Subscribe to RSS
Download PDF
DOI: 10.1055/a-1528-0499
Mechanism, Functions, and Diagnostic Relevance of FXII Activation by Foreign Surfaces
Funding/Acknowledgment T.R. acknowledges the Deutsche Forschungsgemeinschaft (DFG, German Research Foundation) for grants A11/SFB 877, B8/SFB 841, and P6/KFO 306.
- Abstract
- Zusammenfassung
- Proteins of the Plasma Contact System
- FXII: Domains and Their Functions
- FXII: Zinc Binding
- FXII: Glycosylation
- FXII: Activation
- Relevance of FXII for Diagnostic Coagulation Tests
- Conclusion
- References
Abstract
Factor XII (FXII) is a serine protease zymogen produced by hepatocytes and secreted into plasma. The highly glycosylated coagulation protein consists of six domains and a proline-rich region that regulate activation and function. Activation of FXII results from a conformational change induced by binding (“contact”) with negatively charged surfaces. The activated serine protease FXIIa drives both the proinflammatory kallikrein–kinin pathway and the procoagulant intrinsic coagulation cascade, respectively. Deficiency in FXII is associated with a prolonged activated partial thromboplastin time (aPTT) but not with an increased bleeding tendency. However, genetic or pharmacological deficiency impairs both arterial and venous thrombosis in experimental models. This review summarizes current knowledge of FXII structure, mechanisms of FXII contact activation, and the importance of FXII for diagnostic coagulation testing and thrombosis.
Zusammenfassung
Faktor XII (FXII) ist das Zymogen der Serinprotease FXIIa, wird von Hepatozyten produziert und ins Plasma sekretiert. Das Plasmaprotein besteht aus sechs Domänen sowie einer Prolin-reichen Region und ist stark glykosyliert. Die Aktivierung von FXII erfolgt durch eine Konformationsänderung, die durch die Bindung (den „Kontakt“) mit negativ geladenen Oberflächen hervorgerufen wird. In der Folge aktiviert FXIIa sowohl das proinflammatorische Kallikrein-Kinin-System, welches Bradykinin produziert, als auch die intrinsische Gerinnungskaskade. Eine FXII-Defizienz oder Dysfunktionalität ist mit einer verzögerten aktivierten partiellen Thromboplastinzeit (aPTT) assoziiert, nicht aber mit einer erhöhten Blutungsneigung. Dennoch zeigen experimentelle Modelle, dass FXII essentiell für die Bildung arterieller und venöser, Gefäß-verschließender Thrombosen ist. Diese Übersichtsarbeit fasst das aktuelle Wissen über die Struktur von FXII, den Mechanismus der FXII-Kontaktaktivierung und die Bedeutung von FXII für diagnostische Gerinnungstests zusammen.
Proteins of the Plasma Contact System
The factor XII (FXII)-driven plasma contact system is a proinflammatory and procoagulant plasma protease cascade that is initiated by FXII, in a reaction involving high-molecular-weight kininogen (HK) and plasma prekallikrein (PK; [Fig. 1]).[1] [2] [3] Upon binding to negatively charged surfaces, the FXII zymogen is autocatalytically converted to the serine protease FXIIa, which cleaves PK to active plasma kallikrein (PKa). FXIIa initiates the intrinsic pathway of coagulation and leads to the PKa-mediated liberation of the proinflammatory peptide hormone bradykinin (BK) from the precursor HK (kallikrein–kinin pathway) in vivo. BK, in turn, is rapidly metabolized to vasoactive and eventually inactive peptides. Furthermore, FXIIa has the capacity to activate the fibrinolytic and complement systems in vitro. However, a possible in vivo relevance of FXII contact activation for these reactions remains to be demonstrated.[4] In contrast to other coagulation factors, deficiency in FXII is not associated with obvious coagulation abnormalities in humans and mice. FXII-deficient individuals are phenotypically normal and do not bleed excessively. Our laboratory originally found that both arterial and venous thrombus formation is defective in FXII-deficient (F12−/− ) mice while their hemostatic capacity is within the normal range.[5] It has also been shown that genetic ablation of F12 in mice leads to impaired venous thrombus formation in an inferior vena cava (IVC) stenosis and femoral vein electrolytic injury model, but not in an IVC stasis model.[6] Even so, challenging the dogma of a coagulation “balance,” F12−/− animals have a normal hemostatic capacity but are largely protected from thromboembolic diseases such as ischemic stroke,[7] pulmonary embolism,[8] cancer-driven thrombosis,[9] or sepsis-associated thrombosis.[10] In addition, pharmacological inhibition of FXIIa-driven coagulation provides safe thromboprotection in large animals.[11] [12] Peptides, proteins, and small-molecular-weight inhibitors targeting FXII and FXIIa are discussed in detail by Davoine et al.[13] In addition to coagulation, FXIIa initiates an inflammatory reaction by generation of the peptide hormone BK.[14] [15] Further processing of BK by removal of the C-terminal arginine through carboxypeptidase N results in des-Arg9-BK. Binding of BK and des-Arg9-BK to its G-protein-coupled kinin B2 and B1 receptors (B2R and B1R) initiates intracellular Ca2+-dependent signaling pathways that induce a plethora of inflammatory processes[16] [17] leading to cytoskeleton rearrangement in endothelial[18] [19] and epithelial cells.[20] Deficiency in C1 esterase inhibitor (C1INH, the major endogenous inhibitor of FXIIa and PKa) or FXII gain-of-function mutations are associated with a BK-mediated, life-threatening inflammatory disorder, referred to as hereditary angioedema (HAE).[21] [22] [23]
FXII: Domains and Their Functions
The plasma protein FXII is secreted by the liver into the circulatory system as an inactive, single-chain enzyme precursor (zymogen). In addition, some blood cells such as neutrophils express FXII[2] [24] (https://www.proteinatlas.org/ENSG00000131187-F12/tissue). An N-terminal 19-residue signal sequence mediates secretion of the FXII zymogen. In healthy individuals, the 80 kDa glycoprotein (596 amino acids) circulates in plasma at a concentration of 30 to 35 µg/mL (375 nmol/L).[25] Proteolysis of FXII zymogen occurs at the single peptide bond Arg353–Val354 leading to formation of the active protease FXIIa. Formation of FXIIa proceeds via two principal mechanisms: (1) binding (“contact”) to negatively charged surfaces that induce a conformational change and limited enzymatic activity (autoactivation) or (2) by proteases including PKa and plasmin (fluid-phase activation). FXIIa is composed of two chains termed the “heavy chain” (353 residues) and the “light chain” (243 residues). Both chains are linked by an intramolecular disulfide bond spanning cysteine residues 340 and 467. The light chain comprises the catalytic domain with the typical triad of a serine protease (His393, Asp442, Ser544). The heavy chain is composed of individual domains, starting with the N-terminal fibronectin type II (Fib-II) domain, followed by a first epidermal growth factor-like (EGF-I) domain, a fibronectin type I (Fib-I) domain, a second EGF-like (EGF-II) domain, a kringle domain, and a C-terminal proline-rich (PR) region. In particular, the heavy chain mediates contact to other proteins and surfaces with implications for zymogen activation ([Table 1]). A FXII fragment that completely lacks the heavy chain was unable to contact activate.[11] However, the site(s) required for contact activation has/have remained enigmatic and different studies came to discrepant results.
|
Attribute |
Fib-II |
EGF-I |
Fib-I |
EGF-II |
KR |
PR |
Catalytic domain |
|---|---|---|---|---|---|---|---|
|
Potential surface-binding site |
✓[33] |
||||||
|
Putative Zn2+-binding site |
✓[35] |
✓[35] |
|||||
|
FXI interaction |
✓[28] |
||||||
|
Cell attachment |
✓[104] |
||||||
|
Heparin-binding site |
✓[105] |
||||||
|
Fibrin-binding site |
✓[105] |
||||||
|
Catalytic triad (His393, Asp442, Ser544) |
✓[106] |
Abbreviations: Fib-II, fibronectin type II domain; EGF-I, first epidermal growth factor-like domain; Fib-I, fibronectin type I domain; EGF-II, second epidermal growth factor-like domain; KR, kringle domain; PR, proline-rich region.
Anti-FXII antibodies that interfere with FXII contact activation have been used to identify residues involved in surface binding. Monoclonal antibodies P5-2-1 and B7C9 identified a region within the Fib-II domain as a FXII surface binding site.[26] [27] Challenging a role of residues 1–28 in the Fib-II domain for FXII contact activation, a FXII deletion mutant lacking residues 3–19 was readily contact activatable by dextran sulfate (DXS).[28] The monoclonal antibody B7C9 identified amino acids 134–153 as a part of the Fib-I domain as potential polyanionic surface binding site.[29] Furthermore, anti-FXII antibody KOK5 that recognizes a discontinuous epitope in the Fib-II domain involving residues 30–33, 40–47, and 57–60 inhibits kaolin-triggered FXII contact system activation.[30] However, a 319-amino-acids-deleted FXII mutant, rFXII.lpc, that consists of the light chain and the C-terminal part of the PR region but lacks the entire KOK5 epitope, binds to kaolin and is activated by the anionic surface.[31] A FXII mutant spanning the EGF-II domain, kringle domain, and PR region, as well as the light chain (rFXII-U-like) binds to surfaces and undergoes contact activation.[32] Moreover, a recent study based on recombinant N-terminal FXII deletion mutants indicated that truncated FXII variants lacking the Fib-II domain (FXII Δ1–71) are more prone for autoactivation.[33] This suggests that the Fib-II domain is involved in zymogen contact activation by shielding its activation site. Using various deletion mutants, it was further shown that the Fib-II domain is dispensable for FXII binding to kaolin or polyphosphate (polyP), whereas the EGF-I domain appeared as indispensable.[33] This result is demonstrated in pull-down assays with recombinant FXII variants lacking the EGF-I domain (FXII Δ1–112) that are defective in binding to kaolin and polyP.[33] Together, these studies reveal the complexity in activation of the FXII zymogen and suggest a systematic approach to identify the regions of FXII involved in surface-triggered autoactivation. Functions related to the kringle domain and PR region are not well characterized. Based on in vitro experiments, these domains influence the conformation of FXII and accordingly the exposure of its cleavage site at Arg353-Val354. A recently described FXII point mutation (Trp268Arg) located in the kringle domain next to the PR region disturbs zymogen quiescence and accelerates FXII activation leading to rash and urticaria[34]; however, the underlying FXII-dependent mechanism remains to be characterized.
FXII: Zinc Binding
The divalent cation zinc (Zn2+) is involved in the binding and activation of FXII on negatively charged surfaces. In particular, Zn2+ promotes the stabilization of the transition states formed during the conformational change of FXII upon its autocatalytic cleavage. Putative Zn2+ binding sites within the Fib-II domain (residues His40–His44 and His78–His82) and the EGF-like domains (residues His94–His131 and His174–His176) were described for FXII.[35] Zn2+ circulates in plasma bound to proteins and is released by activated platelets. In vitro studies have also shown that binding of FXII-stimulated platelets is enhanced in the presence of Zn2+.[36] Moreover, Zn2+ facilitates FXII binding to endothelial and smooth muscle cells promoting mitogenic activity in these cell types.[37] FXII binds urokinase-type plasminogen activator receptor (uPAR) and induces proliferation via β1 integrin and EGF receptor (EGFR) signaling that leads to phosphorylation of pERK1/2 and Akt.[38] In addition to uPAR, the globular C1q receptor (gC1qR) provides an attachment site for contact system proteins on the cell surface. The interaction of C1q with gC1qR is known to activate the classical complement cascade[39]; however, gC1qR also binds to FXII and HK and promotes their assembly on cell surfaces.[40] Complex formation with contact system proteins is facilitated by anionic loops of gC1qR, whereas a cell-binding site allows attachment of gC1qR to plasma membrane proteins, such as integrins.[41] Recent structural analysis revealed that the N-terminal Fib-II domain of FXII requires the presence of Zn2+ for interaction with gC1qR.[42] By clustering FXII and HK into a planar ternary complex with a molecular weight of 500 kDa, cell surface–bound gC1qR may enable initiation of the FXII-driven intrinsic coagulation and kallikrein-mediated BK liberation.[42] However, other studies have shown that gC1qR has a mitochondrial targeting sequence sufficient to localize the protein to intracellular compartments, challenging its proposed role as a cell surface receptor for plasma proteins.[43]
FXII: Glycosylation
FXII is a glycoprotein of the β2 globulin fraction of serum electrophoresis separation. Carbohydrates constitute for 14.2 kDa (17.8%) of the apparent molecular protein mass of 80 kDa. In human FXII, two N- and seven putative O-glycosylation sites have been identified ([Table 2]). Most of the glycosylation sites are located within the PR region. Glycosylation is crucial for the functionality and the physical properties of FXII. Consistent with this, a nonglycosylated FXII variant expressed in Escherichia coli has very low or no solubility (unpublished observation of the authors). While glycosylation is critical for solubility of the plasma protein, carbohydrates also regulate FXII contact activation. For example, contact activation of a hypoglycosylated FXII variant with a missense mutation at position 309 (Thr309Lys/Arg; identical to position 328 counting the 19 amino acid signal peptide) is largely accelerated.[44] Lack of a single O-linked FXII glycosylation leads to a gain-of-autoactivation.[45] Furthermore, the mutation produces an additional site for activation of the zymogen by plasmin.[46] Synergistically, gain-of-contact activation and an extra cleavage site lead to excessive production of BK. BK-signaling increases microvascular permeability leading to the inherited swelling disease HAE. Three distinct types of HAE can be differentiated: mutations in the gene SERPING1 encoding for C1INH are causative for HAE type I and HAE type II. Patients suffering from these forms of HAE exhibit a decreased plasma concentration and impaired functionality of C1INH, respectively. In contrast, the third type represents HAE with normal C1INH (HAE-nC1INH) associated with mutations of genes other than SERPING1, such as KNG1,[47] ANGPT1,[48] PLG,[49] or F12.[50] A molecular aberration in F12 leads to the aforementioned Thr309Lys/Arg FXII mutation and causes HAE-FXII due to the increased susceptibility of FXII for contact activation.[45]
|
FXII domain/region |
Type of glycosylation |
Amino acid |
Amino acid position |
Reference |
Related findings |
Reference |
|---|---|---|---|---|---|---|
|
EGF-I |
O-linked |
Thr |
90 |
[107] |
||
|
Kringle |
N-linked |
Asn |
230 |
Asn230Lys mutation (recombinant model, Schneider 2 (S2) cells): lack of glycosylation results in increased intracellular FXII levels and defective secretion |
[109] |
|
|
Proline-rich |
O-linked |
Thr |
280 |
[102] |
||
|
O-linked |
Thr |
286 |
[102] |
|||
|
O-linked |
Ser |
289 |
[102] |
|||
|
O-linked |
Thr |
309 |
[102] |
Thr309Lys/Arg mutation: loss of glycosylation leads to increased FXII activity in HAE-FXII patient plasma |
[45] |
|
|
O-linked |
Thr |
310 |
[102] |
|||
|
O-linked |
Thr |
318 |
[102] |
|||
|
Catalytic domain |
N-linked |
Asn |
414 |
Hypoglycosylated type of FXII in plasma of PMM2-CDG patients: FXII contact activation is unaffected |
[109] |
Abbreviation: EGF-I, first epidermal growth factor-like domain.
