{{short description|Type of RNA}} [[Image:shRNA Lentivirus.svg|thumb|upright=2.9|300px|right|Lentiviral delivery of shRNA and the mechanism of RNA interference in mammalian cells.]]
A '''short hairpin RNA''' or '''small hairpin RNA''' ('''shRNA'''/Hairpin Vector) is an artificial RNA molecule with a tight hairpin turn that can be used to silence target gene expression via RNA interference (RNAi).<ref>{{cite journal | vauthors = Paddison PJ, Caudy AA, Bernstein E, Hannon GJ, Conklin DS |author-link3=Emily Bernstein| title = Short hairpin RNAs (shRNAs) induce sequence-specific silencing in mammalian cells | journal = Genes & Development | volume = 16 | issue = 8 | pages = 948–58 | date = April 2002 | pmid = 11959843 | pmc = 152352 | doi = 10.1101/gad.981002 }}</ref><ref>{{cite journal | vauthors = Brummelkamp TR, Bernards R, Agami R | title = A system for stable expression of short interfering RNAs in mammalian cells | journal = Science | volume = 296 | issue = 5567 | pages = 550–3 | date = April 2002 | pmid = 11910072 | doi = 10.1126/science.1068999 | bibcode = 2002Sci...296..550B | author-link2 = René Bernards | hdl = 1874/15573 | hdl-access = free }}</ref><ref>{{cite journal | vauthors = McManus MT, Petersen CP, Haines BB, Chen J, Sharp PA | title = Gene silencing using micro-RNA designed hairpins | journal = RNA | volume = 8 | issue = 6 | pages = 842–850 | date = June 2002 | article-number = S1355838202024032 | pmid = 12088155 | pmc = 137036 | doi = 10.1017/s1355838202024032 }}</ref> Expression of shRNA in cells is typically accomplished by delivery of plasmids or through viral or bacterial vectors. shRNA is an advantageous mediator of RNAi in that it has a relatively low rate of degradation and turnover. However, it requires use of an expression vector, which has the potential to cause side effects in medicinal applications.<ref name="WangRao2011">{{cite journal | vauthors = Wang Z, Rao DD, Senzer N, Nemunaitis J | title = RNA interference and cancer therapy | journal = Pharmaceutical Research | volume = 28 | issue = 12 | pages = 2983–95 | date = December 2011 | pmid = 22009588 | doi = 10.1007/s11095-011-0604-5 | s2cid = 36738846 }}</ref>
The promoter choice is essential to achieve robust shRNA expression. At first, polymerase III promoters such as U6 and H1 were used; however, these promoters lack spatial and temporal control.<ref name="WangRao2011"/> As such, there has been a shift to using polymerase II promoters, which are inducible, to regulate shRNA expression.
==Delivery==
Expression of shRNA in cells can be obtained by delivery of plasmids or through viral or bacterial vectors.
Delivery of plasmids to cells through transfection to obtain shRNA expression can be accomplished using commercially available reagents ''in vitro''. However, this method is not applicable ''in vivo'' and thus has limited utility.
Use of a bacterial vector to obtain shRNA expression in cells is a relatively recent approach. It builds off research showing that recombinant ''Escherichia coli'', containing a plasmid with shRNA, fed to mice can knock-down target gene expression in the intestinal epithelium.<ref name="XiangFruehauf2006">{{cite journal | vauthors = Xiang S, Fruehauf J, Li CJ | title = Short hairpin RNA-expressing bacteria elicit RNA interference in mammals | journal = Nature Biotechnology | volume = 24 | issue = 6 | pages = 697–702 | date = June 2006 | pmid = 16699500 | doi = 10.1038/nbt1211 | s2cid = 17700388 }}</ref> This approach was used in 2012 in clinical trials to try to treat patients with Familial Adenomatous Polyposis.<ref name="BurnettRossi2011">{{cite journal | vauthors = Burnett JC, Rossi JJ, Tiemann K | title = Current progress of siRNA/shRNA therapeutics in clinical trials | journal = Biotechnology Journal | volume = 6 | issue = 9 | pages = 1130–46 | date = September 2011 | pmid = 21744502 | pmc = 3388104 | doi = 10.1002/biot.201100054 }}</ref>
A variety of viral vectors can be used to obtain shRNA expression in cells including adeno-associated viruses (AAVs), adenoviruses, and lentiviruses. With adeno-associated viruses and adenoviruses, the genomes remain episomal. This is advantageous as insertional mutagenesis is avoided. It is disadvantageous in that the progeny of the cell will lose the virus quickly through cell division unless the cell divides very slowly. AAVs differ from adenoviruses in that the viral genes have been removed and they have diminished packing capacity. Lentiviruses integrate into sections of transcriptionally active chromatin and are thus passed on to progeny cells. With this approach there is increased risk of insertional mutagenesis; however, the risk can be reduced by using an integrase-deficient lentivirus.<ref name="LombardoGenovese2007">{{cite journal | vauthors = Lombardo A, Genovese P, Beausejour CM, Colleoni S, Lee YL, Kim KA, Ando D, Urnov FD, Galli C, Gregory PD, Holmes MC, Naldini L | title = Gene editing in human stem cells using zinc finger nucleases and integrase-defective lentiviral vector delivery | journal = Nature Biotechnology | volume = 25 | issue = 11 | pages = 1298–306 | date = November 2007 | pmid = 17965707 | doi = 10.1038/nbt1353 | s2cid = 16008349 }}</ref>
[[File:2ffl-by-domain.png|thumb|left|The dicer protein from ''Giardia intestinalis''.<ref name="Macrae">{{cite journal | vauthors = Macrae IJ, Zhou K, Li F, Repic A, Brooks AN, Cande WZ, Adams PD, Doudna JA | title = Structural basis for double-stranded RNA processing by Dicer | journal = Science | volume = 311 | issue = 5758 | pages = 195–8 | date = January 2006 | pmid = 16410517 | doi = 10.1126/science.1121638 | bibcode = 2006Sci...311..195M | s2cid = 23785494 }}</ref>]]
==Mechanism of action== Once the vector has integrated into the host genome, the shRNA is then transcribed in the nucleus by polymerase II or polymerase III depending on the promoter choice. The product mimics pri-microRNA (pri-miRNA) and is processed by Drosha. The resulting pre-shRNA is exported from the nucleus by Exportin 5. This product is then processed by Dicer and loaded into the RNA-induced silencing complex (RISC). The sense (passenger) strand is degraded. The antisense (guide) strand directs RISC to mRNA that has a complementary sequence. In the case of perfect complementarity, RISC cleaves the mRNA. In the case of imperfect complementarity, RISC represses translation of the mRNA. In both of these cases, the shRNA leads to target gene silencing.
