Serine/threonine protein kinase WNK4 also known as WNK lysine deficient protein kinase 4 or WNK4, is an
enzyme that in humans is encoded by the WNK4gene.[5] Missense mutations cause a genetic form of pseudohypoaldosteronism type 2, also called
Gordon syndrome.
WNK4 is a member of a
serine/threonine kinase family that comprises four members. The family is so named because unlike other serine/threonine kinases, WNKs are characterized by the lack of the lysine in the subdomain II of the catalytic domain.[6] Instead, a lysine in the β2 strand of subdomain I of the catalytic domain is responsible for the kinase activity.[6]
The WNK4 gene is located on chromosome 17q21-q22. It produces a 1,243-amino acid protein encoded by a 3,732-nucleotide
open reading frame within a 4 kb cDNA transcript.[7] WNK4 protein is highly expressed in the
distal convoluted tubule (DCT) and the
cortical collecting duct (CDD) of the
kidney.[7] WNK4 is also present in the brain, lungs, liver, heart, and colon of various mammalian species.[8][9]
Gene mutations in WNK4 has been found in patients with
pseudohypoaldosteronism type II (PHAII),[7] also known as familial hyperkalemic hypertension (FHHt)[10] or Gordon syndrome.[11] PHAII is an
autosomal dominant hereditary disease characterized by
hyperkalemia,
hypertension, and
metabolic acidosis. WNK4 plays a critical role in the regulation of various transporters and channels in the kidney. PHAII-causing mutations in WNK4 result in the dysregulation of renal sodium and potassium transporters and channels, leading to defects in sodium and potassium retention by the kidney, and in turn, elevated
blood pressure and potassium level (
hyperkalemia).
Structure
The
tertiary structure of WNK4 has not been elucidated to date. Nevertheless, several individual
domain structures of the protein are identified. These include a
kinase domain near the
amino terminus followed by an autoinhibitory domain, an acidic motif, two
coiled-coil domains, and a
calmodulin-binding domain in the
C-terminal segment (Fig. 1). The structures for the kinase and autoinhibitory domains of
WNK1 have been revealed. The high level of structural similarity between WNK4 and
WNK1 allows us to deduce key structural details of WNK4 based on the insights gained from the corresponding regions within
WNK1. The kinase domain of WNK4 has an 83%
sequence identity with that of
WNK1. The overall fold of the kinase domain of
WNK1 resembles those of other protein kinases that have a typical dual-domain architecture.[12] The C-terminal domain of WNK4 bears a high degree of similarity to other kinases within the family. On the other hand, the N-terminal domain is unique in having a six-stranded instead of a five-stranded
β sheet to form a complete
β barrel.[12]
Fig. 1. Domain structure of WNK4 and the positions of the initially identified PHAII-causing mutations. The amino-acid (aa) positions of the domains are provided in parentheses. Some important PHAII mutations are localized in the acidic motif and calmodulin-binding domain, respectively.
A chloride ion binding site has been identified in the region 320DLG323 of the kinase domain in WNK4.[13] The binding of chloride Cl− in this region inhibits the activation of WNK4. The autoinhibitory domain is a homolog of the RFXV-binding PASK/FRAY homology 2 (PF2) domain.[14] Structural studies have revealed that the autoinhibitory domain consists of three β-strands and two
α-helices.[15] Notably, the RFXV‐binding groove is formed by the β3-αA interface of WNK proteins where RFXV peptide ligand interacts directly with residues Phe524, Asp531, and Glu539 of WNK1.[15] The interaction between the RFXV motif and the autoinhibitory domain makes it possible for the C-terminal region of WNK4 to be in close proximity of the kinases domain and subsequently regulate its activity.
Function
Fig. 2.The WNK4-SPAK/OSR1-NCC phosphorylation cascade. WNK4 phosphorylates and activates SPAK/OSR1, which in turn phosphorylate and activates NCC. In this manner, WNK4 regulates sodium reabsorption in the distal convoluted tubule and downstream potassium secretion through its positive effects on NCC.