FXII: Activation
Endogenous Activators
Over the years, an array of physiological structures with anionic surfaces have been identified as putative FXII contact activators. Here, we focus on some of them, including mast cell heparin, misfolded protein aggregates, polyP, and cell-derived extracellular vesicles. A complete overview on FXII contact activators can be found here.[1]
Heparin, a polysaccharide with a high degree of sulfation and acetylation, is released from mast cells stimulated by IgE/antigen. Mast cell heparin initiates FXII contact activation in human plasma and in mice.[23] Subsequently, BK is released by the kallikrein–kinin system,[15] inducing vasodilation and an increase in permeability with implications for anaphylaxis[51] and edema.[23] In contrast, deficiency of FXII or B2R that is associated with defective BK signaling interferes with mast cell heparin-driven acute swelling events in vivo.[23]
The amyloid β (Aβ) peptide is one of the pathological hallmarks of Alzheimer's disease (AD) and, in its aggregated form, has the capacity to initiate FXII contact activation. In particular, the Aβ42 isoform induces thrombin generation via the intrinsic coagulation cascade in a FXIIa-mediated manner[52] and induces inflammatory reactions by the activated kallikrein–kinin system. Elevated levels of FXIIa are found in the plasma of AD patients,[53] consistent with a role of the contact system in procoagulant and proinflammatory states associated with AD.
Polyphosphate
It is known for decades that activated platelets promote coagulation in a FXII-dependent manner,[54] [55] [56] [57] [58] [59] but the platelet-derived FXII activator had remained unknown. Platelets store high concentrations of the inorganic polymer polyP in their dense granules.[60] PolyP is a linear polymer composed of orthophosphate [P]i monomers that are linked by energy-rich phosphoanhydride bonds. PolyP complexed with calcium ions (Ca2+) is packed in dense granules in high concentrations (up to the molar range) leading to characteristic dark spots in transmission electron microscopy images. Activated platelet-derived polyP potently initiates FXII contact activation[8] providing the long-sought link of primary and secondary hemostasis.[61] PolyP is instable in plasma and is degraded by endogenous phosphatases.[62] Targeting polyP using synthetic and recombinant binding proteins or exopolyphosphatases, enzymes that degrade polyP in bacteria and yeast, interferes with the activity of the polymer to induce FXII contact activation.[63] Only a small portion of platelet polyP (<5%) is released into the cell supernatant upon activation,[63] but the vast majority remains attached to the plasma membrane, indicating that the polymer operates on cell surfaces. In contrast to synthetic polyP, naturally occurring polymers are bound to divalent metal cations such as Ca2+ (and possibly others, e.g., Zn2+). The resulting aggregate formation leads to insoluble polyP nanoparticles that are retained on the platelet membrane.[64] Intravital microscopy has visualized polyP nanoparticles on the surfaces of activated platelets and within platelet-rich thrombi confirming that the majority of platelet polyP is retained on the plasma membrane.[65]
The insoluble Ca2+ and Zn2+-rich polyP nanoparticles found in nature challenge the hypothesis that size of individual polymers would determine polyP function in coagulation. While chain length of synthetic polyP determines its activity on coagulation reactions in plasma,[66] natural platelet polyP forms insoluble Ca2+-rich nanoparticles. These particles function in coagulation reactions independently of the chain length of the individual polyP molecule.[65] Furthermore, these particulate polyP form triggers FXII activation on plasma membranes of platelets, megakaryocytes, various cancer cells, and exosomes/microparticles derived from these cells, with implications for thrombosis in murine models.[9] In contrast to insoluble particulate polyP, a potential in vivo function of soluble polyP remains to be shown. Notably, soluble polyP may have anticoagulant effects since Ca2+-free synthetic short-chain polyP acts as a chelator for Ca2+ ions in plasma.[66]
Platelets release small amounts of short chain polyP (around 80 monomers) that is soluble and found in the supernatant. However, and similar to other cells the majority of platelet polyP comprises long chain insoluble polymers with a chain length > 200 [P]i subunits. Methods to isolate polyP from cells and tissues have been established. The phenol/chloroform extraction method (Werner's protocol[67]) selects for water soluble (short chain) polyP, while anion exchanger is based on purification of both soluble (short chain) and insoluble (long chain) polyP.[68] Despite that polyP is found in every cell in nature, the biosynthesis of the polymer is a topic of ongoing research. So far, mainly prokaryotes but also yeast have served as model organisms for the analysis of enzymes that synthesize polyP with different chain lengths.[68] In yeast, intracellular levels of polyP and inositol pyrophosphate are interdependent from each other and inositol pyrophosphate modulates the cellular [P]i influx.[69] The concentrations of both molecular species are regulated by inositol hexakisphosphate kinase (IP6K1) activity. In Saccharomyces cerevisiae and mice, genetic ablation of Ip6k1 severely reduces polyP and inositol pyrophosphate levels.[70] While reduced inositol pyrophosphate levels do not significantly affect secondary hemostasis, decreased platelet polyP impairs activation of the coagulation cascade in a FXII-dependent manner.[71] Consequently, IP6K1 deficiency protects genetically modified mice from lethal venous thromboembolic events. The xenotropic and polytropic receptor 1 (XPR1) that was originally desired as [P]i exporter represents another polyP-regulating protein. Genetic and pharmacologic targeting of XPR1 interferes with [P]i export and results in polyP accumulation in platelets.[72] Accordingly, surface exposure of polyP from stimulated XPR1-deficient platelets is increased. Excess platelet polyP has no effect on hemostasis but accelerates arterial and venous thrombosis in a FXII-dependent manner. Therefore, modulating proteins that regulate polyP content in platelets may be useful for the prevention of thrombotic disorders.
Cell-Derived Extracellular Vesicles
Extracellular vesicles (EV) modulate blood coagulation under physiological and pathological conditions. Originally, platelet-derived EV termed “microparticles” have been shown to initiate FXII contact activation, while red blood cell–derived EV were inactive in producing FXIIa.[73] Flow cytometric and biochemical analyses with EV isolated from platelet concentrates confirmed that EV support thrombin generation in an FXII-dependent manner. However, in that specific study, red blood cells were also found to contribute to EV-driven FXIIa production,[74] suggesting that distinct populations or age-dependent effects on the coagulation system exist in red blood cells. Red blood cell–derived EV participate in activation of the intrinsic coagulation pathway by two mechanisms: (1) the classical contact activation and (2) a FXII-independent pathway involving PK activation followed by direct stimulation of factor IX (FIX) by a yet unknown protease.[75] Recently, and in line with the previous study, PKa-mediated FIX activation was confirmed in plasma ex vivo.[76] The clinical consequence of red blood cell–triggered coagulation may explain the procoagulant state in patients after blood transfusions.
Biogenesis of EV is accompanied by the translocation of the phospholipid phosphatidylserine (PS) from the inner to the outer membrane leaflet.[77] In addition, exposure of PS on the cell surface is a hallmark of programmed cell death. Apoptotic cells are procoagulant by presenting PS as an attachment site for FXII.[78] A role of phospholipids in FXII-triggered contact activation is also known from circulating triglyceride-rich particles. Thromboelastography and thrombin generation assays revealed that very low density lipoproteins mediate FXII contact activation in a phosphatidylethanolamine- but not PS-dependent manner.[79] In conclusion, further studies are required to analyze, whether phospholipids, especially PS, have a supportive role in FXII-driven coagulation or whether they are capable to directly induce FXII contact activation.
Exogenous Activators
The white clay material kaolin mainly contains kaolinite, a hydrated aluminum silicate. Similar to Ca2+-polyP, Ca2+-kaolin provides a negatively charged surface for FXII binding and subsequent contact activation.[80] Due to these procoagulant activities, hemostatic wound dressings (QuikClot Combat Gauze) are coated with kaolin to rapidly control trauma-induced bleeding. However, long-term exposure of the injured tissue to these hemostatic dressings increases the thromboembolic risk, as kaolin can enter the circulation and trigger clot formation.[81] Wounds rarely remain clean and are more often contaminated with soil, especially in terrestrial vertebrates. Soil is predominantly composed of silicate minerals and induces activation of the intrinsic coagulation cascade in a FXII-dependent manner.[82] Consistent with previous studies showing that birds and some marine mammals are deficient in FXII,[83] [84] soil-stimulated clotting was defective in dolphin or chicken blood.[82] In a murine bleeding model, treatment of an injured vessel with a polyacrylic acid–coated filter paper reduced underlying blood loss in a FXII-dependent manner, indicating that the polymer functions as a contact activator.[85]
In addition to kaolin and other silica-rich materials, glass, sulfatides, and ellagic acid (EA) also represent artificial surfaces that initiate FXII contact activation.[86] [87] EA is a polyphenolic compound associated with antiproliferative and antioxidant effects. Similarly with kaolin and polyP, EA forms complexes with divalent metal ions[88] and only these EA particles, but not soluble free EA molecules, are capable to induce FXII contact activation.[88] Administration of an infusion containing EA caused thrombosis in patients by direct activation of FXII or platelet stimulation.[89]
A well-known FXII contact activator is the sulfated polysaccharide DXS. High-molecular-weight DXS (500 kDa) stimulates FXII contact activation, whereas short-chain DXS (5 kDa) is inactive for zymogen activation.[90] Challenging pigs with DXS led to a BK-mediated drop in blood pressure[91] but did not induce thrombosis. This suggests that DXS specifically triggers the kallikrein–kinin system leading to inflammation but is inactive for driving coagulation. Therefore, injection of the polymer is useful to analyze BK-mediated edema independently on coagulation in mouse models.[92] The synthetic polysaccharide oversulfated chondroitin sulfate (OSCS) acts similarly with high-molecular-weight DXS. OSCS is a potent FXII contact activator. Infusion of heparin contaminated with OSCS led to hypotonic shock[93] with fatal outcome due to BK-mediated hypersensitivity reactions.[94]
The structurally related glycosaminoglycan fucosylated chondroitin sulfate (FCS) also activates the contact system in human plasma. Based on carbohydrate–protein interaction studies, PK binds readily to FCS in the presence of the other contact system proteins, leading to the hypothesis that FXIIa is generated mainly by PKa-mediated fluid-phase activation.[95]
All of the described endogenous and exogenous FXII contact activators have a net negative surface charge, which appears to be necessary for binding/activation of FXII. Vice versa, the positively charged polyethylenimine and the inert polymer Teflon AF failed to induce FXII contact activation human plasma.[96]
Relevance of FXII for Diagnostic Coagulation Tests
FXII contact activation is the mechanistic basis for one of the most commonly performed diagnostic coagulation screening tests, the activated partial thromboplastin time (aPTT). aPTT assays are performed more than 5 billion times annually and are used for (1) preoperative screening; (2) monitoring of intravenous application of heparin; (3) detection of lupus anticoagulants/antiphospholipid syndrome; and (4) identification of deficiency in the contact system proteins including FXII, PK, and HK and the coagulation factors FXI, FIX, and FVIII. Kaolin, micronized silica, or EA is commonly used to trigger FXII-dependent clotting in aPTT assays. Initially, citrated plasma is incubated with artificial surfaces for up to 90 seconds. Within that time a substantial amount of FXII zymogen undergoes conversion to FXIIa that subsequently activates factor XI (FXI) to FXIa. Upon recalcification, the coagulation cascade proceeds and eventually forms fibrin. Accordingly, aPTT represents the time that elapses from recalcification to the formation of a fibrin clot. FXII-deficient plasma has a prolonged/abnormal aPTT, as clotting is impaired in vitro. Notably, extending the incubation time with artificial surfaces normalizes aPTT in PK-deficient plasma due to surface-mediated FXII contact activation that compensates for the absence of PKa-mediated fluid-phase FXII activation.[97] aPTT assays could be discussed as a tool for diagnosing C1INH-HAE, as in one study, approximately 73% of HAE patients with C1INH deficiency had a shortened aPTT compared with HAE patients with functional C1INH.[98]
On the basis of abnormal prolonged aPTT results and sequencing analysis, several mutations in the F12 gene have been identified that were not associated with a history of bleeding events or pathological hemostatic capacity ([Table 3] [Fig. 2]). This may be one reason why congenital FXII deficiency, as an autosomal recessive inherited disorder, tends to be diagnosed incidentally during routine coagulation testing, e.g., prior to surgery. Most of the reported F12 mutations result in a quantitative defect (cross-reacting material [CRM]-negative FXII deficiency) represented by a markedly reduced FXII activity (FXII:C) and antigen levels (FXII:Ag). However, a few genetic variations within the F12 gene are causative for a qualitative defect (CRM-positive FXII deficiency) indicated by a decreased FXII:C but nearly normal FXII:Ag.
