Protocol

The review protocol involves study of all existing published literature on molecular pathology of RBDs from India. As every relevant report in published English literature on RBDs from India has been included, the study is holistic and comprehensive.

Eligibility criteria and Information source

Studies describing molecular pathologies in RBDs in human patients (case series, review, original papers, were used to compile the present report).

Search

To search the published literature from India on the molecular pathology of RBDs, Pubmed search was used (www.pubmed.com). To compare the distribution of the types of mutations reported in Indian studies, with that of world literature, the Human Gene Mutation Database (HGMD) was referred up to August 2013 (www.hgmd.org). The key words used for pubmed search were: “rare bleeding disorders”, “mutations”, “ India”, “fibrinogen”, “afibrinogenemia”, “factor II deficiency”, “prothrombin”, “factor VII deficiency”, “factor V deficiency”, “factor X deficiency”, “factor XI deficiency”, “combined factor V and VIII deficiency”, “factor XIII deficiency”, “Bernard Soulier syndrome” and “Glanzmanns thrombasthenia” in different combinations. A total of 60 relevant articles were returned using these key words (Flow Diagram S1).

Data Collection process

The data was tabulated in master sheets, which were subsequently tabulated separately for each RBD. To keep the presentation uniform throughout, the reporting format of the mutations/polymorphisms was converted in accordance to the HGVS nomenclature, wherever possible.

Data Items

The following data items were collected: deficiency, inheritance, bleeding, complications, laboratory findings, molecular pathologies in congenital/inherited fibrinogen disorders, FII, FV, FV+FVIII, FVII, FX, FXI, FXIII deficiencies and platelet disorders, GT and BSS.

Risk of bias in individual studies and across studies

As all the studies are hospital based, the main bias is that, symptomatically milder patients may have been missed unless a family study has been done where one patient had severe manifestations.

Additional analysis

As this study is a descriptive additive data, it did not require any additional analysis.

Fibrinogen deficiency

Mutations in three genes (FGA, FGB, FGG) encoding fibrinogen α-, β- and γ-chains lead to congenital fibrinogen deficiency, which is an extremely rare hereditary bleeding disorder, affecting 1 in 1,000,000 individuals [4], [5]. There are two reports of molecular characterization of fibrinogen deficiency in Indian patients which collectively report the molecular pathology of 28 patients [4], [5]. The first report of “Fibrinogen Mumbai” describes a novel homozygous c.G8017A transition in exon 8 found in FGB gene. The resulting p.G434D missense mutation involves a highly conserved amino acid residue, located in the C-terminal globular D domain. This p.G434D substitution causes severe hypofibrinogenemia by impairing fibrinogen secretion as confirmed by expression data [5]. Another study describes a series of 27 patients with fibrinogen deficiency and the underlying molecular pathologies [4].

Fibrinogen alpha (FGA), beta (FGB), gamma (FGG) genes collectively were found to have a total of 15 disease causing mutations with 8 frameshift, 3 splice site, 3 missense and 1 nonsense mutation in 27 patients. 13 of them were novel; 7 were frame shift (FGA: p.Asp296fs*59, p.Thr466fs*17 and p.Lys575fs*74; FGB: p.Gly414fs*2 and FGG: p.Ser81fs*5, p.Lys185fs*13 and p.Asp278_279 fs*17), 3 splice site mutations (FGA c. G364+1A; c.T510+2 G; FGB c.G851+1A), 2 missense substitutions (FGB p.Gly288Ser; p.Arg445Thr); a nonsense mutation in FGA (p.Tyr127*) and two common mutations (FGA: c. G364+1A, FGG: p.Lys185fs*13) in 14 patients have been reported [4]. FGG: p.Lys185fs*13 is the most common mutation observed in one third of the Indian patients, while the second mutation, a splice site variant i.e. FGA: c.G364+1A was observed in 5 out of 27 patients (18.5%) analyzed. This finding is significant as it provides a first line screening strategy for mutation detection in this gene in Indian patients. The nucleotide and the resultant amino acid variations reported are summarized in Table 1.

