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3. Spectrum and origin of mutations in sporadic cases of haemophilia A in China

Author

Xianjin Wang, Jifeng Dai, Qiulan Ding, Wenman Wu, Guoling You, Xi Wu, Yeling Lu, and Y. Xin

Subjects
Male, 0301 basic medicine, China, Genetic counseling, Haemophilia A, 030204 cardiovascular system & hematology, Hemophilia A, medicine.disease_cause, 03 medical and health sciences, 0302 clinical medicine, Genetic linkage, medicine, Humans, Copy-number variation, Genotyping, Genetics (clinical), Genetics, Mutation, business.industry, Point mutation, Hematology, General Medicine, medicine.disease, 030104 developmental biology, Microsatellite, Female, business
Abstract

Introduction About 30% of haemophilia A (HA) patients are sporadic cases. It is important to confirm the mutation origin and carrier status in these families. Aim To describe the spectrum and origin of the mutations in 393 Chinese sporadic HA families and identify potential mosaics among non-carrier mothers. Methods AccuCopy quantification combined with long-distance PCR was used for genotyping intron 22/1 inversion (Inv22/Inv1) and Inv22 mosaicism. F8 gene sequences were analysed by direct sequencing. Copy number variations of F8 gene were detected by AccuCopy method. Six short tandem repeats related to F8 gene were applied for linkage analysis. Mosaicism of point mutations/small deletions/insertions was determined by ddNTP primer extension method. Results Most of sporadic patients' mothers are carriers, in 257 cases with integral family members, 60% have the mutations tracing back to their fathers, 12% to their mothers. 28% had de novo mutations with non-carrier mothers as revealed by routine genetic studies. Mutation spectrum of sporadic families was different in groups with different origins of mutations. Point mutation (51%) was the predominant mutation type in pedigrees with de novo mutations. While, in families with mutations inherited from maternal grandfathers, Inv22 was the main type (51%). We found somatic mosaic in mothers of 30% (3/10) pedigrees with de novo Inv22 and 11.5% (3/26) pedigrees with point mutations. Conclusion The spectrum of F8 genetic variants identified in sporadic families was fairly diverse. The high prevalence of chimaeras in carriers suggests that more cautions should be taken in genetic counselling of sporadic haemophilia families.

Published
2018
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4. An exonic missense mutation c.28G>A is associated with weak B blood group by affecting RNA splicing of theABOgene

Author

Chengrui Qian, Qiulan Ding, Wenman Wu, Hang Lei, Wei Zou, Xiaohong Cai, Xuefeng Wang, and Dong Xiang

Subjects
0301 basic medicine, Messenger RNA, Immunology, Hematology, Transfection, 030204 cardiovascular system & hematology, Biology, Molecular biology, 03 medical and health sciences, Exon, 030104 developmental biology, 0302 clinical medicine, ABO blood group system, Complementary DNA, RNA splicing, Immunology and Allergy, Missense mutation, Minigene
Abstract

BACKGROUND The amino acid substitutions caused by ABO gene mutations are usually predicted to impact glycosyltransferase's function or its biosynthesis. Here we report an ABO exonic missense mutation that affects B-antigen expression by decreasing the mRNA level of the ABO gene rather than the amino acid change. STUDY DESIGN AND METHODS Serologic studies including plasma total GTB transfer capacity were performed. The exon sequences of the ABO gene were analyzed by Sanger sequencing. B310 cDNA with c.28G>A (p.G10R) mutation was expressed in HeLa cells and total GTB transfer capacity in cell supernatant was measured. Flow cytometry was performed on these HeLa cells after transfection, and agglutination of Hela-Bweak cells was also examined. The mRNA of the ABO gene was analyzed by direct sequencing and real-time reverse transcriptase–polymerase chain reaction. A minigene construct was prepared to evaluate the potential of splicing. RESULTS While plasma total GTB transfer capacity was undetectable in this B3-like individual, the relative percentage of antigen-expressing cells and mean fluorescence index of the Bweak red blood cells (RBCs) were 19 and 14% of normal B RBCs, respectively. There was no significant difference of total GTB transfer capacity in cell supernatant and B-antigen expression on cell surfaces between HeLa cells transfected with B310 cDNA and B cDNA. The mRNA expression level of B310 in peripheral whole blood was significantly reduced. The amount of splicing is significantly lower in c.28G>A construct compared to that in wild-type construct after transfection in K562 cells. CONCLUSION ABO c.28G>A mutation may cause B3-like subgroup by affecting RNA splicing of the ABO gene.

