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8. Adenovirus-associated virus vector-mediated gene transfer in hemophilia B.

Author

Nathwani AC, Tuddenham EG, Rangarajan S, Rosales C, McIntosh J, Linch DC, Chowdary P, Riddell A, Pie AJ, Harrington C, O'Beirne J, Smith K, Pasi J, Glader B, Rustagi P, Ng CY, Kay MA, Zhou J, Spence Y, and Morton CL

Abstract

Background: Hemophilia B, an X-linked disorder, is ideally suited for gene therapy. We investigated the use of a new gene therapy in patients with the disorder.Methods: We infused a single dose of a serotype-8-pseudotyped, self-complementary adenovirus-associated virus (AAV) vector expressing a codon-optimized human factor IX (FIX) transgene (scAAV2/8-LP1-hFIXco) in a peripheral vein in six patients with severe hemophilia B (FIX activity, <1% of normal values). Study participants were enrolled sequentially in one of three cohorts (given a high, intermediate, or low dose of vector), with two participants in each group. Vector was administered without immunosuppressive therapy, and participants were followed for 6 to 16 months.Results: AAV-mediated expression of FIX at 2 to 11% of normal levels was observed in all participants. Four of the six discontinued FIX prophylaxis and remained free of spontaneous hemorrhage; in the other two, the interval between prophylactic injections was increased. Of the two participants who received the high dose of vector, one had a transient, asymptomatic elevation of serum aminotransferase levels, which was associated with the detection of AAV8-capsid-specific T cells in the peripheral blood; the other had a slight increase in liver-enzyme levels, the cause of which was less clear. Each of these two participants received a short course of glucocorticoid therapy, which rapidly normalized aminotransferase levels and maintained FIX levels in the range of 3 to 11% of normal values.Conclusions: Peripheral-vein infusion of scAAV2/8-LP1-hFIXco resulted in FIX transgene expression at levels sufficient to improve the bleeding phenotype, with few side effects. Although immune-mediated clearance of AAV-transduced hepatocytes remains a concern, this process may be controlled with a short course of glucocorticoids without loss of transgene expression. (Funded by the Medical Research Council and others; ClinicalTrials.gov number, NCT00979238.). [ABSTRACT FROM AUTHOR]

Published
2011
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11. Clinical experience with polyelectrolyte-fractionated porcine factor VIII concentrate in the treatment of hemophiliacs with antibodies to factor VIII

Author

Kernoff, PB, Thomas, ND, Lilley, PA, Matthews, KB, Goldman, E, and Tuddenham, EG

Abstract

Circulating antibodies to factor VIII (anti-VIII, “inhibitors”) occurring in patients with hemophilia neutralize porcine factor VIII less readily than human factor VIII in vitro. Over an 18-mo period, 8 patients with anti-VIII were treated with 45 courses (297 infusions) of polyelectrolyte-fractionated porcine factor VIII concentrate (PE porcine VIII). Where no anti-PE porcine VIII was detectable, mean post- infusion rise in plasma factor VIII was 1.29 U/dl/units infused/kg. Above 13 Old Oxford units of anti-PE porcine VIII and 48 Bethesda units of anti-human VIII, there were no postinfusion rises in plasma factor VIII. Where postinfusion rises were detected, clinical responses were good and conventional methods could be used to guide dosage. Ten percent of infusions were followed by febrile reactions, but these were usually mild and decreased in frequency and severity with increasing exposure. Multiple and prolonged courses of therapy were given to some patients without evidence of loss of clinical or laboratory efficacy. PE porcine VIII could provoke anamnestic rises of anti-VIII in susceptible patients, but appeared to have a lower immunogenic potential than human VIII. PE porcine VIII is a rational and effective therapeutic alternative for patients with anti-VIII, particularly those with intermediate level inhibitors who cannot be managed effectively using human factor VIII.

Published
1984
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12. Purification and characterization of factor VIII 1,689-Cys: a nonfunctional cofactor occurring in a patient with severe hemophilia A

Author

O'Brien, DP and Tuddenham, EG

Abstract

We have purified the factor VIII from a CRM+ Hemophilia A plasma (90 U/dL VIII:Ag but 0 U/dL VIII:C) and analyzed the protein before and after thrombin activation by Western blotting with monoclonal antibodies (MoAbs). Normal or patient citrated plasma was ultracentrifuged, cryo-ethanol-precipitated and chromatographed on Sepharose 6B. The void volume fractions were reduced and subjected to ion exchange chromatography yielding material of specific activity approximately 1,000 U/mg protein (VIII:C or VIII:Ag). Factor VIII purified in this way from normal plasma is fully activatable by thrombin with proteolytic fragmentation as previously described by F. Rotblat et al (Biochemistry 24: 4294, 1985). Factor VIII 1,689-Cys has the normal distribution of factor VIII light and heavy chains prior to thrombin activation. After exposure to thrombin the heavy chain polypeptides were fully proteolysed but the light chain was totally resistant to cleavage. This is consistent with the demonstration in the patient's leucocyte DNA of a C to T transition in codon 1,689 converting Arg to Cys at the light chain thrombin cleavage site as previously described by J. Gitschier et al (Blood 72:1022, 1988). Uncleaved light chain of Factor VIII 1,689-Cys is not released from von Willebrand factor (vWF) by thrombin, but this is not the sole cause of the functional defect since the protein purified free of vWF has no coagulant activity. We conclude that the functional defect in factor VIII 1,689-Cys is a consequence of failure to release the acidic peptide from the light chain upon thrombin activation.

Published
1989
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13. Preparation of factor IX deficient human plasma by immunoaffinity chromatography using a monoclonal antibody

Author

Goodall, AH, Kemble, G, O'Brien, DP, Rawlings, E, Rotblat, F, Russell, GC, Janossy, G, and Tuddenham, EG

Abstract

A murine hybridoma clone is described that grows continuously in culture and produces a monoclonal antibody we have called Royal Free Monoclonal Antibody to factor IX No. 1 (RFF-IX/1). This has high affinity for a coagulation site on factor IX. RFF-IX/1 immobilised on sepharose can be used to deplete factor IX from normal human plasma. This immunoaffinity depleted plasma is indistinguishable from severe Christmas disease plasma and can be used as the substrate in a one stage coagulation assay for factor IX. The affinity column has high capacity and can be regenerated so that large scale production from normal plasma of factor IX deficient plasma as a diagnostic reagent is now feasible.

Published
1982
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14. Mutations of factor VIII cleavage sites in hemophilia A

Author

Gitschier, J, Kogan, S, Levinson, B, and Tuddenham, EG

Abstract

Hemophilia A is caused by a defect in coagulation factor VIII, a protein that undergoes extensive proteolysis during its activation and inactivation. To determine whether some cases of hemophilia are caused by mutations in important cleavage sites, we screened patient DNA samples for mutations in these sites by a two-step process. Regions of interest were amplified from genomic DNA by repeated rounds of primer- directed DNA synthesis. The amplified DNAs were then screened for mutations by discriminant hybridization using oligonucleotide probes. Two cleavage site mutations were found in a survey of 215 patients. A nonsense mutation in the activated protein C cleavage site at amino acid 336 was discovered in a patient with severe hemophilia. In another severely affected patient, a mis-sense mutation results in a substitution of cysteine for arginine in the thrombin activation site at amino acid 1689. This defect is associated with no detectable factor VIII activity, but with normal levels of factor VIII antigen. The severe hemophilia in this patient was sporadic; analysis of the mother suggested that the mutation originated in her gametes or during her embryogenesis. The results demonstrate that this approach can be used to identify factor VIII gene mutations in regions of the molecule known to be important for function.

