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No | Ctr | Title | PubDate | Int.Class | Appl.No | Applicant | Inventor | ||||
| 1. | US | 20090304705 - Biomarkers for chronic transplant dysfunction | 10.12.2009 |
| 12297258 | Novartis AG | Grass Peter | ||||
The invention relates to the analysis and identification of genes that are modulated in transplant rejection. This alteration of gene expression provides a molecular signature to accurately detect transplant rejection. | |||||||||||
| 2. | WO | WO/2007/121922 - BIOMARKERS FOR CHRONIC TRANSPLANT DYSFUNCTION | 01.11.2007 |
| PCT/EP2007/003437 | NOVARTIS AG | GRASS, Peter | ||||
The invention relates to the analysis and identification of genes that are modulated in transplant rejection. This alteration of gene expression provides a molecular signature to accurately detect transplant rejection.
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| 3. | WO | WO/2013/007563 - FUSION PROTEINS RELEASING RELAXIN AND USES THEREOF | 17.01.2013 |
| PCT/EP2012/062956 | BAYER INTELLECTUAL PROPERTY GMBH | HAUPTS, Ulrich | ||||
The present invention provides Relaxin fusion proteins, wherein a linker connects the carboxy-terminus of Relaxin with a proteinaceous half-life extending moiety and the linker comprises a protease cleavage site. Therefore, the invention provides Relaxin fusion polypeptides with extended half-life whereby the fusion protein by itself serves as a depot for release of the biologically active Relaxin. Furthermore, the invention provides nucleic acid sequences encoding the foregoing fusion polypeptides, vectors containing the same, cells expressing the Relaxin fusion polypeptides, pharmaceutical compositions and medical use of such fusion polypeptides.
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| 4. | US | 20110236953 - EMBRYONIC CEREBROSPINAL FLUID (e-CSF), PROTEINS FROM e-CSF, AND RELATED METHODS AND COMPOSITIONS | 29.09.2011 |
| 12672009 | Beth Israel Deaconness Medical Center | Walsh Christopher A. | ||||
We have performed a proteomic analysis of embryonic cerebrospinal fluid (e-CSF) in human and rats. Based on this discovery, the invention features methods and compositions for cell culture including components of e-CSF or fragments thereof. Also provided are methods for extraction of e-CSF. | |||||||||||
| 5. | EP | 1957644 - ENZYMATIC ENCODING METHODS FOR EFFICIENT SYNTHESIS OF LARGE LIBRARIES | 20.08.2008 |
| 06818144 | NUEVOLUTION AS | FRANCH THOMAS | ||||
Disclosed is a method for obtaining a bifunctional complex comprising a molecule linked to a single stranded identifier oligonucleotide, wherein a nascent bifunctional complex comprising a chemical reaction site and a priming site for enzymatic addition of a tag is a) reacted at the chemical reaction site with one or more reactants, and b) reacted enzymatically at the priming site with one or more tag(s) identifying the reactant(s).
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| 6. | US | 20040072160 - Molecular toxicology modeling | 15.04.2004 |
| 10152319 | Ocimum Biosolutions, Inc. | Mendrick Donna | ||||
The present invention is based on the elucidation of the global changes in gene expression and the identification of toxicity markers in tissues or cells exposed to a known renal toxin. The genes may be used as toxicity markers in drug screening and toxicity assays. The invention includes a database of genes characterized by toxin-induced differential expression that is designed for use with microarrays and other solid-phase probes. | |||||||||||
| 7. | US | 20060078900 - Methods for determining renal toxins | 13.04.2006 |
| 11036196 | Ocimum Biosolutions, Inc. | Mendrick Donna | ||||
The present invention is based on the elucidation of the global changes in gene expression and the identification of toxicity markers in tissues or cells exposed to a known renal toxin. The genes may be used as toxicity markers in drug screening and toxicity assays. The invention includes a database of genes characterized by toxin-induced differential expression that is designed for use with microarrays and other solid-phase probes. | |||||||||||
| 8. | US | 20070015147 - Primary rat hepatocyte toxicity modeling | 18.01.2007 |
| 10357507 | Ocimum Biosolutions, Inc. | Mendrick Donna L. | ||||
The present invention is based on the elucidation of the global changes in gene expression and the identification of toxicity markers in tissues or cells exposed to a known toxin. The genes may be used as toxicity markers in drug screening and toxicity assays. The invention includes a database of genes characterized by toxin-induced differential expression that is designed for use with microarrays and other solid-phase probes. | |||||||||||
| 9. | WO | WO/2007/059966 - DETECTION AND TREATMENT OF DRUG ASSOCIATED ANGIOEDEMA | 31.05.2007 |
| PCT/EP2006/011245 | DEWALD, Georg | DEWALD, Georg | ||||
The present invention relates to an in vitro method of diagnosing a drug-associated angioedema or a predisposition thereto in a subject being suspected of having developed or of having a predisposition to develop a drug-associated angioedema or in a subject being suspected of being a carrier for a drug-associated angioedema or in a subject being intended to be treated with a drug associated with the development of angioedema, the method comprising determining in a biological sample from said subject the presence or absence of a disease-associated mutation in a nucleic acid molecule regulating the expression of or encoding coagulation factor XII; wherein the presence of such a mutation is indicative of a drug- associated angioedema or a predisposition thereto. The present invention also relates to a method of diagnosing a drug-associated angioedema or a predisposition thereto in a subject being suspected of having developed or of having a predisposition to develop a drug-associated angioedema or in a subject being suspected of being a carrier for a drug-associated angioedema or in a subject being intended to be treated with a drug associated with the development of angioedema, the method comprising assessing the presence, amount and/or activity of coagulation factor XII in said subject and including the steps of: (a) determining from a biological sample of said subject in vitro, the presence, amount and/or activity of: (i) a (poly)peptide encoded by the coagulation factor XII gene; (ii) a substrate of the (poly)peptide of (i); or (iii) a (poly)peptide processed by the substrate mentioned in (ii); (b) comparing said presence, amount and/or activity with that determined from a reference sample; and (c) diagnosing, based on the difference between the samples compared in step (b), the pathological condition of a drug-associated angioedema or a predisposition thereto. The present invention also relates to a method of identifying a compound modulating coagulation factor XII activity which is suitable as a medicament or a lead compound for a medicament for the treatment and/or prevention of drug-associated angioedema, the method comprising the steps of: (a) in vitro contacting a coagulation factor XII (poly)peptide or a functionally related (poly)peptide with the potential modulator; and (b) testing for modulation of coagulation factor XII activity, wherein modulation of coagulation factor XII activity is indicative of a compound's suitability as a medicament or a lead compound for a medicament for the treatment and/or prevention of drug-associated angioedema. Furthermore, the present invention relates to gene therapy methods and to a kit for diagnosing drug-associated angioedema.
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| 10. | EP | 2336315 - Enzymatic encoding methods for efficient synthesis of large libraries | 22.06.2011 |
| 10192717 | NUEVOLUTION AS | FRANCH THOMAS | ||||
Disclosed is a method for obtaining a bifunctional complex comprising a molecule linked to a single stranded identifier oligonucleotide, wherein a nascent bifunctional complex comprising a chemical reaction site and a priming site for enzymatic addition of a tag is a) reacted at the chemical reaction site with one or more reactants, and b) reacted enzymatically at the priming site with one or more tag(s) identifying the reactant(s).
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