As a typical
kinase, WNK4 accomplishes the
phosphorylation of its substrate proteins by adding a phosphate moiety in an
ATP-dependent manner. This
structural modification usually results in functional alterations of downstream substrates. Some currently known substrates of WNK4 includes kinases STE20-serine-proline alanine-rich kinase (SPAK) and oxidative stress response 1 kinase (OSR1), which in turn can phosphorylate and activate the thiazide-sensitive
sodium-chloride cotransporter (NCC)[16][17] (Fig. 2). Similarly, WNK4 activates
NKCC1 and deactivate
KCC2 through a SPAK-dependent mechanism.[18] The kinase activity of WNK4 has been demonstrated in vitro using the WNK4 kinase domain purified from E. coli.[19] This phosphorylation cascade is critical in regulating sodium and potassium
homeostasis dysregulation which is tied to the pathogenesis of PHAII.
In addition to NCC, WNK4 also regulates multiple ions channels and cotransporters in the kidney through various mechanisms. These include
epithelial Na+ channel (ENaC),
renal outer medullary potassium channel (ROMK),
transient receptor potential vanilloid member 4 and
5 (TRPV4/5, calcium channels), Na-K-2Cl cotransporter 1 and 2 (
NKCC1/2),
K+-Cl− cotransporter type 2 (KCC2), and other channels/transporters. WNK4 inhibits the functions of ENaC, ROMK, and TRPV4 by reducing the total and cell surface expression of these channels.[20][21][22] WNK4 enhances
TRPV5 by increasing its forward trafficking to the
plasma membrane in a kinase-dependent manner.[23] The inhibitory effect of WNK4 on
ROMK is reversed by
serum and glucocorticoid kinase 1 (SGK1) or by a corresponding phosphomimetic S1169D mutation on WNK4.[21] The N-terminal segment of WNK4 containing the kinase domain and acidic motif is required for the WNK4-mediated inhibition of ROMK.[24] The second coiled-coil domain of WNK4 mediates the downregulation of TRPV4. WNK4 and
calcium-binding protein 39 (Cab39) act together to activate transporters NKCC1 and NKCC2.[25]
Role in pseudohypoaldosteronism type 2
Dysregulation of WNK4 kinase activity
In 2001, four
missense mutations in the WNK4 gene were identified in patients with pseudohypoaldosteronism type 2 (PHAII) (Fig. 1).[7] Three of these mutations (E562K, D564A, and Q565E) are charge-changing substitutions in the acidic motif of WNK4, which are conserved among all members of the WNK family in human and rodent species. The fourth substitution (R1185C) is located in the
calmodulin-binding domain near the second
coiled-coil domain. Few other PHAII mutations in WNK4 have also been reported. Examples of these mutations include E560G,[26] P561L,[27] and D564H,[28] all of which are located close to or in the acidic motif; and K1169E [29] which is located between the
coiled-coil 2 and the
calmodulin-binding domain.
Fig. 3. Proposed mechanisms by which PHAII-causing mutations in WNK4, KLHL3, and Cullin 3 lead to increased kinase activity of WNK4.Left panel, under physiological condition, angiotensin II elicits an increase in intracellular Ca2+. Ca2+ ions interact with the acidic motif of WNK4 and increase the kinase activity. Ca2+/calmodulin (CaM) also binds to the C-terminal CaM-binding domain and relieves the inhibition of the kinase activity of WNK4. WNK4 protein is degraded by the KLHL3-Cullin 3 ubiquitin E3 ligase. Right panel, under PHAII condition, PHAII mutations in the acidic motif mimic the Ca2+ binding state and lead to an increase in kinase activity. The R1185C mutation relieves the inhibitory effect of the C-terminal domain on the kinase activity of WNK4. Mutations in KLHL3 or Cullin 3 impair the degradation of WNK4 protein, leading to an increase in total kinase activity.