|
Case no. |
Exon/Intron |
Genetic variation |
Comments |
Protein |
Condition |
c.-4 genotype |
FXII:C |
FXII:Ag |
Reference |
|---|---|---|---|---|---|---|---|---|---|
|
1 |
Exon 1 |
c.-13C > T |
5′ UTR |
– |
Heterozygous FXII deficiency |
C/T |
22% |
– |
[112] |
|
2 |
Exon 1 |
c.-13C > T |
5′ UTR |
– |
Compound heterozygous FXII deficiency; CRM-negative |
– |
< 1% |
< 1% |
[113] |
|
c.-8C > G |
5′ UTR |
– |
|||||||
|
3 |
Exon 1 |
c.-8C > G |
5′ UTR |
– |
Homozygous FXII deficiency |
T/T |
< 1% |
– |
[112] |
|
4 |
Exon 1 |
c.-8C > G |
5′ UTR |
– |
Homozygous FXII deficiency; CRM negative |
– |
< 1% |
1% |
|
|
Intron B |
c.116–224C > T |
TaqI restriction site |
– |
||||||
|
5 |
Exon 1 |
c.-8C > G |
5′ UTR |
– |
Compound heterozygous FXII deficiency; CRM-negative |
– |
< 1% |
< 1% |
[113] |
|
Exon 13 |
c.1558T > C |
Missense mutation |
p.Gln520* (Gln501*) |
||||||
|
6 |
Exon 1 |
c.-8C > G |
5′ UTR |
– |
Compound heterozygous FXII deficiency; CRM-negative |
– |
< 1% |
< 1% |
[113] |
|
Exon 14 |
c.1697C > T |
Missense mutation |
p.Pro566Leu (Pro547Leu) |
||||||
|
7 |
Exon 3 |
c.158A > G |
Missense mutation |
p.Tyr53Cys (Tyr34Cys) |
FXII Tenri, homozygous FXII deficiency; CRM-negative |
– |
3% |
3% |
[116] |
|
8 |
Exon 4 |
c.218G > C |
Missense mutation |
p.Cys73Ser (Cys54Ser) |
Heterozygous FXII deficiency |
T/T |
1% |
– |
|
|
9 |
Exon 4 |
c.249delG |
Frameshift mutation |
p.Gln83Hisfs*12 (Gln64Hisfs*12) |
Compound heterozygous FXII deficiency |
C/T |
< 0.5% |
– |
[119] |
|
Exon 6 |
c.405C > A |
Nonsense mutation |
p.Cys135* (Cys116*) |
||||||
|
10 |
Exon 4 |
c.251G > C |
Missense mutation |
p.Arg84Pro (Arg65Pro) |
Homozygous FXII deficiency |
T/T |
< 10% |
<17% |
[120] |
|
11 |
Exon 5 |
c.303_304delCA |
Frameshift mutation |
p.His101Glufs*36 (His82Glufs*36) |
Heterozygous carrier |
C/T |
39% |
41.6% |
[121] |
|
12 |
Exon 5 |
c.303_304delCA |
Frameshift mutation |
p.His101Glufs*36 (His82Glufs*36) |
Homozygous FXII deficiency |
T/T |
0% |
1.2% |
[121] |
|
13 |
Exon 6 |
c.405C > A |
Nonsense mutation |
p.Cys135* (Cys116*) |
Homozygous FXII deficiency |
T/T |
<0.5% |
– |
|
|
14 |
Exon 6 |
c.425G > C |
Missense mutation |
p.Arg142Pro (Arg123Pro) |
Homozygous FXII deficiency; CRM-negative |
T/T |
<1% |
<10% |
[123] |
|
15 |
Exon 7 |
c.583delC |
Frameshift mutation |
p.His195Thr*55 (His176Thr*55) |
Heterozygous carrier |
C/T |
53.4% |
– |
[118] |
|
16 |
Exon 7 |
c.583delC |
Frameshift mutation |
p.His195Thr*55 (His176Thr*55) |
Compound heterozygous FXII deficiency |
T/T |
<1% |
– |
[118] |
|
Exon 10 |
c.1092_1093insC |
Frameshift mutation |
p.Lys365fs*68 (Lys346fs*68) |
||||||
|
17 |
Exon 8 |
c.721T > G |
Missense mutation |
p.Trp241Gly (Trp222Gly) |
Heterozygous carrier |
– |
40% |
55% |
[124] |
|
18 |
Exon 8 |
c.721T > G |
Missense mutation |
p.Trp241Gly (Trp222Gly) |
Compound heterozygous FXII deficiency; CRM-negative |
– |
<3% |
<10% |
[124] |
|
Exon 12 |
c.1396C > A |
Missense mutation |
p.Arg466Ser (Arg447Ser) |
||||||
|
19 |
Exon 8 |
c.776G > A |
Missense mutation |
p. Gly259Glu (Gly240Glu) |
Homozygous FXII deficiency; CRM-negative |
C/C |
0.6% |
<1% |
[125] |
|
20 |
Exon 8 |
c.799C > G |
Missense mutation |
p.Arg267Gly (Arg248Gly) |
Homozygous FXII deficiency; CRM-negative |
C/C |
1.5% |
<1% |
[125] |
|
21 |
Exon 9 |
c.809_811delACA |
Deletion mutation |
p.Asn271del (Asn252del) |
Compound heterozygous FXII deficiency |
– |
2.0% |
5.2% |
[126] |
|
Exon 10 |
c.1078G > A |
Missense mutation |
p.Gly360Arg (Gly341Arg) |
||||||
|
22 |
Exon 9 |
c.856_864delAGCTGGGAG |
Frameshift mutation |
p.Ser286_Glu288 (Ser267_Glu269) |
Heterozygous FXII deficiency; CRM-negative |
T/T |
<1% |
<1% |
[127] |
|
23 |
Exon 10 |
c.1027G > C |
Missense mutation |
p.Ala343Pro (Ala324Pro) |
Heterozygous carrier |
T/T |
29% |
30% |
[128] |
|
24 |
Exon 10 |
c.1027G > C |
Missense mutation |
p.Ala343Pro (Ala324Pro) |
Compound heterozygous FXII deficiency; CRM-negative (Ala324Pro) and CRM-positive (Gly531Glu) |
T/C |
35% |
81% |
[128] |
|
Exon 13 |
c.1649G > A |
Missense mutation |
p.Gly550Glu (Gly531Glu) |
||||||
|
25 |
Exon 10 |
c.1078G > A |
Missense mutation |
p.Gly360Arg (Gly341Arg) |
Homozygous FXII deficiency |
T/T |
12% |
10% |
[129] |
|
26 |
Exon 10 |
c.1078G > A |
Missense mutation |
p.Gly360Arg (Gly341Arg) |
Heterozygous carrier |
C/T |
35% |
38% |
[129] |
|
27 |
Exon 10 |
c.1078G > A |
Missense mutation |
p.Gly360Arg (Gly341Arg) |
Compound heterozygous FXII deficiency |
– |
2.0% |
1.0% |
[126] |
|
Exon 13 |
c.1561G > A |
Missense mutation |
p.Glu521Lys (Glu502Lys) |
||||||
|
28 |
Exon 10 |
c.1093_1094insC |
Frameshift mutation |
p.Lys365fs*68 (Lys346fs*68) |
Heterozygous carrier |
T/T |
17.1% |
– |
[118] |
|
29 |
Exon 10 |
c.1092_1093insC |
Frameshift mutation |
p.Lys365Glnfs*69 (Lys346Glnfs*69) |
Compound heterozygous FXII deficiency |
C/T |
<0.5% |
– |
|
|
Exon 14 |
c.1744G > A |
Missense mutation |
p.Gly582Ser (Gly563Ser) |
||||||
|
30 |
Exon 10 |
c.1095G > C |
Missense mutation |
p.Lys365Asn (Lys346Asn) |
FXII Ofunato, CRM-reduced FXII deficiency |
T/T |
5% |
4.5% |
[130] |
|
31 |
Exon 10 |
c.1115G > C |
Missense mutation |
p.Arg372Pro (Arg353Pro) |
FXII Locarno, CRM-positive FXII deficiency |
– |
<1% |
46% |
|
|
32 |
Exon 10 |
c.1231G > A |
Missense mutation |
p.Ala411Thr (Ala392Thr) |
Factor XII Shizuoka, homozygous FXII deficiency; CRM-negative |
T/T |
<3% |
<10% |
[133] |
|
33 |
Exon 10 |
c.1240C > A |
Missense mutation |
p.Leu414Met (Leu395Met) |
Heterozygous carrier |
– |
<28% |
34% |
[115] |
|
34 |
Exon 10 |
c.1240C > A |
Missense mutation |
p.Leu414Met (Leu395Met) |
Compound heterozygous FXII deficiency; CRM-negative |
– |
<5% |
5% |
[115] |
|
Intron M |
c.1681–1G > A |
Acceptor splice site mutation |
– |
||||||
|
35 |
Exon 11 |
c.1318C > A |
Missense mutation |
p.Gln440Lys (Gln421Lys) |
Heterozygous carrier; CRM-negative |
C/T |
23% |
28% |
[123] |
|
36 |
Exon 12 |
c.1515G > C |
Missense mutation |
p.Trp505Cys (Trp486Cys) |
FXII Mie-1, homozygous FXII deficiency |
T/T |
<5% |
<5% |
[134] |
|
37 |
Exon 13 |
c.1561G > A |
Missense mutation |
p.Glu521Lys (Glu502Lys) |
Homozygous FXII deficiency; CRM-negative |
C/C |
4% |
3.8% |
[125] |
|
38 |
Exon 13 |
c.1561G > A |
Missense mutation |
p.Glu521Lys (Glu502Lys) |
Heterozygous carrier |
C/C |
34% |
33% |
[135] |
|
39 |
Exon 13 |
c.1561G > A |
Missense Mutation |
p.Glu521Lys (Glu502Lys) |
Compound heterozygous FXII deficiency; CRM-negative |
C/T |
4% |
5% |
[135] |
|
c.1637T > C |
Missense mutation |
p.Met546Thr (Met527Thr) |
|||||||
|
40 |
Exon 13 |
c.1583C > T |
Missense mutation |
p.Ser528Phe (Ser509Phe) |
Heterozygous carrier |
T/T |
29% |
– |
[122] |
|
41 |
Exon 13 |
c.1583C > T |
Missense mutation |
p.Ser528Phe (Ser509Phe) |
Compound heterozygous FXII deficiency |
T/T |
5% |
– |
|
|
Exon 14 |
c.1744G > A |
Missense mutation |
p.Gly582Ser (Gly563Ser) |
||||||
|
42 |
Exon 13 |
c.1637T > C |
Missense mutation |
p.Met546Thr (Met527Thr) |
Heterozygous carrier |
C/T |
30% |
32% |
[135] |
|
43 |
Exon 13 |
c.1669G > A |
Missense mutation |
p.Asp557Asn (Asp538Asn) |
Heterozygous FXII deficiency |
– |
5% |
6.8% |
[136] |
|
44 |
Intron M |
c.1681–1G > A |
Acceptor splice site mutation |
– |
Heterozygous carrier |
– |
<26% |
<40% |
[115] |
|
45 |
Intron M |
c.1681–1G > A |
Acceptor splice site mutation |
– |
Homozygous FXII deficiency; CRM-negative |
– |
<1% |
<1% |
|
|
46 |
Exon 14 |
c.1681G > A |
Missense mutation |
p.Gly561Ser (Gly542Ser) |
Homozygous FXII deficiency |
– |
<1% |
<1% |
[126] |
|
47 |
Exon 14 |
c.1765G > C |
Missense mutation |
p.Gly589Arg (Gly570Arg) |
Heterozygous carrier; CRM-positive |
– |
10% |
74% |
[115] |
|
48 |
Exon 14 |
c.1768T > A |
Missense mutation |
p.Cys590Ser (Cys571Ser) |
FXII Washington, CRM-positive FXII deficiency |
– |
<1% |
80% |
[138] |
|
49 |
Exon 14 |
c.1744G > A |
Missense mutation |
p.Gly582Ser (Gly563Ser) |
Heterozygous carrier |
T/T |
25% |
– |
[122] |
Abbreviations: CRM, cross-reacting material; FXII:C, factor XII activity; FXII:Ag, factor XII antigen levels.