Published
1988
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16. Coronary thrombosis and the platelet glycoprotein IIIA gene PLA2 polymorphism

Author

Graham Davies, Giuseppe Ruggiero, Edward G. D. Tuddenham, Nabeel Ahmed, Emanuele Durante-Mangoni, DURANTE MANGONI, Emanuele, Davies, Gj, Ahmed, N, Ruggiero, G, and Tuddenham, Eg

Subjects
Adult, Pathology, medicine.medical_specialty, Myocardial Infarction, Platelet Glycoprotein GPIIb-IIIa Complex, Chest pain, Angina Pectoris, Coronary thrombosis, Risk Factors, Internal medicine, medicine, Humans, cardiovascular diseases, Myocardial infarction, Survivors, Allele, Gene, Alleles, Polymorphism, Genetic, business.industry, Vascular disease, Coronary Thrombosis, Hematology, Middle Aged, medicine.disease, Thrombosis, Cardiology, Platelet Membrane Glycoprotein IIb, medicine.symptom, business
Abstract

SummaryMyocardial infarction results from a platelet-rich occlusive coronary thrombus. Platelet membrane glycoprotein IIb/IIIa plays an important role in platelet adhesion and aggregation. Two polymorphisms of the gene encoding the IIIa subunit, PLA1 and PLA2, have been identified. We investigated the frequency of these polymorphisms in 114 consecutive patients with a history of angina-like chest pain admitted for coronary arteriography. Forty-three of these patients had previously suffered a myocardial infarction. The PLA2 polymorphism was found in 21% of the patients with previous myocardial infarction and in 27% of the patients with angina-like chest pain but no previous myocardial infarction (p = 0.634). There was also no significant association with the extent of coronary disease. There is no evidence, therefore, from this study of an association between the PLA polymorphisms and the occurrence of myocardial infarction.

Published
1998

18. Thrombin generation assay identifies individual variability in responses to low molecular weight heparin in pregnancy: implications for anticoagulant monitoring.

Author

Chowdary P, Adamidou D, Riddell A, Aghighi S, Griffioen A, Priest P, Moghadam L, Kelaher N, Huq FY, Kadir RA, Tuddenham EG, and Gatt A

Subjects
Adult, Female, Humans, Pregnancy, Retrospective Studies, Thrombin Time methods, Anticoagulants administration & dosage, Anticoagulants pharmacokinetics, Factor Xa Inhibitors blood, Heparin, Low-Molecular-Weight administration & dosage, Heparin, Low-Molecular-Weight pharmacokinetics, Monitoring, Physiologic, Pregnancy Complications, Hematologic blood, Pregnancy Complications, Hematologic drug therapy, Thrombophilia blood, Thrombophilia drug therapy
Abstract

Low molecular weight heparin (LMWH) given to inhibit coagulation and reduce the risk of thrombosis, is typically monitored by anti-Xa assay. However, anti-Xa levels may not necessarily provide an accurate measure of coagulation inhibition. Moreover, pregnancy is associated with hypercoagulability, which may compromise the efficacy of LMWH. We looked at the association between anti-Xa levels and parameters of thrombin generation assay [TGA; area under the curve (AUC), peak height (PH) and time to peak (ttP)] using samples from 41 pregnant women receiving LMWH and 40 normal pregnant women controls. TGA results confirmed the physiological hypercoagulability of normal pregnancy (mean normalised values: AUC 119%; PH 157%; ttP 72%). Although anti-Xa measures correlated with all three TGA parameters, this group correlation masked significant inter-individual variability, demonstrated by the R(2) value or coefficient of determination. Anti-Xa levels contributed to 74% of variation in AUC values, 63% of variation in PH values and only 53% of variation in ttP values. The remainder reflects the contribution of patients' intrinsic coagulation status. Hence, some patients with 'safe' anti-Xa levels may potentially be under-anticoagulated, particularly in pregnancy. Measuring coagulability directly with TGA may lower the risk of adverse events due to under-anticoagulation in selected patients., (© 2014 John Wiley & Sons Ltd.)

Published
2015
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19. Long-term safety and efficacy of factor IX gene therapy in hemophilia B.

Author

Nathwani AC, Reiss UM, Tuddenham EG, Rosales C, Chowdary P, McIntosh J, Della Peruta M, Lheriteau E, Patel N, Raj D, Riddell A, Pie J, Rangarajan S, Bevan D, Recht M, Shen YM, Halka KG, Basner-Tschakarjan E, Mingozzi F, High KA, Allay J, Kay MA, Ng CY, Zhou J, Cancio M, Morton CL, Gray JT, Srivastava D, Nienhuis AW, and Davidoff AM

Subjects
Adult, Alanine Transaminase blood, Dependovirus genetics, Factor IX metabolism, Follow-Up Studies, Gene Expression, Hemophilia B blood, Hemophilia B genetics, Humans, Infusions, Intravenous, Male, Middle Aged, Transgenes, Young Adult, Factor IX genetics, Genetic Therapy adverse effects, Genetic Vectors administration & dosage, Hemophilia B therapy
Abstract

Background: In patients with severe hemophilia B, gene therapy that is mediated by a novel self-complementary adeno-associated virus serotype 8 (AAV8) vector has been shown to raise factor IX levels for periods of up to 16 months. We wanted to determine the durability of transgene expression, the vector dose-response relationship, and the level of persistent or late toxicity., Methods: We evaluated the stability of transgene expression and long-term safety in 10 patients with severe hemophilia B: 6 patients who had been enrolled in an initial phase 1 dose-escalation trial, with 2 patients each receiving a low, intermediate, or high dose, and 4 additional patients who received the high dose (2×10(12) vector genomes per kilogram of body weight). The patients subsequently underwent extensive clinical and laboratory monitoring., Results: A single intravenous infusion of vector in all 10 patients with severe hemophilia B resulted in a dose-dependent increase in circulating factor IX to a level that was 1 to 6% of the normal value over a median period of 3.2 years, with observation ongoing. In the high-dose group, a consistent increase in the factor IX level to a mean (±SD) of 5.1±1.7% was observed in all 6 patients, which resulted in a reduction of more than 90% in both bleeding episodes and the use of prophylactic factor IX concentrate. A transient increase in the mean alanine aminotransferase level to 86 IU per liter (range, 36 to 202) occurred between week 7 and week 10 in 4 of the 6 patients in the high-dose group but resolved over a median of 5 days (range, 2 to 35) after prednisolone treatment., Conclusions: In 10 patients with severe hemophilia B, the infusion of a single dose of AAV8 vector resulted in long-term therapeutic factor IX expression associated with clinical improvement. With a follow-up period of up to 3 years, no late toxic effects from the therapy were reported. (Funded by the National Heart, Lung, and Blood Institute and others; ClinicalTrials.gov number, NCT00979238.).

Published
2014
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20. Solution structure of the major factor VIII binding region on von Willebrand factor.

Author

Shiltagh N, Kirkpatrick J, Cabrita LD, McKinnon TA, Thalassinos K, Tuddenham EG, and Hansen DF

Subjects
Binding Sites, Crystallography, X-Ray, Factor VIII genetics, Factor VIII metabolism, Humans, Protein Stability, Protein Structure, Quaternary, Protein Structure, Secondary, Protein Structure, Tertiary, Static Electricity, von Willebrand Factor genetics, von Willebrand Factor metabolism, Factor VIII chemistry, von Willebrand Factor chemistry
Abstract

Although much of the function of von Willebrand factor (VWF) has been revealed, detailed insight into the molecular structure that enables VWF to orchestrate hemostatic processes, in particular factor VIII (FVIII) binding and stabilization in plasma, is lacking. Here, we present the high-resolution solution structure and structural dynamics of the D' region of VWF, which constitutes the major FVIII binding site. D' consists of 2 domains, trypsin-inhibitor-like (TIL') and E', of which the TIL' domain lacks extensive secondary structure, is strikingly dynamic and harbors a cluster of pathological mutations leading to decreased FVIII binding affinity (type 2N von Willebrand disease [VWD]). This indicates that the backbone malleability of TIL' is important for its biological activity. The principal FVIII binding site is localized to a flexible, positively charged region on TIL', which is supported by the rigid scaffold of the TIL' and E' domain β sheets. Furthermore, surface-charge mapping of the TIL'E' structure reveals a potential mechanism for the electrostatically guided, high-affinity VWF⋅FVIII interaction. Our findings provide novel insights into VWF⋅FVIII complex formation, leading to a greater understanding of the molecular basis of the bleeding diathesis type 2N VWD., (© 2014 by The American Society of Hematology.)