Published
2017
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5. Thromboelastography predicts risks of obstetric complication occurrence in (hypo)dysfibrinogenemia patients under non-pregnant state

Author

Lin-lin Jiang, Qian Liang, Qiulan Ding, Xi Wu, Yu Xin, Yaopeng Chen, Jingyi Zhou, Hongli Wang, Jing Dai, Xuefeng Wang, and Yeling Lu

Subjects
Adult, Risk, medicine.medical_specialty, Physiology, 030204 cardiovascular system & hematology, Fibrinogen, Asymptomatic, 03 medical and health sciences, 0302 clinical medicine, Pregnancy, Physiology (medical), medicine, Humans, Dysfibrinogenemia, Kaolin, Pharmacology, Receiver operating characteristic, medicine.diagnostic_test, Obstetrics, business.industry, Odds ratio, Afibrinogenemia, medicine.disease, Confidence interval, Thromboelastography, Thrombelastography, Pregnancy Complications, 030220 oncology & carcinogenesis, Female, medicine.symptom, business, medicine.drug
Abstract

Congenital (hypo)dysfibrinogenemia patients may have obstetric complications during their pregnancies. This study aimed to evaluate thromboelastography (TEG) as a potential tool for assessing the tendency for obstetric complications in those patients in a non-pregnant state. A total of 22 female subjects with congenital (hypo)dysfibrinogenemia were recruited. Nine subjects had histories of obstetric complications and the other 13 subjects had at least one uneventful pregnancy without obstetric complications as yet. Detailed clinical investigation and phenotype/genotype detection were carried out, and both kaolin-activated TEG and functional fibrinogen TEG (FF-TEG) were applied in all subjects. Significant differences were identified in all TEG parameters except for R and angle between these two groups (P < 0.05) by covariance analysis. Receiver operating characteristic (ROC) analysis of discrimination between these two groups of patients was performed for TEG parameters. Significantly high odds ratio (OR) of obstetric complications occurrence were demonstrated in K ≥ 3.8 min, maximum amplitude (MA) ≤ 54.2 mm, comprehensive index (CI) ≤ -3 (11.67, 95% CI 1.527-89.121, P < 0.05 in all), and MA-CFF ≤ 12.1 mm (20.00, 95% confidence interval (95% CI) 1.967-203.322, P = 0.002). Moreover, MA-CFF had better prognostic performance, with a corresponding area under the receiver operating curve of 0.923 (range 0.815-1.031, P = 0.001). This study suggests that (hypo)dysfibrinogenemia patients with values outside of the cut-off values of TEG assays under non-pregnant state may have a higher risk of obstetric complications occurring when they are pregnant. No parameters under non-pregnant state in clinical laboratory have ever been reported to be risk factors for obstetric complication occurrence in (hypo)dysfibrinogenemia patients. This study explored such parameters in TEG assays and found that parameters of TEG assays under non-pregnant status might predict the occurrence of obstetric complications, which could provide physicians with important information about whether fibrinogen replacement therapy is required, so as to prevent the occurrence of obstetric complications, especially for patients who are asymptomatic in daily life.

