Your search keyword '"Dixon, P H"' showing total 4 results

1. Contribution of variant alleles of ABCB11 to susceptibility to intrahepatic cholestasis of pregnancy.

Author

Dixon, P. H., van Mil, S. W. C., Chambers, J., Strautnieks, S., Thompson, R. J., Lammert, F., Kubitz, R., Keitel, V., Glantz, A., Mattsson, L.-Å., Marschall, H.-U., Molokhia, M., Moore, G. E., Linton, K. J., and Williamson, C.

Subjects

*CHOLESTASIS, *PREGNANT women, *ETIOLOGY of diseases, *GENETIC mutation, *GENETIC polymorphisms, *GENE frequency, *DNA, *GENETICS

Abstract

Background: Intrahepatic cholestasis of pregnancy (ICP) has a complex aetiology with a significant genetic component. ABCB11 encodes the bile salt export pump (BSEP); mutations cause a spectrum of cholestatic disease, and are implicated in the aetiology of ICP. Methods: ABCB11 variation in ICP was investigated by screening for five mutant alleles (E297G, D482G, N591S, D676Y and G855R) and the V444A polymorphism (c.1331T>C, rs2287622) in two ICP cohorts (n = 333 UK, n = 158 continental Europe), and controls (n = 261) for V444A. PCR primers were used to amplify and sequence patient and control DNA. The molecular basis for the observed phenotypes was investigated in silico by analysing the equivalent residues in the structure of the homologous bacterial transporter Sav1866. Results: E297G was observed four times and D482G once. N591S was present in two patients; D676Y and G855R were not observed. The V444A polymorphism was associated with ICP (allelic analysis for C vs T: OR 1.7 (95% CI 1.4 to 2.1, p<0.001)). In addition, CC homozygotes were more likely to have ICP than TT homozygotes: OR 2.8 (95% CI 1.7 to 4.4 p<0.0001). Structural analyses suggest that E297G and D482G destabilise the protein fold of BSEP. The molecular basis of V444A and N591S was not apparent from the Sav1866 structure. Conclusions: Heterozygosity for the common ABCB11 mutations accounts for 1% of European ICP cases; these two mutants probably reduce the folding efficiency of BSEP. N591S is a recurrent mutation; however, the mechanism may be independent of protein stability or function. The V444A polymorphism is a significant risk factor for ICP in this population. [ABSTRACT FROM AUTHOR]

Published

2009

2. Complementary Functions of the Flippase ATP8B1 and the Floppase ABCB4 in Maintaining Canalicular Membrane Integrity.

Author

Groen, Annemiek, Romero, Marta Rodriguez, Kunne, Cindy, Hoosdally, Sarah J., Dixon, Peter H., Wooding, Carol, Williamson, Catherine, Seppen, Jurgen, van den Oever, Karin, Mok, Kam S., Paulusma, Coen C., Linton, Kenneth J., and Oude Elferink, Ronald P.J.

Subjects

FAMILIAL diseases, DISEASE progression, CELL membranes, GENETIC mutation, PHOSPHOLIPIDS, CHROMOSOMAL translocation, LACTATE dehydrogenase, PHOSPHATIDYLSERINES