Published
2014
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21. An interactive mutation database for human coagulation factor IX provides novel insights into the phenotypes and genetics of hemophilia B.

Author

Rallapalli PM, Kemball-Cook G, Tuddenham EG, Gomez K, and Perkins SJ

Subjects
Amino Acid Sequence, Computational Biology, Crystallography, X-Ray, Factor IX chemistry, Factor IXa genetics, Genetic Predisposition to Disease, Hemophilia B blood, Humans, Models, Molecular, Molecular Sequence Data, Phenotype, Polymorphism, Genetic, Protein Conformation, Severity of Illness Index, Structure-Activity Relationship, Blood Coagulation genetics, DNA Mutational Analysis, Databases, Genetic, Factor IX genetics, Hemophilia B genetics, Mutation
Abstract

Background: Factor IX (FIX) is important in the coagulation cascade, being activated to FIXa on cleavage. Defects in the human F9 gene frequently lead to hemophilia B., Objective: To assess 1113 unique F9 mutations corresponding to 3721 patient entries in a new and up-to-date interactive web database alongside the FIXa protein structure., Methods: The mutations database was built using MySQL and structural analyses were based on a homology model for the human FIXa structure based on closely-related crystal structures., Results: Mutations have been found in 336 (73%) out of 461 residues in FIX. There were 812 unique point mutations, 182 deletions, 54 polymorphisms, 39 insertions and 26 others that together comprise a total of 1113 unique variants. The 64 unique mild severity mutations in the mature protein with known circulating protein phenotypes include 15 (23%) quantitative type I mutations and 41 (64%) predominantly qualitative type II mutations. Inhibitors were described in 59 reports (1.6%) corresponding to 25 unique mutations., Conclusion: The interactive database provides insights into mechanisms of hemophilia B. Type II mutations are deduced to disrupt predominantly those structural regions involved with functional interactions. The interactive features of the database will assist in making judgments about patient management., (© 2013 International Society on Thrombosis and Haemostasis.)

Published
2013
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22. Therapeutic levels of FVIII following a single peripheral vein administration of rAAV vector encoding a novel human factor VIII variant.

Author

McIntosh J, Lenting PJ, Rosales C, Lee D, Rabbanian S, Raj D, Patel N, Tuddenham EG, Christophe OD, McVey JH, Waddington S, Nienhuis AW, Gray JT, Fagone P, Mingozzi F, Zhou SZ, High KA, Cancio M, Ng CY, Zhou J, Morton CL, Davidoff AM, and Nathwani AC

Subjects
Animals, Blotting, Western, Factor VIII genetics, Factor VIII immunology, Glycosylation, Hemophilia A genetics, Humans, Immune Tolerance, Liver metabolism, Macaca mulatta, Male, Mice, Mice, Inbred C57BL, Mice, Knockout, Peptide Fragments genetics, Peptide Fragments metabolism, Promoter Regions, Genetic genetics, Dependovirus genetics, Factor VIII pharmacology, Genetic Therapy, Genetic Variation genetics, Genetic Vectors administration & dosage, Hemophilia A therapy
Abstract

Recombinant adeno-associated virus (rAAV) vectors encoding human factor VIII (hFVIII) were systematically evaluated for hemophilia A (HA) gene therapy. A 5.7-kb rAAV-expression cassette (rAAV-HLP-codop-hFVIII-N6) containing a codon-optimized hFVIII cDNA in which a 226 amino acid (aa) B-domain spacer replaced the entire B domain and a hybrid liver-specific promoter (HLP) mediated 10-fold higher hFVIII levels in mice compared with non-codon-optimized variants. A further twofold improvement in potency was achieved by replacing the 226-aa N6 spacer with a novel 17-aa peptide (V3) in which 6 glycosylation triplets from the B domain were juxtaposed. The resulting 5.2-kb rAAV-HLP-codop-hFVIII-V3 cassette was more efficiently packaged within AAV virions and mediated supraphysiologic hFVIII expression (732 ± 162% of normal) in HA knock-out mice following administration of 2 × 10(12) vector genomes/kg, a vector dose shown to be safe in subjects with hemophilia B. Stable hFVIII expression at 15 ± 4% of normal was observed at this dose in a nonhuman primate. hFVIII expression above 100% was observed in 3 macaques that received a higher dose of either this vector or the N6 variant. These animals developed neutralizing anti-FVIII antibodies that were abrogated with transient immunosuppression. Therefore, rAAV-HLP-codop-hFVIII-V3 substantially improves the prospects of effective HA gene therapy.

Published
2013
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24. Journal rubric. Haemophilic pseudotumour of the carotid artery.

Author

Malam Y, Tsui J, Sheikh SE, Tuddenham EG, and Baker DM

Subjects
Aged, Carotid Artery Diseases etiology, Carotid Artery Diseases surgery, Carotid Artery, Internal surgery, Endarterectomy, Carotid, Hematoma etiology, Hematoma surgery, Hemophilia A complications, Hemophilia A surgery, Humans, Male, Treatment Outcome, Ultrasonography, Doppler, Duplex, Carotid Artery Diseases pathology, Carotid Artery, Internal pathology, Hematoma pathology, Hemophilia A pathology
Published
2012
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25. AAV-mediated gene transfer in the perinatal period results in expression of FVII at levels that protect against fatal spontaneous hemorrhage.

Author

Binny C, McIntosh J, Della Peruta M, Kymalainen H, Tuddenham EG, Buckley SM, Waddington SN, McVey JH, Spence Y, Morton CL, Thrasher AJ, Gray JT, Castellino FJ, Tarantal AF, Davidoff AM, and Nathwani AC

Subjects
Animals, Animals, Newborn, Codon, Factor VII analysis, Factor VII biosynthesis, Factor VII genetics, Factor VII Deficiency blood, Factor VII Deficiency genetics, Factor VII Deficiency physiopathology, Female, Fetal Therapies adverse effects, Gene Expression, Genetic Therapy adverse effects, Hemorrhage etiology, Hep G2 Cells, Humans, Injections, Intravenous, Macaca mulatta, Male, Mice, Pregnancy, Sex Characteristics, Survival Analysis, Dependovirus genetics, Factor VII therapeutic use, Factor VII Deficiency therapy, Genetic Therapy methods, Genetic Vectors administration & dosage, Genetic Vectors adverse effects, Hemorrhage prevention & control, Perinatal Care
Abstract

We explored adeno-associated viral vector (AAV)-mediated gene transfer in the perinatal period in animal models of severe congenital factor VII (FVII) deficiency, a disease associated with early postnatal life-threatening hemorrhage. In young adult mice with plasma FVII < 1% of normal, a single tail vein administration of AAV (1 × 10(13) vector genomes [vg]/kg) resulted in expression of murine FVII at 266% ± 34% of normal for ≥ 67 days, which mediated protection against fatal hemorrhage and significantly improved survival. Codon optimization of human FVII (hFVIIcoop) improved AAV transgene expression by 37-fold compared with the wild-type hFVII cDNA. In adult macaques, a single peripheral vein injection of 2 × 10(11) vg/kg of the hFVIIcoop AAV vector resulted in therapeutic levels of hFVII expression that were equivalent in males (10.7% ± 3.1%) and females (12.3% ± 0.8%). In utero delivery of this vector in the third trimester to fetal monkeys conferred expression of hFVII at birth of 20.4% ± 3.7%, with a gradual decline to > 1% by 7 weeks. Re-administration of an alternative serotype at 12 months postnatal age increased hFVII levels to 165% ± 6.2% of normal, which remained at therapeutic levels for a further 28 weeks without toxicity. Thus, perinatal AAV-mediated gene transfer shows promise for disorders with onset of pathology early after birth.

