Morpholino



  In molecular biology, a Morpholino is a kind of morpholine ring; this article discusses only the Morpholino antisense oligos.

Morpholinos are usually used as a research tool for reverse genetics by knocking down gene function. This is achieved by preventing cells from making a targeted encoded by that exon. These molecules have been applied to studies in several model organisms, including mice, zebrafish and frogs.[3]

Morpholinos are also in development as AVI BioPharma Inc.).

Structure

Morpholinos are pH range, so Morpholinos in organisms or cells are uncharged molecules. The entire backbone of a Morpholino is made from these modified subunits. Morpholinos are most commonly used as single-stranded oligos, though heteroduplexes of a Morpholino strand and a complementary DNA strand may be used in combination with cationic cytosolic delivery reagents.[8]

Function

Morpholinos do not degrade their target RNA molecules, unlike many antisense structural types (e.g. phosphorothioates, siRNA). Instead, Morpholinos act by "steric blocking", binding to a target sequence within an RNA and simply getting in the way of molecules which might otherwise interact with the RNA.[1]

Morpholino oligos are often used to investigate the role of a specific mRNA transcript in an embryo. Developmental biologists inject Morpholino oligos into eggs or embryos of zebrafish,[9] African clawed frog (Xenopus),[10] chick,[11] and sea urchin,[12] producing morphant embryos. With appropriate cytosolic delivery systems, Morpholinos are effective in cell culture.[8]

Morpholinos are being developed as pharmaceuticals under the name "clinical trials as anticancer therapies.[14]

Normal gene expression in eukaryotes

  In eukaryotic organisms, pre-mRNA is DNA, is converted into the structure of a protein. A Morpholino can modify splicing or block translation, depending on the Morpholino's base sequence.

Blocking translation

  Bound to the Western blot (e.g. figure 1 in:[15]).

Modifying pre-mRNA splicing

  Morpholinos can interfere with pre-mRNA processing steps either by preventing splice-directing small nuclear ribonucleoproteins (snRNP) complexes from binding to their targets at the borders of introns on a strand of pre-mRNA, or by blocking the gel electrophoresis of RT-PCR products.[2]

Blocking other mRNA sites

Morpholinos have been used to block ribozyme activity[23]. U2 and U12 snRNP functions have been inhibited by Morpholinos.[24] Morpholinos targeted to "slippery" mRNA sequences within protein coding regions can induce translational frameshifts.[25] Activities of Morpholinos against this variety of targets suggest that Morpholinos can be used as a general-purpose tool for blocking interactions of proteins or nucleic acids with mRNA.

Specificity, stability and non-antisense effects

Morpholinos have become a standard knockdown tool in animal embryonic systems, which have a broader range of gene expression than adult cells and can be strongly affected by an off-target interaction. Following initial injections into frog or fish embryos at the single-cell or few-cell stages, Morpholino effects can often be measured five days later, after most of the processes of organogenesis and differentiation are past, with observed phenotypes consistent with target-gene knockdown. Control oligos with irrelevant sequences usually produce no change in embryonic phenotype, evidence of the Morpholino oligo's sequence-specificity and lack of non-antisense effects.

mRNA rescue experiments can often restore the wild-type phenotype to the embryos and provide evidence for the specificity of a Morpholino. In an mRNA rescue, a Morpholino is co-injected with an mRNA that codes for the same protein that the Morphlino is targeted to knock down. However, the rescue mRNA has a modified 5'-UTR (untranslated region) so that the rescue mRNA contains no target for the Morpholino but the rescue mRNA's coding region encodes the protein of interest. Translation of the rescue mRNA replaces production of the protein which was knocked down by the Morpholino. Since the rescue mRNA would not affect phenotypic changes due to modulation of off-target gene expression by the Morpholino, this return to wild-type phenotype is further evidence of Morpholino specificity.

Because of their completely unnatural backbones, Morpholinos are not recognized by cellular proteins. methylation of DNA.

A cause for concern in the use of Morpholinos is the potential for "off target" effects. Up to 18% of Morpholinos appear to have non-target related phenotypes including cell death in the central nervous system and somite tissues of zebrafish embryos.[28] Most of these effects have been shown to be due to activation of apoptosis, and can be suppressed by co-injection of an anti-p53 Morpholino along with the experimental Morpholino.[29] It appears that these effects are sequence specific, as in most cases if a Morpholino is associated with non-target effects, the 4-base mismatch Morpholino will not trigger these effects. The question of whether an observed morphant phenotype is due to the intended knockdown or an off-target interaction can often be addressed by running another experiment to confirm that the observed morphant phenotype results from the knockdown of the expected target. This can be done by recapitulating the morphant phenotype with a second, non-overlapping Morpholino targeting the same mRNA or by confirmation of the observed phenotypes by use of a mutant strain or dominant negative methods. As mentioned above, rescue of observed phenotypes by coinjecting a rescue mRNA is, when feasible, a reliable test of specificity of a Morpholino.