Notes: Letter prefixes indicate the type of reference sequence: “c.”—coding DNA reference sequence (NM_000505.4), “p.”—protein reference sequence (NP_000496.2). The protein reference sequence contains an N-terminal signal peptide with a length of 19 amino acids. Changes in the amino acid sequence of the mature FXII protein are described in (parentheses). The c.-4 genotype indicates a C/T polymorphism localized in the 5′ untranslated region (5′ UTR) at nucleotide position four upstream of the translation initiation codon ATG. Nucleotide as well as amino acid changes are depicted as follows: “ > ”—substitution, “del”—deletion, “ins”—insertion, “fs”—frameshift, “*”—translation termination codon.
In addition to the F12 mutations described in [Table 3], a polymorphism in the 5′-untranslated region of F12 at nucleotide position four upstream of the translation initiation codon ATG (c.-4C > T, referred to as 46 C/T)[99] has additional implications for FXII:C and FXII:Ag. Transcriptional and translational analyses showed that this 46 T allele is associated with decreased translational efficiency compared with 46 C, resulting in low FXII:C and FXII:Ag.[99]
Reduced FXII levels may also be associated with the transfusion of blood cell or platelet concentrates.[100] Platelet activation and subsequent microparticle release occurs upon extended storage times,[101] which then drives FXII activation by exposure to PS and platelet membrane-bound polyP. Thus, reduced FXII levels appear as a consequence of zymogen “consumption” in patients receiving platelet concentrates.
Conclusion
Because of its selective role in thrombosis-sparing hemostasis, FXII has gained considerable interest as a target for safe anticoagulation over the last decades. In addition, FXII is a promising target for interference with proinflammatory BK-mediated responses. Contact activation of FXII is still incompletely understood, and identification of the “FXII contact activation site” will represent a major step forward. Detailed insight into the mechanism of FXII activation will help develop specific FXII contact inhibitors for potential clinical and diagnostic applications.
Conflict of Interest
The authors declare that they have no conflict of interest.
-
References
- 1 Long AT, Kenne E, Jung R, Fuchs TA, Renné T. Contact system revisited: an interface between inflammation, coagulation, and innate immunity. J Thromb Haemost 2016; 14 (03) 427-437
- 2 Renné T, Stavrou EX. Roles of factor XII in innate immunity. Front Immunol 2019; 10: 2011
- 3 Schmaier AH, Emsley J, Feener EP. et al. Nomenclature of factor XI and the contact system. J Thromb Haemost 2019; 17 (12) 2216-2219
- 4 Renné T, Schmaier AH, Nickel KF, Blombäck M, Maas C. In vivo roles of factor XII. Blood 2012; 120 (22) 4296-4303
- 5 Renné T, Pozgajová M, Grüner S. et al. Defective thrombus formation in mice lacking coagulation factor XII. J Exp Med 2005; 202 (02) 271-281
- 6 Grover SP, Olson TM, Cooley BC, Mackman N. Model-dependent contributions of FXII and FXI to venous thrombosis in mice. J Thromb Haemost 2020; 18 (11) 2899-2909
- 7 Kleinschnitz C, Stoll G, Bendszus M. et al. Targeting coagulation factor XII provides protection from pathological thrombosis in cerebral ischemia without interfering with hemostasis. J Exp Med 2006; 203 (03) 513-518
- 8 Müller F, Mutch NJ, Schenk WA. et al. Platelet polyphosphates are proinflammatory and procoagulant mediators in vivo. Cell 2009; 139 (06) 1143-1156
- 9 Nickel KF, Ronquist G, Langer F. et al. The polyphosphate-factor XII pathway drives coagulation in prostate cancer-associated thrombosis. Blood 2015; 126 (11) 1379-1389
- 10 Zilberman-Rudenko J, Reitsma SE, Puy C. et al. Factor XII activation promotes platelet consumption in the presence of bacterial-type long-chain polyphosphate in vitro and in vivo. Arterioscler Thromb Vasc Biol 2018; 38 (08) 1748-1760
- 11 Larsson M, Rayzman V, Nolte MW. et al. A factor XIIa inhibitory antibody provides thromboprotection in extracorporeal circulation without increasing bleeding risk. Sci Transl Med 2014; 6 (222) 222ra17
- 12 Matafonov A, Leung PY, Gailani AE. et al. Factor XII inhibition reduces thrombus formation in a primate thrombosis model. Blood 2014; 123 (11) 1739-1746
- 13 Davoine C, Bouckaert C, Fillet M, Pochet L. Factor XII/XIIa inhibitors: their discovery, development, and potential indications. Eur J Med Chem 2020; 208: 112753
- 14 Kenne E, Nickel KF, Long AT. et al. Factor XII: a novel target for safe prevention of thrombosis and inflammation. J Intern Med 2015; 278 (06) 571-585
- 15 Björkqvist J, Jämsä A, Renné T. Plasma kallikrein: the bradykinin-producing enzyme. Thromb Haemost 2013; 110 (03) 399-407
- 16 Ikeda Y, Hayashi I, Kamoshita E. et al. Host stromal bradykinin B2 receptor signaling facilitates tumor-associated angiogenesis and tumor growth. Cancer Res 2004; 64 (15) 5178-5185
- 17 Renné T, Schuh K, Müller-Esterl W. Local bradykinin formation is controlled by glycosaminoglycans. J Immunol 2005; 175 (05) 3377-3385
- 18 Benz PM, Blume C, Moebius J. et al. Cytoskeleton assembly at endothelial cell-cell contacts is regulated by alphaII-spectrin-VASP complexes. J Cell Biol 2008; 180 (01) 205-219
- 19 Benz PM, Blume C, Seifert S. et al. Differential VASP phosphorylation controls remodeling of the actin cytoskeleton. J Cell Sci 2009; 122 (Pt 21): 3954-3965
- 20 Anton KA, Sinclair J, Ohoka A. et al. PKA-regulated VASP phosphorylation promotes extrusion of transformed cells from the epithelium. J Cell Sci 2014; 127 (Pt 16): 3425-3433
- 21 Björkqvist J, Sala-Cunill A, Renné T. Hereditary angioedema: a bradykinin-mediated swelling disorder. Thromb Haemost 2013; 109 (03) 368-374
- 22 Maas C, Oschatz C, Renné T. The plasma contact system 2.0. Semin Thromb Hemost 2011; 37 (04) 375-381
- 23 Oschatz C, Maas C, Lecher B. et al. Mast cells increase vascular permeability by heparin-initiated bradykinin formation in vivo. Immunity 2011; 34 (02) 258-268
- 24 Stavrou EX, Fang C, Bane KL. et al. Factor XII and uPAR upregulate neutrophil functions to influence wound healing. J Clin Invest 2018; 128 (03) 944-959
- 25 Saito H, Ratnoff OD, Pensky J. Radioimmunoassay of human Hageman factor (factor XII). J Lab Clin Med 1976; 88 (03) 506-514
- 26 Saito H, Ishihara T, Suzuki H, Watanabe T. Production and characterization of a murine monoclonal antibody against a heavy chain of Hageman factor (factor XII). Blood 1985; 65 (05) 1263-1268
- 27 Clarke BJ, Côté HC, Cool DE. et al. Mapping of a putative surface-binding site of human coagulation factor XII. J Biol Chem 1989; 264 (19) 11497-11502
- 28 Citarella F, Fedele G, Roem D, Fantoni A, Hack CE. The second exon-encoded factor XII region is involved in the interaction of factor XII with factor XI and does not contribute to the binding site for negatively charged surfaces. Blood 1998; 92 (11) 4198-4206
- 29 Pixley RA, Stumpo LG, Birkmeyer K, Silver L, Colman RW. A monoclonal antibody recognizing an icosapeptide sequence in the heavy chain of human factor XII inhibits surface-catalyzed activation. J Biol Chem 1987; 262 (21) 10140-10145
- 30 Citarella F, te Velthuis H, Helmer-Citterich M, Hack CE. Identification of a putative binding site for negatively charged surfaces in the fibronectin type II domain of human factor XII--an immunochemical and homology modeling approach. Thromb Haemost 2000; 84 (06) 1057-1065
- 31 Citarella F, Aiuti A, La Porta C. et al. Control of human coagulation by recombinant serine proteases. Blood clotting is activated by recombinant factor XII deleted of five regulatory domains. Eur J Biochem 1992; 208 (01) 23-30
- 32 Citarella F, Ravon DM, Pascucci B, Felici A, Fantoni A, Hack CE. Structure/function analysis of human factor XII using recombinant deletion mutants. Evidence for an additional region involved in the binding to negatively charged surfaces. Eur J Biochem 1996; 238 (01) 240-249
- 33 Clark CC, Hofman ZLM, Sanrattana W, den Braven L, de Maat S, Maas C. The fibronectin type II domain of factor XII ensures zymogen quiescence. Thromb Haemost 2020; 120 (03) 400-411
- 34 Hofman ZLM, Clark CC, Sanrattana W. et al. A mutation in the kringle domain of human factor XII that causes autoinflammation, disturbs zymogen quiescence, and accelerates activation. J Biol Chem 2020; 295 (02) 363-374
- 35 Røjkaer R, Schousboe I. Partial identification of the Zn2+-binding sites in factor XII and its activation derivatives. Eur J Biochem 1997; 247 (02) 491-496
- 36 Chaudhry SA, Serrata M, Tomczak L. et al. Cationic zinc is required for factor XII recruitment and activation by stimulated platelets and for thrombus formation in vivo. J Thromb Haemost 2020; 18 (09) 2318-2328
- 37 Gordon EM, Venkatesan N, Salazar R. et al. Factor XII-induced mitogenesis is mediated via a distinct signal transduction pathway that activates a mitogen-activated protein kinase. Proc Natl Acad Sci U S A 1996; 93 (05) 2174-2179
- 38 LaRusch GA, Mahdi F, Shariat-Madar Z. et al. Factor XII stimulates ERK1/2 and Akt through uPAR, integrins, and the EGFR to initiate angiogenesis. Blood 2010; 115 (24) 5111-5120
- 39 Ghebrehiwet B, Lim BL, Peerschke EI, Willis AC, Reid KB. Isolation, cDNA cloning, and overexpression of a 33-kD cell surface glycoprotein that binds to the globular “heads” of C1q. J Exp Med 1994; 179 (06) 1809-1821
- 40 Joseph K, Ghebrehiwet B, Peerschke EI, Reid KB, Kaplan AP. Identification of the zinc-dependent endothelial cell binding protein for high molecular weight kininogen and factor XII: identity with the receptor that binds to the globular “heads” of C1q (gC1q-R). Proc Natl Acad Sci U S A 1996; 93 (16) 8552-8557
- 41 Feng X, Tonnesen MG, Peerschke EI, Ghebrehiwet B. Cooperation of C1q receptors and integrins in C1q-mediated endothelial cell adhesion and spreading. J Immunol 2002; 168 (05) 2441-2448
- 42 Kaira BG, Slater A, McCrae KR. et al. Factor XII and kininogen asymmetric assembly with gC1qR/C1QBP/P32 is governed by allostery. Blood 2020; 136 (14) 1685-1697
- 43 Dedio J, Jahnen-Dechent W, Bachmann M, Müller-Esterl W. The multiligand-binding protein gC1qR, putative C1q receptor, is a mitochondrial protein. J Immunol 1998; 160 (07) 3534-3542
- 44 Cichon S, Martin L, Hennies HC. et al. Increased activity of coagulation factor XII (Hageman factor) causes hereditary angioedema type III. Am J Hum Genet 2006; 79 (06) 1098-1104
- 45 Björkqvist J, de Maat S, Lewandrowski U. et al. Defective glycosylation of coagulation factor XII underlies hereditary angioedema type III. J Clin Invest 2015; 125 (08) 3132-3146
- 46 de Maat S, Björkqvist J, Suffritti C. et al. Plasmin is a natural trigger for bradykinin production in patients with hereditary angioedema with factor XII mutations. J Allergy Clin Immunol 2016; 138 (05) 1414-1423.e9
- 47 Bork K, Wulff K, Rossmann H. et al. Hereditary angioedema cosegregating with a novel kininogen 1 gene mutation changing the N-terminal cleavage site of bradykinin. Allergy 2019; 74 (12) 2479-2481
- 48 Bafunno V, Firinu D, D'Apolito M. et al. Mutation of the angiopoietin-1 gene (ANGPT1) associates with a new type of hereditary angioedema. J Allergy Clin Immunol 2018; 141 (03) 1009-1017
- 49 Bork K, Wulff K, Steinmüller-Magin L. et al. Hereditary angioedema with a mutation in the plasminogen gene. Allergy 2018; 73 (02) 442-450
- 50 Dewald G, Bork K. Missense mutations in the coagulation factor XII (Hageman factor) gene in hereditary angioedema with normal C1 inhibitor. Biochem Biophys Res Commun 2006; 343 (04) 1286-1289
- 51 Sala-Cunill A, Björkqvist J, Senter R. et al. Plasma contact system activation drives anaphylaxis in severe mast cell-mediated allergic reactions. J Allergy Clin Immunol 2015; 135 (04) 1031-1043.e6
- 52 Zamolodchikov D, Renné T, Strickland S. The Alzheimer's disease peptide β-amyloid promotes thrombin generation through activation of coagulation factor XII. J Thromb Haemost 2016; 14 (05) 995-1007
- 53 Zamolodchikov D, Chen ZL, Conti BA, Renné T, Strickland S. Activation of the factor XII-driven contact system in Alzheimer's disease patient and mouse model plasma. Proc Natl Acad Sci U S A 2015; 112 (13) 4068-4073
- 54 Bäck J, Sanchez J, Elgue G, Ekdahl KN, Nilsson B. Activated human platelets induce factor XIIa-mediated contact activation. Biochem Biophys Res Commun 2010; 391 (01) 11-17
- 55 Johne J, Blume C, Benz PM. et al. Platelets promote coagulation factor XII-mediated proteolytic cascade systems in plasma. Biol Chem 2006; 387 (02) 173-178
- 56 Walsh PN, Griffin JH. Contributions of human platelets to the proteolytic activation of blood coagulation factors XII and XI. Blood 1981; 57 (01) 106-118
- 57 Latour JG, McKay DG, Parrish MH. Activation of Hageman factor by cardiac arrest. Thromb Diath Haemorrh 1972; 27 (03) 543-553
- 58 Walsh PN. The role of platelets in the contact phase of blood coagulation. Br J Haematol 1972; 22 (02) 237-254
- 59 Castaldi PA, Larrieu MJ, Caen J. Availability of platelet factor 3 and activation of factor XII in thrombasthenia. Nature 1965; 207 (995) 422-424
- 60 Ruiz FA, Lea CR, Oldfield E, Docampo R. Human platelet dense granules contain polyphosphate and are similar to acidocalcisomes of bacteria and unicellular eukaryotes. J Biol Chem 2004; 279 (43) 44250-44257
- 61 Müller F, Renné T. Platelet polyphosphates: the nexus of primary and secondary hemostasis. Scand J Clin Lab Invest 2011; 71 (02) 82-86
- 62 Nickel KF, Spronk HM, Mutch NJ, Renné T. Time-dependent degradation and tissue factor addition mask the ability of platelet polyphosphates in activating factor XII-mediated coagulation. Blood 2013; 122 (23) 3847-3849
- 63
Labberton L,
Kenne E,
Long AT.