Prothrombin deficiency

Prothrombin (coagulation factor II) is the precursor of thrombin, a serine protease in the coagulation cascade. The Prothrombin gene is located on chromosome 11 (11p11–q12 [2]. Prothrombin deficiency occurs in approximately 1: 2,000,000 individuals, with diverse molecular basis. The mutations or polymorphisms in F7 gene are known to cause both thrombosis and bleeding [6], [7]. Six mutations have been reported by different groups from the Indian literature so far, which lead to prothrombin deficiency [6], [7]. Two of these mutations are novel; p.Ala405Thr change affecting ‘B’ chain of α-thrombin i.e. Prothrombin Vellore located in the Histidine disulfide loop of the thrombin B chain [6] and the other one, Prothrombin Mumbai i.e. c.G269C mutation which caused a p.Cys90Ser substitution in the primary protein [7]. Mutations in F2 gene generally do not lead to complete absence of the protein as severe prothrombin deficiency is incompatible with life. The F2 mutations reported from India are shown in Table 2.

Factor V deficiency

Congenital factor V (FV) deficiency is generally associated with moderate to severe bleeding symptoms. In the world literature, a total of 104 mutations, located in the F5 gene, have been described in patients with severe FV deficiency (http://www.hgmd.org/). Most of the mutations reported are localized to exon 13 of the F5 gene. There is one report from the Indian literature so far, where mutations in 5 unrelated patients were reported, of which 3 were novel small deletions, present in homozygous state, g.50936–50937delAA or AG and g.51660delA, occurring in two different patients, and g.52162delC in another patient [8]. Interestingly, the mutations reported by this group were all found in exon 13. Screening for mutations in exon 13 should be the first step before proceeding to the remaining exons in this gene. Table 3 summarizes the mutations reported in this study.

Combined FV and FVIII deficiency

Combined FV and FVIII deficiency is a rare autosomal recessive bleeding disorder occurring in 1: 1,000,000 individuals. Mutations in one of the two genes encoding the proteins i.e. lectin mannose binding protein (LMAN1) and multiple coagulation factor deficiency 2 (MCFD2) lead to deficiencies of FV and FVIII. 13 patients with combined FV and FVIII deficiency have been reported in the Indian literature by two different groups, where a complete molecular characterization has been done [9], [10]. In one of the families mutation was not detected in both the genes which suggests the existence of a third locus involved in the secretion pathway of FV and FVIII and associated with the combined deficiency [10]. The mutations reported by these groups are summarized in Table 4. Three of them, a 72 bp deletion in LMAN1 (c.813_822+62del72, p.K272fs), a 35-bp deletion in MCFD2 (c.210_244del35) and a missense mutation in MCFD2 (p.D122V) were identified in 4 patients. A nonsense mutation, i.e. G to T substitution, in exon 2 of the LMAN1 gene, was novel [9].

Factor VII deficiency

FVII is a vitamin K-dependant serine protease synthesized in the liver and has a very important position in the coagulation cascade. Factor VII deficiency is a rare (1: 500,000) autosomal recessive disorder of blood coagulation caused by heterogeneous mutations (∼140) in F7 gene [10]. The clinical features are quite variable in patients with FVII deficiency. The severity of bleeding is not well correlated with the FVII activity. Mutations in 26 patients with FVII deficiency have been characterized and 21 mutations and 6 polymorphisms have been reported from various studies from India [11]–[13]. Two mutations occurred in double heterozygous form in a patient, p. Asp302Asn and p. His408Arg substitution in the 8th exon of the F7 gene. p.Asp302 is one of three absolutely conserved active-site residues found in all serine proteases, whereas p. His408Arg substitution is located in exon 8 of F7 corresponding to the catalytic domain of the enzyme.

A total of 18 missense, 2 nonsense, and 1 frame shift mutation has been reported, of which 10 were novel variations. It is interesting to note that 15 of these 26 patients were found to have the disease causing mutations in exon 8; 7 had the mutations in exon 6 of the F7 gene and 6 of the mutations were located in the region corresponding to the catalytic serine protease domain. Using haplotype analysis, it was shown that p.Leu55fs in the pro-peptide region and p.Gln287* in the catalytic domain which resulted in premature termination codon in two patients had a common founder. Successful prenatal diagnosis in the second trimester of pregnancy by cordocentesis, followed by FVII and other coagulation factor assays could be given to a family with one affected child [13].

Another study showed that functional polymorphisms in F7 gene affect the phenotype of patients with severe Hemophilia. F7353Q allele was shown to be associated with a severe phenotype. F7 Arg/Gln and Gln/Gln genotypes were found to be significantly higher in patients with severe phenotype when compared to patients with milder phenotype (P = 0.045) [14]. The mutations reported from Indian studies are presented in Table 5.