Delivery

For a Morpholino to be effective, it must be delivered past the cell membrane into the cytosol of a cell. Once in the cytosol, Morpholinos freely diffuse between the cytosol and nucleus, as demonstrated by the nuclear splice-modifying activity of Morpholinos observed after microinjection into the cytosol of cells. Different methods are used for delivery into embryos, into cultured cells or into adult animals. A microinjection apparatus is usually used for delivery into an embryo, with injections most commonly performed at the single-cell or few-cell stage; an alternative method for embryonic delivery is electroporation, which can deliver oligos into tissues of later embryonic stages[30]. Common techniques for delivery into cultured cells include the Endo-Porter peptide (which causes the Morpholino to be released from endosomes)[31], the Special Delivery system (using a Morpholino-DNA heteroduplex and an ethoxylated polyethylenimine delivery reagent)[8], electroporation[32] or scrape loading[33]. Delivery into adult tissues is usually difficult, though there are a few systems allowing useful uptake of unmodified Morpholino oligos (including the inherently leaky muscle cells caused by Duchenne muscular dystrophy[34] or the vascular endothelial cells stressed during balloon angioplasty[35]). Systemic delivery into many cells in adult organisms can be accomplished by using covalent conjugates of Morpholino oligos with cell penetrating peptides, and while some toxicity has been associated with the peptides[36][37] they have been used in vivo for effective oligo delivery at doses below those causing observed toxicity[5][38].

Intellectual property

Gene Tools, LLC and AVI BioPharma Inc. claim intellectual property on aspects of Morpholino oligo.[39]

