RNAi - Technologies, Markets and Companies
05-May-2011 | News-Press Release
RNA interference (RNAi) or gene silencing involves the use of double stranded  RNA (dsRNA). Once inside the cell, this material is processed into short 21-23  nucleotide RNAs termed siRNAs that are used in a sequence-specific manner to  recognize and destroy complementary RNA. The report compares RNAi with other  antisense approaches using oligonucleotides, aptamers, ribozymes, peptide  nucleic acid and locked nucleic acid.
 
 Various RNAi technologies are described, along with design and methods of  manufacture of siRNA reagents. These include chemical synthesis by in vitro  transcription and use of plasmid or viral vectors. Other approaches to RNAi  include DNA-directed RNAi (ddRNAi) that is used to produce dsRNA inside the  cell, which is cleaved into siRNA by the action of Dicer, a specific type of  RNAse III. MicroRNAs are derived by processing of short hairpins that can  inhibit the mRNAs. Expressed interfering RNA (eiRNA) is used to express dsRNA  intracellularly from DNA plasmids.
 
 Delivery of therapeutics to the target tissues is an important consideration.  siRNAs can be delivered to cells in culture by electroporation or by  transfection using plasmid or viral vectors. In vivo delivery of siRNAs can be  carried out by injection into tissues or blood vessels or use of synthetic and  viral vectors.
 
 Because of its ability to silence any gene once the sequence is known, RNAi has  been adopted as the research tool to discriminate gene function. After the  genome of an organism is sequenced, RNAi can be designed to target every gene in  the genome and target for specific phenotypes. Several methods of gene  expression analysis are available and there is still need for sensitive methods  of detection of gene expression as a baseline and measurement after gene  silencing. RNAi microarray has been devised and can be tailored to meet the  needs for high throughput screens for identifying appropriate RNAi probes. RNAi  is an important method for analyzing gene function and identifying new drug  targets that uses double-stranded RNA to knock down or silence specific genes.  With the advent of vector-mediated siRNA delivery methods it is now possible to  make transgenic animals that can silence gene expression stably. These  technologies point to the usefulness of RNAi for drug discovery.
 
 RNAi can be rationally designed to block the expression of any target gene,  including genes for which traditional small molecule inhibitors cannot be found.  Areas of therapeutic applications include virus infections, cancer, genetic  disorders and neurological diseases. Side effects can result from unintended  interaction between an siRNA compound and an unrelated host gene. If RNAi  compounds are designed poorly, there is an increased chance for non-specific  interaction with host genes that may cause adverse effects in the host.
 
 Regulatory, safety and patent issues are discussed. There are no major safety  concerns and regulations are in preliminary stages as the clinical trials are  just starting. Many of the patents are still pending.
 
 The markets for RNAi are difficult to define as no RNAi-based product is  approved yet but several are in clinical trials. The major use of RNAi reagents  is in research but it partially overlaps that of drug discovery and therapeutic  development. Various markets relevant to RNAi are analyzed from 2010 to 2020.  Markets are also analyzed according to breakdown of technologies and use of  siRNAs, miRNAs, etc.
 
 Profiles of 157 companies involved in developing RNAi technologies are presented  along with 212 collaborations. They are a mix of companies that supply reagents  and technologies (nearly half of all) and companies that use the technologies  for drug discovery. Out of these, 31 are developing RNAi-based therapeutics and  28 are involved in microRNAs. The bibliography contains selected 500  publications that are cited in the report. The text is supplemented with 35  tables and 10 figures.
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