled, fluorescent, chemiluminescent or colorimetric cDNA probes, preferably fluorescent or colorimetric labeling when using glass or silicon chip arrays, are generated from each poly A+RNA
and hybridized to the array according to the manufacturer's recommendations.
Autoradiography is performed by exposing the blots to film at about -70°C for 4-96 hr.
Quantification of the hybridization is carried out using an imaging system, which can detect the fluorescence or chemiluminesence then capture the image and analyze the data, such as the SigmaGel software. Multiple exposures are used in order to detect -g_ genes expressed at low levels. The three internal controls, ubiquitin, G3PDH
and J3 actin are used to compare the relative expression levels of the detected gene products in the control and the extract-treated cells. Experimental variations are corrected using the ratios of gene expression versus the internal controls. The effect of the extract treatment on each gene product is expressed as % of control (untreated) cells.
An example of the foregoing type of gene expression profile is as follows. The Atlas human cDNA expression array I from Clontech (Palo AIto,CA) contains 588 human PCR-amplified cDNA fragments of 200-500 by long immobilized on a positively charged nylon membrane. MDA-231 cells were treated with and without 20 p,glml EGB
761 ~ for 48 hours. Poly A+ RNA was isolated from control and EGB 761 ~-treated cells. 32P-labeled cDNA probes were generated from each poly A+RNA and hybridized to the Atlas array according to the manufacturer's recommendations.
Autoradiography was performed by exposing the blots to X-GMAT AR film (Kodak, Rochester, NY) at -70°C for 4-96 hr. Quantification of the hybridization seen was carried out using the SigmaGel software (Jandel Scientific, San Rafael, CA). Multiple exposures were used in order to detect genes expressed at low levels. The three internal controls, ubiquitin, G3PDH and (3-actin were used to compare the relative expression levels of the detected gene products in the control and EGB 761 ~-treated cells.
Experimental variations were corrected using the ratios of gene expression versus the internal controls. The effect of the EGB 761~ treatment on each gene product is expressed as of control (untreated) cells. The results of this experiment, which is presented in Table I, show genes affected consistently, at a level above 30% of control, by the EGB
761~ treatment. In summary, Table I shows that the treatment increased the expression of the c-Myc protooncogene and decreased the expression of 35 gene products, including oncogenes (AP-1, PE-1, RhoA, n-Myc), cell cycle regulators (CDK2, p55CDC, PCNA p120), signal transduction modulators (NET1, ERK2), apoptosis related products (SGP-2, NIP1) receptors (A2A, RXR-beta, Grb2), transcription factors (Id-2, ATF-4, ETR101, ETR-103), growth factors (HB-EGF, HGF-like), and cell adhesion molecules (CD19, L1CAM, integrins a3, a4, a6, ~i5, Mac-1, ~i-catenin) which are directly involved in various pathways regulating cell proliferation.
Gene expression profiles can be established for Ginkgo biloba extracts of known origin and then can be compared with the gene expression profile of Ginkgo bifoba extracts of unknown origin or extracts that purport to be a certain commercial _g_ extract. The comparison of the profiles can thus be used as a screening means to authenticate the origin of an extract.
Table I: Effect of EGB 761~ on MDA-231 gene expression examined using the Atlas human cDNA expression array as described under Nucleic Acid Arrays.
