Your search keyword '"Whittall, Ros"' showing total 10 results

1. Analysis of the frequency and spectrum of mutations recognised to cause familial hypercholesterolaemia in routine clinical practice in a UK specialist hospital lipid clinic.

Author

Futema, Marta, Whittall, Ros A., Kiley, Amy, Steel, Louisa K., Cooper, Jackie A., Badmus, Ebele, Leigh, Sarah E., Karpe, Fredrik, Neil, H. Andrew W., and Humphries, Steve E.

Subjects

*GENETIC mutation, *HYPERCHOLESTEREMIA, *PHYSICIAN practice patterns, *LIPID analysis, *CHOLESTEROL, *TRIGLYCERIDES

Abstract

Abstract: Aim: To determine the frequency and spectrum of mutations causing Familial Hypercholesterolaemia (FH) in patients attending a single UK specialist hospital lipid clinic in Oxford and to identify characteristics contributing to a high mutation detection rate. Methods: 289 patients (272 probands) were screened sequentially over a 2-year period for mutations in LDLR, APOB and PCSK9 using standard molecular genetic techniques. The Simon Broome (SB) clinical diagnostic criteria were used to classify patients and a separate cohort of 409 FH patients was used for replication. Results: An FH-causing mutation was found in 101 unrelated patients (LDLR = 54 different mutations, APOB p.(Arg3527Gln) = 10, PCSK9 p.(Asp374Tyr) = 0). In the 60 SB Definite FH patients the mutation detection rate was 73% while in the 142 with Possible FH the rate was significantly lower (27%, p < 0.0001), but similar (14%, p = 0.06) to the 70 in whom there was insufficient data to make a clinical diagnosis. The mutation detection rate varied significantly (p = 9.83 × 10−5) by untreated total cholesterol (TC) levels (25% in those <8.1 mmol/l and 74% in those >10.0 mmol/l), and by triglyceride levels (20% in those >2.16 mmol/l and 60% in those <1.0 mmol/l (p = 0.0005)), with both effects confirmed in the replication sample (p for trend = 0.0001 and p = 1.8 × 10−6 respectively). There was no difference in the specificity or sensitivity of the SB criteria versus the Dutch Lipid Clinic Network score in identifying mutation carriers (AROC respectively 0.73 and 0.72, p = 0.68). Conclusions: In this genetically heterogeneous cohort of FH patients the mutation detection rate was significantly dependent on pre-treatment TC and triglyceride levels. [Copyright &y& Elsevier]

Published

2013

2. The genetic spectrum of familial hypercholesterolemia in Pakistan.

Author

Ahmed, Waqas, Whittall, Ros, Riaz, Moeen, Ajmal, Muhammad, Sadeque, Ahmed, Ayub, Humaira, Qamar, Raheel, and Humphries, Steve E.

Subjects

*HYPERCHOLESTEREMIA, *AUTOSOMAL recessive polycystic kidney, *LOW density lipoprotein receptors, *PROPROTEIN convertases, *DYSLIPIDEMIA

Abstract

Abstract: Background: Familial hypercholesterolemia (FH) is an autosomal dominant disease caused by mutations in the genes coding for the low density lipoprotein receptor (LDLR), proprotein convertase subtilisin/kexin type-9 (PCSK9) or apo-lipoprotein B-100 (APOB). The aim of the present work was to determine the genetic basis of dyslipidemia in 11 unrelated Pakistani families. Methods: High resolution melting (HRM), sequencing and restriction fragment length polymorphism (RFLP). Results: Probands were screened for the promoter and all coding regions, including intron/exon boundaries, of LDLR and PCSK9 and part of exon 26 of APOB including p.(R3527Q). Two families were identified with previously unreported LDLR mutations (c.1019_1020delinsTG, p.(C340L) and c.1634G>A, p.(G545E)). Both probands had tendon xanthomas or xanthelasma and/or a history of cardiovascular disease. Co-segregation with hypercholesterolemia was demonstrated in both families. In silico studies predicted these variations to be damaging. In two families, novel PCSK9 variations were identified (exon2; c.314G>A, p.(R105Q) and exon3; c.464C>T, p.(P155L)). In silico studies suggested both were likely to be damaging, and family members carrying the p.(105Q) allele had lower total cholesterol levels, suggesting this is a loss-of-function mutation. For c.464C>T p.(P155L) the small number of relatives available precluded any strong inference. Conclusion: This report brings to seven the number of different LDLR mutations reported in FH patients from Pakistan and, as expected in this heterogeneous population, no common LDLR mutation has been identified. [Copyright &y& Elsevier]

Published

2013

3. Mutation detection in Croatian patients with Familial Hypercholesterolemia.

Author

Pećin, Ivan, Whittall, Ros, Futema, Marta, Sertić, Jadranka, Reiner, Željko, Leigh, Sarah E. A., and Humphries, Steve E.

