Your search keyword '"Rh-Hr Blood-Group System immunology"' showing total 13 results

1. A novel RHD allele caused by c.739 G> C mutation was identified in a Chinese individual.

Author

Lyu H, Jiao S, Ma W, and Hu B

Subjects

Alleles, China ethnology, Exons genetics, Female, Humans, Mutation genetics, Phenotype, Polymerase Chain Reaction methods, Rh-Hr Blood-Group System immunology, Asian People genetics, Pregnancy blood, Rh-Hr Blood-Group System genetics

Abstract

The blood sample of a pregnant Chinese woman of the north Han population was confirmed as D variation by serologic method, and subsequent detection of RHD Exons 1 through 10 by the polymerase chain reaction-sequence-specific primer test showed that all exons were present. To further clarify the molecular mechanism of this sample, we sequenced the RHD Exons 1 through 10 and found that it was a novel allele caused by c.739 G> C in Exon 5., (© 2020 AABB.)

Published

2021

2. Safety issues related to the electronic cross-matching of blood in mainland China: A prospective cohort study involving cross-matching of 40,228 blood samples.

Author

Wang YJ, Liu JR, and Liu Y

Subjects

ABO Blood-Group System immunology, Blood Donors, Blood Grouping and Crossmatching methods, China epidemiology, Female, Humans, Prospective Studies, Rh-Hr Blood-Group System immunology, Blood Group Incompatibility epidemiology, Blood Grouping and Crossmatching adverse effects, Isoantibodies analysis

Abstract

Although the electronic cross-matching of blood has been widely applied in some developed countries and regions, concern over the risk of undetected red blood cell (RBC) antibodies has limited its application in mainland China.This study was performed to explore the missed detection rate of RBC antibodies in a Chinese population from 2011 to 2016. If the results of 2 consecutive tests of ABO/RhD blood group identification were consistent and antibody screening results were negative, electronic cross-matching of the blood was performed. In addition, traditional serological cross-matching of blood (polybrene method) and a parallel experiment for electronic cross-matching of blood were performed to analyze the missed detection of unexpected RBC antibodies in blood donors and recipients.Using the polybrene method, 40,228 blood samples were tested by parallel traditional serological cross-matching of blood; among these samples, blood compatibility was found in 40,222 cases, primary incompatibility (incompatibility of the donor's erythrocytes with the recipient's serum) was found in 6 cases, and no secondary incompatibility was found. Identification of antibody specificity was performed using panel cells, and all unexpected RBC antibodies were confirmed as anti-Mur alloantibodies in the MNS system.Further improvements in the erythrocyte antigenic spectrum, especially the Mur antigen in Asian populations, are expected to ensure the safety of implementing electronic cross-matching in China.

Published

2019

3. Effects of RHD gene polymorphisms on distinguishing weak D or DEL from RhD- in blood donation in a Chinese population.

Author

Shi J and Luo Y

Subjects

Adult, Blood Coagulation Tests, Blood Donors classification, China, Female, Humans, Male, Phenotype, Rh-Hr Blood-Group System immunology, Polymorphism, Single Nucleotide, Rh-Hr Blood-Group System genetics

Abstract

Background: Weak D or DEL red blood cell units may be mistyped as RhD- by current serology assays, which can lead to incompatible transfusion to RhD- recipients and further cause anti-D immunization. Molecular RHD blood group typing is a very effective method for overcoming current technical limits. The purpose of this study was to identify RHD single-nucleotide polymorphisms (SNPs) and compare the genotype prevalence among confirmed RhD- individuals in a Chinese population as well as explore effective biomarkers for current weak D or DEL detection before blood transfusion., Methods: In the present study, 125 weak D (1, 2, 3, and 4.1) or DEL and 185 RhD- blood samples from donors detected by current standard serology were collected. Genotyping system was used to analyze the SNPs of RHD in each sample., Results: Seven SNPs (rs592372, rs11485789, rs6669352, rs3118454, rs1053359, rs590787, and rs3927482) were detected in the RHD region. Rs3118454, rs1053359, rs590787, and rs3927482 showed significant differences between the weak D (1, 2, 3 and 4.1) or DEL and RhD- groups. Further combined analysis of the allelic distribution of these four SNPs revealed their higher frequencies in the RhD- group., Conclusion: The SNPs rs3118454, rs1053359, rs590787, and rs3927482 in RHD showed a significantly higher frequency among an RhD- Chinese population and are potential biomarkers., (© 2019 The Authors. Molecular Genetics & Genomic Medicine published by Wiley Periodicals, Inc.)

