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Compositions and Methods of Use for Variant Csy4 Endoribonucleases

技术优势
Detects as few as a single copy of a target polyribonucleotide
技术应用
Detect a target nucleotide (e.g., of a pathogen in a biological sample) Purify a particular target RNA (or RNA protein complex) from within a complex mixture  Delivery of modular components (e.g., effector domains) in conjunction with Cas9 Modulate expression of RNA molecules in eukaryotic cells RNA processing enzyme
详细技术说明
None
*Abstract

DNA restriction enzymes transformed molecular biology in the 1970s by making it possible to cleave specific DNA sequences at will. Sequencing of RNA molecules currently entails copying the RNA into a DNA strand that is then sequenced by conventional methods. This approach, also known as RNASeq, is robust and can yield many millions of sequence reads. However, the necessity of generating cDNA introduces inherent bias due to sequence-dependent efficiencies of individual steps.

UC Berkeley researchers discovered variant Csy4 endoribonucleases, nucleic acids encoding the variant Csy4 endoribonucleases, and host cells genetically modified with the nucleic acids that can be used to detect the presence of a particular sequence in a polyribonucleotide, (e.g., to detect the presence of pathogen in a biological sample).  . The variant Csy4 endoribonucleases find use in a variety of applications, which are also provided. The present disclosure also provides methods of detecting a specific sequence in a target polyribonucleotide; and methods of regulating production of a target RNA in a eukaryotic cell. 

*IP Issue Date
Aug 25, 2015
*Principal Investigation

Name: Jennifer Doudna

Department:


Name: Rachel Haurwitz Smoligovets

Department:


Name: Blake Wiedenheft

Department:


Name: Martin Jinek

Department:

申请号码
9115348
其他

Related Materials

Sequence- and Structure-Specific RNA Processing by a CRISPR Endonuclease


Additional Technologies by these Inventors


Tech ID/UC Case

19837/2010-028-0


Related Cases

2010-028-0

国家/地区
美国

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