Published
2016
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6. Characterisation and validation of a novel panel of the six short tandem repeats for genetic counselling in Chinese haemophilia A pedigrees

Author

Qiulan Ding, Yeling Lu, Jifeng Dai, X. F. Wang, Xiaodong Xi, and Hongsheng Wang

Subjects
Genetics, Genetic counseling, Haemophilia A, Haplotype, Pedigree chart, Hematology, General Medicine, Biology, Gene mutation, medicine.disease, Genetic linkage, Genotype, medicine, Microsatellite, Genetics (clinical)
Abstract

Summary. Haemophilia A (HA) is the most common hereditary bleeding disorder caused by F8 gene mutation. Linkage analysis is an auxiliary strategy to direct mutation analysis for genetic counselling of HA. Here we characterize and validate a novel panel of six short tandem repeat (STR) loci for genetic counselling in Chinese HA pedigrees. The panel was analysed in 116 unrelated healthy female patients and 108 male patients, and verified in 169 unrelated pedigrees with HA. The six STR loci in the panel spanned a distance of 0.3 Mb from each side of the F8 gene. Three of them, F8Up226, F8Up146 and F8Down48, were first described here. Markers F8Up226, F8Up146, F8Int13, F8Int25, F8Down48 and DXS1073 exhibited the number of alleles 16, 9, 8, 6, 9 and 10, and heterozygosity rates of 74.8%, 44.8%, 60.9%, 42.6%, 61.7% and 62.0% respectively. Haplotype frequencies analysis suggested that the genotypes of haplotype provided a highly informative content (56.5%). The panel was informative in 167 of 169 unrelated haemophilic pedigrees with the combined diagnostic rate of 98.8%. In eight pedigrees could not be diagnosed by mutation detection linkage studies using the panel were informative in all the pedigrees and a reliable diagnosis was made in seven pedigrees. The novel panel of the six STR loci represents a high degree of informativeness and a low fraction of recombination. Linkage analysis using this panel provides an alternative strategy when direct mutation detection is not feasible for genetic counselling in Chinese HA families.

Published
2012
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7. The status of carrier and prenatal diagnosis of haemophilia in China

Author

Xianjin Wang, Yeling Lu, Xiaodong Xi, Jifeng Dai, Qiulan Ding, and Hui Wang

Subjects
Genetics, business.industry, Haemophilia A, Genetic Carrier Screening, Prenatal diagnosis, Hematology, General Medicine, Haemophilia, medicine.disease, DNA sequencing, Genetic linkage, medicine, SNP, Haemophilia B, business, Genetics (clinical)
Abstract

Haemophilia A (HA) and haemophilia B (HB) are the most common X-linked inherited bleeding disorders. It is important to detect the carrier women in families with HA/HB and subsequent antenatal diagnosis of confirmed carriers. This study consists of 102 HA families which include 68 mothers for prenatal diagnosis and 107 female relatives for carrier diagnosis, and 29 HB families which include 16 mothers and 31 female relatives respectively. The rapid fluorescent PCR with two groups of different combined polymorphism markers was applied for linkage analysis in HA and HB families respectively. The Amelogenin gene was added to help the detection of gender diagnosis. Gene sequencing was also used to detect the mutations directly. There were 37 causative F8C mutations (23 novel) and 24 causative F9C mutations (eight novel) found in this cohort of patients. Few of the women could not be diagnosed due to homologous recombination and/or inability to locate the mutation. Complicated cases have been found in some families. With regard to carrier and prenatal diagnosis, it was considered that genetic diagnosis by linkage analysis and direct sequencing was successful. Some special families might require combination of the linkage analysis and gene sequence for a successful diagnosis. New intragenic SNP and STR sites special to Chinese population need to be discovered.

Published
2011
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8. A case of factor XI deficiency caused by compound heterozygous F11 gene mutation

Author

Dao Li, Qiulan Ding, Hong-li Wang, Qihua Fu, Jing Wang, Xuefeng Wang, Jing Dai, and Lisong Shen

Subjects
Genetics, Nonsense mutation, Hematology, General Medicine, Biology, Gene mutation, Compound heterozygosity, Molecular biology, Ashkenazi jews, Mutation (genetic algorithm), Missense mutation, Liver function, Factor XI, Genetics (clinical)
Abstract