Published

2019

4. Molecular basis and zygosity determination of D variants including identification of four novel alleles in Chinese individuals.

Author

He J, Ying Y, Hong X, Xu X, Zhu F, and Lv H

Subjects

Blood Grouping and Crossmatching, China, Ethnicity genetics, Gene Dosage, Genetic Variation, Genotype, Humans, Multiplex Polymerase Chain Reaction, Mutation, Polymerase Chain Reaction, Rh-Hr Blood-Group System immunology, Sequence Analysis, DNA, Alleles, Asian People genetics, Rh-Hr Blood-Group System genetics

Abstract

Background: The frequency and molecular basis of the D variants have been reported in the Caucasian and African populations, but relatively little information was known in the Chinese population. Here, a study was investigated in Chinese persons with weak or discrepant D serologic typing., Study Design and Methods: D variant was typed with a serologic method. The full coding regions of RHD of these variants were amplified with polymerase chain reaction and then directly sequenced. RHD zygosity test was performed using the hybrid Rhesus box technique and a multiplex ligation-dependent probe amplification (MLPA) assay was also used to analyze the variant alleles and RHD gene copy number., Results: Twelve distinct RHD mutation alleles were found in 32 D variant individuals, with eight weak D and four partial D alleles. Weak D Type 15 and DVI Type 3 were the major weak D and partial D alleles in Zhejiang Han persons. Three novel weak D alleles (RHD weak D 95A, 779G, and 670G) and one new partial D allele (RHD130-132 del TCT) were identified. The results of RHD zygosity in three individuals disagreed between the RHD zygosity test and the MLPA assay. The most known variant alleles can be detected, but four novel alleles were missed using the RH-MLPA assay., Conclusion: The molecular basis and zygosity of D variants in Zhejiang Han persons were analyzed, and four novel RHD alleles were identified. These data extend the information of D variants and may help to improve the transfusion strategy of the D variants., (© 2014 AABB.)

Published

2015

5. [Molecular basis for real RhD negative and RhDel phenotypes in Yiwu population of Zhejiang Province in China].

Author

Jin XD, Fu GC, Xu XG, Zhu FM, and Yan LX

Subjects

Alleles, Asian People genetics, Base Sequence, China, Exons, Genotype, Humans, Molecular Sequence Data, Phenotype, Polymorphism, Genetic, Rh-Hr Blood-Group System immunology, Rh-Hr Blood-Group System genetics

Abstract

This study was purposed to investigate the molecular basis for RhD negative phenotype in Yiwu population in Zhejiang Province of China. The RhD negative samples were screened by saline agglutination test in blood donors. Some real RhD negative and RhDel phenotypes were identified using anti-human globulin test and absorbtion elution test. Ten exons of RHD gene in these samples were amplified by PCR-SSP, and positive exons were DNA sequenced. The results indicated that 30 real RhD negative and 8 RhDel phenotypes were identified in 38 initial RhD negative samples. Ten exons were complete negative in 28 real RhD negative samples and only exon 1, 2 and 10 were positive in 2 real RhD negative samples amplified by PCR. All 10 exons in 8 RbDel samples were positive and a DNA variant (1227G > A) was found in 8 RhDel samples. It is concluded that all exons are absence in most real RhD negative phenotypes, and the partial exons absence is also found in some real negative phenotypes among Yiwu population in Zhejiang province of China. The G to A mutation at position 1227 is found in all RhDel phenotypes.