et al.
Neutralizing blood-borne polyphosphate in vivo provides safe thromboprotection. Nat
Commun 2016; 7: 12616
MissingFormLabel
- 64 Donovan AJ, Kalkowski J, Smith SA, Morrissey JH, Liu Y. Size-controlled synthesis of granular polyphosphate nanoparticles at physiologic salt concentrations for blood clotting. Biomacromolecules 2014; 15 (11) 3976-3984
- 65 Verhoef JJ, Barendrecht AD, Nickel KF. et al. Polyphosphate nanoparticles on the platelet surface trigger contact system activation. Blood 2017; 129 (12) 1707-1717
- 66 Smith SA, Choi SH, Davis-Harrison R. et al. Polyphosphate exerts differential effects on blood clotting, depending on polymer size. Blood 2010; 116 (20) 4353-4359
- 67 Werner TP, Amrhein N, Freimoser FM. Novel method for the quantification of inorganic polyphosphate (iPoP) in Saccharomyces cerevisiae shows dependence of iPoP content on the growth phase. Arch Microbiol 2005; 184 (02) 129-136
- 68 Mailer RKW, Hänel L, Allende M, Renné T. Polyphosphate as a target for interference with inflammation and thrombosis. Front Med (Lausanne) 2019; 6: 76
- 69 Norbis F, Boll M, Stange G. et al. Identification of a cDNA/protein leading to an increased Pi-uptake in Xenopus laevis oocytes. J Membr Biol 1997; 156 (01) 19-24
- 70 Auesukaree C, Tochio H, Shirakawa M, Kaneko Y, Harashima S. Plc1p, Arg82p, and Kcs1p, enzymes involved in inositol pyrophosphate synthesis, are essential for phosphate regulation and polyphosphate accumulation in Saccharomyces cerevisiae . J Biol Chem 2005; 280 (26) 25127-25133
- 71 Ghosh S, Shukla D, Suman K. et al. Inositol hexakisphosphate kinase 1 maintains hemostasis in mice by regulating platelet polyphosphate levels. Blood 2013; 122 (08) 1478-1486
- 72 Mailer RK, Allende M, Heestermans M. et al. Xenotropic and polytropic retrovirus receptor 1 regulates procoagulant platelet polyphosphate. Blood 2021; 137 (10) 1392-1405
- 73 Van Der Meijden PE, Van Schilfgaarde M, Van Oerle R, Renné T, ten Cate H, Spronk HM. Platelet- and erythrocyte-derived microparticles trigger thrombin generation via factor XIIa. J Thromb Haemost 2012; 10 (07) 1355-1362
- 74 Tripisciano C, Weiss R, Karuthedom George S, Fischer MB, Weber V. Extracellular vesicles derived from platelets, red blood cells, and monocyte-like cells differ regarding their ability to induce factor XII-dependent thrombin generation. Front Cell Dev Biol 2020; 8: 298
- 75 Noubouossie DF, Henderson MW, Mooberry M. et al. Red blood cell microvesicles activate the contact system, leading to factor IX activation via 2 independent pathways. Blood 2020; 135 (10) 755-765
- 76
Kearney KJ,
Butler J,
Posada OM.
et al.
Kallikrein directly interacts with and activates Factor IX, resulting in thrombin
generation and fibrin formation independent of Factor XI. Proc Natl Acad Sci U S A
2021; 118 (03) e2014810118
MissingFormLabel
- 77 Leventis PA, Grinstein S. The distribution and function of phosphatidylserine in cellular membranes. Annu Rev Biophys 2010; 39: 407-427
- 78 Yang A, Chen F, He C. et al. The Procoagulant activity of apoptotic cells is mediated by interaction with Factor XII. Front Immunol 2017; 8: 1188
- 79 Klein S, Spannagl M, Engelmann B. Phosphatidylethanolamine participates in the stimulation of the contact system of coagulation by very-low-density lipoproteins. Arterioscler Thromb Vasc Biol 2001; 21 (10) 1695-1700
- 80 Zhu S, Diamond SL. Contact activation of blood coagulation on a defined kaolin/collagen surface in a microfluidic assay. Thromb Res 2014; 134 (06) 1335-1343
- 81 Otrocka-Domagała I, Jastrzębski P, Adamiak Z. et al. Safety of the long-term application of QuikClot Combat Gauze, ChitoGauze PRO and Celox Gauze in a femoral artery injury model in swine - a preliminary study. Pol J Vet Sci 2016; 19 (02) 337-343
- 82 Juang LJ, Mazinani N, Novakowski SK. et al. Coagulation factor XII contributes to hemostasis when activated by soil in wounds. Blood Adv 2020; 4 (08) 1737-1745
- 83 Robinson AJ, Kropatkin M, Aggeler PM. Hageman factor (factor XII) deficiency in marine mammals. Science 1969; 166 (3911): 1420-1422
- 84 Doolittle RF. Step-by-step evolution of vertebrate blood coagulation. Cold Spring Harb Symp Quant Biol 2009; 74: 35-40
- 85 Forbes GL, Merkulova A, Pinheiro A. et al. Poly (acrylic acid) (PAA) is a contact system activator with properties to stop hemorrhage. Thromb Res 2020; 193: 142-145
- 86 Tans G, Griffin JH. Properties of sulfatides in factor-XII-dependent contact activation. Blood 1982; 59 (01) 69-75
- 87 España F, Ratnoff OD. The role of prekallikrein and high-molecular-weight kininogen in the contact activation of Hageman factor (factor XII) by sulfatides and other agents. J Lab Clin Med 1983; 102 (04) 487-499
- 88 Bock PE, Srinivasan KR, Shore JD. Activation of intrinsic blood coagulation by ellagic acid: insoluble ellagic acid-metal ion complexes are the activating species. Biochemistry 1981; 20 (25) 7258-7266
- 89 Girolami A, Cliffton EE. Hypercoagulable state induced in humans by the intravenous administration of purified ellagic acid. Thromb Diath Haemorrh 1967; 17 (1-2): 165-175
- 90 Samuel M, Pixley RA, Villanueva MA, Colman RW, Villanueva GB. Human factor XII (Hageman factor) autoactivation by dextran sulfate. Circular dichroism, fluorescence, and ultraviolet difference spectroscopic studies. J Biol Chem 1992; 267 (27) 19691-19697
- 91 Siebeck M, Cheronis JC, Fink E. et al. Dextran sulfate activates contact system and mediates arterial hypotension via B2 kinin receptors. J Appl Physiol (1985) 1994; 77 (06) 2675-2680
- 92 Björkqvist J, Lecher B, Maas C, Renné T. Zinc-dependent contact system activation induces vascular leakage and hypotension in rodents. Biol Chem 2013; 394 (09) 1195-1204
- 93 Corbier A, Le Berre N, Rampe D. et al. Oversulfated chondroitin sulfate and OSCS-contaminated heparin cause dose- and route-dependent hemodynamic effects in the rat. Toxicol Sci 2011; 121 (02) 417-427
- 94 Guerrini M, Beccati D, Shriver Z. et al. Oversulfated chondroitin sulfate is a contaminant in heparin associated with adverse clinical events. Nat Biotechnol 2008; 26 (06) 669-675
- 95 Lin L, Xu L, Xiao C. et al. Plasma contact activation by a fucosylated chondroitin sulfate and its structure-activity relationship study. Glycobiology 2018; 28 (10) 754-764
- 96 Sperling C, Maitz MF, Grasso S, Werner C, Kanse SM. A positively charged surface triggers coagulation activation through Factor VII activating protease (FSAP). ACS Appl Mater Interfaces 2017; 9 (46) 40107-40116
- 97 Weiss AS, Gallin JI, Kaplan AP. Fletcher factor deficiency. A diminished rate of Hageman factor activation caused by absence of prekallikrein with abnormalities of coagulation, fibrinolysis, chemotactic activity, and kinin generation. J Clin Invest 1974; 53 (02) 622-633
- 98 Bork K, Witzke G. Shortened activated partial thromboplastin time may help in diagnosing hereditary and acquired angioedema. Int Arch Allergy Immunol 2016; 170 (02) 101-107
- 99 Kanaji T, Okamura T, Osaki K. et al. A common genetic polymorphism (46 C to T substitution) in the 5′-untranslated region of the coagulation factor XII gene is associated with low translation efficiency and decrease in plasma factor XII level. Blood 1998; 91 (06) 2010-2014
- 100 Bachler M, Niederwanger C, Hell T. et al. Influence of factor XII deficiency on activated partial thromboplastin time (aPTT) in critically ill patients. J Thromb Thrombolysis 2019; 48 (03) 466-474
- 101 Marcoux G, Duchez AC, Rousseau M. et al. Microparticle and mitochondrial release during extended storage of different types of platelet concentrates. Platelets 2017; 28 (03) 272-280
- 102 McMullen BA, Fujikawa K. Amino acid sequence of the heavy chain of human alpha-factor XIIa (activated Hageman factor). J Biol Chem 1985; 260 (09) 5328-5341
- 103 Schousboe I. Contact activation in human plasma is triggered by zinc ion modulation of factor XII (Hageman factor). Blood Coagul Fibrinolysis 1993; 4 (05) 671-678
- 104 Mahdi F, Madar ZS, Figueroa CD, Schmaier AH. Factor XII interacts with the multiprotein assembly of urokinase plasminogen activator receptor, gC1qR, and cytokeratin 1 on endothelial cell membranes. Blood 2002; 99 (10) 3585-3596
- 105 Yamada KM. Cell surface interactions with extracellular materials. Annu Rev Biochem 1983; 52: 761-799
- 106 Cool DE, MacGillivray RT. Characterization of the human blood coagulation factor XII gene. Intron/exon gene organization and analysis of the 5′-flanking region. J Biol Chem 1987; 262 (28) 13662-13673
- 107 Harris RJ, Ling VT, Spellman MW. O-linked fucose is present in the first epidermal growth factor domain of factor XII but not protein C. J Biol Chem 1992; 267 (08) 5102-5107
- 108 Liu T, Qian WJ, Gritsenko MA. et al. Human plasma N-glycoproteome analysis by immunoaffinity subtraction, hydrazide chemistry, and mass spectrometry. J Proteome Res 2005; 4 (06) 2070-2080
- 109 López-Gálvez R, de la Morena-Barrio ME, López-Lera A. et al. Factor XII in PMM2-CDG patients: role of N-glycosylation in the secretion and function of the first element of the contact pathway. Orphanet J Rare Dis 2020; 15 (01) 280
- 110 Bunkenborg J, Pilch BJ, Podtelejnikov AV, Wiśniewski JR. Screening for N-glycosylated proteins by liquid chromatography mass spectrometry. Proteomics 2004; 4 (02) 454-465
- 111 Naudin C, Burillo E, Blankenberg S, Butler L, Renné T. Factor XII contact activation. Semin Thromb Hemost 2017; 43 (08) 814-826
- 112 Sabater-Lleal M, Chillón M, Mordillo C. et al. Combined cis-regulator elements as important mechanism affecting FXII plasma levels. Thromb Res 2010; 125 (02) e55-e60
