Morpholinos do not trigger the degradation of 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, inhibiting molecules that might otherwise interact with the RNA. 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, African clawed frog (
Xenopus),
sea urchin and killifish (
F. heteroclitus) producing
morphant embryos, or
electroporate Morpholinos into
chick embryos at later development stages. With appropriate cytosolic delivery systems, Morpholinos are effective in
cell culture. Vivo-Morpholinos, in which the oligo is covalently linked to a delivery
dendrimer, enter cells when administered systemically in adult animals or in tissue cultures.
Gene knockdown is achieved by reducing the expression of a particular gene in a cell. In the case of protein-coding genes, this usually leads to a reduction in the quantity of the corresponding protein in the cell. Knocking down gene expression is a method for learning about the function of a particular protein; in a similar manner, causing a specific
exon to be spliced out of the RNA transcript encoding a protein can help to determine the function of the protein
moiety encoded by that exon or can sometimes knock down the protein activity altogether. These molecules have been applied to studies in several
model organisms, including
mice,
zebrafish,
frogs and
sea urchins. Morpholinos can also modify the
splicing of
pre-mRNA or inhibit the maturation and activity of miRNA. Techniques for targeting Morpholinos to RNAs and delivering Morpholinos into cells have recently been reviewed in a journal article and in book form.
Normal gene expression in eukaryotes In
eukaryotic organisms, pre-mRNA is
transcribed in the nucleus,
introns are
spliced out, then the mature mRNA is exported from the
nucleus to the
cytoplasm. The small subunit of the
ribosome usually starts by binding at the 5' end of the mRNA and is joined there by various other
eukaryotic initiation factors, forming the initiation complex. The initiation complex scans along the mRNA strand until it reaches a
start codon, and then the large subunit of the ribosome attaches to the small subunit and
translation of a
protein begins. This entire process is referred to as gene expression; it is the process by which the information in a
gene, encoded as a sequence of bases in
DNA, is converted into the structure of a protein. A Morpholino can modify splicing, block translation, or block other functional sites on RNA depending on the Morpholino's base sequence.
Blocking translation Bound to the
5'-untranslated region of messenger RNA (mRNA), Morpholinos can interfere with progression of the
ribosomal initiation complex from the 5' cap to the start codon. This prevents
translation of the coding region of the targeted
transcript (called "
knocking down"
gene expression). This is useful experimentally when an investigator wishes to know the function of a particular protein; Morpholinos provide a convenient means of knocking down expression of the protein and learning how that knockdown changes the cells or organism. Some Morpholinos knock down expression so effectively that, after degradation of preexisting proteins, the targeted proteins become undetectable by
Western blot. In 2016 a synthetic peptide-conjugated PMO (PPMO) was found to inhibit the expression of
New Delhi Metallo-beta-lactamase, an enzyme that many drug-resistant bacteria use to destroy carbapenems.
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
nucleophilic adenine base and preventing it from forming the splice lariat structure, or by interfering with the binding of splice regulatory proteins such as splice silencers and
splice enhancers. Preventing the binding of snRNP
U1 (at the donor site) or
U2/
U5 (at the polypyrimidine moiety and acceptor site) can cause modified
splicing, commonly excluding
exons from the mature mRNA. Targeting some splice targets results in intron inclusions, while activation of cryptic splice sites can lead to partial inclusions or exclusions. Targets of
U11/
U12 snRNPs can also be blocked. Splice modification can be conveniently assayed by reverse-transcriptase polymerase chain reaction (
RT-PCR) and is seen as a band shift after
gel electrophoresis of RT-PCR products. and maturation. Morpholinos can block
ribozyme activity. U2 and U12 snRNP functions have been inhibited by Morpholinos. Morpholinos targeted to "slippery" mRNA sequences within protein coding regions can induce translational
frameshifts. Morpholinos can block RNA editing, poly(A) tailing and translocation sequences. Morpholino activities 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==