.
Foundation Wnt signaling begins when a Wnt protein binds to the N-terminal extra-cellular cysteine-rich domain of a
Frizzled (Fz) family receptor. However, to facilitate Wnt signaling,
co-receptors may be required alongside the interaction between the Wnt protein and Fz receptor. Examples include
lipoprotein receptor-related protein (
LRP)-5/6,
receptor tyrosine kinase (RTK), and
ROR2.
Canonical and noncanonical pathways The three best characterized Wnt signaling pathways are the canonical Wnt pathway, the noncanonical planar cell polarity pathway, and the noncanonical Wnt/calcium pathway. As their names suggest, these pathways belong to one of two categories: canonical or noncanonical. The difference between the categories is that a canonical pathway involves the protein
beta-catenin (β-catenin) while a noncanonical pathway operates independently of it.
Canonical pathway The canonical Wnt pathway (or Wnt/
β-catenin pathway) is the Wnt pathway that causes an accumulation of
β-catenin in the cytoplasm and its eventual translocation into the
nucleus to act as a transcriptional
coactivator of
transcription factors that belong to the
TCF/LEF family. Without Wnt, β-catenin would not accumulate in the cytoplasm since a destruction complex would normally degrade it. This destruction complex includes the following proteins:
Axin,
adenomatosis polyposis coli (APC),
protein phosphatase 2A (PP2A),
glycogen synthase kinase 3 (GSK3) and
casein kinase 1α (CK1α). It degrades β-catenin by targeting it for
ubiquitination, which subsequently sends it to the
proteasome to be digested. transcription factors. and Parafibromin/Hyrax. The complexity of the transcriptional complex assembled by
β-catenin is beginning to emerge thanks to new high-throughput
proteomics studies. However, a unified theory of how β‐catenin drives target gene expression is still missing, and tissue-specific players might assist β‐catenin to define its target genes. The extensivity of the
β-catenin interacting proteins complicates our understanding: β-catenin may be directly phosphorylated at Ser552 by Akt, which causes its disassociation from cell-cell contacts and accumulation in cytosol, thereafter
14-3-3ζ interacts with β-catenin (pSer552) and enhances its nuclear translocation.
BCL9 and
Pygopus have been reported, in fact, to possess several
β-catenin-independent functions (therefore, likely, Wnt signaling-independent).
Noncanonical pathways The noncanonical planar cell polarity (PCP) pathway does not involve β-catenin. It does not use LRP-5/6 as its co-receptor and is thought to use
NRH1,
Ryk,
PTK7 or
ROR2. The PCP pathway is activated via the binding of Wnt to Fz and its co-receptor. The receptor then recruits
Dsh, which uses its PDZ and DIX domains to form a complex with Dishevelled-associated activator of
morphogenesis 1 (
DAAM1). Daam1 then activates the small
G-protein Rho through a
guanine exchange factor. Rho activates
Rho-associated kinase (ROCK), which is one of the major regulators of the
cytoskeleton. Dsh also forms a complex with
rac1 and mediates
profilin binding to
actin. Rac1 activates
JNK and can also lead to
actin polymerization.
Profilin binding to actin can result in restructuring of the cytoskeleton and
gastrulation. The noncanonical Wnt/calcium pathway also does not involve
β-catenin. Its role is to help regulate calcium release from the
endoplasmic reticulum (ER) in order to control intracellular calcium levels. Like other Wnt pathways, upon ligand binding, the activated Fz receptor directly interacts with Dsh and activates specific Dsh-protein domains. The domains involved in Wnt/calcium signaling are the PDZ and DEP domains. However, if PDE is activated, calcium release from the ER is inhibited. PDE mediates this through the inhibition of PKG, which subsequently causes the inhibition of calcium release. Some evidence for this was found for one Wnt ligand (Wnt5A). Evidence for a convergent Wnt signaling pathway that shows integrated activation of Wnt/Ca2+ and Wnt/
β-catenin signaling, for multiple Wnt ligands, was described in mammalian cell lines.
Other pathways Wnt signaling also regulates a number of other signaling pathways that have not been as extensively elucidated. One such pathway includes the interaction between Wnt and
GSK3. During cell growth, Wnt can inhibit GSK3 in order to activate
mTOR in the absence of β-catenin. However, Wnt can also serve as a negative regulator of mTOR via activation of the
tumor suppressor TSC2, which is upregulated via Dsh and GSK3 interaction. During
myogenesis, Wnt uses
PA and
CREB to activate
MyoD and
Myf5 genes. Wnt also acts in conjunction with
Ryk and
Src to allow for regulation of neuron repulsion during
axonal guidance. Wnt regulates
gastrulation when
CK1 serves as an inhibitor of
Rap1-ATPase in order to modulate the cytoskeleton during gastrulation. Further regulation of gastrulation is achieved when Wnt uses ROR2 along with the
CDC42 and
JNK pathway to regulate the expression of
PAPC. Dsh can also interact with aPKC,
Pa3,
Par6 and
LGl in order to control cell polarity and
microtubule cytoskeleton development. While these pathways overlap with components associated with PCP and Wnt/Calcium signaling, they are considered distinct pathways because they produce different responses. For example, Wnt proteins are
palmitoylated. The protein
porcupine mediates this process, which means that it helps regulate when the Wnt ligand is secreted by determining when it is fully formed. Secretion is further controlled with proteins such as
GPR177 (wntless) and
evenness interrupted and complexes such as the
retromer complex. Upon
secretion, the ligand can be prevented from reaching its receptor through the binding of proteins such as the stabilizers
Dally and
glypican 3 (GPC3), which inhibit diffusion. In cancer cells, both the heparan sulfate chains and the core protein of GPC3 are involved in regulating Wnt binding and activation for cell proliferation. Wnt recognizes a heparan sulfate structure on GPC3, which contains IdoA2S and GlcNS6S, and the 3-O-sulfation in GlcNS6S3S enhances the binding of Wnt to the heparan sulfate glypican. A cysteine-rich domain at the N-lobe of GPC3 has been identified to form a Wnt-binding hydrophobic groove including phenylalanine-41 that interacts with Wnt. Blocking the Wnt binding domain using a nanobody called HN3 can inhibit Wnt activation.
secreted Frizzled-related proteins (SFRP),
Cerberus,
Frzb,
Wise,
SOST, and
Naked cuticle. These constitute inhibitors of Wnt signaling. However, other molecules also act as activators.
Norrin and
R-Spondin2 activate Wnt signaling in the absence of Wnt ligand. Interactions between Wnt signaling pathways also regulate Wnt signaling. As previously mentioned, the Wnt/calcium pathway can inhibit TCF/β-catenin, preventing canonical Wnt pathway signaling. == Induced cell responses ==