- 113 Lombardi AM, Bortoletto E, Scarparo P, Scapin M, Santarossa L, Girolami A. Genetic study in patients with factor XII deficiency: a report of three new mutations exon 13 (Q501STOP), exon 14 (P547L) and -13C>T promoter region in three compound heterozygotes. Blood Coagul Fibrinolysis 2008; 19 (07) 639-643
- 114 Hofferbert S, Müller J, Köstering H, von Ohlen WD, Schloesser M. A novel 5′-upstream mutation in the factor XII gene is associated with a TaqI restriction site in an Alu repeat in factor XII-deficient patients. Hum Genet 1996; 97 (06) 838-841
- 115 Schloesser M, Zeerleder S, Lutze G. et al. Mutations in the human factor XII gene. Blood 1997; 90 (10) 3967-3977
- 116 Kondo S, Tokunaga F, Kawano S, Oono Y, Kumagai S, Koide T. Factor XII Tenri, a novel cross-reacting material negative factor XII deficiency, occurs through a proteasome-mediated degradation. Blood 1999; 93 (12) 4300-4308
- 117 Feng Y, Ye X, Pang Y, Dai J, Wang XF, Zhou XH. A novel mutation in a patient with congenital coagulation factor XII deficiency. Chin Med J (Engl) 2008; 121 (13) 1241-1244
- 118 Singhamatr P, Kanjanapongkul S, Rojnuckarin P. Molecular analysis of factor XII gene in Thai patients with factor XII deficiency. Blood Coagul Fibrinolysis 2013; 24 (06) 599-604
- 119 Kim HJ, Kim HJ, Kwon EH, Lee KO, Park IA, Kim SH. Novel deleterious mutation in the F12 gene in a Korean family with severe coagulation factor XII deficiency. Blood Coagul Fibrinolysis 2010; 21 (07) 683-686
- 120 Matsuki E, Miyakawa Y, Okamoto S. A novel factor XII mutation, FXII R84P, causing factor XII deficiency in a patient with hereditary spastic paraplegia. Blood Coagul Fibrinolysis 2011; 22 (03) 227-230
- 121 Ye X, Feng Y, Ding Q, Dai J, Wang X. Genetic analysis of a pedigree with combined factor XII and factor XI deficiency. Blood Coagul Fibrinolysis 2011; 22 (02) 118-122
- 122 Kwon MJ, Kim HJ, Lee KO, Jung CW, Kim SH. Molecular genetic analysis of Korean patients with coagulation factor XII deficiency. Blood Coagul Fibrinolysis 2010; 21 (04) 308-312
- 123 Kanaji T, Kanaji S, Osaki K. et al. Identification and characterization of two novel mutations (Q421 K and R123P) in congenital factor XII deficiency. Thromb Haemost 2001; 86 (06) 1409-1415
- 124 Matsukuma E, Gotoh Y, Kuroyanagi Y. et al. A case of atypical hemolytic uremic syndrome due to anti-factor H antibody in a patient presenting with a factor XII deficiency identified two novel mutations. Clin Exp Nephrol 2011; 15 (02) 269-274
- 125 Jin P, Jiang W, Yan H. et al. Novel mutations in congenital factor XII deficiency. Front Biosci 2016; 21: 419-429
- 126 Yang L, Wang Y, Zhou J. et al. Identification of genetic defects underlying FXII deficiency in four unrelated Chinese patients. Acta Haematol 2016; 135 (04) 238-240
- 127 Xie H, Lv M, Yang X. et al. [Identification of a novel mutation of factor XII gene in a family with coagulation FXII deficiency]. Zhonghua Yi Xue Yi Chuan Xue Za Zhi 2013; 30 (03) 313-317
- 128 Iijima K, Arakawa Y, Sugahara Y. et al. Factor XII Osaka: abnormal factor XII with partially defective prekallikrein cleavage activity. Thromb Haemost 2011; 105 (03) 473-478
- 129 Cheng X, Yang L, Huang G, Jin Y, Hao X, Wang M. Genetic analysis of a hereditary factor XII deficiency pedigree of a consanguineous marriage due to a homozygous F12 gene mutation: Gly341Arg. Hematology 2017; 22 (05) 310-315
- 130 Suzuki K, Murai K, Suwabe A, Ishida Y. Factor XII Ofunato: Lys346Asn mutation associated with blood coagulation factor XII deficiency causes impaired secretion through a proteasome-mediated degradation. Thromb Res 2010; 125 (05) 438-443
- 131 Wuillemin WA, Furlan M, Stricker H, Lämmle B. Functional characterization of a variant factor XII (F XII Locarno) in a cross reacting material positive F XII deficient plasma. Thromb Haemost 1992; 67 (02) 219-225
- 132 Hovinga JK, Schaller J, Stricker H, Wuillemin WA, Furlan M, Lämmle B. Coagulation factor XII Locarno: the functional defect is caused by the amino acid substitution Arg 353-->Pro leading to loss of a kallikrein cleavage site. Blood 1994; 84 (04) 1173-1181
- 133 Oguchi S, Ishii K, Moriki T. et al. Factor XII Shizuoka, a novel mutation (Ala392Thr) identified and characterized in a patient with congenital coagulation factor XII deficiency. Thromb Res 2005; 115 (03) 191-197
- 134 Wada H, Nishioka J, Kasai Y. et al. Molecular characterization of coagulation factor XII deficiency in a Japanese family. Thromb Haemost 2003; 90 (01) 59-63
- 135 Zhang H, Liu S, Lin C. et al. Compound heterozygous mutations Glu502Lys and Met527Thr of the FXII gene in a patient with factor XII deficiency. Hematology 2019; 24 (01) 420-425
- 136 Li M, Xie H, Wang M, Ding H. Molecular characterization of a novel missense mutation (Asp538Asn) in a Chinese patient with factor XII deficiency. Clin Lab 2015; 61 (12) 1967-1971
- 137 Schloesser M, Hofferbert S, Bartz U, Lutze G, Lämmle B, Engel W. The novel acceptor splice site mutation 11396(G-->A) in the factor XII gene causes a truncated transcript in cross-reacting material negative patients. Hum Mol Genet 1995; 4 (07) 1235-1237
- 138 Miyata T, Kawabata S, Iwanaga S, Takahashi I, Alving B, Saito H. Coagulation factor XII (Hageman factor) Washington D.C.: inactive factor XIIa results from Cys-571----Ser substitution. Proc Natl Acad Sci U S A 1989; 86 (21) 8319-8322
Address for correspondence
Publication History
Received: 17 January 2021
Accepted: 11 June 2021
Article published online:
30 September 2021
© 2021. Thieme. All rights reserved.
Georg Thieme Verlag KG
Rüdigerstraße 14, 70469 Stuttgart, Germany
-
References
- 1 Long AT, Kenne E, Jung R, Fuchs TA, Renné T. Contact system revisited: an interface between inflammation, coagulation, and innate immunity. J Thromb Haemost 2016; 14 (03) 427-437
- 2 Renné T, Stavrou EX. Roles of factor XII in innate immunity. Front Immunol 2019; 10: 2011
- 3 Schmaier AH, Emsley J, Feener EP. et al. Nomenclature of factor XI and the contact system. J Thromb Haemost 2019; 17 (12) 2216-2219
- 4 Renné T, Schmaier AH, Nickel KF, Blombäck M, Maas C. In vivo roles of factor XII. Blood 2012; 120 (22) 4296-4303
- 5 Renné T, Pozgajová M, Grüner S. et al. Defective thrombus formation in mice lacking coagulation factor XII. J Exp Med 2005; 202 (02) 271-281
- 6 Grover SP, Olson TM, Cooley BC, Mackman N. Model-dependent contributions of FXII and FXI to venous thrombosis in mice. J Thromb Haemost 2020; 18 (11) 2899-2909
- 7 Kleinschnitz C, Stoll G, Bendszus M. et al. Targeting coagulation factor XII provides protection from pathological thrombosis in cerebral ischemia without interfering with hemostasis. J Exp Med 2006; 203 (03) 513-518
- 8 Müller F, Mutch NJ, Schenk WA. et al. Platelet polyphosphates are proinflammatory and procoagulant mediators in vivo. Cell 2009; 139 (06) 1143-1156
- 9 Nickel KF, Ronquist G, Langer F. et al. The polyphosphate-factor XII pathway drives coagulation in prostate cancer-associated thrombosis. Blood 2015; 126 (11) 1379-1389
- 10 Zilberman-Rudenko J, Reitsma SE, Puy C. et al. Factor XII activation promotes platelet consumption in the presence of bacterial-type long-chain polyphosphate in vitro and in vivo. Arterioscler Thromb Vasc Biol 2018; 38 (08) 1748-1760
- 11 Larsson M, Rayzman V, Nolte MW. et al. A factor XIIa inhibitory antibody provides thromboprotection in extracorporeal circulation without increasing bleeding risk. Sci Transl Med 2014; 6 (222) 222ra17
- 12 Matafonov A, Leung PY, Gailani AE. et al. Factor XII inhibition reduces thrombus formation in a primate thrombosis model. Blood 2014; 123 (11) 1739-1746
- 13 Davoine C, Bouckaert C, Fillet M, Pochet L. Factor XII/XIIa inhibitors: their discovery, development, and potential indications. Eur J Med Chem 2020; 208: 112753
- 14 Kenne E, Nickel KF, Long AT. et al. Factor XII: a novel target for safe prevention of thrombosis and inflammation. J Intern Med 2015; 278 (06) 571-585
- 15 Björkqvist J, Jämsä A, Renné T. Plasma kallikrein: the bradykinin-producing enzyme. Thromb Haemost 2013; 110 (03) 399-407
- 16 Ikeda Y, Hayashi I, Kamoshita E. et al. Host stromal bradykinin B2 receptor signaling facilitates tumor-associated angiogenesis and tumor growth. Cancer Res 2004; 64 (15) 5178-5185
- 17 Renné T, Schuh K, Müller-Esterl W. Local bradykinin formation is controlled by glycosaminoglycans. J Immunol 2005; 175 (05) 3377-3385
- 18 Benz PM, Blume C, Moebius J. et al. Cytoskeleton assembly at endothelial cell-cell contacts is regulated by alphaII-spectrin-VASP complexes. J Cell Biol 2008; 180 (01) 205-219
- 19 Benz PM, Blume C, Seifert S. et al. Differential VASP phosphorylation controls remodeling of the actin cytoskeleton. J Cell Sci 2009; 122 (Pt 21): 3954-3965
- 20 Anton KA, Sinclair J, Ohoka A. et al. PKA-regulated VASP phosphorylation promotes extrusion of transformed cells from the epithelium. J Cell Sci 2014; 127 (Pt 16): 3425-3433
- 21 Björkqvist J, Sala-Cunill A, Renné T. Hereditary angioedema: a bradykinin-mediated swelling disorder. Thromb Haemost 2013; 109 (03) 368-374
- 22 Maas C, Oschatz C, Renné T. The plasma contact system 2.0. Semin Thromb Hemost 2011; 37 (04) 375-381
- 23 Oschatz C, Maas C, Lecher B. et al. Mast cells increase vascular permeability by heparin-initiated bradykinin formation in vivo. Immunity 2011; 34 (02) 258-268
- 24 Stavrou EX, Fang C, Bane KL. et al. Factor XII and uPAR upregulate neutrophil functions to influence wound healing. J Clin Invest 2018; 128 (03) 944-959
- 25 Saito H, Ratnoff OD, Pensky J. Radioimmunoassay of human Hageman factor (factor XII). J Lab Clin Med 1976; 88 (03) 506-514
- 26 Saito H, Ishihara T, Suzuki H, Watanabe T. Production and characterization of a murine monoclonal antibody against a heavy chain of Hageman factor (factor XII). Blood 1985; 65 (05) 1263-1268
- 27 Clarke BJ, Côté HC, Cool DE. et al. Mapping of a putative surface-binding site of human coagulation factor XII. J Biol Chem 1989; 264 (19) 11497-11502