The PHAII mutations appear to disrupt the mechanisms underlying Ca2+-sensitivity of WNK4 kinase. Two mechanisms are important in this regard. First, the PHAII-causing mutations in the acidic motif make the kinase domain insensitive to Ca2+ concentration. The acidic motif of WNK4 potentially acts as a Ca2+ sensor, and WNK4 kinase activity rises when Ca2+ concentration is elevated. This has been demonstrated using isolated WNK4 kinase domain truncated to contain the acidic motif.[19] The kinase activity is elevated when a PHAII-causing mutation is present in the acidic motif, similar to what is observed in a Ca2+-binding state (Fig. 3). Second, the WNK4 C-terminal region containing the calmodulin-binding domain and multiple SGK1 phosphorylation sites inhibits the WNK4 activity at the resting state.[30] However, when Ca2+ levels are elevated, Ca2+/calmodulin complex binds to the C-terminal region, derepressing WNK4 kinase activity. Additionally, the RFXV motif is believed to interact with the autoinhibitory domain and subsequently triggers a conformational change that brings the C-terminal and kinase domain close for the inhibitory effect to take place.
Angiotensin II increases the SPAK phosphorylation and activates NCC through a WNK-dependent mechanism.[31] The activation of SPAK and NCC by angiotensin II is abrogated by WNK4 knockdown.[32] Activation of
angiotensin II receptor AT1 couples to
Gq/11 to activate
phospholipase C and to increase the intracellular Ca2+ concentration. An increase in Ca2+ concentration then elevates WNK4 activity through mechanisms described above (Fig. 3, left panel). The PHAII-causing mutations in the acidic motif and the R1185C mutation in the
calmodulin-binding domain constitutively activate the WNK4 kinase domain allowing it to function despite the absence of angiotensin II (Fig. 3, right panel).
Angiotensin II stimulates the secretion of
aldosterone, which induces
SGK1. SGK1 influences both the WNK-SPAK-NCC [33] and SGK1-ENaC signaling cascades.[34] There are multiple SGK1 phosphorylation sites in the C-terminal region of WNK4 located within or close to the
calmodulin-binding domain. SGK1-mediated phosphorylation of these sites is thought to disrupt the effect of the C-terminal inhibitory domain and concomitantly increase WNK4 kinase activity.[30] The alteration of SGK1 phosphorylation by the R1185C mutation is another indication that the mutation disrupts the C-terminal inhibitory mechanism in WNK4 (Fig. 3, right panel).
Dysregulation of WNK4 abundance
Besides WNK1 and WNK4, mutations in two other genes, CUL3 (encoding
Cullin 3) and KLHL3 (encoding
Kelch Like Family Member 3) have been found in patients with PHAII.[35][36] These two proteins are part of the
ubiquitin E3 ligase complex involved in the ubiquitin-mediated degradation of
WNK1 and WNK4. The PHAII-causing mutations in
KLHL3 and
cullin 3 prevent the interactions of these proteins with each other and with WNK1/4. The mutations in these proteins impair the degradation of WNK1/4. This in turn increases the protein abundance of WNK1/4 and concomitantly enhances the total kinase activity.[37] The increased WNK4 kinase activity leads to the
hyperactivation of NCC through WNK4-SPAK and/or the OSR1-NCC cascades, ultimately resulting in the retention of sodium and potassium by the kidney.
Elevated WNK4 activity
Fig. 4. The physiological consequence of elevated NCC activity due to the increased WNK4 kinase activity in PHAII. Shown are the renal tubule segments containing the distal convoluted tubule and the aldosterone-sensitive connecting tubule and collecting duct under normal and PHAII conditions due to mutations in WNK4, KLHL3, or cullin 3. The net effects of these mutations are to elevate WNK4 kinase activity in the distal convoluted tubule. This leads to the increased reabsorption of Na+ in the distal convoluted tubule and thereby less Na+ reabsorption and K+ secretion. The consequence is the retention of Na+ and K+, leading to high blood pressure and hyperkalemia over time.