Summary. Inherited factor XI (FXI) deficiency is a rare autosomal recessive bleeding disorder in most populations except for Ashkenazi Jews. In this report, a 25-year-old Chinese female FXI deficiency case has been studied. Routine clotting tests showed significantly prolonged activated partial thromboplastin time (69.5 s, control 35 ± 10 s) while prothrombin time (12.3 s, control 13 ± 3 s) was normal. FXI:C and FXI:Ag were 2.6% and 2.5%, respectively, indicating that this case was cross-reacting material negative. The activities of other coagulation factors and liver function were in normal range. The DNA sequence results of the 15 exons and their boundaries of F11 gene revealed a novel G3733C missense mutation in exon 2, and a recurrent C16642T nonsense mutation in exon 8. The G3733C mutation caused G-1R substitution in FXI signal peptide, which might impair the protein’s secretion and introduced a new BssSI enzyme digestion site. The C16642T mutation led a premature stop codon at amino acid position 263(Q263Term). G-1R and Q263Term compound heterozygous mutations in F11 gene were the cause of FXI deficiency for this proband. G-1R mutation was a novel F11 gene mutation causing inherited FXI deficiency.

Published
2009
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9. Identification of a novel splicing mutation in the fibrinogen Aα chain gene leading to hypofibrinogenaemia in a Chinese pedigree

Author

Hua-Yun Chen, Qiulan Ding, Xiaodong Xi, Guan-qun Xu, X. F. Wang, Yeling Lu, F Yang, X Su, Hui Wang, and Jing Dai

Subjects
Genetics, business.industry, Fibrinogen Aalpha, Hematology, General Medicine, Fibrinogen, RNA splicing, Mutation (genetic algorithm), medicine, Chain gene, Base sequence, Identification (biology), business, Genetics (clinical), medicine.drug
Published
2009
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10. Molecular characterization of two novel mutations causing factor X deficiency in a Chinese pedigree

Author

Zhen-yi Wang, Hongli Wang, Qiulan Ding, Y.-Q. Hu, Rong-fu Zhou, Qi-hua Fu, X. Wang, Wen-bin Wang, and Wen-man Wu

Subjects
China, Heterozygote, Adolescent, Mutant, Mutagenesis (molecular biology technique), Genes, Recessive, Biology, Transfection, Compound heterozygosity, medicine.disease_cause, Autoantigens, Cell Line, chemistry.chemical_compound, Autosomal recessive trait, Cricetinae, medicine, Animals, Humans, Factor X Deficiency, Genetics (clinical), Mutation, Reverse Transcriptase Polymerase Chain Reaction, Factor X, HEK 293 cells, Hematology, General Medicine, Molecular biology, Reverse transcriptase, Alternative Splicing, chemistry, Mutagenesis, Site-Directed, Female, Partial Thromboplastin Time
Abstract

Summary. Factor X (FX) deficiency is a rare bleeding disorder inherited as an autosomal recessive trait. In this study, we investigated the molecular basis of FX deficiency in a Chinese pedigree. The proposita showed a markedly prolonged activated partial thromboplastin time and a mild prolongation of prothrombin time. The levels of FX antigen and FX activity were 58.6% and 2.5%, respectively. Molecular analysis revealed that the proposita was compound heterozygous for two novel mutations: IVS1 + 1G > A and G1185A (Arg347His). The aberrant transcripts from the IVS1 + 1G > A mutant allele were not detected by analyzing the splicing pattern of ectopic transcripts in leukocytes of the patient with nested polymerase chain reaction after reverse transcription. We thus hypothesize that the mRNA molecules originating from the IVS1 + 1G > A mutation were rapidly destroyed in vivo. Site-directed mutagenesis of FX cDNA was used to introduce FXG1185A mutation, and wild-type as well as mutant FX proteins were expressed by transient transfection in HEK 293 cells. Normal FX antigen levels both in the conditioned media of cells expressing the mutant and in cell lysates were detected by an enzyme-linked immunoadsorbent assay. Evaluation of wild-type and mutant coagulant activity demonstrated that the FX molecules carrying the Arg347His mutation have dramatically decreased activity.