Factor X deficiency

Factor X (FX) deficiency is a rare autosomal recessive bleeding disorder that is estimated to occur in 1: 100,000 individuals worldwide. The gene encoding F10 is located on the long arm of chromosome 13, consists of 27 Kb of nucleotide sequence with eight exons and seven introns [15]. 103 variants, comprising deletions, missense, frameshift and splice site mutations have been reported in F10 gene (http://www.hgmd.org/). Most mutations are missense and the common sites of mutations have been localized to exon 2 (Gla domain) and exons 7 and 8 (catalytic domains). Mutations in a total of 22 patients with FX deficiency from India and 1 from Nepal have been characterized and reported by Indian groups. 17 mutations and 5 polymorphisms have been reported, of which 15 are missense, 1 frame-shift and 1 nonsense mutation. 13 novel mutations and 1 novel polymorphism have been documented [15], [16]. Nine of the patients were found to have the mutation in exon 8. p.Gly406Ser which resulted in a cross reactive material positive phenotype with FX antigen levels similar to wild-type but undetectable activity was the disease causing mutation in 3 of the patients. The polymorphism c.C793T (p.Thr264Thr) was found in 9 patients from two independent study groups. Second trimester prenatal diagnosis by phenotypic factor assays in cord blood sample was given to a family with one child affected with FX deficiency [15]. The various mutations and polymorphisms studied in FX deficiency patients from India are summarized in table 6.

Factor XI deficiency

Factor XI is present in the plasma as a zymogen. It exists as a homodimer consisting of two identical polypeptide chains linked by disulfide bonds. During activation, an internal peptide bond is cleaved by factor XIIa, resulting in activated factor XIa, which activates factor IX. Deficiency of FXI is referred to as Rosenthal syndrome or Hemophilia C. The prevalence of FXI deficiency in the world literature is estimated to be about 1 in 100,000 to 1 in 1 million. Though a few cases of FXI deficiency have been identified in the Indian population [18], [19], there is only one report on molecular characterization of FXI deficiency in 2 patients and one patient with combined FIX and FXI deficiency [17]. There are only 3 mutations reported in F11 gene from India. One patient had a double coagulation defect, a novel c.T31166G transversion (p.Phe349Val) in F9 corresponding to the catalytic domain of FIX, along with a homozygous p.Gly460Arg mutation in F11 corresponding to the catalytic domain of FXI. Another patient was shown to have the p.Gly460Arg mutation in heterozygous state with a novel p.Val271Leu mutation that affected the apple-3 domain of FXI (Table 7) [17]. This mutation was predicted to abolish the physiological donor splice site and result in an abnormal FXI transcript. The third patient was detected to have a novel p.Tyr351Ser mutation in exon 10 of F11 corresponding to the apple-4 domain in FXI. This group also reported 2 polymorphisms -138C in intron A and p.Gly379Gly in heterozygous state (Pt.1) or a homozygous state (Pt.2) in two patients (Table 7) [17].

FXIII deficiency

Factor XIII is a plasma transglutaminase protein that is essential for normal haemostasis and fibrinolysis. FXIII deficiency is a rare autosomal (1: 2,000,000) recessive disorder of blood coagulation. Mutations are mostly reported in the F13A gene. FXIII deficiency leads to serious bleeding diathesis, the common symptoms being bleeding from the umbilical stump, prolonged bleeding post-injury, menorrhagia, poor healing of wounds, intra cranial bleed and spontaneous abortions. From the Indian studies, 15 patients of FXIII deficiency have been characterized for their molecular pathology. A total of 15 mutations have been identified, out of which 8 are missense, 2 duplications, 1 heterozygous deletion, 1 splice site and 3 nonsense mutations. Some polymorphisms were also identified, of which 1 was novel. Three mutations were detected in exon 10 in 4 patients and four mutations in exon 6 of F13A. The IVS1 A246G polymorphism was found to be present in 6 unrelated patients [20], [21]. It would be interesting to study the heterozygosity frequency of this polymorphism, which may be a useful marker for offering possible prenatal diagnoses for the affected families. The mutations and polymorphisms identified are presented in Table 8.

Inherited disorders of platelet function