Published

2010

6. Transfusion of RhD-positive blood in "Asia type" DEL recipients.

Author

Shao CP

Subjects

China, Epitopes, Female, Humans, Pregnancy, Retrospective Studies, Asian People, Blood Transfusion, Rh-Hr Blood-Group System immunology

Published

2010

7. [Detection and analysis of anti-Rh blood group antibodies].

Author

Wu YJ, Wu Y, Chen BC, and Liu Y

Subjects

Adolescent, Adult, Aged, Aged, 80 and over, Child, Child, Preschool, China, Female, Humans, Immunoglobulin G blood, Immunoglobulin G immunology, Immunoglobulin M blood, Immunoglobulin M immunology, Infant, Infant, Newborn, Isoantibodies immunology, Male, Middle Aged, Pregnancy, Young Adult, Isoantibodies blood, Rh-Hr Blood-Group System immunology

Abstract

Aim: To study the prevalence and distribution of anti-Rh blood group antibodies in Chinese population and its clinical significance., Methods: Irregular antibodies were screened and identified by Microcolum Gel Coomb's test. For those identified as positive anti-Rh samples, monoclonal antibodies (anti-D, -C, -c, -E and -e) were used to identify the specific antigen and confirm the accuracy of the irregular antibody tests. The titers, Ig-types and 37 Degrees Celsius-reactivity were tested to confirm its clinical significance. For evaluation of the origin of irregular antibodies, histories of pregnancy and transfusion were reviewed. For the newborns who had positive antibodies, their mothers were tested simultaneously to confirm the origin of the antibodies., Results: 47 out of 54 000 (0.087%) patients were identified as positive with Rh blood group antibodies.Of them, 27 cases had history of pregnancy, 13 had transfusion and 1 had the histories of both. 6 newborns had antibodies derived form their mothers. The specificity of the antibody was as follows: 29 with anti-E (61.70%), 8 with anti-D (17.02%), anti-cE 5(10.64%), 4 with anti-c (8.51%) and 1 with anti-C (2.13%). All the 47 Rh blood group antibodies were IgG or IgG+IgM, and were reactive to red blood cells with corresponding antigens at 37 Degrees Celsius, with a highest titer of 1:4 096., Conclusion: The prevalence of Rh antibodies is lower in Chinese population as compared with that in White population.Of all the antibodies, anti-E is most frequently identified and anti-D was declining. Alloimmunization by pregnancy and transfusion is the major cause of Rh antibody production. Rh blood group antibodies derived from mothers are the major cause of Non-ABO-HDN.

Published

2008

8. [Screening analysis of irregular antibodies from random donor population in Shaoguan area].

Author

Zhu JY, Lan JC, and Luo HQ

Subjects

Adolescent, Adult, China, Female, Humans, Male, Mass Screening, Middle Aged, Rh-Hr Blood-Group System blood, Rho(D) Immune Globulin, Blood Donors, Erythrocytes immunology, Isoantibodies blood, Rh-Hr Blood-Group System immunology

Abstract

The study was purposed to analyze the frequency and distribution of irregular antibodies in Shaoguan area. Screening 15 033 random donor antibodies in Shaoguan area by screening cells, polybrene and antiglobulin tests. The results indicated that the irregular antibodies were found in 42 samples. The frequency of irregular antibodies in female was higher than that in male (P < 0.001), and Rh blood group antibodies such as anti-D, anti-E, and anti-Ec C were common (47.6%). 2 samples of Le antibodies were failed to be found by polybrene test. 2 samples of irregular antibodies with titer 2 were undiscovered by screening test of 10 pooled samples. In conclusion, because of irregular antibodies resulting in hemolytic transfusion reaction, the investigation of frequency and distribution of irregular antibodies is very important for safe transfusion. Antibody screening must be done for female donors, and especially for massive plasma transfusion of patients with severe and dangerous illness and infants so as to ensure safety.

