首页> 外文期刊>Transfusion and apheresis science: official journal of the World Apheresis Association : official journal of the European Society for Haemapheresis >Investigation of pseudogenes RHDΨ and RHD -CE-D hybrid gene in D-negative blood donors by the real time PCR method
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Investigation of pseudogenes RHDΨ and RHD -CE-D hybrid gene in D-negative blood donors by the real time PCR method

机译:实时PCR法检测D阴性献血者假基因RHD R和RHD-CE-D杂种基因

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Introduction: The Rh system is the most polymorphic and immunogenic of all systems of blood groups. Currently more than 49 antigens were identified with five major antigens D, C, c, E, e. Knowledge of the molecular basis of the Rh system permitted the understanding of both the mechanism of Rh phenotype on the antigen variants of RHD and RHCE In Caucasians the primary mechanism of D-negative phenotype is the complete deletion of RHD gene, while the black Africans is the presence of pseudogene and gene hybrid RHD-CE (3-7)-D. Objective: To determine the prevalence gene pseudogene and hybrid gene and standardization of molecular techniques in method of Taqman on real-time PCR for RHD genotyping. Patients and methods: 203 samples of D-negative donor were used to establish and validate the effectiveness of RHD genotyping in real-time PCR using Taqman technology. The extraction was performed using a commercial kit QIAmp DNA mini kit. Samples exon 10 and 7 positive were submitted to amplification of exon 5, confirming the pseudogene RHDΨ, whereas exon 10. +. exon 7 - for the hybrid gene (C) cdes and mutation C733G (Leu245Val) of the RHCE gene. Results: Twenty-five (12.3%) samples were positive, 14 amplified for both exons 10 and 7 while in 11 only for the exon 10. When extended the screening using exon 10, 7 and 5, only 06 amplified. The pseudogene was present in 07 samples (3.5%) and the hybrid RHD-CE (3-7) in 04 (1.97%), while in 177 (87.2%) of Rh negative donors were RHD gene deletion. In 07 samples not amplified for exon 3 had mutated and the mutation C733G antigen. Conclusion: The prevalence of pseudogene was 3.5% and the gene hybrid RHD-CE of 1.9%. This approach for real-time PCR as a complementary tool is technically feasible and the results of this study helped develop a new strategy for RHD genotyping.
机译:简介:Rh系统是所有血型系统中最具多态性和免疫原性的。目前,鉴定出超过49种抗原与5种主要抗原D,C,c,E,e。了解Rh系统的分子基础可以了解Rh表型对RHD和RHCE抗原变体的机制。在白种人中,D阴性表型的主要机制是RHD基因的完全缺失,而黑人则是RHD基因的完全缺失。假基因和基因杂合RHD-CE(3-7)-D的存在。目的:通过Taqman实时荧光定量PCR检测RHD基因型,确定流行基因的假基因和杂种基因,并进行分子技术的标准化。患者和方法:使用Taqman技术,使用203个D阴性供体样本建立并验证RHD基因分型在实时PCR中的有效性。使用商业试剂盒QIAmp DNA mini试剂盒进行提取。将外显子10和7阳性的样品送至外显子5的扩增,确认假基因RHD +,而外显子10 +。外显子7-RHCE基因的杂种基因(C)cdes和突变C733G(Leu245Val)。结果:二十五个(12.3%)样品为阳性,第10外显子和第7外显子均扩增14个,而第10外显子仅在11中扩增。当使用第10、7和5外显子扩展筛选时,仅扩增06。该假基因存在于07个样品中(3.5%),而杂种RHD-CE(3-7)中存在04个样品(1.97%),而177个(87.2%)Rh阴性供体中存在RHD基因缺失。在07中未扩增的外显子3样品中发生了突变,并且突变C733G抗原。结论:假基因患病率为3.5%,基因杂种RHD-CE为1.9%。这种实时PCR作为补充工具的方法在技术上是可行的,这项研究的结果有助于开发一种新的RHD基因分型策略。

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