References

  1. ^ a b Summerton, J (1999). "Morpholino Antisense Oligomers: The Case for an RNase-H Independent Structural Type." (Pubmed). Biochimica et Biophysica Acta 1489: 141-58.
  2. ^ a b Draper, BW; Morcos, PA, Kimmel, CB (2001). "Inhibition of zebrafish fgf8 pre-mRNA splicing with morpholino oligos: A quantifiable method for gene knockdown." (Pubmed). Genesis 30 (3): 154-6.
  3. ^ Heasman J (2002). "Morpholino oligos: making sense of antisense?". Dev. Biol. 243 (2): 209-14. PMID 11884031.
  4. ^ Geller BL (2005). "Antibacterial antisense". Curr. Opin. Mol. Ther. 7 (2): 109-13. PMID 15844617.
  5. ^ a b Deas, TS; Bennett CJ, Jones SA, Tilgner M, Ren P, Behr MJ, Stein DA, Iversen PL, Kramer LD, Bernard KA, Shi PY (2007). "In vitro resistance selection and in vivo efficacy of morpholino oligomers against West Nile virus." (Pubmed). Antimicrob Agents Chemother.: Epub ahead of print.
  6. ^ McClorey, G; Fall AM, Moulton HM, Iversen PL, Rasko JE, Ryan M, Fletcher S, Wilton SD (2006). "Induced dystrophin exon skipping in human muscle explants." (Pubmed). Neuromuscul Disord. 16 (9-10): 583-90.
  7. ^ a b Summerton, J; Weller D (1997). "Morpholino Antisense Oligomers: Design, Preparation and Properties." (Pubmed). Antisense & Nucleic Acid Drug Development 7*: 187-95.
  8. ^ a b c Morcos, PA (2001). "Achieving efficient delivery of morpholino oligos in cultured cells." (Pubmed). Genesis 30 (3): 94-102.
  9. ^ Nasevicius, A; Ekker SC (2000). "Effective targeted gene 'knockdown' in zebrafish." (Pubmed). Nature Genetics 26 (2): 216 - 20.
  10. ^ Heasman, J; Kofron M, Wylie C (2000). "Beta-catenin signaling activity dissected in the early Xenopus embryo: a novel antisense approach." (Pubmed). Developmental Biology 222: 124-34.
  11. ^ Kos, R; Reedy MV, Johnson RL, Erickson CA (2001). "The winged-helix transcription factor FoxD3 is important for establishing the neural crest lineage and repressing melanogenesis in avian embryos." (Pubmed). Development 128 (8): 1467-79.
  12. ^ Howard, EW; Newman LA, Oleksyn DW, Angerer RC, Angerer LM (2001). "SpKrl: a direct target of (beta)-catenin regulation required for endoderm differentiation in sea urchin embryos." (Pubmed). Development 128 (3): 365-75.
  13. ^ Coonrod, SA; Bolling LC, Wright PW, Visconti PE, Herr JC (2001). "A morpholino phenocopy of the mouse MOS mutation." (Pubmed). Genesis 30 (3): 198-200.
  14. ^ Devi GR, Beer TM, Corless CL, Arora V, Weller DL, Iversen PL (2005). "In vivo bioavailability and pharmacokinetics of a c-MYC antisense phosphorodiamidate morpholino oligomer, AVI-4126, in solid tumors". Clin. Cancer Res. 11 (10): 3930-8. PMID 15897595.
  15. ^ Stancheva, I; Collins AL, Van den Veyver IB, Zoghbi H, Meehan RR (2003). "A mutant form of MeCP2 protein associated with human Rett syndrome cannot be displaced from methylated DNA by notch in Xenopus embryos." (Pubmed). Mol Cell 12 (2): 425-35.
  16. ^ Bruno, IG; Jin W, Cote GJ (2004). "Correction of aberrant FGFR1 alternative RNA splicing through targeting of intronic regulatory elements." (Pubmed). Hum Mol Genet 3 (20): 2409-20.
  17. ^ Vetrini, F; Tammaro R, Bondanza S, Surace EM, Auricchio A, De Luca M, Ballabio A, Marigo V (2006). "Aberrant splicing in the ocular albinism type 1 gene (OA1/GPR143) is corrected in vitro by morpholino antisense oligonucleotides." (Pubmed). Hum Mutat 27 (5): 420-6.
  18. ^ Morcos, PA (2007). "Achieving targeted and quantifiable alteration of mRNA splicing with Morpholino oligos." (Pubmed). Biochem Biophys Res Commun.
  19. ^ König, H; Matter N, Bader R, Thiele W, Müller F (2007). "Splicing Segregation: The Minor Spliceosome Acts outside the Nucleus and Controls Cell Proliferation." (Pubmed). Cell 131 (4): 718-29.
  20. ^ Kloosterman, WP; Wienholds E, Ketting RF, Plasterk RH (2004). "Substrate requirements for let-7 function in the developing zebrafish embryo." (Pubmed). Nucleic Acids Res 32 (21): 6284-91.
  21. ^ Flynt, AS; Li N, Thatcher EJ, Solnica-Krezel L, Patton JG (2007). "Zebrafish miR-214 modulates Hedgehog signaling to specify muscle cell fate." (Pubmed). Nature Genetics 39: 259-263.
  22. ^ Kloosterman, WP; Lagendijk AK, Ketting RF, Moulton JD, Plasterk RHA (2007). "Targeted inhibition of miRNA maturation with morpholinos reveals a role for miR-375 in pancreatic islet development." (Pubmed). PLoS Biol. 5 (8): e203.