Abstract

Background & Aims: Progressive familial intrahepatic cholestasis can be caused by mutations in ABCB4 or ATP8B1; each encodes a protein that translocates phospholipids, but in opposite directions. ABCB4 flops phosphatidylcholine from the inner to the outer leaflet, where it is extracted by bile salts. ATP8B1, in complex with the accessory protein CDC50A, flips phosphatidylserine in the reverse direction. Abcb4 −/− mice lack biliary secretion of phosphatidylcholine, whereas Atp8b1-deficient mice have increased excretion of phosphatidylserine into bile. Each system is thought to have a role protecting the canalicular membrane from bile salts. Methods: To investigate the relationship between the mechanisms of ABCB4 and ATP8B1, we expressed the transporters separately and together in cultured cells and studied viability and phospholipid transport. We also created mice with disruptions in ABCB4 and ATP8B1 (double knockouts) and studied bile formation and hepatic damage in mice fed bile salts. Results: Overexpression of ABCB4 was toxic to HEK293T cells; the toxicity was counteracted by coexpression of the ATP8B1–CDC50A complex. In Atp8b1-deficient mice, bile salts induced extraction of phosphatidylserine and ectoenzymes from the canalicular membrane; this process was not observed in the double-knockout mice. Conclusions: ATP8B1 is required for hepatocyte function, particularly in the presence of ABCB4. This is most likely because the phosphatidylserine flippase complex of ATP8B1–CDC50A counteracts the destabilization of the membrane that occurs when ABCB4 flops phosphatidylcholine. Lipid asymmetry is therefore important for the integrity of the canalicular membrane; ABCB4 and ATP8B1 cooperate to protect hepatocytes from bile salts. [ABSTRACT FROM AUTHOR]

Published

2011

3. Identification of 13 novel NLRP7 mutations in 20 families with recurrent hydatidiform mole; missense mutations cluster in the leucine-rich region.

Author

Wang, C. M., Dixon, P. H., Decordova, S., Hodges, M. D., Sebire, N. J., Ozalp, S., Fallahian, M., Sensi, A., Ashrafi, F., Repiska, V., Zhao, J., Xiang, Y., Savage, P. M., Seckl, M. J., and Fisher, R. A.

Subjects

GENETIC mutation, LEUCINE, NEVUS, PREGNANCY, AMINO acids, DNA

Abstract

Background: NLRP7 (NALP7) has recently been identified as the causative gene for familial recurrent hydatidiform mole (FRHM), a rare autosomal recessive condition in which affected women have recurrent molar pregnancies of diploid biparental origin. To date only a small number of affected families have been described. Our objectives were to investigate the diversity of mutations and their localisation to one or both isoforms of NLRP7, by screening a large series of women with FRHM and to examine the normal expression of NLRP7 in ovarian tissue. Methods: Fluorescent microsatellite genotyping of molar tissue was used to establish a diagnosis of FRHM. Twenty families were subsequently screened for mutations in NLRP7 using DNA sequencing. Expression of NLRP7 in the ovary was examined by immunohistochemical staining. Results: 16 different mutations were identified in the study, 13 of which were novel. Missense mutations were found to be present in transcript variant 2 of NLRP7 and cluster in the leucine-rich region (LRR). A man with two affected sisters and homozygous for the p.R693P mutation had normal reproductive outcomes. In the normal human ovary, NLRP7 expression is confined to the oocytes and present at all stages from primordial to tertiary follicles. Conclusion: 13 novel mutations in NLRP7 were identified. We confirm that mutations in NLRP7 affect female but not male reproduction, and provide evidence that transcript variant 2 of NLRP7 is the important isoform in this condition. The mutation clustering seen confirms that the LRR is critical for normal functioning of NLRP7. [ABSTRACT FROM AUTHOR]

Published

2009

4. Obstetric cholestasis caused by a novel mutation in the MDR3 gene which causes abnormal protein folding and trafficking.

Author

Williamson, C., Weerasekera, N., Linton, K. J., Dixon, P. H., Chambers, J., Elias, E., Weaver, J., Nelson-Piercy, C., Higgins, C. F., De Swiet, M., and McCarthy, M. I.

Subjects

CHOLESTASIS, MULTIDRUG resistance, GENETIC mutation, PROTEIN folding

Abstract

The article presents an abstract of the research paper "Obstetric cholestasis caused by a novel mutation in the MDR3 gene which causes abnormal protein folding and trafficking," by C. Williamson, N. Weerasekera, K. J. Linton, P. H. Dixon, J. Chambers, E. Elias, J. Weaver, C. Nelson-Piercy, C. F. Higgins, M. de Swiet, and M. I. McCarthy. Analysis indicates that loss-of-function multidrug resistance 3 mutations may be responsible for obstetric cholestasis in a subgroup of women with raised GGT.

Published

2000