Published

2007

9. [RHD 1227A allele frequency among Rh negative population and random population].

Author

Wu JJ, Hong XZ, Xu XG, Ma KR, Zhu FM, and Yan LX

Subjects

Asian People genetics, Base Sequence, China, Cloning, Molecular, Gene Deletion, Humans, Molecular Sequence Data, Rh-Hr Blood-Group System immunology, Sequence Analysis, DNA, Chromosome Deletion, Gene Frequency genetics, Polymorphism, Genetic, Rh-Hr Blood-Group System genetics

Abstract

To investigate the frequency of RHD 1227A allele in Rh negative population and random population, an AS-PCR (allele specific-polymerase chain reaction) method was employed to detect RHD 1227A allele. RHD gene copy was determined by D zygosity test and RHD exon 9 nucleotide sequence analysis. The results showed that among 143 Rh negative donors, forty-one RHD 1227A allele carriers were detected, and 8 (19.51%) out of which were RhCCdee, 32 (78.05%) were RhCcdee, and 1 (2.44%) was RhCcdEe. Thirty-five Rh negative RHD 1227A carriers had RHD gene deletion, and the remaining carriers were RHD 1227A homozygous. Seven (1.43%) individuals were detected with RHD 1227A allele among 489 random donors. They were all G/A heterozygous at RHD 1227 site. Serological test indicated that they were normal Rh positive phenotype. It is concluded that the frequency of RHD 1227A allele is 16.43% among Rh negative population and 0.72% among the random population.

Published

2006

10. [Establishment of genotyping method for DEL phenotype in Zhejiang Han population].

Author

Wu JJ, Hong XZ, Ma KR, Xu XG, Fu QH, and Yan LX

Subjects

Adult, Alleles, Asian People genetics, Blood Donors, China ethnology, Erythrocytes metabolism, Female, Genotype, Humans, Male, Phenotype, Polymerase Chain Reaction methods, Rh-Hr Blood-Group System immunology, Erythrocytes immunology, Polymorphism, Genetic, Rh-Hr Blood-Group System genetics

Abstract

In order to establish a genotyping method for DEL phenotype in Zhejiang Han population, an AS-PCR method was developed according to the RHD 1227A allele sequence. Its specificity and sensitivity were assessed in two Rh negative populations whose RHD 1227A or DEL phenotype status was known. The results showed that in evaluation of the method by detecting 50 RHD 1227A positive and 50 RHD 1227A negative individuals, the genotyping method displayed a sensitivity of 100% and a specificity of 100%; in evaluation of the method by detecting 33 DEL positive and 89 DEL negative individuals, the sensitivity was 100%, however, there were two serologically negative samples which were confirmed as positive using genotyping method. After re-testing these two samples with serological method and sequence analysis, it was found that original serological method gave false negative results and genotyping method still showed 100% specificity. The minimal target DNA concentration of this genotyping method is 8.13 ng/microl. In conclusion, designed genotyping method can be used to identify DEL phenotype efficiently in Zhejiang Han Rh negative population.

Published

2006

11. [Molecular background of weak D type 15 as the predominant weak D type found in Chinese population].