Function Oncoaenes and Tumor Suppressers c-Myc +7596 -basic helix-loop-helix-leucine (37) zipper transcription factor -Myc/Max heterodimers induce cell-cycle progression, apoptosis, and malignant transformation c-Jun -7896 -part of the AP-1 transcription (38) factor that regulates genes involved in cell proliferation RhoA -93.b -GTP-binding protein that is an (39) important regulator of cell proliferation -RhoA inactivation inhibits HL60 (40) cell proliferation APC -59~ -APC mutations are associated with (41 both hereditary and sporadic ) colorectal cancers (42) -a negative post-translational regulator of p-catenin PE-1 -42,6 -transcription factor (43) Cell C,~cle Control Proteins Prothymosin-a -7996 -acidic nuclear protein that is (44) upregulated in proliferating thymocytes, lymphocytes from leukemia patients, and in malignant breast lesions Myeloblastin -66~ -a serine protease involved in leukemia(45) cell differentiation p55CDC -6396 -similar to mitosis regulators CDC4(46) and CDC20 -expression positively correlated with cell proliferation status p120 Proliferating-cell-6896 -nucleolar protein expressed in (47) proliferating cells Nuclear Antigen -a prognostic indicator for breast (48) cancer patients and prostate adenocarcinoma CDK2 -83% -cyclin-dependent tyrosine kinase (49) involved in progression through the cell cycle -cyclin ElCdk2 inactivates the retinoblastoma tumor suppresser to allow the cell to progress to S (50) phase -Vitamin D inhibition of LNCaP cell proliferation coincided with a reduction in Cdk2 activity Intracellular Transducers NET1 -5596 -RhoA-specific guanine exchange (51 factor ) -NIH3T3-transforming protein ERK2 -466 -member of the extracellular signal-related(52) protein kinase family -activated upon cell stimulation A~optosis-Related Proteins Adenosine A2A -40.6 -G protein-coupled receptor involved(53) Receptor in the cAMP signaling pathway FIt3 ligand -58~ -ligand for the FIt3 cytokine receptor(54) tyrosine kinase -induces proliferation of leukemic myeloid cells Grb2 -70~ -an adapter protein that links receptor(55) tyrosine kinases to the Ras/MAPK signaling pathway via its SH2 domain Clusterin -5496 -a glycoprotein associated with (56, cell adhesion and apoptosis 57) -increased expression is linked (58) to Alzheimer's disease RXR-[3 -5596 -retiniod-activated transcription (59) factor -inhibition of chondrocyte proliferation(60) by retinoic acid causes a reduction in RXR-p mRNA expression Glutathione -3996 -a multi-drug resistance gene that (61, S-transferase is overexpressed in various human 62) P tumors (63) -chemical inhibition of GST-P inhibits proliferation of Jurkat T cells N-Myc -7496 -c-myc family member (64) -associated with early-onset retinoblastoma TRADD -5196 -TNFR-associated death domain protein(65) -involved in TNFR-induced cell growth and differentiation NIP-1 -406 -originally described as a yeast (66) nuclear transport protein -part of the translation initiation(67) facfor 3 (eIF3) core complex DNA-BindinglTranscription Factors Id-2 -65~6 -a member of the Id helix-loop-helix(68) family of transcriptional inhibitors -involved in proliferation of human pancreatic cancer cells ATF4 -4296 -a member of the ATFICREB family (69) of transcription factors -regulates Ras-induced transformation of NIH3T3 cells ETR103 -65,6 -a macrophage-associated immediate (70) early gene ETR101 -6096 -a lymphocyte-associated immediate (71 early gene ) References Cell Surface Antioens and Adhesion Molecules CD19 B-lymphocyte-62,6 -B-lymphocyte integral membrane (72) protein Antigen -expression is down-regulated during retinoid-inhibition of lymphoblastoid B-cell proliferation L1 CAM -72~, -neural cell adhesion molecule (73) -increased L1 CAM expression is associated with high-grade migration of glioma cells p-catenin -58,6 -involved in cadherin-mediated cell-cell(74) interactions -interacts with the TCF/LEF transcription factors in the Wnt signaling pathway Integrin Subunits aM -41 ,b -mediates cellular adherence of (75) human neutrophils with LFA-1 p -cc subunit of the elastase receptor [35 -55.6 -[3 subunit of the vitronectin receptor(76) (VR) -involved in cessation of oligodendrocyte(77) proliferation -involved in murine retinal angiogenesis (78) a4 -49,6 -cross-linking a4 integrins inhibits(79) LB lymphoma cell proliferation -also involved in metastasis of melanoma (80) and lymphoma cells a3 -7796 -a functionally perturbing a3 integrin(81 antibody inhibits human epithelial ) cell