Published
2012
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26. Human congenital diseases with mixed modes of inheritance have a shortage of recessive disease. A demographic scenario?

Author

Mitchison NA, Bhattacharya S, and Tuddenham EG

Subjects
Demography, Genes, Dominant, Humans, Inheritance Patterns, Mutation, Selection, Genetic, Genes, Recessive, Genetic Diseases, Inborn genetics
Abstract

An archive of congenital human diseases is presented, aiming to contain all those where recessive (biallelic) can be compared with X-linked and/or dominant (monoallelic) inheritance. A significant deficit of recessive inheritance is evident, both in disease inheritance and in contribution to inheritance per known disease gene. The deficit contrasts with expectation derived from the cell biology of mutation, and from the importance of recessive mutation in evolution and its preponderance in N-ethyl-N-nitrosourea (ENU) mutagenesis. The deficit fits well with the standard model of demographic change since the neolithic era, and may also reflect natural selection acting on heterozygotes., (© 2011 The Authors Annals of Human Genetics © 2011 Blackwell Publishing Ltd/University College London.)

Published
2011
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27. Noninvasive prenatal diagnosis of hemophilia by microfluidics digital PCR analysis of maternal plasma DNA.

Author

Tsui NB, Kadir RA, Chan KC, Chi C, Mellars G, Tuddenham EG, Leung TY, Lau TK, Chiu RW, and Lo YM

Subjects
Algorithms, Chromosomes, Human, X, DNA analysis, Female, Genotype, Gestational Age, Hemophilia A blood, Hemophilia A genetics, Humans, Male, Polymerase Chain Reaction instrumentation, Polymorphism, Single Nucleotide, Pregnancy, Prenatal Diagnosis instrumentation, Sensitivity and Specificity, Signal Processing, Computer-Assisted, DNA blood, Hemophilia A diagnosis, Microfluidic Analytical Techniques methods, Mothers, Polymerase Chain Reaction methods, Prenatal Diagnosis methods
Abstract

Hemophilia is a bleeding disorder with X-linked inheritance. Current prenatal diagnostic methods for hemophilia are invasive and pose a risk to the fetus. Cell-free fetal DNA analysis in maternal plasma provides a noninvasive mean of assessing fetal sex in such pregnancies. However, the disease status of male fetuses remains unknown if mutation-specific confirmatory analysis is not performed. Here we have developed a noninvasive test to diagnose whether the fetus has inherited a causative mutation for hemophilia from its mother. The strategy is based on a relative mutation dosage approach, which we have previously established for determining the mutational status of fetuses for autosomal disease mutations. In this study, the relative mutation dosage method is used to deduce whether a fetus has inherited a hemophilia mutation on chromosome X by detecting whether the concentration of the mutant or wild-type allele is overrepresented in the plasma of heterozygous women carrying male fetuses. We correctly detected fetal genotypes for hemophilia mutations in all of the 12 studied maternal plasma samples obtained from at-risk pregnancies from as early as the 11th week of gestation. This development would make the decision to undertake prenatal testing less traumatic and safer for at-risk families.

Published
2011
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28. Codon optimization of human factor VIII cDNAs leads to high-level expression.

Author

Ward NJ, Buckley SM, Waddington SN, Vandendriessche T, Chuah MK, Nathwani AC, McIntosh J, Tuddenham EG, Kinnon C, Thrasher AJ, and McVey JH

Subjects
Amino Acid Sequence, Animals, Animals, Newborn, Enzyme-Linked Immunosorbent Assay, Factor VIII metabolism, Female, Gene Expression, Genetic Vectors administration & dosage, Genetic Vectors genetics, HEK293 Cells, Hemophilia A blood, Hemophilia A genetics, Humans, Injections, Intravenous, Lentivirus genetics, Male, Mice, Mice, 129 Strain, Mice, Knockout, Molecular Sequence Data, Mutation, Promoter Regions, Genetic genetics, Reverse Transcriptase Polymerase Chain Reaction, Sequence Homology, Amino Acid, Spleen Focus-Forming Viruses genetics, Codon genetics, Factor VIII genetics, Genetic Therapy methods, Hemophilia A therapy
Abstract

Gene therapy for hemophilia A would be facilitated by development of smaller expression cassettes encoding factor VIII (FVIII), which demonstrate improved biosynthesis and/or enhanced biologic properties. B domain deleted (BDD) FVIII retains full procoagulant function and is expressed at higher levels than wild-type FVIII. However, a partial BDD FVIII, leaving an N-terminal 226 amino acid stretch (N6), increases in vitro secretion of FVIII tenfold compared with BDD-FVIII. In this study, we tested various BDD constructs in the context of either wild-type or codon-optimized cDNA sequences expressed under control of the strong, ubiquitous Spleen Focus Forming Virus promoter within a self-inactivating HIV-based lentiviral vector. Transduced 293T cells in vitro demonstrated detectable FVIII activity. Hemophilic mice treated with lentiviral vectors showed expression of FVIII activity and phenotypic correction sustained over 250 days. Importantly, codon-optimized constructs achieved an unprecedented 29- to 44-fold increase in expression, yielding more than 200% normal human FVIII levels. Addition of B domain sequences to BDD-FVIII did not significantly increase in vivo expression. These significant findings demonstrate that shorter FVIII constructs that can be more easily accommodated in viral vectors can result in increased therapeutic efficacy and may deliver effective gene therapy for hemophilia A.

Published
2011
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29. Enhanced thrombin generation in patients with cirrhosis-induced coagulopathy.

Author

Gatt A, Riddell A, Calvaruso V, Tuddenham EG, Makris M, and Burroughs AK

Subjects
Aged, Anticoagulants therapeutic use, Blood Coagulation, Female, Fibrinolytic Agents therapeutic use, Hemorrhage, Humans, Intercellular Signaling Peptides and Proteins, International Normalized Ratio, Male, Middle Aged, Peptides therapeutic use, Risk, Blood Coagulation Disorders therapy, Fibrosis blood, Fibrosis therapy, Liver pathology, Protein C chemistry, Thrombin chemistry
Abstract

Background: Prothrombin time (PT) and the international normalized ratio (INR) are still routinely measured in patients with liver cirrhosis to 'assess' their bleeding risk despite the lack of correlation with the two. Thrombin generation (TG) assays are global assays of coagulation that are showing promise in assessing bleeding and thrombosis risks., Aim: To study the relationship between the INR and TG profiles in cirrhosis-induced coagulopathy., Methods: Seventy-three patients with cirrhosis were studied. All TG parameters were compared with those from a normal control group. Contact activation was prevented using corn trypsin inhibitor. TG was also assayed in the presence of Protac(®). The endogenous thrombin potential (ETP) ratio was derived by dividing the ETP with Protac® by the ETP without Protac®., Results: The INR (mean 1.7) did not correlate with the ETP and the velocity of TG (P > 0.05). There was no difference between the lag time and ETP of the two groups (P > 0.05). The velocity of TG was increased in cirrhosis (67.95 ± 34.8 vs. 45.05 ± 25.9 nM min⁻¹ ; P = 0.016) especially in patients with INRs between 1.21 and 2.0. Both the ETP with Protac(®) and the ETP ratio were increased in cirrhosis (mean 1074 ± 461.4 vs. 818 ± 357.9 nM min, P = 0.004 and 0.80 ± 0.21 vs. 0.44 ± 0.15, P ≤ 0.0001, respectively)., Conclusion: Despite a raised INR, TG parameters are consistent with a hypercoagulable profile in cirrhosis-related coagulopathy. This confirms that the PT or INR should not be used to assess bleeding risk in these patients, and other parameters, such as TG, need to be explored as clinical markers of coagulopathy., (© 2010 International Society on Thrombosis and Haemostasis.)