The primary effect of the elevated WNK4 kinase activity is the increase of NCC-mediated sodium reabsorption in the
distal convoluted tubule of the kidney. The increase in sodium reabsorption in this segment of the
nephron reduces the sodium load in the
collecting duct, where sodium reabsorption by the
ENaC provides the driving force for potassium secretion through
ROMK (Fig. 4). The sodium reabsorption by hyperactive
NCC overrides the loss of reabsorption by
ENaC, and the net effect is moderate sodium retention. Over time, this potentially contributes to the elevated blood pressure observed in PHAII patients. The reduction of potassium secretion by
ROMK contributes to the development of
hyperkalemia. The direct effects of the elevated WNK4 activity on other channels and transporters, such as ENaC, ROMK, and Ca2+-activated maxi K+ channels, may also contribute to the pathogenesis of PHAII; however, the primary features of PHAII could be explained by the gain-of-function of NCC.
^Arnold JE, Healy JK (September 1969). "Hyperkalemia, hypertension and systemic acidosis without renal failure associated with a tubular defect in potassium excretion". The American Journal of Medicine. 47 (3): 461–72.
doi:
10.1016/0002-9343(69)90230-7.
PMID5808659.
^Gordon RD, Geddes RA, Pawsey CG, O'Halloran MW (November 1970). "Hypertension and severe hyperkalaemia associated with suppression of renin and aldosterone and completely reversed by dietary sodium restriction". Australasian Annals of Medicine. 19 (4): 287–94.
doi:
10.1111/imj.1970.19.4.287.
PMID5490655.
^Gagnon KB, England R, Delpire E (January 2006). "Volume sensitivity of cation-Cl- cotransporters is modulated by the interaction of two kinases: Ste20-related proline-alanine-rich kinase and WNK4". American Journal of Physiology. Cell Physiology. 290 (1): C134-42.
doi:
10.1152/ajpcell.00037.2005.
PMID15930150.
^Fu Y, Subramanya A, Rozansky D, Cohen DM (June 2006). "WNK kinases influence TRPV4 channel function and localization". American Journal of Physiology. Renal Physiology. 290 (6): F1305-14.
doi:
10.1152/ajprenal.00391.2005.
PMID16403833.
^Jiang Y, Ferguson WB, Peng JB (February 2007). "WNK4 enhances TRPV5-mediated calcium transport: potential role in hypercalciuria of familial hyperkalemic hypertension caused by gene mutation of WNK4". American Journal of Physiology. Renal Physiology. 292 (2): F545-54.
doi:
10.1152/ajprenal.00187.2006.
PMID17018846.
S2CID12884928.
^Murthy M, Cope G, O'Shaughnessy KM (October 2008). "The acidic motif of WNK4 is crucial for its interaction with the K channel ROMK". Biochemical and Biophysical Research Communications. 375 (4): 651–4.
doi:
10.1016/j.bbrc.2008.08.076.
PMID18755144.
^Gong H, Tang Z, Yang Y, Sun L, Zhang W, Wang W, et al. (June 2008). "A patient with pseudohypoaldosteronism type II caused by a novel mutation in WNK4 gene". Endocrine. 33 (3): 230–4.
doi:
10.1007/s12020-008-9084-8.
PMID19016006.
S2CID45040268.
^Zhang C, Wang Z, Xie J, Yan F, Wang W, Feng X, et al. (2011). "Identification of a novel WNK4 mutation in Chinese patients with pseudohypoaldosteronism type II". Nephron Physiology. 118 (3): 53–61.
doi:
10.1159/000321879.
PMID21196779.
S2CID11164311.
^Louis-Dit-Picard H, Barc J, Trujillano D, Miserey-Lenkei S, Bouatia-Naji N, Pylypenko O, et al. (March 2012). "KLHL3 mutations cause familial hyperkalemic hypertension by impairing ion transport in the distal nephron". Nature Genetics. 44 (4): 456–60, S1-3.
doi:
10.1038/ng.2218.
PMID22406640.
S2CID112724.