Subjects

*HYPERCHOLESTEREMIA, *LOW density lipoprotein receptors, *GENETIC mutation, *PREVENTION of heart diseases, *BIOLOGICAL variation, *POLYMERASE chain reaction, *GENETICS

Abstract

Familial hypercholesterolemia (FH) is caused by mutations in the genes for LDLR, APOB or PCSK9, and identification of the causative mutation provides definitive diagnosis so that the patient can be treated, their relatives tested and, therefore, premature heart disease prevented. DNA of eight unrelated individuals with clinically diagnosed FH were analyzed using a High-Resolution Melting method (HRM) for the LDLR gene (coding region, promoter and intron/exon boundaries), the APOB gene (part exon 26) and the PCSK9 gene (exon7). Variations found were sequenced and the effect on function of confirmed variants examined using predictive algorithms. Gross deletions and insertions were analysed using MLPA. Three novel LDLR variants were found, p.(S470C), p.(C698R) and c.2312-2A>C. All were predicted to be pathogenic using predictive algorithms. Three previously reported disease-causing mutations were identified (p.(G20R), p.(N272T) and p.(S286R); the latter was also carried by a hypercholesterolaemic relative. One patient carried the pathogenic APOB variant p.(R3527Q). No large LDLR deletions nor insertions were found, neither were any PCSK9 variants identified. HRM is a sensitive method for screening for mutations. While the causative mutation has been identified in 88% of these clinically defined FH patients, there appears to be a high degree of allelic heterogeneity in Croatian patients. [ABSTRACT FROM AUTHOR]

Published

2013

4. Use of targeted exome sequencing as a diagnostic tool for Familial Hypercholesterolaemia.

Author

Futema, Marta, Plagnol, Vincent, Whittall, Ros A., Neil, H. Andrew W., and Humphries, Steve Eric

Subjects

HYPERCHOLESTEREMIA, GENETIC mutation, FAMILIAL diseases, NUCLEOTIDE sequence, MEDICAL genetics, DISEASE risk factors, GENETICS

Abstract

Background Familial Hypercholesterolaemia (FH) is an autosomal dominant disease, caused by mutations in LDLR, APOB or PCSK9, which results in high levels of LDL-cholesterol (LDL-C) leading to early coronary heart disease. An autosomal recessive form of FH is also known, due to homozygous mutations in LDLRAP1. This study assessed the utility of an exome capture method and deep sequencing in FH diagnosis. Methods Exomes of 48 definite FH patients, with no mutation detected by current methods, were captured by Agilent Human All Exon 50Mb assay and sequenced on the Illumina HiSeq 2000 platform. Variants were called by GATK and SAMtools. Results The mean coverage of FH genes varied considerably (PCSK9=23x, LDLRAP1=36x, LDLR=56x and APOB=93x). Exome sequencing detected 17 LDLR mutations, including three copy number variants, two APOB mutations, missed by the standard techniques, two LDLR novel variants likely to be FH-causing, and five APOB variants of uncertain effect. Two variants called in PCSK9 were not confirmed by Sanger sequencing. One heterozygous mutation was found in LDLRAP1. Conclusions High-throughput DNA sequencing demonstrated its efficiency in well-covered DNA regions, in particular LDLR. This highly automated technology is proving to be effective for heterogeneous diseases and may soon replace laborious conventional methods. However, the poor coverage of gene promoters and repetitive, or GC-rich sequences, remains problematic, and validation of all identified variants is currently required. [ABSTRACT FROM AUTHOR]

Published

2012

5. Low-Density Lipoprotein Receptor Gene Familial Hypercholesterolemia Variant Database: Update and Pathological Assessment.

Author

Usifo, Ebele, Leigh, Sarah E. A., Whittall, Ros A., Lench, Nicholas, Taylor, Alison, Yeats, Corin, Orengo, Christine A., Martin, Andrew C. R., Celli, Jacopo, and Humphries, Steve E.

Subjects

LOW density lipoproteins, HYPERCHOLESTEREMIA, DATABASES, PROMOTERS (Genetics), COMPUTER software, LOCUS (Genetics)