proliferation a6 -53~ -overexpression of a6 integrin collaborates(82) with ErbB2 to induce a more malignant phenotype in NIH3T3 cells Extracellular signalin4lCommunication Proteins Macrophage Colony--31 ~ -regulates the proliferation, differentiation,(83) and survival of monocytes, stimulating macrophages and their precursors (84) Factor-1 (CSF-1) -initiates a mitogenic signal that is required throughout G1 phase -CSF-1 stably transfected ovarian granulosa cells exhibit enhanced cell proliferation Heparin-binding-6296 -overexpressed in numerous human (85) EGF-like glioma cell lines and in a majority Growth Factor of glioblastomas (HB-EGF) -sfimulates human glioma ce!! proliferation Hepatocyte Growth-8196 -a transmembrane protein tyrosine (86) kinase found to be overexpressed Factor-like in hepatoblastoma and In human primary (87) Protein liver carcinoma (HGFLP) -induces proliferation and migration of murine keratinocytes Inhibin a -69.6 -a member of the inhibin family (88) of heterodimeric growth factors -inhibin a is a marker of trophoblastic (89) neoplasia and is highly References:
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Claims (7)
1. A method of establishing a gene regulation profile of a Gingko biloba extract or a component of the Ginkgo biloba extract, which comprises the steps of:
obtaining at least one batch of untreated cells;
treating a first batch of cells with an extract of Ginkgo biloba or a component of the Ginkgo biloba extract to obtain a treated batch of cells;
quantifying an affect on the expression of one or more genes of the treated cells to obtain a quantity of affected genes; and comparing the quantity of affected genes with a quantity of genes of cells not treated with Ginkgo biloba or a component of the Ginkgo biloba extract to obtain the gene regulation profile of the Ginkgo biloba extract or a component of the Ginkgo biloba extract.
obtaining at least one batch of untreated cells;
treating a first batch of cells with an extract of Ginkgo biloba or a component of the Ginkgo biloba extract to obtain a treated batch of cells;
quantifying an affect on the expression of one or more genes of the treated cells to obtain a quantity of affected genes; and comparing the quantity of affected genes with a quantity of genes of cells not treated with Ginkgo biloba or a component of the Ginkgo biloba extract to obtain the gene regulation profile of the Ginkgo biloba extract or a component of the Ginkgo biloba extract.
2. A method according to claim 1 wherein the quantifying comprises:
isolating poly A+ RNA from the treated batch of cells to obtain treated poly A+
RNA;
isolating poly A+ RNA from a batch of untreated cells to obtain untreated poly A+ RNA;
generating labeled cDNA probes from the treated poly A+ RNA to obtain treated labeled cDNA probes;
generating labeled cDNA probes from the untreated poly A+ RNA to obtain untreated labeled cDNA probes;
hybridizing the treated cDNA probes to an array having one or more cDNA to obtain a treated hybridized array of cDNA;
hybridizing the untreated cDNA probes to an array having one or more cDNA to obtain an untreated hybridized array of cDNA;
quantifying each of the cDNA of the treated hybridized array of cDNA to obtain quantities of treated cDNA;
quantifying each of the cDNA of the untreated hybridized array of cDNA to obtain quantities of untreated cDNA; and comparing the quantities of each of the treated cDNA with the quantities of untreated cDNA to obtain the gene regulation profile.
isolating poly A+ RNA from the treated batch of cells to obtain treated poly A+
RNA;
isolating poly A+ RNA from a batch of untreated cells to obtain untreated poly A+ RNA;
generating labeled cDNA probes from the treated poly A+ RNA to obtain treated labeled cDNA probes;
generating labeled cDNA probes from the untreated poly A+ RNA to obtain untreated labeled cDNA probes;
hybridizing the treated cDNA probes to an array having one or more cDNA to obtain a treated hybridized array of cDNA;
hybridizing the untreated cDNA probes to an array having one or more cDNA to obtain an untreated hybridized array of cDNA;
quantifying each of the cDNA of the treated hybridized array of cDNA to obtain quantities of treated cDNA;
quantifying each of the cDNA of the untreated hybridized array of cDNA to obtain quantities of untreated cDNA; and comparing the quantities of each of the treated cDNA with the quantities of untreated cDNA to obtain the gene regulation profile.