- 28 Citarella F, Fedele G, Roem D, Fantoni A, Hack CE. The second exon-encoded factor XII region is involved in the interaction of factor XII with factor XI and does not contribute to the binding site for negatively charged surfaces. Blood 1998; 92 (11) 4198-4206
- 29 Pixley RA, Stumpo LG, Birkmeyer K, Silver L, Colman RW. A monoclonal antibody recognizing an icosapeptide sequence in the heavy chain of human factor XII inhibits surface-catalyzed activation. J Biol Chem 1987; 262 (21) 10140-10145
- 30 Citarella F, te Velthuis H, Helmer-Citterich M, Hack CE. Identification of a putative binding site for negatively charged surfaces in the fibronectin type II domain of human factor XII--an immunochemical and homology modeling approach. Thromb Haemost 2000; 84 (06) 1057-1065
- 31 Citarella F, Aiuti A, La Porta C. et al. Control of human coagulation by recombinant serine proteases. Blood clotting is activated by recombinant factor XII deleted of five regulatory domains. Eur J Biochem 1992; 208 (01) 23-30
- 32 Citarella F, Ravon DM, Pascucci B, Felici A, Fantoni A, Hack CE. Structure/function analysis of human factor XII using recombinant deletion mutants. Evidence for an additional region involved in the binding to negatively charged surfaces. Eur J Biochem 1996; 238 (01) 240-249
- 33 Clark CC, Hofman ZLM, Sanrattana W, den Braven L, de Maat S, Maas C. The fibronectin type II domain of factor XII ensures zymogen quiescence. Thromb Haemost 2020; 120 (03) 400-411
- 34 Hofman ZLM, Clark CC, Sanrattana W. et al. A mutation in the kringle domain of human factor XII that causes autoinflammation, disturbs zymogen quiescence, and accelerates activation. J Biol Chem 2020; 295 (02) 363-374
- 35 Røjkaer R, Schousboe I. Partial identification of the Zn2+-binding sites in factor XII and its activation derivatives. Eur J Biochem 1997; 247 (02) 491-496
- 36 Chaudhry SA, Serrata M, Tomczak L. et al. Cationic zinc is required for factor XII recruitment and activation by stimulated platelets and for thrombus formation in vivo. J Thromb Haemost 2020; 18 (09) 2318-2328
- 37 Gordon EM, Venkatesan N, Salazar R. et al. Factor XII-induced mitogenesis is mediated via a distinct signal transduction pathway that activates a mitogen-activated protein kinase. Proc Natl Acad Sci U S A 1996; 93 (05) 2174-2179
- 38 LaRusch GA, Mahdi F, Shariat-Madar Z. et al. Factor XII stimulates ERK1/2 and Akt through uPAR, integrins, and the EGFR to initiate angiogenesis. Blood 2010; 115 (24) 5111-5120
- 39 Ghebrehiwet B, Lim BL, Peerschke EI, Willis AC, Reid KB. Isolation, cDNA cloning, and overexpression of a 33-kD cell surface glycoprotein that binds to the globular “heads” of C1q. J Exp Med 1994; 179 (06) 1809-1821
- 40 Joseph K, Ghebrehiwet B, Peerschke EI, Reid KB, Kaplan AP. Identification of the zinc-dependent endothelial cell binding protein for high molecular weight kininogen and factor XII: identity with the receptor that binds to the globular “heads” of C1q (gC1q-R). Proc Natl Acad Sci U S A 1996; 93 (16) 8552-8557
- 41 Feng X, Tonnesen MG, Peerschke EI, Ghebrehiwet B. Cooperation of C1q receptors and integrins in C1q-mediated endothelial cell adhesion and spreading. J Immunol 2002; 168 (05) 2441-2448
- 42 Kaira BG, Slater A, McCrae KR. et al. Factor XII and kininogen asymmetric assembly with gC1qR/C1QBP/P32 is governed by allostery. Blood 2020; 136 (14) 1685-1697
- 43 Dedio J, Jahnen-Dechent W, Bachmann M, Müller-Esterl W. The multiligand-binding protein gC1qR, putative C1q receptor, is a mitochondrial protein. J Immunol 1998; 160 (07) 3534-3542
- 44 Cichon S, Martin L, Hennies HC. et al. Increased activity of coagulation factor XII (Hageman factor) causes hereditary angioedema type III. Am J Hum Genet 2006; 79 (06) 1098-1104
- 45 Björkqvist J, de Maat S, Lewandrowski U. et al. Defective glycosylation of coagulation factor XII underlies hereditary angioedema type III. J Clin Invest 2015; 125 (08) 3132-3146
- 46 de Maat S, Björkqvist J, Suffritti C. et al. Plasmin is a natural trigger for bradykinin production in patients with hereditary angioedema with factor XII mutations. J Allergy Clin Immunol 2016; 138 (05) 1414-1423.e9
- 47 Bork K, Wulff K, Rossmann H. et al. Hereditary angioedema cosegregating with a novel kininogen 1 gene mutation changing the N-terminal cleavage site of bradykinin. Allergy 2019; 74 (12) 2479-2481
- 48 Bafunno V, Firinu D, D'Apolito M. et al. Mutation of the angiopoietin-1 gene (ANGPT1) associates with a new type of hereditary angioedema. J Allergy Clin Immunol 2018; 141 (03) 1009-1017
- 49 Bork K, Wulff K, Steinmüller-Magin L. et al. Hereditary angioedema with a mutation in the plasminogen gene. Allergy 2018; 73 (02) 442-450
- 50 Dewald G, Bork K. Missense mutations in the coagulation factor XII (Hageman factor) gene in hereditary angioedema with normal C1 inhibitor. Biochem Biophys Res Commun 2006; 343 (04) 1286-1289
- 51 Sala-Cunill A, Björkqvist J, Senter R. et al. Plasma contact system activation drives anaphylaxis in severe mast cell-mediated allergic reactions. J Allergy Clin Immunol 2015; 135 (04) 1031-1043.e6
- 52 Zamolodchikov D, Renné T, Strickland S. The Alzheimer's disease peptide β-amyloid promotes thrombin generation through activation of coagulation factor XII. J Thromb Haemost 2016; 14 (05) 995-1007
- 53 Zamolodchikov D, Chen ZL, Conti BA, Renné T, Strickland S. Activation of the factor XII-driven contact system in Alzheimer's disease patient and mouse model plasma. Proc Natl Acad Sci U S A 2015; 112 (13) 4068-4073
- 54 Bäck J, Sanchez J, Elgue G, Ekdahl KN, Nilsson B. Activated human platelets induce factor XIIa-mediated contact activation. Biochem Biophys Res Commun 2010; 391 (01) 11-17
- 55 Johne J, Blume C, Benz PM. et al. Platelets promote coagulation factor XII-mediated proteolytic cascade systems in plasma. Biol Chem 2006; 387 (02) 173-178
- 56 Walsh PN, Griffin JH. Contributions of human platelets to the proteolytic activation of blood coagulation factors XII and XI. Blood 1981; 57 (01) 106-118
- 57 Latour JG, McKay DG, Parrish MH. Activation of Hageman factor by cardiac arrest. Thromb Diath Haemorrh 1972; 27 (03) 543-553
- 58 Walsh PN. The role of platelets in the contact phase of blood coagulation. Br J Haematol 1972; 22 (02) 237-254
- 59 Castaldi PA, Larrieu MJ, Caen J. Availability of platelet factor 3 and activation of factor XII in thrombasthenia. Nature 1965; 207 (995) 422-424
- 60 Ruiz FA, Lea CR, Oldfield E, Docampo R. Human platelet dense granules contain polyphosphate and are similar to acidocalcisomes of bacteria and unicellular eukaryotes. J Biol Chem 2004; 279 (43) 44250-44257
- 61 Müller F, Renné T. Platelet polyphosphates: the nexus of primary and secondary hemostasis. Scand J Clin Lab Invest 2011; 71 (02) 82-86
- 62 Nickel KF, Spronk HM, Mutch NJ, Renné T. Time-dependent degradation and tissue factor addition mask the ability of platelet polyphosphates in activating factor XII-mediated coagulation. Blood 2013; 122 (23) 3847-3849
- 63
Labberton L,
Kenne E,
Long AT.
et al.
Neutralizing blood-borne polyphosphate in vivo provides safe thromboprotection. Nat
Commun 2016; 7: 12616
MissingFormLabel
- 64 Donovan AJ, Kalkowski J, Smith SA, Morrissey JH, Liu Y. Size-controlled synthesis of granular polyphosphate nanoparticles at physiologic salt concentrations for blood clotting. Biomacromolecules 2014; 15 (11) 3976-3984
- 65 Verhoef JJ, Barendrecht AD, Nickel KF. et al. Polyphosphate nanoparticles on the platelet surface trigger contact system activation. Blood 2017; 129 (12) 1707-1717
- 66 Smith SA, Choi SH, Davis-Harrison R. et al. Polyphosphate exerts differential effects on blood clotting, depending on polymer size. Blood 2010; 116 (20) 4353-4359
- 67 Werner TP, Amrhein N, Freimoser FM. Novel method for the quantification of inorganic polyphosphate (iPoP) in Saccharomyces cerevisiae shows dependence of iPoP content on the growth phase. Arch Microbiol 2005; 184 (02) 129-136
- 68 Mailer RKW, Hänel L, Allende M, Renné T. Polyphosphate as a target for interference with inflammation and thrombosis. Front Med (Lausanne) 2019; 6: 76
- 69 Norbis F, Boll M, Stange G. et al. Identification of a cDNA/protein leading to an increased Pi-uptake in Xenopus laevis oocytes. J Membr Biol 1997; 156 (01) 19-24
- 70 Auesukaree C, Tochio H, Shirakawa M, Kaneko Y, Harashima S. Plc1p, Arg82p, and Kcs1p, enzymes involved in inositol pyrophosphate synthesis, are essential for phosphate regulation and polyphosphate accumulation in Saccharomyces cerevisiae . J Biol Chem 2005; 280 (26) 25127-25133
- 71 Ghosh S, Shukla D, Suman K. et al. Inositol hexakisphosphate kinase 1 maintains hemostasis in mice by regulating platelet polyphosphate levels. Blood 2013; 122 (08) 1478-1486
- 72 Mailer RK, Allende M, Heestermans M. et al. Xenotropic and polytropic retrovirus receptor 1 regulates procoagulant platelet polyphosphate. Blood 2021; 137 (10) 1392-1405
- 73 Van Der Meijden PE, Van Schilfgaarde M, Van Oerle R, Renné T, ten Cate H, Spronk HM. Platelet- and erythrocyte-derived microparticles trigger thrombin generation via factor XIIa. J Thromb Haemost 2012; 10 (07) 1355-1362
- 74 Tripisciano C, Weiss R, Karuthedom George S, Fischer MB, Weber V. Extracellular vesicles derived from platelets, red blood cells, and monocyte-like cells differ regarding their ability to induce factor XII-dependent thrombin generation. Front Cell Dev Biol 2020; 8: 298
- 75 Noubouossie DF, Henderson MW, Mooberry M. et al. Red blood cell microvesicles activate the contact system, leading to factor IX activation via 2 independent pathways. Blood 2020; 135 (10) 755-765
- 76
Kearney KJ,
Butler J,
Posada OM.
et al.