Abstract

Familial hypercholesterolemia (FH) is caused predominately by variants in the low-density lipoprotein receptor gene ( LDLR). We report here an update of the UCL LDLR variant database to include variants reported in the literature and in-house between 2008 and 2010, transfer of the database to LOVDv.2.0 platform (https://grenada.lumc.nl/LOVD2/UCL-Heart/home.php?select_db=LDLR) and pathogenicity analysis. The database now contains over 1288 different variants reported in FH patients: 55% exonic substitutions, 22% exonic small rearrangements (<100 bp), 11% large rearrangements (>100 bp), 2% promoter variants, 10% intronic variants and 1 variant in the 3' untranslated sequence. The distribution and type of newly reported variants closely matches that of the 2008 database, and we have used these variants ( n= 223) as a representative sample to assess the utility of standard open access software (PolyPhen, SIFT, refined SIFT, Neural Network Splice Site Prediction Tool, SplicePort and NetGene2) and additional analyses (Single Amino Acid Polymorphism database, analysis of conservation and structure and Mutation Taster) for pathogenicity prediction. In combination, these techniques have enabled us to assign with confidence pathogenic predictions to 8/8 in-frame small rearrangements and 8/9 missense substitutions with previously discordant results from PolyPhen and SIFT analysis. Overall, we conclude that 79% of the reported variants are likely to be disease causing. [ABSTRACT FROM AUTHOR]

Published

2012

6. A functional mutation in the LDLR promoter (−139C>G) in a patient with familial hypercholesterolemia.

Author

Smith, Andrew J. P., Ahmed, Fayha, Nair, Devi, Whittall, Ros, Wang, Darrell, Taylor, Alison, Norbury, Gail, and Humphries, Steve E.

Subjects

GENETIC mutation, LOW density lipoproteins, PROMOTERS (Genetics), HYPERCHOLESTEREMIA, GENETIC disorders, HUMAN genetics

Abstract

A novel sequence change in repeat 3 of the promoter of the low-density lipoprotein receptor (LDLR) gene, −139C>G, has been identified in a patient with familial hypercholesterolemia (FH). LDLR -139G has been passed to one offspring who also shows an FH phenotype. Transient transfection studies using luciferase gene reporter assays revealed a considerable reduction (74±1.4% SEM) in reporter gene expression from the −139G variant sequence compared to the wild-type sequence, strongly suggesting that this change is the basis for FH in these patients. Analysis using electrophoretic mobility shift assay demonstrated the loss of Sp1 binding to the variant sequence in vitro, explaining the reduction of transcription.European Journal of Human Genetics (2007) 15, 1186–1189; doi:10.1038/sj.ejhg.5201897; published online 11 July 2007 [ABSTRACT FROM AUTHOR]

Published

2007

7. The A370T Variant ( StuI Polymorphism) in the LDL Receptor Gene is not Associated with Plasma Lipid Levels or Cardiovascular Risk in UK Men.

Author

Vieira, José Ricardo S., Whittall, Ros A., Cooper, Jackie A., Miller, George J., and Humphries, Steve E.

Subjects

*LOW density lipoproteins, *HYPERCHOLESTEREMIA, *GENETIC polymorphisms, *ALANINE, *CORONARY disease, *MYOCARDIAL infarction, *APOLIPOPROTEINS

Abstract

Over 800 different missense mutations in the low density lipoprotein (LDL) receptor gene ( LDLR) have been identified in patients with familial hypercholesterolaemia (FH). Only two of them, including the Alanine to Threonine change at position 370 (A370T), have been discovered in FH patients but do not cause FH. The frequency of the 370T allele has been reported worldwide to be between 0.022 and 0.070, with no clear association with high cholesterol levels or risk for coronary heart disease (CHD) and stroke. To explore this relationship in more detail we have determined this genotype in 2,659 healthy middle-aged (50–61 years) men participating in the prospective Second Northwick Park Heart Study, with 236 CHD and 67 stroke incident events. The genotype distribution was in Hardy-Weinberg equilibrium and in the no-event group the frequency of 370T was 0.046 (95% CI 0.040–0.052). Overall, there was no significant association of the 370T allele with any measured plasma lipid trait, and there was no difference in genotype distribution or allele frequency between the no-event and CHD (0.059; 95% CI 0.040–0.085) or stroke (0.037; 95% CI 0.012–0.085) groups ( p= 0.18 and 0.65, respectively). There was evidence for significant interaction ( p= 0.006) between body mass index (BMI) and genotype on CHD risk, with 370A homozygotes showing the expected higher CHD risk for those with higher BMI, whilst risk for 370T allele carriers was highest in men in the lowest tertile of BMI. The explanation for this association is unclear, and may simply be chance. Thus, these data confirm the absence of a significant impact of the A370T polymorphism on LDL receptor function, at least as measured by the effect on plasma lipid levels and CHD risk. [ABSTRACT FROM AUTHOR]

Published

2006

8. The molecular basis of familial hypercholesterolaemia in Turkish patients

Author

Sözen, M. Mert, Whittall, Ros, Öner, Cihan, Tokatlı, Ayşegül, Kalkanoğlu, H. Serap, Dursun, Ali, Coşkun, Turgay, Öner, Reyhan, and Humphries, Steve E.