==Applications in gene therapy== Due to the ability of shRNA to provide specific, long-lasting, gene silencing there has been great interest in using shRNA for gene therapy applications. Three examples of shRNA-based therapies are discussed below.
Gradalis, Inc. developed the FANG vaccine, which is used in treatment of advanced cancers. FANG relies on a bifunctional shRNA (bi-shRNA) against the immunosuppressive transforming growth factors (TGF) β1 and β2.<ref name="SenzerBarve2011">{{cite journal | vauthors = Senzer N, Barve M, Kuhn J, Melnyk A, Beitsch P, Lazar M, Lifshitz S, Magee M, Oh J, Mill SW, Bedell C, Higgs C, Kumar P, Yu Y, Norvell F, Phalon C, Taquet N, Rao DD, Wang Z, Jay CM, Pappen BO, Wallraven G, Brunicardi FC, Shanahan DM, Maples PB, Nemunaitis J | title = Phase I trial of "bi-shRNAi(furin)/GMCSF DNA/autologous tumor cell" vaccine (FANG) in advanced cancer | journal = Molecular Therapy | volume = 20 | issue = 3 | pages = 679–86 | date = March 2012 | pmid = 22186789 | pmc = 3293620 | doi = 10.1038/mt.2011.269 }}</ref> Autologous tumor cells were harvested from patients and a plasmid encoding the bifunctional shRNA and granulocyte-macrophage colony-stimulating factor (GMCSF) was introduced ''ex vivo'' through electroporation. These cells were later irradiated and injected back into the patient.
Marina Biotech developed CEQ508 which is used to treat Familial Adenomatous Polyposis. CEQ508 uses a bacterial vector to deliver shRNA against β-catenin.
Gradalis, Inc. developed bifunctional shRNA-STMN1 (pbi-shRNA STMN1), which is used to treat advanced and/or metastatic cancers. This pbi-shRNA STMN1 is against stathmin 1 and is delivered intratumorally through bilamellar invaginated vesicle (BIV) lipoplex (LP) technology.
Several challenges typically confront shRNA-based therapeutics. The most significant challenge is delivery. shRNA is typically delivered through use of a vector, and although they are generally efficient, they pose significant safety concerns. In particular, viral based gene therapy approaches have proved dangerous in past clinical trials. In the first generation of retro viral gene therapy, some patients treated with viral vectors for Wiskott–Aldrich syndrome developed acute T-cell leukaemia. This was determined to have been caused by viral vector insertion location.<ref>{{cite journal | vauthors = Persons DA, Baum C | title = Solving the problem of γ-retroviral vectors containing long terminal repeats | journal = Molecular Therapy | volume = 19 | issue = 2 | pages = 229–31 | date = February 2011 | pmid = 21289636 | pmc = 3034864 | doi = 10.1038/mt.2010.305 }}</ref> Potential oversaturation of RISC is also a problem. If the shRNA is expressed at levels that are too high, the cell might not be able to correctly process the endogenous RNA which could cause significant problems. Another challenge is the possibility that the patient might mount an immune response against the therapy.<ref>{{cite journal | vauthors = Whitehead KA, Dahlman JE, Langer RS, Anderson DG | title = Silencing or stimulation? siRNA delivery and the immune system | journal = Annual Review of Chemical and Biomolecular Engineering | volume = 2 | pages = 77–96 | year = 2011 | pmid = 22432611 | doi = 10.1146/annurev-chembioeng-061010-114133 }}</ref> Finally, there might be off-target effects and the shRNA could silence other unintended genes. In developing successful new shRNA-based therapeutics, all of these challenges must be taken into account.
== See also == * Small interfering RNA * VIRsiRNAdb
== References == {{reflist|colwidth=32em}} {{Types of RNA}} {{Nucleic acids}}
Category:RNA Category:RNA interference