Published
2010
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30. Menorrhagia in adolescents with inherited bleeding disorders.

Author

Chi C, Pollard D, Tuddenham EG, and Kadir RA

Subjects
Adolescent, Child, Contraceptives, Oral, Hormonal therapeutic use, Female, Hemostatics therapeutic use, Humans, Menorrhagia drug therapy, Retrospective Studies, Young Adult, Blood Coagulation Disorders, Inherited complications, Blood Platelet Disorders complications, Menorrhagia etiology, Quality of Life
Abstract

Study Objectives: We reviewed the management and treatment outcomes of menorrhagia in adolescents with inherited bleeding disorders and assessed the impact of menorrhagia on their quality of life., Design: Retrospective review of case notes and a questionnaire study., Setting: Comprehensive-care hemophilia treatment center., Participants: Adolescents with inherited bleeding disorders who had registered at the center and were attending the multidisciplinary hemophilia and gynecology clinic for management of menorrhagia., Interventions: Review of medical records and assessment of menstrual blood loss using the pictorial blood assessment chart and quality of life measurements during menstruation using a questionnaire., Main Outcome Measures: Scores on pictorial blood assessment charts and quality of life measurements before and after treatment., Results: Of 153 girls aged 12 to 19 years who had registered at the center and had an inherited bleeding disorder, 42 (27%) attended the multidisciplinary clinic for management of menorrhagia. The majority (38/42; 90%) had experienced menorrhagia since menarche. Of the group, 5 (12%) required hospital admission for acute menorrhagia and severe anemia. Treatment options for menorrhagia included tranexamic acid, desmopressin, combined oral contraceptive pills, clotting factor concentrate, and the levonorgestrel intrauterine system. These treatment modalities, alone or in combination, were associated with a reduction in menstrual blood loss (median pre- and posttreatment pictorial blood assessment chart scores were 215 and 88, respectively) and improvement in quality of life scores (median pre- and posttreatment were 26 and 44, respectively)., Conclusions: Menorrhagia is a common symptom in adolescents with inherited bleeding disorders. It can present acutely, and it adversely affects quality of life. Treatment options include hemostatic and/or hormonal therapies and can improve the quality of life of affected girls., (Copyright 2010 North American Society for Pediatric and Adolescent Gynecology. Published by Elsevier Inc. All rights reserved.)

Published
2010
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31. Bernard Soulier syndrome in pregnancy: a systematic review.

Author

Peitsidis P, Datta T, Pafilis I, Otomewo O, Tuddenham EG, and Kadir RA

Subjects
Adult, Blood Transfusion statistics & numerical data, Female, Humans, Hysterectomy statistics & numerical data, Infant, Newborn, Platelet Count, Postpartum Hemorrhage epidemiology, Pregnancy, Pregnancy Outcome, Thrombocytopenia, Neonatal Alloimmune epidemiology, Young Adult, Bernard-Soulier Syndrome complications, Pregnancy Complications
Abstract

Bernard Soulier syndrome (BSS) is a rare disorder of platelets, inherited mainly as an autosomal recessive trait. It is characterised by qualitative and quantitative defects of the platelet membrane glycoprotein (GP) Ib-IX-V complex. The main clinical characteristics are thrombocytopenia, prolonged bleeding time and the presence of giant platelets. Data on the clinical course and outcome of pregnancy in women with Bernard Soulier syndrome is scattered in individual case reports. In this paper, we performed a systematic review of literature and identified 16 relevant articles; all case reports that included 30 pregnancies among 18 women. Primary postpartum haemorrhage was reported in 10 (33%) and secondary in 12 (40%) of pregnancies, requiring blood transfusion in 15 pregnancies. Two women had an emergency obstetric hysterectomy. Alloimmune thrombocytopenia was reported in 6 neonates, with one intrauterine death and one neonatal death. Bernard Soulier syndrome in pregnancy is associated with a high risk of serious bleeding for the mother and the neonate. A multidisciplinary team approach and individualised management plan for such women are required to minimise these risks. An international registry is recommended to obtain further knowledge in managing women with this rare disorder.

Published
2010
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32. Structural analysis of eight novel and 112 previously reported missense mutations in the interactive FXI mutation database reveals new insight on FXI deficiency.

Author

Saunders RE, Shiltagh N, Gomez K, Mellars G, Cooper C, Perry DJ, Tuddenham EG, and Perkins SJ

Subjects
Amino Acid Sequence, Amino Acid Substitution, Base Sequence, Crystallography, X-Ray, DNA genetics, Databases, Genetic, Dimerization, Factor XI Deficiency blood, Genes, Dominant, Humans, Models, Molecular, Molecular Sequence Data, Phenotype, Polymorphism, Single Nucleotide, Protein Folding, Protein Structure, Quaternary, Protein Structure, Tertiary, Sequence Homology, Amino Acid, Factor XI chemistry, Factor XI genetics, Factor XI Deficiency genetics, Mutation, Missense
Abstract

Factor XI (FXI) functions in blood coagulation. FXI is composed of four apple (Ap) domains and a serine protease (SP) domain. Deficiency of FXI leads to an injury-related bleeding disorder, which is remarkable for the lack of correlation between bleeding symptoms and FXI coagulant activity (FXI:C). The number of mutations previously reported in our interactive web database (http://www.FactorXI.org) is now significantly increased to 183 through our new patient studies and from literature surveys. Eight novel missense mutations give a total of 120 throughout the FXI gene (F11). The most abundant defects in FXI are revealed to be those from low-protein plasma levels (Type I: CRM-) that originate from protein misfolding, rather than from functional defects (Type II: CRM+). A total of 70 Ap missense mutations were analysed using a consensus Ap domain structure generated from the FXI dimer crystal structure. This showed that all parts of the Ap domain were affected. The 47 SP missense mutations were also distributed throughout the SP domain structure. The periphery of the Ap beta-sheet structure is sensitive to structural perturbation caused by residue changes throughout the Ap domain, yet this beta-sheet is crucial for FXI dimer formation. Residues located at the Ap4:Ap4 interface in the dimer are much less directly involved. We conclude that the abundance of Type I defects in FXI results from the sensitivity of the Ap domain folding to residue changes within this, and discuss how structural knowledge of the mutations improves our understanding of FXI deficiencies.

Published
2009
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33. Optimizing warfarin reversal--an ex vivo study.