Published
2005
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11. Identification of three F5 gene mutations associated with inherited coagulation factor V deficiency in two Chinese pedigrees

Author

Y.-Q. Hu, Rong-fu Zhou, Wen-bin Wang, Hongli Wang, Wen-man Wu, Qi-hua Fu, X. Wang, Lu Liu, Qiulan Ding, and Zhen-yi Wang

Subjects
Adult, Male, Proband, Gene mutation, medicine.disease_cause, Exon, Complementary DNA, medicine, Humans, Missense mutation, Gene, Genetics (clinical), Genetics, Mutation, Polymorphism, Genetic, biology, Factor V, DNA, Sequence Analysis, DNA, Hematology, General Medicine, Molecular biology, Pedigree, Phenotype, biology.protein, Female, Factor V Deficiency, Polymorphism, Restriction Fragment Length
Abstract

Summary. To investigate the molecular defects in two Chinese pedigrees with inherited factor V (FV) deficiency. A 37-year-old male (proband 1) and an 18-month-old boy (proband 2) were diagnosed as inherited coagulation FV deficiency by severely reduced plasma levels of FV activity and antigen. All 25 exons and their flanking sequence of F5 gene were amplified by polymerase chain reaction (PCR) for both probands and the PCR products were directly sequenced. Total RNA was extracted from the peripheral lymphocytes of proband 1 for detecting the changes at mRNA level. The homozygous deletion IVS8 −2A>G was identified in the F5 gene of proband 1 and complementary DNA (cDNA) analysis revealed the abolishment of the canonical splicing site by the mutation and the activation of the cryptic acceptor site 24 bp upstream instead. The insertion introduced eight additional amino acids (AA) into the FV protein. Two heterozygous mutations of F5 gene were discovered in proband 2. The 2238-9del AG in exon 13 introduced a premature termination code at 689 AA and the substitution of G6410 by T in exon 23 lead to the missense mutation Gly2079Val. Three F5 gene mutations, IVS8 −2A>G, 2238-9del AG and G6410T, have been identified in two Chinese pedigree with congenital FV deficiency, respectively.

Published
2004
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12. Prothrombin Shanghai: hypoprothrombinaemia caused by substitution of Gla29 by Gly

Author

Rong-fu Zhou, Hongli Wang, Qi-hua Fu, Y.-Q. Hu, Wen-bin Wang, Wen-man Wu, Qiulan Ding, Zhen-yi Wang, and X. Wang

Subjects
Prothrombin time, Gla domain, Mutation, medicine.diagnostic_test, Biological activity, Hematology, General Medicine, Biology, Gene mutation, medicine.disease_cause, Molecular biology, Autosomal recessive trait, Coagulation, hemic and lymphatic diseases, medicine, Genetics (clinical), circulatory and respiratory physiology, Partial thromboplastin time
Abstract

Summary. Prothrombin deficiency is a rare bleeding disorder inherited as an autosomal recessive trait. In this study, we reported a Chinese family with hereditary prothrombin deficiency. The proposita had a prolonged activated partial thromboplastin time (APTT, 71.6 s) and prothrombin time (PT, 28.0 s). The coagulation factors activities were normal except that prothrombin coagulation activity was markedly reduced, and the prothrombin antigen level was moderately decreased. Nucleotide sequencing of amplified DNA revealed a novel mutation, Glu (GAG) to Gly (GGG) at residue 29, which normally undergoes γ-carboxylation within the Gla domain of prothrombin. The proposita was identified as homozygous, while her father, mother and maternal grandmother were heterozygous for the mutation. Gla29 has been demonstrated as one of the key residue for Ca2+-binding, membrane interaction and biological activity of prothrombin.