Kallikrein directly interacts with and activates Factor IX, resulting in thrombin
generation and fibrin formation independent of Factor XI. Proc Natl Acad Sci U S A
2021; 118 (03) e2014810118
MissingFormLabel
- 77 Leventis PA, Grinstein S. The distribution and function of phosphatidylserine in cellular membranes. Annu Rev Biophys 2010; 39: 407-427
- 78 Yang A, Chen F, He C. et al. The Procoagulant activity of apoptotic cells is mediated by interaction with Factor XII. Front Immunol 2017; 8: 1188
- 79 Klein S, Spannagl M, Engelmann B. Phosphatidylethanolamine participates in the stimulation of the contact system of coagulation by very-low-density lipoproteins. Arterioscler Thromb Vasc Biol 2001; 21 (10) 1695-1700
- 80 Zhu S, Diamond SL. Contact activation of blood coagulation on a defined kaolin/collagen surface in a microfluidic assay. Thromb Res 2014; 134 (06) 1335-1343
- 81 Otrocka-Domagała I, Jastrzębski P, Adamiak Z. et al. Safety of the long-term application of QuikClot Combat Gauze, ChitoGauze PRO and Celox Gauze in a femoral artery injury model in swine - a preliminary study. Pol J Vet Sci 2016; 19 (02) 337-343
- 82 Juang LJ, Mazinani N, Novakowski SK. et al. Coagulation factor XII contributes to hemostasis when activated by soil in wounds. Blood Adv 2020; 4 (08) 1737-1745
- 83 Robinson AJ, Kropatkin M, Aggeler PM. Hageman factor (factor XII) deficiency in marine mammals. Science 1969; 166 (3911): 1420-1422
- 84 Doolittle RF. Step-by-step evolution of vertebrate blood coagulation. Cold Spring Harb Symp Quant Biol 2009; 74: 35-40
- 85 Forbes GL, Merkulova A, Pinheiro A. et al. Poly (acrylic acid) (PAA) is a contact system activator with properties to stop hemorrhage. Thromb Res 2020; 193: 142-145
- 86 Tans G, Griffin JH. Properties of sulfatides in factor-XII-dependent contact activation. Blood 1982; 59 (01) 69-75
- 87 España F, Ratnoff OD. The role of prekallikrein and high-molecular-weight kininogen in the contact activation of Hageman factor (factor XII) by sulfatides and other agents. J Lab Clin Med 1983; 102 (04) 487-499
- 88 Bock PE, Srinivasan KR, Shore JD. Activation of intrinsic blood coagulation by ellagic acid: insoluble ellagic acid-metal ion complexes are the activating species. Biochemistry 1981; 20 (25) 7258-7266
- 89 Girolami A, Cliffton EE. Hypercoagulable state induced in humans by the intravenous administration of purified ellagic acid. Thromb Diath Haemorrh 1967; 17 (1-2): 165-175
- 90 Samuel M, Pixley RA, Villanueva MA, Colman RW, Villanueva GB. Human factor XII (Hageman factor) autoactivation by dextran sulfate. Circular dichroism, fluorescence, and ultraviolet difference spectroscopic studies. J Biol Chem 1992; 267 (27) 19691-19697
- 91 Siebeck M, Cheronis JC, Fink E. et al. Dextran sulfate activates contact system and mediates arterial hypotension via B2 kinin receptors. J Appl Physiol (1985) 1994; 77 (06) 2675-2680
- 92 Björkqvist J, Lecher B, Maas C, Renné T. Zinc-dependent contact system activation induces vascular leakage and hypotension in rodents. Biol Chem 2013; 394 (09) 1195-1204
- 93 Corbier A, Le Berre N, Rampe D. et al. Oversulfated chondroitin sulfate and OSCS-contaminated heparin cause dose- and route-dependent hemodynamic effects in the rat. Toxicol Sci 2011; 121 (02) 417-427
- 94 Guerrini M, Beccati D, Shriver Z. et al. Oversulfated chondroitin sulfate is a contaminant in heparin associated with adverse clinical events. Nat Biotechnol 2008; 26 (06) 669-675
- 95 Lin L, Xu L, Xiao C. et al. Plasma contact activation by a fucosylated chondroitin sulfate and its structure-activity relationship study. Glycobiology 2018; 28 (10) 754-764
- 96 Sperling C, Maitz MF, Grasso S, Werner C, Kanse SM. A positively charged surface triggers coagulation activation through Factor VII activating protease (FSAP). ACS Appl Mater Interfaces 2017; 9 (46) 40107-40116
- 97 Weiss AS, Gallin JI, Kaplan AP. Fletcher factor deficiency. A diminished rate of Hageman factor activation caused by absence of prekallikrein with abnormalities of coagulation, fibrinolysis, chemotactic activity, and kinin generation. J Clin Invest 1974; 53 (02) 622-633
- 98 Bork K, Witzke G. Shortened activated partial thromboplastin time may help in diagnosing hereditary and acquired angioedema. Int Arch Allergy Immunol 2016; 170 (02) 101-107
- 99 Kanaji T, Okamura T, Osaki K. et al. A common genetic polymorphism (46 C to T substitution) in the 5′-untranslated region of the coagulation factor XII gene is associated with low translation efficiency and decrease in plasma factor XII level. Blood 1998; 91 (06) 2010-2014
- 100 Bachler M, Niederwanger C, Hell T. et al. Influence of factor XII deficiency on activated partial thromboplastin time (aPTT) in critically ill patients. J Thromb Thrombolysis 2019; 48 (03) 466-474
- 101 Marcoux G, Duchez AC, Rousseau M. et al. Microparticle and mitochondrial release during extended storage of different types of platelet concentrates. Platelets 2017; 28 (03) 272-280
- 102 McMullen BA, Fujikawa K. Amino acid sequence of the heavy chain of human alpha-factor XIIa (activated Hageman factor). J Biol Chem 1985; 260 (09) 5328-5341
- 103 Schousboe I. Contact activation in human plasma is triggered by zinc ion modulation of factor XII (Hageman factor). Blood Coagul Fibrinolysis 1993; 4 (05) 671-678
- 104 Mahdi F, Madar ZS, Figueroa CD, Schmaier AH. Factor XII interacts with the multiprotein assembly of urokinase plasminogen activator receptor, gC1qR, and cytokeratin 1 on endothelial cell membranes. Blood 2002; 99 (10) 3585-3596
- 105 Yamada KM. Cell surface interactions with extracellular materials. Annu Rev Biochem 1983; 52: 761-799
- 106 Cool DE, MacGillivray RT. Characterization of the human blood coagulation factor XII gene. Intron/exon gene organization and analysis of the 5′-flanking region. J Biol Chem 1987; 262 (28) 13662-13673
- 107 Harris RJ, Ling VT, Spellman MW. O-linked fucose is present in the first epidermal growth factor domain of factor XII but not protein C. J Biol Chem 1992; 267 (08) 5102-5107
- 108 Liu T, Qian WJ, Gritsenko MA. et al. Human plasma N-glycoproteome analysis by immunoaffinity subtraction, hydrazide chemistry, and mass spectrometry. J Proteome Res 2005; 4 (06) 2070-2080
- 109 López-Gálvez R, de la Morena-Barrio ME, López-Lera A. et al. Factor XII in PMM2-CDG patients: role of N-glycosylation in the secretion and function of the first element of the contact pathway. Orphanet J Rare Dis 2020; 15 (01) 280
- 110 Bunkenborg J, Pilch BJ, Podtelejnikov AV, Wiśniewski JR. Screening for N-glycosylated proteins by liquid chromatography mass spectrometry. Proteomics 2004; 4 (02) 454-465
- 111 Naudin C, Burillo E, Blankenberg S, Butler L, Renné T. Factor XII contact activation. Semin Thromb Hemost 2017; 43 (08) 814-826
- 112 Sabater-Lleal M, Chillón M, Mordillo C. et al. Combined cis-regulator elements as important mechanism affecting FXII plasma levels. Thromb Res 2010; 125 (02) e55-e60
- 113 Lombardi AM, Bortoletto E, Scarparo P, Scapin M, Santarossa L, Girolami A. Genetic study in patients with factor XII deficiency: a report of three new mutations exon 13 (Q501STOP), exon 14 (P547L) and -13C>T promoter region in three compound heterozygotes. Blood Coagul Fibrinolysis 2008; 19 (07) 639-643
- 114 Hofferbert S, Müller J, Köstering H, von Ohlen WD, Schloesser M. A novel 5′-upstream mutation in the factor XII gene is associated with a TaqI restriction site in an Alu repeat in factor XII-deficient patients. Hum Genet 1996; 97 (06) 838-841
- 115 Schloesser M, Zeerleder S, Lutze G. et al. Mutations in the human factor XII gene. Blood 1997; 90 (10) 3967-3977
- 116 Kondo S, Tokunaga F, Kawano S, Oono Y, Kumagai S, Koide T. Factor XII Tenri, a novel cross-reacting material negative factor XII deficiency, occurs through a proteasome-mediated degradation. Blood 1999; 93 (12) 4300-4308
- 117 Feng Y, Ye X, Pang Y, Dai J, Wang XF, Zhou XH. A novel mutation in a patient with congenital coagulation factor XII deficiency. Chin Med J (Engl) 2008; 121 (13) 1241-1244
- 118 Singhamatr P, Kanjanapongkul S, Rojnuckarin P. Molecular analysis of factor XII gene in Thai patients with factor XII deficiency. Blood Coagul Fibrinolysis 2013; 24 (06) 599-604
- 119 Kim HJ, Kim HJ, Kwon EH, Lee KO, Park IA, Kim SH. Novel deleterious mutation in the F12 gene in a Korean family with severe coagulation factor XII deficiency. Blood Coagul Fibrinolysis 2010; 21 (07) 683-686
- 120 Matsuki E, Miyakawa Y, Okamoto S. A novel factor XII mutation, FXII R84P, causing factor XII deficiency in a patient with hereditary spastic paraplegia. Blood Coagul Fibrinolysis 2011; 22 (03) 227-230
- 121 Ye X, Feng Y, Ding Q, Dai J, Wang X. Genetic analysis of a pedigree with combined factor XII and factor XI deficiency. Blood Coagul Fibrinolysis 2011; 22 (02) 118-122
- 122 Kwon MJ, Kim HJ, Lee KO, Jung CW, Kim SH. Molecular genetic analysis of Korean patients with coagulation factor XII deficiency. Blood Coagul Fibrinolysis 2010; 21 (04) 308-312
- 123 Kanaji T, Kanaji S, Osaki K. et al. Identification and characterization of two novel mutations (Q421 K and R123P) in congenital factor XII deficiency. Thromb Haemost 2001; 86 (06) 1409-1415
- 124 Matsukuma E, Gotoh Y, Kuroyanagi Y. et al. A case of atypical hemolytic uremic syndrome due to anti-factor H antibody in a patient presenting with a factor XII deficiency identified two novel mutations. Clin Exp Nephrol 2011; 15 (02) 269-274
- 125 Jin P, Jiang W, Yan H. et al. Novel mutations in congenital factor XII deficiency. Front Biosci 2016; 21: 419-429
- 126 Yang L, Wang Y, Zhou J. et al. Identification of genetic defects underlying FXII deficiency in four unrelated Chinese patients. Acta Haematol 2016; 135 (04) 238-240
- 127 Xie H, Lv M, Yang X. et al. [Identification of a novel mutation of factor XII gene in a family with coagulation FXII deficiency]. Zhonghua Yi Xue Yi Chuan Xue Za Zhi 2013; 30 (03) 313-317
- 128 Iijima K, Arakawa Y, Sugahara Y. et al. Factor XII Osaka: abnormal factor XII with partially defective prekallikrein cleavage activity. Thromb Haemost 2011; 105 (03) 473-478
- 129 Cheng X, Yang L, Huang G, Jin Y, Hao X, Wang M. Genetic analysis of a hereditary factor XII deficiency pedigree of a consanguineous marriage due to a homozygous F12 gene mutation: Gly341Arg. Hematology 2017; 22 (05) 310-315
- 130 Suzuki K, Murai K, Suwabe A, Ishida Y. Factor XII Ofunato: Lys346Asn mutation associated with blood coagulation factor XII deficiency causes impaired secretion through a proteasome-mediated degradation. Thromb Res 2010; 125 (05) 438-443
- 131 Wuillemin WA, Furlan M, Stricker H, Lämmle B. Functional characterization of a variant factor XII (F XII Locarno) in a cross reacting material positive F XII deficient plasma. Thromb Haemost 1992; 67 (02) 219-225
- 132 Hovinga JK, Schaller J, Stricker H, Wuillemin WA, Furlan M, Lämmle B. Coagulation factor XII Locarno: the functional defect is caused by the amino acid substitution Arg 353-->Pro leading to loss of a kallikrein cleavage site. Blood 1994; 84 (04) 1173-1181
- 133 Oguchi S, Ishii K, Moriki T. et al. Factor XII Shizuoka, a novel mutation (Ala392Thr) identified and characterized in a patient with congenital coagulation factor XII deficiency. Thromb Res 2005; 115 (03) 191-197
- 134 Wada H, Nishioka J, Kasai Y. et al. Molecular characterization of coagulation factor XII deficiency in a Japanese family. Thromb Haemost 2003; 90 (01) 59-63
- 135 Zhang H, Liu S, Lin C. et al. Compound heterozygous mutations Glu502Lys and Met527Thr of the FXII gene in a patient with factor XII deficiency. Hematology 2019; 24 (01) 420-425
- 136 Li M, Xie H, Wang M, Ding H. Molecular characterization of a novel missense mutation (Asp538Asn) in a Chinese patient with factor XII deficiency. Clin Lab 2015; 61 (12) 1967-1971
- 137 Schloesser M, Hofferbert S, Bartz U, Lutze G, Lämmle B, Engel W. The novel acceptor splice site mutation 11396(G-->A) in the factor XII gene causes a truncated transcript in cross-reacting material negative patients. Hum Mol Genet 1995; 4 (07) 1235-1237
- 138 Miyata T, Kawabata S, Iwanaga S, Takahashi I, Alving B, Saito H. Coagulation factor XII (Hageman factor) Washington D.C.: inactive factor XIIa results from Cys-571----Ser substitution. Proc Natl Acad Sci U S A 1989; 86 (21) 8319-8322