Author

Gatt A, Riddell A, van Veen JJ, Kitchen S, Tuddenham EG, and Makris M

Subjects
Humans, International Normalized Ratio, Anticoagulants therapeutic use, Warfarin therapeutic use
Abstract

Background: Warfarin reversal is a common clinical situation. This is commonly performed using vitamin K and, depending on the urgency, fresh frozen plasma (FFP), prothrombin complex concentrates (PCCs), or activated factor VII. Even though PCCs are widely used, the ideal dosing regimen is far from established., Objectives: To verify differences in warfarin reversal patterns using FFP, recombinant FVIIa (rFVIIa), and PCC; and to test the hypothesis that supratherapeutic International Normalized Ratios (INRs) might not correlate with thrombin generation (TG) and identify the ideal concentrations of PCC required to reverse various INR thresholds., Methods: We studied the effects of FFP, rFVIIa and Beriplex P/N on the INR and TG, using the calibrated automated thrombography assay in ex vivo warfarinized plasma. Plasmas with different INRs were spiked with different concentrations of Beriplex P/N., Results: Beriplex P/N was the only agent that completely normalized TG and the INR. The endogenous thrombin potential (ETP) and the peak thrombin showed a significant negative correlation with all INRs. The ETP and velocity of TG reached a plateau at an INR of approximately 4.0. A concentration equivalent to a dose of 30 IU kg(-1) Beriplex P/N normalized the ETP, the INR, FII, FVII, FIX and FX of samples with INRs > or = 4.0. Higher doses resulted in hypercoagulable TG patterns. A concentration equivalent to a dose of 20 IU kg(-1) was sufficient to reverse warfarin at an INR range of 2.0-3.9, as judged by the same tests., Conclusions: Warfarin reversal algorithms could be simplified with the adoption of this strategy utilizing two doses of PCC, depending on the INR of the patient. This would also lead to cost reductions and, possibly, a reduction in thrombotic risk.

Published
2009
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34. Alpha1-antitrypsin Pittsburgh in a family with bleeding tendency.

Author

Hua B, Fan L, Liang Y, Zhao Y, and Tuddenham EG

Subjects
Adolescent, Adult, Blood Coagulation Tests, Blood Protein Electrophoresis, DNA Mutational Analysis, Factor X metabolism, Factor XI metabolism, Factor XII metabolism, Family Health, Female, Hemorrhagic Disorders blood, Hemorrhagic Disorders diagnosis, Heterozygote, Humans, Male, Pedigree, Hemorrhagic Disorders genetics, Mutation, alpha 1-Antitrypsin genetics
Abstract

We describe a 16-year-old girl and her 41-year-old father who both had a bleeding tendency, dramatic prolongation of all standard clotting assays, undetectable levels of plasma protein C activity, and low or borderline levels of factors X, XI and XII. Plasma and serum electrophoresis revealed a minor peak following the main alpha(1) globulin peak, of which the proportion was increased. Platelet aggregation by thrombin (final concentration 1 U/mL) was absent in both patients, but this inhibition can be overcome by increasing the concentration of thrombin (4 U/mL). The molecular defect responsible for these coagulation abnormalities was identified by genomic sequencing. Both patients are heterozygous for alpha(1)-antitrypsin Met 358 to Arg (alpha(1)-antitrypsin Pittsburgh). Seven other members of this pedigree had normal coagulation tests and do not carry the same genetic mutation. This unique family with alpha1-antitrypsin Pittsburgh sheds some light on the study of this extremely rare mutation and its inheritance.

Published
2009
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35. Consensus protocol for the use of recombinant activated factor VII [eptacog alfa (activated); NovoSeven] in elective orthopaedic surgery in haemophilic patients with inhibitors.

Author

Giangrande PL, Wilde JT, Madan B, Ludlam CA, Tuddenham EG, Goddard NJ, Dolan G, and Ingerslev J

Subjects
Adolescent, Adult, Aged, Blood Loss, Surgical prevention & control, Child, Child, Preschool, Clinical Protocols, Elective Surgical Procedures, Hemophilia A complications, Humans, Middle Aged, Orthopedic Procedures adverse effects, Treatment Outcome, Young Adult, Consensus Development Conferences as Topic, Factor VIIa therapeutic use, Hemophilia A drug therapy, Joint Diseases surgery, Postoperative Hemorrhage prevention & control, Recombinant Proteins therapeutic use
Abstract

Patients with haemophilia complicated by inhibitors have a significant burden of joint disease, which is associated with a negative impact on their quality of life. Successful elective orthopaedic surgery can result in decreased bleed frequency into a new joint, less time spent in hospital, increased mobility and improved well being. This paper describes a new protocol for use of recombinant activated factor VII (rFVIIa) in elective orthopaedic surgery, based on a review of published data as well as the personal experience of a group of expert physicians. The protocol offers guidance on the planning of the surgery and preoperative testing as well as the bolus schedule for rFVIIa and advice on the concomitant use of antifibrinolytic agents and fibrin sealants. A total of 10 operations involving 13 procedures in eight patients in five comprehensive care centres have been undertaken until now using the protocol, which employs an initial bolus dose of rFVIIa in the range of 120-180 microg kg(-1) to cover surgery. The clinical experience reported here encompasses all cases of elective orthopaedic surgery using rFVIIa as initial treatment carried out in the UK and Republic of Ireland over the last 2 years. In all cases, there was good control of haemostasis during surgery and the final outcome was rated as 'excellent' or 'extremely satisfactory' by the reporting clinicians. Although the initial cost of product to cover surgery such as arthroplasty is high, it needs to be borne in mind that this may be offset in subsequent years by savings resulting from avoidance of bleeding episodes in the affected joint.

Published
2009
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39. Genetic aspects and research development in haemostasis.

Author

Tuddenham EG, Ingerslev J, Sørensen LN, Christiansen K, Mariani G, Peyvandi F, Waddington SN, Buckley SM, Kochanek S, Chuah MK, Vandendriessche T, and Berntorp E

Subjects
Cohort Studies, Factor VII genetics, Factor VII Deficiency genetics, Genetic Therapy trends, Hemostasis genetics, Humans, Polymorphism, Single Nucleotide genetics, Blood Coagulation Factor Inhibitors genetics, Factor VII Deficiency complications, Hemostasis physiology, Polymorphism, Single Nucleotide physiology
Published
2008
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41. Genotype-phenotype correlation in combined deficiency of factor V and factor VIII.

Author

Zhang B, Spreafico M, Zheng C, Yang A, Platzer P, Callaghan MU, Avci Z, Ozbek N, Mahlangu J, Haw T, Kaufman RJ, Marchant K, Tuddenham EG, Seligsohn U, Peyvandi F, and Ginsburg D

Subjects
Animals, Blood Platelets physiology, COS Cells, Chlorocebus aethiops, Factor V metabolism, Factor V Deficiency blood, Factor VIII metabolism, Family Health, Female, Gene Deletion, Genes, Recessive, Genotype, Hemophilia A blood, Humans, Male, Mannose-Binding Lectins metabolism, Membrane Proteins metabolism, Mutation, Missense, Phenotype, Vesicular Transport Proteins metabolism, Factor V Deficiency genetics, Hemophilia A genetics, Mannose-Binding Lectins genetics, Membrane Proteins genetics, Vesicular Transport Proteins genetics
Abstract

Combined deficiency of factor V and factor VIII (F5F8D) is caused by mutations in one of 2 genes, either LMAN1 or MCFD2. Here we report the identification of mutations for 11 additional F5F8D families, including 4 novel mutations, 2 in MCFD2 and 2 in LMAN1. We show that a novel MCFD2 missense mutation identified here (D81Y) and 2 previously reported mutations (D89A and D122V) abolish MCFD2 binding to LMAN1. Measurement of platelet factor V (FV) levels in 7 F5F8D patients (4 with LMAN1 and 3 with MCFD2 mutations) demonstrated similar reductions to those observed for plasma FV. Combining the current data together with all previous published reports, we performed a genotype-phenotype analysis comparing patients with MCFD2 mutations with those with LMAN1 mutations. A previously unappreciated difference is observed between these 2 classes of patients in the distribution of plasma levels for FV and factor VIII (FVIII). Although there is considerable overlap, the mean levels of plasma FV and FVIII in patients with MCFD2 mutations are significantly lower than the corresponding levels in patients with LMAN1 mutations. No differences in distribution of factor levels are observed by sex. These data suggest that MCFD2 may play a primary role in the export of FV and FVIII from the ER, with the impact of LMAN1 mediated indirectly through its interaction with MCFD2.