  23. ^ Yen, L; Svendsen J, Lee JS, Gray JT, Magnier M, Baba T, D'Amato RJ, Mulligan RC (2004). "Exogenous control of mammalian gene expression through modulation of RNA self-cleavage." (Pubmed). Nature 431 (7007): 471-6.
  24. ^ Matter, N; Konig H (2005). "Targeted 'knockdown' of spliceosome function in mammalian cells." (Pubmed). Nucleic Acids Res 33 (4): e41.
  25. ^ Howard, MT; Gesteland RF, Atkins JF* (2004). "Efficient stimulation of site-specific ribosome frameshifting by antisense oligonucleotides." (Pubmed). RNA 10 (10): 1653-61.
  26. ^ Hudziak, RM; Barofsky E, Barofsky DF, Weller DL, Huang SB, Weller DD (1996). "Resistance of morpholino phosphorodiamidate oligomers to enzymatic degradation." (Pubmed). Antisense Nucleic Acid Drug Dev 6 (4): 267-72.
  27. ^ Youngblood, DS; Hatlevig SA, Hassinger JN, Iversen PL, Moulton HM (2007). "Stability of cell-penetrating peptide-morpholino oligomer conjugates in human serum and in cells." (Pubmed). Bioconjug Chem. 18 (1): 50-60.
  28. ^ Ekker, SC; Larson JD (2001). "Morphant Technology in Model Developmental Systems." (Pubmed). Genesis 30 (3): 89-93.
  29. ^ Robu, ME; Larson JD, Nasevicius A, Beiraghi S, Brenner C, Farber SA, Ekker SC (2007). "p53 activation by knockdown technologies." (Pubmed). PLoS Genetics 3 (5): e78.
  30. ^ Cerda, GA; Thomas JE, Allende ML, Karlstrom RO, Palma V (2006). "Electroporation of DNA, RNA, and morpholinos into zebrafish embryos." (Pubmed). Methods 39 (3): 207-11.
  31. ^ Summerton, JE (2005). "Endo-porter: a novel reagent for safe, effective delivery of substances into cells." (Pubmed). Ann N Y Acad Sci. 1058: 62-75.
  32. ^ Jubin, R (2004). "Optimizing electroporation conditions for intracellular delivery of morpholino antisense oligonucleotides directed against the hepatitis C virus internal ribosome entry site." (Pubmed). Methods Mol Med. 106: 309-22.
  33. ^ Partridge, M; Vincent A, Matthews P, Puma J, Stein D, Summerton J (1996). "A simple method for delivering morpholino antisense oligos into the cytoplasm of cells." (Pubmed). Antisense Nucleic Acid Drug Dev. 6 (3): 169-75.
  34. ^ Fletcher, S; Honeyman K, Fall AM, Harding PL, Johnsen RD, Wilton SD (2006). "Dystrophin expression in the mdx mouse after localised and systemic administration of a morpholino antisense oligonucleotide." (Pubmed). J Gene Med. 8 (2): 207-16.
  35. ^ Kipshidze, NN; Kim HS, Iversen P, Yazdi HA, Bhargava B, New G, Mehran R, Tio F, Haudenschild C, Dangas G, Stone GW, Iyer S, Roubin GS, Leon MB, Moses JW (2002). "Intramural coronary delivery of advanced antisense oligonucleotides reduces neointimal formation in the porcine stent restenosis model." (Pubmed). J Am Coll Cardiol. 39 (10): 1686-91.
  36. ^ Abes, S; Moulton HM, Clair P, Prevot P, Youngblood DS, Wu RP, Iversen PL, Lebleu B (2006). "Vectorization of morpholino oligomers by the (R-Ahx-R)(4) peptide allows efficient splicing correction in the absence of endosomolytic agents." (Pubmed). J Control Release 116 (3): 304-13.
  37. ^ Burrer, R; Neuman BW, Ting JPC, Stein DA, Moulton HM, Iversen PL, Kuhn P, Buchmeier MJ (2007). "Antiviral effects of antisense morpholino oligomers in murine coronavirus infection models." (Pubmed). J. Virol. 81 (11): 5637-48.
  38. ^ Amantana, A; Moulton HM, Cate ML, Reddy MT, Whitehead T, Hassinger JN, Youngblood DS, Iversen PL (2007). "Pharmacokinetics, Biodistribution, Stability and Toxicity of a Cell-Penetrating Peptide-Morpholino Oligomer Conjugate." (Pubmed). Bioconjug Chem [Epub ahead of print].
  39. ^ Gene Tools, LLC [1]

Further reading

  • Wiley-Liss, Inc. Special Issue: Morpholino Gene Knockdowns of genesis Volume 30, Issue 3 Pages 89-200 (July 2001). A special issue of Genesis, comprised of a series of peer-reviewed short papers utilizing morpholino knock downs of gene function in various animal and tissue culture systems.
  • Moulton, Jon (2007), , in Beaucage, Serge, , New Jersey: John Wiley & Sons, Inc., ISBN 978-0-471-24662-6


Nucleobases: Cytosine)
Nucleosides: Thymidine | Cytidine/Deoxycytidine
Nucleotides: monophosphates (cADPR)
Deoxynucleotides: monophosphates (dAMP, dGDP, TDP, dCDP) | triphosphates (dATP, dGTP, TTP, dCTP)
Ribonucleic acids: snoRNA
Deoxyribonucleic acids: mtDNA
Nucleic acid analogues: TNA | morpholino
Cloning vectors: phagemid | plasmid | lambda phage | cosmid | P1 phage | fosmid | BAC | YAC | HAC
 
This article is licensed under the GNU Free Documentation License. It uses material from the Wikipedia article "Morpholino". A list of authors is available in Wikipedia.