3. A method according to claim 2, wherein the cells are MDA-231 cells; the Ginkgo biloba extract is EGB 761®; and the array is a gene chip having multiple genes.
4. A method according to claim 3 wherein the gene regulation profile of EGB 761® comprises increased expression of c-Myc protooncogene, and decreased expression of the following genes: prothymosin-a, CDK2, p55CDC, myeloblastin p120 proliferating-cell nuclear antigen, NET1, ERK2, Adenosine A2A Receptor, FIt3 ligand, Grb2, Clusterin, RXR-.beta., Glutathione S-transferase P, N-Myc, TRADD, SGP-2, NIP-1, Id-2, ATF-4, ETR101, ETR-103, macrophage colony-stimulating factor-1, heparin-binding EGF-like growth factor, hepatocyte growth factor-Pike protein, inhibin a, CD19 B-lymphocyte antigen, L1CAM, .beta.-catenin, integrin subunit a3, integrin subunit a4, integrin subunit a6, integrin subunit .beta.5, integrin subunit aM, APC, PE-1, RhoA, c-Jun, prothymosin-a, CDK2, p55CDC and myeloblastin.
5. A method according to claim 4 wherein the gene regulation profile of EGB 761® is about:
c-Myc = +75%, c-Jun = -78%, RhoA = -93%, APC = -59%, PE-1 = -42%, Prothymosin-a = -79%, Myeloblastin = -66%, p55CDC = -63%, p120 Proliferating-cell Nuclear Antigen = -68%, CDK2 = -83%, NET1 = -55%, ERK2 = -46%, Adenosine A2A Receptor = -40%, FIt3 ligand = -58%, Grb2 = -70%, Clusterin = -54%, RXR-.beta. = -55%, Glutathione S-transferase P = -39%, N-Myc = -74%, TRADD = -51 %, NIP-9 = -40%, Id-2 = -65%, ATF4 = -42%, ETR103 = -65%, ETR101 = -60%, CD19 B-lymphocyte Antigen = -62%, L1 CAM = -72%, .beta.-catenin = -58%, Integrin Subunit .alpha.M = -41 %, Integrin Subunit .beta.5 = -55%, Integrin Subunit .alpha.4 = -49%, Integrin Subunit .alpha.3 = -77%, Integrin Subunit .alpha.6 = -53%, Macrophage Colony-stimulating Factor-1 (CSF-1) = -31%, Heparin-binding EGF-like Growth Factor (HB-EGF) = -62%, Hepatocyte Growth Factor-like Protein (HGFLP) = -81 %, and Inhibin a = -69%, wherein the percentages shown can be ~20%.
5. A method according to claim 4 wherein the gene regulation profile of EGB 761® is about:
c-Myc = +75%, c-Jun = -78%, RhoA = -93%, APC = -59%, PE-1 = -42%, Prothymosin-a = -79%, Myeloblastin = -66%, p55CDC = -63%, p120 Proliferating-cell Nuclear Antigen = -68%, CDK2 = -83%, NET1 = -55%, ERK2 = -46%, Adenosine A2A Receptor = -40%, FIt3 ligand = -58%, Grb2 = -70%, Clusterin = -54%, RXR-.beta. = -55%, Glutathione S-transferase P = -39%, N-Myc = -74%, TRADD = -51 %, NIP-9 = -40%, Id-2 = -65%, ATF4 = -42%, ETR103 = -65%, ETR101 = -60%, CD19 B-lymphocyte Antigen = -62%, L1 CAM = -72%, .beta.-catenin = -58%, Integrin Subunit .alpha.M = -41 %, Integrin Subunit .beta.5 = -55%, Integrin Subunit .alpha.4 = -49%, Integrin Subunit .alpha.3 = -77%, Integrin Subunit .alpha.6 = -53%, Macrophage Colony-stimulating Factor-1 (CSF-1) = -31%, Heparin-binding EGF-like Growth Factor (HB-EGF) = -62%, Hepatocyte Growth Factor-like Protein (HGFLP) = -81 %, and Inhibin a = -69%, wherein the percentages shown can be ~20%.