Published
2008
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42. Safe and efficient transduction of the liver after peripheral vein infusion of self-complementary AAV vector results in stable therapeutic expression of human FIX in nonhuman primates.

Author

Nathwani AC, Gray JT, McIntosh J, Ng CY, Zhou J, Spence Y, Cochrane M, Gray E, Tuddenham EG, and Davidoff AM

Subjects
Animals, Antibody Formation, Factor IX pharmacokinetics, Genetic Vectors pharmacokinetics, Humans, Macaca, Tissue Distribution, Treatment Outcome, Factor IX administration & dosage, Genetic Therapy methods, Genetic Vectors administration & dosage, Hemophilia B therapy, Liver metabolism, Transduction, Genetic methods
Abstract

The safety and efficacy of peripheral venous administration of a self-complementary adeno-associated viral vector encoding the human FIX gene (scAAV-LP1-hFIXco) was evaluated in nonhuman primates for gene therapy of hemophilia B. Peripheral vein infusion of 1x10(12) vg/kg scAAV-LP1-hFIXco pseudotyped with serotype 8 capsid, in 3 macaques, resulted in stable therapeutic expression (more than 9 months) of human FIX (hFIX) at levels (1.1+/-0.5 microg/mL, or 22% of normal) that were comparable to those achieved after direct delivery of the same vector dose into the portal circulation (1.3+/-0.3 microg/mL, or 26% of normal). Importantly, the pattern of vector biodistribution after systemic and portal vein administration of scAAV-LP1-hFIXco was almost identical. Additionally, comparable levels of gene transfer were achieved in macaques with preexisting immunity to AAV8 following peripheral vein administration of 1x10(12) vg/kg AAV5-pseudotyped scAAV-LP1-hFIXco. This confirms that alternative serotypes can circumvent preexisting naturally acquired immunity to AAV. Thus, peripheral venous administration of AAV5 and AAV8 vectors is safe and as effective at transducing the liver in nonhuman primates as direct vector administration into the portal circulation. These results should make vector administration to patients, especially those with a severe bleeding diathesis, significantly easier and safer.

Published
2007
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43. Identification of factor IX mutations in Iranian haemophilia B patients by SSCP and sequencing.

Author

Karimipoor M, Zeinali S, Nafissi N, Tuddenham EG, Lak M, and Safaee R

Subjects
Amino Acid Sequence, Genotype, Humans, Iran, Polymerase Chain Reaction, Factor IX genetics, Hemophilia B genetics, Molecular Sequence Data, Point Mutation, Polymorphism, Single-Stranded Conformational
Abstract

Different kinds of mutations, mostly point mutations, in the coagulation factor IX (FIX) gene F9 result in a recessive X-linked bleeding disorder known as haemophilia B. In this study, molecular analysis of 76 unrelated Iranian haemophilia B patients was performed by PCR, single strand conformational polymorphism (SSCP) on important functional regions of the F9 gene followed by sequencing on samples with different migration pattern. Using this approach we found mutation in 52 out of 76 patients. Our data showed that the pathologic mechanisms are heterogeneous as recorded for patients in haemophilia B mutation database and seven of the mutations are previously undescribed.

Published
2007
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44. Postinjury vascular intimal hyperplasia in mice is completely inhibited by CD34+ bone marrow-derived progenitor cells expressing membrane-tethered anticoagulant fusion proteins.

Author

Chen D, Weber M, Shiels PG, Dong R, Webster Z, McVey JH, Kemball-Cook G, Tuddenham EG, Lechler RI, and Dorling A

Subjects
Animals, Aorta metabolism, Arteriosclerosis therapy, Blood Vessels pathology, Carotid Arteries pathology, Humans, Inflammation, Mice, Mice, Transgenic, Muscle, Smooth metabolism, Phenotype, Anticoagulants metabolism, Antigens, CD34 biosynthesis, Bone Marrow Cells metabolism, Cell Membrane metabolism, Gene Expression Regulation, Recombinant Fusion Proteins metabolism, Stem Cells metabolism
Abstract

Background: Coagulation proteins promote neointimal hyperplasia and vascular remodelling after vessel injury, but the precise mechanisms by which they act in vivo remain undetermined., Objectives: This study, using an injury model in which the neointima is derived from bone marrow (BM)-derived cells, compared inhibition of tissue factor or thrombin on either BM-derived or existing vascular smooth muscle cells., Methods: Two transgenic (Tg) mouse strains expressing membrane-tethered tissue factor pathway inhibitor (TFPI) or hirudin (Hir) fusion proteins driven by an alpha smooth muscle actin (SMA) promoter were generated (alpha-TFPI-Tg and alpha-Hir-Tg) and the phenotype after wire-induced endovascular injury was compared with that in wild-type (WT) controls., Results: WT mice developed progressive neointimal expansion, whereas injury in either Tg was followed by repair back to a preinjured state. This was also seen when WT mice were reconstituted with BM from Tg mice but not when Tgs were reconstituted with WT BM, in which injury was followed by slowly progressive neointimal expansion. Injection of CD34+ cells from Tg mice into injured WT mice resulted in the accumulation of fusion protein-expressing cells from day 3 onwards and an absence of neointimal hyperplasia in those areas., Conclusions: Neointimal development after wire-induced endovascular injury in mice was completely inhibited when BM-derived cells infiltrating the damaged artery expressed membrane tethered anticoagulant fusion proteins under an alpha-SMA promoter. These findings enhance our understanding of the pathological role that coagulation proteins play in vascular inflammation.

Published
2006
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45. Detection of functional differences between different platelet membrane glycoprotein Ibalpha variable number tandem repeat and Kozak genotypes as shown by the PFA-100 system.

Author

Douglas H, Davies GJ, Michaelides K, Gorog DA, Timlin H, Ahmed N, and Tuddenham EG

Subjects
Aspirin pharmacology, Enzyme-Linked Immunosorbent Assay, Genotype, Humans, Male, Middle Aged, Platelet Aggregation Inhibitors pharmacology, Platelet Function Tests methods, Platelet Glycoprotein GPIb-IX Complex genetics, Tandem Repeat Sequences genetics
Published
2006
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46. Self-complementary adeno-associated virus vectors containing a novel liver-specific human factor IX expression cassette enable highly efficient transduction of murine and nonhuman primate liver.

Author

Nathwani AC, Gray JT, Ng CY, Zhou J, Spence Y, Waddington SN, Tuddenham EG, Kemball-Cook G, McIntosh J, Boon-Spijker M, Mertens K, and Davidoff AM

Subjects
Animals, Dependovirus genetics, Genetic Therapy methods, Genetic Vectors, Genome, Viral, Humans, Macaca mulatta, Male, Mice, Primates, Transduction, Genetic methods, Dependovirus physiology, Factor IX genetics, Hemophilia B therapy, Liver physiology, Liver virology
Abstract

Transduction with recombinant adeno-associated virus (AAV) vectors is limited by the need to convert its single-stranded (ss) genome to transcriptionally active double-stranded (ds) forms. For AAV-mediated hemophilia B (HB) gene therapy, we have overcome this obstacle by constructing a liver-restricted mini-human factor IX (hFIX) expression cassette that can be packaged as complementary dimers within individual AAV particles. Molecular analysis of murine liver transduced with these self-complementary (sc) vectors demonstrated rapid formation of active ds-linear genomes that persisted stably as concatamers or monomeric circles. This unique property resulted in a 20-fold improvement in hFIX expression in mice over comparable ssAAV vectors. Administration of only 1 x 10(10) scAAV particles led to expression of hFIX at supraphysiologic levels (8I U/mL) and correction of the bleeding diathesis in FIX knock-out mice. Of importance, therapeutic levels of hFIX (3%-30% of normal) were achieved in nonhuman primates using a significantly lower dose of scAAV than required with ssAAV. Furthermore, AAV5-pseudotyped scAAV vectors mediated successful transduction in macaques with pre-existing immunity to AAV8. Hence, this novel vector represents an important advance for hemophilia B gene therapy.