Author

Sun GD, Duan XM, Zhang YP, Yin ZZ, Niu XL, Li YF, Zhao YL, and Niu HJ

Subjects

Asian People genetics, Base Sequence, Blood Donors, China ethnology, Exons genetics, Genotype, Haplotypes, Humans, Molecular Sequence Data, Phenotype, Polymerase Chain Reaction methods, Rh-Hr Blood-Group System immunology, Sequence Analysis, DNA, Erythrocytes immunology, Point Mutation, Polymorphism, Genetic, Rh-Hr Blood-Group System genetics

Abstract

This study was aimed to investigate the molecular genetic basis and serological phenotype of Rh weak D type 15 individuals. Samples were identified by serological tests and genotyped by sequence specific primer-PCR (SSP-PCR), and were sequenced to detect the changes of all ten RHD exons. The number of gene RHD was detected through SSP-PCR. The results showed that in tested individuals of weak D type confirmed by the IAT, 18 cases (56% in weak D) were weak D type 15. Rh factors found in 2 weak D type 15 individuals (11%) were C+c+E+e; Rh factors found in 2 weak D type 15 individuals (11%) were C+c+E-e+; others (78%) were c-c+E+e+. The results by serological tests were consistent with the results genotyped by PCR-SSP method. In all 18 samples, the sequencing result revealed a gene mutation 845G > A at the exon 6 of the RHD and the point mutation changed amino acid G282D of the RhD polypeptide. The zygosity test demonstrated that 2 out of 18 weak D type 15 individuals were RHD(+)/RHD(+) homozygous (two DCe/DcE), 16 cases were RHD(+)/RHD(-) heterozygous (two DCe/dce and fourteen DcE/dce). It is concluded that Weak D type 15 is predominant in weak D individuals of Chinese Han Nationality, and most of them are heterozygous with various RH haplotypes.

Published

2006

12. [Molecular basis of Rh DEL phenotype in Zhejiang Han population].

Author

Chen AX, Wu JJ, Xu FJ, Zhang LY, Ni YH, and Fu QH

Subjects

Alleles, Asian People genetics, Base Sequence, Blood Donors, China ethnology, Exons genetics, Humans, Molecular Sequence Data, Phenotype, Polymerase Chain Reaction methods, Rh-Hr Blood-Group System immunology, Sequence Analysis, DNA, Erythrocytes immunology, Point Mutation, Polymorphism, Genetic, Rh-Hr Blood-Group System genetics

Abstract

This study was purposed to investigate the molecular basis of Rh DEL phenotype. Rh DEL phenotypes were identified by a serologic adsorption-elution method, the nucleotide sequences of ten RHD exons and exon-intron boundary regions were evaluated by a RHD gene-specific PCR-SSP (PCR-SSP, polymerase chain reaction-sequence specific primer) and sequencing. The results showed that out of 122 random Rh negative donors 35 Rh DEL phenotypes were identified through serologic method, including 6 RhCCdee (17.14%), 28 RhCcdee (80.00%), and 1RhCcdEe (2.86%). Sequence analysis indicated that all DEL phenotypes harbored a RHD 1227 G > A mutation in exon 9. D zygosity test revealed that 29 DEL phenotypes (28 RhCcdee and 1 RhCcdEe) had one RHD gene deleted, and 6 DEL phenotypes (6 RhCCdee) had homogenous RHD gene. It is concluded that RHD 1227A is an important genetic marker for Rh DEL phenotype in Zhejiang Han population.

Published

2006

13. Rh(D) fraction incompatibility causing hemolytic disease of the newborn. Report of two cases in a Chinese family.

Author

Lee SK, Tham KT, Cheung KP, and Jenkins WJ

Subjects

Adult, Antibodies analysis, China ethnology, Erythroblastosis, Fetal immunology, Female, Humans, Infant, Newborn, Japan, Pregnancy, Erythroblastosis, Fetal genetics, Rh-Hr Blood-Group System immunology

Abstract

Two cases of hemolytic disease of new born in a Chinese family are reported. The hemolysis was due to the production in the mother of antibodies against fractions A, C, and D of Rh(D) antigen. The fractions were absent in the mother's red blood cells which are Rh(DB) but present in her babies. Rh(DB) may be detected by the use of two types of anti-D sera, one with and the other without anti-DB activity. For transfusion purpose, all DB patients so tested, would be regarded as Rh(D) negative.

Published

1982