5. A method according to claim 2, wherein the cells are MDA-231 cells; the component of the Ginkgo biloba extract is Ginkgolide B; and the array is a gene chip having multiple genes.
6. A method of verifying the identity of a Ginkgo biloba extract which comprises the steps of:
obtaining a gene regulation profile of the Gingko biloba extract to obtain a gene regulation profile;
obtaining a gene regulation profile of EGB 761® to yield an EGB 761®
gene regulation profile;
comparing the gene regulation profile of the Gingko biloba extract with the EGB
761® gene regulation profile;
determining whether the values of the gene regulation profile of the Ginkgo biloba extract is within ~10% of the values of the EGB 761® gene regulation profile to obtain verification of the identity of the Ginkgo biloba extract.
obtaining a gene regulation profile of the Gingko biloba extract to obtain a gene regulation profile;
obtaining a gene regulation profile of EGB 761® to yield an EGB 761®
gene regulation profile;
comparing the gene regulation profile of the Gingko biloba extract with the EGB
761® gene regulation profile;
determining whether the values of the gene regulation profile of the Ginkgo biloba extract is within ~10% of the values of the EGB 761® gene regulation profile to obtain verification of the identity of the Ginkgo biloba extract.
7. A method according to claim 6, wherein the method of obtaining a gene regulation profile of the Ginkgo biloba extract and the EGB 761® gene regulation profile comprises the steps of:
isolating poly A+ RNA from the treated batch of cells to obtain treated poly A+
RNA;
isolating poly A+ RNA from a batch of untreated cells to obtain untreated poly A+ RNA;
generating labeled cDNA probes from the treated poly A+ RNA to obtain treated labeled cDNA probes;
generating labeled cDNA probes from the untreated poly A+ RNA to obtain untreated labeled cDNA probes;
hybridizing the treated cDNA probes to an array having one or more cDNA to obtain a treated hybridized array of cDNA;
hybridizing the untreated cDNA probes to an array having one or more cDNA to obtain an untreated hybridized array of cDNA;
quantifying each of the cDNA of the treated hybridized array of cDNA to obtain quantities of treated cDNA;
quantifying each of the cDNA of the untreated hybridized array of cDNA to obtain quantities of untreated cDNA; and comparing the quantities of each of the treated cDNA with the quantities of untreated cDNA to obtain the gene regulation profile.
isolating poly A+ RNA from the treated batch of cells to obtain treated poly A+
RNA;
isolating poly A+ RNA from a batch of untreated cells to obtain untreated poly A+ RNA;
generating labeled cDNA probes from the treated poly A+ RNA to obtain treated labeled cDNA probes;
generating labeled cDNA probes from the untreated poly A+ RNA to obtain untreated labeled cDNA probes;
hybridizing the treated cDNA probes to an array having one or more cDNA to obtain a treated hybridized array of cDNA;
hybridizing the untreated cDNA probes to an array having one or more cDNA to obtain an untreated hybridized array of cDNA;
quantifying each of the cDNA of the treated hybridized array of cDNA to obtain quantities of treated cDNA;
quantifying each of the cDNA of the untreated hybridized array of cDNA to obtain quantities of untreated cDNA; and comparing the quantities of each of the treated cDNA with the quantities of untreated cDNA to obtain the gene regulation profile.