Published
2006
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47. Combined deficiency of factor V and factor VIII is due to mutations in either LMAN1 or MCFD2.

Author

Zhang B, McGee B, Yamaoka JS, Guglielmone H, Downes KA, Minoldo S, Jarchum G, Peyvandi F, de Bosch NB, Ruiz-Saez A, Chatelain B, Olpinski M, Bockenstedt P, Sperl W, Kaufman RJ, Nichols WC, Tuddenham EG, and Ginsburg D

Subjects
Alleles, Blotting, Western methods, Carrier Proteins metabolism, DNA Mutational Analysis methods, Endoplasmic Reticulum genetics, Endoplasmic Reticulum metabolism, Factor V metabolism, Factor V Deficiency metabolism, Factor VIII metabolism, Golgi Apparatus genetics, Golgi Apparatus metabolism, Hemophilia A metabolism, Humans, Mannose-Binding Lectins metabolism, Membrane Proteins metabolism, Multiprotein Complexes genetics, Multiprotein Complexes metabolism, Protein Transport genetics, RNA, Messenger genetics, RNA, Messenger metabolism, Vesicular Transport Proteins, Amino Acid Substitution, Carrier Proteins genetics, Factor V Deficiency genetics, Hemophilia A genetics, Mannose-Binding Lectins genetics, Membrane Proteins genetics, Mutation, Missense, Point Mutation
Abstract

Mutations in LMAN1 (ERGIC-53) or MCFD2 cause combined deficiency of factor V and factor VIII (F5F8D). LMAN1 and MCFD2 form a protein complex that functions as a cargo receptor ferrying FV and FVIII from the endoplasmic reticulum to the Golgi. In this study, we analyzed 10 previously reported and 10 new F5F8D families. Mutations in the LMAN1 or MCFD2 genes accounted for 15 of these families, including 3 alleles resulting in no LMAN1 mRNA accumulation. Combined with our previous reports, we have identified LMAN1 or MCFD2 mutations as the causes of F5F8D in 71 of 76 families. Among the 5 families in which no mutations were identified, 3 were due to misdiagnosis, with the remaining 2 likely carrying LMAN1 or MCFD2 mutations that were missed by direct sequencing. Our results suggest that mutations in LMAN1 and MCFD2 may account for all cases of F5F8D. Immunoprecipitation and Western blot analysis detected a low level of LMAN1-MCFD2 complex in lymphoblasts derived from patients with missense mutations in LMAN1 (C475R) or MCFD2 (I136T), suggesting that complete loss of the complex may not be required for clinically significant reduction in FV and FVIII.

Published
2006
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48. Live birth following the first mutation specific pre-implantation genetic diagnosis for haemophilia A.

Author

Michaelides K, Tuddenham EG, Turner C, Lavender B, and Lavery SA

Subjects
Adult, DNA Mutational Analysis, Embryo Transfer, Family Health, Female, Humans, Live Birth, Polymerase Chain Reaction, Pregnancy, Factor VIII genetics, Hemophilia A diagnosis, Mutation, Preimplantation Diagnosis
Abstract

Haemophilia A is an X-linked, recessive, inherited bleeding disorder which affects 1 in 5000 males born worldwide. It is caused by mutations in the FactorVIII (F8) gene on chromosome Xq28. We describe for the first time two mutation specific, single cell protocols for pre-implantation genetic diagnosis (PGD) of haemophilia. A that enable the selection of both male and female unaffected embryos. This approach offers an alternative to sexing, frequently used for X-linked disorders, that results in the discarding of all male embryos including the 50% that would have been normal. Two families with a history of severe haemophilia. A requested carrier diagnosis and subsequently proceeded to PGD. The mutation in family 1 is a single nucleotide substitution c.5953C > T, R1966X in exon 18 and in family 2, c.5122C > T, R1689C in exon 14 of the F8 gene. Amplification efficiency was compared between distilled water and SDS/proteinase K cell lysis (98.0%, 96/98 and 80%, 112/140 respectively) using 238 single lymphocytes. Blastomeres from spare IVF cleavage-stage embryos donated for research showed amplification efficiencies of 83.3% (45/54) for the R1966X and 92.9% (13/14) for the R1689C mutations. The rate of allele dropout (ADO) on heterozygous lymphocytes was 1.1% (1/93) for R1966X and 5.94% (6/101) for R1689C mutations. A single PGD treatment cycle for family 1 resulted in two embryos for transfer but these failed to implant. However, with family 2, two embryos were transferred to the uterus on day 4 resulting in a successful singleton pregnancy and subsequent live birth of a normal non-carrier female.

Published
2006
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49. Ways to bypass a blocked tenase complex.

Author

Tuddenham EG

Subjects
Animals, Anticoagulants pharmacology, Anticoagulants therapeutic use, Autoantibodies blood, Blood Coagulation drug effects, Hemophilia A blood, Hemophilia A drug therapy, Humans, Lipoproteins antagonists & inhibitors, Mice, Neoplasm Proteins antagonists & inhibitors, Pentosan Sulfuric Polyester pharmacology, Pentosan Sulfuric Polyester therapeutic use, Polysaccharides pharmacology, Polysaccharides therapeutic use, Cysteine Endopeptidases immunology, Factor IXa immunology, Factor VIIIa immunology, Neoplasm Proteins immunology
Published
2006

50. A common ancestral glycoprotein (GP) 9 1828A>G (Asn45Ser) gene mutation occurring in European families from Australia and Northern Europe with Bernard-Soulier Syndrome (BSS).

Author

Liang HP, Morel-Kopp MC, Clemetson JM, Clemetson KJ, Kekomaki R, Kroll H, Michaelides K, Tuddenham EG, Vanhoorelbeke K, and Ward CM

Subjects
Alleles, Amino Acid Substitution, Australia ethnology, Bernard-Soulier Syndrome ethnology, Europe epidemiology, Europe ethnology, Founder Effect, Haplotypes, Heredity, Heterozygote, Homozygote, Humans, Mutation, Polymorphism, Single Nucleotide, Selection, Genetic, Time Factors, Bernard-Soulier Syndrome genetics, Evolution, Molecular, Platelet Glycoprotein GPIb-IX Complex genetics
Abstract

Bernard-Soulier syndrome (BSS) is an extremely rare hereditary bleeding disorder, caused by mutations occurring in the Glycoprotein (GP) Ibalpha, GPIbbeta and GP9 genes that encode for the corresponding subunits of platelet GPIb-V-IX adhesion receptor complex. BSS has been reported in many populations, mostly behaving in an autosomal-recessive manner.While the great majority of BSS mutations are unique to a single individual or family, the GP9 1828A>G Asn45Ser mutation, which we have identified in an undocumented Australian Caucasian, has already been reported in multiple unrelated Caucasian families from various Northern and Central European countries. Haplotype analysis of 19 BSS patients from 15 unrelated Northern European families (including 2 compound heterozygote siblings from a British family previously published, and 17 1828A>G Asn45Ser homozygotes), showed that 14 of these BSS patients from 11 of the 1828A>G Asn45Ser homozygote families share a common haplotype at the chromosomal region 3' to the GP9 gene. Hence, the results suggest that the GP9 1828A>GAsn45Ser mutation in these families is ancient, and its frequent emergence in the European population is the result of a founder effect rather than recurrent mutational events. Association of the 1828A>G Asn45Ser mutation with variant haplotypes in 4 other Northern European BSS families raised the possibility of a second founder event, or rare recombinations in these families. Additional members from these 'atypical' lineages would need to be screened to resolve this question.

Published
2005
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