Published
2004
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13. Type I coagulation factor V deficiency caused by compound heterozygous mutation of F5 gene

Author

Y.-Q. Hu, Hongli Wang, Qiulan Ding, Qi-hua Fu, Wen-man Wu, X. Wang, and Zhen-yi Wang

Subjects
Silent mutation, Prothrombin time, Mutation, biology, medicine.diagnostic_test, Factor V, Hematology, General Medicine, Gene mutation, medicine.disease_cause, Compound heterozygosity, Molecular biology, biology.protein, medicine, Missense mutation, Genetics (clinical), Partial thromboplastin time
Abstract

A 16-year-old Chinese female with prolonged bleeding after surgery has been studied. Routine clotting tests revealed a prolonged activated partial thromboplastin time (APTT; 126.6 s) and prothrombin time (PT; 42.8 s). The coagulation factors activities were normal except for factor V, which was only 0.3% of normal. DNA analysis of the FV gene revealed five nucleotide substitutions in exons, including two silent mutations (G327A and A5112G), one polymorphism (G1628A), a G1348T missense mutation and 4887 approximately 8delG. These abnormalities were associated with her FV deficiency, perhaps by causing a Gly392Cys substitution in FV amino acid sequence or by introducing a premature stop codon at amino acid position 1390. This is the third case in which FV deficiency is caused by compound heterozygous mutation of F5 gene, and is the first report from a Chinese family.

Published
2003
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14. The prevalence of factor VIII inhibitors and genetic aspects of inhibitor development in Chinese patients with haemophilia A

Author

Qiulan Ding, Xinbing Wang, Heng Ge, Hongsheng Wang, Yiqiang Q. Zhao, Xueqin Zhang, Renchi Yang, Junde Wu, and Jing Sun

Subjects
China, Genotype, DNA Mutational Analysis, Haemophilia A, Nonsense mutation, Hemophilia A, Haemophilia, medicine.disease_cause, Asian People, Prevalence, medicine, Humans, Missense mutation, Genotyping, Genetics (clinical), Mutation, Factor VIII, Blood Coagulation Factor Inhibitors, business.industry, Hematology, General Medicine, medicine.disease, Virology, Cryoprecipitate, business
Abstract

The prevalence of inhibitors in Chinese haemophiliacs has not yet been reported. The aim of this study was to identify the prevalence of factor VIII (FVIII) inhibitors among haemophiliacs who are treated only with plasma-derived FVIII (pdFVIII), cryoprecipitate or fresh frozen plasma (FFP), and tried to explore the relationship between the generation of inhibitors and particular FVIII deficiency genotypes. Clinical information and blood samples of 1435 patients with haemophilia A (HA) were collected by six haemophilia centres in China. The Nijmegen modification of the Bethesda assay was used to detect inhibitors. Multiplex PCR, long-range PCR and direct sequencing were performed for genotyping. The overall prevalence of inhibitors in Chinese HA patients was 3.9% and the prevalence of severe haemophiliacs was 4.3%; 18 of the 56 patients with inhibitors had high titres. A total of 38 different mutations were identified in the 55 patients with inhibitors, including 15 intron 22 and 3 intron 1 inversions, seven large deletions, 14 small deletion/insertions, seven nonsense mutations, one splice site mutations and eight missense mutations. Of 38 mutations, 28 were novel. Patients with large deletions and nonsense mutations were prone to have high titre inhibitors, with incidence rates of 57.1% (4/7) and 42.9% (3/7), respectively. In conclusion, the prevalence of inhibitors in Chinese HA patients is much lower than that reported for other ethnic groups and the large deletion and nonsense mutations are high risk factors for high titre inhibitor development.

Published
2010
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15. Prevalence of the factor 8 gene intron 1 inversion in Chinese haemophiliacs and its application to carrier detection and prenatal diagnosis in haemophilia A families

Author

Yeling Lu, X. D. Xi, Hongsheng Wang, Qiulan Ding, Jifeng Dai, and X. Wang

Subjects
Genetics, Pediatrics, medicine.medical_specialty, business.industry, Haemophilia A, Intron, Prenatal diagnosis, Hematology, General Medicine, medicine.disease, Medicine, business, Gene, Genetics (clinical), Chromosomal inversion
Published
2010
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