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| US60/193,889 | 2000-03-31 | ||
| PCT/US2001/009832 WO2001075181A2 (en) | 2000-03-31 | 2001-03-27 | Method of identifying ginko biloba in a plant extract by gene profiling |
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| JP (1) | JP2003529377A (en) |
| KR (1) | KR100479151B1 (en) |
| CN (1) | CN1185354C (en) |
| AU (2) | AU2001247832B2 (en) |
| CA (1) | CA2403303A1 (en) |
| CZ (1) | CZ20023275A3 (en) |
| HK (1) | HK1053150A1 (en) |
| HU (1) | HUP0301997A3 (en) |
| IL (1) | IL151856A0 (en) |
| MX (1) | MXPA02009412A (en) |
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| PL (1) | PL365418A1 (en) |
| RU (1) | RU2271393C2 (en) |
| WO (1) | WO2001075181A2 (en) |
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| Publication number | Priority date | Publication date | Assignee | Title |
|---|---|---|---|---|
| WO2011079261A2 (en) * | 2009-12-23 | 2011-06-30 | Curna, Inc. | Treatment of hepatocyte growth factor (hgf) related diseases by inhibition of natural antisense transcript to hgf |
| CN109694903A (en) * | 2019-01-09 | 2019-04-30 | 中国药科大学 | The method for synthesizing key gene with gene expression association analysis screening ginkgolides based on ginkgolides content |
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| AU2341999A (en) * | 1998-01-26 | 1999-08-09 | Schering Aktiengesellschaft | Gene expression methods for screening compounds |
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2001
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- 2001-03-27 NZ NZ521728A patent/NZ521728A/en unknown
- 2001-03-27 HU HU0301997A patent/HUP0301997A3/en unknown
- 2001-03-27 KR KR10-2002-7012597A patent/KR100479151B1/en not_active IP Right Cessation
- 2001-03-27 CA CA002403303A patent/CA2403303A1/en not_active Abandoned
- 2001-03-27 PL PL01365418A patent/PL365418A1/en not_active Application Discontinuation
- 2001-03-27 CZ CZ20023275A patent/CZ20023275A3/en unknown
- 2001-03-27 AU AU2001247832A patent/AU2001247832B2/en not_active Ceased
- 2001-03-27 CN CNB018074847A patent/CN1185354C/en not_active Expired - Fee Related
- 2001-03-27 EP EP01920817A patent/EP1292706A2/en not_active Withdrawn
- 2001-03-27 JP JP2001573053A patent/JP2003529377A/en active Pending
- 2001-03-27 AU AU4783201A patent/AU4783201A/en active Pending
- 2001-03-27 IL IL15185601A patent/IL151856A0/en unknown
- 2001-03-27 WO PCT/US2001/009832 patent/WO2001075181A2/en not_active Application Discontinuation
- 2001-03-27 RU RU2002129104/13A patent/RU2271393C2/en not_active IP Right Cessation
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2002
- 2002-09-26 NO NO20024611A patent/NO20024611L/en not_active Application Discontinuation
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2003
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Also Published As
| Publication number | Publication date |
|---|---|
| WO2001075181A3 (en) | 2002-11-07 |
| IL151856A0 (en) | 2003-04-10 |
| PL365418A1 (en) | 2005-01-10 |
| AU4783201A (en) | 2001-10-15 |
| AU2001247832B2 (en) | 2005-07-21 |
| NO20024611L (en) | 2002-11-19 |
| CZ20023275A3 (en) | 2003-03-12 |
| WO2001075181A2 (en) | 2001-10-11 |
| JP2003529377A (en) | 2003-10-07 |
| CN1185354C (en) | 2005-01-19 |
| NO20024611D0 (en) | 2002-09-26 |
| RU2271393C2 (en) | 2006-03-10 |
| KR100479151B1 (en) | 2005-03-28 |
| KR20020089409A (en) | 2002-11-29 |
| CN1439059A (en) | 2003-08-27 |
| HUP0301997A3 (en) | 2005-11-28 |
| HUP0301997A2 (en) | 2003-09-29 |
| NZ521728A (en) | 2004-10-29 |
| HK1053150A1 (en) | 2003-10-10 |
| MXPA02009412A (en) | 2005-02-03 |
| EP1292706A2 (en) | 2003-03-19 |
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