Subjects

*HYPERCHOLESTEREMIA, *JUVENILE diseases, *AMINO acids, *HYPERLIPIDEMIA

Abstract

Abstract: Familial hypercholesterolaemia (FH) is an autosomal dominant disorder of lipoprotein metabolism. In the majority of patients FH is caused by mutations in the gene for the low-density lipoprotein receptor (LDLR), and to date more than 700 mutations have been reported worldwide. In this study, 36 paediatric patients with a clinical diagnosis of FH (20 homozygous and 16 heterozygotes) were screened for mutations in the LDLR gene. Each exon, with intron–exon junctions, was screened by capillary fluorescent SSCP (F-SSCP) and heteroduplex analysis. Samples showing different band patterns were sequenced. Ten novel (including three frame shift small deletions or insertions) and seven known mutations were detected. A total of 37 out of the predicted 56 FH-causing alleles were identified (66.1%). No patients with the R3500Q mutation in the APOB gene were found. W556R was the most common mutation, explaining 21.4% of the predicted defective LDLR alleles. The novel sequence changes were deemed to be pathogenic if they altered a conserved amino acid (L143P, D147E, Q233H-C234G, C347G) or occurred in or close to a splice site (IVS 16+5) and were absent in DNA from 50 healthy Turkish subjects. These data confirm the genetic heterogeneity of FH in Turkey, and demonstrate the usefulness of F-SSCP for mutation detection. [Copyright &y& Elsevier]

Published

2005

9. Molecular genetics of familial hypercholesterolemia in Israel–revisited.

Author

Durst, Ronen, Ibe, Uche Ken, Shpitzen, Shoshi, Schurr, Daniel, Eliav, Osnat, Futema, Marta, Whittall, Ros, Szalat, Auryan, Meiner, Vardiella, Knobler, Hilla, Gavish, Dov, Henkin, Yaakov, Ellis, Avishay, Rubinstein, Ardon, Harats, Dror, Bitzur, Rafael, Hershkovitz, Bruno, Humphries, Steve E., and Leitersdorf, Eran

Subjects

*MOLECULAR genetics, *HYPERCHOLESTEREMIA, *LOW density lipoprotein receptors, *APOLIPOPROTEIN B, *PROPROTEIN convertases, *POPULATION

Abstract

Background and aims Familial hypercholesterolemia (FH) is an autosomal dominant disease caused by mutations in the genes for LDL receptor ( LDLR ), apolipoprotein B ( APOB ) and proprotein convertase subtilisin/kexin type9 ( PCSK9). The purpose of the current investigation was to define the current spectrum of mutations causing FH in Israel. Methods New families were collected through the MEDPED (Make Early Diagnosis Prevent Early Death) FH program. Molecular analysis of the LDLR , PCSK9 and APOB genes was done using High Resolution Melt and direct sequencing in 67 index cases. A 6-SNP LDL-C gene score calculation for polygenic hypercholesterolaemia was done using TaqMan genotyping. Results Mean serum cholesterol was 7.48 ± 1.89 mmol/L and the mean serum LDL-C was 5.99 ± 1.89 mmol/L. Mutations in the LDLR and APOB gene were found in 24 cases (35.8%), with 16 in LDLR, none in PCSK9 and one, p.(R3527Q), in the APOB gene, which is the first APOB mutation carrier identified in the Israeli population. Of the LDLR mutations, two were novel; p.(E140A) and a promoter variant, c.-191C > A. The c.2479G > A p.(V827I) in exon 17 of the LDLR gene was found in 8 patients (33.3% of the mutations) with modestly elevated LDL-C, but also in a compound heterozygous patient with a clinical homozygous FH phenotype, consistent with this being a “mild” FH-causing variant. A significantly higher 6-SNP LDL-C score was found in mutation-negative cases compared with a normal Caucasian cohort ( p = 0.03), confirming that polygenic inheritance of common LDL-C raising SNPs can produce an FH phenocopy. Conclusions The results indicate a different spectrum of genetic causes of FH from that found previously, in concordance with the heterogeneous and changing origins of the Israeli population, and confirm that a polygenic cause is also contributing to the FH phenotype in Israel. [ABSTRACT FROM AUTHOR]

Published

2017

10. A World Wide Web site for low-density lipoprotein receptor gene mutations in familial hypercholesterolemia: sequence-based, tabular, and direct submission data handling.

Author

Wilson, Darren J., Gahan, Mike, Haddad, Lema, Heath, Karen, Whittall, Ros A., Williams, Roger R., Humphries, Steve E., Day, Ian N.M., Wilson, D J, Gahan, M, Haddad, L, Heath, K, Whittall, R A, Williams, R R, Humphries, S E, and Day, I N

Subjects

*LOW density lipoproteins, *HYPERCHOLESTEREMIA

Abstract

Familial hypercholesterolemia is an autosomal dominant inherited condition characterized by a mutation in the low-density lipoprotein receptor (LDLR) gene. A database has been set up on the World Wide Web for mutations in the LDLR gene. [ABSTRACT FROM AUTHOR]

Published

1998